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大肠杆菌双精氨酸转运酶亚基的突变通过对转运活性或tat复合物结构的不同影响来阻断功能。

Mutations in subunits of the Escherichia coli twin-arginine translocase block function via differing effects on translocation activity or tat complex structure.

作者信息

Barrett Claire M L, Mangels Dorothea, Robinson Colin

机构信息

Department of Biological Sciences, University of Warwick, Coventry CV4 7AL, UK.

出版信息

J Mol Biol. 2005 Mar 25;347(2):453-63. doi: 10.1016/j.jmb.2005.01.026. Epub 2005 Jan 22.

DOI:10.1016/j.jmb.2005.01.026
PMID:15740752
Abstract

We have used a combination of blue-native (BN) gel electrophoresis and protein purification to analyze the effects of TatA or TatC mutations on the structures of the primary TatABC and multimeric TatA complexes in Escherichia coli. Expression of wild-type TatABC leads to the production of a single major TatABC complex of 370 kDa and a heterogeneous set of TatA complexes of <100 kDa to approximately 500 kDa. Two TatC mutations that block translocation have different effects on complex structures. P48A causes massive defects in TatABC assembly, including a marked separation of the TatBC subunits and the production of TatB and TatC aggregates. In contrast, TatABC complexes from the inactive TatC F94A mutant are structurally intact, suggesting that this mutation affects translocation activity rather than assembly. Neither TatC mutation affects the separate TatA complexes, showing that assembly of the TatA complexes is independent of TatABC assembly or activity. In contrast, three TatA mutations affect both the TatA and TatABC complexes. F39A assembles into smaller, incorrectly organized TatA complexes and the TatABC complexes contain an incorrect TatB:TatC ratio and unusually large amounts of TatA. A triple mutant in the amphipathic region forms slightly larger TatA complexes that are likewise disorganized, and a mutant containing three glycine substitutions in the transmembrane (TM) span assembles as grossly affected TatA complexes that are much larger than wild-type complexes. These mutants lead to a partial failure of TatB to assemble correctly. The data show that the amphipathic and TM regions play critical roles in TatA complex assembly. All of the TatA mutations lead to partial or substantial defects in TatABC complex formation, demonstrating that the properties of TatA can have a marked influence on the TatABC complex.

摘要

我们运用蓝色非变性(BN)凝胶电泳和蛋白质纯化相结合的方法,分析了TatA或TatC突变对大肠杆菌中主要TatABC复合物和多聚体TatA复合物结构的影响。野生型TatABC的表达会产生一个370 kDa的单一主要TatABC复合物,以及一组分子量小于100 kDa至约500 kDa的异质性TatA复合物。两个阻断转运的TatC突变对复合物结构有不同影响。P48A导致TatABC组装出现大量缺陷,包括TatBC亚基明显分离以及TatB和TatC聚集体的产生。相比之下,来自无活性TatC F94A突变体的TatABC复合物结构完整,这表明该突变影响转运活性而非组装。两个TatC突变均不影响单独的TatA复合物,表明TatA复合物的组装独立于TatABC的组装或活性。相反,三个TatA突变同时影响TatA和TatABC复合物。F39A组装成更小、组织错误的TatA复合物,且TatABC复合物中TatB:TatC比例不正确,TatA含量异常高。两亲区域的一个三重突变体形成稍大但同样无序的TatA复合物,而在跨膜(TM)区段含有三个甘氨酸取代的突变体组装成严重受影响的TatA复合物,其比野生型复合物大得多。这些突变导致TatB部分无法正确组装。数据表明两亲区域和TM区段在TatA复合物组装中起关键作用。所有TatA突变均导致TatABC复合物形成出现部分或严重缺陷,表明TatA特性可对TatABC复合物产生显著影响。

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