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Biophysical studies of the translation-regulating add adenine riboswitch from Vibrio vulnificus
(2017)
Bacterial gene expression can be regulated at mRNA level by cis-acting mRNA elements termed riboswitches. Riboswitches operate by conformational switching between a ligand-free and a ligand-bound state with different structures that either activate or inhibit gene expression. This PhD thesis contributes to the molecular level understanding of full-length purine riboswitches. It presents biophysical investigations on the ligand-dependent folding of the full-length translation-regulating add adenine riboswitch from the gram-negative human pathogenic marine bacterium Vibrio vulnificus (Asw). Asw has the typical bipartite riboswitch architecture with a 5’ ligand-sensing aptamer domain and a 3’ regulatory domain termed expression platform. According to the working hypothesis, Asw employs a unique thermodynamically-controlled 3-state conformational switching mechanism between an apoB, an apoA and a holo conformation to regulate translation initiation in a temperature-compensated manner. The two apo conformations are the putative translation-OFF states and the holo conformation is the putative translation-ON state of Asw. In the main project of this PhD thesis, an integrated nuclear magnetic resonance (NMR) and smFRET spectroscopic study of the full-length 112-nucleotide Asw (112Asw) was performed. The adenine-dependent folding of 112Asw was monitored at the level of base pairing interactions by NMR of the RNA imino protons, and at the level of three long-range intramolecular distances by smFRET of immobilized molecules. The integrated NMR and smFRET spectroscopic study of 112Asw yielded two major findings. First, NMR and smFRET both revealed that adenine binding to 112Asw impedes apoB formation by stabilizing the apoA secondary structure in the holo conformation without modulating tertiary structural interactions between the two riboswitch domains. This highlights the central role of competitive P1 and P4 helix formation at the interface of the aptamer and the expression platform for switching the accessibility of the ribosome binding site of 112Asw. Moreover, it strongly corroborates the hypothesis that purine riboswitches in general operate according to the key principle of a spatially decoupled secondary structural allosteric switch that proceeds without ligand-induced tertiary structural interactions between the aptamer domain and the expression platform. Second, it was uncovered by smFRET that the apoA and the holo conformation of 112Asw do not adopt a single folding state at near-physiological Mg2+ concentration. Instead, apoA and holo exhibit a persistent dynamic equilibrium between substates with an undocked (U), a short-lived docked (D1; ~s) and a Mg2+-bound long-lived docked (D2; ~10 s) aptamer kissing loop motif. In the holo conformation, the fractional population of the long-lived docked substate is ~2-fold increased compared to the apoA conformation, but undocked and docked substates are still comparably stable. The here described multiple folding states of the apoA and the holo conformation might have regulatory properties that are in between the apoB translation-OFF state and the holo-D2 translation-ON state. Additonally, an integrated NMR and smFRET analysis of 127-nucleotide Asw (127Asw) is presented. Compared to 112Asw, 127Asw is 3’-elongated by 15 nucleotides of the adenosine deaminase encoding sequence of the add gene from Vibrio vulnificus. 127Asw was chosen as mRNA template for future investigations of the interaction between Asw and the 30S ribosomal subunit. The NMR spectra of 127Asw demonstrated that 127Asw has the same overall secondary structure as 112Asw. Like for 112Asw, the combined NMR and smFRET analysis of 127Asw showed that adenine binding impedes apoB formation and stabilizes a long-lived docked aptamer kissing loop fold. However, compared to 112Asw, 127Asw has a destabilized aptamer kissing loop motif and a stabilized P4 helix in the expression platform. Finally, ligand-observed studies of the transient encounter complex between Asw and the near-cognate ligand hypoxanthine are described. By competition binding WaterLOGSY NMR experiments with hypoxanthine and the adenine analogue 2,6-diaminopurine, it could be shown that hypoxanthine binds to the same binding site of 112Asw as the cognate ligand adenine. The hypoxanthine binding constant measured with the WaterLOGSY method is in the low mM range (1.8 mM) and substantially exceeds the physiological hypoxanthine concentration in E. coli (~0.3 mM), thus ruling out that hypoxanthine binding can significantly impact the translational regulation of Asw in vivo. Also, preliminary FTIR difference spectra of 13C,15N-labelled and unlabelled hypoxanthine in complex with the pbuE adenine riboswitch aptamer and the xpt guanine riboswitch aptamer are discussed. These spectra showed a pattern of multiple IR bands that appeared to be characteristic for the respective complex.
In der organischen Elektronik werden Moleküle mit konjugierten pi-Elektronensystemen als Halbleiter und Lichtemitter eingesetzt. Für die Fabrikation fortschrittlicher elektronischer Bauelemente, wie z. B.organischer Leuchtdioden, werden Materialien mit besonderen optoelektronischen Eigenschaften benötigt.Die Stoffklasse der Arylamine ist für den Transport positiver Ladungen etabliert, da die exozyklischen Stickstoffatome Elektronenlöcher mesomer zu stabilisieren vermögen. Komplementär dazu sind auch Materialien für den Transport negativer Ladungen in der organischen Elektronik unverzichtbar. Zu diesem Zweck sollten borhaltige Verbindungen ideal geeignet sein, da das Element Bor weniger Valenzelektronen als Kohlenstoff besitzt und Arylborane daher im Vergleich zu den entsprechenden Kohlenwasserstoffen eine geringere Elektronendichte aufweisen. Als Halbleitermaterialien sind Arylborane jedoch nicht so weit verbreitet wie Arylamine, da die Instabilität vieler Vertreter gegenüber Luft und Feuchtigkeit sowie der Mangel an effizienten Synthesemethoden ihre Anwendung verzögert haben. Um geeignete organische Elektronenleiter bereitzustellen, ist die Entwicklung stabiler, pi-konjugierter Borane erstrebenswert. Ansatzpunkte für diese Arbeit waren Erkenntnisse aus der vorangegangenen Masterarbeit, sowie Beispiele für hydrolysestabile Arylborane, welche in der jüngeren Vergangenheit von M. Wagner et al. Und S. Yamaguchi et al. veröffentlicht wurden. Im Rahmen der vorliegenden Arbeit gelang die Entwicklung einer modularen Synthesestrategie, die einen vielseitigen Zugang zur Stoffklasse der borhaltigen polyzyklischen aromatischen Kohlenwasserstoffe (PAKs) ermöglicht: Ausgehend von einem gut verfügbaren siliziumhaltigen Startmaterial und diversen, zum Großteil kommerziell erhältlichen, Carbonylverbindungen wurden mehr als zwanzig verschiedene Triarylborane dargestellt. Dabei wurde eine Auswahl spezieller Reaktionstypen nach den jeweiligen Erfordernissen in geeigneter Weise miteinander kombiniert. Zu diesen gehörte die Peterson-Olefinierung zum Aufbau drei- und vierfach substituierter Alkene, die Photozyklisierung der resultierenden Stilben-artigen Verbindungen, eine Ru(II)-katalysierte Reaktion zur Benzanellierung und der Silizium/Bor Austausch mittels BBr3. An wichtigen Zwischenprodukten wurden Reaktivitätsstudien durchgeführt, um die Anwendungsmöglichkeiten und Einschränkungen dieser Synthesestrategie zu ergründen. Um die Stabilität der Produkte gegenüber Luft und Feuchtigkeit zu gewährleisten, wurden die reaktiven Borzentren in bewährter Weise durch Einführung eines sterisch anspruchsvollen Mesitylsubstituenten kinetisch abgeschirmt. Die überwiegende Zahl der synthetisierten borhaltigen PAKs erwies sich als absolut unempfindlich gegenüber Wasser und konnte mit den gängigen Methoden der organischen Chemie (z. B. Säulenchromatographie an Kieselgel) gereinigt werden. Als Alternative zur sterischen Abschirmung wurde der Einbau des Boratoms in ein starres Molekülgerüst an einem Ausführungsbeispiel verwirklicht. Diese zweite Möglichkeit der Stabilisierung stellte sich in Bezug auf die Eigenschaften des Produkts als vergleichbar heraus, erforderte aber einen größeren synthetischen Aufwand und lieferte eine geringere Ausbeute über die gesamte Reaktionssequenz. Die in dieser Arbeit dargestellten borhaltigen PAKs wurden mittels Röntgenkristallographie umfassend strukturell charakterisiert. Die intensiv genutzten Methoden Cyclovoltammetrie, UV/vis- und Fluoreszenzspektroskopie gewährten zusätzlich einen detaillierten Einblick in ihre elektronischen Strukturen. Die Synthese und systematische Variation der Moleküle führten zu neuen Erkenntnissen über grundlegende Struktur-Eigenschafts-Beziehungen. Insbesondere zeigten diese Vergleiche, dass in ladungsneutralen Triarylboranen keine Delokalisation der pi-Elektronen über das leere p-Orbital eines Boratoms stattfindet. Von entscheidender Bedeutung für die elektronische Struktur borhaltiger PAKs ist das Gerüst aus sp2-hybridisierten Kohlenstoffatomen: Wenn mindestens zwei der Arylsubstituenten am Boratom zu einem gemeinsamen Gefüge verbrückt sind, zeigen diese Verbindungen elektronische Übergänge im sichtbaren Bereich des elektromagnetischen Spektrums und in den meisten Fällen auch eine intensive Fluoreszenz. Des Weiteren besitzen diese borhaltigen PAKs eine hohe Elektronenaffinität und lassen sich elektrochemisch reversibel reduzieren. Damit erfüllen sie bedeutende Kriterien für eine mögliche Anwendung als Elektronenleiter. Von den Molekülen mit ausgedehntem pi-Elektronensystem ließen sich manche zusätzlich reversibel oxidieren und zeichnen sich daher durch eine außergewöhnlich hohe elektrochemische Stabilität aus. An Arylboranen, deren Farbe sich durch externe Stimuli verändern lässt, wurden grundlegende Untersuchungen im Kontext der molekularen Sensorik durchgeführt. Einige der synthetisierten Verbindungen ändern ihr Absorptions- und Emissionsspektrum bei Kontakt mit Fluorid-Ionen, bei Oxidation integrierter Schwefelatome durch ein Carbonsäureperoxid, bei elektrochemischer Reduktion oder in Abhängigkeit der Polarität ihrer Umgebung. Die Ergebnisse dieser Arbeit wurden in vier Fachartikeln beschrieben und veröffentlicht (siehe Anhang). Sie können zu einem besseren Verständnis der elektronischen Eigenschaften borhaltiger PAKs beitragen und die Entwicklung neuer Halbleitermaterialien auf der Basis dieser Stoffklasse erleichtern.
