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- Biochemie, Chemie und Pharmazie (154)
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Additive manufacturing or 3D printing as an umbrella term for various materials processing methods has distinct advantages over many other processing methods, including the ability to generate highly complex shapes and designs. However, the performance of any produced part not only depends on the material used and its shape, but is also critically dependent on its surface properties. Important features, such as wetting or fouling, critically depend mainly on the immediate surface energy. To gain control over the surface chemistry post-processing modifications are generally necessary, since it′s not a feature of additive manufacturing. Here, we report on the use of initiator and catalyst-free photografting and photopolymerization for the hydrophilic modification of microfiber scaffolds obtained from hydrophobic medical-grade poly(ε-caprolactone) via melt-electrowriting. Contact angle measurements and Raman spectroscopy confirms the formation of a more hydrophilic coating of poly(2-hydroxyethyl methacrylate). Apart from surface modification, we also observe bulk polymerization, which is expected for this method, and currently limits the controllability of this procedure.
The stress-dependent dynamics of Saccharomyces cerevisiae tRNA and rRNA modification profiles
(2021)
RNAs are key players in the cell, and to fulfil their functions, they are enzymatically modified. These modifications have been found to be dynamic and dependent on internal and external factors, such as stress. In this study we used nucleic acid isotope labeling coupled mass spectrometry (NAIL-MS) to address the question of which mechanisms allow the dynamic adaptation of RNA modifications during stress in the model organism S. cerevisiae. We found that both tRNA and rRNA transcription is stalled in yeast exposed to stressors such as H2O2, NaAsO2 or methyl methanesulfonate (MMS). From the absence of new transcripts, we concluded that most RNA modification profile changes observed to date are linked to changes happening on the pre-existing RNAs. We confirmed these changes, and we followed the fate of the pre-existing tRNAs and rRNAs during stress recovery. For MMS, we found previously described damage products in tRNA, and in addition, we found evidence for direct base methylation damage of 2′O-ribose methylated nucleosides in rRNA. While we found no evidence for increased RNA degradation after MMS exposure, we observed rapid loss of all methylation damages in all studied RNAs. With NAIL-MS we further established the modification speed in new tRNA and 18S and 25S rRNA from unstressed S. cerevisiae. During stress exposure, the placement of modifications was delayed overall. Only the tRNA modifications 1-methyladenosine and pseudouridine were incorporated as fast in stressed cells as in control cells. Similarly, 2′-O-methyladenosine in both 18S and 25S rRNA was unaffected by the stressor, but all other rRNA modifications were incorporated after a delay. In summary, we present mechanistic insights into stress-dependent RNA modification profiling in S. cerevisiae tRNA and rRNA.
The prevalence and specificity of local protein synthesis during neuronal synaptic plasticity
(2021)
To supply proteins to their vast volume, neurons localize mRNAs and ribosomes in dendrites and axons. While local protein synthesis is required for synaptic plasticity, the abundance and distribution of ribosomes and nascent proteins near synapses remain elusive. Here, we quantified the occurrence of local translation and visualized the range of synapses supplied by nascent proteins during basal and plastic conditions. We detected dendritic ribosomes and nascent proteins at single-molecule resolution using DNA-PAINT and metabolic labeling. Both ribosomes and nascent proteins positively correlated with synapse density. Ribosomes were detected at ~85% of synapses with ~2 translational sites per synapse; ~50% of the nascent protein was detected near synapses. The amount of locally synthesized protein detected at a synapse correlated with its spontaneous Ca2+ activity. A multifold increase in synaptic nascent protein was evident following both local and global plasticity at respective scales, albeit with substantial heterogeneity between neighboring synapses.
Bezüglich der Arzneimittelforschung galt für sehr lange Zeit das Paradigma "ein Gen, ein Medikament, eine Krankheit". In jüngerer Zeit ändert sich dieses Paradigma jedoch auf Grund von redundanten Funktionen und alternativen sich kompensierenden Signalmustern, die insbesondere bei Krebserkrankungen vorherrschend sind. Daher kann die logische Konsequenz nur sein, Multi-Target-Strategien gegenüber Single-Target-Ansätzen in Betracht zu ziehen. Auf Grund der Schwierigkeit, mit einer Kombination von zwei Einzelwirkstoffen, in diesem Fall BET- und HDAC-Inhibitoren eine konsistente Biodistribution und Pharmakokinetik zu erreichen, wurde nach Einzelmolekülen gesucht, die mehrere inhibitorische Aktivitäten aufweisen. Dies wurde hier zunächst durch die einfache Konjugation von zwei unterschiedlichen Pharmakophoren erreicht.
Insgesamt wurden vier verschiedene Liganden dieses Typs synthetisiert und einer von ihnen, Verbindung 14, zeigte sehr vielversprechende Ergebnisse. 14 vereint den BET Inhibitor JQ1- mit dem HDAC Inhibitor CI994 und hat eine hemmende Wirkung sowohl gegen BRD4- als auch HDAC-Proteine wie durch DSF- und nanoBRET-Assay gezeigt werden konnte. Außerdem zeigten in vitro Assays in PDAC-Zellen, dass 14 ein noch potenterer dualer BET/HDAC-Inhibitor ist als die Kombination aus JQ1 und CI994. Während die Effekte von 14 auf das BETi-Antwortgen MYC denen von JQ1 ziemlich ähnlich sind, sind insbesondere die HDAC-inhibitorischen Effekte nachhaltiger und verstärkt, wahrscheinlich aufgrund einer längeren Verweildauer von 14 auf HDAC als dies bei CI994 der Fall ist. Dies ist durch das hohe Niveau der acetylierten Lysine von Histon H3 im Western Blot erkennbar. Dieses veränderte Expressionsverhalten hatte einen großen Einfluss auf das Zellwachstum und überleben in allen getesteten PDAC-Zelllinien. Hier wurde die Überlegenheit von 14 gegenüber der gleichzeitigen Behandlung der Zellen mit JQ1 und CI994 sehr deutlich. Wurden PDAC-Zellen mit dem dualen Inhibitor 14 behandelt, hatte dies ein geringeres Wachstum und Überleben der Krebszellen zur Folge als mit beiden ursprünglichen Molekülen, unabhängig davon, ob diese einzeln oder simultan verabreicht wurden. Außerdem wurde 14 mit Gemcitabin, einem gut verträglichen Chemotherapeutikum, kombiniert, dass bei PDAC allein nur eine begrenzte Aktivität aufweist. Es stellte sich heraus, dass die Reihenfolge, in der die Medikamente verabreicht werden, einen großen Einfluss auf die Effektivität hatte. Der durch 14 induzierte Stopp des Zellzyklus verhindert den Einbau von Gemcitabin in die DNA, wenn 14 vor oder gleichzeitig mit Gemcitabin verabreicht wird. Wenn jedoch die Behandlung mit 14 nach der Verabreichung von Gemcitabin folgt, wird der durch Gemcitabin induzierte S-Phasen-Arrest und Replikationsstress aufrechterhalten. Im Vergleich zu den meisten früheren Studien, die sich mit dualen BET/HDAC-Inhibitoren beschäftigten, ist dies eine große Verbesserung, da es bisher keinen signifikanten Unterschied zwischen der Verwendung eines dualen BET/HDAC-Inhibitors und der Kombination von zwei Einzelinhibitoren gab.
Als Proof of Concept unterstützten die Daten weitere Bemühungen zur Entwicklung zusätzlicher dualer BET/HDAC-Inhibitoren. Daher wurden zwei weitere Generationen dualer BET/HDAC Inhibitoren entwickelt, die jedoch bisher nicht an die Eigenschaften von 14 anknüpfen konnten. Vor allem die 3. Generation bietet jedoch Raum für Optimierungen, so dass hier möglicherweise noch ein potenter dualer Inhibitor zu finden ist. Sollte es in Zukunft einen zugelassenen dualen BET/HDAC-Inhibitor geben, ist es jedoch nicht unwahrscheinlich, dass keine der hier verwendet BET inhibierenden Strukturen verwendet werden, aber Struktur des HDAC inhibierenden Teils immer noch vergleichbar ist. Der Grund dafür ist, dass die HDAC Inhibitoren größtenteils relativ einfach aufgebaut. So lange das wichtigste, die zinkbindende Gruppe vorhanden ist, scheint der Linker sowie die Capping-Gruppe zweitranging zu sein. Die größere Herausforderung wird vermutlich die Suche nach dem passenden BET Inhibitor sein und die Wahlmöglichkeiten sind schon jetzt vielfältig.
Generell lässt sich sagen, dass die Idee der dualen BET/HDAC-Inhibitoren äußerst vielversprechend und es wert ist, weiter verfolgt zu werden. Dies liegt vor allem an den guten Testergebnissen, die mit Verbindung 14 erzielt wurden. Mit Hilfe dieser Art von Inhibitoren könnte es in Zukunft möglich sein, die Überlebensrate von PDAC-Patienten zu erhöhen, wenn nicht als alleiniges Medikament, so vielleicht als Zusatz zur Chemotherapie. Darüber hinaus scheint der Einsatz von dualen BET/HDAC-Inhibitoren nicht nur auf die Behandlung von PDAC beschränkt zu sein und kann auch bei anderen Krebsarten angewendet werden. NMC zum Beispiel ist ein ebenso seltener wie tödlicher Subtyp des schlecht differenzierten Plattenepithelkarzinoms und zeichnet sich durch eine Fusion des NUT-Gens mit BRD4 aus, wodurch es potenziell anfällig für eine BET-Inhibition ist. Tatsächlich zeigte 14 auch hier einen größeren positiven Effekt auf die getesteten NMC-Zellen als JQ1 oder CI994 und veranlasste die Zellen unter anderem zur Differenzierung. ...
Standard biorelevant media reflect the average gastrointestinal (GI) physiology in healthy volunteers. The use of biorelevant media in in vitro experiments has become an important strategy to predict drug behaviour in vivo and is often combined with in silico tools in order to simulate drug plasma profiles over time. In addition to the healthy population, the effects of disease state or co-administration of other drugs on plasma profiles must be considered to assure drug efficacy and safety. Thus, there is a need for a more accurate representation of the human GI physiology when it is altered by disease or co-administered drugs in in vitro dissolution experiments.
This thesis focused on the development of biorelevant media and dissolution tests reflecting GI physiology in circumstances where the gastric pH is elevated. Diseases linked to an elevated gastric pH are hypochlorhydria and achlorhydria, but these days treatment with acid-reducing agents (ARAs) is the single greatest cause of elevation in gastric pH. pH-dependent drug-drug interactions (DDIs) with ARAs are frequent, as the ARAs are used in a number of diseases using a variety of drugs. As the drugs currently on the market are often poorly soluble and ionisable, their dissolution is highly dependent on the pH of the GI tract, especially the gastric pH.
The thesis research consisted of several steps. In the first step, physiological changes in the human GI tract during the therapy with ARAs were identified. Parameters of the standard biorelevant gastric medium FaSSGF were adjusted to the identified changes to reflect the impact of ARA co-administration on the gastric physiology. The media aim to assess the potential extent of the ARA impact on gastric physiology by introducing biorelevant media pairs, ARA pH 4 and pH 6 media, of which one reflects a lesser, and the other a stronger impact of ARAs.
In the second step these ARA media were implemented in in vitro dissolution set-ups.
The dissolution of poorly soluble ionisable drugs was assessed using one-stage, two-stage and transfer model set-ups, as well as using a more evolved in vitro system TIM-1. Comparison of results from dissolution set-ups using the standard, low pH, gastric biorelevant medium FaSSGF (pH 1.6 or 2), and the same set-ups using ARA pH 4 and pH 6 media, shows a decrease in dissolution rate and extent for weakly basic compounds PSWB 001 and dipyridamole, and an increase in rate and extent of dissolution for the weakly acidic compound raltegravir potassium, when the gastric pH is elevated. Due to different physicochemical properties, the extent of the impact of physiological changes during ARA therapy (when either ARA pH 4 or pH 6 medium is selected) on dissolution varied among the model drugs. Thus, the bracketing approach, which considers a range of the possible ARA co-administration impact on drug dissolution, was confirmed to be best practice in assessing the impact of ARAs.
In the third step, dissolution data from in vitro experiments with ARA media was implemented into in silico models. The predictions using various in silico model approaches in Simcyp™ Simulator (minimal and full PBPK model, dissolution input using DRM and DLM) successfully bracketed in vivo data on drug administration during ARA therapy and correctly predicted an overall decrease in plasma concentration for the two model weakly basic compounds and an increase in plasma concertation for the model weakly acidic compound.
In all assessed scenarios, the ARA methods proved to be an essential part of evaluating and predicting the impact of ARAs on drug pharmacokinetics, and appropriately predicted the extent of a possible impact of ARAs on the drug plasma profiles. Thus, the ARA biorelevant media and dissolution tests were demonstrated to be valuable tools reflecting administration of drugs when the gastric pH is elevated and able to predict the impact of ARA therapy on drug administration.
The ability to evaluate the impact of human (patho) physioloy on drug behaviour in the gastrointestinal tract is of great importance, as the GI conditions play a significant role in drug release and absorption. Thus, there is great interest on the part of the pharmaceutical industry and regulatory agencies to develop best practices in this field, especially for pH-dependent DDIs. The media and dissolution tests developed in this thesis are biorelevant methods appropriate for evaluation of the impact of elevated gastric pH on drug efficacy and safety. Such methods, used as a risk assessment tool, in connection with evaluation of the efficacy window and potential toxicity, may help to increase confidence about decisions as to whether a pH-effect will occur and whether it is relevant or not, prior to conducting clinical studies. They may also enable changes in inclusion/exclusion criteria during recruiting for large-scale efficacy trials. In fact, the biopharmaceutic approach to drug development is becoming standard practice on a number of fronts, including metabolic DDIs, renal and hepatic insufficiency, powering decision-making process and possibly even waiving certain types of clinical studies.
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Bacteria are true artists of survival, which rapidly adapt to environmental changes like pH shifts, temperature changes and different salinities. Upon osmotic shock, bacteria are able to counteract the loss of water by the uptake of potassium ions. In many bacteria, this is accomplished by the major K+ uptake system KtrAB. The system consists of the K+-translocating channel subunit KtrB, which forms a dimer in the membrane, and the cytoplasmic regulatory RCK subunit KtrA, which binds non-covalently to KtrB as an octameric ring. This unique architecture differs strongly from other RCK-gated K+ channels like MthK or GsuK, in which covalently tethered cytoplasmic RCK domains regulate a single tetrameric pore. As a consequence, an adapted gating mechanism is required: The activation of KtrAB depends on the binding of ATP and Mg2+ to KtrA, while ADP binding at the same site results in inactivation, mediated by conformational rearrangements. However, it is still poorly understood how the nucleotides are exchanged and how the resulting conformational changes in KtrA control gating in KtrB is still poorly understood.
Here,I present a 2.5-Å cryo-EM structure of ADP-bound, inactive KtrAB, which for the first time resolves the N termini of both KtrBs. They are located at the interface of KtrA and KtrB, forming a strong interaction network with both subunits. In combination with functional and EPR data we show that the N termini, surrounded by a lipidic environment, play a crucial role in the activation of the KtrAB system. We are proposing an allosteric network, in which an interaction of the N termini with the membrane facilitates MgATP-triggered conformational changes, leading to the active, conductive state.
The knob-associated histidine-rich protein (KAHRP) plays a pivotal role in the pathophysiology of Plasmodium falciparum malaria by forming membrane protrusions in infected erythrocytes, which anchor parasite-encoded adhesins to the membrane skeleton. The resulting sequestration of parasitized erythrocytes in the microvasculature leads to severe disease. Despite KAHRP being an important virulence factor, its physical location within the membrane skeleton is still debated, as is its function in knob formation. Here, we show by super-resolution microscopy that KAHRP initially associates with various skeletal components, including ankyrin bridges, but eventually colocalizes with remnant actin junctions. We further present a 35 Å map of the spiral scaffold underlying knobs and show that a KAHRP-targeting nanoprobe binds close to the spiral scaffold. Single-molecule localization microscopy detected ~60 KAHRP molecules/knob. We propose a dynamic model of KAHRP organization and a function of KAHRP in attaching other factors to the spiral scaffold.
T-cell development is a highly dynamic and stepwise process comprimising T lineage commitment, T-cell receptor (TCR) gene rearrangements and subsequent selection. From a quantitative point of view, only a few hundred progenitor cells migrate from the bone marrow into the thymus. Developing thymocytes (termed double negative (DN), CD4-CD8-) can be further divided into DN1-4 cells based on the expression of CD25 and CD44. These developmental events are interspersed by proliferative bursts which ultimately lead to the generation of millions of double positive (DP, CD4+CD8+) thymocytes that then undergo selection. As a consequence, a proportion of naïve T-cells evolves to ensure adaptive, but not autoreactive immunity.
Previous studies of our lab focused on the quantification of thymus colonization and identified thymus entry to be dependent on expression of the chemokine receptors CCR7 and CCR9 (Krueger et al., 2010; Ziętara et al., 2015). CCR7/9 double knockout (DKO) mice are almost completely devoid of the most immature thymocyte populations (DN1 and DN2), but show near normal DN3 cellularity. Interestingly, a similar defect during early development but a virtually complete recovery of later stages and total thymocyte numbers was also observed in thymi of miR-17~92 deficient mice. Here, a failure of prethymic IL-7 signaling dampens early T-cell development (Regelin et al., 2015). For this reason, we hypothesized a tight regulation of thymocyte population size through alterations in the underlying cell cycle kinetics.
In this thesis, we employed in vivo single- and dual-nucleoside pulse labeling combined with determination of DNA replication over time in different WT thymocyte subsets at steady-state. Based on this, we assessed alterations in cell cycle kinetics of CCR7/9 and miR-17~92 defcicient mice and identified compensatory mechanisms of thymocytes on the level of cell cycle phase distribution and cell cycle speed. In addition, single-cell RNA sequencing helped to obtain information on cell cycle dynamics of early thymocyte subsets, exemplarily shown for WT and CCR7/9 DKO mice. Lastly, we performed cell cycle analyses in a model of endogenous thymic repair upon sublethal total body irradiation which provided insight into intrathymic cell cycle regulation as an adjustable system to re-establish normal thymus cellularity.
In the second part of the thesis, we addressed the role of miR-21 in the thymus. In various studies, we and others identified miRNAs as key posttranscriptional regulators of the immune system and especially for T-cell development (Regelin et al. 2015; Mildner et al. 2017; Li et al. 2007; Ebert et al. 2009; Ziętara et al. 2013; Schaffert et al. 2015). The dynamic expression of miR-21 during T-cell development (Neilson et al. 2007; Kirigin et al. 2012; Kuchen et al. 2010) prompted us to hypothesize that miR-21 has a regulatory function in the thymus. A miR 21-knockout mouse model allowed us to study the role of this miRNA for the development of T-cells in the thymus and the maintenance of T-cells in the periphery. In addition, we performed competitive bone marrow chimera experiments in the context of miR-21 deficiency and overexpression. Further insights were provided by exploring the function of miR-21 in negative selection in vivo as well as in T-cell differentiation in coculture experiments in vitro. To unravel implications of miR-21 to regulate cellular stress responses, we assessed the contribution of miR-21 in a model of endogenous regeneration of the thymus after sublethal irradiation. We could not provide evidence for a prominent role for miR-21 during T-cell development. Together, our experiments revealed that miR-21 is largely dispensable for physiologic T-cell development despite high and dynamic expression in the thymus (Kunze Schumacher et al., 2018). The apparent discrepancy between dynamic expression but lack of a regulatory function in the thymus led us to conclude that miR-21 is rather fine tuning T-cell responses than controlling a developmental event.
The specific and precise arrangement of proteins and biomolecules in 3D is an important prerequisite for the study of cell migration, cellular signal transduction and the production of artificial tissue. In a variety of research approaches, proteins have been immobilized on rigid surfaces such as glass or gold to observe protein-protein or protein-cell interactions. While these commonly used analytical platforms offer advantages such as rapid washing steps and easy use, due to their rigidity and two-dimensionality, they cannot replicate the extracellular matrix (ECM) the native environment of cells. This severe deviation from the natural environment results in significant changes in cell structure and cellular processes such as the polarization of the cell, its morphology, and signal transduction. In order to maintain the functionality of the immobilized proteins, it is also enormously important that the proteins are oriented and anchored in the material under mild conditions.
An immobilization strategy that makes this possible is bioaffinity. For this, the specific interaction of a biomolecule with an interaction partner anchored on a surface is used to immobilize the biomolecule. Such an interaction is for example the nitrilotriacetic acid (NTA)/His-tag binding. NTA is a chelator molecule that, when bound to divalent metal ions such as Ni(II), forms an octahedral complex with oligohistidines. The oligo histidine-tag can be competed out of the complex by free histidine or imidazole due to structural similarity. This is exploited in immobilized metal affinity chromatography (IMAC). The binding of a monoNTA/His-tag complex (KD=10 µM) is not stable enough to be used for immobilizations. Therefore, multivalent variants of the chelator were developed, like trisNTA which has a high affinity for His6 tagged proteins (KD= 10 nM). The PA-trisNTA developed in a preliminary work was the first light-activatable system based on the trisNTA chelator head.
The aim of this work was to synthesize a new two-photon (2P) activatable trisNTA (TPA trisNTA) interaction molecule, to analyze its photophysical characteristics and to apply it for two- and three dimensional (2D/3D) biomolecule patterning. The final goal was to use TPA trisNTA for cellular applications in order to manipulate membrane protein organization. Therefore, TPA trisNTA was designed to maintain a stable autoinhibition enabling the immobilization of proteins under physiological conditions with high precision in the x/y, as well as z dimension only upon light activation. 2P activation brings some outstanding advantages: i) the use of near-infrared (NIR) light is less harmful to cells compared to ultraviolet (UV) light, ii) the longer wavelength allows the radiation to penetrate deeper into tissues, iii) the precision of focal irradiation is more accurate because only a focal volume (about 1 fL) is excited and, unlike UV light, scattered light does not lead to activation.
Several backbones for TPA-trisNTA were considered as 2P cleavable groups due to their 2P absorption ability and small size: 3 nitrodibenzofuran (NDBF), 6 bromo 7 hydroxycoumarin (Bhc), and 7 diethylaminocoumarin (DEAC). Initially, suitable synthetic routes were developed for the respective carbaldehydes, since these represented an important intermediate for both the construction of amino acid (aa) derivatives as well as ß hydroxy acids. ß Hydroxy acids were important intermediates because their photocleavage differs from aa derivatives. To establish the conversion from carbaldehydes to hydroxy acids via Reformatsky reaction, commercially available carbaldehydes of the nitroveratral (NV) or nitropiperonal (NP) group were used in addition. The conversion of NDBF, NV, NP proved to be difficult, whereas the ß-hydroxy acid was successfully synthesized from Bhc as well as from DEAC.
Starting from DEAC ß hydroxy acid, a Fmoc protected amino acid derivative was synthesized. To ensure high cleavage efficiency, the DEAC ß hydroxy acid was linked to monoFmoc ethylenediamine through a carbamate linker. Subsequently, the photocleavable group was successfully incorporated into the linker of TPA-trisNTA by solid-phase peptide synthesis (SPPS).
The functional principle of TPA-trisNTA, similar to PA-trisNTA, is based on the autoinhibition of the multivalent chelator head trisNTA, which is linked to an intramolecular oligohistidine sequence by a peptide linker. In presence of Ni(II) ions, trisNTA forms a metal ion-mediated complex with histidine, causing TPA-trisNTA to self-inactivate. The cleavage site is the DEAC based photocleavable amino acid. In contrast to PA-trisNTA, the incorporation of two photocleavable amino acids was omitted. Instead, only one photocleavable DEAC was incorporated in front of the His tag. To avoid a second DEAC group within the His tag, a His5 tag was used instead of an His6 tag. It is known from preliminary work that a His5 tag is sufficient to maintain autoinhibition in the presence of His6-tagged proteins of interest (POIs), but can be displaced from the complex after light-driven cleavage of the peptide backbone. Placement of a cysteine in the peptide linker between the trisNTA and the DEAC group allowed for permanent surface anchoring after photocleavage of the linker.
