大肠杆菌glyA基因的MetR结合位点的表征
Characterization of the MetR binding sites for the glyA gene of Escherichia coli.
作者信息
Lorenz E, Stauffer G V
机构信息
Department of Microbiology, University of Iowa, Iowa City 52242, USA.
出版信息
J Bacteriol. 1995 Jul;177(14):4113-20. doi: 10.1128/jb.177.14.4113-4120.1995.
Abstract
Sequence analysis of the glyA control region of Escherichia coli identified two regions with homology to the consensus binding sequence for MetR, a lysR family regulatory protein. Gel shift assays and DNase I protection assays verified that both sites bind MetR. Homocysteine, a coregulator for MetR, increased MetR binding to the glyA control region. The MetR binding sites were cloned into the pBend2 vector. Although the DNA did not show any significant intrinsic bend, MetR binding resulted in a bending angle of about 33 degrees. MetR-induced bending was independent of homocysteine. To verify that the MetR binding sites play a functional role in glyA expression, site-directed mutagenesis was used to alter the two binding sites in a lambda glyA-lacZ gene fusion phage. Changing the binding sites toward the consensus MetR binding sequence caused an increase in glyA-lacZ expression. Changing either binding site away from the consensus sequence caused a decrease in expression, suggesting that both sites are required for normal glyA regulation.
摘要
对大肠杆菌glyA调控区的序列分析鉴定出两个区域,它们与赖氨酸R家族调控蛋白MetR的共有结合序列具有同源性。凝胶迁移试验和DNase I保护试验证实这两个位点均能结合MetR。同型半胱氨酸是MetR的一个共调节因子,它能增强MetR与glyA调控区的结合。将MetR结合位点克隆到pBend2载体中。虽然该DNA未显示出任何明显的固有弯曲,但MetR结合导致约33度的弯曲角度。MetR诱导的弯曲与同型半胱氨酸无关。为了验证MetR结合位点在glyA表达中发挥功能作用,利用定点诱变来改变λ glyA-lacZ基因融合噬菌体中的两个结合位点。使结合位点向MetR共有结合序列改变导致glyA-lacZ表达增加。使任一结合位点远离共有序列则导致表达降低,这表明两个位点对于正常的glyA调控都是必需的。
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