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Ubiquitin ligases and beyond
(2012)
First paragraph (this article has no abstract): In a review published in 2004 [1] and that still repays reading today, Cecile Pickart traced the evolution of research on ubiquitination from its origins in the proteasomal degradation of proteins through the revelation that it has a central role in cell cycle regulation and the recognition of regulatory roles for ubiquitin in intracellular membrane transport, cell signalling, transcription, translation, and DNA repair.
In dieser Arbeit wurden Methoden entwickelt, mit denen das Auflösungsverhalten schwer wasserlöslicher schwacher Säuren verbessert werden kann. Als Modellwirkstoffe wurden drei Vertreter der Sulfonylharnstoff-Gruppe (Glibenclamid, Glipizid und Glimepirid) gewählt. Diese Wirkstoffe, werden zur oralen Standardtherapie des Typ 2 Diabetes eingesetzt. Die Ergebnisse aus den Löslichkeits- und Freisetzungsuntersuchungen der reinen Arzneistoffe bildeten in dieser Arbeit den Ausgangspunkt der Entwicklungsarbeit. Um den Einfluss der galenischen Methoden auf das Freisetzungsverhalten der entwickelten Formulierungen besser zu beurteilen, wurden ebenfalls entsprechende Handelspräparate (Euglucon N 3,5 mg, Luditec 5 mg und Amaryl 4 mg) untersucht. Zunächst wurden mit Glibenclamid und dem natürlichen ?-CD sowie verschieden Cyclodextrin-Derivaten (M-?-CD und HP-?-CD) binäre Komplexe im molaren Verhältnis von 1:2 (Glibenclamid:CD) hergestellt und charakterisiert. Anschließend wurden feste Lösungen aus Glibenclamid und Kollicoat(r) IR bzw. PVP K30 entwickelt. Bei den nachfolgenden Freisetzungsuntersuchungen zeichnete sich im Falle der binären Cyclodextrin-Komplexe ab, dass der Glibenclamid-HP-?-CD-Komplex das beste Freisetzungsverhalten von Glibenclamid in den untersuchten Medien erreichte. Bei den festen Lösungen von Glibenclamid gab es zwischen den beiden untersuchten Polymeren keine signifikanten Unterschiede im Ausmaß der Glibenclamidfreisetzung. Im nächsten Schritt wurden ternäre Komplexe (Glibenclamid-HP-?-CD-Polymer) entwickelt, eine Kombination aus binären CD- Komplexen und festen Lösungen. Als dritte Komponente wurden Kollicoat(r) IR, PVP K30 und PEG 6000 in unterschiedlichen Zusätzen, 5, 10 und 20% bezogen auf den zugrunde liegenden binären Glibenclamid-HP-?-CD-Komplex eingearbeitet. Die Charakterisierung der verschiedenen ternären Komplexe ergab, dass das beste Freisetzungsverhalten bei den Komplexen, welche einen 10%igen Kollicoat(r) IR- bzw. 20%igen PVP K30-Zusatz enthielten, generiert werden konnte. Bei den drei verwendeten Methoden (binäre-, ternäre Komplexe und feste Lösungen) erhielt man während der Freisetzungsuntersuchungen in den Medien mit einem pH-Wert unterhalb des pKs-Wertes von Glibenclamid (5,4) eine übersättigte Wirkstofflösung, was zum Teil innerhalb kürzester Zeit zum Präzipitieren des Wirkstoffes führte. Initiale DSC-Untersuchungen hatten gezeigt, dass Glibenclamid in den beschriebenen Präformulierungen in amorpher Form vorlag, was der Grund für die rasche Freisetzung war. Anschließend wurde versucht, das Präzipitieren zu verlangsamen und im besten Fall zu verhindern. Hierfür wurde HPMC in verschiedenen Formen verwendet. Das einfache Hinzumischen von HPMC in eine Gelatine-Kapsel zu der Glibenclamid-Formulierung führte aufgrund von Agglomeratbildungen zu einer deutlichen Verzögerung der Wirkstofffreisetzung. Pankreatin als Zusatz zum Freisetzungsmedium konnte die Bildung eines Agglomerates nicht verhindern, was darauf schließen ließ, dass dieses nicht durch sogenanntes "Cross-linking" der Gelatine entstanden war. In einem nächsten Schritt wurden HPMC-Kapseln eingesetzt. Die Glibenclamidfreisetzung konnte durch einfaches Austauschen der Gelatine-Kapseln gegen Vcaps(r) Plus-Kapseln in allen untersuchten Medien deutlich gesteigert werden, was auf die durch die Anwesenheit von HPMC verzögerte Präzipitation des Wirkstoffes im Freisetzungsmedium zurückzuführen war. Im nächsten Schritt wurde, die Formulierungsmethode von Glibenclamid, auf Glipizid übertragen. Es wurde analog zu Glibenclamid ein binärer Glipizid-HP-?-CD-Komplex im molaren Verhältnis von 1:2 (Glipizid:HP-?-CD) hergestellt. Dieser Komplex führte zu einer deutlichen Verbesserung des Auflösungsverhaltens von Glipizid, was zu einer annähernd 100%igen Wirkstofffreisetzung in allen untersuchten Medien führte. Weiterhin wurden die mit Glibenclamid entwickelten Methoden auch auf Glimepirid übertragen. Die Formulierung von Glimepirid zu einem binären Glimepirid-HP-?-CD-Komplex führte zu einer höheren Wirkstofffreisetzung, verglichen mit der kristallinen Reinsubstanz und des Handelspräparates. Durch die Verarbeitung von Glimepirid in ternären Komplexen erhöhte sich das Ausmaß der Wirkstofffreisetzung deutlich. Mit Kollicoat(r) IR konnte eine Wirkstofffreisetzung von ca. 60% der Dosis und mit PVP K30 als dritter Komponente sogar ca. 85% Wirkstofffreisetzung in Blank FeSSIF erzielt werden. Das Präzipitieren des Wirkstoffes nach initialer Wirkstofffreisetzung in Blank FeSSIF konnte durch den Einsatz von Vcaps(r) Plus-Kapseln deutlich reduziert werden. Stabilitätsuntersuchungen, welche mit den in dieser Arbeit verwendeten Präformulierungen durchgeführt wurden zeigten, dass der jeweilige Wirkstoff auch nach einem Jahr der Lagerung bei Raumtemperatur und < 30% rel. Luftfeuchte, in amorpher Form in den entsprechenden Präformulierungen vorlag. All diese Untersuchungen zeigten eindrucksvoll, dass sich Cyclodextrin-Derivate in Kombination mit hydrophilen Polymeren, dazu eigneten, die Verfügbarkeit schwer löslicher Wirkstoffe im Dünndarm für deren Resorption zu verbessern. Es wurde gezeigt, dass die Herstellungsmethodik der Cyclodextrin-Komplexe einen wesentlichen Einfluss auf die Wirkstofffreisetzung hatte.
Die Translokation von gelösten Stoffen über zelluläre Membranen ist ein essentieller biologischer Prozess, der durch eine Vielfalt an integralen Membranproteinen vermittelt wird. Diese sind in den selektiven Austausch verschiedenster Stoffe bzw. Teilchen involviert und ermöglichen somit die Kommunikation zwischen den einzelnen Zellkompartimenten untereinander bzw. mit der extrazellulären Umgebung. Eine der größten Familien paraloger Proteine, die den vektoriellen Transport von Substanzen über Zellmembranen katalysieren, stellen die ATP‐binding cassette (ABC)‐Transporter dar. Mitglieder dieser Proteinfamilie sind in allen bisher untersuchten Organismen von Prokaryoten bis hin zu höheren Eukaryoten vertreten und übernehmen essentielle Funktionen in einer Vielzahl von zellulären Abläufen. ABC‐Transporter zeichnen sich durch eine breite Substratdiversität aus, d.h. sie energetisieren unter ATP‐Verbrauch die Translokation zahlreicher, strukturell und chemisch unterschiedlicher Substanzen wie Zucker, Lipide, Ionen, Aminosäuren, Proteine oder auch zelltoxische Stoffe. In Bakterien können sie sowohl als Importproteine fungieren, welche hauptsächlich die Aufnahme von Nährstoffen vermitteln, als auch als Exportproteine, deren Hauptaufgabe es ist, zelltoxische Substanzen aus der Zelle heraus zu schleusen. Eukaryotische ABC‐Transporter sind sowohl in der Plasmamembran als auch in den intrazellulären Membranen zu finden – beispielsweise in denen des Endoplasmatischen Retikulums, des Golgi Apparats, der Lysosomen, der Peroxisomen und der Mitochondrien. Sie fungieren als Exportproteine und sind z.B. an der Ionen‐Homöostase, der Antigenprozessierung, der Insulinfreisetzung oder am Cholesterol‐ und Lipidtransport beteiligt. ...
Die Synthese des Coenzymmodells Flavin-benzimidazol-dinucleotid * gelang durch Kondensation von Benzimidazolribotid-imidazolid 1 oder Benzimidazolribotid-guanidiniumamidat 2 mit Flavinmononucleotid. Das Coenzymmodell war enzymatisch nicht aktiv und bildete keinen Enzym-Coenzym-Komplex. Im Absorptionsspektrum konnte eine Extinktionszunahme nach der Spaltung der Pyrophosphatbrücke nur im Bereich von 260 mμ beobachtet werden. Das Molekül liegt daher vermutlich in einer gefalteten Form vor. Ein Komplex zwischen Flavin- und Benzimidazolteil konnte nicht nachgewiesen werden. Eine Fluoreszenzunterdrückung, die im FAD durch die Komplexbildung zwischen Flavin- und Adeninteil bedingt wird, wurde im FBD-Coenzymmodell nicht beobachtet.
