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Transport processes across the membrane are essential to ensure survival of every living cell. Therefore, the exchange of membrane impermeable molecules is mediated by specific transport proteins, which are embedded in the lipid bilayer.
One important class comprises secondary active transporters, which couple very efficiently the uphill transport of the main substrate against its concentration gradient to the downhill transport of an additional substrate. These transporters are widely distributed among all kingdoms of life and accomplish many crucial functions. One function is to counteract the deleterious effect of hyperosmotic stress in bacteria. Several members of the BCCT (betaine-choline-carnitinetransport) family of secondary transporters mediate osmostress protection by the accumulation of the compatible solute betaine or its precursor choline (Lamark et al., 1991; Peter et al., 1996; Ziegler et al., 2010). Besides osmo-dependent sodium or proton-coupled symporters, the BCCT family includes few rare representatives of osmo-independent transporters such as the substrate:product antiporter CaiT from E. coli (Jung et al., 2002; Ziegler et al., 2010).
The best-characterized member of the BCCT family is the sodium-coupled betaine transporter BetP from Corynebacterium glutamicum. BetP together with the ABCtransporter OpuA and the H+-solute symporter ProP, became a paradigm for osmoregulated osmolyte transport. Although, all three transporters were extensively studied, the general mechanism of osmoregulation is still far from being understood. Thus, one task of this thesis was to elucidate further the regulatory properties of BetP.
BetP is tightly regulated by osmotic stress and is able to increase its basal betaine uptake activity dramatically upon elevated osmolalities within one second (Peter et al., 1998a). The osmotic stress is sensed by BetP via two stimuli, one is the increase of the internal K+ concentration above a threshold of 220 mM (Rübenhagen et al., 2001), the second is related to a change in the physical state of the membrane (Maximov et al., 2014). So far, several solved crystal structures in combination with functional and computational analysis provided insights into the coupling mechanism of betaine and its co-substrate sodium (Khafizov et al., 2012; Perez et al., 2012). Despite the wealth of data, the precise regulatory mechanism of trimeric BetP is still unclear.
The increasing resistance of almost all pathogenic bacteria to antibiotics (multidrug resistance) causes a severe threat to public health. The mechanisms underlying multidrug resistance include the induced over expression of multidrug transporters which extrude a variety of lipophilic and toxic substrates in an energy dependent fashion through the membrane out of the cell. These proteins are found in all transporter families. The work described in this thesis is dedicated to drug-proton antiporters from the small multidrug resistance (SMR) family. These efflux pumps with just four transmembrane helices per monomer are so far the smallest transporters discovered. Their oligomeric state, topology, three dimensional structure, catalytic cycle and transport mechanism are still rather controversial. Therefore, the aim of this thesis was to directly address these questions for the small multidrug resistance proteins Halobacterium salinarium Hsmr and Escherichia coli (E. coli) EmrE using a number of biophysical methods such as NMR, transport assays, mass spectrometry and analytical ultracentrifugation. Especially the work on Hsmr has been challenging due to the halophilic nature of this protein. In Chapter 1, key questions and the most important biophysical techniques are introduced followed by Material and Methods in Chapter 2. Depending on experimental requirements, cell free or ‘classical’ in vivo expression has been used for this thesis. Cell free expression as an option for the production of small multidrug transporters has been explored in Chapter 3. It has been possible to produce the SMR family members Hsmr, EmrE, TBsmr and YdgF in vitro. The expression of Hsmr was investigated in more detail under different experimental conditions. Hsmr was either refolded from precipitate or maintained in a soluble form during expression in the presence of detergents and liposomes. Furthermore, amino acids for which no auxotrophic strains were available could be labelled successfully. This expression system has been also used for preparing labelled samples of EmrE as described in Chapter 9. In vivo in E. coli expression of Hsmr, as described in Chapter 4, provided large amounts of proteins if fermenter production was used. Uniform labelling and selective unlabelling with stable isotopes (13C, 15N) for NMR spectroscopy was achieved in vivo in a more efficient and cost effective manner than using the cell free approach for this protein. Hsmr could be purified successfully from both in vitro and in vivo expression media. Hsmr is expressed in vivo and in vitro with N-terminal formylation. The Nterminal formylation is unstable and Hsmr in the presence of low salt concentrations was amenable to N-terminal degradation. It was found that Hsmr shows longest stability in Fos-ß-choline® 12 and sodium dodecyl sulphate, but best reconstitution conditions were found, when dodecyl maltoside is used and exchanged with Escherichia coli lipids. A molar protein lipid ratio of 1 to 100, amenable to solid state nuclear magnetic resonance, has been achieved. Sample homogeneity was shown by freeze fracture electron microscopy. The oligomeric state of Hsmr in detergent has been assessed by SDS PAGE, blue native PAGE, size exclusion chromatography, analytical ultracentrifugation and laser induced liquid bead ion desorption mass spectrometry (LILBID) as described in Chapter 5. A concentration and detergent dependent monomer-oligomer equilibrium has been found by all methods. The activity of Hsmr under the sample preparation conditions used here was shown using radioactive and fluorescence binding as well as fluorescence and electrochemical transport assays (Chapter 6). For transport studies, a stable pH gradient was generated by co-reconstitution of Hsmr with bacteriorhodopsin and subsequent sample illumination. Based on the observed long term stability of Hsmr in Fos-ß-choline® 12 and sodium dodecyl sulphate, liquid state NMR experiments were attempted in order to assess the correct folding of Hsmr in detergent micelles (Chapter 7). 