首页> 外文期刊>Biochemistry >Solution Structure of the 30 kDa Polysulfide-Sulfur Transferase Homodimer from Wolinella succinogenes(,).
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Solution Structure of the 30 kDa Polysulfide-Sulfur Transferase Homodimer from Wolinella succinogenes(,).

机译:Wolinella succinogenes(,)的30 kDa多硫化物-硫转移酶Homodimer的溶液结构。

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摘要

The periplasmic polysulfide-sulfur transferase (Sud) protein encoded by Wolinella succinogenes is involved in oxidative phosphorylation with polysulfide-sulfur as a terminal electron acceptor. The polysulfide-sulfur is covalently bound to the catalytic Cys residue of the Sud protein and transferred to the active site of the membranous polysulfide reductase. The solution structure of the homodimeric Sud protein has been determined using heteronuclear multidimensional NMR techniques. The structure is based on NOE-derived distance restraints, backbone hydrogen bonds, and torsion angle restraints as well as residual dipolar coupling restraints for a refinement of the relative orientation of the monomer units. The monomer structure consists of a five-stranded parallel beta-sheet enclosing a hydrophobic core, a two-stranded antiparallel beta-sheet, and six alpha-helices. The dimer fold is stabilized by hydrophobic residues and ion pairs found in the contact area between the two monomers. Similar to rhodaneseenzymes, Sud catalyzes the transfer of the polysulfide-sulfur to the artificial acceptor cyanide. Despite their similar functions and active sites, the amino acid sequences and structures of these proteins are quite different.
机译:Wolinella succinogenes编码的周质多硫化物硫转移酶(Sud)蛋白参与氧化磷酸化,其中多硫化物硫为末端电子受体。多硫化物硫与Sud蛋白的催化Cys残基共价结合,并转移到膜状多硫化物还原酶的活性位点。同源二聚体Sud蛋白的溶液结构已使用异核多维NMR技术确定。该结构基于NOE衍生的距离约束,主链氢键和扭转角约束以及残余的偶极耦合约束,以优化单体单元的相对方向。单体结构由包围疏水核的五链平行β-折叠,两链反平行β-折叠和六个α-螺旋组成。通过在两个单体之间的接触区域中发现的疏水性残基和离子对,可以稳定二聚体折叠。与Rhodaneseenzymes相似,Sud催化多硫化物硫向人工受体氰化物的转移。尽管它们具有相似的功能和活性位点,但这些蛋白质的氨基酸序列和结构却截然不同。

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