Structural Model of the Fe-Hydrogenase/Cytochrome c553 Complex Combining Transverse Relaxation-optimized Spectroscopy Experiments and Soft Docking Calculations

doi:10.1074/jbc.M909835199

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Structural Model of the Fe-Hydrogenase/Cytochrome c₅₅₃ Complex Combining Transverse Relaxation-optimized Spectroscopy Experiments and Soft Docking Calculations^*

Xavier Morelli, Mirjam Czjzek^§, Claude E. Hatchikian, Olivier Bornet, Juan C. Fontecilla-Camps^¶, Nuno P. Palma^**, Jose J. G. Moura, and Françoise Guerlesquin

From the Unité de Bioénergétique et Ingénierie des Protéines, IBSM-CNRS, Marseille Cedex 20, France, the ^§ Architecture et Fonction des Macromolécules Biologiques, IBSM-CNRS, Marseille Cedex 20, France, the ^¶ Laboratoire de Cristallographie et de Cristallogénèse des Protéines, Institut de Biologie Structurale Jean-Pierre Ebel, CEA-CNRS, Grenoble, France, the Departamento de Química, Centro Química Fina e Biotecnologia, Faculdade de Ciências e Tecnologia, Universidade Nova de Lisboa, Portugal, and the ^** Instituto Superior de Ciências da Saúde, Sul, Portugal

Received for publication, December 8, 1999, and in revised form, March 15, 2000

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Fe-hydrogenase is a 54-kDa iron-sulfur enzyme essential for hydrogen cycling in sulfate-reducing bacteria. The x-ray structureof Desulfovibrio desulfuricans Fe-hydrogenase has recently beensolved, but structural information on the recognition of its redoxpartners is essential to understand the structure-function relationshipsof the enzyme. In the present work, we have obtained a structuralmodel of the complex of Fe-hydrogenase with its redox partner,the cytochrome c₅₅₃, combining docking calculations and NMR experiments.The putative models of the complex demonstrate that the smallsubunit of the hydrogenase has an important role in the complexformation with the redox partner; 50% of the interacting siteon the hydrogenase involves the small subunit. The closest contactbetween the redox centers is observed between Cys-38, a ligandof the distal cluster of the hydrogenase and Cys-10, a ligandof the heme in the cytochrome. The electron pathway from the distalcluster of the Fe-hydrogenase to the heme of cytochrome c₅₅₃ wasinvestigated using the software Greenpath and indicates that theobserved cysteine/cysteine contact has an essential role. Thespatial arrangement of the residues on the interface of the complexis very similar to that already described in the ferredoxin-cytochromec₅₅₃ complex, which therefore, is a very good model for the interactingdomain of the Fe-hydrogenase-cytochrome c₅₅₃.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Sulfate-reducing bacteria of the genus Desulfovibrio utilize hydrogen or organic substrates as electron donors and exhibita strictly anaerobic mode of growth based on the reduction ofsulfate as the terminal electron acceptor (1). These microorganismscouple energy generation to the dissimilatory reduction of sulfatevia electron transfer-linked phosphorylation (2). Dissimilatorysulfate reduction with hydrogen is a transmembrane redox processin which H₂ oxidation and sulfate reduction take place on oppositesides of the cytoplasmic membrane (3). Sulfate-reducing bacteriahave been investigated for many years as a model for respiratoryelectron transfer chains. The structures of many compounds inthis system have been obtained using x-ray crystallography. Amongthese metalloproteins, the structurally unrelated NiFe- and Fe-hydrogenases(4) catalyze the oxidation of molecular hydrogen or protonreduction according to the following reaction (5):

<UP>H</UP>2 ⇔ 2<UP>H</UP>++2<UP>e</UP>− (Eq. 1)

Both enzymes are periplasmic and use c-type cytochromes as electron transfer partners (6). One of the oxidoreduction partnersof Fe-hydrogenase is the periplasmic low potential cytochromec₅₅₃. The monohemic cytochrome c₅₅₃ is homologous to mitochondrialcytochromes (7). The relative high exposure of the heme tothe solvent is the structural parameter modulating the low oxidoreductionpotential of this cytochrome (20 mV) (8). Kinetic experiments(6) have shown that cytochrome c₅₅₃ has a rather high affinityfor hydrogenase (K_m 46 µM) and that the electron transferrate constant (k_cat 710 s¹) is comparable to those generally reported in bimolecular electrontransfercomplexes.

