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蛋白水解切割使金黄色葡萄球菌脂磷壁酸合成酶失活。

Proteolytic cleavage inactivates the Staphylococcus aureus lipoteichoic acid synthase.

机构信息

Section of Microbiology, Imperial College London, London SW7 2AZ, United Kingdom.

出版信息

J Bacteriol. 2011 Oct;193(19):5279-91. doi: 10.1128/JB.00369-11. Epub 2011 Jul 22.

DOI:10.1128/JB.00369-11
PMID:21784926
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3187375/
Abstract

Lipoteichoic acid (LTA) is a crucial cell envelope component in Gram-positive bacteria. In Staphylococcus aureus, the polyglycerolphosphate LTA molecule is synthesized by LtaS, a membrane-embedded enzyme with five N-terminal transmembrane helices (5TM domain) that are connected via a linker region to the C-terminal extracellular enzymatic domain (eLtaS). The LtaS enzyme is processed during bacterial growth, and the eLtaS domain is released from the bacterial membrane. Here we provide experimental evidence that the proteolytic cleavage following residues 215Ala-Leu-Ala217 is performed by the essential S. aureus signal peptidase SpsB, as depletion of spsB results in reduced LtaS processing. In addition, the introduction of a proline residue at the +1 position with respect to the cleavage site, a substitution known to inhibit signal peptidase-dependent cleavage, abolished LtaS processing at this site. It was further shown that the 5TM domain is crucial for enzyme function. The observation that the construction of hybrid proteins between two functional LtaS-type enzymes resulted in the production of proteins unable to synthesize LTA suggests that specific interactions between the 5TM and eLtaS domains are required for function. No enzyme activity was detected upon expression of the 5TM and eLtaS domains as separate fragments, indicating that the two domains cannot assemble postsynthesis to form a functional enzyme. Taken together, our data suggest that only the full-length LtaS enzyme is active in the LTA synthesis pathway and that the proteolytic cleavage step is used as a mechanism to irreversibly inactivate the enzyme.

摘要

脂磷壁酸 (LTA) 是革兰氏阳性菌细胞外膜的重要组成部分。在金黄色葡萄球菌中,多聚甘油磷酸化的 LTA 分子由 LtaS 合成,LtaS 是一种膜结合酶,具有五个 N 端跨膜螺旋(5TM 结构域),通过连接区与 C 端细胞外酶结构域(eLtaS)相连。LtaS 酶在细菌生长过程中被加工,eLtaS 结构域从细菌膜上释放出来。本研究提供了实验证据表明,残基 215Ala-Leu-Ala217 之后的蛋白水解切割是由必需的金黄色葡萄球菌信号肽酶 SpsB 完成的,因为 spsB 的缺失导致 LtaS 加工减少。此外,在切割位点的+1 位引入脯氨酸残基,这是一种已知抑制信号肽依赖性切割的取代,可使 LtaS 在该位点的加工被阻断。进一步表明,5TM 结构域对于酶功能至关重要。观察到两个功能性 LtaS 型酶之间的杂交蛋白的构建导致不能合成 LTA 的蛋白质的产生表明,5TM 和 eLtaS 结构域之间的特定相互作用对于功能是必需的。当分别表达 5TM 和 eLtaS 结构域作为单独的片段时,未检测到酶活性,表明这两个结构域不能在合成后组装形成具有功能的酶。综上所述,我们的数据表明,只有全长 LtaS 酶在 LTA 合成途径中具有活性,并且蛋白水解切割步骤被用作不可逆失活酶的机制。

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