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Der Cytochrom-bc1-Komplex katalysiert die Elektronenübertragung von Ubihydrochinon auf Cytochrom c in der Atmungskette und in der bakteriellen Photosynthese. Das Enzym stellt somit das Bindeglied zwischen den Ubihydrochinon bildenden Dehydrogenasen und der Cytochrom c oxidierenden Cytochrom-c-Oxidase dar. Im Rahmen der vorliegenden Arbeit wurden die Wechselwirkungen des Cytochrom-bc1-Komplexes aus Saccharomyces cerevisiae mit seinen Substraten Ubichinon und Cytochrom c sowie mit Phospholipiden der inneren Mitochondrienmembran untersucht. Durch Analyse von Gesamtlipidextrakten aus Proben des Cytochrom-bc1-Komplexes konnte gezeigt werden, daß das Enzym in Anwesenheit von vier verschiedenen Phospholipiden gereinigt und kristallisiert werden kann. In der Kristallstruktur des Enzyms bei 2,3 Å Auflösung wurden fünf Bindungsstellen für Phospholipide und eine Bindungsstelle für ein Detergensmolekül identifiziert. Die Bindungsstelle für eines der Phospholipide, ein Cardiolipin-Molekül, liegt am Eingang eines von zwei Protonierungspfaden für die Ubichinon-Reduktionsstelle (Qi-Bindungsstelle). Ein Phosphatidylinosit-Molekül befindet sich in einer außergewöhnlichen Position unweit der flexiblen "Linker"-Region des Rieske Eisen-Schwefel-Proteins und trägt vermutlich zur Stabilisierung dieser katalytischen Untereinheit bei. Durch Röntgenbeugung an Kokristallen bestehend aus Cytochrom-bc1-Komplex und gebundenem Cytochrom c konnte die dreidimensionale Struktur dieses transienten Enzym-Substrat-Komplexes bei 2,97 Å ermittelt werden. Die Kristallstruktur ist die erste Struktur des Cytochrom c im Komplex mit einem seiner beiden Redoxpartner aus der Atmungskette. Sie zeigt, daß das Cytochrom c hauptsächlich durch hydrophobe Wechselwirkungen an das Cytochrom c1 bindet und daß die Nähe der beiden c-Typ Hämgruppen eine schnelle Reduktion des Cytochrom c erlaubt. Im homodimeren Cytochrom-bc1-Komplex ist nur eine der beiden Bindungsstellen für Cytochrom c besetzt. Diese hälftige Substratbindung zeigte sich auch für das Ubichinon in der Qi- Bindungsstelle und weist darauf hin, daß die beiden Monomere des Enzyms unabhängig voneinander oder sequentiell arbeiten können. Möglicherweise dient dies der Regulation der Enzymaktivität des Cytochrom-bc1-Komplexes. Durch partielle Reduktion des Cytochrom-bc1-Komplexes in Anwesenheit von Ubichinon konnte ein proteingebundenes Ubisemichinonradikal erzeugt und durch Schockgefrieren stabilisiert werden. Die spektralen Eigenschaften dieses Radikals sind typisch für ein Ubisemichinon an der Qi-Bindungsstelle. Durch Spektroskopie an einer Probe, die einem Wasserstoff/Deuterium-Austausch unterzogen wurde, konnte gezeigt werden, daß dieses Radikal von Protonen koordiniert wird, die mit dem Solvens im Austausch stehen. Dies steht in Übereinstimmung mit der Theorie des Q-Zyklus und wurde durch die hochauflösenden Kristallstruktur des Enzyms bei 2,3 Å vorhergesagt. Die erzielten Ergebnisse zeigen neue Informationen zum Wechselspiel des Cytochrom- bc1-Komplexes mit Phospholipiden aus der inneren Mitochondrienmembran. Die Bestimmung der Struktur des transienten Komplexes bestehend aus Enzym und Cytochrom c erweitert das Bild über den Elektronentransfer durch Cytochrom c zwischen dem Cytochrom-bc1-Komplex und der Cytochrom-c-Oxidase. Das mögliche Zusammenwirken der Bindungstellen für Cytochrom c und Ubichinon ist ein neuer mechanistischer Aspekt, der auf eine Regulation der Enzymaktivität schließen läßt.
