新生的Lep在YidC、SecY和SecA附近插入大肠杆菌内膜。

Nascent Lep inserts into the Escherichia coli inner membrane in the vicinity of YidC, SecY and SecA.

作者信息

Houben E N, Scotti P A, Valent Q A, Brunner J, de Gier J L, Oudega B, Luirink J

机构信息

Department of Microbiology, Institute of Molecular Biological Sciences, Biocentrum Amsterdam, The Netherlands.

出版信息

FEBS Lett. 2000 Jul 7;476(3):229-33. doi: 10.1016/s0014-5793(00)01735-x.

DOI:10.1016/s0014-5793(00)01735-x

PMID:10913619

Abstract

Targeting and assembly of the Escherichia coli inner membrane protein leader peptidase (Lep) was studied using a homologous in vitro targeting/translocation assay. Assembly of full-length Lep was efficient in the co-translational presence of membrane vesicles and hardly occurred when membranes were added post-translationally. This is consistent with the signal recognition particle-dependent targeting of Lep. Crosslinking experiments showed that the hydrophilic region P1 of nascent membrane-inserted Lep 100-mer was in the vicinity of SecA and SecY, whereas the first transmembrane domain H1 was in the vicinity of YidC. These results suggested that YidC, together with the Sec translocase, functions in the assembly of Lep. YidC might be a more generic component in the assembly of inner membrane proteins.

摘要

利用同源体外靶向/转位分析方法，对大肠杆菌内膜蛋白前导肽酶（Lep）的靶向和组装进行了研究。在膜泡共翻译存在的情况下，全长Lep的组装效率很高，而在翻译后添加膜时几乎不发生组装。这与Lep的信号识别颗粒依赖性靶向一致。交联实验表明，新生的插入膜的Lep 100聚体的亲水区P1靠近SecA和SecY，而第一个跨膜结构域H1靠近YidC。这些结果表明，YidC与Sec转位酶一起参与Lep的组装。YidC可能是内膜蛋白组装中更普遍的成分。

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新生的Lep在YidC、SecY和SecA附近插入大肠杆菌内膜。

Nascent Lep inserts into the Escherichia coli inner membrane in the vicinity of YidC, SecY and SecA.

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