From a global viewpoint, a lot of time is spent within the indoor air compartment of vehicles. A German study on mobility has revealed that, on average, people spend 45 minutes per day inside vehicles. In recent years the number of cars has increased to around 43 million vehicles in private households. This means that more than one car can be used in every household. The ratio has been growing, especially in eastern Germany and rural areas. "Overall and especially outside the cities, the car remains by far number one mode of transport, especially in terms of mileage". Therefore, numerous international studies have addressed different aspects of indoor air hygiene, in the past years. In this paper, meaningful original studies on car indoor air pollution, related to VOCs, COx, PMs, microbials, BFRs, OPFRs, cigarettes, electronic smoking devices, high molecular weight plasticizer, and NOx are summarized in the form of a review. This present review aimed to summarize recently published studies in this important field of environmental medicine and points to the need for further studies with special recommendations for optimizing the interior air hygiene.
Secondary multidrug (Mdr) transporters utilize ion concentration gradients to actively remove antibiotics and other toxic compounds from cells. The model Mdr transporter MdfA from Escherichia coli exchanges dissimilar drugs for protons. The transporter should open at the cytoplasmic side to enable access of drugs into the Mdr recognition pocket. Here we show that the cytoplasmic rim around the Mdr recognition pocket represents a previously overlooked important regulatory determinant in MdfA. We demonstrate that increasing the positive charge of the electrically asymmetric rim dramatically inhibits MdfA activity and sometimes even leads to influx of planar, positively charged compounds, resulting in drug sensitivity. Our results suggest that unlike the mutants with the electrically modified rim, the membrane-embedded wild-type MdfA exhibits a significant probability of an inward-closed conformation, which is further increased by drug binding. Since MdfA binds drugs from its inward-facing environment, these results are intriguing and raise the possibility that the transporter has a sensitive, drug-induced conformational switch, which favors an inward-closed state.
Mechanistic and structural studies of membrane proteins require their stabilization in specific conformations. Single domain antibodies are potent reagents for this purpose, but their generation relies on immunizations, which impedes selections in the presence of ligands typically needed to populate defined conformational states. To overcome this key limitation, we developed an in vitro selection platform based on synthetic single domain antibodies named sybodies. To target the limited hydrophilic surfaces of membrane proteins, we designed three sybody libraries that exhibit different shapes and moderate hydrophobicity of the randomized surface. A robust binder selection cascade combining ribosome and phage display enabled the generation of conformation-selective, high affinity sybodies against an ABC transporter and two previously intractable human SLC transporters, GlyT1 and ENT1. The platform does not require access to animal facilities and builds exclusively on commercially available reagents, thus enabling every lab to rapidly generate binders against challenging membrane proteins.
Membrane-Phloretin Interaction, Infrared Raman, ESR Spectroscopy The transport inhibitor phloretin was bound to human red cell membrane and the concomitant structural changes were observed by spectroscopic methods. By the spin labeling method a decrease in fluidity of the membrane was found at 1 and 10 |iM concentrations of the reagent. This result was obtained with the 2-(3-Carboxypropyl)-4,4-dimethyl-2-tridecyl-3-oxazolidinyloxyl, and the 2-(14-Carboxytetradecyl)-2-ethyl-4,4-dimethyl-3-oxazolidinyloxyl lipid spin labels. Infrared spectroscopy of modified membranes revealed an intensity increase of the POO~ band at about 1250 cm-1. Moreover, a shift of the peak at 1050 cm -1 to 1100 cm-1 was observed in the presence of phloretin. Raman spectroscopy of the membranes did not contradict the results found with infrared and ESR spectroscopy: In the phloretin modified membrane we observed a lack of the band at 1085 cm-1, which leads to suggest that the POO" and/or C-C regions are less fluid. Changes of the extracted red cell membrane lipids were less characteristic, and the results differed from those found in red cell membrane.
Proton-pumping complex I of the mitochondrial respiratory chain is among the largest and most complex membrane protein complexes. The enzyme contributes substantially to oxidative energy-conversion in eukaryotic cells. Its malfunctions are implicated in many hereditary and degenerative disorders. Here, we report the X-ray structure of mitochondrial complex I at 3.6- 3.9 Å resolution describing in detail the central subunits that execute the bioenergetic function. A continuous axis of basic and acidic residues running centrally through the membrane arm connects the ubiquinone reduction site in the hydrophilic arm to four putative proton-pumping units. The binding position for a substrate analogous inhibitor and blockage of the predicted ubiquinone binding site provide a model for the ‘deactive’ form of the enzyme. The proposed transition into the active form is based on a concerted structural rearrangement at the ubiquinone reduction site rendering support for a two-state stabilization-change mechanism of protonpumping.
Membrane-bound complex I (NADH:ubiquinone oxidoreductase) of the respiratory chain is considered the main site of mitochondrial radical formation and plays a major role in many mitochondrial pathologies. Structural information is scarce for complex I, and its molecular mechanism is not known. Recently, the 49-kDa subunit has been identified as part of the "catalytic core" conferring ubiquinone reduction by complex I. We found that the position of the 49-kDa subunit is clearly separated from the membrane part of complex I, suggesting an indirect mechanism of proton translocation. This contradicts all hypothetical mechanisms discussed in the field that link proton translocation directly to redox events and suggests an indirect mechanism of proton pumping by redox-driven conformational energy transfer.
A metal–organic framework (MOF) material, [Zn2(adc)2(dabco)] (adc = anthracene-9,10-dicarboxylate, dabco = 1,4-diazabicyclo[2.2.2]octane), the fluorescence of which depends on the loading of its nanopores, was synthesized in two forms: as free-flowing nanocrystals with different shapes and as surface-attached MOFs (SURMOFs). For the latter, we used self-assembled monolayers (SAMs) bearing functional groups, such as carboxylate and pyridyl groups, capable of coordinating to the constituents of the MOF. It could be demonstrated that this directed coordination also orients the nanocrystals deposited at the surface. Using two different patterning methods, i.e., microcontact printing and electron-beam lithography, the lateral distribution of the functional groups could be determined in such a way that the highly localized deposition of the SURMOF films became possible.
Metallorganische Netzwerke (engl. metal-organic frameworks, MOFs) sind eine neuartige Klasse mikro/mesoporöser Materialien, für die eine Vielzahl von möglichen Anwendungen demonstriert werden konnte. Das Ziel dieser Arbeit besteht in der Synthese von MOF Mikro/Nanopartikeln sowie der Herstellung von sogenannten Oberflächen-deponierten MOFs (engl. surface-attached metal-organic frameworks, SURMOFs). MOF Partikel mit kontrollierbarer Morphologie und Größe wurden unter milden Bedingungen synthetisiert. Um MOFs als Sensoren, intelligente Membrane, oder in nanotechnologischen Bauelementen verwenden zu können, ist die Integration auf der jeweiligen Oberfläche wichtig. Daher beschäftigt sich der Großteil dieser Arbeit mit der kontrollierten Abscheidung von SURMOFs auf verschiedenartigen Trägermaterialien. Etliche interessante Eigenschaften (z.B. die Fluoreszenz in Abhängigkeit von der Gegenwart von Gastmolekülen und die dynamische Gasadsorptionskapazität) der SURMOFs wurden untersucht.
Reciprocal t(9;22) ABL/BCR fusion proteins: leukemogenic potential and effects on B cell commitment
(2009)
Background: t(9;22) is a balanced translocation, and the chromosome 22 breakpoints (Philadelphia chromosome – Ph+) determine formation of different fusion genes that are associated with either Ph+ acute lymphatic leukemia (Ph+ ALL) or chronic myeloid leukemia (CML). The "minor" breakpoint in Ph+ ALL encodes p185BCR/ABL from der22 and p96ABL/BCR from der9. The "major" breakpoint in CML encodes p210BCR/ABL and p40ABL/BCR. Herein, we investigated the leukemogenic potential of the der9-associated p96ABL/BCR and p40ABL/BCR fusion proteins and their roles in the lineage commitment of hematopoietic stem cells in comparison to BCR/ABL. Methodology: All t(9;22) derived proteins were retrovirally expressed in murine hematopoietic stem cells (SL cells) and human umbilical cord blood cells (UCBC). Stem cell potential was determined by replating efficiency, colony forming - spleen and competitive repopulating assays. The leukemic potential of the ABL/BCR fusion proteins was assessed by in a transduction/transplantation model. Effects on the lineage commitment and differentiation were investigated by culturing the cells under conditions driving either myeloid or lymphoid commitment. Expression of key factors of the B-cell differentiation and components of the preB-cell receptor were determined by qRT-PCR. Principal Findings: Both p96ABL/BCR and p40ABL/BCR increased proliferation of early progenitors and the short term stem cell capacity of SL-cells and exhibited own leukemogenic potential. Interestingly, BCR/ABL gave origin exclusively to a myeloid phenotype independently from the culture conditions whereas p96ABL/BCR and to a minor extent p40ABL/BCR forced the B-cell commitment of SL-cells and UCBC. Conclusions/Significance: Our here presented data establish the reciprocal ABL/BCR fusion proteins as second oncogenes encoded by the t(9;22) in addition to BCR/ABL and suggest that ABL/BCR contribute to the determination of the leukemic phenotype through their influence on the lineage commitment.
