直接鉴定分子伴侣 SecB 与易位子马达 SecA 氨基末端结合部位。
Direct identification of the site of binding on the chaperone SecB for the amino terminus of the translocon motor SecA.
机构信息
Department of Biochemistry, University of Missouri, Columbia, Missouri 65211, USA.
出版信息
Protein Sci. 2010 Jun;19(6):1173-9. doi: 10.1002/pro.392.
Abstract
Protein export mediated by the general secretory Sec system in Escherichia coli proceeds by a dynamic transfer of a precursor polypeptide from the chaperone SecB to the SecA ATPase motor of the translocon and subsequently into and through the channel of the membrane-embedded SecYEG heterotrimer. The complex between SecA and SecB is stabilized by several separate sites of contact. Here we have demonstrated directly an interaction between the N-terminal residues 2 through 11 of SecA and the C-terminal 13 residues of SecB by isothermal titration calorimetry and analytical sedimentation velocity centrifugation. We discuss the unusual binding properties of SecA and SecB in context of a model for transfer of the precursor along the pathway of export.
摘要
大肠杆菌中由一般分泌 Sec 系统介导的蛋白质输出是通过前体多肽从伴侣蛋白 SecB 到易位子的 SecA ATP 酶马达的动态转移,然后进入并穿过膜嵌入的 SecYEG 异源三聚体的通道来进行的。SecA 和 SecB 之间的复合物通过几个单独的接触点稳定。在这里,我们通过等温滴定量热法和分析沉降速度离心直接证明了 SecA 的 N 端残基 2 至 11 与 SecB 的 C 端 13 残基之间的相互作用。我们讨论了 SecA 和 SecB 的异常结合特性,该特性与前体沿着输出途径转移的模型有关。
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本文引用的文献
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Mapping polypeptide interactions of the SecA ATPase during translocation.在易位过程中映射 SecA ATP 酶的多肽相互作用。
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Maximal efficiency of coupling between ATP hydrolysis and translocation of polypeptides mediated by SecB requires two protomers of SecA.SecB介导的ATP水解与多肽转运之间耦合的最大效率需要两个SecA原聚体。
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6
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