1D proton and 2D HSQC spectra of U-15N Hsmr revealed a poor spectral dispersion, low resolution and only a small number of peaks. These are at least partly due to long rotational correlation times of the large protein detergent complex. This problem has been overcome by applying solid-state NMR to Hsmr reconstituted into E. coli lipids (Chapter 8). Uniform 13C labelled samples were prepared and two dimensional proton-driven spin diffusion and double quantum-single quantum correlation spectra were acquired successfully. Unfortunately, the spectral resolution was not yet sufficient for further structural studies. Reasons for the observed linebroadening could be structural heterogeneity or molecular motions which interfere with the NMR timescale. Therefore, the protein mobility has been probed using static 2H solid state NMR on Ala-d3-Hsmr. It could be shown, that parts of Hsmr are remarkably mobile in the membrane and that this mobility can be limited by the addition of the substrate ethidium bromide. Ethidium bromide as well as tetraphenylphosphonium (TPP+) is typical multidrug transporter substrates. The membrane interaction of TPP+ in DMPC membranes has been resolved by 1H MAS NMR. It was found that it penetrates into the interface region of the lipid bilayers and therefore behaves like many other transporter substrates adding to the hypothesis that the membrane could act as a pre-sorting filter. Finally, Chapter 9 is dedicated to the characterisation of the essential and highly conserved residue Glu-14 in EmrE by solid-state NMR. In order to avoid spectral overlap, the single Glu EmrE E25A mutant was chosen instead of the wildtype. The protein has been produced in vitro to take advantage of reduced isotope scrambling in the cell free expression system as verified by analytical NMR spectroscopy. Correct labelling of EmrE was tested by MALDI-TOF and solid-state NMR. The dimeric state of DDM solubilised EmrE has been probed by LILBID. The labelled protein was reconstituted into E. coli lipids to ensure a native membrane environment. Activity was determined by measuring ethidium bromide transport. Freeze fracture EM revealed very homogeneous protein incorporation even after many days of MAS NMR experiments. 2D 13C double quantum filtered experiments were used to obtain chemical shift and lineshape information of Glu-14 in EmrE. Two distinct populations were found with backbone chemical shift differences of 4 - 6 ppm which change upon substrate binding. These findings indicate a structural asymmetry at the assumed dimerisation interface and are discussed in the context of a model for shared substrate/proton binding. These studies represent the first successful use of cell free expression to prepare labelled membrane proteins for solid-state NMR and allow for the first time an NMR insight into the binding pocket of a multidrug efflux pump.
Biological membranes separate the cell interior from the outside and have diverse functions from signal transduction, apoptosis to transportations of ions and small molecules in and out of the cell. Most of these functions are fulfilled by proteins incorporated in the membrane. However, lipids as the main component of membrane not only serve as structural element for bilayer formation but they are also directly involved e.g. signalling processes and bilayer properties are important to mediate protein interactions. To fully understand the role of lipids, it is necessary to develop a molecular understanding of how certain membrane components modify bulk bilayer structure and dynamics. Membranes are known to have many different motions in different conditions and time scales. Temperature, pH, water content and many other conditions change membrane dynamics in a high degree. In addition to this, time scales of motions in membranes vary from ns to ms range corresponding to fast motion and slow motion, respectively. Therefore, membranes are needed to be studied systematically by varying the conditions and using methods to investigate motions in various time scales separately. The aim of this study was therefore perform a combined solid-state NMR / molecular dynamics study on model membranes. Different substrates, such as potential drugs, polarizing agents and signaling lipids were incorporated into bilayers and their location within the membrane and their effect onto the membrane was probed. NSAIDs (non-steroidal anti-inflammatory drugs), pirinixic acid derivatives, ceramides and polarizing agents were the substrates for membranes in this study. There were several experimental methods that were applied in order to investigate effects of these substrates on membrane dynamics. Different kind of phospholipids including POPC, DMPC and DPPC were used. In addition to experimental work, with the information gathered from solid state NMR experiments molecular dynamics simulations were performed to obtain more information about the membranes at the molecular level. As a result, combination of solid-state NMR with molecular dynamics simulations provides very systematic way of investigating membrane dynamics in a large range of time scales.
