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大肠杆菌中铁超氧化物歧化酶的Fur正调控:sodB启动子的功能分析

Fur positive regulation of iron superoxide dismutase in Escherichia coli: functional analysis of the sodB promoter.

作者信息

Dubrac S, Touati D

机构信息

Institut Jacques Monod, CNRS-Universités Paris 6 et Paris 7, 75251 Paris Cedex 05, France.

出版信息

J Bacteriol. 2000 Jul;182(13):3802-8. doi: 10.1128/JB.182.13.3802-3808.2000.

DOI:10.1128/JB.182.13.3802-3808.2000
PMID:10850997
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC94553/
Abstract

In Escherichia coli, the expression of sodB, which encodes iron superoxide dismutase, has been suggested to be activated by Fur, the iron-responsive global regulator initially characterized as a transcriptional repressor. We investigated sodB regulation by functional analysis of the sodB promoter using sodB-lac fusions with various truncated and mutated promoters. Several cis- and trans-acting elements involved in sodB regulation have been identified. The beta-galactosidase activity of sodB-lacZ reporter fusions and RNA analysis showed sevenfold iron-dependent, Fur-mediated activation of expression. A region just downstream from -10, including a large palindromic sequence encompassing the +1 position followed by a 14-bp AT-rich motif, is the site of Fur positive regulation, and the integrity of both sequences was required for full Fur-mediated activation. The life span of sodB mRNA was three times longer in a fur(+) strain, indicating that Fur-mediated activation proceeds, at least in part, at the posttranscriptional level. The H-NS and IHF histone-like factors also affected sodB expression. IHF slightly repressed sodB expression independently of Fur regulation. In contrast, H-NS negative regulation operated only in the absence of Fur. Remarkably, psodB behaved like a "pure extended -10" promoter. Deletion of the -35 region did not affect expression, whereas expression was totally abolished by a TG-to-CC mutation in the extended -10 sequence TGcTACCCT.

摘要

在大肠杆菌中,有人提出编码铁超氧化物歧化酶的sodB的表达是由Fur激活的,Fur是一种铁响应性全局调节因子,最初被表征为转录阻遏物。我们使用具有各种截短和突变启动子的sodB - lac融合体,通过对sodB启动子的功能分析来研究sodB的调控。已经鉴定出了几个参与sodB调控的顺式和反式作用元件。sodB - lacZ报告融合体的β - 半乳糖苷酶活性和RNA分析表明,存在七倍的铁依赖性、Fur介导的表达激活。位于 - 10下游的一个区域,包括一个围绕 +1位置的大回文序列,后面跟着一个14bp富含AT的基序,是Fur正调控的位点,两个序列的完整性对于Fur介导的完全激活是必需的。在fur(+)菌株中,sodB mRNA的寿命长三倍,这表明Fur介导的激活至少部分发生在转录后水平。H - NS和IHF组蛋白样因子也影响sodB的表达。IHF独立于Fur调控轻微抑制sodB的表达。相反,H - NS的负调控仅在没有Fur时起作用。值得注意的是,psodB表现得像一个“纯延伸 - 10”启动子。 - 35区域的缺失不影响表达,而延伸 - 10序列TGcTACCCT中的TG到CC突变则完全消除了表达。

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