Fettsäuresynthasen vom Typ I (FAS I), hier bezeichnet als Fettsäuremegasynthasen,sind Multienzymkomplexe, in denen sämtliche funktionellen Domänen für die de-novo-Synthese von Fettsäuren einen strukturellen Verbund eingehen. Auch das für den Transport von Edukten und Intermediaten nötige Acyl Carrier Protein (ACP) ist kovalent gebundener Teil dieses Komplexes, der so zu einer hocheffizienten molekularen Maschine zur Massenproduktion dieser grundlegend essentiellen Zellbausteine wird. Die FAS I aus Pilzen (fFAS), als Gegenstand dieser Arbeit, mit einer Masse von bis zu 2,7 MDa ist heute in ihrer Struktur durch Röntgenkristallographische sowie elektronenmikroskopische Methoden gut charakterisiert. 48 funktionelle Domänen sind zu einem geschlossenen Reaktionskörper angeordnet, indem sie in einer strukturgebenden Matrix aus Expansionen und Insertionen bzgl. der enzymatischen Kerndomänen eingebettet sind, die 50% des gesamten Proteins ausmacht. Neben den zahlreichen strukturellen Informationen über fFAS ist jedoch noch wenig über ihre Assemblierung verstanden. Dabei ist sie nicht nur als ein Beispiel für das generelle Verständnis von Assemblierungsmechanismen von Multienzymkomplexen interessant, sondern wird hier auch als Ziel eines inhibitorischen Eingriffs betrachtet, um eine neue antimykotische Wirkstrategie abseits des Ausschaltens aktiver Zentren zu evaluieren. Nur wenn die Mechanismen und Wechselwirkungen im Assemblierungsprozess offen gelegt sind, lassen sie sich später gezielt attackieren. Essentielle Sekundärstrukturmotive müssen identifiziert und bewertet werden, um sie einer weiteren Evaluation als Drug-Target-Kandidaten zugänglich zu machen. In dieser Arbeit werden Resultate aus in-vivo-Experimenten an rational mutierten fFAS-Konstrukten unter Zuhilfenahme einer evolutionären Betrachtung der fFAS gemeinsam mit Erkenntnissen aus andernorts geleisteten in-vitro-Experimenten an fFAS-Fragmenten zu einem geordneten Assemblierungsweg der fFAS zusammengeführt. Dabei werden Evidenzen aus den Kausaltäten zentraler Anforderungen an einen Assemblierungsmechanismus der fFAS zu drei konsequenten Schlüsselschritten verdichtet, die (i) eine frühe Interaktion zweier komplementärer Polypeptidketten zu einer Pseudo-Einzelkette, (ii) eine posttranslationale Modifikation von ACP und (iii) die geordnete Reifung zum fertigen Komplex durch Selbstassemblierung der beteiligten Domänen umfassen. Durch rationale Mutationen an den Schnittstellenmotiven für die Pseudo-Einzelkettenbildung, werden diese als Schwachstelle der Assemblierung unterschiedlicher fFAS-Typen charakterisiert, wobei für S. cerevisiae nicht weniger als zwei gezielte Punktmutationen ausreichen, um die Assemblierung des gesamten Komplexes zu verhindern. Darüber hinaus zeigen Experimente mit fFAS-Konstrukten, deren Schnittstellenmotive einer intramolekular kompetitiven Wechselwirkung ausgesetzt sind, prinzipiell die Möglichkeit zur Inhibierung der fFAS-Assemblierung durch Störung der Pseudo-Einzelkettenbildung.
Membrane proteins are biological macromolecules that are located in a cell’s membrane and are responsible for essential functions within an organism, which makes them to prominent drug targets. The extraction of membrane proteins from the hydrophobic membrane bilayer to determine high-resolution crystal structures is a difficult task and only 2% of all solved proteins structures are membrane proteins. Computational methods may help to gain deeper insights into membrane protein structures and their functions. This study will give an overview of such computational methods on a representative set of membrane proteins and will provide ideas for future computational and experimental research on membrane proteins.
In a first step (chapter 2), I updated an earlier, manually-curated data set of homologous membrane proteins (HOMEP) to more recent versions in 2010 (HOMEP2) and 2013 (HOMEP3) using an automated clustering approach. High-resolution structures of membrane proteins listed in the PDB_TM database were structurally aligned and subsequently clustered using structural similarity scores. Both data sets were used as a standard gold reference set for subsequent work.
Subsequently, I have updated and applied the sequence alignment program AlignMe to determine protein descriptors that are suitable for detecting evolutionary relationship between homologous a-helical membrane proteins. Single input descriptors were tested alone and in combination with each other in different modes of AlignMe by optimizing gap penalties on the HOMEP2 data set. Most accurate alignments and homology models on the HOMEP2 data set were observed when using position-specific substitution information (P), secondary structure propensities (S) and transmembrane propensities (T) in the AlignMe PST mode. An evaluation on an independent reference set of membrane protein sequence alignments from the BAliBASE collection showed that different modes of AlignMe are suitable for different sequence similarity levels. The AlignMe PST mode improved the alignment accuracy significantly for distantly related proteins, whereas for closely-related proteins from the BAliBASE set the AlignMe PS mode was more suitable. This work was published in March 2013 in PLOS ONE. In order to allow also an easier usage of the AlignMe program, I have implemented a web server of AlignMe (chapter 4) that provides the optimized settings and gap penalties for the AlignMe P, PS and PST modes. A comparison to other recent alignment web server shows that the alignments of AlignMe are similar or even more accurate than those of other methods, especially for very distantly related proteins for which the inclusion of membrane protein information has been shown to be suitable. This work was published in the NAR web server issue in July 2014.
Although membrane-specific information has been shown to be suitable for aligning distantly related membrane proteins on a sequence level, such information was not incorporated into structural alignment programs making it unclear which method is the most suitable for aligning membrane proteins. Thus, I compared 13 widely-used pairwise structural alignment methods on an updated reference set of homologous membrane protein structures (HOMEP3) and evaluated their accuracy by building models based on the underlying sequence alignments and used scoring functions (e.g., AL4 or CAD-score) to rate the model accuracy (chapter 5). The analysis showed that fragment-based approaches such as FR-TM-align are the most useful for aligning structures of membrane proteins that have undergone large conformational changes whereas rigid approaches were more suitable for proteins that were solved in the same or a similar state. However, no method showed a significant higher accuracy than any other. Additionally, all methods lack a measure to rate the reliability of the accuracy for a specific position within a structure alignment. In order to solve these problems, I propose a consensus-type approach that combines alignments from four different methods, namely FR-TM-align, DaliLite, MATT and FATCAT and assigns a confidence value to each position of the alignment that describes the agreement between the methods. This work has been published 2015 in the journal “PROTEINS: structure, function and bioinformatics”.
Consensus alignments were then generated for each pair of proteins of the HOMEP3 data set and subsequently analyzed for single evolutionary events within membrane spanning segments and for irregular structures (e.g., 310- and p-helices) (chapter 6). Interestingly, single insertions and deletions could be observed with the help of consensus alignments in the conserved membrane-spanning segments of membrane proteins in four protein families. The detection of such single InDels might help to identify crucial residues for a proteins function.
If the biotechnological production of chemicals can further replace or support regular synthetic chemistry, industry will be able to move away from fossil oils towards renewable sources. However, in many cases the much needed adaptation of biotechnological production systems is not yet developed to the necessary level.
For processes where short fatty acids (FA) are needed, as for example in the microbial production of biofuels in the gasoline range, protein engineering had not yet delivered feasible solutions. In this thesis, several approaches to introduce chain length control on type I fatty acid synthases (FAS) were established and made available in a publication and two patents. Therein, engineering was focused on rational design based on available structural information.
First, the type I FAS from C. ammoniagenes was used as a model enzyme to probe modifications on FAS in a low complex in vitro environment in order to gain information about structure-function relationships. At this stage, engineering was conducted in several rounds, first addressing possible ways to alter product distributions by changing substrate affinities through concise mutations in binding channels. Several FAS constructs were generated ranging from first successes, where short FA were produced as side products, to FAS where native chain length programming was overwritten and only short FA were produced.
Furthermore, another engineering target was addressed with the modification of domain-domain interactions on FAS. For its exploitation to direct synthesis, contact surfaces on catalytic domains were changed to interfere with acyl carrier protein binding. This channeling of the kinetic process on the enzyme led to similar successes and short FA became the primary product.
The two approaches have proven to be potent tools to introduce systems of chain length control in FAS. This rational engineering has the big advantage that it is mostly minimally invasive and due to the high conservation of de novo FA synthesis, individual mutations could easily be used in other FAS (and their organisms) as well. Even heterologous expression of modified FAS genes is feasible.
Engineering was not only tested in a defined in vitro environment and but also in S. cerevisiae as an exemplary in vivo system. The results eventually confirmed the in vitro findings and proved that the chosen engineering could be transferred to more complex systems. Even before any optimization for highest output, the titers of short FA from S. cerevisiae fermentation matched previous reports with 118 mg/L.