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Treatment of hexachloropropene (Cl2C[double bond, length as m-dash]C(Cl)–CCl3) with Si2Cl6 and [nBu4N]Cl (1 : 4 : 1) in CH2Cl2 results in a quantitative conversion to the trisilylated, dichlorinated allyl anion salt [nBu4N][Cl2C[double bond, length as m-dash]C(SiCl3)–C(SiCl3)2] ([nBu4N][1]). Tetrachloroallene Cl2C[double bond, length as m-dash]C[double bond, length as m-dash]CCl2 was identified as the first intermediate of the reaction cascade. In the solid state, [1]− adopts approximate Cs symmetry with a dihedral angle between the planes running through the olefinic and carbanionic fragments of [1]− of C[double bond, length as m-dash]C–Si//Si–C–Si = 78.3(1)°. One-electron oxidation of [nBu4N][1] with SbCl5 furnishes the distillable blue radical 1˙. The neutral propene Cl2C[double bond, length as m-dash]C(SiCl3)–C(SiCl3)2H (2) was obtained by (i) protonation of [1]− with HOSO2CF3 (HOTf) or (ii) H-atom transfer to 1˙ from 1,4-cyclohexadiene. Quantitative transformation of all three SiCl3 substituents in 2 to Si(OMe)3 (2OMe) or SiMe3 (2Me) substituents was achieved by using MeOH/NMe2Et or MeMgBr in CH2Cl2 or THF, respectively. Upon addition of 2 equiv. of tBuLi, 2Me underwent deprotonation with subsequent LiCl elimination, 1,2-SiMe3 migration and Cl/Li exchange to afford the allenyl lithium compound Me3Si(Li)C[double bond, length as m-dash]C[double bond, length as m-dash]C(SiMe3)2 (Li[4]), which is an efficient building block for the introduction of Me, SiMe3, or SnMe3 (5) groups. The trisilylated, monochlorinated allene Cl3Si(Cl)C[double bond, length as m-dash]C[double bond, length as m-dash]C(SiCl3)2 (6), was obtained from [nBu4N][1] through Cl−-ion abstraction with AlCl3 and rearrangement in CH2Cl2 (1˙ forms as a minor side product, likely because the system AlCl3/CH2Cl2 can also act as a one-electron oxidant).
Photoacids attract increasing scientific attention, as they are valuable tools to spatiotemporally control proton-release reactions and pH values of solutions. We present the first time-resolved spectroscopic study of the excited state and proton-release dynamics of prominent merocyanine representatives. Femtosecond transient absorption measurements of a pyridine merocyanine with two distinct protonation sites revealed dissimilar proton-release mechanisms: one site acts as a photoacid generator as its pKa value is modulated in the ground state after photoisomerization, while the other functions as an excited state photoacid which releases its proton within 1.1 ps. With a pKa drop of 8.7 units to −5.5 upon excitation, the latter phenolic site is regarded a super-photoacid. The 6-nitro derivative exhibits only a phenolic site with similar, yet slightly less photoacidic characteristics and both compounds transfer their proton to methanol and ethanol. In contrast, for the related 6,8-dinitro compound an intramolecular proton transfer to the ortho-nitro group is suggested that is involved in a rapid relaxation into the ground state.
The knob-associated histidine-rich protein (KAHRP) plays a pivotal role in the pathophysiology of Plasmodium falciparum malaria by forming membrane protrusions in infected erythrocytes, which anchor parasite-encoded adhesins to the membrane skeleton. The resulting sequestration of parasitized erythrocytes in the microvasculature leads to severe disease. Despite KAHRP being an important virulence factor, its physical location within the membrane skeleton is still debated, as is its function in knob formation. Here, we show by super-resolution microscopy that KAHRP initially associates with various skeletal components, including ankyrin bridges, but eventually colocalizes with remnant actin junctions. We further present a 35 Å map of the spiral scaffold underlying knobs and show that a KAHRP-targeting nanoprobe binds close to the spiral scaffold. Single-molecule localization microscopy detected ~60 KAHRP molecules/knob. We propose a dynamic model of KAHRP organization and a function of KAHRP in attaching other factors to the spiral scaffold.
Komplexe biologische Phänotypen resultieren aus einem koordinierten Zusammenspiel von einer Vielzahl von Genen. Um zu verstehen, wie Krankheiten durch genetische Dysfunktionen
entstehen können, ist es unabdingbar die genetischen Interaktionsnetzwerke in menschlichen Zellen zu entschlüsseln. Eine Identifizierung von Kontext-abhängigen genetischen Interaktionen kann bedeutende Erkenntnisse über die Beziehung von Phänotyp und Genotyp liefern und erklären, wie synergistische Gen-Funktionen die Entstehung von komplexen Krankheiten bedingen.
Gepoolte, kombinatorische CRISPR (kurz für: clustered regularly interspaced short palindromic repeats) Screens stellen eine wirkungsvolle Methode zur simultanen Untersuchung potentieller Interaktionen von einer großen Anzahl von Genen dar. Mit sogenannten multiplex CRISPR
gRNA Bibliotheken werden im Rahmen großangelegter Screens vielzählige kombinatorische Gen-Knockouts in Zellen generiert. Diese multiplex CRISPR gRNA Bibliotheken können aus bis zu hunderttausenden Plasmiden bestehen, die jeweils für eine andere gRNA-Kombination kodieren und auf ein spezifisches Gen-Paar abzielen. Im Gegensatz zu CRISPR Screens für Einzel-Knockouts gehen multiplex CRISPR Screens zur Identifizierung von genetischen Interaktionen mit zusätzlichen Herausforderungen einher: Zum einen wächst der verbundene Arbeitsaufwand für die Konstruktion der multiplex CRISPR gRNA Bibliotheken proportional mit der Anzahl der gewünschten Ziel-Gene, welche die Diversität der Bibliothek bestimmt. In einer idealen gRNA-Bibliothek wären alle gRNA-Sequenzen gleich häufig vorhanden. Jedoch weisen
gRNA-Bibliotheken aufgrund von technischen Beschränkungen gRNA-Sequenzen mit höherer, beziehungsweise niedriger Abundanz auf. Konventionelle Methoden zur Herstellung von
gRNA-Bibliotheken basieren beispielsweise auf iterativen, gepoolten Klonierungsschritten mit PCR-amplifizierten Oligonucleotiden, welche zu einer Ungleichverteilung oder zum Verlust von gRNA-Sequenzen führen können. Daher bieten Methoden zur gRNA-Bibliotheken-Generierung Optimierungspotenzial. Da die Reproduzierbarkeit der Screen-Ergebnisse durch die sogenannte Screening Coverage sichergestellt werden muss, erfordert eine Erhöhung der
Bibliotheks-Diversität gleichzeitig auch eine Vergrößerung des Versuchsmaßstabs und ist mit umfangreichem Zellkultur-Arbeitsaufwand verbunden. Die Screening Coverage gibt die
durchschnittliche Abundanz der einzelnen gRNA-Sequenzen in der Zellpopulation während des Screens an. Aktuelle Richtlinien empfehlen eine Screening Coverage, die zwischen dem 200- bis 1000-fachen Wert der Bibliotheks-Diversität liegt, allerdings fehlen bisher genaue Angaben die auf die verwendete gRNA Bibliothek abgestimmt sind. Deshalb stellt die benötigte Screening Coverage bisher einen limitierenden Faktor dar, der die Anzahl der möglichen Ziel-Gene-Kombinationen in einem Screen beschränkt.
In der vorliegenden Arbeit stellen wir eine neue Methode zur Generierung von multiplex gRNA Bibliotheken mit hohen Diversitäten vor. Die Methode, genannt 3Cs (covalently-closed circular-synthesized) Multiplexing, umgeht iterative, gepoolte Klonierugsschritte mit Restriktionsenzymen und PCR-Amplifikation von gRNA-kodierenden Oligonucleotiden. Wir
zeigen, dass 3Cs Multiplexing auf robuste Weise zur Herstellung von gleichmäßig verteilten multiplex gRNA Bibliotheken verwendet werden kann. Der Verteilungs-Skew, auch Skew-Ratio oder Bibliotheksbreite genannt, ist ein Maß zur Ermittlung der Gleichverteilung der gRNA-Sequenzen in der Bibliothek. Wir zeigen, dass 3Cs multiplex Bibliotheken typischerweise einen Verteilungs-Skew von 2.5 aufweisen, was unter den üblichen Werten von Einzel-gRNA Bibliotheken liegt.
Wir nahmen an, dass die gRNA-Bibliotheksverteilung die Robustheit von gepoolten CRISPR Screens beeinflussen könne und deshalb bei der Auswahl einer geeigneten Screening
Coverage berücksichtigt werden müsse. Um den Einfluss der gRNA-Bibliotheksverteilung auf die Screen-Qualität in Abhängigkeit von der verwendeten Screening Coverage zu untersuchen, generierten wir zwei künstlich fehlverteilte multiplex gRNA-Bibliotheken. Diese wurden, zusätzlich zu einer nahezu gleichverteilten multiplex gRNA-Bibliothek, jeweils mit einer 20- und 200-fachen Screening Coverage in einem kombinatorischen Proliferationsscreen angewandt.
Dadurch konnten wir die gRNA-Bibliotheksverteilung als den bestimmenden Parameter für die benötigte Screening Coverage identifizieren. Zusätzlich konnten wir zeigen, dass 3Cs multiplex gRNA-Bibliotheken auf Grund ihrer gleichmäßigen Verteilung mit minimierter Screening Coverage eingesetzt werden können, was zu einer 10-fachen Reduktion des assoziierten Arbeitsaufwands führt. Während bisherige Richtlinien für gepoolte CRISPR Screens die initiale
gRNA-Bibliotheksverteilung nicht berücksichtigen, empfehlen wir die Screening Coverage an dieser auszurichten.
Autophagie ist ein streng regulierter zellulärer Prozess, der den Lysosomen Abbau von intrazellulärem Material steuert und im Zusammenhang mit zahlreichen menschlichen Erkrankungen steht. Da Autophagie in eine Vielzahl von Signalwegen integriert ist, bietet es außerdem therapeutische Ansatzpunkte zur Behandlung von Krankheiten. Die Identifizierung von synergistischen Funktionen zwischen Autophagie-Genen könnte unser Verständnis über die molekularen Mechanismen, die der Regulation der Autophagie zu Grunde liegen, erweitern und dadurch neuartige Behandlungen ermöglichen.
Um genetische Interaktionen von Autophagie-Genen zu untersuchen haben wir eine 3Cs multiplex gRNA Bibliothek generiert, die auf menschliche Autophagie-Genkombinationen
abzielt. In dieser Arbeit demonstrieren wir die Funktionalität der 3Cs Autophagie multiplex gRNA Bibliothek unter Anwendung minimierter Screening Coverage in zwei verschiedenen Screen-Ausführungen: In einem Proliferationsscreen konnten wir Geninteraktionen
identifizieren, deren Verlust zu einer gesteigerten oder verringerten Zellproliferation führt. Unter diesen resultierte der Knockout von WDR45B-PIK3R4 zur stärksten Suppression der Proliferation, während die Depletion von ATG7-KEAP1 zu extrem verstärkter Proliferation beitrug. Unter Einsatz eines Autophagie-Reporters konnten wir in einem Autophagie Screen genetische Interaktionen aufdecken, die essentiell für Autophagie sind, darunter die
Interaktionen zwischen ATG2A-ATG2B , GABARAPL2-WIPI2 und ULK4-SQSTM1.
Wir glauben, dass 3Cs Multiplexing in Zukunft breite Anwendung in verschiedenen biologisch relevanten Feldern finden kann und die Entschlüsselung von kontext-abhängigen genetischen Interaktionen voranbringen und so das Verständnis für die Entstehung von komplexen pathologischen Phänotypen erweitern wird.
In vivo inducible reverse genetics in patients' tumors to identify individual therapeutic targets
(2021)
High-throughput sequencing describes multiple alterations in individual tumors, but their functional relevance is often unclear. Clinic-close, individualized molecular model systems are required for functional validation and to identify therapeutic targets of high significance for each patient. Here, we establish a Cre-ERT2-loxP (causes recombination, estrogen receptor mutant T2, locus of X-over P1) based inducible RNAi- (ribonucleic acid interference) mediated gene silencing system in patient-derived xenograft (PDX) models of acute leukemias in vivo. Mimicking anti-cancer therapy in patients, gene inhibition is initiated in mice harboring orthotopic tumors. In fluorochrome guided, competitive in vivo trials, silencing of the apoptosis regulator MCL1 (myeloid cell leukemia sequence 1) correlates to pharmacological MCL1 inhibition in patients´ tumors, demonstrating the ability of the method to detect therapeutic vulnerabilities. The technique identifies a major tumor-maintaining potency of the MLL-AF4 (mixed lineage leukemia, ALL1-fused gene from chromosome 4) fusion, restricted to samples carrying the translocation. DUX4 (double homeobox 4) plays an essential role in patients’ leukemias carrying the recently described DUX4-IGH (immunoglobulin heavy chain) translocation, while the downstream mediator DDIT4L (DNA-damage-inducible transcript 4 like) is identified as therapeutic vulnerability. By individualizing functional genomics in established tumors in vivo, our technique decisively complements the value chain of precision oncology. Being broadly applicable to tumors of all kinds, it will considerably reinforce personalizing anti-cancer treatment in the future.
A highly diastereoselective one-pot synthesis of the 1,3-diamino-2-alcohol unit bearing three continuous stereocenters is described. This method utilizes 2-oxyenamides as a novel type of building block for the rapid assembly of the 1,3-diamine scaffold containing an additional stereogenic oxygen functionality at the C2 position. A stereoselective preparation of the required (Z)-oxyenamides is reported as well.
Designed polypharmacology presents as an attractive strategy to increase therapeutic efficacy in multi-factorial diseases by a directed modulation of multiple involved targets with a single molecule. Such an approach appears particularly suitable in non-alcoholic steatohepatitis (NASH) which involves hepatic steatosis, inflammation and fibrosis as pathological hallmarks. Among various potential pharmacodynamic mechanisms, activation of the farnesoid X receptor (FXRa) and inhibition of leukotriene A4 hydrolase (LTA4Hi) hold promise to counteract NASH according to preclinical and clinical observations. We have developed dual FXR/LTA4H modulators as pharmacological tools, enabling evaluation of this polypharmacology concept to treat NASH and related pathologies. The optimized FXRa/LTA4Hi exhibits well-balanced dual activity on the intended targets with sub-micromolar potency and is highly selective over related nuclear receptors and enzymes rendering it suitable as tool to probe synergies of dual FXR/LTA4H targeting.
The desensitized channelrhodopsin-2 photointermediate contains 13 -cis, 15 -syn retinal Schiff base
(2021)
Channelrhodopsin-2 (ChR2) is a light-gated cation channel and was used to lay the foundations of optogenetics. Its dark state X-ray structure has been determined in 2017 for the wild-type, which is the prototype for all other ChR variants. However, the mechanistic understanding of the channel function is still incomplete in terms of structural changes after photon absorption by the retinal chromophore and in the framework of functional models. Hence, detailed information needs to be collected on the dark state as well as on the different photointermediates. For ChR2 detailed knowledge on the chromophore configuration in the different states is still missing and a consensus has not been achieved. Using DNP-enhanced solid-state MAS NMR spectroscopy on proteoliposome samples, we unambiguously determined the chromophore configuration in the desensitized state, and we show that this state occurs towards the end of the photocycle.
Polymorphic G-quadruplex (G4) secondary DNA structures have received increasing attention in medicinal chemistry owing to their key involvement in the regulation of the maintenance of genomic stability, telomere length homeostasis and transcription of important proto-oncogenes. Different classes of G4 ligands have been developed for the potential treatment of several human diseases. Among them, the carbazole scaffold with appropriate side chain appendages has attracted much interest for designing G4 ligands. Because of its large and rigid π-conjugation system and ease of functionalization at three different positions, a variety of carbazole derivatives have been synthesized from various natural or synthetic sources for potential applications in G4-based therapeutics and biosensors. Herein, we provide an updated close-up of the literatures on carbazole-based G4 ligands with particular focus given on their detailed binding insights studied by NMR spectroscopy. The structure-activity relationships and the opportunities and challenges of their potential applications as biosensors and therapeutics are also discussed. This review will provide an overall picture of carbazole ligands with remarkable G4 topological preference, fluorescence properties and significant bioactivity; portraying carbazole as a very promising scaffold for assembling G4 ligands with a range of novel functional applications.
Chemical language models enable de novo drug design without the requirement for explicit molecular construction rules. While such models have been applied to generate novel compounds with desired bioactivity, the actual prioritization and selection of the most promising computational designs remains challenging. Herein, we leveraged the probabilities learnt by chemical language models with the beam search algorithm as a model-intrinsic technique for automated molecule design and scoring. Prospective application of this method yielded novel inverse agonists of retinoic acid receptor-related orphan receptors (RORs). Each design was synthesizable in three reaction steps and presented low-micromolar to nanomolar potency towards RORγ. This model-intrinsic sampling technique eliminates the strict need for external compound scoring functions, thereby further extending the applicability of generative artificial intelligence to data-driven drug discovery.
Two subvalent, redox-active diborane(4) anions, [3]4− and [3]2−, carrying exceptionally high negative charge densities are reported: Reduction of 9-methoxy-9-borafluorene with Li granules without stirring leads to the crystallization of the B(sp3)−B(sp2) diborane(5) anion salt Li[5]. [5]− contains a 2,2′-biphenyldiyl-bridged B−B core, a chelating 2,2′-biphenyldiyl moiety, and a MeO substituent. Reduction of Li[5] with Na metal gives the Na+ salt of the tetraanion [3]4− in which two doubly reduced 9-borafluorenyl fragments are linked via a B−B single bond. Comproportionation of Li[5] and Na4[3] quantitatively furnishes the diborane(4) dianion salt Na2[3], the doubly boron-doped congener of 9,9′-bis(fluorenylidene). Under acid catalysis, Na2[3] undergoes a formal Stone–Wales rearrangement to yield a dibenzo[g,p]chrysene derivative with B=B core. Na2[3] shows boron-centered nucleophilicity toward n-butyl chloride. Na4[3] produces bright blue chemiluminescence when exposed to air.
SARS-CoV-2 contains a positive single-stranded RNA genome of approximately 30 000 nucleotides. Within this genome, 15 RNA elements were identified as conserved between SARS-CoV and SARS-CoV-2. By nuclear magnetic resonance (NMR) spectroscopy, we previously determined that these elements fold independently, in line with data from in vivo and ex-vivo structural probing experiments. These elements contain non-base-paired regions that potentially harbor ligand-binding pockets. Here, we performed an NMR-based screening of a poised fragment library of 768 compounds for binding to these RNAs, employing three different 1H-based 1D NMR binding assays. The screening identified common as well as RNA-element specific hits. The results allow selection of the most promising of the 15 RNA elements as putative drug targets. Based on the identified hits, we derive key functional units and groups in ligands for effective targeting of the RNA of SARS-CoV-2.
Diversity-oriented synthesis (DOS) is a rich source for novel lead structures in Medicinal Chemistry. In this study, we present a DOS-compatible method for synthesis of compounds bearing a free thiol moiety. The procedure relies on Rh(II)-catalyzed coupling of dithiols to diazo building blocks. The synthetized library was probed against metallo-β-lactamases (MBLs) NDM-1 and VIM-1. Biochemical and biological evaluation led to identification of novel potent MBL inhibitors with antibiotic adjuvant activity.
B-cell acute lymphoblastic leukaemia (B-ALL) is characterized by the overproduction of lymphoblasts in the bone marrow (BM), and it is the most common cancer in children while being comparatively uncommon in adults. On the other hand, in chronic myeloid leukaemia (CML), 70% of cases are found in patients older than 50 years, making it uncommon in children. All CML cases and up to 3% of paediatric B- ALL (and 25% of adult B-ALL) cases are due to fusion gene BCR-ABL1, which gives rise to the cytoplasmatic, constitutively active oncoprotein, tyrosine kinase BCR-ABL1 through a reciprocal translocation between chromosomes 9 and 22. The constitutively active BCR-ABL tyrosine kinase leads to deregulation of different signal transduction pathways such as cell growth, proliferation and cell survival. The role of the bone marrow microenvironment (BMM) can mediate disease initiation (only in mice), progression, therapy resistance, and relapse, as has been increasingly recognized over the last two decades. In general, the BMM is a very complex arrangement of various cell types such as osteoblasts, osteoclasts, endothelial cells, adipocytes, mesenchymal stromal cells, macrophages and several others. In addition, the BMM is composed of multiple chemical and mechanical factors and extra cellular matrix (ECM) proteins which contribute to the BMM’s features influencing leukaemia behaviour. Considering the incidence of B-ALL and CML in children and in adults respectively, we hypothesized that the young and/or an aged BMM might also play a previously unrecognized role in the aggressiveness of B-ALL and CML. We proposed that BM, transduced with BCR-ABL1-expressing retrovirus in the murine transduction/transplantation model of B-ALL, transplanted into young versus old recipient mice would lead to a more aggressive disease in young mice, and similarly CML would be more aggressive in old recipient mice. In close recapitulation with the human incidence, induction of CML led to a significantly shorted survival in old recipient mice. On the other hand, induction of B-ALL showed a shortened survival in young compared to old syngeneic mice, as well as in a xenotransplantation model. Among the highly heterogenous composition of the BMM, we implicate young BM macrophages as a supportive niche for B-ALL cells. The results were found to be mostly due to potential soluble factors differentially secreted from young and old macrophages. Therefore, we hypothesized that the chemokine CXCL13, which has been demonstrated to play a role in B cell migration and act as a diagnostic marker in the cerebrospinal fluid of patients with neuroborreliosis, might be responsible for the observed phenotype. CXCL13 was found to be more highly expressed in healthy and leukaemic young mice as well as in conditioned medium of young macrophages. Using a variety of in vitro experiments, CXCL13 showed to significantly increase the proliferation and the migration of leukaemia cells when exposed to young macrophages, and the phenotype was rescued while using a CXCL13 neutralizing antibody. The CXCL13 role was also confirmed in vivo, since macrophage ablation led to a prolongation of survival in young mice and a reduction of CXCL13 levels. The use of an additional mouse model, leukaemia cells with CXCR5 deficiency, led to a significant prolongation of survival of young mice, confirming the importance of the CXCL13-CXCR5 axis in B-ALL. In line with our murine results, we found that human macrophages and CXCL13 levels were higher in pediatric B-ALL patients than in adults. Consistent with our murine data, the expression level of CXCR5 may act as a prognostic marker in B-ALL, as well as a predictive marker for central nervous system relapse in human B-ALL. The overall findings show that a young BMM, and in particular macrophages, influences B-ALL progression. We specifically identified CXCL13, secreted by young macrophages, as a promoter of proliferation of B-ALL cells, influencing survival in B-ALL via CXCR5. The CXCR5-CXCL13 axis may be relevant in human B-ALL, and higher CXCR5 expression in human B-ALL may act as a predictive marker.
Precise control of blood clotting and rapid reversal of anticoagulation are essential in many clinical situations. We were successful in modifying a thrombin-binding aptamer with a red-light photocleavable linker derived from Cy7 by Cu-catalyzed Click chemistry. We were able to show that we can successfully deactivate the modified aptamer with red light (660 nm) even in human blood—restoring the blood's natural coagulation capability.
In this report, we perform structure validation of recently reported RNA phosphorothioate (PT) modifications, a new set of epitranscriptome marks found in bacteria and eukaryotes including humans. By comparing synthetic PT-containing diribonucleotides with native species in RNA hydrolysates by high-resolution mass spectrometry (MS), metabolic stable isotope labeling, and PT-specific iodine-desulfurization, we disprove the existence of PTs in RNA from E. coli, S. cerevisiae, human cell lines, and mouse brain. Furthermore, we discuss how an MS artifact led to the initial misidentification of 2′-O-methylated diribonucleotides as RNA phosphorothioates. To aid structure validation of new nucleic acid modifications, we present a detailed guideline for MS analysis of RNA hydrolysates, emphasizing how the chosen RNA hydrolysis protocol can be a decisive factor in discovering and quantifying RNA modifications in biological samples.
The intriguing (μ-hydrido)diboranes(4) with their prominent pristine representative [B2H5]− have mainly been studied theoretically. We now describe the behavior of the planarized tetraaryl (μ-hydrido)diborane(4) anion [1H]− in cycloaddition reactions with the homologous series of heterocumulenes CO2, iPrNCO, and iPrNCNiPr. We show that a C=O bond of CO2 selectively activates the B−B bond of [1H]−, while the μ-H ligand is left untouched ([2H]−). The carbodiimide iPrNCNiPr, in contrast, neglects the B−B bond and rather adds the B-bonded H− ion to its central C atom to generate a formamidinate bridge across the B2 pair ([3]−). As a hybrid, the isocyanate iPrNCO combines the reactivity patterns of both its congeners and gives two products: one of them ([4H]−) is related to [2H]−, the other ([5]−) is an analog of [3]−. We finally propose a mechanistic scenario that rationalizes the individual reaction outcomes and combines them to a coherent picture of B–B vs. B–H bond activation.
The crystal structures of sodium ethoxide (sodium ethanolate, NaOEt), sodium n-propoxide (sodium n-propanolate, NaOnPr), sodium n-butoxide (sodium n-butanolate, NaOnBu) and sodium n-pentoxide (sodium n-amylate, NaOnAm) were determined from powder X-ray diffraction data. NaOEt crystallizes in space group P421m, with Z = 2, and the other alkoxides crystallize in P4/nmm, with Z = 2. To resolve space-group ambiguities, a Bärnighausen tree was set up, and Rietveld refinements were performed with different models. In all structures, the Na and O atoms form a quadratic net, with the alkyl groups pointing outwards on both sides (anti-PbO type). The alkyl groups are disordered. The disorder becomes even more pronounced with increasing chain length. Recrystallization from the corresponding alcohols yielded four sodium alkoxide solvates: sodium ethoxide ethanol disolvate (NaOEt·2EtOH), sodium n-propoxide n-propanol disolvate (NaOnPr·2nPrOH), sodium isopropoxide isopropanol pentasolvate (NaOiPr·5iPrOH) and sodium tert-amylate tert-amyl alcohol monosolvate (NaOtAm·tAmOH, tAm = 2-methyl-2-butyl). Their crystal structures were determined by single-crystal X-ray diffraction. All these solvates form chain structures consisting of Na+, –O− and –OH groups, encased by alkyl groups. The hydrogen-bond networks diverge widely among the solvate structures. The hydrogen-bond topology of the iPrOH network in NaOiPr·5iPrOH shows branched hydrogen bonds and differs considerably from the networks in pure crystalline iPrOH.