The x-ray structure of Fe-hydrogenase is essential in understanding the reactivity of the enzyme (9). D. desulfuricansATCC 7757 Fe-hydrogenase, which is identical to the homologousenzyme from D. vulgaris on the basis of its amino acid sequenceand spectroscopic properties (10, 11), comprises two differentsubunits of 42.5 and 11 kDa. The large subunit contains a ferredoxin-likedomain composed of two [4Fe-4S] clusters and an unusual activeFe-S center, termed the H cluster. From x-ray studies, it hasbeen shown that the H cluster is constituted of a typical [4Fe-4S]cubane bridged to a binuclear active site. The observed spatialarrangement of the three [4Fe-4S] clusters separated by center-to-centerdistances of 12 Å provides one plausible electron transfer pathwaygoing from the buried binuclear active site to the distal [4Fe-4S]cluster located close to the molecular surface. Furthermore, thecalculated electrostatic potential at the molecular surface surroundingthe distal cluster is negative (9). These observations indicatethat this region might be involved in electrostatic interactionswith cytochrome c₅₅₃ (see Fig. 1), which exhibits a high contentof basic residues around the heme pocket (12). The mature smallsubunit, which is preceded by a N-terminal signal peptide, isprobably involved in the export of the enzyme to the periplasm(11). It shows an unusual topology, which sheds some light onthe evolutionary pathway of Fe-hydrogenase. Indeed, this heterodimericperiplasmic enzyme is very similar to Clostridium pasteurianumFe-hydrogenase and may have evolved from a common ancestral monomericenzyme. However, the structural role of the small subunit in Fe-hydrogenaseis not yet well understood. Although a wealth of biological andstructural data have been gathered on Fe-hydrogenase and cytochromec₅₅₃, the various types of interaction involved in the recognitionand the binding of the two electron transfer partners as wellas the interacting molecular surfaces of both redox partners havenot been investigated. Furthermore, the detailed mechanisms ofintra- and intermolecular electron transfer between the two redoxpartners still require extensiveresearch.

In the present work, we develop a structural approach to study the cytochrome c₅₅₃-Fe-hydrogenase complex using protein dockingcalculations and heteronuclear NMR experiments. Docking algorithmsare currently being developed for protein-ligand complex analysis.For protein-protein interactions the use of such algorithms ismore difficult, and it is essential that experimental data beused to select the best model. We have recently described an experimentalab initio approach using the software BiGGER in which we haveimplemented an NMR filter (13). This approach developed forsmall complexes was carried out using heteronuclear single quantumcoherence experiments. Recently, Pervushin et al. (14) introducedtransverse relaxation-optimized spectroscopy (TROSY),¹ in which constructive interference between dipolar relaxationand relaxation due to chemical shift anisotropy was exploitedto reduce the line width in both dimensions in high magnetic fields.The method has clear advantages for structural investigation ofhigh molecular weight complexes when compared with the regularheteronuclear single quantum coherence experiment. Therefore,we have carried out TROSY experiments on ¹⁵N-labeled cytochrome in the absence and presence of Fe-hydrogenase.On the basis of proton and nitrogen chemical shift variations,a mapping of the interacting site on the cytochrome has been obtained.These NMR data were used as a filter to choose the most accuratestructure obtained from the ab initio docking solutions proposedby the software BiGGER (15). We have recently demonstrated (13,16) that the use of NMR filters necessitates the labeling ofboth proteins so that NMR constraints are applied on both partnersof the complex. In the present work, the labeling of hydrogenaseis not possible because of the poor expression of the enzyme inthe sulfate-reducing bacteria. Moreover, if ¹⁵N labeling allows structural studies of high molecular weightproteins, double labeling (¹⁵N and ¹³C) would be necessary here, to accomplish the full assignmentof the Fe-hydrogenase. For this reason, we have first analyzeda complex where ferredoxin from Desulfomicrobium norvegicum wasused as a model of the ferredoxin-like domain of the Fe-hydrogenase(16). In the present work, we have developed a new approachfor high molecular weight complexes, where NMR constraints areonly deduced from ¹H and ¹⁵N chemical shifts observed on the smaller, labeled protein. Thesimilarities of the model complex and the physiological complexareanalyzed.

