首页> 外文期刊>Nucleic Acids Research >Posttranscriptional repression of the cel gene of the ColE7 operon by the RNA-binding protein CsrA of Escherichia coli.
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Posttranscriptional repression of the cel gene of the ColE7 operon by the RNA-binding protein CsrA of Escherichia coli.

机译:大肠杆菌的RNA结合蛋白CsrA对ColE7操纵子的cel基因进行转录后抑制。

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摘要

Carbon storage regulator (CsrA) is a eubacterial RNA-binding protein that acts as a global regulator of many functionally diverse chromosomal genes. Here, we reveal that CsrA represses expression from an extrachromosomal element of Escherichia coli, the lysis gene (cel) of the ColE7 operon (cea-cei-cel). This operon and colicin expression are activated upon SOS response. Disruption of csrA caused approximately 5-fold increase of the lysis protein. Gel mobility shift assays established that both the single-stranded loop of the T1 stem-loop distal to cei, and the putative CsrA binding site overlapping the Shine-Dalgarno sequence (SD) of the cel gene are important for CsrA binding. Substitution mutations at SD relieved CsrA-dependent repression of the cel gene in vivo. Steady-state levels and half-life of the cel mRNA were not affected by CsrA, implying that regulation is mediated at the translational level. Levels of CsrB and CsrC sRNAs, which bind to and antagonize CsrA, were drastically reduced upon induction of the SOS response, while the CsrA protein itself remained unaffected. Thus, CsrA is a trans-acting modulator that downregulates the expression of lysis protein, which may confer a survival advantage on colicinogenic E. coli under environment stress conditions.
机译:碳储存调节剂(CsrA)是一种真细菌RNA结合蛋白,可作为许多功能多样的染色体基因的全局调节剂。在这里,我们揭示了CsrA抑制大肠杆菌的染色体外元件,即ColE7操纵子的裂解基因(cel)(cea-cei-cel)的表达。该操纵子和大肠菌素表达在SOS反应后被激活。 csrA的破坏导致裂解蛋白增加约5倍。凝胶迁移率迁移分析确定,cei远端的T1茎环的单链环和与cel基因的Shine-Dalgarno序列(SD)重叠的推定CsrA结合位点对于CsrA结合都很重要。 SD的取代突变可缓解体内cel基因的CsrA依赖性抑制。 cel mRNA的稳态水平和半衰期不受CsrA的影响,这表明调节是在翻译水平上介导的。结合并拮抗CsrA的CsrB和CsrC sRNAs的水平在诱导SOS反应后急剧降低,而CsrA蛋白本身不受影响。因此,CsrA是一种下调裂解蛋白表达的反式调节剂,可在环境压力条件下赋予大肠埃希氏菌以生存优势。

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