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Structure of a translocation signal domain mediating conjugative transfer by type IV secretion systems

机译:通过IV型分泌系统介导共轭转移的易位信号域的结构

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摘要

Relaxases are proteins responsible for the transfer of plasmid and chromosomal DNA from one bacterium to another during conjugation. They covalently react with a specific phosphodiester bond within DNA origin of transfer sequences, forming a nucleo-protein complex which is subsequently recruited for transport by a plasmid-encoded type IV secretion system. In previous work we identified the targeting translocation signals presented by the conjugative relaxase TraI of plasmid R1. Here we report the structure of TraI translocation signal TSA. In contrast to known translocation signals we show that TSA is an independent folding unit and thus forms a bona fide structural domain. This domain can be further divided into three subdomains with striking structural homology with helicase subdomains of the SF1B family. We also show that TSA is part of a larger vestigial helicase domain which has lost its helicase activity but not its single-stranded DNA binding capability. Finally, we further delineate the binding site responsible for translocation activity of TSA by targeting single residues for mutations. Overall, this study provides the first evidence that translocation signals can be part of larger structural scaffolds, overlapping with translocation-independent activities.
机译:松弛酶是负责在接合过程中将质粒和染色体DNA从一种细菌转移到另一种细菌的蛋白质。它们与转移序列的DNA起点内的特定磷酸二酯键共价反应,形成核蛋白复合物,随后将其募集用于通过质粒编码的IV型分泌系统进行转运。在以前的工作中,我们鉴定了由质粒R1的共轭松弛酶TraI呈现的靶向易位信号。在这里,我们报告TraI易位信号TSA的结构。与已知的易位信号相反,我们表明TSA是一个独立的折叠单元,因此形成了真正的结构域。该结构域可进一步分为三个与SF1B家族的解旋酶亚结构域具有显着结构同源性的亚结构域。我们还显示,TSA是更大的残留解旋酶结构域的一部分,该结构已失去其解旋酶活性,但没有其单链DNA结合能力。最后,我们通过针对突变的单个残基进一步描述了负责TSA转运活性的结合位点。总的来说,这项研究提供了第一个证据,即易位信号可能是较大的结构支架的一部分,与不依赖位的活动重叠。

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