Pirinixic acid derivatives were special interest of this study because of their activity on peroxisome proliferator-activated receptor (PPAR) as an agonist as well as on enzymes of microsomal prostaglandin E2 synthase-1 (PGE2s) -1 and 5-lipoxygenase (5-LO) as dual inhibitor. Two potent pirinixic acid derivatives, 2-(4-chloro-6-(quinolin-6-ylamino)pyrimidin-2-ylthio)octanoic acid (compound 2) and 2-(4-chloro-6-(quinolin-6-ylamino)pyrimidin-2-ylthio)octanoate (compound 3), have been worked and their insertion depts were investigated by combining of solid state NMR and molecular dynamics simulations. Both experimental and theoretical results pointed out that compound 3 was inserted the phospholipid bilayer more deeply than 2. NSAIDs – lipid mixtures have been also studied here. It is known that consumption of NSAIDs as in mixture with lipids results much fewer side effects than consumption of the drugs alone. Thus, it is crucial to understand interactions of NSAIDs with lipids and investigate the possible complex formation of drugs with lipids. In this study, interactions of three widely used NSAIDs, ibuprofen, diclofenac and piroxicam, with DPPC were investigated by solid-state NMR. 1H and 31P NMR results depicted that ibuprofen and diclofenac had interactions with lipids, which is an indication of drug-lipid complex formation whereas piroxicam didn’t show any interactions with lipids suggesting that no complex formation occurred in the case of piroxicam. Ceramides are known to play key roles in many cell processes and many studies showed that the functions of ceramides are related with the ceramide effects on biological membranes. Therefore, in this study, influences of ceramides on biophysics of lipid bilayers were investigated by using various solid state NMR techniques and molecular dynamics simulations. Results from molecular dynamics simulations clearly showed that ceramide and lipids have strong interactions. More evidences about ceramide-lipid interactions were provided from 1H and 14N NMR results. In addition, it was indicated by both simulation and experimental methods that ceramide increased the rigidity of DMPC by increasing chain order parameters. BTbk is a biradical, which is used as polarizing agent for dynamic nuclear polarization (DNP) experiments and found to be more efficient than other widely used polarizing agents such as TOTAPOL. Since it is a hydrophobic compound, which prefers to stay inside lipid bilayer it is important to investigate the location and orientation of bTbk along the bilayer in order to understand its enhancement profile in DNP measurements. In this study, both NMR relaxation time measurements and molecular dynamics simulations revealed that bTbk tends to stay more close to hydrophobic chain of lipids than the interfacial part of lipids at bilayer surface.
In the first part of this work, a brief introduction on lipid membranes as well as a theoretical summary on both methods of solid-state NMR and molecular dynamics simulations is given. Then, in the second part methodology is introduced for both solid-state NMR spectrometer and theoretical calculations. Afterwards, results of different membrane systems are discussed in the following parts for both solid state NMR and MD. Finally, in the last part, a summary and the conclusion of the overall results together with some future plans are explained.
Die Familie der ubiquitären ATP binding cassette (ABC)-Membranproteine katalysiert unter Hydrolyse von ATP die Translokation von Substraten über biologische Membranen. In der hier vorliegenden Arbeit wurde die Struktur und Funktion des osmoprotectant uptake (Opu) Systems A aus B. subtilis untersucht, das aus drei Untereinheiten, der ATPase OpuAA, dem integralen Membranprotein OpuAB und dem Substrat-Bindeprotein OpuAC, besteht und unter hyperosmolaren Bedingungen die kompatiblen Solute Glycin-Betain (GB) und Prolin-Betain (PB) in die Zelle importiert, um eine Plasmolyse zu verhindern. Sämtliche Untereinheiten wurden getrennt oder als OpuAA/AB Komplex in E. coli überproduziert und bis zur Homogenität isoliert. OpuAA zeigte ein dynamisches Monomer-Dimer Gleichgewicht (KD= 6 µM), das durch Nukleotide beeinflusst wurde. Unter Bedingungen hoher Ionenstärke konnten Monomer und Dimer getrennt isoliert und analysiert werden. Die Affinitäten und Stöchiometrien der OpuAA/Nukleotid Komplexe wurden unter Verwendung des fluoreszierenden TNP-ATP bzw. einer Nukleotid-sensitiven Trp-Mutante des OpuAA untersucht. Das Monomer hatte ein Molekül TNP-ATP gebunden, während zwei Moleküle TNP-ATP in dimerem OpuAA detektiert wurden. Die Affinität von Nukleotiden zu OpuAA nahm in folgender Reihe zu: ATP<ATP/Mg2+<ADP/Mg2+. Eine Erhöhung der Ionenstärke bewirkte nicht nur eine Erniedrigung der KD-Werte von OpuAA/Nukleotid Komplexen, sondern auch eine Steigerung der ATPase Aktivität. In 1 M NaCl zeigte das Monomer basale ATPase Aktivität, während das Dimer nur sehr geringe Aktivität hatte, jedoch durch Zugabe von OpuAB und OpuAC aktiviert wurde. K+ wurde als ein Modulator der ATPase Aktivität von OpuAA identifiziert. Die Zugabe von TNP-ADP/Mg2+ induzierte in dimeren OpuAA einen konformellen Wechsel, der zu einem Zerfall des Dimers führte. Monomer und Dimer hatten gegenüber Nukleotiden unterschiedliche Affinitäten, was eine unterschiedliche Architektur der Nukleotid-Bindetasche implizierte. Die Architektur des OpuAA Dimers wurde mittels FRET untersucht. Dazu wurde OpuAA ortspezifisch mit Fluorophoren markiert und ein Verfahren etabliert, in dem die intermolekularen Distanzen des Dimers bestimmt werden konnten. Ein Vergleich der Distanzen mit anderen NBD Dimeren zeigte, dass OpuAA eine zu BtuD oder MalKE. coli vergleichbare Dimer Architektur mit einer head-to-tail Orientierung hat. Die Struktur des OpuAC/GB und OpuAC/PB Komplexes wurde durch Röntgenstrukturanalyse mit einer Auflösung von 2,7 Å bzw. 2,8 Å aufgeklärt und zeigte zwei globuläre Domänen, die über zwei Peptidsegmente miteinander verbunden waren. Die delokalisierte positive Ladung des Liganden war von einem cluster aus drei Trp-Resten, dem sog. "Tryptophan-Prisma", über kationische-p-Interaktion komplexiert. Nach Ligandenbindung wurden beide Domänen durch eine Wasserstoffbrücke zwischen den konservierten Asp22 und Trp178 überbrückt. Dieser molekulare Schalter wurde von OpuAC genutzt, um Affinitäten von GB und PB zu regulieren.
