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大肠杆菌K-12两个甲硫氨酸起始转运RNA基因的差异转录调控

Differential transcriptional control of the two tRNA(fMet) genes of Escherichia coli K-12.

作者信息

Nagase T, Ishii S, Imamoto F

机构信息

Laboratory of Molecular Genetics, Tsukuba Life Science Center, RIKEN, Ibaraki, Japan.

出版信息

Gene. 1988 Jul 15;67(1):49-57. doi: 10.1016/0378-1119(88)90007-8.

Abstract

The metZ gene of Escherichia coli, which encodes the tRNA(f1Met), was cloned. Using the nucleotide sequence, in vitro transcription, and S1 nuclease mapping analyses, we identified the promoter region, transcriptional start point, the two tandem tRNA(f1Met) structural genes separated by an intergenic space of 33 bp, and the two Rho-independent transcriptional termination sites, in that order. We compared the promoter region of the metZ gene with that of the metY gene, which encodes the tRNA(f2Met) and is located in the promoter-proximal portion of the nusA operon. A G + C-rich sequence (5'-GCGCATCCAC-3'), similar to the corresponding sequence of the rrn promoters that are under stringent control, was found between the Pribnow box and the transcriptional start point of the metZ promoter, but not in the metY promoter region. We therefore examined the effect of guanosine 3'-diphosphate, 5'-diphosphate (ppGpp), the chemical mediator of stringent control, and found that ppGpp inhibited the transcription of the metZ gene, but not that of the metY gene. These data suggested that the promoters for metZ and metY have different physiological functions and are regulated by different mechanisms.

摘要

编码tRNA(f1Met)的大肠杆菌metZ基因被克隆。通过核苷酸序列分析、体外转录和S1核酸酶图谱分析,我们依次确定了启动子区域、转录起始点、由33 bp基因间隔区隔开的两个串联tRNA(f1Met)结构基因以及两个不依赖Rho的转录终止位点。我们将metZ基因的启动子区域与metY基因的启动子区域进行了比较,metY基因编码tRNA(f2Met),位于nusA操纵子的启动子近端部分。在metZ启动子的Pribnow框和转录起始点之间发现了一个富含G + C的序列(5'-GCGCATCCAC-3'),类似于受严格控制的rrn启动子的相应序列,但在metY启动子区域未发现。因此,我们研究了严格控制的化学介质鸟苷3'-二磷酸、5'-二磷酸(ppGpp)的作用,发现ppGpp抑制metZ基因的转录,但不抑制metY基因的转录。这些数据表明,metZ和metY的启动子具有不同的生理功能,且受不同机制调控。

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