首页> 美国卫生研究院文献>Journal of Bacteriology >CsrA Regulates Translation of the Escherichia coli Carbon Starvation Gene cstA by Blocking Ribosome Access to the cstA Transcript
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CsrA Regulates Translation of the Escherichia coli Carbon Starvation Gene cstA by Blocking Ribosome Access to the cstA Transcript

机译:CsrA通过阻止核糖体获取cstA转录本来调节大肠杆菌碳饥饿基因cstA的翻译。

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摘要

CsrA is a global regulator that binds to two sites in the glgCAP leader transcript, thereby blocking ribosome access to the glgC Shine-Dalgarno sequence. The upstream CsrA binding site (GCACACGGAU) was used to search the Escherichia coli genomic sequence for other genes that might be regulated by CsrA. cstA contained an exact match that overlapped its Shine-Dalgarno sequence. cstA was previously shown to be induced by carbon starvation and to encode a peptide transporter. Expression of a cstA′-′lacZ translational fusion in wild-type and csrA mutant strains was examined. Expression levels in the csrA mutant were approximately twofold higher when cells were grown in Luria broth (LB) and 5- to 10-fold higher when LB was supplemented with glucose. It was previously shown that cstA is regulated by the cyclic AMP (cAMP)-cAMP receptor protein complex and transcribed by Εσ70. We investigated the influence of σS on cstA expression and found that a σS deficiency resulted in a threefold increase in cstA expression in wild-type and csrA mutant strains; however, CsrA-dependent regulation was retained. The mechanism of CsrA-mediated cstA regulation was also examined in vitro. Cross-linking studies demonstrated that CsrA is a homodimer. Gel mobility shift results showed that CsrA binds specifically to cstA RNA, while coupled-transcription-translation and toeprint studies demonstrated that CsrA regulates CstA synthesis by inhibiting ribosome binding to cstA transcripts. RNA footprint and boundary analyses revealed three or four CsrA binding sites, one of which overlaps the cstA Shine-Dalgarno sequence, as predicted. These results establish that CsrA regulates translation of cstA by sterically interfering with ribosome binding.
机译:CsrA是一种全局调节剂,可与glgCAP前导转录物中的两个位点结合,从而阻止核糖体进入glgC Shine-Dalgarno序列。上游CsrA结合位点(GCACACGGAU)用于搜索大肠杆菌基因组序列,寻找可能受CsrA调控的其他基因。 cstA包含与Shine-Dalgarno序列重叠的完全匹配项。先前显示cstA被碳饥饿诱导并编码肽转运蛋白。检查了cstA'-'lacZ翻译融合在野生型和csrA突变株中的表达。当细胞在Luria肉汤(LB)中生长时,csrA突变体中的表达水平高约两倍,而在LB中添加葡萄糖时,其表达水平高5至10倍。先前已证明cstA受环状AMP(cAMP)-cAMP受体蛋白复合物调控,并被Εσ 70 转录。我们研究了σ S 对cstA表达的影响,发现σ S 缺乏导致野生型和csrA突变菌株中cstA表达增加了三倍。但是,保留了CsrA依赖性调节。体外还检查了CsrA介导的cstA调节的机制。交联研究表明CsrA是同源二聚体。凝胶迁移率变化结果表明CsrA与cstA RNA特异性结合,而偶联转录翻译和脚印研究表明CsrA通过抑制核糖体与cstA转录物的结合来调节CstA的合成。 RNA足迹和边界分析揭示了三个或四个CsrA结合位点,其中一个与 cstA Shine-Dalgarno序列重叠,如预期的那样。这些结果表明,CsrA通过空间干扰核糖体结合来调节 cstA 的翻译。

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