Cytochrome c oxidases are among the most important and fundamental enzymes of life. Integrated into membranes they use four electrons from cytochrome c molecules to reduce molecular oxygen (dioxygen) to water. Their catalytic cycle has been considered to start with the oxidized form. Subsequent electron transfers lead to the E-state, the R-state (which binds oxygen), the P-state (with an already split dioxygen bond), the F-state and the O-state again. Here, we determined structures of up to 1.9 Å resolution of these intermediates by single particle cryo-EM. Our results suggest that in the O-state the active site contains a peroxide dianion and in the P-state possibly an intact dioxygen molecule, the F-state may contain a superoxide anion.
Lack of efficacy of a partial adenosine A1 receptor agonist in neuropathic pain models in mice
(2021)
Previous studies suggest that adenosine A1 receptors (A1R) modulate the processing of pain. The aim of this study was to characterize the distribution of A1R in nociceptive tissues and to evaluate whether targeting A1R with the partial agonist capadenoson may reduce neuropathic pain in mice. The cellular distribution of A1R in dorsal root ganglia (DRG) and the spinal cord was analyzed using fluorescent in situ hybridization. In behavioral experiments, neuropathic pain was induced by spared nerve injury or intraperitoneal injection of paclitaxel, and tactile hypersensitivities were determined using a dynamic plantar aesthesiometer. Whole-cell patch-clamp recordings were performed to assess electrophysiological properties of dissociated DRG neurons. We found A1R to be expressed in populations of DRG neurons and dorsal horn neurons involved in the processing of pain. However, administration of capadenoson at established in vivo doses (0.03–1.0 mg/kg) did not alter mechanical hypersensitivity in the spared nerve injury and paclitaxel models of neuropathic pain, whereas the standard analgesic pregabalin significantly inhibited the pain behavior. Moreover, capadenoson failed to affect potassium currents in DRG neurons, in contrast to a full A1R agonist. Despite expression of A1R in nociceptive neurons, our data do not support the hypothesis that pharmacological intervention with partial A1R agonists might be a valuable approach for the treatment of neuropathic pain.
The stem-loop (SL1) is the 5'-terminal structural element within the single-stranded SARS-CoV-2 RNA genome. It is formed by nucleotides 7–33 and consists of two short helical segments interrupted by an asymmetric internal loop. This architecture is conserved among Betacoronaviruses. SL1 is present in genomic SARS-CoV-2 RNA as well as in all subgenomic mRNA species produced by the virus during replication, thus representing a ubiquitous cis-regulatory RNA with potential functions at all stages of the viral life cycle. We present here the 1H, 13C and 15N chemical shift assignment of the 29 nucleotides-RNA construct 5_SL1, which denotes the native 27mer SL1 stabilized by an additional terminal G-C base-pair.
Glutathione has long been suspected to be the primary low molecular weight compound present in all cells promoting the oxidative protein folding, but twenty years ago it was found “not guilty”. Now, new surprising evidence repeats its request to be the “smoking gun” which reopens the criminal trial revealing the crucial involvement of this tripeptide.
In this thesis, we characterized megasynthases such as fatty acid synthases (FASs) and polyketide synthases. The obtained insights into structure and function were used to engineer such systems to produce new-to-nature compounds.
The in vitro characterization of megasynthases requires reproducible access to these enzymes in high quality. Therefore, we established purification strategies for the yeast FAS and the methylsalicylic acid synthase (MSAS) from Saccharopolyspora erythraea (SerMSAS) and applied the latter one on MSAS from Penicillium patulum (PenPaMSAS) and on 6-deoxyerythronolide B synthase (DEBS) module 6. With the purified samples, we were able to obtain initial structural data for SerMSAS and solve the complete structure of the yeast FAS (PDB: 6TA1). On the example of the yeast FAS, we could show that the sample can suffer from adsorption to the water-air interface during the grid preparation for electron microscopy and presented how the use of graphene-based grids can overcome this problem. The combined structural and functional analysis of the yeast FAS showed that the structural domains trimerization module and dimerization module 2 are not essential for the assembly of the whole system. Therefore, they can potentially be used for domain exchange approaches. The in-depth functional analysis of SerMSAS revealed that not SerMSAS itself releases the product, but a 3-oxoacyl-(acyl-carrier protein) synthase like enzyme within the gene cluster transfers 6-methyl salicylic acid from SerMSAS to another carrier protein for subsequent modifications. In contrast, we showed that PenPaMSAS can release its product by hydrolysis and that non-native substrates can be incorporated although at significantly slower turnover rates compared to the native starter substrate. Our further investigation demonstrated that the substrate specificity of the acyltransferase (AT) is a critical factor for the incorporation of non-native substrates.
With the insight from the functional and structural characterization, we engineered megasynthases for the biosynthesis of natural product derivatives. We targeted the AT of PenPaMSAS for active site mutagenesis and discovered a mutant which can transfer non-native substrates significantly faster (~200-300%). Additionally, the malonyl/acetyl transferase (MAT) of the mammalian FAS was used as a promising target for protein engineering because of its previously reported properties including polyspecificity, fast transfer kinetics, robustness, and plasticity. We showed that the MAT can transfer fluorinated substrates and accept the acyl carrier protein of DEBS module 6. By exchanging the substrate specific AT of DEBS with the polyspecific MAT of the mammalian FAS, we demonstrated an efficient DEBS/FAS hybrid and an optimal truncation site for the applied ATs. In contrast to the wild type system, the DEBS/FAS enzyme was able to synthesize demethylated and fluorinated derivatives. The production and purification of a fluoro-methyl-disubstituted polyketide was of particular interest, as it has a high potential for the generation of new drugs and shows the potential of protein engineering. Furthermore, the incorporation of the disubstituted substrate had important implication in the mechanistic details of the ketosynthase-mediated C-C bond formation.
Specialized transporter proteins facilitate controlled uptake and extrusion of molecules across biological membranes that would otherwise be impermeable to them. The superfamily of solute carriers (SLC) comprises the second largest group of membrane proteins in humans, acting on a variety of small polar and non-polar molecules and ions. Because of their central role in metabolism, malfunctioning of these proteins often is pathogenic. The interest in SLC transporters as drug targets – as well as for drug delivery – has therefore increased in the past years. For many SLC subfamilies, however, structural and functional information remains scarce to date.
The here presented data provides important insights into different aspects of the transport mechanism of the SLC23 and SLC26 protein families. Importantly, we show that SLC23 nucleobase transporters, in contrast to what was been previously reported, work as uniporters rather than as proton-coupled symporters. In order to do so, we developed the first and only in vitro transport assay for the SLC23 family, which enables investigation of protein function in a defined environment. Moreover, we provide a hypothesis on the role of the extremely conserved negative charged substrate binding site residue found not only in the SLC23, but also SLC4 and SLC26 families. Based on a detailed analysis of binding and transport we conclude that this conserved negative charged has a relevance for protein stability rather than for substrate binding, which explains its conservation for all three protein families that otherwise differ in their substrate specificities and modes of transport. Lastly, we investigated the relevance of oligomerization for the SLC23 and SLC26 families, highlighting the importance of the STAS domain for forming active dimers in the SLC26 anion transporter family.
In this thesis, molecular dynamics (MD) simulations are used to study the interaction of different proteins with lipid bilayers. MD simulations can be used as a “computational microscope” to gain atomistic insights into the interactions between proteins and lipids that can barely be accessed in such detail by experimental methods. The different chapters of this thesis address the lipid sensing functionality of amphipathic helices (AHs) when bound to membranes, the folding of AHs at lipid-water interfaces as well as the conformational dynamics of the HIV-1 Env glycoproteins in viral-like and experimental bilayers. In the last chapter the possibilities to enhance the performance of MD simulations are explored, leading to a more efficient usage of computational resources.
Leukemia patients bearing the t(4;11)(q21;q23) translocations can be divided into two subgroups: those expressing both reciprocal fusion genes, and those that have only the MLL-AF4 fusion gene. Moreover, a recent study has demonstrated that patients expressing both fusion genes have a better outcome than patients that are expressing the MLL-AF4 fusion protein alone. All this may point to a clonal process where the reciprocal fusion gene AF4-MLL could be lost during disease progression, as this loss may select for a more aggressive type of leukemia. Therefore, we were interested in unraveling the decisive role of the AF4-MLL fusion protein at an early timepoint of disease development. We designed an experimental model system where the MLL-AF4 fusion protein was constitutively expressed, while an inducible AF4-MLL fusion gene was induced for only 48 h. Subsequently, we investigated genome-wide changes by RNA- and ATAC-Seq experiments at distinct timepoints. These analyses revealed that the expression of AF4-MLL for only 48 h was sufficient to significantly change the genomic landscape (transcription and chromatin) even on a longer time scale. Thus, we have to conclude that the AF4-MLL fusion protein works through a hit-and-run mechanism, probably necessary to set up pre-leukemic conditions, but being dispensable for later disease progression.
Introns of human transfer RNA precursors (pre-tRNAs) are excised by the tRNA splicing endonuclease TSEN in complex with the RNA kinase CLP1. Mutations in TSEN/CLP1 occur in patients with pontocerebellar hypoplasia (PCH), however, their role in the disease is unclear. Here, we show that intron excision is catalyzed by tetrameric TSEN assembled from inactive heterodimers independently of CLP1. Splice site recognition involves the mature domain and the anticodon-intron base pair of pre-tRNAs. The 2.1-Å resolution X-ray crystal structure of a TSEN15–34 heterodimer and differential scanning fluorimetry analyses show that PCH mutations cause thermal destabilization. While endonuclease activity in recombinant mutant TSEN is unaltered, we observe assembly defects and reduced pre-tRNA cleavage activity resulting in an imbalanced pre-tRNA pool in PCH patient-derived fibroblasts. Our work defines the molecular principles of intron excision in humans and provides evidence that modulation of TSEN stability may contribute to PCH phenotypes.
Für jeden Betroffenen ist die Diagnose Krebs ein schwerwiegender Einschnitt in der Lebensqualität und -führung, da die Behandlung oftmals mit langen Chemotherapien einhergeht. Moderne Durchbrüche in der Krebsbehandlung stammen aus dem Forschungsbereich der zielgerichteten Molekulartherapie oder aus dem Gebiet der Immuntherapien, die zu beachtlichen Erfolgen bei der Behandlung von Krebspatienten führten. Trotzdem bleiben auf dem Gebiet der Onkologie weiterhin Fragen zu den grundlegenden biologischen Prozessen unbeantwortet.
Zu den Onkoproteinen, die das Tumorwachstum in Leukemiezellen stark beeinflussen, gehören die Proteine der Klasse der mixed lineage leukemia (MLL) Histonmethyltransferasen. Genetische Fusionen des mll Gens, sogenannte Rearragments, führen zu MLL-fusion Produkten, die erheblich zum Verlauf der aggressiven akuten myeloischen Leukämie (AML) beitragen. Ein weiteres Onkoprotein, das für den Krankheitsverlauf vieler Krebsarten relevant ist, ist die Transkriptionsfaktorfamilie MYC. Überexprimierung von MYC wurde in einem Drittel aller humanen Tumore beobachtet. Zahlreiche Studien belegen, dass hohe MYC Level die Expression von Genen regulieren, die essentiell für den Transformationsprozess und somit das Tumorwachstum sind. Da der Transkriptionsfaktor weder eine sabile tertiäre Proteinstruktur noch eine für Inhibitoren adressierbare Bindetasche aufweist, gilt MYC bis heute als undruggable.
Sowohl die Histonmethyltransferase MLL1, als auch der Transkriptionsfaktor MYC interagieren mit einem ca. 37 kDa Protein namens WD40-repeat containing Protein 5 (WDR5), das durch seine propellerförmige Struktur eine Oberfläche mit insgesamt zwei Bindestellen aufweist. Mehrere Studien zeigten, dass WDR5 die Stabilität und somit die Funktion epigenetischer Proteinkomplexe wie SET/ MLL und NSL gewährleistet. In diesem Kontext wurde WDR5 als relevantes Target für die MLL-rearragend akute lymphatische Leukämie (ALL) postuliert. Weitere Studien zeigten zusätzliche Rollen von WDR5, wie die Interaktion zwischen WDR5 und dem Onkoprotein MYC sowie dessen Rekrutierung zum Chromatin. Seit 2015 wurden erfolgreich mehrere niedermolekulare Wirkstoffe für die Inhibierung von WDR5 entwickelt. Dabei zielten die meisten der literaturbekannten Inhibitoren auf die Argininmotiv-erkennende WDR5-interacting (Win) Bindestelle, eine große, hydrophobe Bindetasche im Zentrum des WDR5-Propellers. Die Resultate der besser erforschten Win Inhibitoren zeigten, dass WDR5 ein erfolgsversprechendes Target zur Inhibierung von leukämischen (MLL-r-abhängigen) und neuroblastomatischen (MYC-abhängigen) Zellwachstum ist.
Da beide Bindestellen des WDR5 Proteins Interaktionen mit onkologisch bedeutsamen Faktoren eingehen, würde eine einseitige Inhibierung nur die Effekte der jeweiligen Bindestelle aufzeigen. Diese Limitierung könnte jedoch durch die Entwicklung von WDR5 PROTACs (Proteolysis targeting chimeras) aufgehoben werden, da alle Gerüstfunktionen des Proteins und Protein-Protein-Interaktionen durch die Degradierung von WDR5 entfernt werden würden. Dabei induzieren die heterobifunktionellen Moleküle den Abbau des Zielproteins über das zelleigene Ubiquitin-Proteasom-System, statt die Enzymfunktion zu inhibieren. Nach dem zelleigenen Abbau des Zielproteins wird der PROTAC freigesetzt und kann einen neuen Zyklus der Proteindegradation einleiten, was die erforderliche Menge an Wirkstoff verringert.
Diese Dissertation beschäftigte sich mit dem Design, der Synthese sowie der biophysikalischen und biologischen Evaluierung von WDR5 PROTACs. Ausgehend von literaturbekannten WDR5 Liganden wurden zwei verschiedene PROTAC Typen entworfen. Diese beiden Molekültypen besitzen einen unterschiedlichen geometrischen Austrittswinkel, wodurch die Chance auf eine erfolgreiche Komplexbildung zwischen WDR5, PROTAC und E3 Ligase erhöht wird. Als Leitstruktur fungierten die Verbindungen OICR-9429 sowie DDO-2117 und ausgehend von Ligand (6d) wurden heterobifunktionelle Moleküle mit verschiedenen Linkersystemen ([PEG]- und alkyl-basiert, sowie aromatisch verbrückt) und verschiedenen E3 Ligase Liganden (Cereblon, VHL und MDM2) synthetisiert. Die anschließenden biochemischen und biophysikalischen Evaluierungen der verschiedenen PROTACs durch Thermofluor (DSF) und ITC zeigten eine hohe in vitro Affinität einiger Moleküle. Die zelluläre Permeabilität der großen Moleküle wurde in einem hier etablierten BRET Assay untersucht. Zur Assay-Etablierung wurden drei Tracer (21a-c), basierend auf BODIPY Konjugaten, synthetisiert und getestet, bevor die PROTACs in intakten und lysierten Zellen vermessen wurden. Während die zellulären Affinitäten von Cereblon- und VHL-adressierenden PROTACs sich im niedrigen μM Bereich bewegten, wurden die nicht zellgängigen MDM2 PROTACs von weiteren Experimenten ausgeschlossen.
Die Degradierungeffizienz der WDR5 PROTACs (7a-e) und (8a-j) wurden in der Leukämie Zellinie MV4-11 untersucht, da diese die am meisten auftretende MLL fusion Mutation AF4 birgt. Dabei wurde der Proteinabbau von WDR5 über den HiBiT Assay sowie Western Blots nachgewiesen. ...
Inducing cell death in tumor cells is a major goal of anti-cancer therapy. However, the preferable mode of cell death to induce is under debate. Apoptosis is known to be an anti-inflammatory and pro-resolving type of programmed cell death, whereas necroptosis results in the release of danger-associated molecular patterns (DAMPs) and is pro-inflammatory. Efferocytosis of apoptotic cells by macrophages results in a pro-resolving switch of macrophages polarization and is required to induce resolution of inflammation. This impact of apoptotic cells on macrophages is a non-desired consequence of cell death in tumors, which are often characterized by an overshooting wound healing response. Moreover, apoptosis resistance is frequently observed in cancer cells. To overcome apoptosis resistance in cancer cells, necroptosis can be induced as an alternative mechanism for cancer treatment. Interferons (IFNs) play an important role in tumor immune responses and act by inducing the expression of IFN-stiumlated genes (ISGs). Furthermore, IFNs were shown to be able to induce necroptosis together with Smac-mimetics when caspases are inhibited in different cancer cell lines. Necroptosis is induced by phosphorylation and activation of receptor-interacting serine/threonine-protein kinase 1 (RIPK1), RIPK3 and pseudokinase mixed lineage kinase domain-like (MLKL).
In my thesis, we first identified MLKL as an ISG in various cancer cell lines. MLKL upregulation was found to be a general feature of IFN signaling since both type I and type II IFNs increase the expression of MLKL. IFNy was able to upregulate MLKL at messenger ribonucleic acid (mRNA) and protein level indicating that MLKL is elevated transcriptionally. Indeed, Actinomycin D chase experiments showed that inhibition of transcription abolished MLKL upregulation upon IFN treatment. Both, knockdown of the IFNy-activated transcription factors interferon regulatory factor 1 (IRF1) and signal transducer and activator of transcription 1 (STAT1) as well as knockout of IRF1 significantly dampened MLKL mRNA upregulation, demonstrating that STAT1 and especially IRF1 are necessary to induce MLKL expression. This first part of the study highlights the upregulation of MLKL by IFNy as valuable tool to sensitize cells towards necroptosis and by that overcome apoptosis resistance in cancers.
When compared to apoptosis, the immune response to necroptotic cells and the polarization of macrophages phagocytosing necroptotic cells is not well studied. In most studies, cell death was induced by biological or chemical compounds, which may lead to artifacts by affecting the macrophages and triggering of unrelated signaling pathways. Therefore, in the second part of my thesis we used a pure cell death system of NIH 3T3 cells expressing either dimerizable caspase 8 or oligomerizable RIPK3 to induce cell death. Addition of B/B-Homodimerizer (dimerizer) to the cells resulted in apoptosis or necroptosis, which was confirmed by caspase 3/7 activation, phosphorylation of MLKL and inhibitor experiments, respectively. We analyzed the effect of dying cells on peritoneal macrophages by establishing a co-culture in a transwell system. The genetic profile of macrophages co-cultured with dying cells was evaluated by whole transcriptome RNA sequencing. In macrophages co-cultured with necroptotic cells genes corresponding to chemotaxis and hypoxia pathways were upregulated. A significant proportion of hypoxia-related pathways are mediated by hypoxia-inducible factor 1-alpha (HIF-1α), which also induces metabolic changes in polarized macrophages. We could show that macrophages co-cultured with necroptotic cells showed a decreased mitochondrial respiration, indicating an inflammatory (M1) polarization. Protein levels of chemokine C-X-C motif ligand 1 (CXCL1), which was increased in the RNA sequencing data, were also upregulated in supernatant of co-cultured macrophages and of necroptotic cells, demonstrating that necroptotic cells both secrete CXCL1 and induce gene expression of CXCL1 in peritoneal macrophages. This may influence the recruitment of neutrophils as inhibition of necroptosis during Zymosan-A-induced peritonits in mice decreased the levels of neutrophils at day 1 of this model of self-resolving inflammation.
Furthermore, RNA sequencing revealed an unexpected impact of apoptotic cells on macrophage biology as cell cycle and cell division pathways were increased. Enhanced proliferation of macrophages was confirmed by two functional assay with peritoneal macrophages isolated from mice and IC-21 macrophages. Inhibition of apoptosis during Zymosan-A-induced peritonits in mice demonstrated decreased mRNA levels of cell cycle mediators in peritoneal macrophages. Simultaneously with cell cycle activation, gene sets of prostaglandin E2 (PGE2) signaling were upregulated during RNA sequencing. In the second part of my thesis we could demonstrate, that apoptotic cells induce transcription of cell cycle genes and proliferation of macrophages and necroptotic cells are able to influence the chemokine profile of macrophages and thereby the recruitment of neutrophils.
Chronic rhinosinusitis (CRS) is often treated by functional endoscopic paranasal sinus surgery, which improves endoscopic parameters and quality of life, while olfactory function was suggested as a further criterion of treatment success. In a prospective cohort study, 37 parameters from four categories were recorded from 60 men and 98 women before and four months after endoscopic sinus surgery, including endoscopic measures of nasal anatomy/pathology, assessments of olfactory function, quality of life, and socio-demographic or concomitant conditions. Parameters containing relevant information about changes associated with surgery were examined using unsupervised and supervised methods, including machine-learning techniques for feature selection. The analyzed cohort included 52 men and 38 women. Changes in the endoscopic Lildholdt score allowed separation of baseline from postoperative data with a cross-validated accuracy of 85%. Further relevant information included primary nasal symptoms from SNOT-20 assessments, and self-assessments of olfactory function. Overall improvement in these relevant parameters was observed in 95% of patients. A ranked list of criteria was developed as a proposal to assess the outcome of functional endoscopic sinus surgery in CRS patients with nasal polyposis. Three different facets were captured, including the Lildholdt score as an endoscopic measure and, in addition, disease-specific quality of life and subjectively perceived olfactory function.
The family of phytochrome photoreceptors contains proteins with different domain architectures and spectral properties. Knotless phytochromes are one of the three main subgroups classified by their distinct lack of the PAS domain in their photosensory core module, which is in contrast to the canonical PAS-GAF-PHY array. Despite intensive research on the ultrafast photodynamics of phytochromes, little is known about the primary kinetics in knotless phytochromes. Here, we present the ultrafast Pr ⇆ Pfr photodynamics of SynCph2, the best-known knotless phytochrome. Our results show that the excited state lifetime of Pr* (~200 ps) is similar to bacteriophytochromes, but much longer than in most canonical phytochromes. We assign the slow Pr* kinetics to relaxation processes of the chromophore-binding pocket that controls the bilin chromophore’s isomerization step. The Pfr photoconversion dynamics starts with a faster excited state relaxation than in canonical phytochromes, but, despite the differences in the respective domain architectures, proceeds via similar ground state intermediate steps up to Meta-F. Based on our observations, we propose that the kinetic features and overall dynamics of the ultrafast photoreaction are determined to a great extent by the geometrical context (i.e., available space and flexibility) within the binding pocket, while the general reaction steps following the photoexcitation are most likely conserved among the red/far-red phytochromes.
2-Aminobenzimidazole 10, although a weak catalyst in the monomeric state, is a successful building block for effective artificial ribonucleases. In an effort to identify new building blocks with improved catalytic potential, RNA cleavage by a variety of heterocyclic amidines and guanidines has been studied. In addition to pKa values and steric effects, the energy difference between tautomeric forms seems to be another important parameter for catalysis. This information is available from quantum chemical calculations on higher levels, but semiempirical methods are sufficient to get a first estimate. According to this assumption, imidazoimidazol 18, characterized by isoenergetic tautomeric forms, is superior to 2-aminoimidazol 6, the best candidate among the simple compounds. By far the largest effects are seen with 2-aminoperimidine 24, which rapidly cleaves RNA even in the micromolar concentration range. The impressive reactivity, however, is related to a tendency of compound 24 to form polycationic aggregates which are the actual catalysts.
2-Aminobenzimidazole 10, although a weak catalyst in the monomeric state, is a successful building block for effective artificial ribonucleases. In an effort to identify new building blocks with improved catalytic potential, RNA cleavage by a variety of heterocyclic amidines and guanidines has been studied. In addition to pKa values and steric effects, the energy difference between tautomeric forms seems to be another important parameter for catalysis. This information is available from quantum chemical calculations on higher levels, but semiempirical methods are sufficient to get a first estimate. According to this assumption, imidazoimidazol 18, characterized by isoenergetic tautomeric forms, is superior to 2-aminoimidazol 6, the best candidate among the simple compounds. By far the largest effects are seen with 2-aminoperimidine 24, which rapidly cleaves RNA even in the micromolar concentration range. The impressive reactivity, however, is related to a tendency of compound 24 to form polycationic aggregates which are the actual catalysts.
In dieser Arbeit wird sowohl das Potenzial von molekularen Photoschaltern als lichtempfindliche Komponenten für photopharmakologische Anwendungen als auch das von künstlichen RNA-Aptameren als regulatorische Schalteinheiten für die Entwicklung von funktionellen Riboschaltern untersucht. Verschiedene wesentliche Aspekte beider Anwendungs-felder wurden eingehend einzeln untersucht und die beiden Schaltsysteme schließlich durch das Design eines synthetischen RNA-Aptamers kombiniert, dessen Ligandbindung durch licht-induzierte Isomerisierung seines Photoschalterliganden reguliert werden kann.