Proteorhodopsin (PR) originally isolated from uncultivated γ-Proteobacterium as a result of biodiversity screens, is highly abundant ocean wide. PR, a Type I retinal binding protein with 26% sequence identity, is a bacterial homologue of Bacteriorhodopsin (BR). The members within this family share about 78% of sequence identity and display a 40 nm difference in the absorption spectra. This property of the PR family members provides an excellent model system for understanding the mechanism of spectral tuning. Functionally PR is a photoactive proton pump and is suggested to exhibit a pH dependent vectorality of proton transfer. This raises questions about its potential role as pH dependent regulator. The abundance of PR in huge numbers within the cell, its widespread distribution ocean wide at different depths hints towards the involvement of PR in utilization of solar energy, energy metabolism and carbon recycling in the Sea. Contrary to BR, which is known to be a natural 2D crystal, no such information is available for PR til date. Neither its functional mechanism nor its 3D structure has been resolved so far. This PhD project is an attempt to gain a deeper insight so as to understand structural and functional characterization of PR. The approach combines the potentials of 2D crystallography, Atomic Force Microscopy and Solid State NMR techniques for characterization of this protein. Wide range of crystalline conditions was obtained as a result of 2D crystallization screens. This hints towards dominant protein protein interactions. Considering the high number of PR molecules reported per cell, it is likely that driven by such interactions, the protein has a native dense packing in the environment. The projection map represented low resolution of these crystals but suggested a donut shape oligomeric arrangement of protein in a hexagonal lattice with unit cell size of 87Å*87Å. Preliminary FTIR measurements indicated that the crystalline environment does not obstruct the photocycle of PR and K as well as M intermediate states could be identified. Single molecule force spectroscopy and atomic force microscopy on these 2D crystals was used to probe further information about the oligomeric state and nature of unfolding. The data revealed that protein predominantly exists as hexamers in crystalline as well as densely reconstituted regions but a small percentage of pentamers is also observed. The unfolding mechanism was similar to the other relatively well-characterized members of rhodopsin family. A good correlation of the atomic force microscopy and the electron microscopy data was achieved. Solid State NMR of the isotopically labeled 2D crystalline preparations using uniformly and selectively labeling schemes, allowed to obtain high quality SSNMR spectra with typical 15N line width in the range of 0.6-1.2 ppm. The measured 15N chemical shift value of the Schiff base in the 2D crystalline form was observed to be similar to the Schiff base chemical shift values for the functionally active reconstituted samples. This provides an indirect evidence for the active functionality of the protein and hence the folding. The first 15N assignment has been achieved for the Tryptophan with the help of Rotational Echo Double Resonance experiments. The 2D Cross Polarization Lee Goldberg measurements reflect the dynamic state of the protein inspite of restricted mobility in the crystalline state. The behavior of lipids as measured by 31P from the lipid head group showed that the lipids are not tightly bound to the protein but behave more like the lipid bilayer. The 13C-13C homonulear correlation experiments with optimized mixing time based on build up curve analysis, suggest that it is possible to observe individual resonances as seen in case of glutamic acid. The signal to noise was good enough to record a decent spectrum in a feasible period. The selective unlabeling is an efficient method for reduction in the spectral overlap. However, more efficient labeling schemes are required for further characterization. The present spectral resolution is good for individual amino acid investigation but for uniformly labeled samples, further improvement is required.
Die 5-Lipoxygenase (5-LO) ist eines der Schlüsselenzyme der Leukotrienbiosynthese. Sie katalysiert zunächst die Umsetzung der freigesetzten Arachidonsäure(AA) zu 5-Hydroperoxyeicosatetraensäure (5-HpETE), in einem zweiten Reaktionsschritt wandelt sie diese in Leukotrien A4 (LTA4) um. Leukotriene sind potente Entzündungsmediatoren und spielen eine wichtige Rolle bei entzündlichen und allergischen Reaktionen. Außerdem wird die Beteiligung an verschiedenen Krebsarten kontrovers diskutiert.
