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Specificity of SecYEG for PhoA precursors and SecA homologs on SecA protein-conducting channels

机译:SecYEG对PhoA前体和SecA蛋白传导通道上SecA同源物的特异性

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摘要

Previous studies showed that Escherichia coli membranes depleted of SecYEG are capable of translocating certain precursor proteins, but not other precursors such as pPhoA, indicating a differential requirement for SecYEG. In this study, we examined the role of SecYEG in pPhoA translocation using a purified reconstituted SecA-liposomes system. We found that translocation of pPhoA, in contrast to that of pOmpA, requires the presence of purified SecYEG. A differential specificity of the SecYEG was also revealed in its interaction with SecA: EcSecYEG did not enhance SecA-mediated pOmpA translocation by purified SecA either from Pseudomonas aeruginosa or Bacillus subtilis. Neither was SecYEG required for eliciting ion channel activity, which could be opened by unfolded pPhoA or unfolded PhoA. Addition of the SecYEG complex did restore the specificity of signal peptide recognition in the ion-channel activity. We concluded that SecYEG confers specificity in interacting with protein precursors and SecAs.
机译:先前的研究表明,耗尽SecYEG的大肠杆菌膜能够转运某些前体蛋白,但不能转运其他前体,例如pPhoA,这表明对SecYEG的需求不同。在这项研究中,我们使用纯化的重组SecA-脂质体系统检查了SecYEG在pPhoA易位中的作用。我们发现,与pOmpA相比,pPhoA的移位需要存在纯化的SecYEG。 SecYEG与SecA的相互作用也显示出不同的特异性:EcSecYEG不能通过铜绿假单胞菌或枯草芽孢杆菌的纯化SecA增强SecA介导的pOmpA易位。引起离子通道活性的SecYEG都不是必需的,离子通道活性可以通过未折叠的pPhoA或未折叠的PhoA打开。 SecYEG复合物的添加确实恢复了离子通道活性中信号肽识别的特异性。我们得出的结论是,SecYEG在与蛋白质前体和SecA相互作用中赋予特异性。

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