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线粒体合成的Cox2结构域从线粒体基质转运至膜间隙。

Translocation of mitochondrially synthesized Cox2 domains from the matrix to the intermembrane space.

作者信息

Fiumera Heather L, Broadley Sarah A, Fox Thomas D

机构信息

Department of Molecular Biology and Genetics, Biotechnology Building, Cornell University, Ithaca, NY 14853-2703, USA.

出版信息

Mol Cell Biol. 2007 Jul;27(13):4664-73. doi: 10.1128/MCB.01955-06. Epub 2007 Apr 23.

Abstract

The N-terminal and C-terminal domains of mitochondrially synthesized cytochrome c oxidase subunit II, Cox2, are translocated through the inner membrane to the intermembrane space (IMS). We investigated the distinct mechanisms of N-tail and C-tail export by analysis of epitope-tagged Cox2 variants encoded in Saccharomyces cerevisiae mitochondrial DNA. Both the N and C termini of a truncated protein lacking the Cox2 C-terminal domain were translocated to the IMS via a pathway dependent upon the conserved translocase Oxa1. The topology of this Cox2 variant, accumulated at steady state, was largely but not completely unaffected in mutants lacking proteins required for export of the C-tail domain, Cox18 and Mss2. C-tail export was blocked by truncation of the last 40 residues from the C-tail domain, indicating that sequence and/or structural features of this domain are required for its translocation. Mss2, a peripheral protein bound to the inner surface of the inner membrane, coimmunoprecipitated with full-length newly synthesized Cox2, whose leader peptide had already been cleaved in the IMS. Our data suggest that the C-tail domain is recognized posttranslationally by a specialized translocation apparatus after the N-tail has been translocated by Oxa1.

摘要

线粒体合成的细胞色素c氧化酶亚基II(Cox2)的N端和C端结构域通过内膜转运到膜间隙(IMS)。我们通过分析酿酒酵母线粒体DNA中编码的表位标记的Cox2变体,研究了N端和C端输出的不同机制。缺乏Cox2 C端结构域的截短蛋白的N端和C端均通过依赖于保守转运酶Oxa1的途径转运到IMS。在缺乏C端结构域输出所需蛋白Cox18和Mss2的突变体中,这种在稳态下积累的Cox2变体的拓扑结构在很大程度上但并非完全不受影响。C端截短最后40个残基会阻断C端输出,表明该结构域的序列和/或结构特征是其转运所必需的。Mss2是一种与内膜内表面结合的外周蛋白,与全长新合成的Cox2共免疫沉淀,其前导肽已在IMS中被切割。我们的数据表明,在N端被Oxa1转运后,C端结构域在翻译后被一种特殊的转运装置识别。

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