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

NMR Samples-- The cytochrome c₅₅₃ from D. vulgaris Hildenborough was expressed and purified from D. desulfuricans G200 as described previously(17). ¹⁵N-Cytochrome c₅₅₃ was obtained as previously reported (16) andwas concentrated in 10 mM Tris-HCl buffer, pH 7.0, on an Amiconmicroconcentrator (PM 3) to a 0.5 mM final concentration. D. desulfuricansATCC 7757 hydrogenase was purified as reported by Hatchikian etal. (10). Hydrogenase was concentrated under argon atmospherein Tris-HCl buffer (10 mM), pH 7.0, on an Amicon microconcentrator(PM 30) to a 0.4 mM final concentration. NMR experiments wererecorded with 0.1 mM cytochrome and 1 or 2 equivalents ofhydrogenase.

NMR Experiments-- The two-dimensional [¹H-¹⁵N]-TROSY pulse sequence uses single transition to single transition polarization transfer (18) whereit affords a <RAD><RCD> 2</RCD></RAD> sensitivity enhancementfor kinetically stable amide groups in proteins. NMR spectra wererecorded at 296 K on a Bruker Avance DRX 500 spectrometer operatingat 11.7 teslas, equipped with an HCN probe and self-shielded tripleaxis gradients. Spectra were acquired accumulating 32 scans perfree induction decay. 128 complex points in F1 and 1K complexpoints in F2 were recorded. The spectral width was 6 and 2 KHzin F2 and F1, respectively. ¹H chemical shifts were referenced with the H₂O resonance calibratedat 4.792 ppm at 296 K. ¹⁵N chemical shifts were referenced indirectly by setting the zeropoint of the nitrogen frequency scale equal to 0.101329118 timesthe proton zero frequency (19). Processing and spectra analysiswere done on Unix workstations using xwinnmr and Aurelia softwareprovided byBruker.

Protein Structures-- The protein coordinates of D. vulgaris Hildenborough cytochrome c₅₅₃ and D. desulfuricans ATCC 7757 Fe-hydrogenase were obtainedfrom the Protein Data Bank from file 1dvh and 1hfe,respectively.

Protein Docking-- Molecular interaction simulations were performed using the docking program BiGGER (15). This algorithm performs a completeand systematic search in the binding space of both molecules.A population of 1000 candidate protein-protein-docked geometriesis generated and selected, based on the geometric complementarityand amino acid pairwise affinities between the two molecular surfaces.In this process, the algorithm enables implicit treatment of molecularflexibility. In a subsequent step, the putative docked structuresare ranked using an interaction scoring function, which combinesseveral interaction terms that are thought to be relevant forthe stabilization of protein complexes: geometric packing of thesurfaces, explicit electrostatic interactions, desolvation energy,and pairwise propensities of the amino acid side chains to contactacross the molecular interface. In the ab initio simulations,the entire molecular surface was searched using absolutely noadditional information regarding the bindingsites.

NMR Filtering-- Chemical shift variations observed in TROSY experiments of cytochrome c₅₅₃ in the presence and absence of hydrogenase havebeen considered to be correlated to the complex formation. Thesevariations were translated into distance parameters (an amide(NH) affected is within 4 Å of any atom belonging to the otherprotein). The 1000 solutions obtained using the program BiGGERwere analyzed using these distance constraints. The solutionswere then ranked according to the NMR constraint violations (TableI). The ab initio solution clustering was not necessary, becauseonly two families of structures were obtained after the NMRranking.

Molecular Dynamics and Minimization of the Complex Structures-- The 10 best structures of the complex, as obtained by the docking algorithm filtered by NMR data, were first minimized ina preparation step, using the conjugate gradient method by Powell(20), with X-PLOR 3.851. Then a molecular dynamics calculation(AMBER force field) was performed on the selected complex structureswith a heat bath temperature of 280 K and initial velocities froma Maxwell-Boltzmann distribution at 280 K (integration of themotion equations at 0.001-ps time steps). The SHAKE constraints(21) were applied for all metal centers, i.e. the bi-atomiccatalytic site, the Fe₄S₄ clusters of the hydrogenase, and theheme group of the cytochrome with a tolerance of 0.0004. The coordinatesof the "best" structure (family 1 (fam1) solution 3) have beendeposited at the Protein Data Bank (code: 1e08).

