Cloning and nucleotide sequences of the genes for the subunits of NAD-reducing hydrogenase of Alcaligenes eutrophus H16

Tran-Betcke, A; Warnecke, U; Böcker, C; Zaborosch, Christiane; Friedrich, Bärbel

doi:10.1128/jb.172.6.2920-2929.1990

Cited by 203 publications

(191 citation statements)

References 52 publications

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“…3) contains four genes which show strong similarity to genes coding for the NAD+-reducing hydrogenase from A. eutrophus but have relatively little similarity to the two structural genes hupL and hupS of the membrane-bound NiFe hydrogenases ( Table 1). Therefore the genes are denoted hoxH, hoxY, hoxU and hoxF as in the case of the A. eutrophus soluble hydrogenase [20]. The hydrogenase gene cluster from A. vuriubilis contains the ORF3 (corresponding to a protein of 199 amino acids, 22.5 kDa) between hoxH and hoxY The deduced protein sequence showed 31 ?b sequence identity to a hypothetical 17.7-kDa protein of unknown function in the BPS 3'-region of the archaebacterium Desulfurolobus ambivalens (W. Kletzin, EMBL accession no.…”

Section: Resultsmentioning

confidence: 99%

Molecular Biological Analysis of a Bidirectional Hydrogenase from Cyanobacteria

Schmitz

Boison

Hilscher

et al. 1995

European Journal of Biochemistry

145

162

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An 8.9-kb segment with hydrogenase genes from the cyanobacterium Anabaena variabilis has been cloned and sequenced. The sequences show homology to the methyl-viologen-reducing hydrogenases from archaebacteria and, even more striking, to the NAD'-reducing enzymes from Alcaligenes eutrophus and Nocardia opaca as well as to the NADP' -dependent protein from Desulfovibrio fructosovorarzs. The cluster from A. variabilis contains genes coding for both the hydrogenase heterodimer (hoxH and hoxv and for the diaphorase moiety (hoxU and hoxfl described for the A. eurroplius enzyme. In A. variabilis the gene cluster is split by two open reading frames (between hoxY and hoxH and between hoxU and hoxl: respectively), and a probably non-coding 0.9-kb segment in an unusual way. The hoxH partial sequence from Anabaena 71 19 and Anucystis nidulan.7 was amplified by PCR. Using the labeled segment from A. 71 19 as probe, Southern analysis revealed homologous gene segments in the cyanobacteria A. 71 19, Anabaena cylindrica, Arzacystis nidulans and A. variabilis. The bidirectional hydrogenase from A. nidulans was purified and digests were sequenced. The amino acid sequences obtained showed partial identities to the amino acid sequences deduced from the DNA data of the 8.9-kb segment from A. variabilis. Therefore the 8.9-kb segment contains the genes coding for the bidirectional, reversible hydrogenase from cyanobacteria. Crude extracts from A. nidulans perform NAD(P)H-dependent H, evolution corroborating the molecular biological demonstration of the NAD(P)'.-dependent hydrogenase in cyanobacteria.

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Section: Resultsmentioning

confidence: 99%

Molecular Biological Analysis of a Bidirectional Hydrogenase from Cyanobacteria

Schmitz

Boison

Hilscher

et al. 1995

European Journal of Biochemistry

145

162

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“…There is a close relationship between the 5 1-kDa subunit, the corresponding subunit of bovine complex I (Pilkington et al, 1991) and the a subunit of the soluble NAD-reducing hydrogenase of Alcaligenes eutruphus (Tran-Betcke et al, 1990). A comparison between these sequences revealed a conserved region of a nucleotidebinding site (Wierenga et al, 1986), a glycine-rich region which could bind FMN (Mathews, 1991) and a conserved sequence motif of (CxxCxxC-----C) indicative of a tetranuclear iron-sulphur cluster (Pilkington et al, 1991).…”

Section: Discussionmentioning

confidence: 99%

Disruption of the gene encoding the NADH‐binding subunit of NADH: ubiquinone oxidoreductase in Neurospora crassa

