Refine
Year of publication
- 2004 (6) (remove)
Document Type
- Doctoral Thesis (6)
Has Fulltext
- yes (6)
Is part of the Bibliography
- no (6)
Keywords
- Biomembran (1)
- Brownsche Bewegung (1)
- Chinon (1)
- Elektrische Ladung (1)
- FTIR-Differenzspektroskopie (1)
- Inhibitoren (1)
- Porin (1)
- Proteine (1)
- Proteinelektrochemie (1)
- Stabilität (1)
Institute
- Physik (6)
Ziel der vorliegenden Arbeit war die Untersuchung der elektrochemischen und spektroskopischen Eigenschaften der bc1-Komplexe aus dem Bodenbakterium Paracoccus denitrificans und der Hefe Saccharomyces cerevisiae im sichtbaren und infraroten Spektralbereich. Das redoxaktive Protein ist Bestandteil der Atmungskette und trägt entscheidend zum Aufbau eines Protonengradienten bei, der zur Bildung des universellen Energieträgers ATP genutzt wird. Der bakterielle P. denitrificans-Komplex besteht aus den drei katalytischen Untereinheiten Cytochrom b, Cytochrom c1 und Rieske-Protein. Der mitochondriale Hefe-bc1-Komplex besitzt neben diesen drei noch acht weitere Untereinheiten, die anscheinend für die Stabilität des Enzyms bedeutsam sind. Um Konformationsänderungen des Proteins infolge von Elektronen- und daran gekoppelten Protonentransferreaktionen zu dokumentieren, wurde der Komplex elektrochemisch in definierte Redoxzustände versetzt. Aus den in diesen Zuständen aufgenommenen Absorptionsspektren berechnen sich Differenzspektren, deren Banden auf die Redoxreaktion zurückzuführende Veränderungen im Protein widerspiegeln. Durch Vergleiche mit Modellspektren isolierter Proteinbestandteile, Spektren ähnlicher Proteine und Informationen aus Kristallstrukturen konnten Beiträge der verschiedenen Kofaktoren, des Proteinrückgrates und einzelner Aminosäuren zu diesen Banden zugeordnet werden. Die elektrochemisch induzierten FTIR-Differenzspektren des P. denitrificans-bc1-Komplexes zeigten vor allem Beiträge der im Komplex gebundenen Chinone, die durch den Vergleich mit Differenzspektren isolierter Chinone identifiziert werden konnten. Ein wichtiges Ergebnis war die Abschätzung der Chinonkonzentration im Protein anhand einer charakteristische Bande bei 1262 cm-1 resultierend aus Schwingungen der Chinon-Methoxygruppen. Das Ergebnis von durchschnittlich 3 Molekülen Chinon pro Protein-Monomer unterstützt das zur Zeit für die Qo-Bindestelle diskutierte double-occupancy-Modell. Interessanterweise konnte die Protonierung einer Glu/Asp-Aminosäureseitenkette in Abhängigkeit vom Chinongehalt beobachtet und daraus abgeleitet Signale eines an der Qo-Bindestelle gebundenen Chinons differenziert werden. Die Beiträge der Cytochrom b und c-Untereinheiten relativ zum Gesamtspektrum des P. denitrificans-bc1-Komplexes wurden mittels Differenzspektren der einzelnen Kofaktoren unterschieden. Anhand ihrer Mittelpunktpotentiale, die zuvor durch Potentialtitrationen im sichtbaren Spektralbereich bestimmt wurden (Häm bL: Em7=-292 mV vs. Ag/AgCl, Häm bH: -144 mV, Häm c1: 89 mV), konnten die Differenzsignale des jeweiligen Kofaktors und seiner durch die Redoxreaktion beeinflußten Umgebung durch Wahl geeigneter Potentialschritte separiert werden. Die Zuordnungen der Signale des Cytochrom c1 und des Rieske-Proteins, die spektroskopisch nicht getrennt werden können, wurden durch Messungen an wasserlöslichen Fragmenten dieser Untereinheiten abgesichert. In allen Spektren konnten typische Beiträge des Proteingrundgerüstes, Schwingungen der Häme und ihrer Substituenten sowie einzelner Aminosäuren vorläufig zugeordnet werden. Die Bindung von Inhibitoren führte zu deutlichen Veränderungen im FTIR-Differenzspektrum. Der Qi-Inhibitor Antimycin A zeigt eigene Differenzsignale im Bereich oberhalb 1734 cm-1, an denen die Bindung des Inhibitors im Protein nachvollzogen werden konnte. Sie führte zur Abnahme der Signalintensität einer Bande, die die Beeinflussung eines protonierten Hämpropionates oder Arginin-bzw. Asparaginseitenketten vermuten lassen. Die Bindung des Qo-Inhibitors Stigmatellin, der selbst redoxaktiv ist, äußerte sich in Veränderungen im Amid I-Bereich des Differenzspektrums. Die Deprotonierung einer Glu/Asp-Seitenkette infolge der Stigmatellinbindung wurde diskutiert. Die FTIR-Differenzspektren des S. cervisiae-bc1-Komplexes gleichen denen des bakteriellen Komplexes in Bezug auf die Bandenpositionen weitestgehend. Die Signalintensitäten sowie die Größenverhältnisse der Banden zueinander unterscheiden sich jedoch. Dies wird durch den geringeren Chinongehalt des Hefeproteins nach der Präparation bedingt. Der Einfluß fünf verschiedener Inhibitoren der Qi- und Qo-Bindestelle auf die Differenzspektren wurde untersucht. Dabei standen von zwei Substanzen isotopenmarkierte Varianten zur Verfügung, die tieferen Einblick in die genaue Wechselwirkung bei der