Characterization of a dual BET/HDAC inhibitor for treatment of pancreatic ductal adenocarcinoma
(2020)
Pancreatic ductal adenocarcinoma (PDAC) is resistant to virtually all chemo‐ and targeted therapeutic approaches. Epigenetic regulators represent a novel class of drug targets. Among them, BET and HDAC proteins are central regulators of chromatin structure and transcription, and preclinical evidence suggests effectiveness of combined BET and HDAC inhibition in PDAC. Here, we describe that TW9, a newly generated adduct of the BET inhibitor (+)‐JQ1 and class I HDAC inhibitor CI994, is a potent dual inhibitor simultaneously targeting BET and HDAC proteins. TW9 has a similar affinity to BRD4 bromodomains as (+)‐JQ1 and shares a conserved binding mode, but is significantly more active in inhibiting HDAC1 compared to the parental HDAC inhibitor CI994. TW9 was more potent in inhibiting tumor cell proliferation compared to (+)‐JQ1, CI994 alone or combined treatment of both inhibitors. Sequential administration of gemcitabine and TW9 showed additional synergistic antitumor effects. Microarray analysis revealed that dysregulation of a FOSL1‐directed transcriptional program contributed to the antitumor effects of TW9. Our results demonstrate the potential of a dual chromatin‐targeting strategy in the treatment of PDAC and provide a rationale for further development of multitarget inhibitors.
This work presents a biochemical, functional and structural characterization of Aquifex aeolicus F1FO ATP synthase obtained using both a native form (AAF1FO) and a heterologous form (EAF1FO) of this enzyme.
F1FO ATP synthases catalyze the synthesis of ATP from ADP and inorganic phosphate driven by ion motive forces across the membrane and therefore play a key cellular function. Because of their central role in supporting life, F1FO ATP synthases are ubiquitous and have been remarkably conserved throughout evolution. For their biological importance, F1FO ATP synthases have been extensively studied for many decades and many of them were characterized from both a functional and a structural standpoint. However, important properties of ATP synthases – specifically properties pertaining to their membrane embedded subunits – have yet to be determined and no structures are available to date for the intact enzyme complex. Therefore, F1FO ATP synthases are still a major focus of research worldwide. Our research group had previously reported an initial characterization of AAF1FO and had indicated that this enzyme presents unique features, i.e. a bent central stalk and a putatively heterodimeric peripheral stalk. Based on such a characterization, this enzyme revealed promising for structural and functional studies on ATP synthases and became the focus of this doctoral thesis. Two different lines of research were followed in this work.
First, the characterization of AAF1FO was extended by bioinformatic, biochemical and enzymatic analyses. The work on AAF1FO led to the identification of a new detergent that maintains a higher homogeneity and integrity of the complex, namely the detergent trans-4-(trans-4’-propylcyclohexyl)cyclohexyl-α-D-maltoside (α-PCC). The characterization of AAF1FO in this new detergent showed that AAF1FO is a proton-dependent, not a sodium ion-dependent ATP synthase and that its ATP hydrolysis mechanism needs to be triggered and activated by high temperatures, possibly inducing a conformational switch in subunit γ. Moreover, this approach suggested that AAF1FO may present unusual features in its membrane subunits, i.e. short N-terminal segments in subunits a and c with implications for the membrane insertion mechanism of these subunits.
Investigating on these unique features of A. aeolicus F1FO ATP synthase could not be done using A. aeolicus cells, because these require a harsh and dangerous environment for growth and they are inaccessible to genetic manipulations. Therefore, a second approach was pursued, in which an expression system was created to produce the enzyme in the heterologous host E. coli. This second approach was experimentally challenging, because A. aeolicus F1FO ATP synthase is a 500-kDa multimeric membrane enzyme with a complicated and still not entirely determined stoichiometry and because its encoding genes are scattered throughout A. aeolicus genome, rather than being organized in one single operon. However, an artificial operon suitable for expression was created in this work and led to the successful production of an active and fully assembled form of Aquifex aeolicus F1FO ATP synthase. Such artificial operon was created using a stepwise approach, in which we expressed and studied first individual subunits, then subcomplexes, and finally the entire F1FO ATP synthase complex. We confirmed experimentally that subunits b1 and b2 form a heterodimeric subcomplex in the E. coli membranes, which is a unique case among ATP synthases of non-photosynthetic organisms. Moreover, we determined that the b1b2 subcomplex is sufficient to recruit the soluble F1 subcomplex to the membranes, without requiring the presence of the other membrane subunits a and c. The latter subunits can be produced in our expression system only when the whole ATP synthase is expressed, but not in isolation nor in the context of smaller FO subcomplexes. These observations led us to propose a novel mechanism for the assembly of ATP synthases, in which first the F1 subcomplex attaches to the membrane via subunit b1b2, and then cring and subunits a assemble to complete the FO subcomplex. Furthermore, we could purify the heterologous ATP synthase (EAF1FO) to homogeneity by chromatography and electro-elution. Enzymatic assays showed that the purified form of EAF1FO is as active as AAF1FO. Peptide mass fingerprinting showed that EAF1FO is composed of the same subunits as AAF1FO and all soluble and membrane subunits could be identified. Finally, single-particle electron microscopy analysis revealed that the structure of EAF1FO is identical to that of AAF1FO. Therefore, the EAF1FO expression system serves as a reliable platform for investigating on properties of AAF1FO.
Specifically, in this work, EAF1FO was used to study the membrane insertion mechanism of rotary subunit c. Subunits c possess different lengths and levels of hydrophobicity across species and by analyzing their N-terminal variability, four phylogenetic groups of subunits c were distinguished (groups 1 to 4). As a member of group 2, the subunit c from A. aeolicus F1FO ATP synthase is characterized by an N-terminal segment that functions as a signal peptide with SRP recognition features, a unique case for bacterial F1FO ATP synthases. By accurately designing mutants of EAF1FO, we determined that such a signal peptide is strictly necessary for membrane insertion of subunit c and we concluded that A. aeolicus subunit c inserts into E. coli membranes using a different pathway than E. coli subunit c. Such a property may be common to other ATP synthases from extremophilic organisms, which all cluster in the same phylogenetic group.
In conclusion, the successful production of the fully assembled and active F1FO ATP synthase from A. aeolicus in E. coli reported in this work provides a novel genetic system to study A. aeolicus F1FO ATP synthase. To a broader extent, it will also serve in the future as a solid reference for designing strategies aimed at producing large multi-subunit complexes with complicated stoichiometry.
Split intein enabled protein trans-splicing (PTS) is a powerful method for the ligation of two protein fragments, thereby paving the way for various protein modification or protein function control applications. PTS activity is strongly influenced by the amino acids directly flanking the splice junctions. However, to date no reliable prediction can be made whether or not a split intein is active in a particular foreign extein context. Here we describe SPLICEFINDER, a PCR-based method, allowing fast and easy screening for active split intein insertions in any target protein. Furthermore we demonstrate the applicability of SPLICEFINDER for segmental isotopic labeling as well as for the generation of multi-domain and enzymatically active proteins.
Background: Novel microscopic techniques which bypass the resolution limit in light microscopy are becoming routinely established today. The higher spatial resolution of super-resolution microscopy techniques demands for precise correction of drift, spectral and spatial offset of images recorded at different axial planes.
Methods: We employ a hydrophilic gel matrix for super-resolution microscopy of cellular structures. The matrix allows distributing fiducial markers in 3D, and using these for drift correction and multi-channel registration. We demonstrate single-molecule super-resolution microscopy with photoswitchable fluorophores at different axial planes. We calculate a correction matrix for each spectral channel, correct for drift, spectral and spatial offset in 3D.
Results and discussion: We demonstrate single-molecule super-resolution microscopy with photoswitchable fluorophores in a hydrophilic gel matrix. We distribute multi-color fiducial markers in the gel matrix and correct for drift and register multiple imaging channels. We perform two-color super-resolution imaging of click-labeled DNA and histone H2B in different axial planes, and demonstrate the quality of drift correction and channel registration quantitatively. This approach delivers robust microscopic data which is a prerequisite for data interpretation.
The isobaric melting and boiling diagrams for the systems: pyridine/methyltrichlorosilane and pyridine/1,1,1-trichloroethane are reproduced. The existence of the congruently melting addition compound CH3SiCl3· (Pyridin)2 could be confirmed. Some measurements of the molar volume of mixtures between pyridine and methyltrichlorosilane and pyridine and 1,1,1-trichloroethane, respectively, are reported. For both systems the molar excess volume and for the system pyridine/methyltrichlorosilane the molar excess enthalpie have been calculated as a function of the mole fractions.
The isobaric melting and boiling diagrams for the systems: dimethyldichlorosilane/pyridine and 2,2-dichloropropane/pyridine are reproduced. The existence of the incongruently melting addition compounds (CH3)2SiCl2 · (Pyridine)2 and [(CH3)2CCl2]3 · Pyridine could be proved. Some measurements of the molar volume of mixtures of pyridine and dimethyldichlorosilane, and pyridine and 2,2-dichloropropane are reported. For both systems the molar excess volume has been calculated as a function of the mole fractions.
The isobaric melting and boiling diagrams for the systems: trimethylchlorosilane/pyridine and trimethylchloromethane/pyridine are reproduced. Some measurements of the molar volume of mixtures between trimethylchlorosilane and pyridine and trimethylchloromethane and pyridine are reported. For both systems the molar excess volume has been calculated as a function of the mole fractions
Site-specific cleavage of RNAs derived from the PIM1 3′-UTR by a metal-free artificial ribonuclease
(2019)
Oligonucleotide conjugates of tris(2-aminobenzimidazole) have been reported previously to cleave complementary RNA strands with high levels of sequence and site specificity. The RNA substrates used in these studies were oligonucleotides not longer than 29-mers. Here we show that ~150–400-mer model transcripts derived from the 3′-untranslated region of the PIM1 mRNA reacted with rates and specificities comparable to those of short oligonucleotide substrates. The replacement of DNA by DNA/LNA mixmers further increased the cleavage rate. Tris(2-aminobenzimidazoles) were designed to interact with phosphates and phosphate esters. A cell, however, contains large amounts of phosphorylated species that may cause competitive inhibition of RNA cleavage. It is thus important to note that no loss in reaction rates was observed in phosphate buffer. This opens the way to in-cell applications for this type of artificial nuclease. Furthermore, we disclose a new synthetic method giving access to tris(2-aminobenzimidazoles) in multigram amounts.