Molekulare Photoschalter wie Azobenzole und Spiropyrane haben sich als vielversprechende photochemische Werkzeuge erwiesen, um lichtgesteuert reversible und biochemisch nutzbare Effekte erzeugen. Spiropyrane bergen aufgrund der drastischen Veränderungen ihrer molekularen Eigenschaften infolge der Photoisomerisierung zum Merocyanin (MC) ein enormes Anwendungs-potenzial. Von den hier untersuchten wasserlöslichen Pyridin- (Py-) und Nitro-BIPS-Derivaten zeigt insbesondere die Py-BIPS-Verbindung 2 ein außerordentlich vielseitiges Verhalten. Im Vergleich zu anderen Vertretern dieser Photoschalterklasse wird ein deutlich höherer MC-Anteil von etwa 50% thermisch innerhalb von wenigen Minuten akkumuliert. Durch lichtinduzierten Ringschluss zum reinen Spiropyran (SP) und thermische Wiederherstellung des Gleichgewichts, kann diese hohe Schaltamplitude über mehrere Zyklen ohne signifikante Zersetzung beibehalten werden. Der Einsatz von schädlichem UV-Licht kann somit vermieden werden, was zusätzlich sehr vorteilhaft für einen möglichen Einsatz in einem biochemischen Kontext ist.
Verbindung 2 weist zudem mehrere Protonierungsstellen auf, die ihr in Abhängigkeit des pH-Wertes faszinierende photosaure Eigenschaften verleihen. Das einfach protonierte HMC Isomer ermöglicht eine lichtstimulierte reversible Kontrolle des pH-Wertes in einem Bereich von etwa 4,5 bis 7,5, mit möglichen pH-Sprüngen von bis zu 1,5 Einheiten. Durch transiente Absorptionsstudien wurde ein Mechanismus für die Protonenfreisetzung nachgewiesen, der lediglich auf der Veränderung des pKs-Wertes der N-protischen Position infolge des lichtinduzierten Ringschlusses beruht. Im Gegensatz dazu wird das phenolische Proton des doppelt protonierten HMCH Isomers innerhalb von 1-2 Pikosekunden nach Anregung aus dem angeregten Zustand an das Lösemittel übertragen. Durch eingehende Ultrakurzzeitmessungen der Freisetzung des phenolischen Protons, konnten die protonierten Spezies der Py- und Nitro-Merocyanine als Superphotosäuren etabliert werden. Sie können somit als ultraschnelle Auslöser für protonenvermittelte Prozesse eingesetzt werden, die zu den fundamentalsten Reaktionen in der Natur gehören.
Was potenzielle pharmakologische Zielsysteme betrifft, so dürfte RNA eine große Zukunft bevorstehen, da sie einfach zu synthetisieren ist und Zugang zu verschiedenen Ebenen zellulärer Regulationsmechanismen bietet. Insbesondere RNA-Aptamere, die in der Lage sind, niedermolekulare Liganden mit außergewöhnlich hoher Affinität und Spezifität zu binden, sind für die Entwicklung von künstlichen Riboschaltern hoch interessant. Während künstliche Aptamere für beliebige Liganden durch einen in vitro Selektionsprozess generiert werden können, ist nicht zur Gänze geklärt warum nur wenige von ihnen als aktive in vivo Riboschalter funktionieren. Die vorliegenden Ergebnisse zeigen die Bedeutung der konformationellen Aptamerdynamik während der Ligandenbindung für das Regulationspotential. Die Mg2+-abhängigen Bindungsstudien des hochfunktionellen Tetrazyklin (TC) -Aptamers zeigen, dass zweiwertige Kationen nicht nur für die korrekte Vorfaltung des Aptamers wichtig sind, sondern auch an der Ligandenbindung und RNA-Strukturanpassung selbst beteiligt sein können. Nach der Assoziation von TC an die Bindungstasche pflanzt sich eine Konformationsanpassung zur entfernten Dreifachhelixregion fort, wo Mg2+ zusätzlich für die Ausbildung endgültig gebundenen Zustandes benötigt wird.
Neben dem Einfluss von Mg2+, zeigen zeitaufgelöste Ligandenbindungsstudien von drei Ciprofloxacin (CFX) -Aptameren eine klare Korrelation zwischen der Kinetik des Struktur-anpassungsschrittes der RNA an den Liganden und dem beobachteten Regulationspotenzial in parallel durchgeführten in vivo Assays. Es wird geschlussfolgert, dass eine beschleunigte und irreversible RNA-Anpassung auf eine Konformationsänderung hindeutet, die ausgeprägt genug ist, um eine Aktivität als Riboschalter zu ermöglichen. Diese Erkenntnisse werden durch die berichteten Ligandenbindungskinetiken von anderen künstlichen Aptameren und auch von natürlichen Riboschaltern bestätigt und sollten weitreichende Implikationen für die Optimierung von Selektionsprotokollen für funktionelle Aptamere haben.
Schließlich wird ein lichtempfindliches RNA-Aptamer vorgestellt, dessen Ligand auf dem Antibiotikum Chloramphenicol (Cm) basiert, welches synthetisch mit einem Azobenzolfragment versehen wurde (azoCm). Durch systematische Optimierung von in vitro Selektionsprotokollen und die erfolgreiche Implementierung eines Belichtungsschrittes zur Isomerisierung des Liganden konnten Aptamere erhalten werden, die spezifisch an die trans-Form von azoCm binden. Bindungsaffinitätsstudien bestätigen diese Selektivität und durch Zirkulardichroismusstudien konnte zudem eine lichtinduzierte reversible Dissoziation des von cis-azoCm gezeigt werden. Damit wird hier eine erfolgreiche Entwicklungsstrategie für lichtabhängige RNA-Aptamer – Ligandsysteme dargelegt, welche wiederum fundamental neuartige Ansätze für die Erschließung lichtstimulierter biologischer Regulationswege zugänglich machen.
An automated NMR chemical shift assignment algorithm was developed using multi-objective optimization techniques. The problem is modeled as a combinatorial optimization problem and its objective parameters are defined separately in different score functions. Some of the heuristic approaches of evolutionary optimization are employed in this problem model. Both, a conventional genetic algorithm and multi-objective methods, i.e., the non-dominated sorting genetic algorithms II and III (NSGA2 and NSGA3), are applied to the problem. The multi-objective approaches consider each objective parameter separately, whereas the genetic algorithm followed a conventional way, where all objectives are combined in one score function. Several improvement steps and repetitions on these algorithms are performed and their combinations are also created as a hyper-heuristic approach to the problem. Additionally, a hill-climbing algorithm is also applied after the evolutionary algorithm steps. The algorithms are tested on several different datasets with a set of 11 commonly used spectra. The test results showed that our algorithm could assign both sidechain and backbone atoms fully automatically without any manual interactions. Our approaches could provide around a 65% success rate and could assign some of the atoms that could not be assigned by other methods.
An accurate measurement of the 140Ce(n,γ) energy-dependent cross-section was performed at the n_TOF facility at CERN. This cross-section is of great importance because it represents a bottleneck for the s-process nucleosynthesis and determines to a large extent the cerium abundance in stars. The measurement was motivated by the significant difference between the cerium abundance measured in globular clusters and the value predicted by theoretical stellar models. This discrepancy can be ascribed to an overestimation of the 140Ce capture cross-section due to a lack of accurate nuclear data. For this measurement, we used a sample of cerium oxide enriched in 140Ce to 99.4%. The experimental apparatus consisted of four deuterated benzene liquid scintillator detectors, which allowed us to overcome the difficulties present in the previous measurements, thanks to their very low neutron sensitivity. The accurate analysis of the p-wave resonances and the calculation of their average parameters are fundamental to improve the evaluation of the 140Ce Maxwellian-averaged cross-section.
The new class of microbial rhodopsins, called xenorhodopsins (XeRs),[1] extends the versatility of this family by inward H+ pumps.[2–4] These pumps are an alternative optogenetic tool to the light-gated ion channels (e.g. ChR1,2), because the activation of electrically excitable cells by XeRs is independent from the surrounding physiological conditions. In this work we functionally and spectroscopically characterized XeR from Nanosalina (NsXeR).[1] The photodynamic behavior of NsXeR was investigated on the ps to s time scale elucidating the formation of the J and K and a previously unknown long-lived intermediate. The pH dependent kinetics reveal that alkalization of the surrounding medium accelerates the photocycle and the pump turnover. In patch-clamp experiments the blue-light illumination of NsXeR in the M state shows a potential-dependent vectoriality of the photocurrent transients, suggesting a variable accessibility of reprotonation of the retinal Schiff base. Insights on the kinetically independent switching mechanism could furthermore be obtained by mutational studies on the putative intracellular H+ acceptor D220.
Photoactivatable compounds for example photoswitches or photolabile protecting groups (PPGs, photocages) for spatiotemporal light control, play a crucial role in different areas of research. For each application, parameters such as the absorption spectrum, solubility in the respective media and/or photochemical quantum yields for several competing processes need to be optimized. The design of new photochemical tools therefore remains an important task. In this study, we exploited the concept of excited-state-aromaticity, first described by N. Colin Baird in 1971, to investigate a new class of photocages, based on cyclic, ground-state-antiaromatic systems. Several thio- and nitrogen-functionalized compounds were synthesized, photochemically characterized and further optimized, supported by quantum chemical calculations. After choosing the optimal scaffold, which shows an excellent uncaging quantum yield of 28 %, we achieved a bathochromic shift of over 100 nm, resulting in a robust, well accessible, visible light absorbing, compact new photocage with a clean photoreaction and a high quantum product (ϵ⋅Φ) of 893 M−1 cm−1 at 405 nm.
The new class of microbial rhodopsins, called xenorhodopsins (XeRs),[1] extends the versatility of this family by inward H+ pumps.[2–4] These pumps are an alternative optogenetic tool to the light-gated ion channels (e.g. ChR1,2), because the activation of electrically excitable cells by XeRs is independent from the surrounding physiological conditions. In this work we functionally and spectroscopically characterized XeR from Nanosalina (NsXeR).[1] The photodynamic behavior of NsXeR was investigated on the ps to s time scale elucidating the formation of the J and K and a previously unknown long-lived intermediate. The pH dependent kinetics reveal that alkalization of the surrounding medium accelerates the photocycle and the pump turnover. In patch-clamp experiments the blue-light illumination of NsXeR in the M state shows a potential-dependent vectoriality of the photocurrent transients, suggesting a variable accessibility of reprotonation of the retinal Schiff base. Insights on the kinetically independent switching mechanism could furthermore be obtained by mutational studies on the putative intracellular H+ acceptor D220.
Redirection of the transcription factor SP1 to AT rich binding sites by a synthetic adaptor molecule
(2021)
The ubiquitous transcription factor SP1 binds to a GC rich consensus sequence. Here we describe an adaptor molecule that mediates binding of SP1 to a non-cognate DNA site rich in AT. The adaptor is comprised of a Dervan-type hairpin polyamide with high affinity to an AT rich hexamer duplex. It also carries a 27mer DNA that contains the SP1 consensus sequence. The synthesis and purification of the polyamide-DNA conjugate is reported. Pulldown experiments and western blot analysis demonstrate adaptor mediated binding of SP1 to the hexamer duplex TTGTTA.
Photoactivatable compounds for example photoswitches or photolabile protecting groups (PPGs, photocages) for spatiotemporal light control, play a crucial role in different areas of research. For each application, parameters such as the absorption spectrum, solubility in the respective media and/or photochemical quantum yields for several competing processes need to be optimized. The design of new photochemical tools therefore remains an important task. In this study, we exploited the concept of excited-state-aromaticity, first described by N. Colin Baird in 1971, to investigate a new class of photocages, based on cyclic, ground-state-antiaromatic systems. Several thio- and nitrogen-functionalized compounds were synthesized, photochemically characterized and further optimized, supported by quantum chemical calculations. After choosing the optimal scaffold, which shows an excellent uncaging quantum yield of 28 %, we achieved a bathochromic shift of over 100 nm, resulting in a robust, well accessible, visible light absorbing, compact new photocage with a clean photoreaction and a high quantum product (ϵ⋅Φ) of 893 M−1 cm−1 at 405 nm.
Internationale Fachkonferenz im Hybrid-Format : Nachbericht zur Frankfurt Cancer Conference 2021
(2021)
Diese Arbeit ist ein detaillierter Bericht über die Forschungsaktivitäten, die ich während meiner Promotion am Max-Planck-Institut für Biophysik durchgeführt habe. Mit dem Aufkommen der direkten Elektronendetektoren erlebte die Transmissionselektronenmikroskopie von gefrorenen hydratisierten Proben (Kryo-EM) einen epochalen Wandel, die sogenannte “Auflösungsrevolution”. Ab den 2010er Jahren ermöglichte die Kommerzialisierung der ersten direkten Detektoren die Erforschung biologischer Phänomene in beispiellosem Detail und machte Kryo-EM zu einer der leistungsstärksten (und gefragtesten) Forschungsmethoden in den Biowissenschaften. Meine Forschung konzentrierte sich auf die Verwendung der Elektronen-Kryotomographie, um zwei herausfordernde Ziele zu erreichen. Das erste bestand darin, die Denaturierung von Proteinen an der Luft-Wasser-Grenzfläche zu untersuchen, und das zweite die molekulare Landschaft eines lichtempfindlichen Chloroplastenvorläufers, des Etioplasten, zu beschreiben. Um die Relevanz, Herausforderungen und Auswirkungen meiner Arbeit zu vermitteln, habe ich diese Arbeit in drei Kapitel unterteilt.
Kapitel eins enthält eine Einführung in die Transmission-Elektronenmikroskopie.
Nach einer kurzen Zusammenfassung der historischen Meilensteine in der Disziplin beschreibe ich die wesentlichen Komponenten des TEM und deren Funktionsweise. Hier lege ich besonderen Wert auf die Struktur elektromagnetischer Linsensysteme, wie sie den Weg der Elektronen beim Durchlaufen der Säule beeinflussen und wie Bilder entstehen. Der hardwarebezogene Teil der Einführung wird durch eine vereinfachte Beschreibung der Elektronendetektoren abgeschlossen, in der ich die revolutionären Aspekte der direkten Elektronendetektoren, mit der Struktur und Funktion von CCD-Detektoren (Charge Coupled Device detector) vergleiche. Als nächstes konzentriere ich mich auf die theoretischen Prinzipien der Bilderzeugung. Um die Hauptphänomene im Zusammenhang mit der Bildqualität in TEM hervorzuheben, stelle ich grundlegende Konzepte wie den Einfluss von Elektronenenergie und optischen Aberrationen vor, gefolgt von einer ausführlicheren Beschreibung des Ursprungs von Kontrast und Rauschen. Der Unterabschnitt schließt mit einigen Überlegungen darüber, wie - und vor allem wie effizient - Detektoren kontinuierliche Elektronenwellen in diskrete Bereiche (Pixel) abtasten. Der folgende Unterabschnitt ist der Erfassung und Verarbeitung tomografischer Daten gewidmet. Hier gebe ich eine vereinfachte Beschreibung, wie Kippserien mit dem Mikroskop erfasst werden und wie die Rohdaten zu einer dreidimensionalen Darstellung der Probe verarbeitet werden. Der Einfluss der Neigungsgeometrie und der Dosisverteilung auf die Rekonstruktionsqualität wird ebenfalls diskutiert. Der zweite Teil des Unterabschnitts befasst sich mit der Strukturbestimmung durch Subtomogramm-Mittelung und der Errechnung der Auflösung von Kryo-EM-Rekonstruktion. Zuletzt schließe ich das Kapitel mit einer Beschreibung der Vorbereitung biologischer Proben für die Kryo-EM-Bildgebung mit einigen abschließenden Bemerkungen zur Dynamik und den Grenzen der Vitrifizierung ab.
Kapitel zwei folgt dem Thema der Kryo-Präparation biologischer Proben mit der Untersuchung der Denaturierung von Proteinen an der Luft-Wasser-Grenzfläche.
Im Einführungsabschnitt skizziere ich die wichtigsten Aspekte dieses Phänomens. Frühe Experimente zum Verhalten von Proteinen in Lösung zeigten ihre Neigung, aus der Lösung zu ihrer Grenzfläche mit der Atmosphäre zu diffundieren. Hier bilden sie meist unlösliche Schichten denaturierter Fibrillen Es wurde vorgeschlagen, dass die Korrelation zwischen Proteindenaturierung und Kontakt mit der Grenzfläche auf einen allmählichen Entfaltungsprozess zurückzuführen ist, bei dem Tausende von Wechselwirkungen pro Sekunde zu einer immer größeren strukturellen Schädigung führen würden. Ein direkter Beweis für diesen Mechanismus wurde jedoch nie dokumentiert. Um einen tieferen Einblick in die Dynamik an der Luft-Wasser-Grenzfläche zu erhalten, sammelte ich Kryotomogramme vitrifizierter Präparate der Fettsäuresynthase (FAS, Fatty Acid Synthase) aus Hefe. Im ersten Unterabschnitt der Ergebnisse beschreibe ich, wie die biochemische und Negativkontrastierung-TEM-Analyse von FAS-Fraktionen zeigte, dass der Komplex während des gesamten Reinigungsverfahrens intakt und katalytisch aktiv blieb. Nach der Vitrifizierung ergab die Einzelpartikelanalyse jedoch, dass 90% aller Komplexe stark beschädigt waren. Die tomographische Rekonstruktion derselben Proben zeigte, dass alle FAS-Komplexe an die Luft-Wasser-Grenzfläche gebunden waren. Die Seite des Moleküls, die der Grenzfläche ausgesetzt war, schien abgeflacht zu sein, während die Seite, in der wässrigen Phase, ihre native Struktur beibehielt. Die Mittelung der Subtomogramme bestätigte, dass eine Seite von fast 90% der Partikel stark beschädigt war. Durch den Vergleich der Ausrichtung dieser beschädigten Seite mit der Position eines Rechenmodells der Luft-Wasser-Grenzfläche konnte ich nachweisen, dass sie perfekt übereinstimmen, was den ersten direkten Beweis dafür liefert, dass die Wechselwirkung mit der Luft-Wasser-Grenzfläche die lokale Denaturierung großer Proteinkomplexe herbeiführt.
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Die Autophagie ist ein in Eukaryonten evolutionär konservierter Prozess, bei dem es zu einem lysosomalen Abbau von cytosolischen Bestandteilen kommt. Die dabei entstehenden biochemischen Bausteine stehen anschließend erneut zum Aufbau benötigter Strukturen zur Verfügung. Verschiedene Stimuli, wie beispielsweise Nährstoffmangel, können die Aktivität der Autophagie erhöhen und ermöglicht Zellen dadurch die Aufrechterhaltung der Zellhomöostase, selbst unter Stressbedingungen. Im Verlauf der Autophagie bildet sich eine tassenförmige Doppelmembran-Struktur, das sogenannte Phagophor. Dieses wächst, um das abzubauende Material zu umschließen und wird dabei von sogenannten Atg-Proteinen (autophagy-related genes) prozessiert. Nach der Schließung spricht man vom Autophagosom, welches letztlich mit einem Lysosom verschmilzt und das Autophagolysosom bildet, welches wiederum die eingeschlossenen Bestandteile zerlegt und die recycelten Bausteine freigibt. Die einzelnen Schritte während der Autophagie sind hochgradig durch die Atg-Proteine reguliert. Eines dieser Atg-Proteine, das Atg8, ist an einigen entscheidenden Schritten wie dem Phagophor-Wachstum, der Autophagosom-Reifung sowie der Schließung beteiligt. Während es in Hefen nur ein einziges Atg8-Protein gibt, so zeigt sich in höheren Eukaryonten meist eine gewisse Diversität. So codiert beispielsweise das humane Genom mindestens sechs Atg8-Homologe. Neben den drei Proteinen der LC3-Familie (A, B, C) zählen auch GABARAP, GABARAPL1 und GABARAPL2 dazu. Die Gründe für diese Diversität sind noch nicht vollständig aufgeklärt, weshalb es wichtig ist, möglichst selektive Modulatoren zu entwickeln, um so die Aufgaben der einzelnen Homologen entschlüsseln zu können. Eine weitere wichtige Aufgabe übernimmt Atg8 beim Binden des abzubauenden Materials über sogenannte Autophagie-Rezeptoren, wie beispielsweise p62. Der Bindevorgang beruht dabei auf der Interaktion von p62 mit ubiquitinierten Zellbestandteilen auf der einen Seite und der Interaktion zwischen p62 und LC3 auf der anderen Seite. Letztgenannte beruht auf dem Binden des LIR-Motivs (LC3-interagierende Region) von p62 an die LDS (LIR-docking site) des LC3-Proteins. Das LIR-Motiv zeichnet sich durch Aminosäure-Sequenz D-D-D-W/F/Y-X1-X2-L/I/V aus. Währende die aromatische Seitenkette (W/F/Y) die hydrophobe Tasche 1 (HP1) der LDS besetzt, ragt die aliphatische Seitenkette (L/I/V) in die HP2 hinein. Damit sollte es möglich sein, die LIR-LC3-Interaktion, durch das Besetzen der LDS zu stören bzw. zu inhibieren. Solche Inhibitoren könnten zum einen der weiteren Aufklärung der Prozesse, an denen die Autophagie beteiligt ist, dienen, zum anderen jedoch auch die Untersuchung fehlerhafter Autophagie ermöglichen. Ausgangspunkt für diese Arbeit stellt die Verbindung Novobiocin dar, die im Rahmen eines Mitteldurchsatz-Screenings als potenzieller Inhibitor der LIR-LC3-Interaktion identifiziert und mittels ITC, TSA und 1H-15N-HSQC verifiziert werden konnte. Die Struktur des Novobiocins setzt sich aus dem 3-Amino-4-hydroxy-8-methylcoumarin-Kern, der über eine Amidbindung an 3-iso-Prenyl-4-Hydroxybenzoesäure gebunden ist, sowie einer O-glykosidischen Bindung in Position C7 des Coumarins mit L-Noviose zusammen. Da es sich bei Novobiocin (XL6) um ein verhältnismäßig komplexes Molekül handelt, wurde der Einfluss einzelner funktionellen Gruppen des Moleküls auf die Bindungsaffinität hin untersucht. Hierfür wurden Synthesestrategien sowohl für die Coumarin-Gerüste als auch verschiedene Benzoesäuren entwickelt. Die erhaltenen Verbindungen wurden mittels ITC und TSA untersucht. Dabei wurde die Verbindung MH507 als geeigneter Ausgangspunkt für die Untersuchung der Struktur-Aktivitätsbeziehungen (SAR) bezüglich der Benzamid-Seite identifiziert. Im Rahmen einer ersten SAR-Untersuchung wurden neben verschiedenen 3-Alkyl-benzoesäuren, auch verschiedene divalente Isostere (-O-, -S-, -NHSO2-) der benzylischen Methylengruppe synthetisiert. Diese, sowie kommerzielle Aminosäuren, wurden mit 3-Amino-4,7-dihydroxycoumarin zu den entsprechenden Endverbindungen gekuppelt. Ergänzend dazu wurden auch eine Verbindung mit umgekehrter Konstitution der Amidbindung dargestellt, um den Einfluss der Reihenfolge zu verifizieren. In einer weiteren SAR-Studie wurden Derivate synthetisiert, die zusätzlich eine Funktionalisierung am C7 des Coumarin-Gerüstes über Amidkupplung, Sulfonamid-Bildung bzw. Suzuki-Reaktion erlauben und somit eine Interaktion mit der HP1 ermöglichen könnten. Dafür wurde eine weitere Synthesestrategie zur Darstellung von 7-Nitro- bzw. 7-Brom-3-amino-4-hydroxycoumarinen ausgearbeitet und eine Reihe von Endverbindungen dargestellt. Neben den Coumarin-Derivaten wurden auch vier Peptidomimetika synthetisierten. Hierfür wurde, basierend auf den Interaktionen zwischen dem LIR-Motiv und der LC3 Proteinoberfläche, ein Pharmakophor-Modell erstellt. Neben einem Pentapeptid wurden auch drei Verbindungen dargestellt, die ein 5-Amino 2-methoxybenzohydrazid-Gerüst besitzen. Um die synthetisierten Verbindungen auf ihre inhibitorische Aktivität auf LC3A bzw. LC3B gegenüber dem LIR-Motiv von p62 hin untersuchen zu können, wurde ein HTRF-basierter Verdrängungsassay entwickelt. Dabei diente ein mit dem LIR-Motiv modifiziertes sGFP als FRET-Akzeptor, während das jeweilige Terbium-Kryptat-gelabelte SNAP-LC3-Fusionsprotein als FRET-Donor fungierte. Neben den Titrationsexperimenten zur Bestimmung der IC50-Werte wurden auch die jeweiligen Dissoziationskonstanten (Kd) von LC3A und LC3B gegenüber dem LIR-sGFP-Fusionsprotein bestimmt, um die IC50-Werte in inhibitorische Konstanten (Ki) zu überführen, da diese untereinander besser vergleichbar sind.
