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Expression of the glucose transporter gene ptsG is regulated at the mRNA degradation step in response to glycolytic flux in Escherichia coli

机译:响应大肠杆菌中的糖酵解通量在mRNA降解步骤调节葡萄糖转运蛋白基因ptsG的表达。

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摘要

We report a novel post-transcriptional control of the ptsG gene encoding the major glucose transporter IICBGlc. We demonstrate that the level of IICBGlc is markedly reduced when the glycolytic pathway is blocked by a mutation in either the pgi or pfkA gene encoding phosphoglucose isomerase or phosphofructokinase, respectively. This down-regulation of ptsG is not exerted at the transcriptional level. Both northern blot and S1 analyses demonstrate that the mutation dramatically accelerates the degradation of ptsG mRNA. The degradation of ptsG mRNA occurs in wild-type cells when α-methylglucoside, a non- metabolizable analog of glucose, is present in the medium. The addition of any one of the glycolytic intermediates downstream of the block prevents the degradation of ptsG mRNA. The rapid degradation of ptsG mRNA is eliminated when RNase E is thermally inactivated. We conclude that the glycolytic pathway controls ptsG expression by modulating RNase E-mediated mRNA degradation. This is the first instance in which the glycolytic flux has been shown to affect the expression of a specific gene through mRNA stability.
机译:我们报道了编码主要葡萄糖转运蛋白IIBC Glc 的ptsG基因的新型转录后控制。我们证明,当糖酵解途径被分别编码磷酸葡萄糖异构酶或磷酸果糖激酶的pgi或pfkA基因中的突变所阻止时,IICB Glc 的水平显着降低。 ptsG的这种下调在转录水平上不起作用。 Northern印迹和S1分析均表明该突变显着加速了ptsG mRNA的降解。当培养基中存在α-甲基葡萄糖苷(一种葡萄糖的不可代谢类似物)时,ptsG mRNA的降解会发生在野生型细胞中。在该嵌段下游添加任何一种糖酵解中间体可防止ptsG mRNA降解。当RNase E热失活时,消除了ptsG mRNA的快速降解。我们得出结论,糖酵解途径通过调节RNase E介导的mRNA降解来控制ptsG表达。这是首次显示糖酵解通量通过mRNA稳定性影响特定基因的表达。

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