The RNA cleaving catalyst tris(2-aminobenzimidazole) when attached to the 5’ terminus of oligonucleotides cuts complementary RNA strands in a highly site-specific manner. Conjugation was previously achieved by the acylation of an amino linker by an active ester of the catalyst. However, this procedure was low yielding and not reliable. Here, a phosphoramidite building block is described that can be coupled to oligonucleotides by manual solid phase synthesis in total yields around 85%. Based on this chemistry, we have now studied the impact of LNA (locked nucleic acids) nucleotides on the rates and the site-specificities of RNA cleaving conjugates. The highest reaction rates and the most precise cuts can be expected when the catalyst is attached to a strong 5’ closing base pair and when the oligonucleotide contains several LNA units that are equally distributed in the strand. However, when placed in the 5’ position, LNA building blocks tend to diminish the specificity of RNA cleavage.
Nach der Entdeckung und strukturellen Aufklärung des Ribosoms war bekannt, dass neben den Proteinen auch regulatorische RNA Sequenzen für die Steuerung biologischer Prozesse im Organismus verantwortlich sind. Dazu zählt unter anderem das trans-activation responsive element (TAR) aus HIV-1, welches am terminalen 5' Bereich (1-59) aller HIV-1 mRNAs eine identische bulge-loop Struktur ausbildet. Die basale Trans-kription des integrierten HIV Promotors ist in Abwesenheit des viralen trans-activator of transcription (Tat) sehr gering (und abhängig von zellulären Transkriptionsfaktoren). Sobald Tat exprimiert wird, bindet es zusammen mit dem humanen positive trancription elongation factor b (p-TEFb) spezifisch an TAR und aktiviert die Transkriptionsrate des viralen Genoms und die Bildung von volllängen Transkripten drastisch. Die Notwendigkeit der Tat-vermittelten Aktivierung als Grundlage einer funktionierenden HIV Replikation macht dieses System zu einem hoch interessanten Target für eine antivirale HIV Therapie. Basierend auf der Hemmung des Tat/TAR Komplexes wurde in den vergangen Jahren eine Reihe von Verbindungen identifiziert, die zwar in-vitro eine inhibierende Wirkung zeigten, aber keine von ihnen konnte bis jetzt als Therapeutikum Verwendung finden. So wäre die noch ausstehende Entdeckung eines effizienten Tat Antagonisten, der ohne die zelleigene Transkription zu beeinträchtigen eine Reduzierung der Virusreplikation von 80 - 90 % akut infizierter Zellen bewirkt, ein bedeutender Durchbruch in der HIV Forschung. Durch eine längere Behandlung von chronisch infizierten Zellen könnte so die Transkription des viralen Genoms abgeschaltet und dadurch eine Eliminierung latenter HIV Reservoirs ermöglichen werden.
Das Ziel dieser Arbeit war die Entwicklung neuartiger TAR Liganden, zunächst auf Grundlage eines nicht auf Strukturmodellen beruhenden Ligandenscreenings, gefolgt von einem strukturbasierten Ligandendesign. Bei der Suche nach potentiellen Wirkstoffen, beschränkte man die Auswahl der untersuchten Verbindungen auf Guanidin- und Amidinanaloga. Dazu zählten einfache Guanidinderivate mit unterschiedlichen aromatischen Resten sowie heterocyclische Verbindungen, wie Isochinoline, Chinazoline, Perimidine und Phenanthridine. Die Bindungsaffinitäten dieser Wirkstoffkandidaten in Bezug zu TAR wurden über einen FRET Assay nach Matsumoto[1] bestimmt. Eine Auswahl an Verbindungen wurde zudem über eine NMR Titration charakterisiert (AK Schwalbe). Dadurch konnte beobachtet werden, an welcher Position die Liganden mit der TAR RNA in Wechselwirkung treten. Bei diesen Untersuchungen zählten 1,7-
Diaminochinolin (IC50 = 150 µM), 2,4,6-Triaminochinazolin (IC50 = 40 µM) sowie 6,8-Diaminophenanthridin (IC50 = 15 µM) zu den aktivsten Verbindungen.
Um eine Aussage über die Bindungsposen treffen zu können, wurde mittels HF-docking Methoden die Komplexgeometrie energetisch optimiert. Ausgehend von diesen Bindungsmodellen entwickelte man eine Leitstruktur, die als Grundlage eines strukturbasierten Ligandendesigns diente. Im Fokus stand hierbei die Entwicklung einer GC-Basenpaar erkennenden Untereinheit. Mit 3,5-Diamino-9-methyl-3,4,9,10-tetrahydro-1H-pyrrolo[3,4-b]phenanthridin-8(2H)-on (IC50 = 45 µM) konnte ein Ligand identifiziert werden, der im NMR Titrationsexperiment ausschließlich am Basenpaar G26/C39 von TAR eine Verschiebung der Iminoprotonen induzierte. In einem weiteren Projekt versuchte man eine Selektivitätssteigerung durch simultane Adressierung zweier Bindungsstellen zu erreichen. Nachdem im NMR Experiment gezeigt werden konnte, dass 2,4,6-Triaminochinazolin mit hoher Affinität an zwei verschiedenen Bereichen der RNA bindet, wurden eine Reihe dimerer 2,4,6-Triaminochinazolinderivate mit unterschiedlich langen Linkern hergestellt. Mit diesem Ansatz gelang es den hoch affinen Liganden N6,N6'-(1,4-phenylenbis(methylen))bis(chinazolin-2,4,6-triamin) (IC50 = 150 nM) zu identifizieren.
The IR-spectra of BaCO3 (80% 13CO32-, 90% 13CO32-) shows small bands in the ν2-region, which are assigned to short waves of 12CO32--chains with three, five or six carbonate ions.
Modern computational molecular quantum chemical studies, such as the present one, typically employ a wide range of theoretical techniques. The latter are often rather complicated and one should not generally expect that an experimental scientist in the area of physical chemistry, a potential reader of this work, should be familiar with all these techniques. To simplify the reading of the Thesis and to make it self-sufficient, it is supplied with an overview of the employed theoretical methodologies (Chapter 1). The overview explains basic quantum-chemical terminology referred to throughout the Thesis, introduces theoretical foundations of the methods and outlines their properties and limitations. In Part 1.1 of Chapter 1, methods for the solution of the molecular Schrödinger equation are introduced, while in the subsequent Parts 1.2 and 1.3 methods for the solution of the electronic Schrödinger equation are presented to find the ground and excited states, respectively. Part 1.4 is dedicated to basis-set effects which are omnipresent in electronic-structure calculations. It contains a number of unusual insights and concepts proposed by the author and, thus, may be insightful also to experts in quantum chemistry.
In Chapter 2, the phenomenon of acetone-water proton exchange catalyzed by tubular as well as amorphous aggregates of calix[4]hydroquinone (CHQ) macromolecules, which has been observed previously in NMR experiments (Ref. D1D), is investigated by means of correlated quantum-chemical methods. The first part of the study (Section 2.3-2.7) considers concerted proton transfer, assisted by several initially neutral OH-groups in the hydrogen-bonded networks of CHQ aggregates. The second part of the study (Section 2.8-2.13) is dedicated to a second mechanism of proton exchange: step-wise proton transfer via formation of ionic intermediates resulting from CHQ pre-dissociation. CHQ application-specific as well as general conclusions, relevant to the main topic of the Thesis (i.e. influence of specific microsolvation on the considered proton transfer processes), are presented in Section 2.14.
The phenomenon of dual fluorescence observed in clusters of methyl 4-N,N-dimethylaminobenzoate ester (DMABME) and two water molecules in the gas phase, is studied in Chapter 3. Experimentally, the dual fluorescence was detected in experiments combining optical and ground-state ion-depletion infrared spectroscopies in ultracold molecular beams (Ref. D2D). In Section 3.3, calculated ground-state infrared spectra are presented that allow to identify the structures of those isomers, which are present in the gas-phase, as well as the structure of the isomer responsible for dual fluorescence. To further understand the reaction mechanism of dual fluorescence, excited-state potential energy surfaces of the identified isomers were computed along the relevant twisted intermolecular charge-transfer formation coordinate and the mechanism of energy dissipation in these complexes was investigated (Section 3.4-3.5) (Ref. D3D). A brief summary of the main results of this chapter and conclusions are given in Section 3.6. Finally, in Section 3.7 a complementary benchmark study of the quality of ground-state potential energy surfaces of prototypical hydrogen-bonded systems (ammonia-water and formic acid-water dimers) obtained at the level of BSSE-corrected MP2 combined with moderate basis sets, has been conducted. The quality of potential energy surfaces was tested with respect to basis-set size, level of electron correlation and anharmonicity effects and the applied methodology to identify the IR spectrum of hydrated DMABME complexes (Section 3.3) has been found to be sufficient to uniquely assign the IR spectra.
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.
