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Three-dimensional structure of the glycine-betaine transporter BetP by cryo electron crystallography
(2008)
The soil bacterium Corynebacterium glutamicum has five secondary transporters for compatible solutes allowing it to cope with osmotic stress. The most abundant of them, the transporter BetP, performs a high affinity uptake of glycine-betain when encountering hyperosmotic stress. BetP belongs to the betaine/carnitine/choline/transporter (BCCT) family, and is predicted to have twelve transmembrane helices with both termini facing the cytoplasm. The goal of this thesis is to facilitate understanding of BetP function by determining a three dimensional (3D) model of its structure. Two-dimensional (2D) crystallization of wild-type (WT) BetP has been successfully performed by reconstitution into a mixture of E. coli lipids and bovine cardiolipin, which resulted in vesicular crystals diffracting to 7.5 Å resolution (Ziegler, Morbach et al. 2004). Diffraction patterns of these crystals however showed unfocused spots, generally due to high mosaicity. Better results were obtained by using the constitutively active mutant BetPdeltaC45 in which the first 45 amino acids of the positively charged C-terminus were removed. BetPdeltaC45 crystals obtained under the same conditions for BetP WT were concluded to be pseudo crystals, based on the inconsistence of symmetry. These crystals had BetPdeltaC45 molecules randomly up/downwards inserted into membrane crystals, and cannot be used for structure determination, even though they diffracted up to 7 Å. The problem of pseudo crystal formation could be solved by changing the lipids used for 2D crystallization to a native lipid extract from C. glutamicum cells. This change of lipids improved the crystals to well-ordered packing with exclusive p121_b symmetry. To understand the role of lipids in crystal packing and order, lipids were extracted at different stages during crystallization, and identified by using multiple precursor ion scanning mass spectrometry. The results show that phosphatidyl glycerol (PG) 16:0-18:1 is the most dominant lipid species in C. glutamicum membranes, and that BetP has a preference for the fatty acid moieties 16:0-18:1. Crystallization with synthetic PG 16:0-18:1 proved that an excess of this lipid prevents pseudo crystal formation, but these crystals did not reach the quality as previously achieved by using the C. glutamicum lipids. Apart from the effect of lipids in crystallinity, the concentration and type of salts influenced crystal growth and morphology. High salt conditions (>400 mM LiCl or KCl) yielded tubular crystals, whereas low salt conditions (<300 mM LiCl, NaCl or KCl) led to formation of up to 10 µm large sheet-like crystals. The intermediate concentration gave a mixture of sheet-like and tubular crystals. In terms of resolution, sheets diffracted better than tubes. The sheet-like crystals used for 3D map reconstruction were obtained from a dialysis buffer containing 200 mM NaCl combined with using C. glutamicum lipids. Electron microscopic images were taken from frozen-hydrated crystals using a helium-cooled JEOL 300 SFF microscope or a liquid nitrogen-cooled FEI Tecnai G2 microscope at 300 kV, which allowed optimal data collection and minimized radiation damage to the sample. More than 1000 images of tilt angles up to 50° were taken and evaluated using optical diffraction of a laser beam. The best 200 images were processed with the MRC image processing software package, and 79 images from different tilt angles were merged to the final data set used for calculation of a 3D map at a planar resolution of 8 Å. The structure shows BetPdeltaC45 as a trimer with each monomer consisting of 12 transmembrane alpha-helices. Protein termini and loop regions could not be determined due to the limited resolution of the map. Six of the twelve helices line a central cavity forming a potential substrate-binding chamber. Each monomer shows a central cavity in different sizes and shapes. Thus, the constitutively active BetPdeltaC45 thus forms an unusual asymmetric homotrimer. BetP most likely reflects three different conformational states of secondary transporters: the cytoplasmically open (C), the occluded (O), and the periplasmically open (P) states. The C and O states are similar to BetP WT projection structure, while the P state is discrepant and highly flexible due to the shape and size of the central cavity as well as the lowest intensity of the density. The observation of the P state corresponds well to the constitutively active property of BetPdeltaC45. For the high resolution structure of the C and O states are available, this work presents the first structural information of the P state of a secondary transporter.
