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DNA binding sites for the Mlc and NagC proteins: regulation of nagE encoding the N-acetylglucosamine-specific transporter in Escherichia coli

机译:Mlc的DNA结合位点 和NagC蛋白:调节nagE编码 大肠杆菌中N-乙酰氨基葡萄糖特异性转运蛋白

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摘要

The NagC and Mlc proteins are homologous transcriptional regulators that control the expression of several phosphotransferase system (PTS) genes in Escherichia coli. NagC represses nagE, encoding the N-acetylglucosamine-specific transporter, while Mlc represses three PTS operons, ptsG, manXYZ and ptsHIcrr, involved in the uptake of glucose. NagC and Mlc can bind to each others operator, at least in vitro. A binding site selection procedure was used to try to distinguish NagC and Mlc sites. The major difference was that all selected NagC binding sites had a G or a C at positions +11/–11 from the centre of symmetry. This is also the case for most native NagC sites, but not the nagE operator, which thus looks like a potential Mlc target. The nagE operator does exhibit a higher affinity for Mlc than NagC, but no regulation of nagE by physiological concentrations of Mlc was detected in vivo. Regulation of wild-type nagE by NagC is achieved because of the chelation effect due to a second high affinity NagC operator covering the nagB promoter. Replacing the A/T at +11/>–11 with C/G allows repression by NagC in the absence of the nagB operator.
机译:NagC和Mlc蛋白是同源转录调节因子,可控制大肠杆菌中几个磷酸转移酶系统(PTS)基因的表达。 NagC抑制编码N-乙酰氨基葡糖特异性转运蛋白的nagE,而Mlc抑制三个参与葡萄糖吸收的PTS操纵子ptsG,manXYZ和ptsHIcrr。 NagC和Mlc至少在体外可以彼此结合。使用结合位点选择程序来尝试区分NagC和Mlc位点。主要区别在于,所有选定的NagC结合位点在距对称中心+ 11 / –11的位置均具有G或C。对于大多数本地NagC站点也是这种情况,但不是nagE运算符,因此看起来像是潜在的Mlc目标。 nagE操纵子确实显示出比NagC对Mlc更高的亲和力,但在体内未检测到生理水平的Mlc对nagE的调节。由于第二种高亲和力的NagC操纵子覆盖了nagB启动子,因此具有螯合作用,因此可以通过NagC调节野生型nagE。用C / G替换+ 11 / > – 11处的A / T,可以在没有nagB运算符的情况下通过NagC进行抑制。

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