Synaptic vesicle (SV) recycling enables ongoing transmitter release, even during prolonged activity. SV membrane and proteins are retrieved by ultrafast endocytosis and new SVs are formed from synaptic endosomes (large vesicles—LVs). Many proteins contribute to SV recycling, e.g., endophilin, synaptojanin, dynamin and clathrin, while the site of action of these proteins (at the plasma membrane (PM) vs. at the endosomal membrane) is only partially understood. Here, we investigated the roles of endophilin A (UNC-57), endophilin-related protein (ERP-1, homologous to human endophilin B1) and of clathrin, in SV recycling at the cholinergic neuromuscular junction (NMJ) of C. elegans. erp-1 mutants exhibited reduced transmission and a progressive reduction in optogenetically evoked muscle contraction, indicative of impaired SV recycling. This was confirmed by electrophysiology, where particularly endophilin A (UNC-57), but also endophilin B (ERP-1) mutants exhibited reduced transmission. By optogenetic and electrophysiological analysis, phenotypes in the unc-57; erp-1 double mutant are largely dominated by the unc-57 mutation, arguing for partially redundant functions of endophilins A and B, but also hinting at a back-up mechanism for neuronal endocytosis. By electron microscopy (EM), we observed that unc-57 and erp-1; unc-57 double mutants showed increased numbers of synaptic endosomes of large size, assigning a role for both proteins at the endosome, because endosomal disintegration into new SVs, but not formation of endosomes were hampered. Accordingly, only low amounts of SVs were present. Also erp-1 mutants show reduced SV numbers (but no increase in LVs), thus ERP-1 contributes to SV formation. We analyzed temperature-sensitive mutants of clathrin heavy chain (chc-1), as well as erp-1; chc-1 and unc-57; chc-1 double mutants. SV recycling phenotypes were obvious from optogenetic stimulation experiments. By EM, chc-1 mutants showed formation of numerous and large endosomes, arguing that clathrin, as shown for mammalian synapses, acts at the endosome in formation of new SVs. Without endophilins, clathrin formed endosomes at the PM, while endophilins A and B compensated for the loss of clathrin at the PM, under conditions of high SV turnover.
The mfl-riboswitch is a transcriptional off-switch, which down-regulates expression of subunit ß of ribonucleotide reductase in Mesoplasma florum upon 2´-deoxyguanosine binding. We characterized binding of 2´-deoxyguanosine to the mfl-aptamer domain (WT aptamer) and a sequence-stabilized aptamer (MT aptamer) under in vitro and ‘in-cell-like’ conditions by isothermal titration calorimetry (ITC) and nuclear magnetic resonance (NMR) spectroscopy. ‘In-celllike’ environment was simulated by Bacillus subtilis cell extract, in which both aptamers remained sufficiently stable to detect the resonances of structural elements and ligand binding in 2D NMR experiments. Under ‘in-cell-like’-environment, (i) the WT aptamer bound the endogenous metabolite guanosine and (ii) 2´-deoxyguanosine efficiently displaced guanosine from the WT aptamer. In contrast, MT aptamer exhibited moderate binding to 2´-deoxyguanosine and weak binding to guanosine. NMR experiments indicated that binding of guanosine was not limited to the aptamer domain of the riboswitch but also the full-length mfl-riboswitch bound guanosine, impacting on the regulation efficiency of the riboswitch and hinting that, in addition to 2´-deoxyguanosine, guanosine plays a role in riboswitch function in vivo. Reporter gene assays in B. subtilis demonstrated the regulation capacity of the WT aptamer, whereas the MT aptamer with lower affinity to 2´ -deoxyguanosine was not able to regulate gene expression.
A small single molecule with multiple photoswitchable subunits, selectively and independently controllable by light of different wavelengths, is highly attractive for applications in multi-responsive materials and biological sciences. Herein, triple photoswitches are presented consisting of three independent azobenzene (AB) subunits that share a common central phenyl ring: the meta-trisazobenzenes (MTA). It is the unique meta-connectivity pattern leading to decoupling of all azo-subunits although they do overlap spatially. Based on this pattern, we design a triple MTA photoswitch, as proof-of-principle, with three different, electronically independent AB branches on the computer, which can be individually photo-excited to trigger ultra-fast E → Z isomerization at the selected AB branch.
Heme-copper oxidases (HCOs) are the terminal enzymes of the aerobic respiratory chain in the inner mitochondrial membrane or the plasma membrane in many prokaryotes. These multi-subunit membrane protein complexes catalyze the reduction of oxygen to water, coupling this exothermic reaction to the establishment of an electrochemical proton gradient across the membrane in which they are embedded. The energy stored in the electrochemical proton gradient is used e.g. by the FOF1-ATP synthase to generate ATP from ADP and inorganic phosphate. The superfamily of HCOs is phylogenetically classified into three major families: A, B and C. The A-family HCOs, represented by the well-studied aa3-type cytochrome c oxidases (aa3-CcOs), are found in mitochondria and many bacteria. The B-family of HCOs contains a number of bacterial and archaeal oxidases. The C-family comprises only the cbb3-type cytochrome c oxidase (cbb3-CcO) and is most distantly related to the mitochondrial respiratory oxidases.
Das Hauptziel dieser Dissertation lag in der Verbesserung einzelner Schritte im Prozess der automatischen Proteinstrukturbestimmung mittels Kernmagnetischer Resonanz (NMR). Dieser Prozess besteht aus einer Reihe von sequenziellen Schritten, welche zum Teil bereits erfolgreich automatisiert wurden. CYANA ist ein Programmpaket, welches routinemäßig zur automatischen Zuordnung der chemischen Verschiebungen, der Nuclear Overhauser Enhancement (NOE) Signalen und der Strukturrechnung von Proteinen verwendet wird. Einer der Schritte, der noch nicht erfolgreich automatisiert wurde, stellt die Signalidentifizierung von NMR Spektren dar. Dieser Schritt ist besonders wichtig, da Listen von NMR-Signalen Grundlage aller Folgeschritte sind. Fehler in den Signallisten pflanzen sich in allen Folgeschritten der Datenauswertung fort und können am Ende in falschen Strukturen resultieren. Daher war ein Ziel dieser Arbeit, einen robusten und verlässlichen Algorithmus zur Signalidentifizierung von NMR Spektren in CYANA zu implementieren. Dieser Algorithmus sollte mit dem in FLYA implementierten Ansatz zur automatischen Resonanzzuordnung, der automatischen NOE-Zuordnung und der Strukturrechnung mit CYANA kombiniert werden. Der in CYANA implementierte CYPICK Algorithmus ahmt den von Hand durchgeführten Ansatz nach. Bei der manuellen Methode schaut sich der Wissenschaftler zweidimensionale Konturliniendarstellungen der NMR Spektren an und entscheidet anhand verschiedener Geomtrie- und Ähnlichkeitskriterien, ob es sich um ein Signal des Proteins oder um einen Artefakt handelt. Proteinsignale sind ähnlich zu konzentrischen Ellipsen und erfüllen bestimmte geometrische Kriterien, wie zum Beispiel ungefähr kreisförmiges Aussehen nach entsprechender Skalierung der spektralen Achsen und gänzlich konvexe Formen, die Artefakte nicht aufzeigen. CYPICK bewertet die Konturlinien lokaler Extrema nach diesen Bedingungen und entscheidet anhand dieser, ob es sich um ein echtes Signal handelt oder nicht. Das zweite Ziel dieser Arbeit war es ein Maß zur Quantifizierung der Information von strukturellen NMR Distanzeinschränkungen zu entwickeln. Der sogenannte Informationsgehalt (I) ist vergleichbar mit der Auflösung in der Röntgenkristallographie. Ein weiteres Projekt dieser Dissertation beschäftigte sich mit der strukturbasierten Medikamentenentwicklung (SBDD). SBDD wird meist von der Röntgenkristallographie durchgeführt. NMR hat jedoch einige Vorteile gegenüber der Röntgenkristallographie, welche interessant für SBDD sind. Daher wurden Strategien entwickelt, die NMR für SBDD zugänglicher machen sollen.
Nicotinamid-3-desazapurindinucleotid * wurde aus den Teilstücken Nicotinamidmononucleotid und 3-Desazapurinribosid-5'-phosphat durch Kondensation mit Dicyclohexylcarbodiimid in wäßrigem Pyridin hergestellt1. Das Coenzymmodell war im enzymatischen Test mit verschiedenen Dehydrogenasen ebenso wirksam wie Nicotinamid-adenin-dinucleotid. Für die Funktion der Wasserstoffübertragung scheint der Stickstoff N 1 im Purinring von Bedeutung zu sein. Auffällig ist, daß die pK-Werte nichtfunktioneller Mononucleotidteile bei Coenzymmodellen, die Nicotinamid-adenin-dinucleotid im enzymatischen Test ersetzen können, über dem Wert 4 liegen. Das optische Verhalten des Coenzymmodells Nicotinamid-3-desazapurin-dinucleotid ähnelt dagegen nichtpurinhaltigen Coenzymmodellen, die sich bisher alle durch eine geringere Coenzymwirksamkeit auszeichneten. Eine schwächere intramolekulare Wechselwirkung zwischen den Heterocyclen zeichnete sich durch die Verschiebung des Dihydronicotinamid-Absorptionsmaximums in dem kurzwelligen Teil des Spektrums aus. Aus den geringeren intramolekularen Wechselwirkungen lassen sich jedoch keine Rückschlüsse auf die enzymatische Wirksamkeit ziehen. Alle nichtpurinhaltigen hydrierten Coenzymmodelle zeigen keine Änderung der Fluoreszenz nach Enzymzugabe.
1- (2̸.3′.4′-O-Triacetyl-1.β-D-glucopyranosyl) 3-carboxamido-pyridiniumchlorid wird aus α-1-Chlor-2.3.4-O-triacetyl-glucopyranose und Nikotinamid hergestellt. Die freie Hydroxylgruppe in 6-Stellung der Glucose wird mit Phosphoroxychlorid verestert. Durch Acylwanderung entsteht außerdem ein isomeres Produkt. Die Acetylgruppen lassen sich sauer verseifen. Durch Kondensation mit Adenosinmonophosphat erhält man ein Gemisch beider Nikotinamidglucosid-Adenin-Dinucleotid-Isomerer. Die Verbindungen sind trotz hoher Affinität zu nucleophilen Agentien auf Grund der sterischen Konfiguration enzymatisch inaktiv.
