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Lineare sowie zyklische 3-Alkylpyridinalkaloide sind vor allem in Schwämmen der Ordnung Haplosclerida, zu der auch Haliclona viscosa zählt, weit verbreitet. Die Synthese der zuvor von C. Volk isolierten Haliclamine C und D, des Viscosamins und des Viscosalin C bildete den Ausgangspunkt dieser Arbeit.[1-4] Sie erfolgte ausgehend von den bekannten Synthesen der Cyclostellettamine und Haliclamine[5-7] und gliedert sich in drei Abschnitte: erstens Synthese eines ω-Hydroxyalkylpyridins aus einem Bromalkohol, zweitens Funktionalisierung der Monomere in Abhängigkeit der gewählten Methode zur Di- bzw. Trimerisierung und drittens Verknüpfung und gegebenenfalls Zyklisierung. Durch Anwendung und Weiterentwicklung der bekannten Synthesewege wurden so insgesamt 14 lineare Monomere, zwei zyklische Monomere, 16 Cyclostellettamine, zwei Isocyclostellettamine, sieben Haliclamine, fünf Viscosaline sowie Viscosamin[8] und ein Analogon mit Heptylkette hergestellt. Dieser synthetische Zugang ermöglichte es, sowohl den finalen Strukturbeweis für die zuvor isolierten Verbindungen zu erbringen, als auch durch die Analyse der Fragmentierungs-muster von synthetischen und natürlichen Verbindungen mehr über das Verhalten dieser Verbindungen unter MS-Bedingungen zu erfahren. Die so gewonnenen Erkenntnisse führten dazu, dass drei unbekannte Verbindungen ohne Isolierung der Reinsubstanz mit einer Kombination von MS- und HPLC-Daten identifiziert werden konnten. So konnten das erste monozyklische 3-Alkylpyridinalkaloid marinen Ursprungs und zwei neue Haliclamine identifiziert und synthetisiert werden Des Weiteren gelang es, für die von C. Volk isolierten, jedoch nicht identifizierten Verbindungen Strukturen zu ermitteln bzw. auf Grund der MS-Daten Strukturvorschläge zu machen. Die durch den synthetischen Zugang große Anzahl verfügbarer 3-Alkylpyridinalkaloide ermöglichte außerdem eine systematische Untersuchung über den Zusammenhang von biologischer Aktivität und Struktur. Die Ergebnisse der am Helmholtz Institut für Infektionsforschung durchgeführten Experimente zu den antibakteriellen sowie cytotoxischen Eigenschaften von natürlichen wie auch rein synthetischen 3-Alkylpyridinalkaloiden zeigten, dass die Aktivität sich schon beim Addieren bzw. Subtrahieren einer Methylengruppe in einer Alkylkette signifikant ändert. [1] C. A. Volk, M. Köck, Org. Lett. 2003, 5, 3567-3569. [2] C. A. Volk, M. Köck, Org. Biomol. Chem. 2004, 2, 1827-1830. [3] C. A. Volk, H. Lippert, E. Lichte, M. Köck, Eur. J. Org. Chem. 2004, 3154-3158. [4] C. A. Volk, Dissertation, Johann Wolfgang Goethe Universität (Frankfurt am Main), 2004. [5] A. Grube, C. Timm, M. Köck, Eur. J. Org. Chem. 2006, 1285-1295 und Referenzen darin. [6] J. E. Baldwin, D. R. Spring, C. E. Atkinson, V. Lee, Tetrahedron 1998, 54, 13655-13680. [7] A. Kaiser, X. Billot, A. Gateau-Olesker, C. Marazano, B. C. Das, J. Am. Chem. Soc. 1998, 120, 8026-8034. [8] C. Timm, M. Köck, Synthesis 2006, 2580-2584.