In sum, this work covers several layers from basic research to preliminary applications. The presented modifications to create short FA producing FAS can be a key step in synthesis pathways and will likely enable a whole range of new succeeding research. It can be seen as a valuable contribution towards establishing novel ways for the production of chemicals from renewable sources.
Identifizierung des vertebraten-spezifischen Proteins C7orf43 als neue TRAPPII Komplexuntereinheit
(2016)
Bei den transport protein particle (TRAPP) Komplexen handelt es sich um eine Familie von Protein Komplexen, die jeweils aus mehreren Untereinheiten bestehen. In der vorliegenden Arbeit konnte das Protein C7orf43 als neue potenzielle TRAPPII Untereinheit identifiziert werden, die - wie auch die beiden anderen TRAPPII-spezifischen Komponenten TRAPPC9 und TRAPPC10 - sowohl für die Erhaltung von ERGIC, Golgi-Apparat und COPI Vesikel als für den ER zu Golgi Transportweg benötigt wird.
Weltweit sind ca. 130–180 Millionen Menschen mit HCV infiziert und jährlich sterben etwa 500.000 Menschen an dessen Folgen. Die neuartigen Therapien versprechen zwar eine sehr hohe Heilungsrate, sind aber aufgrund ihrer enorm hohen Kosten nur in Industrieländern verfügbar. Noch immer gibt es keine prophylaktische Vakzinierung gegen HCV. Deshalb ist es wichtig, den HCV-Lebenszyklus und die Interaktion zwischen Wirtszelle und Virus detailliert zu verstehen, um die Entwicklung von Therapien und Impfungen zu ermöglichen. Außerdem kann ein fundiertes Wissen von HCV translatiert werden und auf neuartige Erreger der Familie der Flaviviridae, wie Denguevirus und Zikavirus, angewendet werden. Während der Zelleintritt und die Replikation von HCV relativ gut charakterisiert sind, bleiben die Assemblierung und Freisetzung der viralen Partikel schlecht verstandene Schritte des HCV-Lebenszyklus. In dieser Arbeit sollte die Rolle des zellulären Proteins α-Taxilin im Lebenszyklus von HCV untersucht werden. In einer späteren Phase der Arbeit wurde der endosomale Freisetzungsweg von HCV untersucht. Dazu wurden HCV Varianten generiert und charakterisiert, die Fluoreszenz-Proteine im NS5A- und E1-Protein enthalten, durch die es möglich ist, den Replikationskomplex und die Viruspartikel zu visualisieren und zu quantifizieren und den viralen Lebenszyklus dadurch besser untersuchen zu können...
FUSE Binding Protein 1 (FUBP1) is a transcriptional regulator, which is overexpressed in various cancer entities, including hepatocellular carcinoma (HCC) and colorectal cancer (CRC). It fulfills pro-proliferative and anti-apoptotic functions in cancer cells, resulting in increased proliferation and reduced sensitivity towards apoptotic stimuli.
Previously, camptothecin (CPT) and its clinically used analog 7-ethyl 10hydroxycamptothecin (SN-38) were shown to inhibit FUBP1 in biophysical interaction displacement assays (AlphaScreen; surface plasmon resonance, SPR), and first insights into the cellular effects of FUBP1 inhibition were obtained. CPT and SN-38 are known to potently inhibit topoisomerase 1 (TOP 1), and until today, these inhibitors were thought to be specific for this target. This could be disproved by our FUBP1 binding studies. An open issue, which is addressed in this thesis, was the contribution of FUBP1 inhibition to SN-38-mediated apoptosis apoptosis.
During this thesis, a low micromolar efficacy of CPT/SN-38-induced inhibition of FUBP1 binding to the Far Upstream Sequence Element (FUSE) oligonucleotide of p21 was determined. Furthermore, FUBP1 was for the first time shown to directly interact with a potential FUSE sequence upstream of the transcription start in pro-apoptotic gene BIK. In proof of-principle experiments, an effective inhibition of the binding of FUBP1 to the FUSE BIK DNA by CPT/SN-38 was verified.
One of the main goals of this thesis was to further elucidate the contribution of cellular FUBP1-inhibition by CPT/SN-38 to the anti-cancer potential of these substances. For this purpose, the TOP 1 mutant and TOP 1 wild type colorectal cancer sub-cell lines HCT116 G7 and HCT116 S were used. CPT/SN-38 was shown to induce apoptosis in single and combinatorial treatments with mitomycin c (MMC), independently of the TOP 1 mutation status of the cells. Furthermore, a prominent induction of a FUBP1 target gene signature was observed upon treatment of both cell lines with CPT/SN-38. Consequently, CPT/SN-38 was able to fulfill its anticancer effects in these cells, although TOP 1 could not be the main target in the mutant cell line.
In a second approach to gain indirect evidence for FUBP1 dependent effects of CPT/SN-38, the TOP 1-specific inhibitors topotecan (TTN) and β lapachone (BL) were used for the treatment of HCC and CRC cell lines. Interestingly, the TOP 1 inhibitors TTN and BL exhibited a reduced potency in apoptosis induction compared to the dual (FUBP1 and TOP 1) inhibitor SN-38.
Finally, two independent screens for a specific FUBP1 inhibitor were performed. In the first approach, a small number of structural and functional CPT-derivatives that exhibited a reduced inhibitory potential against TOP 1, were tested for their ability to interfere with the FUBP1/FUSE binding. Two particular indenoisoquinoline derivatives revealed potent in vitro inhibition of FUBP1 with low micromolar IC50 values.
In a second approach, previously identified candidate FUBP1 inhibitors that had been isolated from the Maybridge Hit Finder library served as lead structures for a structure activity relationship (SAR) study of the inhibition of FUBP1 binding to the FUSE oligonucleotide. After two cycles of optimization, a medium-potent FUBP1 inhibitor was obtained that induced effective deregulation of FUBP1 target genes in cell culture experiments.
Protein synthesis is a central process within every living cell, where information embodied in the nucleotide sequence of the mRNA is translated into the primary sequence of proteins. The translation procedure comprises four steps: initiation, elongation, termination, and recycling. Ribosome recycling orchestrated by the ATP‐binding cassette (ABC) protein ABCE1, renders mRNA translation into a cyclic process, connecting termination with re initiation. In Archaea and Eukarya, the ABC protein ABCE1 catalyzes ribosome recycling by splitting the ribosome (80S/70S) into the small 40S/30S and large 60S/50S subunits, providing them for the next translation round.
The ABC‐type ATPase one of the most conserved proteins, present in all Archaea and Eukarya, but not in Bacteria, is essential for life in all organisms examined so far. ABCE1 was initially identified as RNase L inhibitor (Rli1), involved in the antiviral RNA immunity, and as host protein 68 (HP68) playing a role in HIV capsid assembly. However, the strong sequence conservation of ABCE1 points towards a more fundamental function within cell homeostasis, which was found by its involvement in various translation processes. ABCE1 turned out to be the major ribosome recycling factor indispensable for life in Eukarya and Archaea, being involved in canonical translation, mRNA surveillance, ribosome biogenesis, and translation initiation.
Recent functional and structural data provided first insights into the mechanism of ABCE1 in ribosome recycling. The nucleotide‐binding domains (NBDs) sandwich two ATP molecules in the NBD1‐NBD2 interface causing an NBD engagement, which is released upon ATP hydrolysis. In case of ABCE1, this ATP‐dependent tweezer‐like motion of the NBDs transfers mechanical energy to the ribosome and tears the subunits apart. The FeS‐cluster domain may swing out of the NBD cleft into the inter‐subunit space of the ribosome, which drives the subunits apart either directly or via the bound a/eRF1. Hence, the subunits are released and the post‐splitting complex (PSC, 40S/30S∙ABCE1∙ATP) is available for re‐initiation events, presumably occurring via the known interactions of ABCE1with initiation factors.
One of the most crucial aspects of this model is the nucleotide‐dependent conformational switch of ABCE1, which drives ribosomal subunit splitting. However, the conformational states, which ABCE1 undergoes during ribosome recycling, including their mechanistic importance for its diverse functions, remain unknown. Further, the exact role and movement of the essential FeScluster domain during ribosome recycling are not yet understood. Additional, it remains elusive where ABCE1 is bound in the post‐splitting complex and how the splitting mechanism is regulated concerning the asymmetric NBDs and the coupling of nucleotide binding with NBD closing and ATP hydrolysis.
Thus, in order to monitor the conformational dynamics of the ribosome recycling factor ABCE1 two complementing methods in structural biology, namely single‐molecule based Förster resonance energy transfer (smFRET) and pulsed electron‐electron double resonance (PELDOR) spectroscopy were applied.
Single‐molecule FRET as an integrated biophysical approach based on Förster resonance energy transfer and single‐molecule detection was used to understand the fundamental molecular principles of ABCE1. Contrary to the anticipated two‐state model of ABC proteins, it was shown in this thesis that both nucleotide‐binding sites of ABCE1 are always in a dynamic equilibrium between conformational states with distinct properties: open, intermediate, and closed. The equilibrium in the two nucleotide‐binding sites is distinctly affected when ABCE1 interacts with ribosomal subunits and nucleotides. While ABCE1 can adopt all three conformational states in its free or 30S bound situation, the closed state has the highest affinity for 30S subunit. Further, dissociation of ABCE1 from the small ribosomal subunit, a step that completes the recycling process, is followed by the opening of the NBSs. Hence, the current findings have important implications not only for ribosome recycling but represent a new paradigm for the molecular mechanisms of twin‐ATPases.
The complementing PELDOR measurements provide the advantage of high distance precision and reliability studying macromolecular complexes. Distance distributions of a number of ABCE1 variants even bound to the 1‐MDa post‐splitting complex (30S∙ABCE1∙AMP‐PNP), composed of the 16S rRNA, 28 ribosomal proteins, and ABCE1, was analyzed. Thus, the available crystal structures of ABCE1 in the open state were validated, since all distances of ABCE1 measured in this study perfectly correspond to this crystallized state. Unfortunately, ABCE1 could not be trapped in the closed state under the experimental conditions applied, although plenty different approaches to stabilize this state were performed.