The coenzyme analogue nicotinamide 5-iodouracil-dinucleotide was synthesized by condensation of the two mononucleotides with dicyclohexylcarbodiimide in aqueous pyridine. The enzymatic properties of this compound were compared with those of the nicotinamide-uracil-dinucleotide. Both coenzyme analogues reacted slowly when functioning as a hydrogen carrier in enzymatic tests. The properties were similar to those of nicotinamide-benzimidazole-dinucleotide. The difference spectrum between the intact coenzyme analogue and its mononucleotides showed that the intramolecular interaction between the functional and non-functional moiety was smaller than that in NAD. The interaction corresponded to that of nicotinamide-benzimidazole-dinucleotide. The fluorescence excitation spectrum did not show any energy transfer from the non-functional iodouracil to the dihydronicotinamide part of the analogue. Difference spectra between the coenzyme - enzymecomplex and the two isolated components indicated that the unfolded dihydrocoenzyme was bound to the active site of lactate- and alcohol-dehydrogenase, respectively. Furthermore, they showed aromatic interaction of the non-functional part with parts of the protein. Introduction of iodine into the nicotinamide-uracil-dinucleotide did not remarkably alter the behavior of the analogues. As the iodine is bound very strongly to the coenzyme analogue, it may be useful for X-Ray-investigations of the dehydrogenases.
Darstellung und Eigenschaften des Coenzymanalogen Nicotinamid-4-methyl-5-acetyl-imidazol-dinucleotid
(1970)
Kondensation des Quecksilbersalzes von 4-Methyl-5-acetyl-imidazol ** mit 1-Chlor-2.3.5-O-tribenzoyl-ribofuranose liefert das geschützte Ribosid 3. Zur Strukturaufklärung der Verbindung wurde 4-Methyl-5-acetyl-1-(β-D-0-2′.3′.5′-triacetyl-ribofuranosyl)-imidazol mit Methyljodid in das 3.4-Dimethyl-5-acetyl-1-(β-D-O-2′.3′.5′-triacetyl-ribofuranosyl)-imidazoliumjodid überführt und der Zuckerrest hydrolytisch gespalten. Das entstandene Imidazol-Derivat ist identisch mit 1.5-Dimethyl-4-acetyl-imidazol. 4-Methyl-5-acetyl-1- (β-D-ribofuranosyl) -imidazol wurde mit Aceton in das Isopropyliden-Derivat 4 überführt. Die Phosphorylierung zum Nucleosid-5′-phosphat (5) führten wir mit β-Cyanäthyl-phosphat durch. Durch Kondensation mit Nicotinamid-mononucleotid erhielten wir das Coenzymanaloge Nicotinamid-4-methyl-5-acetyl-imidazol-dinucleotid (6). Die Verbindung liegt im oxydierten Zustand in gefaltener Form vor. Das Fluoreszenz-Anregungsspektrum der Dihydroverbindung zeigt keine Energieübertragung vom nichtfunktionellen 4-Methyl-5-acetyl-imidazol-Teil auf den Dihydronicotinamid-Ring. Das Coenzymanaloge weist eine größere Michaelis- Konstante im Test mit Lactat-Dehydrogenase aus Schweineherz *** auf als das natürliche Nicotinamid-adenindinucleotid ***. Die maximale Umsatzzahl ist trotz der schwächeren Bindung vergrößert. Das unterschiedliche Verhalten des Coenzymanalogen 6 gegenüber NAD läßt, neben der π-Bindung des nichtfunktionellen Teils, eine polare Gruppe im aktiven Zentrum des Enzyms vermuten, die die Ausrichtung des Coenzyms im Coenzym-Enzym-Komplex bewirkt.
Dihydronicotinamid-4-methyl-5-acetyl-imidazol-dinucleotid bildet einen fluoreszierenden Komplex mit der Lactat-Dehydrogenase, der dem des NADH-LDH-Komplexes sehr ähnlich ist.
Fluorescense spectra of lactate dehydrogenase * (E.C. 1.1.1.27) were investigated in the presence of the coenzyme fragments dihydronicotinamide mononucleotide and dihydronicotinamide-ribose-5'-pyrophospho- (P2) -5“-ribose. The reduced mononucleotide is enzymatically less active as a hydrogen donor. However, formation of a complex with the enzyme was not observed under the conditions used. All the other substances: dihydronicotinamide-ribose-5'-pyrophospho- (P2) -5“-ribose, dihydronicotinamide- benzimidazole-dinucleotide, dihydronicotinamide-3-desazapurine-dinucleotide and dihydronicotinamide-6-mercaptopurine-dinucleotide form more or less stable complexes with lactate dehydrogenase. The complexes do not markedly differ from the complex formed with the natural cofactor. In all cases spectra indicate change in conformation of the coenzyme by forming the coenzyme-enzyme-complex which has been proposed by VELICK 1 too. The cysteine residues of the lactate dehydrogenase are not essential for binding the coenzyme to the active center; this was shown with mercury blocked enzyme.
Mechanism of Na+-dependent citrate transport from the structure of an asymmetrical CitS dimer
(2015)
The common human pathogen Salmonella enterica takes up citrate as a nutrient via the sodium symporter SeCitS. Uniquely, our 2.5 Å x-ray structure of the SeCitS dimer shows three different conformations of the active protomer. One protomer is in the outside-facing state. Two are in different inside-facing states. All three states resolve the substrates in their respective binding environments. Together with comprehensive functional studies on reconstituted proteoliposomes, the structures explain the transport mechanism in detail. Our results indicate a six-step process, with a rigid-body 31° rotation of a helix bundle that translocates the bound substrates by 16 Å across the membrane. Similar transport mechanisms may apply to a wide variety of related and unrelated secondary transporters, including important drug targets.
CD69 is a transmembrane lectin that can be expressed on most hematopoietic cells. In monocytes, it has been functionally linked to the 5-lipoxygenase pathway in which the leukotrienes, a class of highly potent inflammatory mediators, are produced. However, regarding CD69 gene expression and its regulatory mechanisms in monocytes, only scarce data are available. Here, we report that CD69 mRNA expression, analogous to that of 5-lipoxygenase, is induced by the physiologic stimuli transforming growth factor-β (TGF-β) and 1α,25-dihydroxyvitamin D3 (1α,25(OH)2D3) in monocytic cells. Comparison with T- and B-cell lines showed that the effect was specific for monocytes. CD69 expression levels were increased in a concentration-dependent manner, and kinetic analysis revealed a rapid onset of mRNA expression, indicating that CD69 is a primary TGF-β/1α,25(OH)2D3 target gene. PCR analysis of different regions of the CD69 mRNA revealed that de novo transcription was initiated and proximal and distal parts were induced concomitantly. In common with 5-lipoxygenase, no activation of 0.7 kb or ~2.3 kb promoter fragments by TGF-β and 1α,25(OH)2D3 could be observed in transient reporter assays for CD69. Analysis of mRNA stability using a transcription inhibitor and a 3′UTR reporter construct showed that TGF-β and 1α,25(OH)2D3 do not influence CD69 mRNA stability. Functional knockdown of Smad3 clearly demonstrated that upregulation of CD69 mRNA, in contrast to 5-LO, depends on Smad3. Comparative studies with different inhibitors for mitogen activated protein kinases (MAPKs) revealed that MAPK signalling is involved in CD69 gene regulation, whereas 5-lipoxygenase gene expression was only partly affected. Mechanistically, we found evidence that CD69 gene upregulation depends on TAK1-mediated p38 activation. In summary, our data indicate that CD69 gene expression, conforming with 5-lipoxygenase, is regulated monocyte-specifically by the physiologic stimuli TGF-β and 1α,25(OH)2D3 on mRNA level, although different mechanisms account for the upregulation of each gene.
Virus-infected cells are eliminated by cytotoxic T lymphocytes, which recognize viral epitopes displayed on major histocompatibility complex class I molecules at the cell surface. Herpesviruses have evolved sophisticated strategies to escape this immune surveillance. During the lytic phase of EBV infection, the viral factor BNLF2a interferes with antigen processing by preventing peptide loading of major histocompatibility complex class I molecules. Here we reveal details of the inhibition mechanism of this EBV protein. We demonstrate that BNLF2a acts as a tail-anchored protein, exploiting the mammalian Asna-1/WRB (Get3/Get1) machinery for posttranslational insertion into the endoplasmic reticulum membrane, where it subsequently blocks antigen translocation by the transporter associated with antigen processing (TAP). BNLF2a binds directly to the core TAP complex arresting the ATP-binding cassette transporter in a transport-incompetent conformation. The inhibition mechanism of EBV BNLF2a is distinct and mutually exclusive of other viral TAP inhibitors.
Nep1 (Emg1) is a highly conserved nucleolar protein with an essential function in ribosome biogenesis. A mutation in the human Nep1 homolog causes Bowen–Conradi syndrome—a severe developmental disorder. Structures of Nep1 revealed a dimer with a fold similar to the SPOUT-class of RNA-methyltransferases suggesting that Nep1 acts as a methyltransferase in ribosome biogenesis. The target for this putative methyltransferase activity has not been identified yet. We characterized the RNA-binding specificity of Methanocaldococcus jannaschii Nep1 by fluorescence- and NMR-spectroscopy as well as by yeast three-hybrid screening. Nep1 binds with high affinity to short RNA oligonucleotides corresponding to nt 910–921 of M. jannaschii 16S rRNA through a highly conserved basic surface cleft along the dimer interface. Nep1 only methylates RNAs containing a pseudouridine at a position corresponding to a previously identified hypermodified N1-methyl-N3-(3-amino-3-carboxypropyl) pseudouridine (m1acp3-Psi) in eukaryotic 18S rRNAs. Analysis of the methylated nucleoside by MALDI-mass spectrometry, HPLC and NMR shows that the methyl group is transferred to the N1 of the pseudouridine. Thus, Nep1 is the first identified example of an N1-specific pseudouridine methyltransferase. This enzymatic activity is also conserved in human Nep1 suggesting that Nep1 is the methyltransferase in the biosynthesis of m1acp3-Psi in eukaryotic 18S rRNAs.