Cytochrome b561 (cyt b561) proteins are members of the recently identified eukaryotic ascorbate reducible protein family named CYBASC (CYtochrome B, ASCorbate reducible). CYBASC proteins are di-heme-b-containing membrane proteins that catalyze the transmembrane electron transfer from ascorbate. The function of the CYBASC proteins has been correlated with ascorbate recycling and/or iron facilitation uptake. Therefore, investigations on this family are of great interest as ascorbate is one of the most powerful antioxidants and iron is essential for cell survival both in animals and plants. As the amino acid sequence conservation of animal and plant CYBASC proteins is relatively high, all CYBASC members are proposed to share the same structural motifs. However, no three-dimensional structure of any representative member of the CYBASC family has been determined to date. In the Arabidopsis thaliana (A. thaliana) genome, two complete putative CYBASC open reading frames (ORFs), artb561-a and artb561-b were identified. In this thesis, these two A. thaliana CYBASC ORFs, encoding for Acytb561-A and Acytb561-B proteins respectively, were investigated and obtained main results are listed. 1. A. thaliana CYBASC proteins were heterologously produced in Pichia pastoris and Escherichia coli and purified by a single-step immobilized metal affinity chromatography (IMAC). To facilitate detection and purification, the recombinant A. thaliana CYBASC proteins were produced in both expression systems with the histidine affinity tag. Pure and stable preparations of the cytochromes were obtained via a single-step IMAC in sufficient amounts to perform biochemical characterizations. 2. Detergent solubilized recombinant Acytb561-A and Acytb561-B are dimers. As previously suggested for other CYBASC proteins, analytical gel filtration experiment suggested that both detergent solubilized cytochromes are dimers. 3. Spectroscopic features of Acytb561-B differed from those of previously described bovine chromaffin granule cyt b561. A distinctive feature of the first identified CYBASC protein, the cyt b561 from bovine chromaffin vesicles of adrenal medulla (Bcytb561-CG), is that its differential visible absorbance spectra (visible-spectra) revealed an asymmetric α-band with a maximum at 562 nm and a clear shoulder at 557 nm. This feature was recently used to discriminate CYBASC proteins from not-CYBASC proteins. However, in this thesis, it is shown for the first time that not all CYBASC proteins display in their reduced-minus-oxidized visible-spectra an asymmetric α- band and therefore, this feature can not be used as a discriminating CYBASC characteristic. 4. Ascorbate dependent reduction of the A. thaliana CYBASC proteins is inhibited by diethylpyrocarbonate (DEPC). As previously reported for the Bcytb561-CG, the ascorbatedependent reduction of the A. thaliana CYBASC proteins was inhibited by DEPC treatment. In addition, the ‘ascorbate protectant’ effect against DEPC that was observed on the Bcytb561-CG was also observed on the Acytb561-A and Acytb561-B proteins. Furthermore, as the physiological electron donor of all CYBASC proteins is supposed to be ascorbate, ascorbate-affinity of Acytb561- A and Acytb561-B was monitored and was found to be in the same range of the one of the Bcytb561- CG. 5. A. thaliana CYBASC proteins are Fe3+-chelate reductases. Recently, the Fe3+-chelate reductase activity of various CYBASC proteins was presented. In this thesis, it is shown that also both A. thaliana CYBASC proteins reduced Fe3+-chelates such as Fe3+-EDTA and Fe3+-citrate. Consistently, heme potentiometric reductive-oxidative titration of purified Acytb561-A and Acytb561-B indicated that the midpoint potential of the two heme centres of both cytochromes was lower than the one of those Fe3+-chelates. The values of both heme centre potentials of Acytb561-A and Acytb561-B are also consistent with the observation that both cytochromes were only partially reducible by ascorbate and were fully reduced with the non-physiological reductant Na-dithionite. In summary, this work describes the heterologous production, purification and initial characterizations of two distinct CYBASC proteins from A. thaliana: Acytb561-A and Acytb561-B. Biochemical characterization of these cytochromes showed that the shape of the α-band in the differential spectra is not a discriminating factor for CYBASC proteins but it is likely the DEPC sensitivity and the Fe3+-chelate reductase activity. Establishment of a purification strategy to obtain sufficient amounts of monodispersed and stable A. thaliana CYBASC proteins has also enabled initial screening of three dimensional crystallization conditions which are a prerequisite for a deeper understanding of this new eukaryotic redox enzyme family.