Die Verbindung MH209 zeigte die höchste Aktivität auf LC3A bzw. LC3B und besitzt aufgrund der Noviose-Einheit eine gute Wasserlöslichkeit, weshalb sie für die weiteren Untersuchungen ausgewählt wurde. Im Zuge von Kristallisationsexperimenten gelang die Isolierung und Vermessung eines Co-Kristalls von LC3A mit Verbindung MH209. Durch die Kristallstruktur wurden wichtige Einblicke in die intermolekularen Wechselwirkungen der 4-Hydroxycoumarine mit der LC3A- bzw. LC3B-Proteinoberfläche gewonnen und die Bindungsmode aufgeklärt. Diese Erkenntnisse passen gut zu den Ergebnissen aus den durchgeführten TSA-, ITC- und HTRF-Assays, wie beispielsweise der korrekten Konstitution der Amidbindung am C3 des Coumarin-Gerüstes. Mittels ITC wurde die Verbindung MH209 auf ihre Bindungsaffinität gegenüber den anderen humanen Homologen der Atg8-Proteinfamilie hin untersucht. Dabei zeigte sich, dass MH209 abgesehen von LC3A und LC3B keinerlei Aktivität auf den humanen Atg8-Homologen besitzt. Diese Selektivität ist nützlich, um die biologische Bedeutung der Diversität von Atg8-Homologen in höheren Eukaryonten zu untersuchen und Prozesse, in die diese involviert sind, aufzuklären.
Ziel dieser Doktorarbeit war es, die Bedeutung der Kristallstrukturbestimmung aus Pulverdaten (SDPD) herauszuarbeiten und etwaige Grenzen durch neue Methodenentwicklungen zu erweitern, insbesondere bei Analyse der Paarverteilungsfunktion (PDF).
Die Effizienz der SDPD konnte anhand der erfolgreich gelösten Kristallstruktur von Carmustin (1,3 Bis-2-chlorethyl-1-nitrosoharnstoff, C5H9Cl2N3O2) aufgezeigt werden. [CS01]
Die Grenzen der SDPD wurden ausgelotet und erfolgreich erweitert. Nach weit verbreiteter kristallographischer Meinung ist die Strukturlösung mittels des simulierten Temperns (simulated annealing, SA) bei mehr als 25 zu bestimmenden Parametern problematisch oder unmöglich. Die pharmazeutischen Salze Lamivudin-Camphersulfonat (LC) und Aminogluthethimid-Camphersulfonat (AC) konnten, trotz ihrer hohen Anzahl an Freiheitsgraden von 31 für LC bzw. 37 für AC erfolgreich bestimmt werden. Die Strukturlösung von AC war herausfordernd und nicht direkt bei Anwendung der SA-Methode möglich. Nach einer intensiven Fehleranalyse stellte sich heraus, dass nicht die Grenzen der SA-Methode ausschlaggebend für das anfängliche Scheitern der Strukturlösung waren, sondern falsch extrahierte Intensitäten des vorangegangenen Pawley-Fits. Nach Behebung dieser Fehlerquelle war die Strukturlösung von AC problemlos. [CS02]
Mittels SDPD kann die absolute Konfiguration chiraler Verbindungen nicht direkt bestimmt werden. Durch Kristallisation der zu bestimmenden chiralen Verbindung mit einem chiralen Gegenion bekannter Konformation in einer simplen Säure-Base-Reaktion zu einem diastereomeren Salz und nachfolgender SDPD konnte eine neue Methode entwickelt werden, um die Konfigurationsbestimmung aus Pulverdaten zu ermöglichen. Diese Methode wurde anhand der drei pharmazeutischen Salze (R)-Flurbiprofen-(R)-Chinin (FQ), (2R5S)-Lamivudin-(R)-Camphersulfonat (LC) und (R)-Aminogluthethimid-(R)-Camphersulfonat (AC) aufgezeigt: In allen drei Fällen konnte die korrekte Konfiguration des pharmazeutischen Wirkstoffes mit den hierfür entwickelten Kriterien erfolgreich bestimmt werden. [CS03, CS04]
Durch Kombination der klassischen SDPD mit neuen methodischen Ansätzen konnten die Kristallstrukturen der schlecht kristallinen organischen Pigmente 2-Monomethylchinacridon (MMC, C21H14N2O2) und 4,11-Difluorchinacridon (DFC, C20H10N2O2F2) bestimmt werden, obwohl aufgrund ihrer geringen Kristallqualität keine sinnvolle Indizierung möglich war.
Für die Kristallstrukturbestimmung von DFC lieferte der neu entwickelte Global-Fit des Programms FIDEL mögliche Strukturmodelle mit ähnlich guter Übereinstimmung an das experimentelle Pulverdiagramm. Die Rietveld-Verfeinerung der Strukturmodelle in Kombination mit der Anpassung der Kristallstruktur an die PDF-Daten und kraftfeldbasierter Gitterenergieminimierung konnte einen geeigneten Strukturrepräsentanten von DFC liefern. [CS05, CS06]
Im Fall von MMC war eine Kombination der Methoden von Rietveld-Verfeinerung, Verfeinerung an die PDF-Daten und Gitterenergieminimierung zielführend zur Bestimmung der Orientierungs-Fehlordnung von MMC im Kristall. MMC ist hierbei die erste organische Verbindung, deren Fehlordnung durch Anpassung an die PDF bestimmt werden konnte. [CS07]
Große Erfolge konnten bei der Methodenentwicklung der PDF-Analyse erzielt werden. Die Bestimmung von Kristallstruktur organischer Verbindungen durch Anpassung an die PDF ohne vorherige Kenntnis der Gitterparameter oder Raumgruppe wurde durch die Entwicklung des PDF-Global-Fits erreicht. Lediglich die PDF-Kurve und eine Molekülstruktur werden als Input benötigt. Die Strukturlösung beruht auf einem globalen Optimierungs-Ansatz, bei welchem in ausgewählten Raumgruppen Zufallsstrukturen erzeugt werden. Die Zufallsstrukturen werden mit den experi¬mentellen Daten verglichen und entsprechend ihres Ähnlichkeitsindexes, basierend auf der Kreuz-Korrelation, sortiert. [CS08, CS09] Die vielversprechendsten Kandidaten werden in einem einge¬schränkten simulierten annealing-Ansatz an die experimentelle PDF angepasst. Eine nachfolgende Strukturverfeinerung der besten Strukturmodelle liefert die korrekte Kristallstruktur. Der Erfolg des PDF-Global-Fits wurde am Beispiel der Barbitursäure aufgezeigt: Ausgehend von 300 000 Zufallsstrukturen konnte die korrekte Kristallstruktur von Barbitursäure bestimmt werden. Barbitursäure ist hierdurch die erste organische Verbindung, deren Lokalstruktur durch Anpassung an die PDF bestimmt wurde, ohne Input oder Vorgabe von Gitterparametern oder Raumgruppe.[CS10]
SixGey alloys are emerging materials for modern semiconductor technology. Well-defined model systems of the bulk structures aid in understanding their intrinsic characteristics. Three such model clusters have now been realized in the form of the SixGey heteroadamantanes [0], [1], and [2] through selective one-pot syntheses starting from Me2GeCl2, Si2Cl6, and [nBu4N]Cl. Compound [0] contains six GeMe2 and four SiSiCl3 vertices, whereas one and two of the GeMe2 groups are replaced by SiCl2 moieties in compounds [1] and [2], respectively. Chloride-ion-mediated rearrangement quantitatively converts [2] into [1] at room temperature and finally into [0] at 60 °C, which is not only remarkable in view of the rigidity of these cage structures but also sheds light on the assembly mechanism.
SixGey alloys are emerging materials for modern semiconductor technology. Well-defined model systems of the bulk structures aid in understanding their intrinsic characteristics. Three such model clusters have now been realized in the form of the SixGey heteroadamantanes [0], [1], and [2] through selective one-pot syntheses starting from Me2GeCl2, Si2Cl6, and [nBu4N]Cl. Compound [0] contains six GeMe2 and four SiSiCl3 vertices, whereas one and two of the GeMe2 groups are replaced by SiCl2 moieties in compounds [1] and [2], respectively. Chloride-ion-mediated rearrangement quantitatively converts [2] into [1] at room temperature and finally into [0] at 60 °C, which is not only remarkable in view of the rigidity of these cage structures but also sheds light on the assembly mechanism.
We performed an X-ray crystallographic study of complexes of protein kinase PIM-1 with three inhibitors comprising an adenosine mimetic moiety, a linker, and a peptide-mimetic (d-Arg)6 fragment. Guided by the structural models, simplified chemical structures with a reduced number of polar groups and chiral centers were designed. The developed inhibitors retained low-nanomolar potency and possessed remarkable selectivity toward the PIM kinases. The new inhibitors were derivatized with biotin or fluorescent dye Cy5 and then applied for the detection of PIM kinases in biochemical solutions and in complex biological samples. The sandwich assay utilizing a PIM-2-selective detection antibody featured a low limit of quantification (44 pg of active recombinant PIM-2). Fluorescent probes were efficiently taken up by U2OS cells and showed a high extent of co-localization with PIM-1 fused with a fluorescent protein. Overall, the developed inhibitors and derivatives represent versatile chemical tools for studying PIM function in cellular systems in normal and disease physiology.
Herpes simplex virus type 1 (HSV-1) is a widespread neurotropic virus. Primary infection of HSV-1 in facial epithelium leads to retrograde axonal transport to the central nervous system (CNS) where it establishes latency. Under stressful conditions, the virus reactivates, and new progeny are transported anterogradely to the primary site of infection. During the late stages of neuronal infection, axonal damage can occur, however, the impact of HSV-1 infection on the morphology and functional integrity of neuronal dendrites during the early stages of infection is unknown. We previously demonstrated that acute HSV-1 infection in neuronal cell lines selectively enhances Arc protein expression - a major regulator of long-term synaptic plasticity and memory consolidation, known for being a protein-interaction hub in the postsynaptic dendritic compartment. Thus, HSV-1 induced Arc expression may alter the functionality of infected neurons and negatively impact dendritic spine dynamics. In this study we demonstrated that HSV-1 infection induces structural disassembly and functional deregulation in cultured cortical neurons, an altered glutamate response, Arc accumulation within the somata, and decreased expression of spine scaffolding-like proteins such as PSD-95, Drebrin and CaMKIIβ. However, whether these alterations are specific to the HSV-1 infection mechanism or reflect a secondary neurodegenerative process remains to be determined.
KdpFABC, a high-affinity K+ pump, combines the ion channel KdpA and the P-type ATPase KdpB to secure survival at K+ limitation. Here, we apply a combination of cryo-EM, biochemical assays, and MD simulations to illuminate the mechanisms underlying transport and the coupling to ATP hydrolysis. We show that ions are transported via an intersubunit tunnel through KdpA and KdpB. At the subunit interface, the tunnel is constricted by a phenylalanine, which, by polarized cation-π stacking, controls K+ entry into the canonical substrate binding site (CBS) of KdpB. Within the CBS, ATPase coupling is mediated by the charge distribution between an aspartate and a lysine. Interestingly, individual elements of the ion translocation mechanism of KdpFABC identified here are conserved among a wide variety of P-type ATPases from different families. This leads us to the hypothesis that KdpB might represent an early descendant of a common ancestor of cation pumps.
Im Rahmen dieser kumulativen Dissertation konnte eine Methode mitentwickelt werden, die die Bestimmung der absoluten Konfiguration pharmazeutischer Verbindungen aus Röntgenpulverbeugungsdaten ermöglicht. Die Methode basiert auf der Bildung von Salzen. Die notwendige Herstellung dieser Salze mit Salzbildnern bekannter Konfiguration wurde hinsichtlich einer minimalen Ansatzgröße optimiert und erlaubt ein Arbeiten mit Mengen von unter zehn Mikrogramm. Die Kristallisation konnte sogar direkt in den Kapillaren für die Aufnahme der Pulverdiagramme durchgeführt werden. Die absolute Konfiguration einiger als Testfälle gewählter pharmazeutischer Wirkstoffe konnte auf diese Art erfolgreich bestimmt werden. Dies stellt eine erfolgreiche Erweiterung bisher verfügbarer Methoden dar.
1,1,3,3-Tetraethyl-5-nitroisoindolin (TENI) und 1,1,3,3-Tetraethyl-5-nitroisoindolin-2-oxyl (TENO) sind Zwischenstufen in der Synthese von RNS-Spinlabeln für die EPR-Spektroskopie. Die Kristallstrukturen beider Verbindungen konnten aus Einkristallbeugungsdaten bestimmt werden. TENI hat einen Schmelzpunkt nahe der Raumtemperatur. TENO hat dagegen einen wesentlich höheren Schmelzpunkt, obwohl das Molekül nur ein Sauerstoffatom zusätzlich hat. Die Kristallstruktur liefert die Erklärung für dieses Phänomen: In der Kristallstruktur von TENI findet sich als stärkste intermolekulare Wechselwirkung eine einzelne schwache, sehr lange Wasserstoffbrückenbindung.
6-Amino-2-iminiumyl-4-oxo-1,2,3,4-tetrahydropyrimidin-5-aminiumsulfat, ein Edukt der Synthese von Leukopterin konnte als Hydrat erhalten werden. Die Kristallstruktur dieses Monohydrats konnte problemlos bestimmt werden, ebenso wie die von synthetisiertem 4-Amino-2,6-dimethylpyrimidin.
Natriumethanolat wurde nach einer 180 Jahre alten Vorschrift von Liebig synthetisiert. Wie die Röntgenpulverdiagramme zeigen, bilden sich dabei jedoch Gemische von verschiedenen Phasen. Die Kristallstruktur von reinem NaOEt konnte aus Pulverdaten bestimmt werden. Ebenfalls wurden ein Diethanolsolvat sowie zwei weitere Phasen identifiziert. Vom Diethanolsolvat NaOEt · 2 HOEt konnten Einkristalle hergestellt und die Kristallstruktur aus diesen bestimmt werden. Die Kristallstrukturen von Natrium-n-propanolat (NaOnPr), Natrium-n-butanolat (NaOnBu) und Natrium-n-amylat (NaOnAm) konnten ebenfalls aus Pulverdaten aufgeklärt werden. Sie weisen ein ähnliches Na-O-Gitter wie Natriumethanolat auf, allerdings kristallisieren sie in der Raumgruppe P 4/n m m. Die abweichende Raumgruppe des NaOEt (P -4 21 m) liegt am sterischen Anspruch der Ethylgruppe. Die längeren Alkylgruppen sind hochgradig fehlgeordnet und somit im Mittel zylinderförmig. Die Ethylgruppe dagegen hat einen weniger symmetrischen Raumbedarf. Die Solvate der Alkalialkoholate wurden mit zunehmender Länge der Alkylketten instabiler. Nichtsdestotrotz konnten drei verschiedene Solvate hergestellt werden: NaOnPr · 2 HOnPr, NaOiPr · 5 HOiPr und NaOtAm · HOtAm. Ihre Kristallstrukturen konnten aus Einkristallbeugungsdaten bestimmt werden. In diesen Strukturen zeigen sich sehr unterschiedliche Strukturmotive, die teilweise die mögliche Existenz weiterer Solvatstufen andeuten.
Die industriellen Rotpigmente Pigment Red 52 und Pigment Red 48 wurden im Labor unter verschiedenen Bedingungen synthetisiert. Dabei wurden neben den kommerziell verfügbaren Phasen einige neue Phasen identifiziert. Erstmals konnten Kristallstrukturen von P.R.52 und P.R.48 bestimmt werden. Von Pigment Red 52 konnte ein bisher unbekanntes Mononatriumsalz hergestellt werden. Von diesem Salz konnte ein DMSO-Solvat-Monohydrat kristallisiert werden. Aus erhaltenen Einkristallen konnte die Struktur bestimmt werden. Von Pigment Red 48 konnte ebenfalls ein bisher nicht literaturbekanntes Mononatriumsalz isoliert werden. Von zwei Hydratstufen dieser Verbindung konnten Einkristalle hergestellt und ihre Kristallstrukturen bestimmt werden. Eine weitere Phase wurde als Anhydrat identifiziert. Vom Di-Natriumsalz des P.R.52 sowie von seinem Calciumsalz wurden insgesamt fünf verschiedene Hydratstufen gefunden. Die Kristallstrukturen dieser Hydrate konnten aus Röntgenpulverbeugungsdaten bestimmt werden. Von einer Hydratstufe konnte ebenfalls ein Einkristall erhalten und die Struktur bestätigt werden. Eine Veröffentlichung ist in Vorbereitung.
Die Isomere des Orangepigments Perinon werden nach gemeinsamer Synthese industriell durch Überführung in „Trennsalze“ getrennt. Weder die Molekülkonstitution der Trennsalz-Ionen, noch die chemische Zusammensetzung der Feststoffe, noch deren Kristallstrukturen waren bisher bekannt. Die industrielle Form des „trans-Trennsalzes“ konnte im Labor hergestellt werden. Eine weitere Phase des trans-Perinontrennsalzes konnte hergestellt und identifiziert werden. Durch die nachfolgende Einkristallstrukturanalyse zeigte sich, dass die Trennsalze eine völlig andere Molekülkonstitution haben, als in der Literatur beschrieben war: Statt eines planaren Perinongerüsts enthält das Trennsalz ein verdrehtes Bis(benzimidazolat)naphthalindicarboxylat-tetraanion, dessen Ladung durch Kalium-Kationen kompensiert wird. Das bisher nie als Feststoff beschriebene cis-Perinontrennsalz wurde hergestellt und kristallisiert. Es konnten Einkristalle hergestellt und die Kristallstruktur aus diesen bestimmt werden. Alle Perinontrennsalze enthalten im Kristallgitter eine beträchtliche Anzahl Wasser- und Ethanolmoleküle. Durch Festkörper-NMR-Spektroskopie konnte gezeigt werden, dass das Wasser-Ethanol-Netzwerk stark dynamisch ist. Bei der Hydrolyse der Trennsalze entstehen wieder die ursprünglichen, wasser- und lösungsmittelfreien Perinonpigmente.
Viele Studien konnten nachweisen, dass die Produktion von cGMP eine entscheidende Funktion im nozizeptiven System einnimmt. Hierbei wurde vor allem die cGMP-Produktion über lösliche Guanylatzyklasen untersucht. Welche Rolle die partikulären Guanlyatzyklasen bei der Entstehung von Schmerzen haben ist weitgehend ungeklärt. Die vorliegende Arbeit zeigte, dass die partikuläre Guanylatzyklase NPR2 stark in DRG-Neuronen exprimiert wird und dort mit cGKI-alpha sowie CRP4 colokalisiert ist. Aktiviert wird NPR2 über den Peptidliganden CNP. Hervorzuheben ist, dass CNP nicht in primär afferenten Neuronen, dafür jedoch vermehrt im Dorsalhorn des Rückenmarks gebildet wird. Tierexperimentelle Untersuchungen zeigten, dass SNS-Npr2-/--Mäuse ein verringertes Schmerzverhalten bei thermischer Stimulation aufwiesen. Während sie im Capsaicin-Test keinen Phänotyp zeigten, wiesen sie in Phase II des Formalin-Modells ein signifikant reduziertes Leckverhalten auf. Diese Ergebnisse liefern Hinweise für eine Beteiligung des CNP/NPR2/cGKI Signalwegs an der Detektion von Hitzeschmerz und an der TRPA1-vermittelten Schmerzantwort. Dabei scheint NPR2 eine pronozizeptive Funktion zu besitzen. CRP4 als Zielprotein scheint hingegen eine antinozizeptive Wirkung zu haben. Zudem kann die Hypothese aufgestellt werden, dass CNP über einen retrograden Transport aus dem Rückenmark die Aktivierung von NPR2 auslösen könnte. Zusammengefasst zeigen die Daten dieser Arbeit, dass eine cGMP-abhängige Aktivierung durch NPR2 primär für die Detektion thermischer Reize zuständig ist, während die Literatur Hinweise darauf gibt, dass lösliche Guanylatzyklasen vor allem an inflammatorischen und neuropathischen Prozessen beteiligt sind. Daher scheinen partikuläre und lösliche Guanylatzyklasen unterschiedliche Eigenschaften im nozizeptiven System zu besitzen.
Die Synthese und Charakterisierung von neuartigen metallorganischen Koordinationsverbindungen hat in den vergangenen Jahrzehnten einen wahren Aufschwung erlebt. Aufgrund ihrer außerordentlichen strukturellen Vielfalt eröffnen sich zahlreiche Anwendungsmöglichkeiten über alle naturwissenschaftlich-technischen Domänen hinweg. Daher besteht ein allgemeines Interesse nicht nur in der Entwicklung neuer Verbindungen und Untersuchungen von Struktur-Eigenschafts-Beziehungen, sondern auch in einer Verbesserung ihrer Darstellungsmethoden.
Diese Dissertation beschäftigt sich mit Koordinationspolymeren und -netzwerken, die aus zweiwertigen 3d-Übergangsmetallhalogeniden (MX2, wie bspw. MnCl2 oder FeBr2) und Pyridin (py) bzw. Pyridinderivaten (CNpy, wie bspw. 3-Cyanopyridin) aufgebaut sind. Die Darstellung der Koordinationsverbindungen erfolgte in erster Linie über gewöhnliche Kristallisationsexperimente in alkoholischer Lösung, bei denen Phasen der Stöchiometrie [MX2(CNpy)4] oder [MX2(CNpy)2]n anfielen. Diese wurden anschließend systematisch erhitzt (“getempert“), was in der Regel zu einer stufenweisen und irreversiblen Abgabe eines Teils der Liganden führte, also bspw. von [MX2(CNpy)2]n zu [MX2(CNpy)1]n. Für diesen sog. „thermischen Abbau“ hat sich die Verwendung eines DTA-TG-Gerätes bewährt. Da die Zielverbindungen als mikrokristalline Pulver anfielen, erfolgte die Bestimmung ihrer Kristallstrukturen auf Basis von Röntgenpulverdaten.
Insgesamt wurden im Rahmen dieser Arbeit 41 neue Phasen synthetisiert und deren Kristallstrukturen aus Röntgenpulverdaten bestimmt. Zusammenfassend ist für die verschiedenen Pyridinderivate folgendes zu konstatieren:
3-Cyanopyridin
Im Falle der MBr2-Serie wurden für M = Mn, Fe, Co und Ni Koordinationsverbindungen der Stöchiometrie [MBr2(3-CNpy)4] erhalten, deren Kristallstrukturen aus diskreten Komplexmolekülen bestehen. Derart ligandenreiche Verbindungen konnten bei keiner der übrigen Serien erhalten werden. Alle Kristallstrukturen der Zusammensetzung [MX2(3-CNpy)2]n zeigen bei M = Mn, Fe, Co, Ni und Cu eine Kettenstruktur, in der die Halogenatome als µ2-Brückenliganden fungieren. Die Ketten weisen eine Fischgrät-Anordnung auf. Im Falle von [ZnX2(3-CNpy)2] werden ausschließlich diskrete Komplexmoleküle beobachtet. In allen Kristallstrukturen der [MCl2(3-CNpy)1]n-Serie liegen Doppelketten mit µ2- und µ3-verbrückenden Cl-Atomen vor. Hingegen weisen die Verbindungen der [MBr2(3-CNpy)1]n-Serie Netzwerkstrukturen auf, in denen, zusätzlich zu µ2-Cl-Atomen, über NCN-Atome gebrückt wird.
3,5-Dicyanopyridin
Aufgrund der umfassenden Erkenntnislage bei [NiCl2(CNpy)x]n und [NiCl(py)x]n- Verbindungen wurde NiCl2 für erste Experimente mit 3,5-Dicyanopyridin als neuem, bifunktionalem Liganden ausgewählt. Erwartungsgemäß führte deren Umsetzung zur Bildung von [NiCl2(3,5-CNpy)2]n, dessen Kristallstruktur das hinlänglich bekannte charakteristische Kettenmotiv aufweist. Thermischer Abbau von [NiCl2(3,5-CNpy)2]n führt indes nicht zur Bildung von [NiCl2(3,5-CNpy)1]n (bzw. grundsätzlich zu [NiCl2(3,5-CNpy)x<2]n (mit bi- oder gar tridentatem Liganden), sondern unmittelbar zur vollständigen Zersetzung in NiCl2 und 3,5-CNpy. Daher sollten weitere Experimente mit NiBr2 als Edukt durchgeführt werden, da in [NiBr2(CNpy)1]n neben Npy auch NCN an Ni-Atome zu koordinieren vermag, wodurch ja deren Netzwerkstrukturen resultieren.
4-Cyanopyridin
Alle Kristallstrukturen der Zusammensetzung [MX2(4-CNpy)2]n zeigen bei M = Mn, Fe, Co, Ni und Cu ebenfalls eine Kettenstruktur, in der die Halogenatome als µ2-Brückenliganden fungieren. Auch in diesen Kristallstrukturen liegt eine Fischgrät-Anordnung der Ketten vor. Im Falle von [ZnX2(4-CNpy)2] werden ausschließlich diskrete Komplexmoleküle beobachtet. In allen Kristallstrukturen der [MX2(4-CNpy)1]n-Serie liegen Netzwerkstrukturen vor, in denen die Metallatome über µ2-Halogenatome und NCN-Atome verbrückt werden. Alle Kristallstrukturen der [MBr2(4-CNpy)1]n-Serie sind charakteristisch fehlgeordnet, da die Orientierung der 4-CNpy-Liganden invertiert wird („Kopf-Schwanz“-Fehlordnung).