Sie besteht aus 673AS, ist 78 kDa schwer und gliedert sich wie alle bisher bekannten Lipoxygenasen in eine N-terminale C2-ähnliche, regulatorische Domäne(AS 1–114) (C2ld), die für die Membran- und Calciumbindung sowie die Interaktion mit dem Coactosin-like Protein (CLP) verantwortlich ist, und in eine C-terminale, katalytische Domäne (AS 121–673), die das Nicht-Häm-gebundene Eisen im aktiven Zentrum trägt. Ein weiteres Strukturmerkmal sind zwei ATP-Bindungsregionen, eine befindet sich in der C2ld (AS 73–83), die andere auf der katalytischen Domäne (AS 193–209), das molare Verhältnis von 5-LO zu ATP konnte dabei auf 1:1 festgelegt werden [167].
Bereits 1982 wurde in einer Veröffentlichung von Parker et al. beschrieben, dass 5-LO aus Rattenzellen in Gegenwart von Calcium auf einer Gelfiltration dimerisieren kann [204], 2008 schließlich wurde von Aleem et al. publiziert, dass humane 12-LO aus Thrombozyten Dimere bilden kann [219]. Somit konnte es möglich sein, dass auch die humane 5-LO zur Dimerisierung fähig ist.
Zunächst wurde aufgereinigtes Enzym mit nativer Gelelektrophorese und anschließender Coomassiefärbung oder Western Blot untersucht, dabei konnten mehrere Banden pro Bahn detektiert werden. Um dieses Phänomen weiter zu untersuchen, wurde im Anschluss eine Gelfiltration etabliert; da die C2ld der 5-LO recht hydrophob ist, war es nötig, 0,5% T20 zum Elutionspuffer PBS/EDTA zuzusetzen, da das Enzym ansonsten unspezifisch mit dem Säulenmaterial interagiert und für seine Größe zu spät eluiert hätte. In Anwesenheit von T20 eluierte 5-LO in zwei getrennten Peaks, die exakt zu den vorher mit Referenzproteinen bestimmten Elutionsvolumina des Monomers und Dimers passten. Weiter wurde getestet, ob niedermolekulare Substanzen einen Einfluss auf das Dimerisierungsverhalten haben, allerdings konnte weder durch Ca2+noch durch ATP eine Verstärkung der Dimerisierung beobachtet werden. Dahingegen konnte, nach Vorinkubation mit GSH und Diamid, das alleinige Monomer auf der Gelfiltration nachgewiesen werden, nach Vorinkubation nur mit Diamid, lag das gesamte Protein ausschließlich als Dimer vor. Durch Gelelektrophorese mit oder ohne Zusatz von ß-Mercaptoethanol und LILBID-MS konnte die Ausbildung von intermolekularen Disulfidbrücken bestätigt werden. Ein Bindungsassay mit radioaktivem 35S-GSH konnte die kovalente Bindung des GSH an die 5-LO bestätigen. Quantifizierungsstudien mit Ellmans Reagens zeigten, dass mindestens eins der Oberflächencysteine mit GSH modifiziert wurde. Die von der Gelfiltration erhaltenen Fraktionen wurden auf enzymatische Aktivität getestet und in allen 5-LO-haltigen Fraktionen konnte Aktivität gefunden werden. Leider war es nicht möglich, eine Aussage darüber zu treffen, ob das Mono- oder das Dimer aktiver war. Es liegt offenbar in einem Fließgleichgewicht vor, da erneute Injektion des Monomerpeaks im bekannten Elutionsprofil aus zwei Peaks resultierte. Außerdem führt die Anwesenheit von 0,5% T20 während des Aktivitätstests zu einer Hemmung des Enzyms und weniger detektierbaren 5-LO-Produkten; es fiel vor allem auf, dass so gut wie keinerlei trans- und epitrans-LTB4, die nicht-enzymatischen Zerfallprodukte der 5-HpETE, nachzuweisen waren. Betrachtet man die Struktur der 5-LO, so findet man zehn Cysteine an der Oberfläche; die Cysteine 159, 300, 416 und 418 liegen dabei in einem Interface. Mutiert man diese Cysteine zu Serinen, so verschwindet der Dimer-induzierende Effekt des Diamids, wohingegen die Mutante weiterhin glutathionylierbar bleibt. Interessanterweise zeigt diese Mutante auch eine wesentlich weniger ausgeprägte Hemmung durch T20. Um eine Aussage treffen zu können, ob auch 5-LO aus humanen Zellen Dimere bilden kann, wurde 5-LO-haltiger S100 aus polymorphkernigen Leukozyten (PMNL) untersucht. Dabei konnte mit Western Blot und einem Aktivitätsnachweis gezeigt werden, dass die 5-LO in einem breiten Bereich von der Gelfiltration eluiert. Das deutet darauf hin, dass sie in PMNL ebenfalls dimerisiert vorliegen kann. In Gegenwart von Ca2+kam es zu einer Verschiebung der 5-LO zu höhermolekularen Gewichten, wobei dieses Phänomen nicht bei S100 aus transformierten E.coli auftrat, was auf einen gerichteten Komplex nach Calciuminduktion in PMNL hindeutet.
