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两个串联的大肠杆菌核糖体RNA启动子之间的功能相互关系。

Functional interrelationship between two tandem E. coli ribosomal RNA promoters.

作者信息

Glaser G, Sarmientos P, Cashel M

出版信息

Nature. 1983 Mar 3;302(5903):74-6. doi: 10.1038/302074a0.

Abstract

The Escherichia coli chromosome carries seven cistrons encoding ribosomal RNA sequences. In all cases studied, in vitro and in vivo, it has been established that transcription is initiated from two tandem promoters. The expression of the rRNA cistrons is regulated in response to growth rate as well as to aminoacyl tRNA availability. In the present study, a plasmid (pPS1) carrying the promoter region of the rrnA cistron fused to the terminator region of rrnB has been used for in vitro transcription experiments. The presence of the terminators (T1 and T2) together with the fact that supercoiled DNA is found to be a highly efficient template, provide an ideal in vitro system in which to study the functional interrelationship between the two tandem promoters of E. coli rRNA cistrons. The results suggest that the rate of rRNA synthesis in E. coli cells growing in various conditions, as reflected by the availability of RNA polymerase, is primarily dependent on the properties of the two tandem rRNA promoters.

摘要

大肠杆菌染色体携带七个编码核糖体RNA序列的顺反子。在所有体外和体内研究的案例中,已确定转录从两个串联启动子起始。核糖体RNA顺反子的表达受生长速率以及氨酰tRNA可用性的调控。在本研究中,携带rrnA顺反子启动子区域与rrnB终止子区域融合的质粒(pPS1)已用于体外转录实验。终止子(T1和T2)的存在以及超螺旋DNA被发现是一种高效模板这一事实,提供了一个理想的体外系统,用于研究大肠杆菌核糖体RNA顺反子两个串联启动子之间的功能相互关系。结果表明,在各种条件下生长的大肠杆菌细胞中,核糖体RNA合成速率(如由RNA聚合酶的可用性所反映)主要取决于两个串联核糖体RNA启动子的特性。

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