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硫醇-二硫键交换参与了肽甲硫氨酸亚砜还原酶的催化机制。

Thiol-disulfide exchange is involved in the catalytic mechanism of peptide methionine sulfoxide reductase.

作者信息

Lowther W T, Brot N, Weissbach H, Honek J F, Matthews B W

机构信息

Institute of Molecular Biology, Howard Hughes Medical Institute and Department of Physics, 1229 University of Oregon, Eugene, OR 97403-1229, USA.

出版信息

Proc Natl Acad Sci U S A. 2000 Jun 6;97(12):6463-8. doi: 10.1073/pnas.97.12.6463.

Abstract

Peptide methionine sulfoxide reductase (MsrA; EC ) reverses the inactivation of many proteins due to the oxidation of critical methionine residues by reducing methionine sulfoxide, Met(O), to methionine. MsrA activity is independent of bound metal and cofactors but does require reducing equivalents from either DTT or a thioredoxin-regenerating system. In an effort to understand these observations, the four cysteine residues of bovine MsrA were mutated to serine in a series of permutations. An analysis of the enzymatic activity of the variants and their free sulfhydryl states by mass spectrometry revealed that thiol-disulfide exchange occurs during catalysis. In particular, the strictly conserved Cys-72 was found to be essential for activity and could form disulfide bonds, only upon incubation with substrate, with either Cys-218 or Cys-227, located at the C terminus. The significantly decreased activity of the Cys-218 and Cys-227 variants in the presence of thioredoxin suggested that these residues shuttle reducing equivalents from thioredoxin to the active site. A reaction mechanism based on the known reactivities of thiols with sulfoxides and the available data for MsrA was formulated. In this scheme, Cys-72 acts as a nucleophile and attacks the sulfur atom of the sulfoxide moiety, leading to the formation of a covalent, tetracoordinate intermediate. Collapse of the intermediate is facilitated by proton transfer and the concomitant attack of Cys-218 on Cys-72, leading to the formation of a disulfide bond. The active site is returned to the reduced state for another round of catalysis by a series of thiol-disulfide exchange reactions via Cys-227, DTT, or thioredoxin.

摘要

肽甲硫氨酸亚砜还原酶(MsrA;EC )通过将甲硫氨酸亚砜(Met(O))还原为甲硫氨酸,逆转了许多因关键甲硫氨酸残基氧化而导致的蛋白质失活。MsrA的活性不依赖于结合的金属和辅因子,但确实需要来自二硫苏糖醇(DTT)或硫氧还蛋白再生系统的还原当量。为了理解这些观察结果,牛MsrA的四个半胱氨酸残基以一系列排列方式突变为丝氨酸。通过质谱分析变体的酶活性及其游离巯基状态,发现催化过程中发生了硫醇 - 二硫键交换。特别地,发现严格保守的Cys - 72对活性至关重要,并且仅在与底物孵育时,才能与位于C末端的Cys - 第218位或Cys - 第227位形成二硫键。在硫氧还蛋白存在下,Cys - 第218位和Cys - 第227位变体的活性显著降低,表明这些残基将还原当量从硫氧还蛋白转运至活性位点。基于硫醇与亚砜的已知反应性以及MsrA的现有数据,制定了一种反应机制。在该方案中,Cys - 72作为亲核试剂攻击亚砜部分的硫原子,导致形成共价四配位中间体。中间体的分解通过质子转移以及Cys - 第218位对Cys - 72的伴随攻击而促进,导致形成二硫键。活性位点通过经由Cys - 第227位、DTT或硫氧还蛋白的一系列硫醇 - 二硫键交换反应恢复到还原状态,以便进行另一轮催化。

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