Außerdem wurde im Rahmen dieser Arbeit der Bindemodus von Sulindac an die 5-LO mittels Crosslinking untersucht. Dabei konnte gezeigt werden, dass konzentrationsabhängig der einfache Komplex aus 5-LO und CLP abnimmt, dafür aber ein hochmolekularer Komplex, der beide Enzyme enthält, entsteht. Weder das Prodrug Sulindac noch der weitere Metabolit Sulindacsulfon oder andere Inhibitoren, die ebenfalls an der C2ld angreifen sollen, zeigten diesen Effekt. Leider konnte nicht weiter geklärt werden, was diesen Effekt verursacht, allerdings liegt die Vermutung nahe, dass es zu einer Aggregation kommt. Weitere Untersuchungen könnten wichtige Hinweise auf das Design von neuen Arzneistoffen bringen, um selektivere und damit nebenwirkungsärmere Inhibitoren zu finden.
Integral membrane proteins (IMPs) account for 20-40% of all open reading frames in fully sequenced genomes and they are target of approximately 60% of all modern drugs. So far, cellular expression systems are often very insufficient for the high-level production of IMPs. Toxic effects, instability or formation of inclusion bodies are frequently observed effects that prevent the synthesis of sufficient amounts of functional protein. I have successfully established an individual cell-free (CF) expression system to overcome these IMP synthesis difficulties. The CF system was established in two different expression modes. If no hydrophobic compartment is provided, the IMPs precipitate in the reaction mixture. Interestingly, these insoluble proteins are found to differ from inclusion bodies as they readily solubilize in mild detergents and the bacterial small multi drug transporter EmrE, expressed in the insoluble mode was shown to reconstitute into liposomes in an active form. Alternatively, IMPs can be synthesized in a soluble way by supplementing the CF system with detergents. A comprehensive overview of 24 commonly used detergents was provided by analyzing their impact on the CF system as well as their ability to keep three structurally very different proteins in solution. The class of long chain polyoxyethylene-alkyl-ethers turned out to be most suitable for soluble expression of a-helical EmrE, the bacterial b-barrel type nucleoside transporter Tsx and the porcine vasopressin receptor type 2, resulting in several mg of protein per mL of reaction mixture. So far IMPs have almost completely been excluded from solution nuclear magnetic resonance (NMR) analyses. I could demonstrate that CF expression enables efficient isotopic labeling of IMPs for NMR analysis and further facilitates selective labeling strategies with combinations of 13C and 15N enriched amino acids that have not been feasible before. Four different G-protein coupled receptors (GPCRs) were successfully CF expressed in preparative scale and for the human endothelin B receptor (ETB), ligand binding ability was observed. A series of truncated ETB derivatives containing nested terminal deletions have been CF produced and functionally characterized. The core area essential for Endothelin-1 binding as well as a central region responsible for ETB oligomer formation was confined to a 39 amino acid fragment including the proposed transmembrane segment 1. The binding constant (KD) of ETB was determined to 6 nM for circular ET-1 by SPR and 29 nM for linear ET-1 by TIRFS. This data indicate a large potential of the established individual CF expression system for functional IMP synthesis.
The transporter associated with antigen processing-like (TAPL) acts as a lysosomal ATP-dependent polypeptide transporter with broad length selectivity. To characterize in detail its substrate specificity, a procedure for solubilization, purification and functional reconstitution of human TAPL was developed. TAPL was expressed in Sf9 insect cells with the baculovirus expression system and solubilized from crude membranes. By intensive screening of detergents, the mild non-ionic detergents digitonin and dodecylmaltoside were found to be ideal for solubilization with respect to efficiency, long term stability, and functionality of TAPL. TAPL was isolated in a two-step procedure with a yield of 500 micro g/L cell culture and, subsequently, reconstituted into proteoliposomes. The KM(pep) for the peptide RRYCfKSTEL (f refers to fluorescence label) and KM(ATP) were determined to be 10.5 ± 2.3 micro M and 97.6 ± 27.5 micro M, respectively, which are in the same range as the Michaelis-Menten constants determined in the membranes. The peptide transport activity of the reconstituted TAPL strongly depends on the lipid composition. Interestingly, the E. coli lipids are prefered over other tested natural lipids extracts. Moreover, phosphatidylcholine, the most abundant phospholipid in eukaryotic cells influenced TAPL activity in a dose dependent manner. In addition, some negatively charged lipids like DOPA and DOPS increased peptide transport activity with preference for DOPS. However, DOPE or egg PG which are also negatively charged had no effect. It seems not only the charge but also the specific head group of phospholipids that has impact on the function of TAPL. With the help of combinatorial peptide libraries containing D-amino acid residues at defined positions as well as bulky fluorescein labeled peptides, the key positions of the peptides were localized to the N- and C-terminal residues with respect to peptide transport. The C-terminal position has the strongest selectivity since modification at this position shows strongest impact on peptide transport. Additionally, positions 2 and 3 of the peptide also have weak influence on peptide selectivity. Subsequently, the residue preferences at the key positions were systematically investigated by combinatorial peptide libraries with defined residues at certain positions. At both ends, TAPL favors positively charged, aromatic, or hydrophobic residues and disfavors negatively charged residues as well as asparagine and methionine. The residue preferences at the key positions are valid for peptide substrates with different length, indicating a general rule for TAPL selectivity. Besides specific interactions of both terminal residues, electrostatic interactions are important, since peptides with positive net charge are more efficiently transported than negatively charged ones. By size exclusion chromatography (SEC) and blue native PAGE, TAPL purified