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The Mycobacterial LysR-Type Regulator OxyS Responds to Oxidative Stress and Negatively Regulates Expression of the Catalase-Peroxidase Gene

机译:分枝杆菌LysR型调节剂OxyS响应氧化应激,并负调控过氧化氢酶过氧化物酶基因的表达。

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摘要

Protection against oxidative stress is one of the primary defense mechanisms contributing to the survival of Mycobacterium tuberculosis in the host. In this study, we provide evidence that OxyS, a LysR-type transcriptional regulator functions as an oxidative stress response regulator in mycobacteria. Overexpression of OxyS lowers expression of the catalase-peroxidase (KatG) gene in M. smegmatis. OxyS binds directly with the katG promoter region and a conserved, GC-rich T-N11-A motif for OxyS binding was successfully characterized in the core binding site. Interestingly, the DNA-binding activity of OxyS was inhibited by H2O2, but not by dithiothreitol. Cys25, which is situated at the DNA-binding domain of OxyS, was found to have a regulatory role for the DNA-binding ability of OxyS in response to oxidative stress. In contrast, the other three cysteine residues in OxyS do not appear to have this function. Furthermore, the mycobacterial strain over-expressing OxyS had a higher sensitivity to H2O2.Thus, OxyS responds to oxidative stress through a unique cysteine residue situated in its DNA-binding domain and negatively regulates expression of the katG gene. These findings uncover a specific regulatory mechanism for mycobacterial adaptation to oxidative stress.
机译:防止氧化应激是有助于结核分枝杆菌在宿主中存活的主要防御机制之一。在这项研究中,我们提供的证据表明,LysR型转录调节剂OxyS在分枝杆菌中起氧化应激反应调节剂的作用。 OxyS的过表达降低了耻垢分枝杆菌中过氧化氢酶过氧化物酶(KatG)基因的表达。 OxyS直接与katG启动子区域结合,并且在核心结合位点成功鉴定了保守的,富含GC的OxyS结合的T-N11-A基序。有趣的是,OxyS的DNA结合活性受H2O2抑制,但不受二硫苏糖醇抑制。发现位于OxyS的DNA结合结构域的Cys25对氧化应激响应的OxyS的DNA结合能力具有调节作用。相反,OxyS中的其他三个半胱氨酸残基似乎不具有此功能。此外,过分表达OxyS的分枝杆菌菌株对H2O2的敏感性更高,因此,OxyS通过位于其DNA结合结构域的独特半胱氨酸残基对氧化应激作出反应,并对katG基因的表达产生负调控。这些发现揭示了分枝杆菌适应氧化应激的特定调节机制。

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  • 作者

    Li, Yuqing; He, Zheng-Guo;

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  • 年度 2012
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  • 原文格式 PDF
  • 正文语种 {"code":"en","name":"English","id":9}
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