Electron Transfer Pathway-- The software Greenpath (22) was used to propose an electron transfer pathway from the electron donor (the hydrogenase distalcluster) to the electron acceptor (the cytochromeheme).

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ionic Strength Dependence of the Cytochrome c₅₅₃-Fe-Hydrogenase-- Cytochrome c has been reported to present a strong dipolar moment induced by the high content of basic residues found aroundthe heme pocket. These lysine residues have been demonstratedto be highly conserved in this class of proteins (7). Complexformation between cytochrome c₅₅₃ and Fe-hydrogenase has beenevaluated in terms of electrostatic interactions. The drasticeffect of the ionic strength (0.5 M NaCl) on the kinetic measurementsof cytochrome c₅₅₃ reduction by Fe-hydrogenase, which we haveobserved, establishes that electrostatic interactions are thedriving force of the complexformation.

Fig. 1 shows electrostatic isopotential curves for cytochrome c₅₅₃ and Fe-hydrogenase. The dipolar moment is easily observablefor cytochrome c_553, and three zones of various charges are observablefor hydrogenase. The heme environment of cytochrome c₅₅₃ and theH cluster environment of the Fe-hydrogenase are found to be positivelycharged, and the environment of one of the two clusters of theferredoxin-like domain (the distal cluster) is negatively charged.Considering the electrostatic properties of the two moleculesand the ionic strength dependence of the complex formation, onecan expect that the distal cluster situated at the extreme endof the domain is the interacting site with cytochrome c₅₅₃.

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Fig. 1. Isopotential representation of Fe-hydrogenase (left) and of cytochrome c₅₅₃ (right). The positive charges are represented in blue, and the negative charges are represented in red. H, P, M, and D designate, respectively, the active center and the proximal, the medial, and the distal clusters of Fe-hydrogenase.

NMR Mapping of the Interacting Site-- TROSY experiments have been recorded on 0.1 mM cytochrome c₅₅₃ solution at 296 K (Fig. 2). Out of the 78 amino acids, 58 NHgroups were assigned. The mapping of the interacting site wasobtained from the induced chemical shifts observed on the cytochromec₅₅₃ NH, in the presence of Fe-hydrogenase in the TROSY experiments(Fig. 3a). Nine NH groups undergo notable ¹⁵N chemical shift variations from 0.1 to 0.45 ppm and ¹H from 0.015 to 0.06 ppm. Analysis of these chemical shifts givesthe mapping of the interacting site on the cytochrome representedin Fig. 3b. The interacting site on the cytochrome is the samewith either ferredoxin (16) or hydrogenase, involving at leastsix conserved residues, i.e. 10, 14, 15, 16, 24, and 59.

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Fig. 2. TROSY spectrum of ¹⁵N-labeled cytochrome c₅₅₃-hydrogenase complex. The spectrum was recorded on a Bruker DRX 500 spectrometer at 296 K.

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Fig. 3. A, ¹H and ¹⁵N chemical shift variations of cytochrome c₅₅₃ NH groups observed in TROSY experiments. B, mapping of the hydrogenase interacting site on the cytochrome c₅₅₃, obtained by heteronuclear experiments. In the top figure, the heme is colored in red, the NH groups whose resonances undergo chemical shift variations are in green, unassigned residues are in blue, and unaffected residues are in white. The bottom figure shows a 180° rotation along the x axis and represents the "back side" of the molecule.