Extracts of frankincense, the gum resin of Boswellia species, have been extensively used in traditional folk medicine since ancient times and are still of great interest as promising anti-inflammatory remedies in Western countries. Despite their common therapeutic use and the intensive pharmacological research including studies on active ingredients, modes of action, bioavailability, pharmacokinetics, and clinical efficacy, frankincense preparations are available as nutraceuticals but have not yet approved as a drug on the market. A major issue of commercially available frankincense nutraceuticals is the striking differences in their composition and quality, especially related to the content of boswellic acids (BAs) as active ingredients, mainly due to the use of material from divergent Boswellia species but also because of different work-up and extraction procedures. Here, we assessed three frequently used frankincense-based preparations for their BA content and the interference with prominent pro-inflammatory actions and targets that have been proposed, that is, 5-lipoxygenase and leukotriene formation in human neutrophils, microsomal prostaglandin E2 synthase-1, and inflammatory cytokine secretion in human blood monocytes. Our data reveal striking differences in the pharmacological efficiencies of these preparations in inflammation-related bioassays which obviously correlate with the amounts of BAs they contain. In summary, high-quality frankincense extracts display powerful anti-inflammatory effectiveness against multiple targets which can be traced back to BAs as bioactive ingredients.
Although overexpression and hyperactivity of protein kinases are causative for a wide range of human cancers, protein kinase inhibitors currently approved as cancer drugs address only a limited number of these enzymes. To identify new chemotypes addressing alternative protein kinases, the basic structure of a known PLK1/VEGF-R2 inhibitor class was formally dissected and reassembled. The resulting 7-(2-anilinopyrimidin-4-yl)-1-benzazepin-2-ones were synthesized and proved to be dual inhibitors of Aurora A kinase and VEGF receptor kinases. Crystal structures of two representatives of the new chemotype in complex with Aurora A showed the ligand orientation in the ATP binding pocket and provided the basis for rational structural modifications. Congeners with attached sulfamide substituents retained Aurora A inhibitory activity. In vitro screening of two members of the new kinase inhibitor family against the cancer cell line panel of the National Cancer Institute (NCI) showed antiproliferative activity in the single-digit micromolar concentration range in the majority of the cell lines.
Leukemia patients bearing t(6;11)(q27;q23) translocations can be divided in two subgroups: those with breakpoints in the major breakpoint cluster region of MLL (introns 9–10; associated mainly with AML M1/4/5), and others with breakpoints in the minor breakpoint cluster region (introns 21–23), associated with T-ALL. We cloned all four of the resulting fusion genes (MLL-AF6, AF6-MLL, exMLL-AF6, AF6-shMLL) and subsequently transfected them to generate stable cell culture models. Their molecular function was tested by inducing gene expression for 48 h in a Doxycycline-dependent fashion. Here, we present our results upon differential gene expression (DGE) that were obtained by the “Massive Analyses of cDNA Ends” (MACE-Seq) technology, an established 3′-end based RNA-Seq method. Our results indicate that the PHD/BD domain, present in the AF6-MLL and the exMLL-AF6 fusion protein, is responsible for chromatin activation in a genome-wide fashion. This led to strong deregulation of transcriptional processes involving protein-coding genes, pseudogenes, non-annotated genes, and RNA genes, e.g., LincRNAs and microRNAs, respectively. While cooperation between the MLL-AF6 and AF6-MLL fusion proteins appears to be required for the above-mentioned effects, exMLL-AF6 is able to cause similar effects on its own. The exMLL-AF6/AF6-shMLL co-expressing cell line displayed the induction of a myeloid-specific and a T-cell specific gene signature, which may explain the T-ALL disease phenotype observed in patients with such breakpoints. This again demonstrated that MLL fusion proteins are instructive and allow to study their pathomolecular mechanisms.
Acinetobacter baumannii is a worldwide opportunistic pathogen responsible for nosocomial infections. One of the main factors contributing to multidrug resistance in A. baumannii is the upregulation of various chromosomally encoded or acquired efflux pumps, which expel toxic compounds out of the cells with high efficiency.
The resistance-nodulation-cell division (RND)-type efflux pump gene deletion strains ∆adeAB, ∆adeFG or ∆adeIJ and the major facilitator superfamily (MFS) chloramphenicol efflux pump gene deletion strain ∆craA of A. baumannii ATCC 19606 were created and a differential gene expression study was conducted via RT-qPCR. The expression of efflux pump genes adeB, adeG, adeJ, craA, and the outer membrane protein ompA were examined in the absence and presence of chloramphenicol. No significant up- or downregulation of these genes for any of these deletion strains in comparision to the wild-type strain in absence of the drug chloramphenicol.
In contrast, craA was significantly up-regulated in A. baumannii exposed to chloramphenicol, emphasizing the importance of CraA in chloramphenicol resistance. CraA is widely present in clinical isolates of A. baumannii. It is homologous to the well-studied multiple-drug efflux transporter MdfA from Escherichia coli (61% similarity), but surprisingly reported to be acting as a specific chloramphenicol transporter of A. baumannii (Roca et al., 2009).
The drug susceptibility assay done with A. baumannii ATCC 19606 ΔcraA showed that CraA could confer resistance towards phenicols (chloramphenicol, thiamphenicol, and florfenicol), which was in line with the previous report. CraA was heterologously overproduced in E. coli BW25113 ∆emrE∆mdfA and its substrate specificity was determined by drug susceptibility assays and whole cell fluorescent dye uptake experiments. We observed that the substrate specificity of craA overexpressed in E. coli was more diverse and resembling that of the E. coli MdfA homolog. Apart from resistance towards phenicols (chloramphenicol, thiamphenicol, and florfenicol), CraA also confer resistance towards monovalent cationic drugs (benzalkonium, TPP+, and ethidium), long dicationic drugs (dequalinium and chlorhexidine), fluoroquinolones (norfloxacin and ciprofoxacin) and anticancer drugs (mitomycin C). We showed that CraA is a drug/H+ antiporter by ACMA quenching in inverted CraA or CraA variant containing membrane vesicles.
To address the molecular determinants for multidrug binding and transport, 45 mostly single Ala-substitution variants of CraA were created. These include substitution variants for membrane-embedded proton-titratable residues (E38, D46, and E338) and residues predicted to be important for binding and transport of drug, as inferred from docking experiments on basis of a MdfA-derived CraA model. The combined results indicated a high degree of functional similarities between MdfA and CraA. The conserved titratable residues E26 and D34 (E38 and D46 in CraA) are important for transport in both these homologs. The CraA variant E38A is inactive against all tested drugs, but D46A is only inactive for some drugs, suggesting that only E38 is involved in H+-transport.
Another focus of this thesis is the three tetracycline transporters of A. baumannii strain AYE, TetA, TetG and TetA(A). Susceptibility assays involving tetracycline, minocycline, doxycycline and the last-resort antibiotic tigecycline were conducted on E. coli BW25113 ∆emrE∆mdfA overexpressing these transporters. TetA(A) was excluded from further study due to toxicity of the cells caused by protein overexpression. Both TetA and TetG confer resistance against tetracycline, minocycline and doxycycline. Although tigecycline was reported not to be recognized by tetracycline efflux pumps, we surprisingly found that TetA is able to transport tigecycline. The role of TetA in tigecycline efflux in A. baumannii was confirmed by conducting tigecycline susceptibility assays on A. baumannii.
We speculate that TetA embedded in the inner membrane acts in cooperation with RND-type tripartite systems that span the inner and outer membrane to extrude tigecycline from the periplasm across the outer membrane. A. baumannii ATCC 19606 ∆adeAB were indeed sensitive to tigecycline in comparison to wild-type strain. Deletion of adeIJ also leads to sensitivity to tigecycline, but less so compared to the DadeAB phenotype, while A. baumannii ATCC 19606 ∆adeFG did not show any difference compared to wild-type strain in tigecycline susceptibility. Differential gene expression analysis of the RND efflux pumps (adeB, adeG and adeJ) and tetA of A. baumannii strain AYE showed that the expression of tetA expression is significantly upregulated when tigecycline is present in the growth medium.
We conclude that craA encodes a broad-spectrum efflux pump rather than a specific chloramphenicol transporter. In A. baumannii, the synergistic effects with the outer membrane and/or the presence of other transporters could result in the discrepancy observed. Thus, the possibility of CraA in conferring multidrug resistance should not be overlooked, especially when it is up-regulated under antibiotic stress conditions.
Leukemia patients bearing t(6;11)(q27;q23) translocations can be divided in two subgroups: those with breakpoints in the major breakpoint cluster region of MLL (introns 9–10; associated mainly with AML M1/4/5), and others with breakpoints in the minor breakpoint cluster region (introns 21–23), associated with T-ALL. We cloned all four of the resulting fusion genes (MLL-AF6, AF6-MLL, exMLL-AF6, AF6-shMLL) and subsequently transfected them to generate stable cell culture models. Their molecular function was tested by inducing gene expression for 48 h in a Doxycycline-dependent fashion. Here, we present our results upon differential gene expression (DGE) that were obtained by the “Massive Analyses of cDNA Ends” (MACE-Seq) technology, an established 3′-end based RNA-Seq method. Our results indicate that the PHD/BD domain, present in the AF6-MLL and the exMLL-AF6 fusion protein, is responsible for chromatin activation in a genome-wide fashion. This led to strong deregulation of transcriptional processes involving protein-coding genes, pseudogenes, non-annotated genes, and RNA genes, e.g., LincRNAs and microRNAs, respectively. While cooperation between the MLL-AF6 and AF6-MLL fusion proteins appears to be required for the above-mentioned effects, exMLL-AF6 is able to cause similar effects on its own. The exMLL-AF6/AF6-shMLL co-expressing cell line displayed the induction of a myeloid-specific and a T-cell specific gene signature, which may explain the T-ALL disease phenotype observed in patients with such breakpoints. This again demonstrated that MLL fusion proteins are instructive and allow to study their pathomolecular mechanisms.
Resistant microbes are a growing concern. It was estimated that about 33,000 of people die because of the infections caused by multidrug resistant bacteria each year in Europe (ECDC, 2018, https://www.ecdc.europa.eu/). Bacteria can acquire resistance against toxic compounds via different mechanisms and intrinsic active efflux is one of the first mechanisms deployed by bacterial cells. The membrane-localized efflux pumps catalysing this reaction, extract toxic compounds from the interior of the cell and transport these to the outside, thereby maintaining sub-lethal toxin levels in the cytoplasm, periplasm and membranes. Gram-negative three-component efflux pumps, analysed in this study, are composed of an inner membrane protein, a member of the Resistance-Nodulation cell Division (RND) superfamily, an Outer Membrane Factor (OMF) protein and a Membrane Fusion Protein (MFP) that connects the two afore mentioned components into an active efflux pump. The pumps described in this work, AcrAB-TolC and EmrAB-TolC, are drug efflux pumps belonging to the RND and MFS superfamilies, respectively, while CusCBA is an efflux pump that belongs to the RND heavy metal efflux family. Another efflux pump that was used as a model for the design of an in vitro assay for the silver ion transport studies, CopA, belongs to the P-type ATPase superfamily. All pumps analysed in this study are part of the resistance system of Escherichia coli, which is a highly clinically relevant pathogen.
In order to examine the AcrAB-TolC, CopA and CusA efflux pumps, the individual components were separately produced in E. coli, purified to monodispersity and reconstituted in large unilamellar vesicles, LUVs. Means for the optimized production and adequate conditions for efficient reconstitution were presented in this study. The activity of AcrB in LUVs was detected using fluorescence quenching of the dye 8-hydroxy-1,3,6 pyrenetrisulfonate (pyranine), which is incorporated inside the proteoliposomes and is sensitive to the pH changes in its surrounding. The inactive AcrB variant with a substitution in the proton relay network, D407N, showed no activity in proteoliposomes, which correlates with the measurements done in empty liposomes. When AcrA was co-reconstituted with AcrB D407N proteoliposomes it did not restore protein activity. To test the assembly of the AcrAB-TolC pump out of its single components, an in vitro assay was established where the complex assembly was tested with AcrAB- and TolC-containing liposomes. These experiments showed putative AcrAB-TolC formation in the presence or absence of a pump substrate, taurocholate, as well as in the presence of the pump inhibitor, MBX3132. The assembly appeared stable over time and results were invariant in the presence or absence of a pH gradient across the AcrAB-containing membrane.
After determination of the ATPase activity of the P-type ATPase, CopA, in detergent micelles, the protein was reconstituted in LUVs. Quenching of the Ag+-sensitive dye Phen Green SK (PGSK), present on the inside of the CopA-containing proteoliposomes, was observed in presence of ATP and Ag+. Under the same conditions, but in absence of Ag+-ions, quenching was reduced by 80 % after 300 seconds. No PGSK-quenching was observed in control liposomes in the presence of ATP and Ag+. The additional presence of sodium azide led to minimal reduction of the PGSK-quenching as expected since sodium azide is not an inhibitor of P-type ATPases, but the quenching rate was similar to that of the same experimental condition with control liposomes.
The RND superfamily member CusA, as part of the tripartite CusCBA efflux pump, has been proposed to sequester Ag+ or Cu+ from either the cytoplasmic or periplasmic side of the inner membrane. The periplasmic transport of silver ions was implied from an in vitro assay where the quenching of a pH sensitive dye, 9-amino-6-chloro-2-methoxyacridine (ACMA), indicates acidification of the lumen of the proteoliposomes containing CusA when an inwardly directed pH was imposed. The same experiment with the CusA D405N variant, which was previously reported to be an inactive variant, also led to ACMA quenching, although at a slightly lower rate. Under application of an inwardly directed pH and a (negative inside), CusA-containing proteoliposomes showed a strong quenching of the incorporated PGSK dye, suggesting strong Ag+ influx.
The Major Facilitator Superfamily-(MFS-) type EmrAB-TolC pump has an analogous structural setup as the RND-type AcrAB-TolC pump. To examine the efflux of one of its substrates, carbonyl - cyanide m-chlorophenylhydrazone (CCCP), a plate-based susceptibility assay was used. The presence of the EmrAB-TolC pump confers lower susceptibility levels towards CCCP in E. coli, compared to cells not expressing the pump or cells expressing only the MFS component, indicating that EmrAB-TolC extrudes CCCP.
The work done in this study opens up a path towards investigation of drug and metal resistance in vitro. The methodologies to obtain proteoliposomal samples of multicomponent efflux pumps and subsequent measurements of drug/metal ion and H+ fluxes, as well as the determination of pump assembly are crucial for the future research on pump catalysis and transport kinetics. The in vivo drug-plate assays done in this work provide initial insights for future investigations of the drug susceptibility of E. coli expressing the MFS-type tripartite efflux pumps.
Die Funktion nukleärer Rezeptoren (NR) beruht auf einem empfindlichen Zusammenspiel zwischen ihren Domänen, Coregulatoren und Liganden. Die meisten Rezeptoren binden die DNA als Homo- oder Heterodimere und transregulieren die Gentranskription in Folge von Ligandenbindung. Klassische Assay-Systeme, die sich auf die Untersuchung der NR-Funktion oder auf die Charakterisierung von Substanzen richten, bilden nur die Coregulator-Rekrutierung zu isolierten NR-Ligandenbindungsdomänen (LBDs) ab und vernachlässigen dabei die NR:NR-Interaktion. Damit klammern sie die NR:NR-Wechselwirkung aus, obwohl die Rekrutierung von Cofaktoren durch allosterischen Crosstalk mit der Oligomerisierung verbunden ist. Dies war die Motivation dafür, Assay-Systeme zu entwickeln, welche die Untersuchung von NR-Interaktionen,
insbesondere der NR-Dimerisierung, und deren Modulation durch verschiedene Arten von Liganden ermöglichen. Im Rahmen dieser Doktorarbeit wird ein vielfältiges modulares Set von Assays für die Untersuchung der NR-Dimerisierung und NR-Coregulator-Rekrutierung vorgestellt und deren Anwendbarkeit auf eine Vielzahl von NRs demonstriert. Die Verwendung einer
rekrutierungsunfähigen RXRα-Variante mit einer mutierten AF-2-Domäne ermöglichte den spezifischen Nachweis der Coaktivatorrekrutierung durch PPARγ im Kontext des Heterodimers mit seinem obligatorischen Dimerpartner RXRα. Außerdem konnte gezeigt werden, dass die Aktivierung der RXRα LBD mit ihrem Agonisten SR11237 zu einer Destabilisierung des RXRα-Homodimers, aber zu einer Förderung der Bildung des Heterodimers mit der PPARγ LBD führte.
Ein zentrales Ergebnis war das Phänomen, dass der Einbau von PPARγ in das Heterodimer zu einem erheblichen Anstieg an Affinität gegenüber Coaktivatoren führt, auch in Abwesenheit von Liganden. Somit fördert die RXRα-Aktivierung die Coaktivator-Rekrutierung von PPARγ indirekt durch eine Verschiebung der Oligomerisierungspräferenz von RXRα in Richtung des Heterodimers. Zusätzlich wurde die Wirkung von Tetrac, einem nicht-klassischen Schilddrüsenhormon, auf PPARγ und RXRα untersucht und dessen Aktivierungsvermögen gegenüber beiden Rezeptoren mit einer deutlich vervielfachten Wirkung auf das Heterodimer demonstriert. Mit Hilfe des neu etablierten Cofaktor-Rekrutierungsscreens konnte die Dynamik
zwischen dem Nurr1 NR und 29 kanonischen Coregulatoren, von denen einige ligandenabhängig hohe Affinitäten zum Rezeptor aufwiesen, beleuchtet werden. Diese Interaktionen wurden
bidirektional durch eine Reihe von strukturell unterschiedlichen nicht-steroidalen Antirheumatika moduliert, die auch die Affinitäten sowohl des Nurr1-Homodimers als auch des Heterodimers mit der RXRα LBD beeinflussen konnten. Die Nurr1-Dimere zeigten zudem auch eine hohe Empfindlichkeit gegenüber dem Endocannabinoid Anandamid. Zusätzlich zu PPARγ, RXRα und Nurr1 wurden erste Schritte zur Untersuchung der TLX NR-Funktion unternommen. Unter Anwendung der entwickelten Assays konnte die Heterodimerbildung der TLX und der RXRα LBD
beschrieben und die ligandenabhängige Rekrutierung des Corepressors SMRT beobachtet werden.
Zusammenfassend beschreibt diese Arbeit einen Satz von Werkzeugen für die Untersuchung von ligandenabhängiger NR-Coregulator-Interaktion und Oligomerisierung. Auf diese Weise trug sie zu einer umfassenderen Identifizierung und Charakterisierung von NR-Liganden bei und stellt eine valide Basis für die weitere Assayentwicklung und Ligandendesign dar.
The deubiquitinase USP32 regulates non-proteolytic ubiquitination in the endosomal-lysosomal system
(2021)
The regulation of essential cellular processes requires tightly controlled and directed transport of proteins and membranes. The highly dynamic endosomal and lysosomal system forms the key network for exchange and trafficking of molecules with its early endosomes, recycling endosomes, late endosomes, lysosomes, and additionally autophagosomes.
In this system, the small GTPase Rab7 has an essential role at the late endosomal stage regulating vesicle transport, tethering, and fusion, and retromer mediated receptor recycling back to the trans-Golgi network (TGN). Thus, Rab7 is also important for autophagosomes and lysosomes.
Lysosomes do not only represent the end point of the degradation pathway with several feeder pathways. But these organelles are also a dynamic signaling hub for a variety of metabolic processes. The ever-important regulator of cellular biosynthetic pathways mTORC1 dynamically associates with lysosomes where it is activated. mTORC1 activation is a complex multi-step process where a series of signaling events converge in dependence of amino acid levels thereby enabling interactions between the lysosomal v-ATPase, Ragulator complex (consisting of LAMTOR1-5), and Rag GTPases.
Ubiquitin signals are involved in almost all cellular processes. With this, their regulatory mechanism is also described for the endosomal-lysosomal system as well as mTORC1 signaling. Deubiquitinases (DUBs) release conjugated ubiquitin from proteins and thereby maintain the dynamic state of the cellular ubiquitinome.
The ubiquitin-specific protease 32 (USP32) is a poorly characterized DUB with only emerging cellular function. However, its predicted domain structure includes two unique domains within the entire DUB family. It has been linked to the development of breast cancer and small cell lung cancer. Furthermore, overexpressed GFP-USP32 was localized at the TGN, and a global mass spectrometry-based DUB interactome study suggested an interaction with the retromer complex. Based on these data, USP32 was a very interesting candidate to study its cellular function in this PhD project.
To investigate the function without disease background, a polyclonal USP32 knockout (USP32KO) RPE1 cell line was generated using the CRISPR/Cas9 technology. First experiments revealed different protein expression levels in various cell lines, and a subcellular localization of USP32 at membranes of the Golgi and lysosomal compartments. In a subsequent SILAC-based ubiquitinome analysis potential substrates of USP32 were identified. Interestingly, various proteins of the endosomal-lysosomal system were detected with enriched non-proteolytic ubiquitination upon USP32 depletion.
The further characterization of Rab7 as USP32 substrate confirmed the USP32-sensitive ubiquitination of Rab7 at lysine (K) residues 191 and 194. The ubiquitination in USP32KO cells did not change the subcellular localization of Rab7, but enhanced the interaction with the effector protein RILP. This implied that Rab7 was either more active or RILP had higher affinity to ubiquitinated Rab7. The subsequent results verified this theory. The retromer mediated recycling of CI-M6PR back to the TGN was faster or more efficient in USP32-depleted cells.
Accompanying this, levels of hydrolases were enriched in lysosomes isolated from USP32KO cells. Notably, USP32 had no direct effect on expression level or assembly of the retromer complex itself.
The observed lysosomal phenotypes connected another identified substrate to the function of USP32 in the endosomal-lysosomal system: LAMTOR1. LAMTOR1 is a component of the Ragulator complex and thus involved in the activation of mTORC1 at the lysosomal surface. Similar as for Rab7, the first experiments to characterize LAMTOR1 as USP32 substrate confirmed the USP32-sensitive ubiquitination at K20 independent of amino acid availability. However, ubiquitination of LAMTOR1 decreased its lysosomal localization in untreated and amino acid starved USP32KO cells. The following label-free interactome study detected a reduced interaction of LAMTOR1 and subunits of the lysosomal v-ATPase upon loss of USP32. This resulted in a shifted subcellular localization of mTOR (subunit of mTORC1) away from lysosomes. Furthermore, direct substrates of mTORC1 were less or slower re-phosphorylated after long amino acid starvation and re-activation of mTORC1 in USP32KO cells indicating a reduced mTORC1 activity.
Both USP32-dependent regulations of Rab7 and LAMTOR1/Ragulator converged in enhanced autophagic processes analyzed by increased LC3 levels upon amino acid starvation and USP32 depletion.
In summary, the presented thesis described the diverse role of USP32 in the endosomal and lysosomal system, and contributes to the understanding of novel ubiquitin signals in this context.
RNA ist vor allem als Vermittler von Erbinformationen bekannt. Doch neben der Translation in Proteine ist sie auch maßgeblich an regulatorischen Prozessen in der Zelle beteiligt. So kommen in vielen Organismen Argonautenproteine vor, die zusammen mit microRNA einen Komplex bilden, der in der Lage ist, mRNA zu spalten oder auf andere Weise deren Translation zu unterdrücken. Da die Deregulierung von microRNA bei verschiedenen Krankheiten wie Krebs, Parkinson oder Alzheimer auftritt, wurden in dieser Arbeit Alkylanzien entwickelt, die zur besseren Inhibierung von microRNA beitragen sollen.
Als Alkylierungsmittel wurden ortho-Chinonmethide verwendet, die zunächst in geschützter Form synthetisiert wurden und nach Aktivierung mit einer Nukleobase reagieren können. Für die Erkennung der miRNA-Sequenz wurden diese zu einem Konjugat mit Peptid-Nukleinsäuren (PNAs) verbunden. Es wurden zwei Arten von Chinonmethid-Präkursoren hergestellt: Mit o Nitrobenzyl photolabil geschützte, die sich mit Licht der Wellenlänge 365 nm aktivieren lassen, und über ein Disulfid geschützte, die mithilfe eines Reduktionsmittels aktiviert werden. Die photolabil geschützten Derivate lassen sich damit gezielt örtlich und zeitlich aktivieren. Vom reduktiv aktivierbaren Präkursor wurden drei Derivate mit sterisch unterschiedlichen Resten am Disulfid (Benzyl-, Isopropyl- oder tert-Butyl-Rest) hergestellt, die einen Einfluss auf die Kinetik der Entschützung haben. Diese Derivate können nach Eintritt in eine Zelle durch die dort vorherrschende hohe Glutathion-Konzentration aktiviert werden, während sie extrazellulär unreaktiv sind.
