Characterization of the Redox and Metal Binding Activity of BsSco, a Protein Implicated in the Assembly of Cytochrome <i>c</i> Oxidase

Imriskova-Sosova, Iveta; Andrews, Diann; Yam, Katherine C.; Davidson, David E.; Yachnin, Brahm J.; Hill, Bruce C.

doi:10.1021/bi051343i

Cited by 32 publications

(47 citation statements)

References 35 publications

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“…We observe a remarkable increase in redox sensitivity when the H135 residue is replaced with a non-coordinating alanine residue traceable to a large decrease in the stability of the Cu(II) form. In contrast to previous studies (4, 12), this variant binds copper but is susceptible to autoreduction of Cu(II) to Cu(I) (coupled to cysteine autoxidation to a disulfide) and exhibits a 10 3 -fold increase in its reactivity towards hydrogen peroxide. Addition of imidazole causes EPR spectral changes consistent with rebinding of the imidazole ring to the Cu(II) center, yet this fails to fully restore the redox stability of the native Cu(II) form suggesting a critical conformational role of the native H135 in stabilizing the Cu(II) state.…”

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confidence: 84%

H135A Controls the Redox Activity of the Sco Copper Center. Kinetic and Spectroscopic Studies of the His135Ala Variant of Bacillus subtilis Sco

et al. 2009

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Sco-like proteins contain copper bound by two cysteines and a histidine residue. Although their function is still incompletely understood, there is a clear involvement with the assembly of cytochrome oxidases which contain the Cu A center in subunit 2, possibly mediating the transfer of copper into the Cu A binuclear site. We are investigating the reaction chemistry of BSco, the homologue from B. subtilis. Our studies have revealed that BSco behaves more like a redox protein than a metallochaperone. The essential H135 residue which coordinates copper, plays a role in stabilizing the Cu(II) rather than the Cu(I) form. When H135 is mutated to alanine, the oxidation rate of both hydrogen peroxide and one-electron outer-sphere reductants increases by two orders of magnitude, suggestive of a redox switch mechanism between His-on and His-off conformational states of the protein. Imidazole binds to the H135A protein restoring the N superhyperfine coupling in the EPR, but is unable to rescue the redox properties of the WT Sco. These findings reveal a unique role for H135 in Sco function. We propose a hypothesis that electron transfer from Sco to the maturing oxidase may be essential for proper maturation and/or protection from oxidative damage during the assembly process. The findings also suggest that interaction of Sco with its protein partner(s) may perturb the Cu(II)-H135 interaction, and thus induce a sensitive redox activity to the protein.Sco1 is an essential accessory protein in the assembly of cytochrome-c-oxidase, the terminal enzyme of the respiratory chain. A large body of evidence links the function of Sco to the metalation of the Cu A center in subunit 2 of the oxidase (Cox2). In both yeast and B. subtilis, Sco mutant strains that impair or eliminate Cu binding produce a phenotype lacking in functional caa 3 oxidase, and high levels of Cu are able to rescue the caa 3 activity of B. subtilis-Sco (BSco) 1 -deficient strains (1-6). These data strongly implicate an interaction of † This work was supported in whole or in part by the National Institutes of Health Grant GM54803 (to NJB). This work was also supported 1 The abbreviations used are: BSco, Bacillus subtilis Sco; IPTG, isopropyl β-D-thiogalactopyranoside; WT, wild-type; NBT, nitroblue tetrazolium; BCIP, 5-bromo-4-chloro-3-indolylphosphate; TMPD, N, N, N′, N′-tetramethyl-p-phenylene diamine; DTT, dithiothreitol; EDTA, ethylenediaminetetraacetic acid; EPR, electron paramagnetic resonance; EXAFS, extended X-ray absorption fine structure; XANES, X-ray absorption near edge structure. NIH Public Access Author ManuscriptBiochemistry. Author manuscript; available in PMC 2010 December 29. (14), and the Cu(II) form shows no tendency towards autoredox to disulfide and Cu(I), although this chemistry was observed in a crystal of the Ni(II) derivative (11). These considerations suggest that Sco-type proteins may exhibit two or more distinct activities which include both copper transfer and redox activities.To further understand the possible function of Sco ...