Inhibitorbindung bringen sollte. Die Bindung der Inhibitoren führte zu Veränderungen in den Spektren. Sie wurden vor dem Hintergrund der Kristallstruktur betrachtet, die aufgrund ihrer Auflösung keine exakten Aussagen über den Protonierungszustand einzelner Proteinbestandteile liefern kann. Der Schwerpunkt der Studien lag auf den Vergleich der Qo- Inhibitoren Stigmatellin und HHDBT. Die Bindung von Stigmatellin führte wie im P. denitrificans-Komplex zur Deprotonierung einer Glu/Asp-Seitenkette. Die Inhibierung mit HHDBT resultierte in der Protonierung vermutlich der gleichen Glu/Asp-Seitenkette. Die Auswirkungen des unterschiedlichen Protonierungszustandes der Aminosäure in Anwesenheit dieser beiden Inhibitoren wurde im Kontext eines vermuteten Chinoloxidations-Mechanismus beleuchtet.
The enzyme quinol:fumarate reductase (QFR) from the anaerobic e-proteobacterium Wolinella succinogenes is part of the anaerobic respiratory system of this organism. It couples the reduction of fumarate to succinate to the oxidation of menaquinol to menaquinone. W. succinogenes uses fumarate as terminal electron acceptor and can use various substrates (e.g., formate or molecular hydrogen) as electron donors. The concerted catalytic substrate turnover of either a hydrogenase or a formate dehydrogenase in conjunction with QFR contributes to the generation of an electrochemical potential gradient across the bacterial plasma membrane, which is used for the phosphorylation of ADP with inorganic phosphate, Pi, to ATP. In addition to an FAD (in subunit A) and three iron-sulfur clusters (in subunit B), QFR binds a low- and a high-potential heme b group in its transmembrane subunit C, as was ultimately shown in the crystal structure at 2.2 Å resolution (Lancaster et al., 1999, Nature 402, 377– 385). Both hemes are part of the electron transport chain between the two catalytic sites of this redox enzyme. The midpoint potentials of the hemes are well established but their assignment to the distal and proximal positions in the structure had not yet been determined. Furthermore, QFR from W. succinogenes has been proposed to exhibit a novel coupling mechanism of transmembrane electron and proton transfer, which has been described in the so-called “E-pathway” hypothesis (Lancaster, 2002, Biochim. Biophys. Acta 1565, 215–231). The aim of this project was to characterize the relationship between structure and function of QFR and to investigate the details of the proposed coupling mechanism (“Epathway”) with the help of computer-based electrostatic calculations on the QFR wild-type (WT) coordinates, and electrochemically induced FTIR and VIS difference spectroscopy on the QFR WT and available variant enzymes (in particular enzyme variant E180Q, in which the glutamic acid at position C180 has been replaced by a glutamine). 1.) It was demonstrated in this study that the diheme-containing QFR exhibits stable and reproducible electrochemically induced FTIR difference bands in the midinfrared range from 1800 cm-1 to 1000 cm-1 that reflect transitions from the reduced to the oxidized state of the enzyme. The spectral features that were observed in the FTIR difference spectra are fully reversible when changing from a reductive to an oxidative reference potential at the working electrode and vice versa. This indicates that the underlying redox reactions of the enzyme at the gold grid working electrode are also fully reversible under the applied experimental conditions. The same reversible spectral redox behavior in the visible range could also be ascertained for the Soret- and a-band of the two heme b groups of QFR. This behavior allowed to reliably determine the heme b midpoint potentials of QFR at various pH values. Analysis of the FTIR difference spectra in the amide I range yields evidence for structural reorganizations of the polypeptide backbone upon the electrochemically induced redox reaction. 2.) The redox titrations of the high- and low-potential heme b of QFR as simulated by multiconformation continuum electrostatics (MCCE) calculations showed a very high level of agreement with respect to the experimentally observed midpoint potentials of the heme b groups at pH 7. As determined with the help of the theoretical calculations, prominent features governing the differences in redox potential between the two hemes are the higher loss of reaction field energy for the proximal heme and the stronger destabilization of the oxidized form of the proximal heme due to several buried and ionized Arg and Lys residues. The explicit incorporation of crystallographically identified water molecules in the calculations had a noticeable effect on the absolute values of the determined midpoint potentials, although the relative difference of the two obtained midpoints did not change significantly. The results of the electrostatic calculations clearly showed that the lowpotential heme corresponds to the distal position bD in the structure, and that the high-potential heme is identical to the proximal heme bP. This assignment could previously not be achieved unequivocally with experimental methods. 