Docking of the Complex-- An ab initio docking of the complex was calculated on the basis of the Protein Data Base files from cytochrome c₅₅₃ and Fe-hydrogenase.1000 putative structures of the complex were obtained from thesoftware BiGGER. These structures were first evaluated and rankedby an ab initio procedure, which uses an interaction score function(Fig. 4A). The next step was to use the NMR filter, explainedabove, in order to rule out solutions incompatible with the NMRdata and to retain a reduced population of plausible structures(Fig. 4B). Eight NH groups of the residues affected by the complexformation were used as a filter for the docking solutions, i.e.5, 10, 14, 15, 16, 24, 32, 54 and 59. This procedure eliminatesthe set of solutions in which the cytochrome would bind at thesecond negatively charged region on the hydrogenase (solutionson the lower left of Fig. 4A). The remaining solutions were rankedaccording to the level of agreement with the NMR constraints.The 50 top solutions (with fewer than three constraints violatedout of eight) involve the binding of the cytochrome at two distinctsites in the surface of the hydrogenase (Fig. 4B). Each site involves,respectively, the distal and the medial cluster of the ferredoxin-likedomain of hydrogenase and corresponds to family1 and family2 solutions.However, it has been reported that the hydrogenase-cytochromec₅₅₃ complex has a 1:1 stoichiometry (6), so only one of thesetwo families of solutions is relevant. At this level, a reciprocalmapping of the interacting site on labeled hydrogenase would behelpful, but unfortunately, due to the poor expression of Fe-hydrogenasein sulfate-reducing bacteria, to date, it is not possible to carryout the labeling of Fe-hydrogenase. Therefore, we did not discardany of these two families at this stage of the analysis. Of the50 best solutions, 10 models have a heme/cluster distance smallerthan 20 Å. Considering that a maximum distance of 20 Å is necessaryfor an effective electron transfer, the 10 resulting solutionswere energy-minimized. These 10 solutions are equally distributedin two families (fam1 and fam2) and are numbered according tothe related family (Table I).

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Fig. 4. Docking of the cytochrome c₅₅₃-hydrogenase complex. A, the 1000 first ab initio docking solutions. B, the 50 best solutions chosen using NMR filtering. Only the hydrogenase backbone is represented; the center of mass of the cytochrome is represented by a small sphere.

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Table I
Structural comparison of the 10 final models of the cytochrome c₅₅₃-hydrogenase complex
The values indicated were obtained after energy minimization.

Energy Minimization of the Docking Solutions-- All 10 solutions were minimized using X-PLOR, and a molecular dynamics calculation was performed to optimize side chain conformationsand interactions on the interface. The resulting properties ofthe complexes after minimization are reported in Table I. Theresults indicate that the five solutions close to the distal cluster(fam1) can be grouped in a unique solution after minimization.The optimal distances between the distal cluster and the hemefor these five solutions range from 12.3 to 14.3 Å, and the finalenergy level varies by less than 0.5%. The solutions on the oppositeside of the ferredoxin-like domain of the hydrogenase, closestto the medial cluster (fam2), represents five different solutions,because the orientations vary by more than 20° and different residuesare involved in intermolecular interactions. Furthermore, theoptimal distances obtained after minimization between the medialcluster and the heme group are clearly less favorable than thesolutions of fam1, which bring the distal cluster closest to theheme of cytochrome c₅₅₃. Therefore, we propose that the electrontransfer involves the distal cluster as the direct interactionsite with the cytochrome(fam1).

Within fam1, analysis of the five solutions involving the distal cluster indicates that it is the same region with small modificationsof interacting residues that forms the interface. The choice ofone representative structure was made with respect to the resultsof site-directed mutagenesis obtained on cytochrome c₅₅₃. We havealready suggested that Lys-63 and Tyr-64 are essential for electrontransfer with the redox partner (12, 23). On the basis ofthese data, fam1 solution 3 seemed to be the best representativestructure.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The model, corresponding to fam1 solution 3 of the cytochrome c₅₅₃-hydrogenase complex, is presented in Fig. 5. The interactingdomain is very similar to the model proposed for the ferredoxin-cytochromec₅₅₃ complex. This is not surprising, considering that the rootmean square distance between the ferredoxin-like domain of Fe-hydrogenaseand the ferredoxin is 1.75 Å and that the distal cluster is theone conserved in the monocluster ferredoxins. The interactingsurface is significantly bigger for hydrogenase (2284 Å) thanit is for ferredoxin (1037 Å). This is directly correlated withthe fact that the interacting site on hydrogenase is not onlyformed by the ferredoxin-like domain but about half of the protein-proteininterface involves the small subunit of Fe-hydrogenase. The hemeto Fe-S distance (12.3 Å) is longer in the hydrogenase complexthan in the ferredoxin complex (10 Å). However, the distributionof hydrophobic and electrostatic atomic contacts are comparablein both complexes. These data demonstrate that ferredoxin is agood model for the ferredoxin-like domain of Fe-hydrogenase withrespect to its properties when interacting with the cytochromec₅₅₃. The use of an isolated functional domain is certainly agood approach for obtaining structural information in high molecularweight complexes.

