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大肠杆菌K-12色氨酸酶启动子处的转录起始

Transcription initiation at the tryptophanase promoter of Escherichia coli K-12.

作者信息

Deeley M C, Yanofsky C

出版信息

J Bacteriol. 1982 Aug;151(2):942-51. doi: 10.1128/jb.151.2.942-951.1982.

Abstract

Restriction fragments containing the region preceding the tryptophanase structural gene, tnaA, were used as templates for in vitro transcription experiments. A transcription initiation site was detected that was dependent on the catabolite gene activator protein (CAP) plus cyclic AMP (cAMP). The mRNA produced in vitro was fingerprinted, and the nucleotide at which transcription was initiated was localized to the vicinity of two guanine residues 316 and 318 base pairs upstream of tnaA. A region exhibiting extensive difold symmetry and homology to the CAP binding site adjacent to the lactose operon promoter exists approximately 60 base pairs preceding the site of transcription initiation. Two HinfI restriction sites are located in this region. Restriction enzyme cleavage at these sites was prevented when DNA containing the promoter region was preincubated with CAP and cAMP. RNA polymerase was incapable of protecting these sites against this cleavage. CAP and cAMP addition did not protect against cleavage at a DdeI restriction site located in the -20 region of the promoter. RNA polymerase did protect against DdeI cleavage but only in the presence of CAP and cAMP. Thus, transcription initiation at the tryptophanase promoter involves cAMP-dependent, CAP-facilitated binding of RNA polymerase to the DNA.

摘要

含有色氨酸酶结构基因tnaA之前区域的限制性片段被用作体外转录实验的模板。检测到一个转录起始位点,它依赖于代谢物基因激活蛋白(CAP)加环腺苷酸(cAMP)。对体外产生的mRNA进行指纹分析,转录起始的核苷酸被定位到tnaA上游316和318个碱基对的两个鸟嘌呤残基附近。在转录起始位点之前约60个碱基对处存在一个与乳糖操纵子启动子相邻的CAP结合位点具有广泛双折叠对称性和同源性的区域。该区域有两个HinfI限制性位点。当含有启动子区域的DNA与CAP和cAMP预孵育时,这些位点的限制性酶切被阻止。RNA聚合酶无法保护这些位点免受这种切割。添加CAP和cAMP不能防止位于启动子-20区域的DdeI限制性位点的切割。RNA聚合酶确实能防止DdeI切割,但仅在存在CAP和cAMP的情况下。因此,色氨酸酶启动子处的转录起始涉及cAMP依赖性、CAP促进的RNA聚合酶与DNA的结合。

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