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利用同步细胞杀伤和蛋白水解切割研究大肠杆菌素E9受体结合和易位的早期事件。

Investigating early events in receptor binding and translocation of colicin E9 using synchronized cell killing and proteolytic cleavage.

作者信息

Zhang Ying, Vankemmelbeke Mireille N, Holland Lisa E, Walker David C, James Richard, Penfold Christopher N

机构信息

School of Molecular Medical Sciences, Institute of Infection, Immunity and Inflammation, Centre for Biomolecular Sciences, University Park, Nottingham NG7 2RD, United Kingdom.

出版信息

J Bacteriol. 2008 Jun;190(12):4342-50. doi: 10.1128/JB.00047-08. Epub 2008 Apr 11.

Abstract

Enzymatic colicins such as colicin E9 (ColE9) bind to BtuB on the cell surface of Escherichia coli and rapidly recruit a second coreceptor, either OmpF or OmpC, through which the N-terminal natively disordered region (NDR) of their translocation domain gains entry into the cell periplasm and interacts with TolB. Previously, we constructed an inactive disulfide-locked mutant ColE9 (ColE9(s-s)) that binds to BtuB and can be reduced with dithiothreitol (DTT) to synchronize cell killing. By introducing unique enterokinase (EK) cleavage sites in ColE9(s-s), we showed that the first 61 residues of the NDR were inaccessible to cleavage when bound to BtuB, whereas an EK cleavage site inserted at residue 82 of the NDR remained accessible. This suggests that most of the NDR is occluded by OmpF shortly after binding to BtuB, whereas the extreme distal region of the NDR is surface exposed before unfolding of the receptor-binding domain occurs. EK cleavage of unique cleavage sites located in the ordered region of the translocation domain or in the distal region of the receptor-binding domain confirmed that these regions of ColE9 remained accessible at the E. coli cell surface. Lack of EK cleavage of the DNase domain of the cell-bound, oxidized ColE9/Im9 complex, and the rapid detection of Alexa Fluor 594-labeled Im9 (Im9(AF)) in the cell supernatant following treatment of cells with DTT, suggested that immunity release occurred immediately after unfolding of the colicin and was not driven by binding to BtuB.

摘要

诸如大肠杆菌素E9(ColE9)之类的酶促大肠杆菌素与大肠杆菌细胞表面的BtuB结合,并迅速募集第二种共受体,即OmpF或OmpC,通过该共受体,其转运结构域的N端天然无序区域(NDR)进入细胞周质并与TolB相互作用。此前,我们构建了一种无活性的二硫键锁定突变体ColE9(ColE9(s-s)),它能与BtuB结合,并且可以用二硫苏糖醇(DTT)还原以同步细胞杀伤。通过在ColE9(s-s)中引入独特的肠激酶(EK)切割位点,我们发现当与BtuB结合时,NDR的前61个残基无法被切割,而插入到NDR第82位残基处的EK切割位点仍然可被切割。这表明在与BtuB结合后不久,大部分NDR被OmpF封闭,而NDR的最远端区域在受体结合结构域展开之前暴露于表面。对位于转运结构域有序区域或受体结合结构域远端区域的独特切割位点进行EK切割,证实了ColE9的这些区域在大肠杆菌细胞表面仍然可及。细胞结合的氧化型ColE9/Im9复合物的DNase结构域缺乏EK切割,以及在用DTT处理细胞后在细胞上清液中快速检测到Alexa Fluor 594标记的Im9(Im9(AF)),表明免疫释放发生在大肠杆菌素展开后立即发生,而不是由与BtuB的结合驱动。

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