In bestimmten methanogenen Archaea wurde vor einigen Jahren eine metallfreie Hydrogenase gefunden, die den reversiblen und stereoselektiven Transfer eines Hydridions von Wasserstoff auf die an den C1-Carrier Tetrahydroniethanopterin (H4MPT) gebundene Methenyl-Gruppe katalysiert. Damit stellt dieses Enzym den ersten und einzigen rein organischen Hydrogenierungskatalysator dar, den man in der Natur kennt. Ziel der vorgelegten Arbeit war die kristallographische Bestimmung der Enzymstruktur. Versuche zur Strukturlösung des in aktiver Form aus M. marburgensis isolierten Enzyms durch mehrfachen isomorphen Ersatz, über die anomale Dispersion an nicht-isomorphen Quecksilberderivaten und die des Selens an mit Selenomethionin markiertem Enzym verliefen nicht erfolgreich. Ursächlich hierfür war die perfekte meroedrische Zwillingsbildung der Kristalle. Für die beiden heterolog produzierten, inaktiven Apoenzyme aus den Hyperthermophilen M. jannaschii und M. kandleri wurden in dieser Arbeit effektive Expressions- und Reinigungsprotokolle entwickelt. Für das Enzym aus M. jannaschii wurden Mikrokristalle erhalten, die lediglich ein Proteolysefragment von etwa der halben Masse des Vollängenproteins enthalten. Kristalle des Enzyms aus M. kandleri konnten durch serielles Microseeding so weit verbessert werden, daß die Durchführung eines MAD-Experiment möglich wurde. Erst unter Verwendung vor kurzem entwickelter direkter Methoden (Shake-and-Bake) gelang die Strukturlösung bei einer Auflösung von 2.8 Å. Die Monomere bilden ein sehr eng assoziiertes Homodimer; zwei dieser Dimere sind zu einem locker assoziierten Tetramer verbunden. Jedes Monomer besitzt zwei Domänen. Die N-terminale Domäne von etwa 255 Resten besitzt eine Faltung, wie sie für Dinukleotid-bindende Enzyme typisch ist, mit einem zentralen, verdrehten achtsträngigen beta-Faltblatt. Die C-terminale Domäne von etwa 100 Resten besitzt dagegen weitgehend alpha-helikale Struktur und ist für die außerordentlich enge Assoziation des Homodimers verantwortlich. Beide Domänen sind durch eine gestreckte, flexible Verbindung verknüpft. Im Dimer entstehen dadurch zwei tiefe Spalten, die von Anteilen der N-terminalen Domäne eines und der C-terminalen Domäne des jeweils anderen Monomers begrenzt werden. Das aktive Zentrum liegt wahrscheinlich in dieser Spalte, wobei postuliert wird, daß der fest gebundene Cofaktor eher mit der größeren N-terminalen Domäne assoziiert ist und das Substrat zwischen den Domänen bindet. An der Bindung dürfte die C-terminale Domäne und möglicherweise auch direkt der Cofaktor beteiligt sein. Die Struktur zeichnet sich durch außergewöhnlich hohe Tenmperaturfaktoren ans. Für das Enzym aus M. marburgensis konnte eine Lösung durch molekularen Ersatz erhalten werden. Da der für die Katalyse benötigte, noch unbekannte Cofaktor nicht in der Struktur enthalten ist, ist eine weitergehende Diskussion des enzymatischen Mechanismus noch nicht möglich. Die Verfügbarkeit eines ersten Strukturmodells der metallfreien Hydrogenase stallt aber bereits einen entscheidenden Schritt auf dem Weg zum Verständnis dieses ungewöhnlichen Hydrogenierungskatalysators dar.