In the second part of this study the architecture yet unknown of the 1‐MDa post splitting complex (40S/30S∙ABCE1∙ATP), concerning especially the ABCE1 binding site and its interactions with translational proteins, was probed by a method, which combines chemical cross linking with mass‐spectrometry (XL‐MS). Following this approach, it was demonstrated that ABCE1 remains bound at the translational GTPase‐binding site after ribosome splitting, contacting the S24e protein of the small subunit. The platform for the intensive contacts to the small ribosomal subunit is thereby provided by the unique helix‐loop‐helix motif of ABCE1. Notably, the FeScluster domain of ABCE1 undergoes a large rotational and translational rearrangement towards the small ribosomal subunit S12 upon nucleotide‐dependent closure of the NBDs. Thus, a key complex in the translational cycle, resembling the link between translation initiation and ribosome recycling processes, was reconstituted and structurally analyzed.
In view of the diverse functionalities of RNA, the search for tools suitable for regulating and understanding RNA grows continuously. Dysfunction of RNA controlled processes can lead to diseases, calling for external regulation mechanisms – a difficult task in view of the complexity of biological systems. One of the recently developed methods that aim to systematically control RNA relates to photoregulation. Here, the RNA functions are triggered by photochromic molecules – for example, azobenzene or spiropyran – which are bound either covalently or non-covalently to the target RNA. This is a flexible approach, which can be improved by using suitably substituted chromophores. However, many issues regarding the details of photocontrol are still open. A detailed understanding of the mechanism of photocontrol is therefore of crucial importance.
The present thesis explores theoretical approaches to the photocontrol of RNA, focussing upon azobenzene chromophores covalently bound to RNA. The aim of the thesis is to characterize, at a molecular level, the effect of trans-to-cis isomerization of the azobenzene chromophore on RNA, and thus understand the mechanism of RNA unfolding triggered by azobenzene isomerization. In particular, we attempt to answer the following questions:
How does azobenzene isomerization happen in an RNA environment, i.e., how is
the isomerization influenced by the local RNA environment?
Conversely, how is RNA dynamics, on a longer time scale, affected by azobenzene attachment and photoisomerization?
Further, can regulation be enhanced by substituted azobenzenes? And, does simulation yield a picture that is consistent with experiment?
Due to the very different times scales of azobenzene isomerization (femtoseconds to picoseconds) and the much slower RNA response (nanoseconds to milliseconds), complementary techniques have been chosen: (i) hybrid quantum-classical approaches, i.e., on-the-fly Quantum Mechanics/Molecular Mechanics (QM/MM), to characterize the isomerization and RNA response on an ultrafast time scale, and (ii) molecular dynamics with enhanced sampling techniques, in particular, Replica Exchange MD (REMD), to explore longer time scales where the effect of RNA unfolding becomes manifest. Furthermore, substituent effects on azobenzene were separately investigated, in collaboration with two experimental groups.
The first part of this thesis is focused on the conformational influence of azobenzene on a small RNA hairpin on longer time scales using REMD simulations. In accordance with experiment, it is found that both the trans and cis form of azobenzene destabilize the RNA system. Trans azobenzene stays stacked in the double strand, whereas the cis form flips out of the RNA. These stacking interactions are the main reason why a trans azobenzene-RNA-complex is more stable than a cis-azobenzene-RNA-complex. Furthermore, the loop region of the RNA hairpin is highly destabilized by the intercalation of azobenzene.
In the second part, on-the-fly QM/MM simulations of the same azobenzene substituted hairpin are undertaken. These simulations use a surface hopping (SH) algorithm in conjunction with hybrid QM/MM electronic structure calculations to give a complete picture of the isomerization process on a picosecond time scale. It is shown that, due to the constraints of the RNA environment, the isomerization time of the azobenzene chromophore is significantly increased (from 300 femtoseconds in the gas phase to around 20 picoseconds in the RNA environment), and the isomerization yield is low. To the best of our knowledge, these are the first QM/MM simulations reported for azobenzene in a nucleic acid environment.
In the third and final part of this thesis, the properties of substituted azobenzenes have been explored, in collaboration with two experimental groups at the department. In particular, para- and meta-hydroxy substituted azobenzenes were suggested as improved photoswitches for the photoregulation of RNA, but spectroscopic investigations showed that isomerization was inefficient in some of the investigated species. Therefore, we investigated the photoisomerisation pathway of the keto/enol-form of para- and meta-hydroxy-azobenzenes by Time-Dependent Density Functional Theory (TDDFT) calculations. These calculations show that the competing keto/enol-tautomerism can result in an unstable cis form, making these substituted chromophores unsuitable as photoswitches.
Overall, the present thesis has contributed to obtaining a molecular-level understanding of photocontrol in azobenzene substituted RNAs, showing that theory and simulations can provide useful guidance for new experiments.
The transporter associated with antigen processing (TAP) is a heterodimeric ATP-binding cassette (ABC) transport complex, which selects peptides for export into the endoplasmic reticulum (ER) and subsequent loading onto major histocompatibility complex class I (MHC I) molecules to trigger adaptive immune responses against virally or malignantly transformed cells. Due to its pivotal role in adaptive immunity, TAP is a target for infectious diseases and malignant disorders, such as bare lymphocyte syndrome type I and cancer. A detailed knowledge about the TAP structure and transport mechanism is fundamental for the development of therapies or drugs against such diseases, but numerous aspects are insufficiently determined to date. The aim of this PhD thesis was to elucidate several structural details of TAP using powerful biochemical and biophysical methods and thereby to contribute to the understanding of the translocation machinery functionality.
High protein yields, an efficient isolation from the lipid environment and subsequent purification of a stoichiometric, stable, and functional TAP complex are prerequisites to get detailed insights into TAP functionality. The natural product digitonin is typically used as detergent to isolate TAP, but suffered from fluctuating purity and high costs. The novel detergent GDN was selected from a number of potential detergents upon their ability to isolate and purify TAP overcoming the limitations of digitonin without compromising on functional integrity. State-of-the-art biophysical techniques, such as solid-state nuclear magnetic resonance (NMR), require highly concentrated protein samples. A new and mild procedure to concentrate TAP was established within this thesis. Freeze drying is superior to conventional concentration techniques, such as ultrafiltration, resulting in TAP inactivation and aggregation already at concentrations of 10 mg/mL. This new procedure enables stabilizing TAP in a condensed glycerol matrix and to concentrate the transport complex up to 30 mg/mL active transporter. The functional integrity of the freeze-dried TAP complex was verified by determining equilibrium dissociation constants, peptide dissociation and ATP-hydrolysis rates as well as long-term stabilities identical to untreated TAP. The combined application of the detergent GDN and the freeze drying procedure facilitates the cost-efficient isolation of functional and highly concentrated TAP and enables to study the structure and mechanism of the peptide transporter TAP using modern analyses methods.
Information on peptide-TAP interactions at atomic level have not been obtained so far. This lack of knowledge hampered the mechanistic understanding of the initial steps of substrate translocation catalyzed by TAP. Dynamic nuclear polarization (DNP) enhanced magic angle spinning (MAS) solid-state NMR on highly concentrated TAP samples prepared with the freeze-drying procedure was used within this thesis to study this challenging membrane protein-substrate complex. The affinity and specificity of peptide binding by TAP are mediated by multiple recognition sites in the N- and C-terminal regions. Side-chains of positions 1, 3, and 9 are most substantially affected upon binding to TAP, revealing recognition principles of the translocation machinery. The nonamer peptide binds to TAP in an extended conformation with an N-to-C terminus distance of ~2.5 nm. Molecular docking revealed that the peptide substrate is locked with its N and C termini between TAP1 and TAP2 and adopts a tilted pose with respect to the membrane plane. The identified contact sites of TAP are consistent with results from earlier crosslinking and mutational analyses on the TAP complex.
The inadequate structure determination and insufficient knowledge about the dynamics of substrate translocation impedes a detailed comprehension of the TAP transport mechanism. Advanced biophysical methods, such as pulsed electron paramagnetic resonance (EPR) or single-molecule Förster resonance energy transfer (FRET), enable to locate the peptide-binding pocket and to elucidate dwell-times, conformational states and dynamics within the translocation cycle of TAP. The specific introduction of spin or fluorescent labels via single cysteines for such studies requires a cysteine-less TAP complex. The endogenous cysteine 213 in TAP2 remained to create a pseudo Cys-less TAP complex within this thesis due to its altered substrate repertoire when mutated to serine as shown in previous studies. Latter complex was used to introduce single-Cys mutations in the cytosolic extensions of transmembrane helices of TAP1. Their functional integrity with respect to peptide binding and translocation was comparable to pseudo Cys-less TAP. All pseudo single cysteines were efficiently labeled, but unintentionally C213TAP2 was labeled as well and TAP concomitantly inactivated. These unsatisfactory initial experiments required the generation of a functional, entirely Cys-less TAP transporter within this thesis. Therefore, C213TAP2 was replaced by all 19 proteinogenic amino acids. All analyzed mutants were capable to bind a high-affinity peptide of TAP, but with varying affinities and binding capacities. The replacement of C213 by isoleucine enabled the generation of a cysteine-less TAP complex with functional characteristics similar to the wild-type transporter and will promote the elucidation of the translocation mechanism of the peptide transporter TAP in future studies using pulsed EPR and single-molecule FRET.