3.) In addition, the currently discussed mechanism of coupled electron and proton transfer in the QFR of W. succinogenes (i.e., the “E-pathway” hypothesis) is further supported by the results of this study. The simulations of intermediate states of electron transfer via the heme b groups show that the protonation state of the key amino acid residue Glu C180 depends on the redox states of the heme groups as suggested in the “E-pathway” hypothesis. This result yields a possible mechanism for the coupling of transient transmembrane proton transfer via Glu C180 to the electron transfer via the heme b groups, since Glu C180 could be part of a “proton wire” and its redox-dependent protonation state could serve as the regulatory element of the “E-pathway”. Furthermore, the results of simulated heme reduction indicate that the side chain of Glu C180 also changes its conformation with respect to the redox state of the hemes. Both major results concerning the role of Glu C180, the change of protonation as well as the reorientation of the side chain upon reduction of the heme groups, are consistent with the results from electrochemically induced FTIR difference spectroscopy: Of particular interest was the spectral range above 1710 cm-1, where C=O stretching vibrations of protonated COOH carboxyl groups absorb, because those groups can act as proton donors, respectively acceptors, and can be involved in intra-protein proton transfer reactions. It was possible to observe signals of such protonated carboxyl groups originating from QFR enzyme, which either change their protonation state and/or experience an environmental change in the course of the induced redox reaction. This finding was supported by the fact that the relevant FTIR difference signals are sensitive to an isotopic hydrogen/deuterium (1H/2H) exchange via the buffer solution, since they were shifted towards lower wavenumbers in D2O. Furthermore, it could be shown with the help of site-directed mutagenesis that the acidic residue Glu C180, which is located in the membranespanning, diheme-containing subunit C of QFR, is contributing to the redox dependent signal of protonated carboxyl groups. The observed residual signal in the FTIR double-difference spectrum of QFR wild-type and enzyme variant E180Q (Glu C180 has been replaced with a Gln residue) could be interpreted as a protonation/deprotonation event that is superimposed by an environmental effect on the specific C=O vibration. This result strongly supports the proposed “E-pathway” of coupled transmembrane electron and proton transfer in the QFR enzyme, which states that residue Glu C180 is an essential constituent of a transient redox-controlled transmembrane proton transfer pathway. 4.) As a second possible constituent of the suggested “E-pathway”, the ring C propionate of the distal heme was found to be unusually fully protonated in all simulated redox states, indicating a possible role as a transient proton donor/acceptor in the “E-pathway”. Similarly to Glu C180, experimental evidence from FTIR difference spectroscopy on a modified QFR with 13C-labeled heme propionates was obtained, which indicates an involvement of at least one of the two propionates of heme bD in proton transfer. The observed signals can tentatively be interpreted as a redox-coupled (de)protonation of the ring C propionate of bD, which is possibly xiii superimposed by a conformational or environmental change of the specific propionate. 5.) Also the observation of a strong redox Bohr effect for both heme b groups in QFR is in line with the proposed “E-pathway” hypothesis, as this effect yields a possible and well-established mechanism for the coupling of proton transfer and redox changes of the heme groups. The comparison of the observed effect in QFR WT and E180Q together with the results from FTIR spectroscopy and MCCE calculation indicate that the ring C propionate of the distal heme is dominating the pHdependence of the midpoint potential of bD, and that the corresponding group for bP is Glu C180. The origin of the redox Bohr effect for bP in the enzyme variant E180Q (which is dramatically changed with respect to the WT) could not be identified unequivocally, but the observation of this redox Bohr effect in the variant implies the presence of other protolytic groups, which interact with heme bP and which may be necessary for a functional “E-pathway”.