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Fig. 5. Model of fam1 solution 3 using Grasp software. A, ribbon model of the cytochrome c₅₅₃-hydrogenase complex. For hydrogenase, the ferredoxin-like domain is in green, the large subunit is in blue, and the small subunit is in yellow. The cytochrome c₅₅₃ is in red. B, view of interface in the cytochrome c₅₅₃-ferredoxin complex (a) and in the cytochrome c₅₅₃-hydrogenase complex (b).

Another significant aspect provided by the model of the cytochrome c₅₅₃-hydrogenase complex is the involvement of the smallsubunit in the interaction site. The N- and C-terminal ends ofthe hydrogenase small subunit interact with the N-terminal partand the axial histidine-containing sequence (residues 12-17) ofthe cytochrome. This finding is strengthened by the TROSY data,where residues 14, 15, and 16 are found affected by the complexformation. From the structural model, the interacting surfaceof cytochrome c₅₅₃ with the small subunit of hydrogenase is around900 Å². This is the first time that a structural role has been proposedfor the small subunit of Fe-hydrogenase. The involvement of thesmall subunit in the recognition of the physiological partneris an additional role that adds to the well established implicationof this subunit in the exportation of the enzyme to the periplasm.These data give a structural meaning to the conservation of thispeptide chain during evolution. The recent structure of the Fe-hydrogenasefrom C. pasteurianum, a cytoplasmic enzyme (24), shows a foldingsimilar to that of the Desulfovibrio periplasmic enzyme (9).The polypeptide chain equivalent to the small subunit of D. desulfuricansFe-hydrogenase exhibits the same unusual topology wrapped aroundthe large subunit. Site-directed mutagenesis should easily confirmthe functional implication of the small subunit in D. desulfuricansFe-hydrogenases in the interactingsite.

The cytochrome c₅₅₃ interacting site on the large subunit of the hydrogenase is located near the distal cluster of the ferredoxin-likedomain. The N-terminal helix of the cytochrome is in close contactto Ala-397 of Fe-hydrogenase. Asp-2, Gly-3, and Ala-4 of the cytochromeare at hydrogen-bonding distance to Ala-397 of the hydrogenase.The NH most affected in TROSY experiments is that of Cys-10, covalentlybound to the cytochrome heme. In the model, Cys-10 is at a distanceof about 3.8 Å from Cys-38 of the hydrogenase (Fig. 5B, part b).The same spatial arrangement of the FeS cluster, the heme andthe two equivalent cysteine residues, was found in the ferredoxin-cytochromec₅₅₃ complex (Fig. 5B, part a). An electron transfer pathway wascalculated with the Greenpath software. In the "best" pathway,the two cysteines facing each other are the site of electron transferbetween the two molecules. The proposed pathway can be describedas follows: the electron comes from the distal cluster and passesthrough the Fe-S bond of hydrogenase Cys-38, via the sigma bondof the cysteine to its carboxylic oxygen, from where it jumpsto Cys-10 of the cytochrome. A further jump from the sulfur lonepair of Cys-10 to the histidine (His-14), the axial ligand ofcytochrome c₅₅₃ heme, completes the path. The atoms of this pathare closely arranged around the straight line between the twoiron atoms (distal cluster Fe2-heme Fe: 12.34 Å). The path lengthas calculated with Greenpath is 14 Å. Covalently bound sulfuratoms are indeed known to be involved in electron transfer ofmetal-organic compounds (25). Interestingly, close cysteine-cysteinecontacts, between cysteines covalently bound to heme groups, hasalso been observed at the dimeric interface of the cytochromec₃ (M_r 26,000) (26). Furthermore, a closely related electrontransfer pathway, including two residues coordinating the [4Fe-4S]clusters, Cys-287 of formaldehyde ferredoxin oxidoreductase andAsp-14 of ferredoxin from Pyrococcus furiosus has recently beendescribed from the analysis of the structure of the cocrystallizedcomplex (27). Such an electron pathway is probably found inmany electron transfer complexes. Site-directed mutagenesis wouldbe an appropriate approach to validate the electron pathway. However,in the cytochrome c₅₅₃-hydrogenase complex, substitution of oneof the two cysteine residues (by Ala, Ser, or Met) is difficultto achieve without drastic modifications to the protein foldingor redox properties. The substitution of hydrogenase Cys-38 bya selenocysteine would be a better approach, but the barriersof heterologous expression of the selenoprotein gene in bacteriaare a limitation of this kind of substitution (28).