in the presence of digitonin or dodecylmaltoside had an apparent molecular weight of 200 kDa which is close to the theoretical molecular mass of the TAPL homodimer (172 kDa). The purified and reconstituted TAPL showed specific ATP hydrolysis activity which can be inhibited by orthovanadate. TAPL in proteoliposomes showed 6-fold higher ATP hydrolysis than digitonin solubilized protein, indicating the phospholipids impact on TAPL function. However, no peptide substrate stimulated ATPase activity was observed. For site-specific labeling of TAPL, eight cysteines in each half transporter were replaced by alanine or valine. The TAPL cys-less mutant showed the same peptide transport activity as TAPL wt. Based on the functional TAPL cys-less mutant, seven single cysteine mutants were introduced into strategic positions. All single cysteine mutants in the TMD did not influence peptide transport, whereas the mutant L701C, which is close to the conserved H-loop motif, displayed impaired transport. TAPL orthologs Haf-4 and Haf-9 from Caenorhabditis elegans possess around 40% sequence identities with TAPL and 50% with each other. Both proteins are putative half transporters and reported to be involved in the intestinal granule formation (Bauer, 2006; Kawai et al., 2009). To further understand the physiological functions of these two proteins, they were expressed in Sf9 insect cells. Haf-4 and Haf-9 showed weak but specific ATP- and peptide-dependent peptide transport activity for the given peptide RRYCfKSTEL. Therefore, it was proposed that the physiological roles for Haf-4 and Haf-9 might be related to their peptide transport activity. Besides forming functional homodimeric complex as estimated by the peptide transport activities, both half transporter could also form heteromers which was confirmed by coimmunoprecipitation. However, the heteromers showed decreased transport activity.
Solid state NMR is a emerging method for the study of membrane proteins, which has received much interest in recent years. Limiting the study of many pharmacologically relevant targets, are the often long measuring times, required to obtain especially higher dimensional solid state NMR spectra of good quality. To address this problem, multiple methods where developed in this work, which can be categorized into two groups. The first set of methods aims at the quality of certain spectra, by implementing a spectral filter, which increases the fidelity of the measured data. The second set of methods, addresses the problem of long measuring times directly, by increasing the sensitivity per unit time, as could be shown, for example, on homo- and heteronuclear singlequantum-singlequantum correlation experiments. The gains in measuring time for the latter group of methods are typically in the order of 2-3, but some experiments allow multiple methods to be employed simultaneously, which can lead to a decrease in measuring time of a factor of up to 8. It is important to mention, that none of the methods introduced in this work require any equipment in addition to the conventional setup present in most sold state NMR laboratories and no changes or addition to the samples under study are required. Therefore the gains reported in this work come at no extra cost and require only minimal implementation effort on the side of the user.
In this thesis the integral membrane protein diacylglycerol kinase (DAGK) from E.coli is investigated with solid-state NMR. The aim is to gain an insight into the enzyme’s mechanism through integration of kinetic, structural and dynamic data. The biological function of DAGK is the transfer of the γ-phosphate group from Mg*ATP to diacylglycerol (DAG) building phosphatidic acid (PA)[6] as port of the membrane-derived oligosaccharide cycle[31,34]. Surprisingly, DAGK does not share structural or sequential similarities with other kinases[12]. Typical sequence motives found in other kinases, which catalyze phosphoryl transfer reactions, are not found[13]. In its physiological form DAGK is a homo-trimer with nine transmembrane helices, three catalytic centers and a size of 39.6 kDa.
First, the set-up of a real-time 31P MAS NMR experiment is shown. This experiment allows measuring in real-time the simultaneous ATP hydrolysis in the aqueous phase and lipid substrate phos-phorylation in the membrane phase with atomic resolution under magic angle spinning[56]. After fast transfer of the sample into the NMR spectrometer the enzymatic reaction is started with a temperature jump. This approach of real-time MAS NMR in a dual-phase system was demonstrated for the lipid substrate analogs dioleoyl- (DOG) and dibutyrylglycerol (DBG), with a C8 and C4 aliphatic chain, respectively. The combination of 31P direct and cross polarization functions as a dynamic filter. In the 31P direct polarized experiment nuclei in both phases are detected, while in the 31P cross polar-ized experiment, only nuclei in the membrane phase are detected. Rates for substrate turnover, i.e. degradation of γP-, βP, αP-ATP and build-up of βP-, αP-ADP, free phosphate as side reaction, and PA are obtained, which reveal a Michaelis-Menten behavior with regard to Mg*ATP and DBG. Here Mg*ATP and DBG follow a random-equilibrium model, where every substrate can bind indepen-dently from the other substrate. Analyses of the peak integrals from educts and products of the enzymatic reaction, revealed the stoichiometry of the reaction: 1.5 ATP molecules are used to phos-phorylate one DBG molecule. The excess of ATP is attributed to the basal ATPase activity. Further-more, experiments with ATPγS, usually regarded as a non-hydrolysable ATP-analog, where carried out. Surprisingly, DAGK hydrolyzes ATPγS and also transfers the thio-phosphate group to the lipid acceptor DBG, which points to a certain degree of plasticity in the active center. A phosphorylated enzyme intermediate was not detected. These results suggest the building of a ternary complex of Mg*ATP, DBG and DAGK performing a direct-phosphoryl transfer reaction, without passing through a phosphorylated enzyme intermediate. Experiments with the transition state analog ortho-vanadate (Vi) showed a decoupling of the ATP hydrolysis activity from lipid substrate phosphorylation. This indicates a specific transfer site for the γ-phosphate group from ATP to DAG, which can be blocked by Vi.