The cytochrome bc1 complex or ubiquinol:cytochrome c oxidoreductase (QCR) catalyses electron transfer from ubiquinol to cytochrome c in respiration and photosynthesis coupled to a vectorial proton transport across the membrane, in which the enzyme resides. In both bacteria and eukaryotic organisms, QCR participates in supramolecular assembly of membrane proteins that comprise the respiratory or photosynthetic chain. In the present work, proton transfer pathways, substrate binding and the supramolecular assembly of the respiratory chain in yeast were probed by structure-based site-directed mutagenesis and characterization of the variants. Both active sites centre P, the place of quinol oxidation, and centre N, where quinone reduction takes place, lack direct access to the bulk solvent necessary for proton release and uptake. Based on the X-ray structure, proton transfer pathways were postulated. Analysis at centre P showed, that E272 and Y132 of cytochrome b are important for QCR catalysis as indicated by increased superoxide production and lowered Cyc1p reductase activity in these variants. Pre-steady state heme reduction kinetics in combination with stigmatellin resistance indicated that charge and length of the side chain at position 272 are crucial for efficient docking of the ISP to form the enzyme substrate complex and for electron bifurcation at centre P. Variants of Y312 and F129, both residues of cytochrome b, showed an increased Km indicating participation of these residues in coordination of ubiquinol or the possible intermediate semiquinone anion radical. F129 proved to be crucial for a functional Q-cycle as indicated by respiratory negative growth phenotype and a lowered H+/e- stoichiometry of F129 variants. At centre N, the postulated CL/K and E/R proton transfer pathways are located at opposite sites of the bound ubiquinone. Variants in the surface residues R218 (cytochrome b) and E52 (Qcr7) of the E/R pathway and E82 (Qcr7) of the CL/K pathway showed instability upon purification indicating an important role of these residues for QCR integrity. The slowed down centre N reduction kinetics in H85 (CL/K), R218 and N208 (both E/R) variant was attributed to a destabilised semiquinone anion consistent with the observed decreased sensitivity towards the site-specific inhibitor antimycin and an increased Km. Variants of residues of both pathway, E82Q and R218M, exhibited a decreased H+/e- stoichiometry indicating a crucial role of both residue for maintaining a working Q-cycle and supporting the proposed protonation of the substrate via the Cl/K and the E/R pathway. Long-range interaction between centre N and centre P were observed by altered reduction kinetics of the high potential chain and increased superoxide production in the centre N variants. The role of the cation-pi-interaction between F230 of Cyt1p and R19 of cytochrome c in binding of the redox carrier to QCR was analysed. In F230L hydrophobic interaction were partially lost as was deduced from the ionic strength dependence of Cyc1p reductase activity and Cycp1 binding, as detected by ionic strength sensitive Kd and Km for Cyc1p. The decreased enzymatic rate of F230W could be explained by a disturbed binding of Cyc1p to the variant enzyme. F230 may influence the heme mid point potential and thereby the electron transfer rate to Cyc1p. Reduction of Cobp via both centre P and centre N was disturbed suggesting an interaction between high and low potential chain. Supramolecular association between QCR and cytochrome c oxidase (COX) in yeast mitochondria was probed by affinity chromatography of a his-tagged QCR in the presence of the mild detergent digitonin. In comparison to purification with laurylmaltoside, the presence of both QCR and COX subunits was detected in the elution fractions by SDS-PAGE, Cyc1p reductase and TMPD oxidase activity assays and immunoblot analysis. The CL-dependent formation of the supercomplex between QCR and COX was analysed by replacement variants in the CL-binding site of QCR in CL containing and CL free environment. With an increasing number of replacements of the three lysines the CL-binding pocket supercomplex formation was not abolished, when CL is present as shown by BN-PAGE analysis. This was supported by the synergetic decrease in enzyme activity for both enzymes upon increased number of replacements. In the CL-free environment, no supracomplex formation was observed for a wildtype CL binding site. By replacements of two lysines in the CL-binding pocket, supercomplex formation could be recovered as revealed by BN-PAGE. This indicates, that CL may serve as a charge neutralizer for the lysines near the presumed interaction domain between complex III and complex IV. The obtained results for centre P provide new information of residues critical for stabilisation of ubiquinol and controlling electron short circuit reactions. The observations for centre N variants clearly support the proposed two proton transfer pathways and the role of the bound phospholipids in centre N kinetics. Variants in the Cyc1p binding site suggest a role for F230 both in Cyc1p binding and electron transfer. Clear interaction between the high and low potential chain in both Cyt1p and centre N variants strongly support long-range interactions in the complex. Studies on the supramolecular association of complex III and complex IV indicate a new role of Cl in stabilising a supracomplex.