The synergetic effects of combining structural biology and epr spectroscopy on membrane proteins
(2017)
Protein structures as provided by structural biology such as X-ray crystallography, cryo-electron microscopy and NMR spectroscopy are key elements to understand the function of a protein on the molecular level. Nonetheless, they might be error-prone due to crystallization artifacts or, in particular in case of membrane-imbedded proteins, a mostly artificial environment. In this review, we will introduce different EPR spectroscopy methods as powerful tools to complement and validate structural data gaining insights in the dynamics of proteins and protein complexes such that functional cycles can be derived. We will highlight the use of EPR spectroscopy on membrane-embedded proteins and protein complexes ranging from receptors to secondary active transporters as structural information is still limited in this field and the lipid environment is a particular challenge.
1. Fab co-complexes of proton pumping NADH:ubiquinone oxidoreductase (complex I) Fab fragments suitable for co-crystallization with complex I were generated using an immobilized papainbased protocol. The binding of the antibody fragments to complex I was verified using Surface Plasmon Resonance and size exclusion chromatography. The binding constants of the antibodies and their respective Fab fragments were found to be in the nanomolar range. This work presents the first report on successful crystallization of complex I (proton pumping NADH:ubiquinone oxidoreductase) from Yarrowia lipolytica with proteolytic Fab fragments. The quality of the crystals was significantly improved when compared to the initial experiments and the best crystals diffracted X-rays to a resolution of ~7 Å. The activity of complex I remained uninfluenced by antibody fragment binding. The initial diffraction data suggest that the complex I/Fab co-complex crystals represent a space group different to the one observed for the native protein. Ongoing experiments are aimed at further enhancements of the diffraction quality of the crystals. Providing a different space group the CI/Fab co-complexes may become a very useful approach for structure determination of the enzyme. Moreover, the bound Fab offers an additional possibility to generate phase information. The antibody-mediated crystallization represents a valuable tool in structural characterization of the NADH:oxidoreductase subcomplexes or even single subunits. 2. UDP-glucose pyrophosphorylase UDP-glucose pyrophosphorylase from Yarrowia lipolytica displays affinity towards Ni2+ NTA and was first detected in a contaminated sample of complex I. Following, separation from complex I, Ugp1p was purified using anion exchange chromatography. Sequence similarity studies revealed high identity to other known pyrophosphorylases. As indicated by laser-based mass spectrometry method (LILBID) Ugp1p from Y. lipolytica builds octamers similarly to the enzyme from Saccharomyces cerevisiae. The initial crystals grew as thin needles favorably in sitting drop setups. The size of the crystals was increased by employment of a micro batch technique. The improved crystals diffracted X-rays to a resolution of 3.2 Å at the synchrotron beamline. Structural characterization is under way using a molecular replacement approach based on the published structure of baker’s yeast UGPase.
Die Arachidonsäurekaskade spielt bei Entzündungsprozessen und der Schmerzentstehung eine wichtige Rolle. Deren primäre Produkte, die Leukotriene und die Prostaglandine, sind entzündungsfördernde Mediatoren und nehmen Einfluss auf den Entzündungs-auflösendenprozess und sind bei einer Dysregulation für diverse Erkrankungen wie z.B. Asthma bronchiale und allergische Rhinitis mitverantwortlich. Die Kaskade gliedert sich mit ihren beiden Hauptenzymen, Cyclooxygenase und 5-Lipoxygenase (5-LO), in zwei Wege auf. Beide Enzyme sind außerdem in der Lage entzündungsauflösenden Mediatoren zu bilden. Die Mediatoren wie z.B. Lipoxin können im Zellstoffwechsel einerseits über die Lipoxygenase-Route, oder andererseits wie „aspirin-triggered“-Lipoxin von der durch geeignete Wirkstoffe acetylierten Cyclooxygenase-2 (COX-2) katalysiert werden. Diese Mediatoren werden benötigt, um (chronische) Entzündungen und beschädigtes Gewebe zurück zur Homöostase zu führen.
Die Pharmakotherapie chronisch entzündlicher Erkrankungen mit guter Wirksamkeit und verträglichem Profil bei Langzeiteinnahme stellt jedoch eine Herausforderung dar. Die Therapie verzögern oft, z. B bei Einnahme von nicht-steroidalen Antirheumatika (NSAR), die Entzündungsauflösung, da die Bildung von entzündungshemmenden und entzündungs-auflösenden Lipidmediatoren gehemmt werden. Die gezielte Modulation und Einflussnahme auf die Arachidonsäurekaskade an einem der beiden Enzyme, stellt daher einen guten Ansatz für eine verbesserte Therapiemöglichkeit von (chronischen) entzündlichen Krankheiten dar. Diese Arbeit beschäftigt sich mit der Synthese von Modulatoren und Inhibitoren der Arachidonsäurekaskade. Zum einen befasst sie sich mit der Entwicklung von irreversiblen COX-2-acetylierenden Substanzen als neues anti-entzündliches und entzündungsauflösendes Prinzip. Zum anderen mit der Untersuchung der Struktur-Wirkungsbeziehung (SAR) von 2-Aminothiazolen als direkte 5-LO-Inhibitoren ausgehend von SKI-II, welches zuvor als Leitstruktur zur Entwicklung von 5-LO-Inhibitoren entdeckt wurde.
Als Leitstrukturen für die irreversiblen COX-2-acetylierenden Substanzen wurden bekannte COX-2 selektive Substanzen ausgewählt sowie vereinzelte nicht-selektive NSAR. Es wurden an der COX-2 Kristallstruktur Docking-Studien durchgeführt, um die geeignetsten Positionen für die Einführung einer (labilen) Acetylgruppe zu identifizieren. Aufgrund dieser Studien wurden drei Positionen ausgewählt zur Derivatisierung. Es wurden daraufhin zahlreiche Derivate synthetisiert von Celecoxib, Valdecoxib, Rofecoxib, Etericoxib, als Vertreter der (COX-2) selektive Inhibitoren, sowie von Acetylsalicylsäure, Diclofenac und Nimesulid-Analoga als Vertreter der nicht-selektiven NSARs. Zusätzlich wurden Derivate synthetisiert mit Michael-Akzeptoren als kovalente bindende Komponente. Alle synthetisierten Substanzen wurden sukzessiv auf ihre COX inhibitorischen Eigenschaften hin untersucht und auf COX-2 Selektivitäten überprüft. Weiterhin wurden von allen Derivaten Auswaschungs-Studien durchgeführt als Vorversuche welche Derivate eine irreversible COX-2-Inhibition hervorrufen. In den Vorversuchen zeigte die Verbindung ST-1650 am deutlichsten eine COX-2-Selektivität sowie eine starke irreversible Inhibition der COX-2. Die Verbindung ST-1650 wurde weiterhin auf indirekte Hinweise zur Entstehung von heilungsfördernden Mediatoren untersucht anhand von: M1-Macrophagen Polarisation und einem Schmerzmodell, dem Zymosan-Überempfindlichkeit Pfotenmodell. Im Makrophagen-Modell konnte ST-1650 keine Phänotypverschiebung hinzu entzündungsauflösenden M2-Makrophagen bewirken, sowie in den Schmerzmodellen leider keine schnellere Schmerzauflösung als die Kontrollgruppe. Ob diese Effekte durch mangelnde oder zu geringer Entstehung von entzündungshemmenden Mediatoren zurückzuführen ist, ist noch unklar.
Für die SAR der 2-Aminothiazole als direkte 5-LO-Inhibitoren wurden über 60 Verbindungen synthetisiert und untersucht. Zu Beginn erfolgte eine Optimierung der Grundstruktur als 5-LO-Inhibitor. Es wurden die Einflüsse der Substituenten des Thiazolsrings und des Aminolinkers auf die 5-LO-Aktivität ermittelt, um die SAR initialer Arbeiten zu vertiefen. Nach der SAR-Untersuchung im intakten Zellsystem konnten durch Kombination bevorzugter Strukturelemente die zwei Verbindungen ST-1853 und ST-1906, als neue potente 5-LO-Inhibitoren entwickelt werden, die sich als nicht-toxisch herausstellten. Diese beiden 5-LO-Inhibitoren wirken um einen Faktor 10 potenter und sind weniger toxisch verglichen mit der Leitstruktur SKI-II. ST-1853 wurde innerhalb der Arachidonsäurekaskade auch auf Off-targets getestet, deren Aktivitäten sie erst bei 100-fach höherer Konzentration beeinflusst, sowie in humanem Vollblut, wo sie sich ihre 10-fach bessere Wirksamkeit im Vergleich zu SKI-II bestätigte. Darüber hinaus erwies sich ST-1853 bei den ersten Überprüfungen seiner Stabilität unter physiologischen Bedingungen wie bei der in vitro Metabolisierung durch Rattenlebermikrosomen als ausreichend stabil und daher zur weiteren Charakterisierung gut geeignet.