Fecke

Sled

Ohnishi

et al. 1994

European Journal of Biochemistry

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In this study, the gene of the 51-kDa NADH-binding subunit of the mitochondrial NADH : ubiquinone oxidoreductase (complex I) in Neurospora crassa was inactivated by homologous replacement with a defective gene copy. The resulting mutant, nuo51, lacks the 51-kDa subunit and shows no complex I activity but still grows at one third of the wild-type growth rate. The enzyme activity of the alternative NADH xbiquinone oxidoreductase(s) is increased twofold while the activities of the other mitochondrial respiratory enzymes are normal. Complex I is almost completely assembled except for the NADH-binding subunit and still possesses three out of the four EPR-detectable iron-sulphur clusters. Since the deleted subunit contains the sequence motif for one tetranuclear iron-sulphur cluster, the missing cluster N-3 is considered to be bound to this subunit.Mitochondria1 NADH : ubiquinone oxidoreductase (complex I) transfers electrons from NADH via FMN and an undefined number of iron-sulphur clusters to ubiquinone, and links this process with proton translocation across the inner membrane. The enzyme complex consists of 35 different subunits in fungi and at least 42 subunits in mammals, of which seven subunits are encoded by the mitochondrial genome Walker, 1992; Arizmendi et al., 1 992).Complex I is not found in Saccharoiriyces cerevisiae (de Vries and Grievell, 1988) and, consequently, the powerful genetic techniques which can be applied to this eucaryotic model organism cannot be used to study complex I. We have therefore studied this complex in the filamentous fungus Neurospora crassa for which we have established a method for the disruption of nuclear genes by homologous recombination. In the obligate aerobic fungus N. crassa, complex I is a constitutively made enzyme, and the lack of synthesis of single subunits of the complex appears not to affect the synthesis of the other subunits. Intermediates in the assembly pathway or partially assembled moieties of the complex are accumulated under these conditions. Recently, we reported that the disruption of the nuclear gene of the 21.3-kDa subunit leads to a mutant (nuo21) which previously assembles the complete peripherally located NADH dehydrogenase component of the complex with all of its redox groups. The mutant is nevertheless unable to fully assemble the intrinsic membrane ubiquinone reductase complex, and subsequentlyCorrespondence to

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“…Halboth & Klein, 1992), usually associated with two regular cubane clusters. In two enzymes, the six Cys residues are missing altogether, and the amino acid sequence of the small subunit terminates shortly after the first four conserved residues (Bohm et al, 1990;Tran-Betcke et al, 1990). This indicates that the clusters coordinated by these Cys residues are not essential for hydrogen activation.…”

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confidence: 99%

Infrared-Detectable Group Senses Changes in Charge Density on the Nickel Center in Hydrogenase from Chromatium vinosum

Bagley

Duin²,

Roseboom³

et al. 1995

Biochemistry

215

217

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An infrared-detectable group senses changes in charge density on the nickel center in hydrogenase from Chromatium vinosum Bagley, K.A.; Duin, E.L.; Roseboom, W.; Albracht, S.P.J.; Woodruff, W.H. General rights It is not permitted to download or to forward/distribute the text or part of it without the consent of the author(s) and/or copyright holder(s), other than for strictly personal, individual use, unless the work is under an open content license (like Creative Commons). Disclaimer/Complaints regulationsIf you believe that digital publication of certain material infringes any of your rights or (privacy) interests, please let the Library know, stating your reasons. In case of a legitimate complaint, the Library will make the material inaccessible and/or remove it from the website. Please Ask the Library: http://uba.uva.nl/en/contact, or a letter to: Library of the University of Amsterdam, Secretariat, Singel 425, 1012 WP Amsterdam, The Netherlands. You will be contacted as soon as possible. ABSTRACT: Fourier transform infrared studies of nickel hydrogenase from Chromatium vinosum reveal the presence of a set of three absorption bands in the 2100-1900 cm-1 spectral region. These bands, which do not arise from carbon monoxide, have line widths and intensities rivaling those of a band arising from the carbon monoxide stretching frequency (v(C0)) in the Ni(I1)CO species of this enzyme

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Cloning and nucleotide sequences of the genes for the subunits of NAD-reducing hydrogenase of Alcaligenes eutrophus H16

Cited by 203 publications

References 52 publications

Molecular Biological Analysis of a Bidirectional Hydrogenase from Cyanobacteria

Molecular Biological Analysis of a Bidirectional Hydrogenase from Cyanobacteria

Disruption of the gene encoding the NADH‐binding subunit of NADH: ubiquinone oxidoreductase in Neurospora crassa

Infrared-Detectable Group Senses Changes in Charge Density on the Nickel Center in Hydrogenase from Chromatium vinosum

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