The centerpiece of all neuronal processes is the synaptic transmission. It consists of a complex series of events. Two key elements are the binding of synaptic vesicles (SV) to the presynaptic membrane and the subsequent fusion of the two membranes. SV are neurotransmitter-filled membranous spheres with many integral and peripheral proteins. The synaptic SNARE complex consists of three interacting proteins, which energize and regulate the fusion of the SV membrane with the presynaptic membrane. Both processes are closely orchestrated to ensure a specific release of neurotransmitter. Already many experiments have been performed, such as genetic screens and proteome analysis of SV, to determine the functions of the various proteins involved. Nevertheless, the functions of the identified proteins are still not fully elucidated. The aim of this thesis was initially applying a tandem affinity purification (TAP) of SV to identify unknown interaction partner of SV and to determine their role. This was supposed to be performed in the model organism Caenorhabditis elegans (C. elegans). The underlying mechanisms are conserved throughout the phylogentic tree and identified interaction partners will help to understand the processes in the mammalian brain. Although there is no neuron-rich tissue in C. elegans as in other model organisms, the diverse genetic methods allows a rapid creation of modified organisms and a prompt determination of the function of identified proteins. The integral SV protein synaptogyrin has been fused to a TAP-tag. The TAP-tag consists of a ProteinA, a TEV protease cleavage site and a calmodulin binding peptide (CBP). Both affinity purification steps are performed sequentially and allow a highly specific native purification of proteins and their interaction partners. Due to technical difficulties the purification strategy was modified several times during the course of this thesis and then finally abandoned for a more promising project, the SNARE complex purification. In conclusion, one of the reasons was the necessary lack of detergent.
The amended aim of this thesis has been the TAP of solubilized SNARE complex to identify unknown interaction partner and to determine their role. In order to increase the specificity of the purification, in terms of formed complexes, the two SNARE subunits, synaptobrevin (SNB-1 in C. elegans) and syntaxin (UNC-64 in C. elegans), were separately fused to the different affinity tags. As the modifications of the proteins could impair their function and lead to false interaction partners, their functionality was tested. For this purpose, the corresponding fusion constructs were expressed in strains with mutated snb¬1 and unc-64. Non-functional synaptic proteins display an altered course of paralysis in an aldicarb assay. The fusion proteins which were expressed in their respective mutant strains displayed a near to wild-type (WT) behavior in contrast to the naive mutant strains. Multiple TAP demonstrated SNB-1 signals in Western blot analysis and complex sets of proteins in the final elution step in a silver staining of SDS-PAGEs. These samples were sent with negative control (WT purification) for MS analysis to various cooperation partners. 119 proteins were identified which appeared only in data sets with SNARE proteins and not in WT samples. If proteins were detected in ≥ 2 SNARE positive MS analysis and had known neural functions or homologies to neuronal proteins in other species, they were selected for further analysis. These candidates were knocked down by RNAi and tested for synaptic function in a following aldicarb assay. The treatment with their specific RNAi resulted for mca-3 in a strong resistance, while frm-2, snap-29, ekl-6, klb-8, mdh-2, pfk-2, piki-1 and vamp-8 resulted in hypersensitivity. The most responsive genes frm-2, snap-29 and mca-3 were examined, whether they displayed a co-localization together with synaptobrevin in promoter fusion constructs or functional fusion constructs. In fluorescence microscopy images only MCA-3::YFP demonstrated neuronal expression.
In order to substantiate the synaptic nature and functionality of the MCA-3::YFP a swimming assay was performed. Here, fusion construct expressing strains, which contained mutated mca-3, were compared with untreated mutant strains and WT strains according to their behavior. In this swimming assay a partial restoration of WT behavior was shown in the MCA-3::YFP expressing mutant strains. Based on these data, we discovered with MCA 3 a new interaction partner of the SNARE complex. MCA-3 is a plasma membrane Ca2+-ATPase and was initially seen only in their role in the endocytosis. Its new putative role is the reduction of Ca2+ concentration at the bound SNARE complex. Since an interaction of syntaxin with Ca2+ channels has been demonstrated, it would be comprehensible to reduce the local concentration of Ca2+ to a minimum by tethering Ca2+ transporters to the SNARE complex.
Das Ziel dieser Arbeit ist die Entwicklung von neuen, experimentellen Ansätzen zur Thematisierung von Siliciumverbindungen im Chemieunterricht, die einen deutlichen lebensweltlichen Bezug aufweisen und moderne Entwicklungen berücksichtigen.
Die Bandbreite der Siliciumverbindungen reicht von den Silicaten im Bereich der Anorganik über elementares Silicium bis hin zu den polymeren Siliconen im Grenzbereich zu der Organik. Diese
große Vielfalt an Verbindungen hat eine Vielzahl von Anwendungen in tagtäglichen Produkten zur Folge. Dies sind einerseits relativ bekannte anorganische Baustoffe, wie Zement oder Sand, die schon seit der Antike von der Menschheit genutzt werden. Andererseits werden kontinuierlich neue Anwendungsmöglichkeiten in Alltag und Industrie für Siliciumverbindungen entwickelt, die in der modernen Lebenswelt der SchülerInnen einen festen Platz haben.
Oft ist das Vorhandensein der Siliciumverbindung gar nicht auf den ersten Blick erkennbar, obwohl sie die Eigenschaften eines Alltagsprodukts maßgeblich beeinflussen kann. Dies ist beispielsweise bei Silica-Verbindungen in der Zahncreme der Fall.
Im Chemieunterricht werden, wenn überhaupt, die „traditionellen“ Verwendungszwecke, wie in der Baustoffchemie, thematisiert, weniger dagegen die Funktion von Siliciumverbindungen in innovativen Produkten neueren Datums. Nur zögerlich werden Ansätze zur Thematisierung von Verbindungen, wie Siliconen, im Chemieunterricht etabliert.
Im Rahmen dieser Forschungsarbeit wurden daher auf der Grundlage einer fachdidaktischen Analyse und Diskussion Experimente zu ausgewählten Siliciumverbindungen entwickelt. Dies sind die Silicone, die Silica-Verbindungen und elementares Silicium. Die Experimente lassen sich größtenteils in der Sekundarstufe II in Anlehnung an verbindlich im Lehrplan thematisierte Inhalte in den Unterricht einbinden. Einige Experimente können nach einer angemessenen didaktischen Reduktion auch bereits in der Sekundarstufe I eingesetzt werden.
Die im Rahmen dieser Arbeit entwickelten Experimente wurden von LehrerInnen und SchülerInnen gleichermaßen erprobt. Es wurden Rückmeldungen zur Versuchen und Versuchsvorschriften eingeholt. Die Ergebnisse der Auswertung wurden zur Optimierung herangezogen.
Development and implementation of novel optogenetic tools in the nematode Caenorhabditis elegans
(2016)
Optogenetics, though still only a decade old field, has revolutionized research in neurobiology. It comprises of methods that allow control of neural activity by light in a minimally-invasive, spatio-temporally precise and genetically targeted manner. The optogenetic actuators or the genetically encoded light sensitive elements mediate light driven manipulation of membrane potential, intracellular signalling, neuronal network activity and behaviour (Fenno et al. 2011; Dugué et al. 2012). These techniques have been particularly useful for dissecting neural circuits and behaviour in the transparent and genetically amenable nematode model system Caenorhabditis elegans (Husson et al. 2013; Fang-yen et al. 2015).
In fact, C. elegans was the first living organism in which microbial rhodopsin based optogenetic tools (Channelrhodopsin-2 or ChR2, and Halorhodopsin or NpHR) were successfully implemented and bimodal 'remote' control of behaviour was achieved (Nagel et al. 2005; Zhang et al. 2007). Since then it has been a prominent model for the development and application of novel optogenetic tools and techniques, especially in the nervous system which comprises of 302 neurons and is organised in a hierarchical organization. The environmental stimuli are sensed by the sensory neurons, leading to the processing of information by the downstream interneurons, that relay to motor neurons which in-turn synapse onto muscles that drive the movement-based responses.
The microbial rhodopsins like ChR2 and NpHR mediate light driven depolarization and hyperpolarization, respectively and thereby activate or inhibit neural activity. However, they do not allow local control of membrane potential as they are expressed all over the plasma membrane of the cell rather than being restricted to specific domains, for example synaptic sites. Moreover, they completely over-ride the intrinsic activity of the cell, completely bypassing the signal transduction processes inside the cell. Thus, in order to study intracellular signalling and to answer questions pertaining to the endogenous role of receptors and channels in an in-vivo context, the optogenetic tool-kit needs to be expanded.
This thesis aimed at developing and implementing novel optogenetic tools in C. elegans that allow for sub-cellular signalling control as well as endogenous receptor control. These are: two light activated guanylyl cyclases (bPGC and BeCyclOp) to modify cyclic guanosine monophosphate (cGMP) mediated signalling in the sensory neurons, as well as attempts towards rendering endogenous C. elegans receptors - glutamate receptor (GLR-3/-6), acetylcholine receptor (ACR-16), glutamate gated chloride channel (GLC-1) light switchable and to understand their biological function in-vivo.
Organisms respond to sensory cues by activation of a primary receptor followed by relay of information downstream to effector targets by secondary signalling molecules. cGMP is a widely used 2nd messenger in cellular signaling, acting via protein kinase G or cyclic nucleotide gated (CNG) channels. In sensory neurons, cGMP allows for signal modulation and amplification, before depolarization. Chemo-, thermo-, and oxygen-sensation in C. elegans involve sensory neurons that use cGMP as the main 2nd messenger. For example, ASJ is the pheromone sensing neuron regulating larval development, AWC is the chemosensory neuron responding to volatile odours and BAG senses oxygen and carbon dioxide in the environment. In these neurons, cGMP acts downstream of the GPCRs and functions by activating cationic TAX-2/-4 CNG channels, thereby depolarising the sensory neuron. Manipulating cGMP levels is required to access signalling between sensation and sensory neuron depolarization, thereby provide insights into signal encoding. We achieve this by implementing two photo-activatable guanylyl cyclases - 1) a mutated version of Beggiatoa sp. bacterial light-activated adenylyl cyclase, with specificity for GTP (Ryu et al. 2010), termed BlgC or bPGC (Beggiatoa photoactivated guanylyl cyclase) and 2) guanylyl cyclase rhodopsin (Avelar et al. 2014) from Blastocladiella emersonii (BeCyclOp).
bPGC is a BLUF (blue light sensing using flavin) domain containing cyclase which uses FAD as the co-factor and catalyses the synthesis of cGMP from GTP upon activation by blue light. Prior to implementation in sensory neurons, a simpler heterologous system with co-expression of the TAX-2/-4 CNG channel in C. elegans body wall muscle (BWM) was used. The cGMP generated by the light activated cyclases activates the CNG channel leading to the muscle depolarization, thereby causing changes in body length which can be easily scored.
