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应激和饥饿诱导的gls24操纵子的失活对粪肠球菌的细胞形态、应激敏感性和基因表达具有多效性影响。

Inactivation of the stress- and starvation-inducible gls24 operon has a pleiotrophic effect on cell morphology, stress sensitivity, and gene expression in Enterococcus faecalis.

作者信息

Giard J C, Rince A, Capiaux H, Auffray Y, Hartke A

机构信息

Laboratoire de Microbiologie de l'Environnement, Université de Caen, 14032 Caen, France.

出版信息

J Bacteriol. 2000 Aug;182(16):4512-20. doi: 10.1128/JB.182.16.4512-4520.2000.

Abstract

Enterococcus faecalis induces the synthesis of at least 42 proteins during 24 h of glucose starvation. Because of its induction during carbohydrate and complete starvation (incubation in tap water) and CdCl(2) and bile salts stresses, one of these proteins (Gls24) was qualified as a "general stress protein" and was analyzed at the molecular level. Its corresponding gene, gls24, seems to be the penultimate gene of an operon composed, altogether, of six open reading frames (ORFs). The ORF preceding gls24 (orf4) showed very strong identity with gls24. The deduced polypeptides of these two genes showed similarity with a 20-kDa hypothetical protein from Lactococcus lactis and an alkaline stress protein from Staphylococcus aureus with no previously known biological significance. Data from the operon sequence and Northern analysis led to the conclusions that (i) gls24 possesses its own promoter which is especially induced at the onset of starvation and (ii) the operon promoter is stress inducible in exponential-phase cells. A mutation in the gls24 gene led to a severe reduction of growth rate and reduction of survival against 0.3% bile salts in the 24-h-starved cells compared to the wild-type strain. Moreover, the chain length of the mutant is significantly reduced during growth. These results argue strongly for a role of the protein Gls24 and/or GlsB in morphological changes and in stress tolerance in E. faecalis. Comparison of two-dimensional protein gels from wild-type cells with those from gls24 mutant cells revealed a pleiotropic effect of the mutation on gene expression. At least nine proteins were present in larger amounts in the mutant. For six of them, the corresponding N-terminal microsequence has been obtained. Three of these sequences map in genes coding for L-lactate dehydrogenase, lipoamide dehydrogenase, and pyruvate decarboxylase, all involved in pyruvate metabolism.

摘要

粪肠球菌在葡萄糖饥饿24小时期间诱导至少42种蛋白质的合成。由于其在碳水化合物饥饿和完全饥饿(在自来水中培养)以及氯化镉和胆盐胁迫期间被诱导,其中一种蛋白质(Gls24)被鉴定为“一般应激蛋白”,并在分子水平上进行了分析。其相应的基因gls24似乎是一个操纵子的倒数第二个基因,该操纵子总共由六个开放阅读框(ORF)组成。gls24之前的ORF(orf4)与gls24具有非常高的同源性。这两个基因推导的多肽与来自乳酸乳球菌的一种20 kDa假想蛋白和来自金黄色葡萄球菌的一种碱性应激蛋白相似,以前没有已知的生物学意义。操纵子序列和Northern分析的数据得出以下结论:(i)gls24拥有自己的启动子,该启动子在饥饿开始时特别被诱导;(ii)操纵子启动子在指数生长期细胞中可被应激诱导。与野生型菌株相比,gls24基因突变导致24小时饥饿细胞的生长速率严重降低,对0.3%胆盐的存活率降低。此外,突变体在生长过程中的链长度显著缩短。这些结果有力地证明了蛋白质Gls24和/或GlsB在粪肠球菌形态变化和应激耐受性中的作用。野生型细胞与gls24突变体细胞的二维蛋白质凝胶比较揭示了该突变对基因表达的多效性影响。突变体中至少有九种蛋白质的含量更高。其中六种蛋白质的相应N端微序列已获得。其中三个序列位于编码L-乳酸脱氢酶、硫辛酰胺脱氢酶和丙酮酸脱羧酶的基因中,这些酶都参与丙酮酸代谢。

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