Die vorliegende Arbeit befaßte sich mit der Untersuchung der Protonenbewegung während des O-E Schrittes im katalytischen Zyklus der Cytochrom-c-Oxidase von P. denitrificans. Die Zuordnung der Protonenbewegung zu den einzelnen Schritten des katalytischen Zyklus der Cytochrom-c-Oxidase ist immer noch ein Gegenstand zahlreicher Kontroversen. Obwohl von Ruitenberg et al. (2000) durch Spannungsmessungen gezeigt wurde, daß die Reduktion von Häm a während des ersten Elektrontransfers in das oxidierte Enzyme eine schnelle Protonenaufnahme von der gegenüberliegenden Seite der Membran bewirkt, wurden diese Ergebnisse angezweifelt. Daher sollte mit einer unabhängigen und direkten Methode herausgefunden werden, ob Protonen bereits während des ersten Schrittes des katalytischen Zyklus aufgenommen werden. Dazu wurde ns-zeitaufgelöste Blitzlicht-Absorptionsspektroskopie in Kombination mit pH-sensitiven Farbstoffen genutzt, und zwar sowohl mit Fluorescein kovalent an der Proteinoberfläche gebunden als auch mit Phenolrot löslich im Medium vorliegend. Zur kovalenten Kopplung von thiolreaktiven Farbstoffen mußten zuerst die nötigen Voraussetzungen geschaffen werden. Dazu wurde in dieser Arbeit ein Mutagenesesystems für sowohl Untereinheit I als auch Untereinheit II etabliert und eine oberflächencysteinfreie Variante und elf Einzelcystein-Varianten hergestellt, exprimiert und aufgereinigt sowie die Enzymaktivitäten überprüft. Danach wurde ein Protokoll zur Kopplung der Einzelcysteinvarianten mit Iodoacetamidfluoresein ausgearbeitet und die Varianten Fluorescein-markiert. Dabei zeigte es sich, daß nur sieben Varianten erfolgreich mit IAF reagierten. Mittels dieser AF-markierten Varianten konnte die Pufferkapazität an der Oberfläche der Cytochrom-c-Oxidase bestimmt werden. Es zeigte sich, daß die Pufferkapazität des Enzyms in Lösung im Vergleich zu Bakteriorhodopsin dreimal so groß ist, an der Oberfläche sogar 10-15mal so groß. Dies deutet auf eine hohe Anzahl protonierbarer Gruppen um die für die Markierung ausgewählten Aminosäuren im Bereich der Eintrittsstellen der Protonen hin. Die gezielte Übertragung eines Elektrons auf die Cytochrom-c-Oxidase erfolgte durch Licht anregbare Rutheniumkomplexe. In unserem Meßsystem war die Elektronentransfereffizienz von [Ruthenium(2,2‘-bipyridin)2]2quarterpyridin am höchsten. Nach einer sorgfältigen Optimierung der Meßbedingungen wie pH-Wert, Ionenstärke und Energie des Lasers konnte eine 10-15 %ige Reduktion von Häm a mit einer Zeitkonstanten von t = 13,7 ± 2,4 µs nachgewiesen werden. Die Protonenkonzentrationsänderungen im Medium konnten durch Phenolrot verfolgt werden. Durch den Vergleich von Funktionsvarianten, bei denen jeweils einer oder beide Protoneneingangswege blockiert sind, konnte ein Modell für die Protonenaufnahme und -abgabe während der Einelektronen-Reduktion der Cytochrom-c-Oxidase entwickelt werden. Dies konnte durch Messungen an in Liposomen inkorporierter wt Cytochrom-c-Oxidase verifiziert werden. Die Nettoprotonenaufnahme von der N-Seite der Cytochrom-c-Oxidase beträgt somit 0,3 H+ für das im O-E Schritt aufgenommene Elektron. Die Variante CS-I302C-AF wurde dazu genutzt, die Oberflächenladungsdichte an der N-Seite der Cytochrom-c-Oxidase zu bestimmen. Die Oberflächenladungsdichte auf der N-Seite des Enzyms in der Nähe zum Eingang des K-Wegs ist negativ und beträgt 0,5 e-/1000 Å2.