Um die Funktionsweise von biologischen Prozessen zu untersuchen, werden Trigger-Signale benötigt, die die Prozesse initiieren können, ohne dabei dem Organismus zu schaden oder Nebenreaktionen hervorzurufen. Ein geeignetes Trigger-Signal stellt Licht dar, da es bei geeigneter Wellenlänge nichtinvasiv ist und nur wenige biologische Prozesse durch Licht gesteuert werden. Um einen Prozess mit Licht aktivierbar zu machen, benötigt man eine lichtsensitive Einheit, beispielsweise eine photolabile Schutzgruppe, die durch die Bestrahlung mit Licht einen zuvor blockierten Bereich freisetzt.
Hauptziel dieser Arbeit war es die Zweiphotonen-Technik für die Photolyse von photolabil geschützten Oligonukleotiden nutzbar zu machen und das Photolyseergebnis zu visualisieren.
Dazu wurden zunächst verschiedene mit Zweiphotonen-sensitiven Schutzgruppen modifizierte Phosphoramidite synthetisiert und über Festphasensynthese in Oligonukleotide eingebaut. Die Oligonukleotide mit den erstmals neu eingebauten Schutzgruppen ANBP und hNDBF wurden zunächst auf ihre Einphotonen-Eigenschaften, wie Schmelzpunkt, Absorptionsverhalten und Quantenausbeute untersucht. Weiterhin wurden erste Versuche zur wellenlängenselektiven Photolyse von hNDBF- und ANBP-geschützten Oligonukleotiden durchgeführt.
Die Existenz eines Zweiphotonen-induzierten Effekts kann durch die quadratische Abhängigkeit des erzeugten Effekts von der eingestrahlten Leistung nachgewiesen werden. Dazu wurde ein Verdrängungs-Assay entwickelt, dessen Doppelstrang-Sonde aus einem FRET-Paar besteht. Der Fluorophor-markierte Strang dient dabei als Gegenstrang zum photolabil geschützten Strang. Durch einen Thiol-Linker am photolabil geschützten Oligonukleotid konnte dieses erfolgreich in Maleimid-Hydrogele immobilisiert werden und der Verdrängungs-Assay im Gel durchgeführt werden. Die immobilisierten Stränge enthielten DEACM bzw. ANBP Schutzgruppen. Neben der quadratischen Abhängigkeit der Photolyse von der eingestrahlten Leistung konnten in diesen Hydrogelen auch 3D-aufgelöste Photolysen realisiert werden, die eindeutig die Zwei-Photonen-Photolyse belegen. Diese 3D-Experimente wurden zusammen mit Dr. Stephan Junek am MPI für Hirnforschung durchgeführt. Durch die Wahl zweier unterschiedlicher Sequenzen für die dTDEACM und dGANBP modifizierten Stränge und zwei unterschiedlicher Fluorophore für die Doppelstrang-Sonden, konnte die orthogonale Zweiphotonen-Photolyse gezeigt werden. Um zu zeigen, dass die Zweiphotonen-Photolyse von Oligonukleotiden auch in Organismen realisiert werden kann ohne das biologische System zu schädigen, wurde versucht den Verdrängungs-Assay auch in Zellen durchzuführen. Durch die Verwendung der Patch-Clamp-Technik in Zusammenarbeit mit Dr. Stephan Junek am MPI für Hirnforschung konnten die Stränge über die Elektrolyt-Lösung in Hippocampus-Neuronen eingebracht werden und durch Zweiphotonen-Bestrahlung dort photolysiert werden, was zu einem deutlichen Fluoreszenzanstieg führte. Durch die angeschlossene Patch-Clamp-Pipette konnten so zusätzlich elektrophysiologische Messungen durchgeführt werden, die zeigten, dass die durchgeführte Zweiphotonen-Bestrahlung nicht invasiv für die Zellen ist.
Die durchgeführten Experimente beweisen, dass Zweiphotonen-sensitive Schutzgruppen auf Oligonukleotiden photolysiert werden können und dass ihr Einsatz auch in biologischen Systemen möglich ist. Der entwickelte Verdrängungs-Assay ermöglicht es weiterhin neue photolabile Schutzgruppen auf Oligonukleotiden auf ihre Zweiphotonen-Sensitivität zu untersuchen.
Ein weiteres Projekt beschäftigte sich mit der Synthese der neuen Schutzgruppe DMA-NDBF-OH, die in-silico von der Arbeitsgruppe von Prof. Andreas Dreuw aus Heidelberg als effiziente Zweiphotonen-sensitive Schutzgruppe beschrieben wird. Es wurde versucht DMA-NDBF-OH über zwei Syntheserouten herzustellen. Eine Route basierte auf der Einführung der Funktionalitäten an einem unmodifizierten Dibenzofuran, die leider an der Bromierung der Seitenkette scheiterte. Die zweite Syntheseroute wurde in Anlehnung an die NDBF-Synthese von Deiters et al., bei der das Dibenzofuran durch eine Kondensation zweier modifizierter Benzolringe und einem Pd-katalysierten Ringschluss aufgebaut wird, durchgeführt. Mit dieser Syntheseroute konnte das DMA-NDBF-OH erfolgreich synthetisiert werden. Aufgrund ihrer starken bathochromen Verschiebung sollte sich diese Schutzgruppe hervorragend für die wellenlängenselektive Photolyse auf Ein- und Zweiphotonenebene eignen.
Für die Optimierung sowie Entwicklung lichtsteuerbarer Systeme für biologische Anwendungen oder neue Materialien ist ein detailliertes Verständnis der zugrunde liegenden komplexen, lichtinduzierten Prozesse eine Voraussetzung. Die Verwendung von Photoschaltern in Makromolekülen ermöglicht eine zeitliche und örtliche Kontrolle über strukturelle Änderungen sowie die entsprechend folgenden (biologischen) Funktionen durch die Verwendung von Licht als externem Auslöser.
Ein wichtiger Bestandteil dieser Arbeit befasst sich mit der Entwicklung eines auf Licht reagierenden Riboschalters, welcher die gezielte Kontrolle über Genexpression ermöglicht. Hierzu wurde eine spektroskopische Charakterisierung von verschiedenen Photoschaltern bezüglich einer Verwendung als biologischer Ligand sowie der Wechselwirkungen zwischen Azobenzolen und RNA, auch hinsichtlich ihrer Bindungsdynamiken durchgeführt. Zunächst wurde die hohe Abhängigkeit der (photo-)chemischen Eigenschaften der Azobenzole von der Wahl der Substituenten untersucht, wobei besonders die Anwendung in wässrigem Milieu betrachtet wurde. In einer detaillierten (zeitaufgelösten) Studie wurde der positionsabhängige Einfluss der Hydroxy-Substitution von Azobenzolen auf die Photoisomerisierung in wässriger Lösung untersucht. Für eine ortho-Substitution ergab sich hierbei ein alternativer Deaktivierungskanal nach Photoanregung, welcher stärker ausgeprägt ist als die Isomerisierung. Hierbei wird ein intramolekularer Protontransfer im angeregten Zustand (ESIPT) beobachtet, welcher mit einer Zeitkonstante von 0.3 ps beschrieben werden kann und in einer Keto-Spezies resultiert. Eine Keto-Enol-Tautomerie konnte für die para-Hydroxy-Substitution schon im Grundzustand beobachtet werden. Somit können beide Spezies gezielt adressiert werden. Durch Acetylierung der Hydroxygruppe verlangsamt sich die thermische Relaxation des cis-Isomer zu dem entsprechenden trans-Isomer signifikant ohne die Isomerisierung zu beeinträchtigen. Dementsprechend ermöglicht eine solche Acetylierung die Verwendung von bekannten Azobenzolderivaten als Photoschalter.
Zudem werden in dieser Arbeit zwei verschiedene Herangehensweisen in der Entwicklung eines Riboschalters beschrieben, welcher sich durch Licht regulieren lässt.
Diese sind durch kovalentes bzw. nicht-kovalentes Einbringen eines Azobenzolderivats in die RNA Struktur charakterisiert. Ein neuer Linker, welcher auf einer Desoxyribose-Struktur beruht, wird für die kovalente Anbindung des Azobenzols an den RNA Strang präsentiert, welcher eine licht-induzierte Dehybridisierung ermöglichen soll. Eine außergewöhnlich hohe Schaltamplitude mit einem cis-Gehalt von etwa 90% konnte für das Azobenzol im RNA Einzelstrang schon bei Raumtemperatur ermittelt werden. Zudem wurde der Einfluss des Photoschalters sowie der benachbarten Nukleotide in der RNA auf die Stabilität der RNA Doppelhelix untersucht. Die zweite Vorgehensweise beruht auf einer nicht-kovalenten Bindung zwischen einem Azobenzolderivat und einem RNA-Aptamer, welche lediglich für eines der Photoisomere ermöglicht wird, wodurch eine örtliche und zeitliche Kontrolle der Ligandenbindung der RNA erfolgt. Im Rahmen dieser Arbeit war es möglich zwei verschiedene photoschaltbare RNA Aptamere zu identifizieren und zu untersuchen, welche eine hohe Spezifität und Affinität aufweisen. Zudem wurde die Photoisomerisierung des Azobenzols innerhalb der RNA-Struktur sowie daraus resultierende lichtinduzierte Konformationsänderungen der RNA mittels zeitaufgelöster Anreg-/Abtastspektroskopie untersucht. Die daraus resultierende Dynamik der photoinduzierten Ligandenbindung sollte eine weitere gezielte Optimierung lichtschaltbarer biologischer Systeme erlauben.
