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σ54增强子旁路突变体的分离与特性

Isolation and properties of enhancer-bypass mutants of sigma 54.

作者信息

Syed A, Gralla J D

机构信息

Department of Chemistry and Biochemistry, University of California, Los Angeles 90095-1569, USA.

出版信息

Mol Microbiol. 1997 Mar;23(5):987-95. doi: 10.1046/j.1365-2958.1997.2851651.x.

Abstract

The N-terminal activation domain of Escherichia coli sigma 54 was randomly mutated to provide a library of changes that might allow the required enhancer function to be bypassed. Five clones harbouring mutant sigma factors were obtained that exhibited this property in that they enhanced growth under nitrogen-limiting conditions in cells lacking NtrC. DNA sequence analysis located all mutations to four leucines in a small region between amino acids 25 and 31. No mutant sigma factors retained the hydrophobic character of the leucine residues. Mutant sigma factors were shown to transcribe in vitro without the need for enhancer binding activator or ATP hydrolysis, confirming the in vivo phenotype. These and other data suggest that a very small set of leucines is critical for keeping polymerase function in check, allowing high responsiveness to physiological induction via enhancer proteins such as NtrC.

摘要

大肠杆菌σ54的N端激活结构域被随机诱变,以提供一个可能绕过所需增强子功能的变化文库。获得了五个携带突变σ因子的克隆,它们表现出这种特性,即在缺乏NtrC的细胞中,在氮限制条件下能促进生长。DNA序列分析将所有突变定位到氨基酸25至31之间一个小区域内的四个亮氨酸上。没有突变σ因子保留亮氨酸残基的疏水特性。突变σ因子在体外转录时无需增强子结合激活剂或ATP水解,这证实了体内表型。这些数据和其他数据表明,一小部分亮氨酸对于控制聚合酶功能至关重要,使得能够通过诸如NtrC等增强子蛋白对生理诱导产生高反应性。

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