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OmpR对含有大肠杆菌ompC和ompF上游调控序列的融合构建体的分层和协同结合。

Hierarchical and co-operative binding of OmpR to a fusion construct containing the ompC and ompF upstream regulatory sequences of Escherichia coli.

作者信息

Bergstrom L C, Qin L, Harlocker S L, Egger L A, Inouye M

机构信息

Department of Biochemistry, Robert Wood Johnson Medical School, Piscataway, NJ 08854, USA.

出版信息

Genes Cells. 1998 Dec;3(12):777-88. doi: 10.1046/j.1365-2443.1998.00228.x.

DOI:10.1046/j.1365-2443.1998.00228.x
PMID:10096019
Abstract

BACKGROUND

OmpR is a transcription factor that regulates the expression of the porin genes ompF and ompC in Escherichia coli. The phosphorylation state of OmpR, directed by the osmosensor EnvZ, determines its ability to bind to the upstream regulatory regions of these genes, a total of 14 phospho-OmpR binding sites. While it has been possible to study the stoichiometry and hierarchy of the OmpR-DNA interaction in the upstream regions of ompF and ompC, their disunited location on the bacterial chromosome has made it difficult to compare the individual binding affinities of respective sites.

RESULTS

Using 1,10-phenanthroline-Cu+ footprinting on a fused construct containing both the ompF and ompC upstream regulatory sequences, and gel shift experiments on oligomers corresponding to individual sites, we have established a comparative hierarchy for OmpR binding, as F1, C1 > F2, F3 > C2 > C3. In addition, the binding patterns reveal an apparent co-operative relationship between OmpR molecules bound at several upstream motifs. Densitometric analyses of the footprinted regions provide support for these observations. Mutational analysis of this construct reveals that the alteration of a conserved cytidine in the F1 motif (-86) causes a loss of OmpR affinity and disrupts hierarchical OmpR-binding in the entire ompF region.

CONCLUSIONS

The present results provide a unique view of the OmpR interaction with the two respective promoters, ompF and ompC, and an insight into the question of how the expression of ompF and ompC are reciprocally regulated by medium osmolarity.

摘要

背景

OmpR是一种转录因子,可调节大肠杆菌中孔蛋白基因ompF和ompC的表达。由渗透压感受器EnvZ指导的OmpR磷酸化状态决定了其与这些基因上游调控区域结合的能力,共有14个磷酸化OmpR结合位点。虽然已经能够研究ompF和ompC上游区域中OmpR-DNA相互作用的化学计量和层次结构,但它们在细菌染色体上的分散位置使得难以比较各个位点的个体结合亲和力。

结果

使用1,10-菲咯啉-Cu +足迹法对包含ompF和ompC上游调控序列的融合构建体进行研究,并对对应于各个位点的寡聚物进行凝胶迁移实验,我们建立了OmpR结合的比较层次结构,即F1、C1 > F2、F3 > C2 > C3。此外,结合模式揭示了在几个上游基序处结合的OmpR分子之间明显的协同关系。对足迹区域的光密度分析为这些观察结果提供了支持。对该构建体的突变分析表明,F1基序(-86)中保守胞嘧啶的改变会导致OmpR亲和力丧失,并破坏整个ompF区域中OmpR结合的层次结构。

结论

目前的结果提供了OmpR与两个各自的启动子ompF和ompC相互作用的独特视角,并深入了解了ompF和ompC的表达如何受培养基渗透压相互调节的问题。

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