Der zweite Teil dieser Arbeit beschäftigt sich mit der zeitaufgelösten Untersuchung eines photoschaltbaren Foldamers. Speziell wurde der strukturelle Übergang des OmPE-Foldamers 10-5 zwischen einer definierten helikalen und einer ungefalteten Konformation auf Grund der Photoisomerisierung der, in das Rückgrat integrierten, Azobenzole untersucht.
Dabei konnten die frühen (Ent-)Faltungsmechanismen des Foldamers im sub-Nanosekunden-Zeitbereich beobachtet werden, welche durch quantenmechanische Rechnungen unterstützt werden konnten. Darüberhinaus, war es möglich einen Anregungsenergietransfer vom PE-Rückgrat des Foldamers auf die Azobenzole nachzuweisen, welcher die Lebensdauer der angeregten Zustände des Systems signifikant verkürzt.
Diese Arbeit liefert wichtige Informationen zu den Reaktionspfaden, den gezielten Wechselwirkungen zwischen Photoschaltern und größeren organischen Molekülen, sowie den daraus resultierenden lichtinduzierten strukturellen Änderungen durch die Anwendung einer Vielzahl an (zeitaufgelösten) spektroskopischen Methoden. Diese Ergebnisse tragen zum weiteren Verständnis komplexer Prozesse in biologischem sowie nicht-biologischem Zusammenhang und somit zu einer weiterführenden Entwicklung neuer Systeme bei.
Metal-organic frameworks (MOFs) have emerged as a promising class of crystalline porous inorganic-organic hybrid materials showing a wide range of applications. In order to realize the integration of MOFs into specific devices, this thesis mainly focuses on the controlled growth and the properties of highly oriented surface-mounted metal-organic frameworks (SURMOFs).
The stepwise layer-by-layer (LbL) growth method exhibits vast advantages for the controllable growth of SURMOFs regarding the crystallite orientation, film thickness and homogeneity. However, up to date, only a few MOFs have been demonstrated to be suited for this protocol. So the first project of this thesis was designed to extend the applicability of the LbL growth. To this end, a semi-rigid linker based [Cu2(sdb)2(bipy)] (sdb = 4,4’-sulfonylbiphenyl dicarboxylate; bipy = 4,4’-bipyridine) MOF was chosen. Employing the LbL growth, [Cu2(sdb)2(bipy)] SURMOFs were successfully grown onto both pyridyl- and carboxyl-terminated surfaces at the temperature range of 15-65 °C. Interestingly, the orientation of the SURMOFs largely depends on temperature on both surfaces. At low temperatures (below 40 °C), SURMOFs with exclusive [010] orientation are obtained. In contrast, at high temperatures (40-65 °C), [001] oriented SURMOF growth is favored. A novel growth mode was demonstrated, which is, instead of surface chemistry, the temperature-induced ripening processes and the tendency to minimize surface energies can dominate the SURMOF growth.
Inspired by the advantages of LbL deposition of isoreticular SURMOFs, the second project was conceived to grow multivariate SURMOFs (MTV-SURMOFs) using mixed dicarboxylate linkers. We advance a hypothesis that linker acidity (expressed by the pKa values) may have an influence on the oriented growth of MTV-SURMOFs. To test the hypothesis, seven isoreticular [Cu2L2(dabco)] (L = single kind of dicarboxylate linker; dabco = 1,4-diazabicyclo[2.2.2]octane) SURMOFs were grown onto pyridyl-terminated surfaces at 60 °C. The quality of [001] orientation is greatly affected by the acidity of the linkers. With this observation, we deposited a series of [Cu2Lm2(dabco)] (Lm = mixed dicarboxylate linkers) SURMOFs under the same conditions. [Cu2Lm2(dabco)] SURMOFs with exclusive [001] orientation are obtained when the growth solution contains two linkers of relatively high pKa value or more than two kinds of linkers (independent of the pKa values), while the mixtures of ligands with relatively low pKa values or a high content of low pKa valued linkers can result in mis-oriented growth of SURMOFs with unexpected [100] orientation.
Moreover, the LbL growth shows enormous potential in the rational construction of functional SURMOFs. Therefore, the third project of this thesis was devised to deposit SURMOFs containing redox-active species. For this, the 4,4’-biphenyldicarboxylic acid (H2(bpdc)) linker was functionalized with ferrocene (Fc) and dimethyl ferrocene (Me2Fc) moieties. [Cu2(bpdc-amide-Fc)2(dabco)] SURMOF (Fc-SURMOF) is perfectly grown along the [100] direction, while mis-oriented growth of [Cu2(bpdc-amide-Me2Fc)2(dabco)] SURMOF (Me2Fc-SURMOF) was observed. Surprisingly, Fc-SURMOF shows excellent electrochemical properties due to the reversible oxidation and reduction of the ferrocene moieties in the oriented pores, while the Me2Fc-SURMOF was found to be a closely packed insulating layer since no extensive charge transfer is observed. A diffusion controlled mechanism of redox reaction is proposed, where the diffusion of the counter anions in the pores limits the current.
Besides the LbL growth protocol, the spin-coating technique is also promising for the oriented growth of SURMOFs. Driven by the specific applications, the fourth project of this thesis was planned to grow functional SURMOFs containing catalytically active units. The Keggin-type polyoxometalates (POMs) with high catalytic activities were chosen to functionalize the HKUST-1 SURMOFs. Combining the technique with methanol vapor induced growth, a series of POM functionalized HKUST-1 SURMOFs (denoted as POM@HKUST-1 SURMOFs) were controllably deposited onto pyridyl-terminated surfaces. The SURMOFs exhibit great potential as electrocatalysts in electrochemical devices due to the excellent redox properties of POMs. In addition, the PTA@HKUST-1 (PTA = phosphotungstic acid) SURMOF can be employed as an ideal platform for the selective loading of methylene blue (MB) dye with high efficiency. Owing to the strong binding between the dye molecules and the framework, the MB dye cannot be desorbed by ion exchange and MB loaded PTA@HKUST-1 SURMOF shows reliable redox properties under inert conditions, further confirming the application potential in electrochemical devices.
Ribosomes are the central cellular assembly lines for protein synthesis. To cope with the translational needs, a proliferating mammalian cell can produce up to 7500-ribosomes per minute. However, under growth limiting conditions, such as nutrient depletion, ribosome synthesis is rapidly shut down exemplifying the importance of a tight coordination between ribosome supply and cellular energy status. In addition to the quantitative regulation, a strict quality control of ribosome synthesis is equally important, because alterations in the composition or function of ribosomes can lead to a variety of pathologies. To cope with these challenges a highly regulated, multi-step pathway of ribosome biogenesis has evolved. In mammals this pathway generates the mature 80S ribosomes that comprise the large 60S and the small 40S subunits. Together they contain around 80 ribosomal proteins and the 28S, 18S, 5.8S and 5S rRNAs. The 28S, 5.8S and 5S rRNAs are assembled into the large subunit, while the 18S rRNA is part of the small subunit. The pathway of ribosome biogenesis is a multi-step cellular process, where specific stages occur in distinct subcellular compartments. Transcription of the 47S rRNA, which is the precursor for the 28S, 18S and 5.8S species, occurs in the nucleolus. Modification of distinct bases and early processing of this precursor also take place in the nucleolus. Subsequently, the 40S and 60S pre-ribosomes take separate maturation routes through the nucleoplasm before their export and final assembly in the cytoplasm. The various stages of preribosomal maturation require the constant and sequential action of a large number of non-ribosomal proteins, known as trans-acting factors. These factors coordinate the delicate remodeling of the pre-ribosomal intermediates and thereby ensure proper progression of the maturation process. The remodeling events largely depend on the dynamics of post-translational modifications, such as phosphorylation or SUMOylation. This requires that the enzymes controlling these modifications are properly targeted to their sites of activity as they fulfill their functions within specific compartments. Here we studied the regulatory principles that govern the subcellular partitioning of the SUMO-specific isopeptidase SENP3 and its associated factor PELP1. Previous work from our laboratory has delineated the importance of the SUMO system for proper ribosome biogenesis in mammalian cells. In particular, we have shown that SENP3 is critically involved in 28S rRNA formation, which is a key step for pre-60S subunit maturation. A critical involvement of SENP3 at this stage of the maturation process is in agreement with the observed enrichment of SENP3 in the nucleolus, since 28S rRNA processing is considered to occur in the nucleolus. Our subsequent work identified the nucleolar scaffold protein NPM1 and the ribosomal trans-acting factor PELP1 as bona fide substrates of SENP3. For both proteins we could demonstrate modification by SUMO2/3 and define SENP3 as the demodifying enzyme. Depletion of SENP3 enhanced the conjugation of SUMO to both proteins and concomitantly reduced conversion of the 32S pre-rRNA to the mature 28S rRNA. PELP1 is part of a larger protein complex consisting of the core components PELP1, TEX10 and WDR18. We could show that the balanced SUMOylation/deSUMOylation of PELP1 controls the nucleolar/nucleoplasmic distribution of this complex. Enhanced SUMOylation, which is observed in the absence of SENP3, triggers the nucleolar release of the complex suggesting that SENP3-mediated deSUMOylation controls the dynamics of nucleolar trans-acting factors. Based on these findings we first wanted to understand, in which cellular compartment(s) SENP3 exerts its function on 28S maturation. Next, we wanted to tackle the question how the subcellular distribution of SENP3 is controlled. Finally
we addressed the question how the SUMOylation of PELP1 determines the subnuclear distribution of the PELP1 complex. This work initially revealed that the nucleolar localization of SENP3 is crucial for proper 28S rRNA formation and 60S ribosome maturation. Importantly, we could demonstrate that the nucleolar compartmentalization of SENP3 depends on its direct physical interaction with NPM1. Further, we could show that the amino-terminal region of SENP3 is necessary for its binding to NPM1 and nucleolar recruitment. Strikingly, this interaction requires the phosphorylation of SENP3, which is brought about by the mTOR kinase. By in-vitro kinase assays and mass-spectrometric approaches we identified five serine/threonine residues within the amino-terminal region of SENP3 that are targeted by mTOR (S/T 25, 26, 141, 142, 143). We could further demonstrate by mutagenesis that these sites in SENP3 are in fact critical for the phospho-dependent binding of SENP3 to NPM1 and its nucleolar recruitment.
