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ClpV,一种致病性变形菌独特的Hsp100/Clp成员。

ClpV, a unique Hsp100/Clp member of pathogenic proteobacteria.

作者信息

Schlieker Christian, Zentgraf Hanswalter, Dersch Petra, Mogk Axel

机构信息

Zentrum für Molekulare Biologie, Universität Heidelberg, Im Neuenheimer Feld 282, D-69120 Heidelberg, Germany.

出版信息

Biol Chem. 2005 Nov;386(11):1115-27. doi: 10.1515/BC.2005.128.

DOI:10.1515/BC.2005.128
PMID:16307477
Abstract

Hsp100/Clp proteins are key players in the protein quality control network of prokaryotic cells and function in the degradation and refolding of misfolded or aggregated proteins. Here we report the identification of a new class of Hsp100/Clp proteins, termed ClpV (virulent strain), that are present in bacteria interacting with eukaryotic cells, including human pathogens. The ClpV proteins are most similar to ClpB proteins within the Hsp100/Clp family, but cluster in a separate phylogenetic tree with a remarkable distance to ClpB. ClpV representatives from Salmonella typhimurium and enteropathogenic Escherichia coli form oligomeric assemblies and display ATP hydrolysis rates comparable to ClpB. However, unlike ClpB, both ClpV proteins failed to solubilize aggregated proteins. This lack of disaggregation activity correlated with the inability of ClpB model substrates to stimulate the ATPase activity of ClpV proteins, indicating differences in substrate selection. Furthermore, we show that clpV genes are generally organized in a conserved gene cluster, encoding a potential secretion system, and we demonstrate that increased levels of a dominant negative variant of either S. typhimurium or Yersinia pseudotuberculosis ClpV strongly reduce the ability of these pathogenic bacteria to invade epithelial cells. We propose a role of this novel and unique class of AAA+ proteins in bacteria-host cell interactions.

摘要

热休克蛋白100/Clp蛋白是原核细胞蛋白质质量控制网络中的关键因子,在错误折叠或聚集蛋白的降解和重折叠过程中发挥作用。在此,我们报告了一类新的热休克蛋白100/Clp蛋白的鉴定结果,这类蛋白被称为ClpV(致病菌株型),存在于与真核细胞相互作用的细菌中,包括人类病原体。ClpV蛋白在热休克蛋白100/Clp家族中与ClpB蛋白最为相似,但在一个单独的系统发育树中聚类,与ClpB有显著距离。来自鼠伤寒沙门氏菌和肠致病性大肠杆菌的ClpV代表形成寡聚体组装体,其ATP水解速率与ClpB相当。然而,与ClpB不同的是,这两种ClpV蛋白都未能溶解聚集蛋白。这种解聚活性的缺乏与ClpB模型底物无法刺激ClpV蛋白的ATP酶活性相关,表明底物选择存在差异。此外,我们发现clpV基因通常组织在一个保守的基因簇中,编码一种潜在的分泌系统,并且我们证明,鼠伤寒沙门氏菌或假结核耶尔森氏菌ClpV的显性负变体水平升高会强烈降低这些病原菌侵入上皮细胞的能力。我们提出这类新颖独特的AAA +蛋白在细菌 - 宿主细胞相互作用中发挥作用。

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