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分泌蛋白转运到大肠杆菌膜泡中需要SecA蛋白。

SecA protein is required for secretory protein translocation into E. coli membrane vesicles.

作者信息

Cabelli R J, Chen L, Tai P C, Oliver D B

机构信息

Department of Microbiology, State University of New York, Stony Brook, 11794.

出版信息

Cell. 1988 Nov 18;55(4):683-92. doi: 10.1016/0092-8674(88)90227-9.

Abstract

The soluble and membrane components of an E. coli in vitro protein translocation system prepared from a secA amber mutant, secA13[Am], contain reduced levels of SecA and are markedly defective in both the cotranslational and posttranslational translocation of OmpA and alkaline phosphatase into membrane vesicles. Moreover, the removal of SecA from soluble components prepared from a wild-type strain by passage through an anti-SecA antibody column similarly abolishes protein translocation. Translocation activity is completely restored by addition of submicrogram amounts of purified SecA protein, implying that the observed defects are solely related to loss of SecA function. Interestingly, the translocation defect can be overcome by reconstitution of SecA into SecA-depleted membranes, suggesting that SecA is an essential, membrane-associated translocation factor.

摘要

从secA琥珀突变体secA13[Am]制备的大肠杆菌体外蛋白质转运系统的可溶性和膜成分中,SecA水平降低,并且在OmpA和碱性磷酸酶向膜囊泡的共翻译和翻译后转运中均存在明显缺陷。此外,通过抗SecA抗体柱处理从野生型菌株制备的可溶性成分中去除SecA同样会消除蛋白质转运。通过添加亚微克量的纯化SecA蛋白可完全恢复转运活性,这意味着观察到的缺陷仅与SecA功能丧失有关。有趣的是,通过将SecA重构到SecA耗尽的膜中可以克服转运缺陷,这表明SecA是一种必需的、与膜相关的转运因子。

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