The interacting surface includes the environment of the axial methionine (Met-57) of the cytochrome. Residues 54, 59, and60 were found affected in TROSY experiments. In the model, a hydrogenbond exists between Asn-59 of the cytochrome and the main chaincarboxyl groups of residues Ile-36 of the large subunit of hydrogenase.This Ile residue in the ferredoxin-like domain of hydrogenaseis conserved in all the ferredoxins (Ile-10). In the present model,as in the ferredoxin-cytochrome c₅₅₃ model, the main chain CO-groupof this Ile residue makes a hydrogen bond with Lys-63 of the cytochrome,and the side chain of Ile-36 of hydrogenase exhibits hydrophobicvan der Waals contacts with the side chain of Tyr-64 of the cytochrome.The role of these two residues in the electron transfer processin cytochrome c₅₅₃ has been previously established (12, 23).The interaction of Tyr-64 of the cytochrome with the conservedIle-36 residue of the hydrogenase assures the correct spatialarrangement by packing forces to bring the two electron transferringcysteines into the optimal position. Furthermore, Tyr-64 of thecytochrome, having a bulky aromatic side chain, probably blocksthe accessibility of the prosthetic group crevice to the solventmolecules, which is certainly essential for the electron transferreaction. By replacing residue Ile-36 by Ala in hydrogenase, boththe importance of the length of the side chain for interactionwith Tyr-64 of the cytochrome and the ability to block the accessof the electron transfer site to the solvent would beelucidated.

Aknowledgements

We thank Susan D. Wells for reading the manuscript. The NMR equipment was partially provided by the Conseil Général desBouches-du-Rhône.

	FOOTNOTES

^* Supported by the French Embassy and by the ICCTI (Project 316C2).The costs of publication of this article were defrayed inpart by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

The atomic coordinates and the structure factors (code 1e08) have been deposited in the Protein Data Bank, Research Collaboratoryfor Structural Bioinformatics, Rutgers University, New Brunswick,NJ (http://www.rcsb.org/).

To whom correspondence should be addressed. Tel.: 33-4-91-16-43-79; Fax: 33-4-91-16-45-78; E-mail: f.guerlesquin@ibsm.cnrs-mrs.fr.

Published, JBC Papers in Press, March 27, 2000, DOI 10.1074/jbc.M909835199

ABBREVIATIONS

The abbreviations used are: TROSY, transverse relaxation-optimized spectroscopy; fam1 and -2, structure families 1 and 2; NH, amide protons.

	REFERENCES

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

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All ASBMB Journals	Molecular and Cellular Proteomics
Journal of Lipid Research	ASBMB Today

				S. ZHU and J. TYTGAT Evolutionary epitopes of Hsp90 and p23: implications for their interaction FASEB J, June 1, 2004; 18(9): 940 - 947. [Abstract] [Full Text] [PDF]

				X. J. Morelli, P. N. Palma, F. Guerlesquin, and A. C. Rigby A novel approach for assesing macromolecular complexes combining soft-docking calculations with NMR data Protein Sci., October 19, 2001; 10(10): 2131 - 2137. [Abstract] [Full Text] [PDF]

Structural Model of the Fe-Hydrogenase/Cytochrome c553 Complex Combining Transverse Relaxation-optimized Spectroscopy Experiments and Soft Docking Calculations*

Structural Model of the Fe-Hydrogenase/Cytochrome c₅₅₃ Complex Combining Transverse Relaxation-optimized Spectroscopy Experiments and Soft Docking Calculations^*