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Analysis of the binding site of the LysR-type transcriptional activator TcbR on the tcbR and tcbC divergent promoter sequences.

机译:分析tcbR和tcbC趋异启动子序列上LysR型转录激活因子TcbR的结合位点。

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摘要

The TcbR transcriptional activator protein, which is encoded by the tcbR gene of Pseudomonas sp. strain P51 (J. R. van der Meer, A. C. J. Frijters, J. H. J. Leveau, R. I. L. Eggen, A. J. B. Zehnder, and W. M. de Vos, J. Bacteriol. 173:3700-3708, 1991), was purified from overproducing Escherichia coli cells by using a two-step chromatographic procedure. Subsequent use of TcbR in gel mobility shift assays with progressively shortened portions of a DNA fragment containing the divergent promoter sequences of the tcbR gene and the tcbCDEF operon showed that the direct binding site of TcbR is located between positions -85 to -40 relative to the tcbCDEF transcriptional start site, containing a LysR-type recognition sequence motif (T-N11-A). DNase I footprinting experiments revealed that TcbR protected an area on both strands of the intercistronic region which was actually larger than this binding site (from positions -74 to -24). This stretch of protected DNA was interrupted by a region (positions -52 to -37) which became strongly hypersensitive to DNase I digestion upon addition of TcbR, suggesting that TcbR induces a bend in the DNA at this site.
机译:TcbR转录激活蛋白,由假单胞菌sp。tcbR基因编码。 P51菌株(JR van der Meer,ACJ Frijters,JHJ Leveau,RIL Eggen,AJB Zehnder和WM de Vos,J.Bacteriol.173:3700-3708,1991)通过使用两分步色谱过程。随后在含有TcbR基因和tcbCDEF操纵子的不同启动子序列的DNA片段的DNA片段的逐渐缩短部分的凝胶迁移分析中使用TcbR,表明TcbR的直接结合位点相对于TcbR位于-85至-40之间tcbCDEF转录起始位点,包含LysR型识别序列基序(T-N11-A)。 DNase I足迹实验表明,TcbR保护了顺反子区域的两条链上实际上比该结合位点大的区域(从-74到-24)。受保护的DNA片段被一个区域(位置-52至-37)打断,该区域在添加TcbR后对DNase I消化变得高度超敏,表明TcbR在该位点诱导DNA弯曲。

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