Nicotinic acid has been used in the clinical treatment of elevated blood lipid levels for over 50 years. Although it has a beneficial effect on myocardial infarction and blood lipid profiles, its widespread use has been hampered by side effects such as skin rashes and a burning sensation on the upper body. Since elevated blood lipid levels, especially ones of VLDL and LDL cholesterol are a frequent indication and high risk factor for coronary and cardiac diseases, finding a compound with an enhanced pharmacological profile, still holding the desired effects, but without inconvenient side effects, is a very appealing aim to many pharmaceutical companies. These efforts have already produced two marketed drugs, Acipimox and Acifran, but they have not been able to overcome the restrictions already imposed on the treatment by nicotinic acid. Although proposed long before, in the year 2000 the gene for the nicotinic acid receptor in mouse PUMA-G was cloned, and in 2003 the discovery of the genes HM74 and HM74A followed, which comprise the homologous low and high affinity receptors for nicotinic acid in humans. The discovery of this G Protein-coupled receptor target allowed a more directed approach for the search of alternative compounds. This work is the first report of the heterologous overexpression of the high affinity GPCR gene HM74A in the methylotrophic yeast Pichia pastoris. The protein product, NAR1, was pharmacologically characterized, and displayed a binding affinity of 224.8 nM to its ligand nicotinic acid, showing a similar activity profile compared to those displayed in human tissue, which were determined to be 60 nM to 90 nM. Additionally, inhibitory constants (Ki) for Acifran and Acipimox were determined to be 4.5 µM and 50.5 µM, respectively. Furthermore, the total yield of NAR1 reached 42 pmol/mg membrane protein, which corresponds to 0.4 mg of receptor produced per liter yeast culture, opening up the perspective of large scale protein production to facilitate high throughput screening drug discovery efforts and structural studies. In addition, NAR1 could be solubilized in n-decyl-β-D-maltopyranoside and purified to homogeneity after immobilized metal affinity chromatography and a second affinity chromatography step on immobilized monomeric avidin, yielding a single peak on gel filtration, while the purified receptor was able to bind ligand, as shown in NMR Saturation Transfer Difference (STD) measurements. It could be shown that NAR1 is desensitized by β-arrestin 1 in vivo in confocal microscopy studies on HEK and BHK cells. This finding provides a native binding partner for the stabilization of the receptor upon solubilization and purification. Finally human β-arrestin 1 could be produced as a constitutively active variant, comprising residues 1-382 in Pichia pastoris and Escherichia coli. The purified protein was used for in vitro binding experiments and shown to be capable of interacting with NAR1. Although the interaction and formation of the complex was only possible to a limited extent, it leaves open the perspective of crystallizing NAR1 in its active conformation, bound to nicotinic acid and β-arrestin 1.
The cytochrome bc1 complex is a cornerstone in bioenergetic electron transfer chains, where it carries out tasks as diverse as respiration, photosynthesis, and nitrogen fixation. This homodimeric multisubunit membrane protein has been studied extensively for several decades and the enzyme mechanism is described with the modified protonmotive Q cycle. Still, the molecular and kinetic description of the catalytic cycle is not complete and questions remain regarding the bifurcation of electron transfer at the quinol oxidation (Qo) site, substrate occupancy, pathways of proton conduction, and the nature of the Rieske protein domain movement. We used competitive inhibitors to study the molecular architecture at the Qo site with X-ray crystallography. The structure of the enzyme with the substrate analog 5-n-heptyl-6-hydroxy-4,7-dioxobenzothiazole (HHDBT) bound at the Qo site was determined at 2.5 Å resolution. Spectroscopic studies showed that HHDBT is negatively charged when bound at the active site. Mechanistic interpretations from inhibitor binding are in line with single occupancy model for quinol oxidation and structural analysis supports the proposed proton transfer pathway. For functional insight into the enzyme mechanism, redox-sensitive protonation changes were studied by Fourier transform infrared spectroscopy. The protein purification procedure was optimized for less delipidation and the isolated enzyme was more active. Furthermore, two new phospholipids were identified in the X-ray structures, including a cardiolipin. Strikingly, conserved lipid binding cavities were observed in structural comparison with homologous enzymes. The functional role of tightly bound phospholipids will be discussed. Finally, the Qo site is a target for various compounds of agricultural and pharmaceutical importance. Importantly, the X-ray structures permit detailed analysis of the molecular reasons for acquired resistance to and treatment failure of Qo site inhibitors, such as atovaquone, that is used to treat malaria and pneumonia, as discussed herein.
