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大肠杆菌MoeB的特性及其在钼蝶呤合酶激活参与钼辅因子生物合成过程中的作用。

Characterization of Escherichia coli MoeB and its involvement in the activation of molybdopterin synthase for the biosynthesis of the molybdenum cofactor.

作者信息

Leimkühler S, Wuebbens M M, Rajagopalan K V

机构信息

Department of Biochemistry, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

J Biol Chem. 2001 Sep 14;276(37):34695-701. doi: 10.1074/jbc.M102787200. Epub 2001 Jul 19.

Abstract

Amino acid sequence comparisons of Escherichia coli MoeB suggested that the MoeB-dependent formation of a C-terminal thiocarboxylate on the MoaD subunit of molybdopterin synthase might resemble the ubiquitin-activating step in the ubiquitin-targeted degradation of proteins in eukaryotes. To determine the exact role of MoeB in molybdopterin biosynthesis, the protein was purified after homologous overexpression. Using purified proteins, we have demonstrated the ATP-dependent formation of a complex of MoeB and MoaD adenylate that is stable to gel filtration. Mass spectrometry of the complex revealed a peak of a molecular mass of 9,073 Da, the expected mass of MoaD adenylate. However, unlike the ubiquitin activation reaction, the formation of a thioester intermediate between MoeB and MoaD could not be observed. There was also no evidence for a MoeB-bound sulfur during the sulfuration of MoaD. Amino acid substitutions were generated in every cysteine residue in MoeB. All of these exhibited activity comparable to the wild type, with the exception of mutations in cysteine residues located in putative Zn-binding motifs. For these cysteines, loss of activity correlated with loss of metal binding.

摘要

大肠杆菌MoeB的氨基酸序列比较表明,钼蝶呤合酶的MoaD亚基上C端硫代羧酸盐的MoeB依赖性形成可能类似于真核生物中泛素靶向蛋白质降解过程中的泛素激活步骤。为了确定MoeB在钼蝶呤生物合成中的具体作用,通过同源过表达纯化了该蛋白质。使用纯化的蛋白质,我们证明了MoeB和MoaD腺苷酸复合物的ATP依赖性形成,该复合物对凝胶过滤稳定。该复合物的质谱分析显示分子量为9073 Da的峰,这是MoaD腺苷酸的预期质量。然而,与泛素激活反应不同,未观察到MoeB和MoaD之间硫酯中间体的形成。在MoaD硫化过程中也没有证据表明存在与MoeB结合的硫。在MoeB的每个半胱氨酸残基中产生了氨基酸取代。除了位于假定的锌结合基序中的半胱氨酸残基发生突变外,所有这些都表现出与野生型相当的活性。对于这些半胱氨酸,活性丧失与金属结合丧失相关。

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