Consistent with these data, we found that chemical inhibitors of the mTOR kinase trigger the nucleolar release of SENP3 and impair its interaction with NPM1. Strikingly, this goes along with severe 28S rRNA maturation defects demonstrating the physiological importance of mTOR signaling in the regulation SENP3 function and rRNA processing. By specifically depleting components of the either mTORC1 or mTORC2, we could attribute the observed effects to signaling by mTORC1 rather than mTORC2. In an attempt to find the negative regulators of SENP3 phosphorylation, we identified PP1-γ as the candidate phosphatase in this pathway. We found a strong physical interaction of SENP3 with PP1-γ and observed a loss of SENP3 nucleolar localization upon ectopic expression of PP1-γ. Thus we could define mTOR/PP1-γ mediated phosphorylation/dephosphorylation of SENP3 as an important
mechanism in the control of ribosome maturation. Given that mTOR activity is controlled by nutrient availability, SENP3 functions as a sensor that couples ribosome synthesis with nutrient availability. The second part of this work delineated the role of SUMOylated PELP1 in nucleoplasmic partitioning of the SENP3-PELP1 complex. It was revealed that the AAA-ATPase MDN1 binds preferentially to SUMO modified PELP1 and likely segregates SUMOylated PELP1 from nucleolar pre-60S particles. We initially found that the PELP1 complex associates with MDN1, a factor known to be involved in the 28S rRNA maturation. Notably, depletion of MDN1 led to an enhanced accumulation of the PELP1 complex in the nucleolus and a strong association of PELP1 with pre-60S particles, suggesting that MDN1 is required for the release of this complex from the pre-ribosomes. Intriguingly, the interaction of PELP1 with MDN1 requires SUMO2/3 and SUMOylated PELP1 shows enhanced binding to MDN1 when compared to unmodified PELP1. Taken together this work provides new insights in the control of the SENP3-PELP1 complex dynamics. We could define several layers for the coordinated spatial regulation of SENP3 and the PELP1 complex. This work therefore underscores the crucial importance of dynamic post-translational modifications for the control of ribosome maturation.
Entwicklung neuer Multikomponentenreaktionen zur Synthese von Amin- und α-Aminosäurederivaten
(2016)
Die Entwicklung neuer Synthesemethoden ist von enormer Bedeutung hinsichtlich der Darstellung von neuen Verbindungen mit speziellen, anwendungsorientierten Eigenschaften und in Bezug auf die Suche nach ökologisch verträglicheren und effizienteren Herstellungsmethoden. Multikomponentenreaktionen (MCRs) bieten hierbei eine gute Ansatzmöglichkeit. Gegenüber den klassischen, linear verlaufenden 2-Stufen-Reaktionen weisen MCRs eine hohe Atom-Ökonomie und effiziente Bindungsbildung auf, können zur Minimierung von Zeit-, Energie-, Material- und Kostenaufwand sowie zur geringeren Generierung von Abfallmengen beitragen und ermöglichen einen schnellen Aufbau diverser Molekülstrukturen. Vor diesem Hintergrund gelang im Rahmen der vorliegenden Arbeit die Entwicklung mehrerer 3-Komponentenreaktionen basierend auf der nukleophilen Addition von Arylboronsäuren an in situ gebildete N-Acyl- bzw. N-Sulfonylimine, womit die Synthese von diversen alpha-substituierten Amiden, chiralen, alpha-substituierten Sulfonamiden, chiralen alpha-Arylglycinen sowie von Arylmethylsulfonamiden erfolgte. Der Schlüssel zu einer erfolgreichen Umsetzung hinsichtlich der Methode mit Amiden war die Verwendung eines dualen Katalysatorsystems aus Lewis-Säure und Pd(II) sowie die Anwesenheit von Wasser. Die enantioselektiven Varianten konnten mittels Sulfonamide anstelle der Amide sowie unter Einsatz von Pd(II) und einem chiralen Oxazolin-Liganden erreicht werden. Die neuen Methoden sind einfach in der Durchführung, weisen einen breiten Substrat-bereich auf und im Falle der asymmetrischen Varianten hohe Enantioselektivitäten.
Allerdings besitzt die Reaktionsführung über Organoboronsäuren zwei entscheidende Nachteile: Zum einen bedarf es der Verwendung vorfunktionalisierter Boronsäuren und zum anderen werden stöchiometrische Mengen borhaltiger Abfälle erzeugt. Daher wurden im Rahmen dieser Arbeit auch Prozesse untersucht, bei denen hinsichtlich der Atom-Ökonomie keine unnötig vorfunktionalisierten Startmaterialien eingesetzt werden und bei denen keine oder nur ökologisch vollkommen unbedenkliche Nebenprodukte entstehen. Ein erster Ansatz in diese Richtung gelang dabei mit der Entwicklung einer neuen 3-Komponentenreaktion basierend auf einer Brønsted-Säurekatalysierten, benzylischen C–H-Bindungsfunktionalisierung von 2-Alkylazaarenen.
Cells perform a wide range of functions such as signalling, transportation, immunoprotection and metabolism. Unravelling the molecular mechanism behind those processes will provide a platform for more targeted and rational drug design. This is achieved by discerning the structural and functional aspects of the biological macromolecules involved. This thesis discusses about the biophysical characterization of protein structures and the biological importance of protein dynamics. Membrane receptors and enzymes which are ubiquitously present in our biological systems and regulate wide variety of functions are excellent choice for such study. From a pharmaceutical point of view, receptor and enzymes are exceptionally important drug targets as they represent the major share (receptor, 30% and enzymes, 47%) of all marketed drugs. Therefore, apart from biological insights, the detailed study of receptors and enzymes will provide the basis for new pharmaceutical applications. Most information about receptor activation and enzyme activity come from the structural and functional analysis of target members of the above mentioned systems.
In “Chapter 1 – General Introduction” the readers are introduced to the world of proteins with special focus on G-protein coupled receptors (GPCRs) and methyltransferases. The first part of this chapter discusses about GPCRs with emphasis on their classification, structural features and functions. GPCRs are the most abundant membrane receptors present in mammalian cells, accounting for almost 15% of all membrane proteins. The GPCR superfamily consists of ~800 members and can be subdivided into six classes (A-F). Class A containing rhodopsin, peptide hormones, olfactory GPCRs, is the most abundant with a large share of 85% of GPCR protein family. GPCRs share a common architecture of 7 transmembrane a-helices, with different ligand binding sites. Although a variety of ligands ranging from subatomic particles (a photon) to large proteins can activate a GPCR, their mechanism of signal transduction is almost similar. There are two major signal transduction pathways identified for GPCRs: the cAMP pathway and the phosphatidylinositol pathway. The therapeutic relevance of GPCRs has also been pointed out here since a large share (30%) of modern marketed drugs target GPCRs.
In the second part of this chapter, the structural and functional characterizations of methyltransferases (MTs) are discussed in detail. Several important biological processes in cells e.g. drug metabolism, gene transcription, epigenetic regulations are modulated by methylation of targets ranging from small biomolecules to large proteins. MTs are the proteins which catalyze this methylation reaction and transfer the methyl group to an acceptor molecule through SN2 like nucleophilic substitution reaction. The MTs can be classified on the basis of the substrate atoms they methylate: O (54% of all MTs), N (23%), C (18%), S (3%) and other acceptors (such as halides; 2%). They can also be categorized into five different classes (Class I-V) depending upon distinctive structural features facilitating substrate binding or catalytic activity. Rossmann fold and SET (acronym acquired from the Drosophila Su(var)3-9 and 'Enhancer of zeste' proteins) domain are the two characteristic structural motifs commonly found in MTs. Similar to GPCRs, MTs dysfunction has been shown to be involved in various diseases including neuropsychiatric diseases and cancer. Therefore they are also interesting targets for drug development. The final part of this chapter discusses the importance of structural biology in gathering information related to structure and conformational dynamics of proteins. The two prominent biophysical techniques used in structural biology, X-ray crystallography and NMR, are discussed with focus on their advantages and limitation. The importance of NMR spectroscopic techniques to investigate different dynamic processes of protein at atomic resolution under physiological conditions is also discussed. Real time NMR spectroscopy required for the analysis of slow protein dynamic processes (protein folding, enzyme catalysis, domain rearrangement) has been explained in detail.
The second part of the thesis (Chapters 3-4), which is the cumulative part, comprises the original publications grouped into 2 chapters according to their topic:
• NMR-spectroscopic characterization of the transiently populated photointermediates of bovine rhodopsin and it’s interaction with arrestin (Chapter 3)
• Structural and biophysical characterization of PaMTH1, a putative SAM dependent O-methyltransferase from filamentous fungi Podospora anserina (Chapter 4)
Each chapter is initiated by a detailed introduction to the topic, providing the framework for the following papers. The personal contribution of this thesis’ author to each publication is stated in the introduction to the respective article.