Zunächst wurde die Kinetik eines photolabil geschützten Konjugats ohne RNA untersucht. Hier kommt es nach Bestrahlung zur Selbstalkylierung, bei der die Nukleobasen der PNA angegriffen werden. Bei 37 °C erfolgte dies mit einer Halbwertszeit von 0.43 h unter Annahme einer Reaktion 1. Ordnung. Die Kinetik der Alkylierung der komplementären RNA ließ sich durch zwei parallel ablaufende Reaktionen 1. Ordnung abbilden. Die Schnelle hatte eine Halbwertszeit von 0.42 h und die Langsame 11 h mit einer Ausbeute von 73 % nach 168 h. Bei Bestrahlung des Konjugats und erst anschließender Zugabe der RNA wurde ebenfalls eine Halbwertszeit von 11 h bei einer einzelnen Reaktionen 1. Ordnung erhalten. Dies lässt sich mit der Reversibilität mancher Reaktionsprodukte erklären. Die schnelle Reaktion entspricht der direkten Reaktion des Chinonmethids mit der RNA, die langsame entsteht durch Umlagerung von reversiblen Addukten.
Die Analyse der RNA-Alkylierung erfolgte mithilfe von denaturierender Polyacrylamid-Gelelektrophorese, bei der in Abhängigkeit der Gel-Temperatur scheinbar unterschiedliche Kinetiken gemessen wurden. Dies ist ebenfalls eine Folge der Reversibilität. Bei 57 °C kann ein Teil der Bindungen zwischen RNA und den Konjugaten brechen und es wird am Anfang der Reaktion eine geringere Ausbeute gemessen als bei 25 °C Geltemperatur. Die Ausbeute nach 168 h änderte sich jedoch nicht, da im Verlauf der Reaktion die reversiblen Addukte in irreversible umgewandelt werden.
Mit miRNA-20a als Ziel wurden mit einem 10mer Konjugat zunächst nur 13 % Ausbeute nach 72 h und mit einem 15mer Konjugat 41 % nach 75 h erreicht. Durch internen Einbau des Chinonmethid-Präkursors in die PNA, sodass es einem Adenosin der RNA gegenübersteht, konnte die Ausbeute auf 75 % nach 72 h gesteigert werden, da Adenosin bevorzugt alkyliert wird.
Bei den reduktiv aktivierbaren Chinonmethid-Präkursoren waren alle synthetisierten Konjugate in Puffer ohne Glutathion (GSH) stabil. Die Reihenfolge der Reaktionsgeschwindigkeit der Disulfidspaltung war bei 0.5 mM und 10 mM GSH: Benzyl > Isopropyl > tert-Butyl. Die Halbwertszeit bei 10 mM GSH betrug weniger als 5 min (Benzyl-Konjugat) bis 2 h (t Butyl Konjugat). Jedoch bildeten sich mit allen Konjugaten bei 10 mM GSH auch Addukte mit GSH.
Die Reaktivitätsreihenfolge blieb bei der Alkylierung von RNA erhalten. Allein das Benzyl-Konjugat erreichte bei einer GSH-Konzentration von 0.5 mM schon die gleiche Reaktionsgeschwindigkeit wie das photolabil geschützte Chinonmethid. Bei 10 mM GSH erreichten die Derivate zwar nach wenigen Stunden ihre maximale Ausbeute, diese betrug jedoch nur 23 % (tert-Butyl-Konjugat) bis 43 % (Benzyl-Konjugat), da die Chinonmethide auch durch GSH als Nukleophil abgefangen werden.
Mit einem Konjugat, das ein photolabiles Chinonmethid sowie Biotin trägt, wurde ein Fluoreszenzpulldown mit Cy5-markierter RNA durchgeführt. Hier zeigte die bestrahlte Probe eine deutlich höhere Fluoreszenz (6.8x), als eine unbestrahlte Vergleichsprobe. Bei einem Pulldown-Versuch mit miRNA-20a bzw. mit RISCs aus HeLa-Zelllysat konnte das Argonautenprotein jedoch nicht eindeutig mittels Westernblot nachgewiesen werden.
Anhand des reduktiv aktivierbaren Benzyl-Konjugats konnte gezeigt werden, dass sich das Konjugat in Zelllysat zersetzt und nur ein Teil zu Addukten mit Nukleobasen reagiert. Die Ursache wurde in der hydrolyselabilen Abgangsgruppe gesehen, sodass weitere photolabil geschützte Derivate mit Dimethylamino-, Trimethylammonium-, Pivaloylester- und Benzoylestergruppe synthetisiert wurden. Von diesen war nur das Benzoylester-Konjugat in der Lage, RNA mit 72 % Ausbeute nach 48 Stunden zu alkylieren. Zudem war es für mindestens 1 h in Zelllysat stabil.
Polyketides are highly valuable natural products, which are widely used as pharmaceuticals due to their beneficial characteristics, comprising antibacterial, antifungal, immunosuppressive, and antitumor properties, among others. Their biosynthesis is performed by large and complex multiproteins, the polyketide synthases (PKSs). This study solely focuses on the class of type I PKSs, which arrange all their enzymatic domains on one or more polypeptides. Despite their high medical value, little is known about mechanistic details in PKSs.
One central domain is the acyl transferase (AT), which is present in all PKSs and channels small acyl substrates into the enzyme. More precisely, the AT loads the substrates onto the essential acyl carrier protein (ACP), which subsequently shuttles the substrates and all intermediates for condensation and modification to additional domains to build the final polyketide.
Some PKSs use their domains several times during biosynthesis and work iteratively – these are called iterative PKSs. Others feature several sets of domains, each being used only once during biosynthesis – these PKSs are called modular PKSs. All PKSs or PKS modules consist of minimum three essential domains to connect the acyl substrates. Three modifying domains are optional and can enlarge the minimal set. According to the domain composition, the acyl substrate is fully reduced, partly reduced, or not reduced at all. This variation of modifying domains accounts for the huge structural and therefore functional variety of polyketides.
Even though the structure of fatty acids is not exactly reminiscent of polyketides, their biosynthetic pathways are closely related. Fatty acid biosynthesis is carried out by fatty acid synthases (FASs), which share many similarities with PKSs. Both megasynthases feature the same domains, performing the same reactions to connect and modify small acyl substrates. In contrast to PKSs, FASs always contain one full set of modifying domains which is used iteratively, leading to fully reduced fatty acids.
The present thesis extensively analyzes the AT of different PKSs in its substrate selectivity, AT-ACP domain-domain interaction, and enzymatic kinetic properties. The following key findings are revealed through comparison: 1.) ATs of PKSs appear slower than the ones of FASs, which may reflect the different scopes of biosynthetic pathways. Fatty acids as essential compounds in all organisms are needed in high amounts for physiological functions, whereas polyketides as secondary metabolites only require basal concentrations to take effect. 2.) The slower ATs from modular PKSs do not load non-native substrates even in absence of the native substrates. This is different to the faster ATs from iterative PKSs and FASs, which indicates high substrate specificity solely for the ATs from modular PKSs and emphasizes their role as gatekeepers in polyketide synthesis. 3.) The substrate selectivity can emerge in either the first or the second step of the AT-mediated ACP loading and is not assured by a hydrolytic proofreading function.
Moreover, a mutational study on the AT-ACP interaction in the modular PKS 6-deoxyerythronolide B synthase (DEBS) shows that single surface point mutations can influence AT-mediated reactions in a complex manner. Data reveals high enzyme kinetic plasticity of the AT-ACP interaction, which was also recently demonstrated for the interaction in a type II FAS.
Based on these findings, the mammalian FAS is engineered towards a modular PKS-like as- sembly line with the long-term goal to rationally synthesize new products. Basically, three important aspects need to be considered: 1.) AT’s loading needs to be splitted in specific loading of a priming substrate by a priming AT and in specific loading of an elongation substrate by an elongation AT. 2.) FAS-based elongation modules need to be designed with varying domain compositions for introducing functional groups in the product. 3.) Covalent and non-covalent linkers need to be designed for connection of priming and elongation modules.
This study focuses on the first aspect, splitting loading of priming and elongation substrates. An elongation substrate-specific AT is installed in the mammalian FAS via domain swapping. Since ATs from modular PKSs were proven to be substrate specific, these are used to exchange the mammalian FAS AT. This work demonstrates that it is extremely challenging to create stable and functional chimeras, but first essential steps are taken. Proper domain boundaries for AT swapping are established and a stable chimera with 70 % wild type AT activity is created. However, this chimera is only of limited value for application in an elongation module due to the intrinsic slow turnover rate of the wild type AT. Using another PKS AT, a stable elongation module is designed and analyzed in its activity in combination with a priming module. These experiments demonstrate that the loading of priming substrates are successfully suppressed in the elongation module, but nonetheless only minor turnover rates are detected in the assembly line.
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Organ-on-a-chip technology has the potential to accelerate pharmaceutical drug development, improve the clinical translation of basic research, and provide personalized intervention strategies. In the last decade, big pharma has engaged in many academic research cooperations to develop organ-on-a-chip systems for future drug discoveries. Although most organ-on-a-chip systems present proof-of-concept studies, miniaturized organ systems still need to demonstrate translational relevance and predictive power in clinical and pharmaceutical settings. This review explores whether microfluidic technology succeeded in paving the way for developing physiologically relevant human in vitro models for pharmacology and toxicology in biomedical research within the last decade. Individual organ-on-a-chip systems are discussed, focusing on relevant applications and highlighting their ability to tackle current challenges in pharmacological research.
In den letzten 20 Jahren haben sich zunehmend Schülerlabore an Universitäten und Forschungszentren etabliert, um naturwissenschaftliche Kompetenzen von Schülern/innen aufzubauen und zu fördern. Das wachsende Feld der Schülerlaborforschung zeigt allerdings auf, dass die Eingangsvoraussetzungen, mit denen die Schüler/innen an der naturwissenschaftlichen Lernumgebung teilnehmen, einen starken Einfluss auf die Annahme sowie die Entwicklung von interessens-, selbstkonzept- und motivationsbezogenen Persönlichkeitsmerkmalen haben können. Diese Erkenntnisse lenken den Blick auf die Entwicklungsumwelt der Familien, in der die Eltern von Geburt an auf die kindliche Persönlichkeitsentwicklung und Lernprozesse einwirken. Die Integration des vielversprechenden familiären Kontexts in eine naturwissenschaftliche Lernumgebung wird seit 2008 anhand des Eltern-Kind-Projekts KEMIE® an der Ruhr-Universität Bochum umgesetzt, indem Eltern-Kind-Paare gemeinsam an alltagsnahen naturwissenschaftlichen Phänomenen experimentieren. Seit 2016 wird KEMIE® zudem an der Goethe-Universität Frankfurt am Main im Goethe-Schülerlabor Chemie durchgeführt.
Am Beispiel des Frankfurter KEMIE®-Projekts will die vorliegende Arbeit das Potential von Eltern-Kind-Interaktionen für naturwissenschaftliche Lernprozesse untersuchen. Mithilfe der Grounded-Theory-Methodologie wurde das zentrale Forschungsdesiderat der Eltern-Kind-Interaktion über die Projektjahre 2016/17 und 2017/18 herausgestellt sowie mögliche Erhebungsmethoden pilotiert. Im Projektjahr 2018/19 konnte dieses schließlich in einer Mixed-Methods-Studie multiperspektivisch beforscht werden. Dafür wurden Interviews, Beobachtungen und Pre-Posttest-Daten von 46 teilnehmenden Eltern-Kind-Paaren sowie weitere Kontrollgruppendaten von 202 Frankfurter Familien erhoben.
Um zunächst die naturwissenschaftliche Lernumgebung zu beschreiben, wurden die vorherrschenden Einflussfaktoren identifiziert, die zugehörigen Phänomene beschrieben sowie die prozess- und personenbezogenen Verhaltensmuster herausgestellt. Über letztere können die Eltern-Kind-Interaktionen in das SELE-Modell elterlicher Unterstützungsmaßnahmen eingeordnet werden, wobei sich das Ermöglichen von Selbsttätigkeit als herausragendes Merkmal für die naturwissenschaftliche Lernumgebung manifestiert. Zudem zeigt sich, dass das Projekt positive Effekte auf naturwissenschaftsbezogene Werteorientierungen der Kinder sowie deren Interesse an den Naturwissenschaften hat.
Anhand der Entwicklung eines induktiven Beobachtungsschemas, konnten die Familien schließlich über die Verhaltensmerkmale der Eltern-Kind-Interaktion gruppiert und Zusammenhänge zu sowohl den Vorbedingungen als auch den Konsequenzen für die psychischen Dispositionen der Kinder aufgedeckt werden. Erste Erkenntnisse dieser explorativen Erhebung zeigen, dass das akademische Selbstkonzept und die naturwissenschaftsbezogenen Werteorientierungen der Eltern und Kinder die Verhaltensmuster in der naturwissenschaftlichen Umgebung determinieren. Auf der anderen Seite können die Kinder gerade hinsichtlich dieser beiden Faktoren am meisten profitieren. Dabei können diese positiven Effekte auf eine Regulation seitens der Eltern, das gemeinsame Ausführen von Tätigkeiten sowie den Einbezug in die Gestaltung der Lernumgebung zurückgeführt werden.
Osteopontin levels in human milk are related to maternal nutrition and infant health and growth
(2021)
Background: Osteopontin (OPN) is a glycosylated phosphoprotein found in human tissues and body fluids. OPN in breast milk is thought to play a major role in growth and immune system development in early infancy. Here, we investigated maternal factors that may affect concentrations of OPN in breast milk, and the possible associated consequences for the health of neonates. Methods: General characteristics, health status, dietary patterns, and anthropometric measurements of 85 mothers and their babies were recorded antenatally and during postnatal follow-up. Results: The mean concentration of OPN in breast milk was 137.1 ± 56.8 mg/L. Maternal factors including smoking, BMI, birth route, pregnancy weight gain, and energy intake during lactation were associated with OPN levels (p < 0.05). Significant correlations were determined between body weight, length, and head circumference, respectively, and OPN levels after one (r = 0.442, p = < 0.001; r = −0.284, p = < 0.001; r = −0.392, p = < 0.001) and three months (r = 0.501, p = < 0.001; r = −0.450, p = < 0.001; r = −0.498, p = < 0.001) of lactation. A negative relation between fever-related infant hospitalizations from 0–3 months and breast milk OPN levels (r = −0.599, p < 0.001) was identified. Conclusions: OPN concentrations in breast milk differ depending on maternal factors, and these differences can affect the growth and immune system functions of infants. OPN supplementation in infant formula feed may have benefits and should be further investigated.
Pancreatic cancer is a common malignant tumor with a high incidence and mortality rate. The prognosis of patients with pancreatic cancer is considerably poor due to the lack of effective treatment in clinically. Despite numerous studies have revealed that baicalein, a natural product, is responsible for suppressing multiple cancer cells proliferation, motility and invasion. The mechanism by which baicalein restraining pancreatic cancer progression remains unclear. In this study, we firstly verified that baicalein plays a critical role in inhibiting pancreatic tumorigenesis in vitro and in vivo. Then we analyzed the alteration of microRNAs (miRNAs) expression levels in Panc-1 cells incubated with DMSO, 50 and 100 μM baicalein by High-Throughput sequencing. Intriguingly, we observed that 20 and 39 miRNAs were accordingly up- and down-regulated through comparing Panc-1 cells exposed to 100 μM baicalein with the control group. Quantitative PCR analysis confirmed that miR-139-3p was the most up-regulated miRNA after baicalein treatment, while miR-196b-5p was the most down-regulated miRNA. Further studies showed that miR-139-3p induced, miR-196b-5p inhibited the apoptosis of Panc-1 cells via targeting NOB1 and ING5 respectively. In conclusion, we demonstrated that baicalein is a potent inhibitor against pancreatic cancer by modulating the expression of miR-139-3p or miR-196b-5p.
2D NOESY plays a central role in structural NMR spectroscopy. We have recently discussed methods that rely on solvent-driven exchanges to enhance NOE correlations between exchangeable and non-exchangeable protons in nucleic acids. Such methods, however, fail when trying to establish connectivities within pools of labile protons. This study introduces an alternative that also enhances NOEs between such labile sites, based on encoding a priori selected peaks by selective saturations. The resulting selective magnetization transfer (SMT) experiment proves particularly useful for enhancing the imino–imino cross-peaks in RNAs, which is a first step in the NMR resolution of these structures. The origins of these enhancements are discussed, and their potential is demonstrated on RNA fragments derived from the genome of SARS-CoV-2, recorded with better sensitivity and an order of magnitude faster than conventional 2D counterparts.
Background and Purpose: The cyclic nucleotides cAMP and cGMP are ubiquitous second messengers regulating numerous biological processes. Malfunctional cNMP signalling is linked to diseases and thus is an important target in pharmaceutical research. The existing optogenetic toolbox in Caenorhabditis elegans is restricted to soluble adenylyl cyclases, the membrane-bound Blastocladiella emersonii CyclOp and hyperpolarizing rhodopsins; yet missing are membrane-bound photoactivatable adenylyl cyclases and hyperpolarizers based on K+ currents.
Experimental Approach: For the characterization of photoactivatable nucleotidyl cyclases, we expressed the proteins alone or in combination with cyclic nucleotide-gated channels in muscle cells and cholinergic motor neurons. To investigate the extent of optogenetic cNMP production and the ability of the systems to depolarize or hyperpolarize cells, we performed behavioural analyses, measured cNMP content in vitro, and compared in vivo expression levels.
Key Results: We implemented Catenaria CyclOp as a new tool for cGMP production, allowing fine-control of cGMP levels. We established photoactivatable membrane-bound adenylyl cyclases, based on mutated versions (“A-2x”) of Blastocladiella and Catenaria (“Be,” “Ca”) CyclOp, as N-terminal YFP fusions, enabling more efficient and specific cAMP signalling compared to soluble bPAC, despite lower overall cAMP production. For hyperpolarization of excitable cells by two-component optogenetics, we introduced the cAMP-gated K+-channel SthK from Spirochaeta thermophila and combined it with bPAC, BeCyclOp(A-2x), or YFP-BeCyclOp(A-2x). As an alternative, we implemented the B. emersonii cGMP-gated K+-channel BeCNG1 together with BeCyclOp.
Conclusion and Implications: We established a comprehensive suite of optogenetic tools for cNMP manipulation, applicable in many cell types, including sensory neurons, and for potent hyperpolarization.
We investigated the folding kinetics of G-quadruplex (G4) structures by comparing the K+-induced folding of an RNA G4 derived from the human telomeric repeat-containing RNA (TERRA25) with a sequence homologous DNA G4 (wtTel25) using CD spectroscopy and real-time NMR spectroscopy. While DNA G4 folding is biphasic, reveals kinetic partitioning and involves kinetically favoured off-pathway intermediates, RNA G4 folding is faster and monophasic. The differences in kinetics are correlated to the differences in the folded conformations of RNA vs. DNA G4s, in particular with regard to the conformation around the glycosidic torsion angle χ that uniformly adopts anti conformations for RNA G4s and both, syn and anti conformation for DNA G4s. Modified DNA G4s with 19F bound to C2′ in arabino configuration adopt exclusively anti conformations for χ. These fluoro-modified DNA (antiTel25) reveal faster folding kinetics and monomorphic conformations similar to RNA G4s, suggesting the correlation between folding kinetics and pathways with differences in χ angle preferences in DNA and RNA, respectively.
The assembly of a specific polymeric ubiquitin chain on a target protein is a key event in the regulation of numerous cellular processes. Yet, the mechanisms that govern the selective synthesis of particular polyubiquitin signals remain enigmatic. The homologous ubiquitin-conjugating (E2) enzymes Ubc1 (budding yeast) and Ube2K (mammals) exclusively generate polyubiquitin linked through lysine 48 (K48). Uniquely among E2 enzymes, Ubc1 and Ube2K harbor a ubiquitin-binding UBA domain with unknown function. We found that this UBA domain preferentially interacts with ubiquitin chains linked through lysine 63 (K63). Based on structural modeling, in vitro ubiquitination experiments, and NMR studies, we propose that the UBA domain aligns Ubc1 with K63-linked polyubiquitin and facilitates the selective assembly of K48/K63-branched ubiquitin conjugates. Genetic and proteomics experiments link the activity of the UBA domain, and hence the formation of this unusual ubiquitin chain topology, to the maintenance of cellular proteostasis.
Lead-optimization strategies for compounds targeting c-Myc G-quadruplex (G4) DNA are being pursued to develop anticancer drugs. Here, we investigate the structure-activity- relationship (SAR) of a newly synthesized series of molecules based on the pyrrolidine-substituted 5-nitro indole scaffold to target G4 DNA. Our synthesized series allows modulation of flexible elements with a structurally preserved scaffold. Biological and biophysical analyses illustrate that substituted 5-nitroindole scaffolds bind to the c-Myc promoter G-quadruplex. These compounds downregulate c-Myc expression and induce cell-cycle arrest in the sub-G1/G1 phase in cancer cells. They further increase the concentration of intracellular reactive oxygen species. NMR spectra show that three of the newly synthesized compounds interact with the terminal G-quartets (5′- and 3′-ends) in a 2 : 1 stoichiometry.
Medicinal plants represent a big reservoir for discovering new drugs against all kinds of diseases including inflammation. In spite the large number of promising anti-inflammatory plant extracts and isolated components, research on medicinal plants proves to be very difficult. Based on that background this review aims to provide a summarized insight into the hitherto known pharmacologically active concentrations, bioavailability, and clinical efficacy of boswellic acids, curcumin, quercetin and resveratrol. These examples have in common that the achieved plasma concentrations were found to be often far below the determined IC50 values in vitro. On the other hand demonstrated therapeutic effects suggest a necessity of rethinking our pharmacokinetic understanding. In this light this review discusses the value of plasma levels as pharmacokinetic surrogates in comparison to the more informative value of tissue concentrations. Furthermore the need for new methodological approaches is addressed like the application of combinatorial approaches for identifying and pharmacokinetic investigations of active multi-components. Also the physiological relevance of exemplary in vitro assays and absorption studies in cell-line based models is discussed. All these topics should be ideally considered to avoid inaccurate predictions for the efficacy of herbal components in vivo and to unlock the “black box” of herbal mixtures.
Metabolic syndrome (MetS) is a highly prevalent disease cluster worldwide. It requires polypharmacological treatment of the single conditions including type II diabetes, hypertension, and dyslipidemia, as well as the associated comorbidities. The complex treatment regimens with various drugs lead to drug-drug interactions and inadequate patient adherence, resulting in poor management of the disease. Multi-target approaches aim at reducing the polypharmacology and improving the efficacy. This review summarizes the medicinal chemistry efforts to develop multi-target ligands for MetS. Different combinations of pharmacological targets in context of in vivo efficacy and future perspective for multi-target drugs in MetS are discussed.
Therapeutic oligonucleotides interact with a target RNA via Watson-Crick complementarity, affecting RNA-processing reactions such as mRNA degradation, pre-mRNA splicing, or mRNA translation. Since they were proposed decades ago, several have been approved for clinical use to correct genetic mutations. Three types of mechanisms of action (MoA) have emerged: RNase H-dependent degradation of mRNA directed by short chimeric antisense oligonucleotides (gapmers), correction of splicing defects via splice-modulation oligonucleotides, and interference of gene expression via short interfering RNAs (siRNAs). These antisense-based mechanisms can tackle several genetic disorders in a gene-specific manner, primarily by gene downregulation (gapmers and siRNAs) or splicing defects correction (exon-skipping oligos). Still, the challenge remains for the repair at the single-nucleotide level. The emerging field of epitranscriptomics and RNA modifications shows the enormous possibilities for recoding the transcriptome and repairing genetic mutations with high specificity while harnessing endogenously expressed RNA processing machinery. Some of these techniques have been proposed as alternatives to CRISPR-based technologies, where the exogenous gene-editing machinery needs to be delivered and expressed in the human cells to generate permanent (DNA) changes with unknown consequences. Here, we review the current FDA-approved antisense MoA (emphasizing some enabling technologies that contributed to their success) and three novel modalities based on post-transcriptional RNA modifications with therapeutic potential, including ADAR (Adenosine deaminases acting on RNA)-mediated RNA editing, targeted pseudouridylation, and 2′-O-methylation.
Fatty acid and polyketide synthases (FASs and PKSs) synthesize physiologically and pharmaceutically important products by condensation of acyl building blocks. The transacylation reaction catalyzed by acyl transferases (ATs) is responsible for the selection of acyl-CoA esters for further processing by FASs and PKSs. In this study, the AT domains of different multidomain (type I) PKS systems are kinetically described in their substrate selectivity, AT−Acyl carrier protein (ACP) domain-domain interaction and enzymatic kinetic properties. We observe that the ATs of modular PKSs, intricate protein complexes occurring in bacteria and responsible for the biosynthesis of bioactive polyketides, are significantly slower than ATs of mammalian FASs, reflecting the respective purpose of the biosynthetic pathways within the organism and their metabolic context. We further perform a mutational study on the kinetics of the AT−ACP interaction in the modular PKS 6-deoxyerythronolide B synthase (DEBS) and find a high plasticity in enzyme properties, which we explain by a high plasticity in AT−ACP recognition. Our study enlarges the understanding of ATs in its molecular properties and is similarly a call for thorough AT-centered PKS engineering strategies.
