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嗜土克雷伯氏菌中控制丁二醇发酵途径的转录激活因子的鉴定。

Identification of the transcriptional activator controlling the butanediol fermentation pathway in Klebsiella terrigena.

作者信息

Mayer D, Schlensog V, Böck A

机构信息

Lehrstuhl für Mikrobiologie, Universität München, Germany.

出版信息

J Bacteriol. 1995 Sep;177(18):5261-9. doi: 10.1128/jb.177.18.5261-5269.1995.

Abstract

The gene budR, whose product is responsible for induction of the butanediol formation pathway under fermentative growth conditions in Klebsiella terrigena, has been cloned and sequenced. This gene is separated from the budABC operon by a nontranslated region of 106 bp and transcribed in the opposite direction. budR codes for a protein of molecular weight 32,124, the sequence of which exhibits characteristics of regulators belonging to the LysR family. When transferred into the heterologous host Escherichia coli, budR activates expression of budA'-lacZ transcriptional and translational fusions with a regulatory pattern identical to that in K. terrigena, namely, induction by acetate, low pH, and anaerobiosis. Induction by acetate was specific, indicating that it is the physiological inducer. Primer extension analysis located the start site of transcription to two positions, 23 and 24 bp upstream of the budR initiation codon, and also showed that BudR strongly autoregulates its own expression. The products of fhlA, arcA, hip, ntrA, and katF did not influence expression of the bud operon. A mutation in fnr, however, led to a threefold increase in expression, indicating that Fnr acts as a repressor. The results support the notion that BudR coordinates the activity of the energy-conserving, nonreductive, but acidifying acetate formation pathway with the expression of the non-energy-conserving, reductive, but nonacidifying butanediol pathway.

摘要

基因budR已被克隆并测序,其产物负责在土生克雷伯氏菌发酵生长条件下诱导丁二醇形成途径。该基因与budABC操纵子被一个106 bp的非翻译区域隔开,并以相反方向转录。budR编码一种分子量为32,124的蛋白质,其序列具有属于LysR家族的调节因子的特征。当转入异源宿主大肠杆菌时,budR激活budA'-lacZ转录和翻译融合体的表达,其调节模式与土生克雷伯氏菌中的相同,即由乙酸盐、低pH和厌氧诱导。乙酸盐诱导具有特异性,表明它是生理诱导剂。引物延伸分析将转录起始位点定位在budR起始密码子上游23和24 bp的两个位置,并且还表明BudR强烈地自我调节其自身的表达。fhlA、arcA、hip、ntrA和katF的产物不影响bud操纵子的表达。然而,fnr中的一个突变导致表达增加三倍,表明Fnr起阻遏作用。结果支持这样的观点,即BudR将能量保守、非还原但酸化的乙酸盐形成途径的活性与非能量保守、还原但非酸化的丁二醇途径的表达协调起来。

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