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EmrR是大肠杆菌多药耐药泵EmrAB的负调控因子。

EmrR is a negative regulator of the Escherichia coli multidrug resistance pump EmrAB.

作者信息

Lomovskaya O, Lewis K, Matin A

机构信息

Department of Microbiology and Immunology, Stanford University School of Medicine, California 94305-5402, USA.

出版信息

J Bacteriol. 1995 May;177(9):2328-34. doi: 10.1128/jb.177.9.2328-2334.1995.

DOI:10.1128/jb.177.9.2328-2334.1995
PMID:7730261
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC176888/
Abstract

The emrAB locus of Escherichia coli encodes a multidrug resistance pump that protects the cell from several chemically unrelated antimicrobial agents, e.g., the protonophores carbonyl cyanide m-chlorophenylhydrazone (CCCP) and tetrachlorosalicyl anilide and the antibiotics nalidixic acid and thiolactomycin. The mprA gene is located immediately upstream of this locus and was shown to be a repressor of microcin biosynthesis (I. del Castillo, J. M. Gomez, and F. Moreno, J. Bacteriol. 173:3924-3929, 1991). There is a putative transcriptional terminator sequence between the mprA and emrA genes. To locate the emr promoter, single-copy lacZ operon fusions containing different regions of the emr locus were made. Only fusions containing the mprA promoter region were expressed. mprA is thus the first gene of the operon, and we propose that it be renamed emrR. Overproduction of the EmrR protein (with a multicopy vector containing the cloned emrR gene) suppressed transcription of the emr locus. A mutation in the emrR gene led to overexpression of the EmrAB pump and increased resistance to antimicrobial agents. CCCP, nalidixic acid, and a number of other structurally unrelated chemicals induced expression of the emr genes, and the induction required EmrR. We conclude that emrRAB genes constitute an operon and that EmrR serves as a negative regulator of this operon. Some of the chemicals that induce the pump serve as its substrates, suggesting that their extrusion is the natural function of the pump.

摘要

大肠杆菌的emrAB基因座编码一种多药耐药泵,可保护细胞免受几种化学性质不相关的抗菌剂的影响,例如质子载体羰基氰化物间氯苯腙(CCCP)和四氯水杨酰苯胺,以及抗生素萘啶酸和硫代乳霉素。mprA基因位于该基因座的紧邻上游,已被证明是微菌素生物合成的阻遏物(I. del Castillo、J. M. Gomez和F. Moreno,《细菌学杂志》173:3924 - 3929,1991)。在mprA和emrA基因之间存在一个推定的转录终止子序列。为了定位emr启动子,构建了包含emr基因座不同区域的单拷贝lacZ操纵子融合体。只有包含mprA启动子区域的融合体被表达。因此,mprA是该操纵子的第一个基因,我们建议将其重新命名为emrR。EmrR蛋白的过量表达(使用含有克隆的emrR基因的多拷贝载体)抑制了emr基因座的转录。emrR基因中的一个突变导致EmrAB泵的过度表达,并增加了对抗菌剂的抗性。CCCP、萘啶酸和许多其他结构不相关的化学物质诱导了emr基因的表达,并且这种诱导需要EmrR。我们得出结论,emrRAB基因构成一个操纵子,并且EmrR作为该操纵子的负调控因子。一些诱导该泵的化学物质是其底物,这表明它们的排出是该泵的天然功能。

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本文引用的文献

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Overexpression of the MarA positive regulator is sufficient to confer multiple antibiotic resistance in Escherichia coli.MarA正调控因子的过表达足以使大肠杆菌产生多重抗生素耐药性。
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