Pulsed electron-electron double resonance (PELDOR) is a well established method concerning nanometer distance measurements involving two nitroxide spin-labels. In this thesis the applicability of this method to count the number of spins is tested. Furthermore, this work explored the limits, up to which PELDOR data obtained on copper(II)-nitroxide complexes can be quantitatively interpreted. Spin counting provides access to oligomerization studies – monitoring the assembly of homo- or hetero-oligomers from singly labeled compounds. The experimental calibration was performed using model systems, which contain one to four nitroxide radicals. The results show that monomers, dimers, trimers, and tetramers can be distinguished within an error of 5% in the number of spins. Moreover, a detailed analysis of the distance distributions in model complexes revealed that more than one distance can be extracted from complexes bearing several spins, as for example three different distances were resolved in a model tetramer – the other three possible distances being symmetry related. Furthermore, systems exhibiting mixtures of oligomeric states complicate the analysis of the data, because the average number of spin centers contributes nonlinearly to the signal and different relaxation behavior of the oligomers has to be treated explicitly. Experiments solving these problems are proposed in the thesis. Thus, for the first time spin counting has been experimentally calibrated using fully characterized test systems bearing up to four spins. Moreover, the behavior of mixtures was quantitatively interpreted. In addition, it has been shown that several spin-spin distances within a molecule can be extracted from a single dataset. In the second part of the thesis PELDOR experiments on a spin-labeled copper(II)-porphyrin have been quantitatively analyzed. Metal-nitroxide distance measurements are a valuable tool for the triangulation of paramagnetic metal ions. Therefore, X-band PELDOR experiments at different frequencies have been performed. The data exhibits only weak orientation selection, but a fast damping of the oscillation. The experimental data has been interpreted based upon quantitative simulations. The influence of orientation selection, conformational flexibility, spin-density distribution, exchange interaction J, as well as anisotropy and strains of the g-tensor has been examined. An estimate of the spin-density delocalization has been obtained by density functional theory calculations. The dipolar interaction tensor was calculated from the point-charge model, the extension of the point-dipole approximation to several spin bearing centers. Even assuming asymmetric spin distributions induced by an ensemble of asymmetrically distorted porphyrins the effect of delocalization on the PELDOR time trace is weak. The observed damping of dipolar oscillations has been only reproduced by simulations, if a small distribution in J was assumed. It has been shown that the experimental damping of dipolar modulations is not solely due to conformational heterogeneity. In conclusion the quantitative interpretation of PELDOR data is extended to copper-nitroxide- and multi-spin-systems. The influence of the mean distance, of the number of coupled spins, of the conformational flexibility, of spin-density distribution and of the electronic structure of the spin centers has been analyzed using model systems. The insights on model compounds mimicking spin-labeled biomacromolecules – in oligomeric or metal bound states – calibrate the method with respect to the information that can be deduced from the experimental data. The resulting in-depth understanding allows correlating experimental results (from for example biological systems) with models of structure and dynamics. It also opens new fields for PELDOR as for example triangulation of metal centers and oligomerization studies. In general, this thesis has demonstrated that modern pulsed electron paramagnetic resonance techniques in combination with quantitative data analysis can contribute to a detailed insight into molecular structure and dynamics.