Sodium proton antiporters are ubiquitous membrane proteins found in the cytoplasmic and organelle membranes of cells of many different origins, including plants, animals and microorganisms. They are involved in cell energetics, and play primary roles in the homeostasis of intracellular pH, cellular Na+ content and cell volume. Adaptation to high salinity and/or extreme pH in plants and bacteria or in human heart muscles requires the action of such Na+/H+ antiporters. NhaA is the essential Na+/H+ antiporter for pH and Na+ homeostasis (at alkaline pH) in Escherichia coli and many other enterobacteria. NhaA is an electrogenic Na+/H+ antiporter that exchanges 2H+ for 1Na+ (or Li+). NhaA shares with many other prokaryotic and eukaryotic antiporters a very strong dependence on pH. In order to achieve three-dimensional structure of NhaA, the previously described NhaA protein preparation was modified: (i) the wild type bacterial strain (TA16) used for homologous over-expression of NhaA was replaced with a delta nhaA strain (RK20). As a result, the purity and homogeneity of the sample was significantly improved; (ii) the previously two-step purification procedure was shortened to a single step affinity chromatography purification; (iii) a wide-range screening of crystallisation conditions, more than 20,000, was performed; (iv) a Seleno-L-methionine (SeMet) NhaA derivative was produced in order to solve the phases during structure determination. In parallel, attempts of production and crystallisation of co-complexes composed of NhaA and antibody fragments have been made. Four different monoclonal antibodies were available against NhaA. Selected antibody fragments were produced and the stability of the complex analysed. Here, the crystal structure of the pH down-regulated secondary transporter NhaA of Escherichia coli is presented at 3.45 Å resolution. A negatively charged ion funnel opens to the cytoplasm and ends in the middle of the membrane at the putative ion-binding site. There, a unique assembly of two pairs of short helices connected by crossed, extended chains creates a balanced electrostatic environment. A possible mechanism is proposed: the binding of charged substrates causes electric imbalance inducing movements, which allow for a rapid alternating access mechanism. This ion exchange machinery is regulated by a conformational change elicited by a pH signal perceived at the cytoplasmic funnel entry. The structure represents a novel fold that provides two major insights: it reveals the structural basis for the mechanism of Na+/H+ exchange and its unique regulation by pH in NhaA and in many other similar antiporters. Furthermore, it is also important for the understanding of the architecture of membrane proteins in general. However, although many aspects of the ion-translocation mechanism and pH regulation are clarified by the NhaA structure, higher resolution structures with Li+ or Na+ bound are required for understanding the ligand binding and the translocation mechanism at the atomic level. The alkaline pH-induced conformation is essential to further understand the pH-control and proton access to the binding site.
Cytochrome c oxidases are among the most important and fundamental enzymes of life. Integrated into membranes they use four electrons from cytochrome c molecules to reduce molecular oxygen (dioxygen) to water. Their catalytic cycle has been considered to start with the oxidized form. Subsequent electron transfers lead to the E-state, the R-state (which binds oxygen), the P-state (with an already split dioxygen bond), the F-state and the O-state again. Here, we determined structures of up to 1.9 Å resolution of these intermediates by single particle cryo-EM. Our results suggest that in the O-state the active site contains a peroxide dianion and in the P-state possibly an intact dioxygen molecule, the F-state may contain a superoxide anion.
NADH:ubiquinone oxidoreductase (Complex Ⅰ) is the first and largest enzyme in the respiratory chain. It catalyzes the transfer of two electrons from NADH to ubiquinone via a series of enzyme-bound redox centers - Flavin mononucleotide (FMN) and iron-sulfur (Fe-S) clusters – and couples the exergonic reaction with the endergonic translocation of four protons across the membranes. Bacteria contain the minimal form of complex I, which is composed of 14 conserved core subunits with a molecular mass of around 550 kDa. Complex Ⅰ has an L-shaped structure which can be subdivided into two major parts (arms). The hydrophilic arm protruding into the bacterial cytosol (or mitochondrial matrix) harbors the binding site for the substrate NADH, the two- to one-electron switch FMN and all one-electron transferring Fe-S clusters and therefore considered as the catalytic unit. The membrane arm consists of the membranespanning subunits and conducts the proton pumping process. The Quinone binding site is located at the interface of both arms. ...