Mit 71 Millionen chronisch erkrankten Patienten im Jahr 2015 stellt die chronische Hepatitis C-Virusinfektion eine wichtige Ursache für Zirrhose, Leberdekompensation und Leberkrebs dar.
Eine grundlegende Eigenschaft des Hepatitis C-Virus (HCV) ist die Biogenese modifizierter intrazellulärer Membranen. Das dabei aus dem endoplasmatischen Reticulum (ER) gebildete, sogenannte membranöse Netz (MW, membranous web) dient im Rahmen des HCV-Lebenszyklus als Gerüst für die Assemblierung eines Multi-Protein-Replikase-Komplexes. Das MW wird durch virale nicht-strukturelle Proteine wie NS5A induziert.
Das Multidomänen-Metalloprotein NS5A ist über seine verschiedenen Domänen sowohl bei der Replikation am MW als auch bei der viralen Assemblierung und Freisetzung in der Nähe von Lipidtropfen (LD, lipid droplet) maßgeblich beteiligt. Seine N-terminale amphipathische Helix (AH) spielt dabei über die vermittelte Assoziation von NS5A mit Membranen eine wichtige Rolle. Damit verbundene spezifische Lipidinteraktionen von NS5A unterliegen molekularen Umstrukturierungen, die benötigt werden, um NS5A für seine
verschiedenen Aufgaben im viralen Lebenszyklus anzupassen. Es liegen zwar Röntgen-strukturmodelle von Domäne 1-Dimeren und NMR-Strukturen zur AH vor, allerdings keine experimentellen Strukturen des NS5A-Proteins vollständiger Länge (NS5A fl) in seinem natürlichen Lipidmilieu. Trotz der essentiellen Bedeutung von NS5A für den HCV-Lebens-zyklus und langjähriger Forschung ist bisher nur wenig zur molekularen Funktionsweise von NS5A bekannt.
Dennoch konnten durch Screening hochpotente NS5A-Inhibitoren entdeckt und weiterentwickelt werden. NS5A-Inhibitoren tragen als direkt wirkende antivirale Arzneimittel(DAA, direct-acting antiviral) entscheidend zum Therapieerfolg bei der Behandlung der Hepatitis C bei. Trotz ihrer Bedeutung in der Therapie und intensiver Forschung ist der Wirk-mechanismus von NS5A-Inhibitoren bisher ungeklärt. Eine durch NS5A-Inhibitoren
induzierte intrazelluläre Umverteilung von NS5A und das ausschließliche Auftreten von Resistenz-assoziierten Mutationen (RAM) nahe der NS5A-Lipid-Interaktionsbereiche weisen jedoch auf einen Effekt der Inhibitoren auf die Lipid-NS5A-Interaktion hin.
Als grundlegende Hypothese dieser Arbeit wurde somit vermutet, dass abhängig vom NS5A umgebenden Lipidmilieu (MW oder LD) spezifische Lipid-Protein-Interaktionen Einfluss auf die Struktur und Funktion von NS5A nehmen und NS5A-Inhibitoren über eine Inhibition dieser Interaktionen wirken. Polyphosphoinositide (PPI) könnten dabei als Lipidinteraktionspartner eine besondere Rolle spielen, da sie bedeutend für die Membran-Kennzeichnung verschiedener Zellkompartimente sind und auch die Funktion von Membranproteinen regulieren können. Eine Interaktion von NS5A mit PtdIns(4,5)P2 wurde bereits publiziert.
Um basierend auf der postulierten Hypothese die mechanistischen Details im Wechselspiel von NS5A und intrazellulären Membranen sowie den dabei möglichen Effekt von
NS5A-Inhibitoren zu untersuchen, musste zunächst NS5A in ausreichender Menge, Reinheit und Qualität rekombinant hergestellt werden. Hierfür wurde ein entsprechendes Protokoll zur Proteinexpression durch Baculovirus-vermittelte Expression in Sf9-Insektenzellen und Strep-Tactin-Reinigung für das full length Protein und trunkierte Varianten etabliert.
In Kooperation mit einem Partner konnte unter Verwendung von giant unilamellar vesicles (GUVs) und konfokaler Mikroskopie gezeigt werden, dass unser full length Protein die Struktur von Membranen verändert (Membran-Remodellierung).
Die Stabilität des gereinigten Proteins und damit Effekte auf die Proteinfaltung wurden mittels Thermal shift assay (TSA) untersucht und dabei auch Effekte des NS5A-Inhibitors
Daclatasvir (DCV) und des Metall-Chelators EDTA überprüft. Die Bindung des Inhibitors hatte einen stabilisierenden Effekt auf die Proteinstruktur zur Folge.
Potentielle Interaktionsmuster mit Membranlipiden wurden mit Hilfe eines Protein lipid overlay assays (PLOA) detektiert. Zusätzlich zum in der Literatur bereits beschriebenen
Interaktionspartner PtdIns(4,5)P2 konnten weitere Lipid-Bindungspartner für NS5A identifiziert werden. Dabei legen die gewonnenen Daten nahe, dass die Interaktion über die Domäne 1 von NS5A vermittelt wird, wobei die Domänen 2 und 3 die Affinität zu den Lipidbindungspartnern erhöht, aber nicht das Phospholipid-Bindungsmuster verändert.
DCV hatte im PLOA keine qualitativen Auswirkungen auf das Lipid-Bindungsmuster. Die Lipidinteraktionen wurden mittels eines Liposomen-Rekonstitutionsmodells validiert.
In silico konnten basierend auf verfügbaren, experimentellen Strukturdaten und einem dynamischen Modell drei Cluster basischer Aminosäuren in NS5A-D1-AH als mögliche
PPI-Bindungsstellen identifiziert werden. Basierend auf dem Strukturmodell wurde eine Mutationsstrategie zur Charakterisierung der potentiellen PPI-Bindungsstellen entwickelt.
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An approach for the comparison of pair distribution functions (PDFs) has been developed using a similarity measure based on cross-correlation functions. The PDF is very sensitive to changes in the local structure, i.e. small deviations in the structure can cause large signal shifts and significant discrepancies between the PDFs. Therefore, a comparison based on pointwise differences (e.g. R values and difference curves) may lead to the assumption that the investigated PDFs as well as the corresponding structural models are not in agreement at all, whereas a careful visual inspection of the investigated structural models and corresponding PDFs may reveal a relatively good match. To quantify the agreement of different PDFs for those cases an alternative approach is introduced: the similarity measure based on cross-correlation functions. In this paper, the power of this application of the similarity measure to the analysis of PDFs is highlighted. The similarity measure is compared with the classical Rwp values as representative of the comparison based on pointwise differences as well as with the Pearson product-moment correlation coefficient, using polymorph IV of barbituric acid as an example.
A method for the ab initio crystal structure determination of organic compounds by a fit to the pair distribution function (PDF), without prior knowledge of lattice parameters and space group, has been developed. The method is called ‘PDF-Global-Fit’ and is implemented by extension of the program FIDEL (fit with deviating lattice parameters). The structure solution is based on a global optimization approach starting from random structural models in selected space groups. No prior indexing of the powder data is needed. The new method requires only the molecular geometry and a carefully determined PDF. The generated random structures are compared with the experimental PDF and ranked by a similarity measure based on cross-correlation functions. The most promising structure candidates are fitted to the experimental PDF data using a restricted simulated annealing structure solution approach within the program TOPAS, followed by a structure refinement against the PDF to identify the correct crystal structure. With the PDF-Global-Fit it is possible to determine the local structure of crystalline and disordered organic materials, as well as to determine the local structure of unindexable powder patterns, such as nanocrystalline samples, by a fit to the PDF. The success of the method is demonstrated using barbituric acid as an example. The crystal structure of barbituric acid form IV solved and refined by the PDF-Global-Fit is in excellent agreement with the published crystal structure data.
Multi-subunit ATPase-dependent chromatin remodelling complexes SWI/SNF (switch/sucrose non-fermentable) are fundamental epigenetic regulators of gene transcription. Functional genomic studies revealed a remarkable mutation prevalence of SWI/SNF-encoding genes in 20–25% of all human cancers, frequently driving oncogenic programmes. Some SWI/SNF-mutant cancers are hypersensitive to perturbations in other SWI/SNF subunits, regulatory proteins and distinct biological pathways, often resulting in sustained anticancer effects and synthetic lethal interactions. Exploiting these vulnerabilities is a promising therapeutic strategy. Here, we review the importance of SWI/SNF chromatin remodellers in gene regulation as well as mechanisms leading to assembly defects and their role in cancer development. We will focus in particular on emerging strategies for the targeted therapy of SWI/SNF-deficient cancers using chemical probes, including proteolysis targeting chimeras, to induce synthetic lethality.
Die vorliegende Arbeit Zeitaufgelöste NMR-spektroskopische Untersuchung konformationeller Dynamiken in DNA G-Quadruplexen befasst sich mit der detaillierten biophysikalischen Untersuchung wichtiger strukturdynamischer Eigenschaften von nicht-kanonischen Nukleinsäure Sekundärstrukturelementen.
Im Genom aller eukaryotischer Lebewesen, insbesondere dem menschlichen Genom finden sich DNA-Sequenzabschnitte, die überdurchschnittlich Guanosin (G)-reich sind. Diese poly-G Abschnitte sind nicht zufällig im Genom verteilt, sondern häufen sich vermehrt in Genabschnitten, die besonders wichtig für die Regulation der Genexpression sind. G-reiche DNA-Sequenzen können unter geeigneten Umständen alternative Sekundärstrukturen ausbilden, die von der doppelsträngigen, kanonischen Watson-Crick Konformation abweichen. In Anwesenheit monovalenter Kationen können sich G-Nukleotide in einer Tetrade über Hoogsteen Interaktionen anlagern. Diese Tetraden können sich stapeln und dadurch sogenannte G-Quadruplexe (G4) ausbilden. Das menschliche cMYC Gen wird typischerweise als proto-Onkogen bezeichnet. Es kodiert für einen unspezifischen Transkriptionsfaktor, der bei einer Vielzahl von systematischen und soliden Tumorerkrankungen stark überexprimiert wird. Die zelluläre Konzentration des Genprodukts kann zu 90% über ein G4 cis-Element in der Promotorregion reguliert werden. Der cMYC G4 hat die Möglichkeit verschiedene Konformationen einzunehmen. Im Falle des cMYC G4 kann man zusätzliche, nicht-konventionelle Formen der konformationellen Isomerie finden. Zum einen gibt es die Möglichkeit, dass bei einem G4, der aus drei Tetraden und vier intramolekularen Strangabschnitten (dreistöckiger G4) besteht, einzelne Strangabschnitte mehr als drei konsekutive G-Nukleotide besitzen. Dadurch können sich Faltungs-Isomere bilden, die sich durch Verschieben des Strangs relativ zum verbleibenden dreistöckigen Tetradengerüst ergeben. Man spricht von G-Register Isomeren. Eine zweite Möglichkeit der Strukturisomerie ergibt sich, wenn in einer Nukleotidsequenz mehr als vier G-reiche Strangabschnitte aufeinander folgen. Jeweils vier dieser Strangabschnitte können in unterschiedlicher Weise kombiniert werden, um ein G4 Isomer auszubilden. In jedem dieser so zustande gekommenen G4 verbleibt ein (oder mehrere) G-reicher Strangabschnitt, der im konkreten Isomer nicht zur Faltung verwendet wird. Diese zusätzlichen G-Stränge werden daher auch Ersatzräder (engl. spare-tires) genannt; man erhält spare-tire Isomere.
Obwohl diese Formen des Polymorphismus, deren biologischer Kontext und die biophysikalischen Konsequenzen in Arbeiten von C. Burrows (2015) und A. Mittermaier (2016) erstmals umfassend beschrieben wurden, gab es bis zum Ausgangspunkt dieser Arbeit keine Kenntnisse über deren strukturelle Dynamik, den Faltungswegen und den zugrundeliegenden molekularen Mechanismen. Zeitaufgelöste Kernspinresonanz (engl. nuclear magnetic resonance, NMR) Spektroskopie ist eine bestens geeignete Methode, um die Dynamik von Biomakromolekülen mit atomarer Auflösung zu studieren. Um solche Experimente durchführen zu können, braucht es geeignete Herangehensweisen für die Präparation eines Nicht-Gleichgewichtszustands. In dieser Arbeit wird eine neu erarbeitete Strategie vorgestellt, die es erlaubt, Einblick in die Faltungs- und Umfaltungskinetiken eines dynamischen Konformations-Ensembles nicht-konventioneller Strukturisomere der cMYC G4 DNA-Sequenz zu erhalten.
Hierzu wurden photolabile Schutzgruppen (engl. Photocages) positionsspezifisch an bestimmten G-Nukleobasen (O6-(R)-NPE) angebracht. Die Schutzgruppen blockieren die Basenpaar-Interaktionen des Nukleotids, wodurch dieses sich nicht mehr an einer Tetradenbildung beteiligen kann. Die Photocages wurden jeweils an den Nukleotiden eingeführt, die nur in jeweils einem der G-Register Isomere an der Tetradenbildung beteiligt sind. Durch diese gezielte Destabilisierung konnten die Isomere getrennt und im gefalteten Zustand isoliert werden. Die so erhaltenen Konformationen wurden umfassend spektroskopisch charakterisiert. Der Ansatz, das konformationelle Gleichgewicht durch Photocages transient zu stören, wurde daraufhin weiterentwickelt. Mehrere Photocages wurden an Nukleobasen in zentraler Position einzelner G-Strangabschnitte angebracht. Dadurch konnte eine ausreichende Destabilisierung erreicht werden, die die Faltung jedweder G4 Strukturen unterbindet. Somit wurde ein ungefalteter Zustand erzeugt, der unter ansonsten frei wählbaren, physiologischen Bedingungen besteht. Durch in situ Photolyse der Schutzgruppen konnte so die Licht-induzierte G4 Faltung unter konstanten Puffer- und Temperaturbedingungen untersucht werden. Dieser Ansatz wurde auf die Untersuchung der Faltungswege, die zu verschiedenen spare-tire Isomeren führen, fokussiert.
Zusammenfassend kann festgestellt werden, dass es insgesamt erstmalig gelungen ist, die Kinetiken der wesentlichen Faltungs- und Umfaltungswege entlang der konformationellen Energielandschaft des cMYC G4 Elements zu untersuchen. Das komplexe, dynamische Zusammenspiel aller relevanten, nicht-konventionellen isomeren G4 Strukturen konnte entworren und umfassend experimentell beschrieben werden. Der dafür weiterentwickelte Ansatz über konformationelle Selektion mit Hilfe photolabiler Schutzgruppen hat dabei experimentelle Einblicke erlaubt, die bislang nicht zugänglich waren. Die Strukturen und Faltungszustämde, die mit den chemisch modifizierten Oligonukleotiden erhalten und isoliert wurden, sind umfassend spektroskopisch untersucht worden. Die Anwendung verschiedener spektroskopischer Ansätze und deren Kombination mit weiteren biophysikalischen Methoden hat eine Methoden-unabhängige Validierung der erhaltenen kinetischen und thermodynamischen Daten ermöglicht.
Background and Purpose: Activation of hepatic thyroid hormone receptor β (THR-β) is associated with systemic lipid lowering, increased bile acid synthesis, and fat oxidation. In patients with non-alcoholic steatohepatitis (NASH), treatment with THR-β agonists decreased hepatic steatosis and circulating lipids, and induced resolution of NASH. We chose resmetirom (MGL-3196), a liver-directed, selective THR-β agonist, as a prototype to investigate the effects of THR-β activation in mice with diet-induced obesity (DIO) and biopsy-confirmed advanced NASH with fibrosis.
Experimental Approach: C57Bl/6J mice were fed a diet high in fat, fructose, and cholesterol for 34 weeks, and only biopsy-confirmed DIO-NASH mice with fibrosis were included. Resmetirom was administered at a daily dose of 3 mg·kg−1 p.o., for 8 weeks. Systemic and hepatic metabolic parameters, histological non-alcoholic fatty liver disease (NAFLD) activity and fibrosis scores, and liver RNA expression profiles were determined to assess the effect of THR-β activation.
Key Results: Treatment with resmetirom did not influence body weight but led to significant reduction in liver weight, hepatic steatosis, plasma alanine aminotransferase activity, liver and plasma cholesterol, and blood glucose. These metabolic effects translated into significant improvement in NAFLD activity score. Moreover, a lower content of α-smooth muscle actin and down-regulation of genes involved in fibrogenesis indicated a decrease in hepatic fibrosis.
Conclusion and Implications: Our model robustly reflected clinical observations of body weight-independent improvements in systemic and hepatic metabolism including anti-steatotic activity.
Probing the photointermediates of light-driven sodium ion pump KR2 by DNP-enhanced solid-state NMR
(2021)
KR2 is a light-driven sodium ion pump found in marine flavobacterium Krokinobacter Eikastus. The protein belongs to the microbial rhodopsin family, which is characterized by seven transmembrane helices and a retinal cofactor covalently bound to a conserved lysine residue through a Schiff base linkage. Specific features of KR2 and other sodium pumping rhodopsins are the NDQ motif, the N-terminal helix capping the protein at the extracellular side, and the sodium ion bound at the protomer interface in the pentameric structure. The ability to pump sodium ions was a surprising discovery since the positive charge at the Schiff base was long thought to hinder the transport of non-proton cations and the Grotthuss mechanism could not be applied to explain the Na+ transport. The photocycle of KR2 revealed by flashed photolysis and ultrafast femtosecond absorption spectroscopy consists of consecutive intermediates, named K, L, M, and O.
Here, DNP-enhanced ssNMR was used to analyze various aspects of these intermediate states. The K/L-state can be generated and trapped by in-situ illumination inside the magnet at 110 K. The trapping of L-state together with the K-state at this temperature is unexpected as this usually leads to the trapping of only K-state in bacteriorhodopsin (BR), proteorhodopsin (PR), and channelrhodopsin 2 (ChR2). This observation suggests a lower energy barrier between K- and L-state in KR2. For the O-state, the intermediate was generated by illuminating outside the magnet, followed by rapid freezing in liquid nitrogen and transfer to the magnet. Based on these procedures, the retinal conformation, and the electrostatic environment at the Schiff base in KR2 dark, K-, L- and O-intermediates were probed using 13C-labeled retinals bound to 15N-labeled KR2 by both 1D and 2D magic angle spinning (MAS) NMR experiments.
The obtained data show an all-trans retinal conformation with the distortion of 150° at H-C14-C15-H in the dark state whereas the retinal has a 13-cis, 15-anti conformation in the K- and L-state after light activation. Differences between K- and L-intermediates were observed. The retinal chemical shifts of the K-state show a large deviation from the model compound behavior between the middle and end part of the polyene chain. In the L-state, these differences are much less pronounced. These observations indicate that the light energy stored in the K-state dissipates into the protein in the subsequent photointermediate states. Furthermore, an additional shielding observed for C14 in L-state indicates the slight rotation toward a more compact 13-cis, 15-syn conformation. The distortion of the H-C14-C15-H angle in the L-state (136°) is larger than in the dark state. This twist of the retinal in the L-state would play an important role in lowering the pKa of the Schiff base, which is a prerequisite for the proton transfer from the Schiff base to the proton acceptor (D116). The electrostatic environments at the Schiff base in K- and L-states cause a de-shielding of the 15N nitrogen compared to the dark state. This indicates a stepwise stronger interaction with the counterion as the Schiff base proton moves away from the Schiff base and comes closer to the D116 in the transition from K- to L-state and approaches the proton transfer step during the M-state formation. In the O-state, the retinal was found to be in the all-trans conformation but differed to the dark state in the C13, C20, and Schiff base nitrogen chemical shifts. The largest effect (9 ppm) was observed for the Schiff base nitrogen, which could be explained by the effect of the positive charge of bound Na+ near the Schiff base in the O-state, coordinated by N112 and D116 as observed in the O-state crystal structure in the pentameric form.
The structural change at the opsin followed the retinal isomerization and the energy transfer from the chromophore to the surrounding were also investigated in this thesis using various amino acids labeling schemes. Moreover, 1H-13C hNOE in combination with CE-DNP was applied to probe the dynamics of retinylidene methyl groups and 23Na MAS NMR was employed to detect the bound sodium ion at the protomer interface in KR2 dark state.
Computational oral absorption models, in particular PBBM models, provide a powerful tool for researchers and pharmaceutical scientists in drug discovery and formulation development, as they mimic and can describe the physiologically processes relevant to the oral absorption. PBBM models provide in vivo context to in vitro data experiments and allow for a dynamic understanding of in vivo drug disposition that is not typically provided by data from standard in vitro assays. Investigations using these models permit informed decision-making, especially regarding to formulation strategies in drug development. PBBM models, but can also be used to investigate and provide insight into mechanisms responsible for complex phenomena such as food effect in drug absorption. Although there are obviously still some gaps regarding the in silico construction of the gastrointestinal environment, ongoing research in the area of oral drug absorption (e.g. the UNGAP, AGE-POP and InPharma projects) will increase knowledge and enable improvement of these models.
PBBM can nowadays provide an alternative approach to the development of in vitro–in vivo correlations. The case studies presented in this thesis demonstrate how PBBM can address a mechanistic understanding of the negative food effect and be used to set clinically relevant dissolution specification for zolpidem immediate release tablets. In both cases, we demonstrated the importance of integrating drug properties with physiological variables to mechanistically understand and observe the impact of these parameters on oral drug absorption.
Various complex physiological processes are initiated upon food consumption, which can enhance or reduce a drug’s dissolution, solubility, and permeability and thus lead to changes in drug absorption. With improvements in modeling and simulation software and design of in vitro studies, PBBM modeling of food effects may eventually serve as a surrogate for clinical food effect studies for new doses and formulations or drugs. Furthermore, the application of these models may be even more critical in case of compounds where execution of clinical studies in healthy volunteers would be difficult (e.g., oncology drugs).
In the fourth chapter we have demonstrated the establishment of the link between biopredictive in vitro dissolution testing (QC or biorelevant method) PBBM coupled with PD modeling opens the opportunity to set truly clinically relevant specifications for drug release. This approach can be extended to other drugs regardless of its classification according to the BCS.
With the increased adoption of PBBM, we expect that best practices in development and verification of these models will be established that can eventually inform a regulatory guidance. Therefore, the application of Physiologically Based Biopharmaceutical Modelling is an area with great potential to streamline late-stage drug development and impact on regulatory approval procedures.
Ginger (Zingiber officinale Roscoe) is widely used as medicinal plant. According to the Committee on Herbal Medicinal Products (HMPC), dried powdered ginger rhizome can be applied for the prevention of nausea and vomiting in motion sickness (well-established use). Beyond this, a plethora of pre-clinical studies demonstrated anti-cancer, anti-oxidative, or anti-inflammatory actions. 6-Shogaol is formed from 6-gingerol by dehydration and represents one of the main bioactive principles in dried ginger rhizomes. 6-Shogaol is characterized by a Michael acceptor moiety being reactive with nucleophiles. This review intends to compile important findings on the actions of 6-shogaol as an anti-inflammatory compound: in vivo, 6-shogaol inhibited leukocyte infiltration into inflamed tissue accompanied with reduction of edema swelling. In vitro and in vivo, 6-shogaol reduced inflammatory mediator systems such as COX-2 or iNOS, affected NFκB and MAPK signaling, and increased levels of cytoprotective HO-1. Interestingly, certain in vitro studies provided deeper mechanistic insights demonstrating the involvement of PPAR-γ, JNK/Nrf2, p38/HO-1, and NFκB in the anti-inflammatory actions of the compound. Although these studies provide promising evidence that 6-shogaol can be classified as an anti-inflammatory substance, the exact mechanism of action remains to be elucidated. Moreover, conclusive clinical data for anti-inflammatory actions of 6-shogaol are largely lacking.
The highly infectious disease COVID-19 caused by the Betacoronavirus SARS-CoV-2 poses a severe threat to humanity and demands the redirection of scientific efforts and criteria to organized research projects. The international COVID19-NMR consortium seeks to provide such new approaches by gathering scientific expertise worldwide. In particular, making available viral proteins and RNAs will pave the way to understanding the SARS-CoV-2 molecular components in detail. The research in COVID19-NMR and the resources provided through the consortium are fully disclosed to accelerate access and exploitation. NMR investigations of the viral molecular components are designated to provide the essential basis for further work, including macromolecular interaction studies and high-throughput drug screening. Here, we present the extensive catalog of a holistic SARS-CoV-2 protein preparation approach based on the consortium’s collective efforts. We provide protocols for the large-scale production of more than 80% of all SARS-CoV-2 proteins or essential parts of them. Several of the proteins were produced in more than one laboratory, demonstrating the high interoperability between NMR groups worldwide. For the majority of proteins, we can produce isotope-labeled samples of HSQC-grade. Together with several NMR chemical shift assignments made publicly available on covid19-nmr.com, we here provide highly valuable resources for the production of SARS-CoV-2 proteins in isotope-labeled form.