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confidence: 84%

H135A Controls the Redox Activity of the Sco Copper Center. Kinetic and Spectroscopic Studies of the His135Ala Variant of Bacillus subtilis Sco

et al. 2009

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“…The comprehension and description of these processes are still in their infancy, and only now knowledge about the structure and functional role of the assisting proteins has begun to become available. Many lines of evidence show that copper insertion into Cu A site of COXII subunit is not a simple, passive copper transfer from Cox17 to Sco1/2 proteins and finally to COXII, but redox reactions are interlinked with the process of copper transfer (12,15,16,27).…”

Section: Discussionmentioning

confidence: 99%

Human Sco1 functional studies and pathological implications of the P174L mutant

Banci

Bertini

Ciofi‐Baffoni

et al. 2007

Proc. Natl. Acad. Sci. U.S.A.

107

138

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“…UV-visible Spectroscopy of ScoI-The method was used to follow the binding of Cu(II) to reduced ScoI (52). Reduction of ScoI sol was achieved by incubation with 2 mM dithiothreitol for 4 h at 4°C.…”

Section: Expression and Purification Of Scoi And Its Mutant Derivative-mentioning

confidence: 99%

“…The addition of CuCl 2 to the protein resulted in an absorbance peak at ϳ360 nm (Fig. 6), reflecting the binding of Cu(II) to the protein (52). Upon incremental copper addition, the peak increased and reached a plateau at a ratio of ϳ0.…”

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confidence: 98%

Disparate Pathways for the Biogenesis of Cytochrome Oxidases in Bradyrhizobium japonicum

Bühler

Rossmann

Landolt

et al. 2010

Journal of Biological Chemistry

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This work addresses the biogenesis of heme-copper terminal oxidases in Bradyrhizobium japonicum, the nitrogen-fixing root nodule symbiont of soybean. B. japonicum has four quinol oxidases and four cytochrome oxidases. The latter include the aa 3 -and cbb 3 -type oxidases. Although both have a Cu B center in subunit I, the subunit II proteins differ in having either a Cu A center (in aa 3 ) or a covalently bound heme c (in cbb 3 ). Two biogenesis factors were genetically studied here, the periplasmically exposed CoxG and ScoI proteins, which are the respective homologs of the mitochondrial copper-trafficking chaperones Cox11 and Sco1 for the formation of the Cu B center in subunit I and the Cu A center in subunit II of cytochrome aa 3 . We could demonstrate copper binding to ScoI in vitro, a process for which the thiols of cysteine residues 74 and 78 in the ScoI polypeptide were shown to be essential. Knock-out mutations in the B. japonicum coxG and scoI genes led to loss of cytochrome aa 3 assembly and activity in the cytoplasmic membrane, whereas the cbb 3 -type cytochrome oxidase apparently remained unaffected. This suggests that subunit I of the cbb 3 -type oxidase obtains its copper cofactor via a different pathway than cytochrome aa 3 . In contrast to the coxG mutation, the scoI mutation caused a decreased symbiotic nitrogen fixation activity. We hypothesize that a periplasmic B. japonicum protein other than any of the identified Cu A proteins depends on ScoI and is required for an effective symbiosis.

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Characterization of the Redox and Metal Binding Activity of BsSco, a Protein Implicated in the Assembly of Cytochrome c Oxidase

Cited by 32 publications

References 35 publications

H135A Controls the Redox Activity of the Sco Copper Center. Kinetic and Spectroscopic Studies of the His135Ala Variant of Bacillus subtilis Sco

H135A Controls the Redox Activity of the Sco Copper Center. Kinetic and Spectroscopic Studies of the His135Ala Variant of Bacillus subtilis Sco

Human Sco1 functional studies and pathological implications of the P174L mutant

Disparate Pathways for the Biogenesis of Cytochrome Oxidases in Bradyrhizobium japonicum

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