A general disadvantage of NMR spectroscopy compared to other spectroscopic methods is its inherent low sensitivity. One possible starting point for the improvement of signal-to-noise per unit time is the reduction of the spin-lattice relaxation time of protons[209]. Usually 95 % of the experi-mental time is required for the relaxation of the 1H to equilibrium. The addition of paramagnetic species can be used to reduce the 1H T1[233]. In a comprehensive study four different paramagnetic agents were tested: Cu2+-EDTA, Cu2+-EDTA-tag, Gd3+-TTAHA and Gd3+-DOTA. The titration of these paramagnetic complexes showed the principle feasibility of this approach, but differences between the tested species exist. The most promising complex is Gd3+-DOTA which, at a concentration of 2 mM, causes a 10-time improvement of signal-to-noise ratio per unit time. This allowed measuring 2D 13C-13C correlation spectra of proteoliposomes in one tenth of the usual required experimental time (i.e. 10 hours vs. 4 days) with good signal-to-noise.
For the investigation of structural or dynamic changes in the protein upon substrate interaction with MAS NMR, the spectral properties CP efficiency and resolution of the DAGK in liposomes needed to be improved. The most critical step during sample preparation is the reconstitution of the membrane protein from detergent micelles into a membrane of synthetic lipids under detergent removal. For this procedure the important criteria are enzymatic activity, measured in a coupled ATPase assay[55], and homogeneity of the proteoliposomes, which was tested e.g. on a discontinuous sucrose step gradient. Therefore an extensive study was carried out, in which different detergents, lipids and lipid mixtures, techniques for detergent removal and different protein-to-lipid ratios were tested. A direct correlation between high ATPase activity and good resolution was not found. Moreover, active DAGK in a mixture of DMPC and cholesterol, which emulates the membrane features of a membrane containing DAG, showed the best CP efficiency and resolution.
The assignment of the protein backbone and amino acid side chains the first mandatory step towards the investigation of structural and dynamical features influencing and defining the enzymatic mechanism by MAS NMR. As the assignment procedure is very time consuming for a total protein, a special labeling scheme for DAGK was developed, which allows assigning most of the protein areas presumably involved in enzyme catalysis. The assignment of DAGK with solution NMR[132] was not transferable to the MAS NMR spectra. Most important for the assignment process were the unique pairs[335], two consecutive amino acids which only appear once in the amino acid sequence. These unique pairs served as anchor points. Five different multinuclear MAS NMR experiments (DARR, NCO, NCA, NCACX, NCOCX) were required for the sequential assignment. It was possible to assign 35 % of the total amino acid sequence with one sample and 8 experiments acquired at 850 MHz. The secondary structure analysis showed subtle differences to the DAGK assignment with solution NMR[132], which can be attributed to the different environment in lipid bilayers and detergent micelles.
Data about structural and dynamical changes under substrate interaction can reveal details about the enzymatic mechanism. Therefore changes in chemical shift in 2D heteronuclear correlation experiments in the apo-state and under substrate saturated conditions with the substrates Mg*AMP-PNP, a non-hydrolysable ATP-analog, DOG, a mixture of Mg*AMP-PNP and DOG as well as inhibited by Vi were recorded. The most significant peak changes were observed at the interface membrane-cytoplasm as well as the the N-terminal amphipathic helix. The residues revealing chemical shift perturbations correlate with conserved residues or such residues, for which importance for catalysis and/or folding could be shown in mutation studies[8]. Especially noticeable were the changes at the amino acids Asn 72, Lys 64, His 87, Tyr 86 and Asp 95.
Beside changes of the chemical shift, changes of line width or signal doubling were observable. These changes can point to a correlation with dynamic reorientations in the μs-ms time regime, which are most relevant for enzymatic processes. The protein backbone dynamics in the apo-state as well as saturated with the substrates or inhibited with Vi were investigated with a 15N-CODEX experiment, which is based on the reorientation of the CSA tensor upon dynamical changes[350]. Specific effects of the different substrates or analogs on the protein backbone dynamic were revealed complementing the structural data and the chemical shift perturbation experiments.