The transporter associated with antigen processing (TAP)-like (TAPL, ABCB9) belongs to the ATP-binding cassette transporter family, which translocates a vast variety of solutes across membranes. The function of this half-size transporter has not yet been determined. Here, we show that TAPL forms a homodimeric complex, which translocates peptides across the membrane. Peptide transport strictly requires ATP hydrolysis. The transport follows Michaelis-Menten kinetics with low affinity and high capacity. Different nucleotides bind and energize the transport with a slight predilection for purine bases. The peptide specificity is very broad, ranging from 6-mer up to at least 59-mer peptides with a preference for 23-mers. Peptides are recognized via their backbone, including the free N and C termini as well as side chain interactions. Although related to TAP, TAPL is unique as far as its interaction partners, transport properties, and substrate specificities are concerned, thus excluding that TAPL is part of the peptide-loading complex in the classic route of antigen processing via major histocompatibility complex class I molecules.
Analyse und Vorhersage von Kristallstrukturen tetraederförmiger Moleküle und fehlgeordneter Phasen
(2012)
Die Kristallstrukturen tetraederförmiger EX4-Moleküle mit E = C, Si, Ge, Sn, Pb und X = F, Cl, Br, I konnten in sieben Strukturtypen eingeteilt werden. In fast allen Verbindungen nehmen die Halogenatome eine verzerrte Kugelpackung (ccp, hcp, bcc, cp) ein. Die E-Atome besetzen in den dichtesten Kugelpackungen 1/8 aller Tetraederlücken, wobei sich für diese Atome ebenfalls eine Anordnung wie für verzerrte Kugelpackungen ergibt (cp, ccp, hcp). In den anderen Fällen (bcc, cp für die Anordnung der Halogenatome) ergibt sich für die Anordnung der E-Atome selbst ebenfalls eine verzerrte Kugelpackung (bcc, s). Dabei steht s für die Anordnung der E-Atome analog der Schwefelatome im Pyrit (FeS2). Jeder Strukturtyp unterscheidet sich in der Art der kürzesten Halogen-Halogen-Wechselwirkungen. Die in der Literatur für halogenierte organische Verbindungen beschriebenen Typen der Wechselwirkung lassen sich auch bei den EX4-Verbindungen finden. Die E-X-X-Winkel liegen in einem Bereich von 80-100° und 130-160° und sind damit etwas kleiner als für die halogenierten organischen Verbindungen. Mit Hilfe von Gitterenergieminimierungen konnten diverse potentielle Polymorphe für die EX4-Verbindungen vorhergesagt werden.
Eine vollständige Kristallstrukturvorhersage wurde für SiBr4 durchgeführt. Für diese Vorhersage wurden die Van-der-Waals-Parameter neu bestimmt. Dazu wurde das Br-Br-Potential mit Hilfe von Vergleichsrechnungen an den beiden experimentellen Strukturen des GeBr4 in den Raumgruppentypen Pa3, Z = 8 (s/ccp), und P21/c, Z = 4 (hcp/hcp), optimiert. Für die Vorhersage des SiBr4 konnten zwei der vorhergesagten Strukturen durch extern durchgeführte Kristallisationsexperimente bestätigt werden. Eine Hochtemperaturmodifikation kristallisiert oberhalb von 168K im Raumgruppentyp Pa3, Z = 8 im Strukturtyp s/ccp. Diese Struktur konnte bei der Vorhersage auf Rang 9 gefunden werden. Die Tieftemperaturmodifikation, die unterhalb von 168K vorliegt, kristallisiert im Raumgruppentyp P21/c, Z = 4 (Strukturtyp hcp/hcp). Diese Struktur hat Rang 4 der Vorhersage. Die vorhergesagten und experimentellen Strukturen zeigen nur geringe Abweichungen voneinander.
Für die tetraederförmigen E(CH3)4-Moleküle wurden für Tetramethylsilan und Tetramethylgerman vollständige Kristallstrukturvorhersagen durchgeführt. Die energetisch günstigste Struktur ist für beide Verbindungen im Raumgruppentyp Pa3 mit Z = 8 zu finden. Die energetisch zweitgünstigste Struktur hat den Raumgruppentyp Pnma mit Z = 4. Für Tetramethylsilan konnten die Strukturen mit Rang 1 und 2 experimentell bestätigt werden. Eine Hochdruckmodifikation des Tetramethylsilans kristallisiert im Raumgruppentyp Pa3 mit Z = 8. Diese Struktur entspricht der berechneten energetisch günstigsten Struktur auf Rang eins. Ihr konnte der Strukturtyp s/ccp zugeordnet werden. Mit Tieftemperatur-Röntgenpulverbeugungsexperimenten konnte eine Tieftemperaturmodifikation bei T = 100 K im Raumgruppentyp Pnma, Z = 4, mit Strukturtyp ccp/hcp gefunden werden.
Gitterenergieberechnungen wurden für die Strukturanalysen von drei fehlgeordneten Phasen eingesetzt. Experimentell bestimmte Kristallstrukturen von Azulen und Pigment Red 194 haben den Raumgruppentyp P21/c, Z = 2. Die Moleküle befinden sich dabei auf einer Punktlage mit Inversionssymmetrie. Da beide Moleküle kein Inversionszentrum aufweisen, kommt es zu einer Orientierungsfehlordnung. Für die rechnerische Analyse der Fehlordnung wurden jeweils sechs geordnete Modelle ausgehend von den fehlgeordneten Strukturen erstellt, die möglichst wenige Moleküle pro Elemenarzelle aufweisen sollten. Gitterenergieberechnungen und die Auswertung der Boltzmann-Verteilung zeigten, dass in bei beiden Kristallstrukturen eine statistische Fehlordnung der Moleküle vorliegt, die sich aus mehreren geordneten Modellen aufbauen lässt. Bei Azulen ist eine geordnete Struktur im Raumgruppentyp Pa, Z = 4, energetisch etwas günstiger als die anderen Modell. Für Pigment Red 194 zeigte sich, dass die Fehlordnung unter der Annahme, dass nur die berechneten Modelle die fehlgeordnete Struktur bilden, mit über 99%iger Wahrscheinlichkeit aus den vier energetisch günstigsten Modellen Pc, Z = 2, P21, Z = 2, P21/c, Z = 4 und Pc, Z = 4 besteht.
Die dritte untersuchte fehlgeordnete Struktur ist die des Natrium-p-chlorphenylsulfonat-Monohydrats. Die Fehlordnung bezieht sich hier nur auf die Phenylringe, die dort mit einer Besetzung von 50% zueinander senkrecht stehen. Mit Hilfe der Order-Disorder-Theorie konnten zwei geordnete Modelle im Raumgruppentyp P21/c und ein weiteres geordnetes Modell im Raumgruppentyp C1c1 (Z = 16, Z'= 2) aufgestellt werden. Gitterenergieminimierungen dieser Modelle zeigten, dass sich die Fehlordnung statistisch aus allen drei Modellen zusammensetzt. Das energetisch günstigste geordnete Modell im Raumgruppentyp P21/c, Z = 8 (Z' = 2), konnte als verzwillingte Struktur aus Einkristalldaten bestätigt werden.
Lactate dehydrogenase from pig heart is inactivated by the NAD+ -analog P1-N6-(4-azidophenylethyl)adenosine-P2-[4-(3-azidopyridinio)butyl]diphosphate (6) upon irradiation with UV light of wavelengths in the range from 300 to 380 nm. The decrease in enzyme activity can be prevented by the addition of NAD+ and oxalate. The modified enzyme shows a reduced binding capacity for its coenzyme as compared to native lactate dehydrogenase. The amount of incorporated coenzyme is deduced from the ribose content of inactivated enzyme. Tryptic digestion of the modified protein and separation of the peptides by HPLC yields 5 ribose-containing fractions. One of them, fraction 6 6 , is split by treatment with nucleotide pyrophosphatase into two subfractions, 63 and 58. Only subfraction 63 contains ribose. Whereas peptide 58 shows a UV absorption spectrum similar to that of 4-(3-aminopyridinio)-butyl phosphate (3). Amino acid analyses of the peptides indicate that the inactivator forms covalent bonds with different parts of the protein: Peptide 63 is characterized by a great portion of hydrophobic amino acids whereas peptide 58 shows a high degree of hydrophilicity.
Sulfhydryl Groups, Methylmercury Containing Inactivator, Coenzyme Analogue Nicotinamide-(S-methylmercury-thioinosine) dinucleotide was formed by reaction of nicotin amide-(6-thiopurine) dinucleotide with methylmercury chloride. The compound exhibits coenzyme properties in the test with LDH (Km=1.5 × 10-4 м , Vmax=12500) and LADH (Km=1.7 × 10-4 м, Vmax=27) and inactivates YADH and GAPDH. From incubations with LDH and LADH the mercury containing coenzyme could be regained by column chromatography. The compound seems to be qualified for the X-ray structure analysis of the coenzyme-enzyme complex for some dehyrogenases based on the proportion of the heavy metal.
Photoelectron (PE) spectra of ethylene and vinylene carbonates and thiocarbonates as well as of methylene trithiocarbonate and some open-chain derivatives are reported.
The low energy bands, well separated in the unsaturated compounds, are assigned to lone pair and π type ionizations. The assignment is based on comparison of PE spectra, modified CNDO calculations, and sulfur Κβ emission spectra. The pronounced substituent effects due to which the first ionization potential varies from 8.4 eV to 11.1 eV are discussed.
To investigate the contribution of hydrophobic residues to the molecular recognition of cytochrome c with cytochrome oxidase, we mutated several hydrophobic amino acids exposed on subunit II of the Paracoccus denitrificans oxidase. KM and kcat values and the bimolecular rate constant were determined under steady- or presteady-state conditions, respectively. We present evidence that Trp-121 which is surrounded by a hydrophobic patch is the electron entry site to oxidase. Mutations in this cluster do not affect the binding of cytochrome c as the KM remains largely unchanged. Rather, the kcat is reduced, proposing that these hydrophobic residues are required for a fine tuning of the redox partners in the initial collisional complex to obtain a configuration optimal for electron transfer.