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ClpX,大肠杆菌ATP依赖性Clp蛋白酶的一种替代亚基。序列及体内活性。

ClpX, an alternative subunit for the ATP-dependent Clp protease of Escherichia coli. Sequence and in vivo activities.

作者信息

Gottesman S, Clark W P, de Crecy-Lagard V, Maurizi M R

机构信息

Laboratory of Molecular Biology, National Cancer Institute, Bethesda, Maryland 20892.

出版信息

J Biol Chem. 1993 Oct 25;268(30):22618-26.

PMID:8226770
Abstract

The ATP-dependent Clp protease of Escherichia coli consists of two subunits, the ClpP subunit, which has the proteolytic active site, and ClpA, which possesses ATPase activity and activates the proteolytic activity of ClpP in vitro. Recently, Zylicz and co-workers (Wojtkowiak, D., Georgopoulos, C., and Zylicz, M. (1993) J. Biol. Chem. 268, 22609-22617) identified another E. coli protein that activated ATP-dependent degradation of lambda O protein in the presence of ClpP. The amino-terminal sequence of this protein corresponds to the translated amino-terminal sequence of a gene that we have named clpX. clpX encodes a protein with M(r) 46,300, similar to that observed for the protein purified by Wojtkowiak et al. clpX is an operon with clpP; both genes are cotranscribed in a single heat-inducible 2200-base mRNA, with clpP the promoter proximal gene. The sequence of ClpX includes a single consensus ATP-binding site motif and has limited homology to regions of ClpA and other members of the ClpA/B/C family. A third group of proteins, ClpY, closely related to ClpX, has been identified by sequence homology. Mutations in either clpX or clpP abolish degradation of the highly unstable lambda O protein in vivo. clpX mutants are not defective in degradation of previously identified ClpA/ClpP substrates such as a ClpA-beta-galactosidase fusion protein. It appears that selectivity of degradation by ClpP in vivo is determined by interaction of ClpP with different regulatory ATPase subunits.

摘要

大肠杆菌的ATP依赖性Clp蛋白酶由两个亚基组成,即具有蛋白水解活性位点的ClpP亚基和具有ATP酶活性并在体外激活ClpP蛋白水解活性的ClpA。最近,齐利茨及其同事(沃伊特科维亚克,D.,乔治opoulos,C.,和齐利茨,M.(1993年)《生物化学杂志》268,22609 - 22617)鉴定出另一种大肠杆菌蛋白,该蛋白在ClpP存在的情况下激活λO蛋白的ATP依赖性降解。这种蛋白的氨基末端序列与我们命名为clpX的基因的翻译后的氨基末端序列相对应。clpX编码一种分子量为46,300的蛋白质,与沃伊特科维亚克等人纯化的蛋白质相似。clpX与clpP是一个操纵子;这两个基因在一个单一的热诱导型2200碱基的mRNA中共同转录,clpP是启动子近端基因。ClpX的序列包括一个单一的共有ATP结合位点基序,并且与ClpA和ClpA/B/C家族的其他成员的区域具有有限的同源性。通过序列同源性鉴定出了第三组与ClpX密切相关的蛋白质ClpY。clpX或clpP中的突变都会消除体内高度不稳定的λO蛋白的降解。clpX突变体在降解先前鉴定的ClpA/ClpP底物(如ClpA - β - 半乳糖苷酶融合蛋白)方面没有缺陷。看来体内ClpP降解的选择性是由ClpP与不同的调节性ATP酶亚基的相互作用决定的。

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