Transmembrane proteins play crucial roles in biological systems as active or passive channels and receptors. Experimentally only few structures could be determined so far. Gaining structural insights enables besides a general understanding of biological mechanisms also further processing such as in drug design. Due to the lack of experimental data, reliable theoretical predictions would be of high value. However, for the same reason, missing data, the knowledge-based class of prediction methods that is well established for soluble proteins can not be applied. The goal of predicting transmembrane protein structures with ab initio methods demands locating the free energy minimum. Main difficulties here are, first, the computational costs of explicitly calculating all involved interactions and, second, providing an algorithm that is capable of finding the minimum within an extremely complex and rugged energy landscape. We have developed promising energy functions that describe the interactions of amino acids on a residue level, reducing computational costs while still containing most information on the atomistic level. We have also found a way to describe the interaction of the residues with its surrounding in a realistic manner by distinguishing residues exposed to the environment from those buried within helices using a sphere algorithm. The sphere algorithm can also be applied for a different purpose: one can measure how densely sidechains are packed for certain helical conformations, and thereby get an estimate of the sidechain entropy. In addition, overcrowding effects can be identified which are not well-described by the energy functions due to the pairwise calculation. To determine the absolute free energy minimum, we assume the helices to be located on an equidistance grid with slightly larger distances than to be expected. Optimizing the helices on the grid provides a starting point that should enable common minimizing algorithms, gradient-based or not, to find the absolute minimum beyond the grid. To simulate the dynamics of the helices on large time scales, we split them into rigid body dynamics and internal dynamics in terms of the dihedrals. The former one is well-known with its inherent problem of numerical drift and plenty of approaches to it, among which we have chosen the quaternions to represent the rotation of the rigid bodies. The latter one requires a detailed analysis of the torque size exerted on the dihedrals caused by the forces acting on the residues.
Stability, unfolding and refolding of the outer membrane protein porin from Paracoccus denitrificans was investigated using genetic and spectroscopic methods. Structural and functional activity studies on wild type and mutant porins: The site-directed mutants were constructed based on conserved residues and evidences on the role of certain amino acids from previous studies with OmpF. Secondary structure analysis of wild type and mutants E81Q, W74C, E81Q/D148N, E81Q/D148N/W74C by FTIR and CD spectroscopy are in line with the fact that porins are predominantly ß-sheet structure. The functional activity studies by black lipid bilayer techniques showed that the wild type and mutants W74C, E81Q/D148N, E81Q/D148N/W74C have a conductance of 3.25 nS. For mutant E81Q conductance of 1.25nS was more predominant over 3.25 nS. The activity of the mutants was observed to be far less than the wild type. This indicates that structural similarities does not implies similar functional activity. Thermal stability analysis of porin in detergent micelles and reconstituted into liposomes: Thermal stability analysis of wild type and mutants in detergent micelles showed changes in secondary and quaternary structure. It was found that wild type porin unfolds into aggregated structure with a high transition temperature of 86.2 °C. For mutants E81Q, W74C, E81Q/D148N the transition temperature was found to be 84.2 °C, 80.3 °C and 80.2 °C respectively. Functional activity assays at high temperatures revealed that the protein tends to loose its activity on heating up to 50 °C. This shows that structural stability does not imply functionality in the case of porins. Thermal stability analysis of porin reconstituted into liposomes showed that there was no change in the secondary and quaternary structure of the protein up to 100 °C, revealing that the protein becomes more thermostable when it is reconstituted into liposomes. Refolding of aggregated porin: This study shows that disaggregation of ß-sheet membrane protein porin is possible by changing its chemical and thermodynamic parameters. An increase of the solution pH to 12 or above results in opening up of the aggregated protein into unordered structure, as observed by FTIR and CD spectroscopy. This unordered structure could be refolded into native-like structure forming trimers. The secondary structure of the refolded protein deviated slightly from the native one. The thermal stability analysis of the native-like refolded proteins showed that the unfolding pattern is entirely different when compared to the native porins. pH dependent unfolding of porin: Thermal stability of porin at different pH values showed that the protein is stable in a pH range of 1-11. At pH 12 and above the protein unfolds into unordered structure instead of aggregating. The high pH unfolding of porin is a reversible process. The secondary structure of the refolded protein varied slightly from the native-one. Whereas thermal stability was entirely different. This shows that even though the unfolding of porin at high pH is reversible, it results in changes in local interaction between the amino acids resulting in a difference in stability. Unfolding in presence of urea and guanidinium hydrochloride (GuHCl): Denaturation of porin in the presence of chemical denaturants like urea and GuHCl showed that porin unfold into unordered structure. The unfolding is a reversible process. Unfolded protein was refolded into detergent micelles and liposomes. Refolding into detergent micelles was faster compared to refolding into liposomes, as seen by kinetic gel shift assays. The refolding into liposomes showed the presence of intermediates similar to those reported for OmpF. This study shows the difference in thermal stability of the outer membrane protein porin from Paracoccus denitrificans in detergent micelles and native-like liposomes. It suggests various unfolding pathways, which can be further investigated for unfolding and refolding kinetics. This report also suggests that it is possible to refold a heat-aggregated protein.