Today the structure of photosystem II, which is the enzyme responsible for the evolution of molecular oxygen by plants, algae and cyanobacteria, is known up to a resolution of about 3.0 Å in cyanobacteria (Loll et al., 2005). Photosystem II of higher plants, which shows some differences compared to the photosystem II of cyanobacteria, is not resolved in such high detail, yet (8-10 Å) (Rhee et al., 1998; Hankamer et al., 2001a). Therefore, the molecular structure of PSII of higher plants and its adjacent antenna complexes remains in the focus of the current research. One of the major problems when working with photosystem II is its relative instability during isolation. Together with the antenna proteins and several other proteins, some of which still have an unclear function, PSII forms a huge multi-protein-complex, which tends to fall apart during classical preparation methods. In order to achieve a faster and milder method of purification for PSII, four different His-tags have been added to one of the subunits of PSII. The gene targeted in this study is called psbE and codes for the α-chain of cytochrome b559, an integral part of PSII. The gene for PsbE is encoded in the chloroplast genome. The His-tags, which were employed in this work, consist of six or ten consecutive histidine aminoacid residues, which were fused to the N-terminus of the protein, either with or without a cleavage site for the protease “Factor Xa”. The N-terminus of PsbE is located on the more accessible stromal side of the thylakoid membrane. After inserting the psbE gene in a vector plasmid, in which the recognition site for the restriction endonuclease SacI had been eliminated, the different His-tags were generated by PCR with purposefully altered primers. In a final cloning step, a gene, which confers resistance to the antibiotics spectinomycin and streptomycin, was added to the DNA construct. Subsequently, the so-called biolistic transformation method (“gene gun”) was applied to introduce this genetically engineered plasmid DNA to Nicotiana tabacum chloroplasts (Bock & Hagemann, 2000). Through the processes of homologous recombination that take place in the chloroplast, the plastid encoded wildtype psbE gene was replaced by its His-tag containing counterparts. After several rounds of regenerating plants on antibiotic-containing medium, successful transformation was confirmed through PCR methods. By self fertilisation of fully regenerated plants, seeds were produced from tobacco strains, which carried only the mutated psbE gene. Plants cultivated from these seeds showed no distinctive phenotype under the chosen growth conditions, in respect to wildtype plants. The presence of the His-tag in this F1 generation was again confirmed with PCR methods. Measurements of oxygen evolution and pulse amplitude modulated fluorescence (PAM), carried out with preparations of wildtype and transgenic tobacco strains, revealed no differences for photochemical or non-photochemical quenching between both types. However, the oxygen evolution capacity of transgenic tobacco thylakoids compared to the wildtype was significantly reduced, although the chlorophyll content in relation to the leaf area was almost identical. This hints at a reduced amount of photosystem II complexes in the thylakoid membranes of transgenic tobacco. This alteration could be related to the mutation of cytochrome b559, because, amongst other functions, this subunit was shown to be important for the assembly of photosystem II (Morais et al., 1998). If solubilised thylakoid preparations of His-tagged plant strains were applied to a Ni-NTA column, photosystem II was selectively bound to the matrix. After washing away most of the contaminations, photosystem II core complexes could be eluted with imidazole-containing buffer. Photosystem II prepared in this way, displayed a drastic reduction of the peripheral light-harvesting complexes (LHCI & LHCII) and photo-system I reaction centres. This could be demonstrated by the loss of chlorophyll b and xanthophyll bands (LHCs) in absorption spectra, a small blue-shift of the chlorophyll a Qy absorption (PSI) and the respective band patterns in polyacrylamide gel electro-phoresis. The photosystem II complexes prepared in this way can now be put to use in different structural studies, like two-dimensional or three-dimensional crystallisation and spectroscopic measurements. Another photosynthetic pigment-protein complex of interest is the fucoxanthin-chlorophyll a/c-binding protein of diatoms, because eukaryotic algae, like diatoms, are important factors of oceanic ecosystems and account for a large part of marine biomass production. In order to facilitate ultra-fast time-resolved transient absorption spectroscopy and subsequent modelling of the kinetic traces, FCPs were prepared by sucrose-gradient ultra-centrifugation and their pigment stoichiometries determined by HPLC. Combining the spectroscopic data (Papagiannakis et al., 2005) with protein sequence alignments (Eppard & Rhiel, 1998) and the structure of the homologous higher plant LHCIIb (Kühlbrandt et al., 1994), a hypothetical model for the structure of FCP could be proposed (Fig. IV.3)