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一种具有羧基酯酶活性的新型细胞壁锚定蛋白的特性研究,该蛋白是结核分枝杆菌毒力所必需的。

Characterization of a novel cell wall-anchored protein with carboxylesterase activity required for virulence in Mycobacterium tuberculosis.

作者信息

Lun Shichun, Bishai William R

机构信息

Department of Medicine, Center for Tuberculosis Research, Johns Hopkins University School of Medicine, Baltimore, Maryland 21231.

Department of Medicine, Center for Tuberculosis Research, Johns Hopkins University School of Medicine, Baltimore, Maryland 21231.

出版信息

J Biol Chem. 2007 Jun 22;282(25):18348-18356. doi: 10.1074/jbc.M700035200. Epub 2007 Apr 11.

DOI:10.1074/jbc.M700035200
PMID:17428787
Abstract

Pooled mutant competition assays have shown that the Mycobacterium tuberculosis MT2282 gene (Rv2224c, annotated as encoding a proteinase) is required for bacterial survival in mice. To understand the mechanism of this requirement, we conducted a genetic and biochemical study of the MT2282 gene and its product. MT2282 encodes a member of the microbial esterase/lipase family with active site consensus sequences of G-X-S-X-G, and we have concluded that the MT2282 protein is, in fact, a cell wall-associated carboxylesterase rather than a proteinase, as initially annotated. The MT2282 gene product preferentially hydrolyzes ester bonds of substrates with intermediate carbon chain length. Purified MT2282 is a monomer with enzymatic catalysis properties that fit in the Michaelis-Menten kinetic model. Esterase activity was inhibited by paraoxon and dichlorvos. Replacement of Ser215, Asp450, and His477 by Ala in the consensus motifs completely abolishes esterase activity, suggesting that Ser215-Asp450-His477 forms a catalytic triad with Ser215 as an active site residue. To evaluate the role of the MT2282 in pathogenesis, the gene was deleted from the M. tuberculosis genome. BALB/c mouse aerosol infections showed reduced colony-forming unit loads in lungs and spleens and less lung pathology for the DeltaMT2282 mutant. High dose intravenous infection of mice with the mutant resulted in a significantly delayed time to death compared with the wild type or complemented mutant. These results indicate that MT2282 encodes a cell wall-associated carboxylesterase, which is required for full virulence of M. tuberculosis. We propose that MT2282 (Rv2224c) and its adjacent paralogous gene MT2281 (Rv2223c) be named caeA and caeB respectively, for carboxylesterase A and B.

摘要

汇集突变体竞争试验表明,结核分枝杆菌MT2282基因(Rv2224c,注释为编码一种蛋白酶)是细菌在小鼠体内存活所必需的。为了解这种必需性的机制,我们对MT2282基因及其产物进行了遗传学和生物化学研究。MT2282编码微生物酯酶/脂肪酶家族的一个成员,其活性位点共有序列为G-X-S-X-G,我们得出结论,MT2282蛋白实际上是一种与细胞壁相关的羧酸酯酶,而不是最初注释的蛋白酶。MT2282基因产物优先水解具有中等碳链长度底物的酯键。纯化的MT2282是一种单体,其酶催化特性符合米氏动力学模型。对氧磷和敌敌畏可抑制酯酶活性。在共有基序中用丙氨酸取代Ser215、Asp450和His477会完全消除酯酶活性,这表明Ser215-Asp450-His477形成了一个催化三联体,其中Ser215是活性位点残基。为了评估MT2282在发病机制中的作用,从结核分枝杆菌基因组中删除了该基因。BALB/c小鼠气溶胶感染显示,DeltaMT2282突变体的肺和脾中集落形成单位负荷降低,肺部病理变化减少。与野生型或互补突变体相比,用该突变体对小鼠进行高剂量静脉感染导致死亡时间显著延迟。这些结果表明,MT2282编码一种与细胞壁相关的羧酸酯酶,这是结核分枝杆菌完全毒力所必需的。我们建议将MT2282(Rv2224c)及其相邻的旁系同源基因MT2281(Rv2223c)分别命名为caeA和caeB,即羧酸酯酶A和羧酸酯酶B。

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