Results were presented from Brownian dynamics simulations for cyt c molecules approximated as spherical particles with diameter 2R ' 3.3 nm interacting with a charged planar membrane surface. Using the well-known Ermak-McCammon algorithm of ref. [36, 37] for solving the Langevin equations (see Chapter 2), a new computer program in C++ was developed. An overview of the way it is implemented is given in Chapter 3. The program in its current state is able to compute the trajectories (translation and rotation) of hundreds of spherical particles in systems with typical dimensions of 103 − 1003 nm3 . As explained in the introductory Chapter 1 the motivation for studying the dynamics of cyt c molecules in such systems came from the progress in the research of photosynthetic bacteria, e.g. While the internal processes of energy transduction (light harvesting, channelling to RC, charge separation) are quite well understood, the dynamics of soluble cyt c as an electron transporter in this context is not yet clear. In many textbooks one can find illustrations where a single cyt c is responsible for the electron transport between two integral membrane proteins (the reaction centre RC and the bc1 complex). But as pointed out in publications like refs. [49], [59], [60], [61] or [62] biological cells are crowded with different molecules. Consequently, one can assume that the electron transport between two integral membrane proteins is not simply taken on by one single cyt c molecule. Instead it is likely that many of these particles are located in a cyt c pool above the membrane and that they perform the electron transport in turns. Thus, it is desirable to have a simulation package that is able to compute the trajectories of many proteins. Note that the detailed processes of electron transfer and binding to membrane proteins are not modelled here. The details of these processes are quite complicated so that we refrained from including them in the coarse-grained simulations. Here, the actual binding is simply defined by a particle distance zb from the membrane which marks the beginning of the attractive potential. ...
Determination of the structure of complex I of Yarrowia lipolytica by single particle analysis
(2004)
Komplex I enthält ein Flavinmononukleotid sowie mindestens acht Eisen- Schwefel Zentren als redoxaktive Cofaktoren. Da ein wesentlicher Teil des mitochondrialen Genoms für Untereinheiten von Komplex I codiert, betrifft eine Vielzahl von mitochondrialen Erkrankungen diesen Enzymkomplex.
Komplex I wurde bisher aus Mitochondrien, Chloroplasten und Bakterien isoliert. Die Minimalform von Komplex I wird in Bakterien gefunden, wo er aus 14 (bzw 13 im Falle einer Genfusion) Untereinheiten besteht und eine Masse von etwa 550 kDa aufweist. Generell werden sieben hydrophile und sieben hydrophobe Untereinheiten mit über 50 vorhergesagten Transmembranhelices gefunden. Im Komplex I aus Eukaryoten wurde eine grössere Anzahl zusätzlicher, akzessorischer Untereinheiten nachgewiesen. Hier werden die sieben hydrophoben Untereinheiten vom mitochondrialen Genom codiert, während alle anderen Untereinheiten kerncodiert sind und in das Mitochondrium importiert werden müssen.
Die obligat aerobe Hefe Yarrowia lipolytica wurde als Modellsystem zur Untersuchung von eukaryotischem Komplex I etabliert. Die bisher am besten untersuchte Hefe Saccharomyces cerevisiae enthält keinen Komplex I. Hier wird die Oxidation von NADH durch eine andere Klasse von sogenannten alternativen NADH Dehydrogenasen durchgeführt. Auch Y. lipolytica enthält ein solches alternatives Enzym, das allerdings mit seiner Substratbindungsstelle zur Aussenseite der inneren Mitochondrienmembran orientiert ist. Durch molekularbiologische Manipulation konnte eine interne Version dieses Enzymes exprimiert werden, wodurch es möglich ist, letale Defekte in Komplex I Deletionsmutanten zu kompensieren. Mittlerweile wurden alle Voraussetzungen geschaffen, um kerncodierte Untereinheiten von Komplex I aus Y. lipolytica gezielt genetisch zu verändern. Die Proteinreinigung wird durch die Verwendung einer auf einem His-tag basierenden Affinitätsreinigung erheblich erleichtert...