首页> 外文OA文献 >Regulation of the molybdate transport operon, modABCD, of Escherichia coli in response to molybdate availability.
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Regulation of the molybdate transport operon, modABCD, of Escherichia coli in response to molybdate availability.

机译:响应钼酸盐的可用性,对大肠杆菌的钼酸盐运输操纵子modABCD进行调节。

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摘要

The mod (chlD) locus at 17 min on the Escherichia coli chromosome encodes a high-affinity molybdate uptake system. To further investigate the structure and regulation of these genes, the DNA region upstream of the previously identified modBC (chlJD) genes was cloned and sequenced. A single open reading frame, designated modA, was identified and appears to encode a periplasmic binding protein for the molybdate uptake system. To determine how the mod genes are regulated in response to molybdate, nitrate, and oxygen, we constructed a series of mod-lacZ operon fusions to the upstream region and introduced them in single copy onto the E. coli chromosome. Whereas molybdate limitation resulted in elevated mod-lacZ expression, neither oxygen nor nitrate had any significant effect on gene expression. A regulatory motif, CATAA, located at the modA promoter was identified and shown to be required for molybdate-dependent control of the modABCD operon. Mutations within this sequence resulted in nearly complete derepression of gene expression and suggest that transcription of the operon is mediated by a molybdenum-responsive regulatory protein.
机译:大肠杆菌染色体上第17分钟的mod(chlD)基因座编码了高亲和力的钼酸盐摄取系统。为了进一步研究这些基因的结构和调控,克隆了先前鉴定的modBC(chJD)基因上游的DNA区域并进行了测序。鉴定出一个单一的开放阅读框,称为modA,似乎编码了钼酸盐摄取系统的周质结合蛋白。为了确定mod基因如何响应钼酸根,硝酸盐和氧气而受到调控,我们在上游区域构建了一系列mod-lacZ操纵子融合体,并将它们以单拷贝形式引入大肠杆菌染色体。钼酸盐的限制导致mod-lacZ表达升高,而氧和硝酸盐均未对基因表达产生任何显着影响。鉴定了位于modA启动子上的调控基序CATAA,并显示其是modABCD操纵子的钼酸盐依赖性控制所必需的。该序列内的突变导致基因表达的几乎完全抑制,表明操纵子的转录是由钼反应性调节蛋白介导的。

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