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大肠杆菌中依赖RelA的RNA聚合酶活性

relA-dependent RNA polymerase activity in Escherichia coli.

作者信息

Ryals J, Bremer H

出版信息

J Bacteriol. 1982 Apr;150(1):168-79. doi: 10.1128/jb.150.1.168-179.1982.

Abstract

Parameters relating to RNA synthesis were measured after a temperature shift from 30 to 42 degrees C, in a relA+ and relA- isogenic pair of Escherichia coli strains containing a temperature-sensitive valyl tRNA synthetase. The following results were obtained: (i) the rRNA chain growth rate increased 2-fold in both strains; (ii) newly synthesized rRNA became unstable in both strains; (iii) the stable RNA gene activity (rRNA and tRNA, measured as stable RNA synthesis rate relative to the total instantaneous rate of RNA synthesis) decreased 1.7-fold in the relA+ strain and increased 1.9-fold in the relA mutant; and (iv) the RNA polymerase activity (measured by the percentage of total RNA polymerase enzyme active in transcription an any instant) decreased from 20 to 3.6% in the relA+ strain and remained unchanged (or increased at most to 22%) in the relA mutant. It is suggested that both rRNA gene activity and the RNA polymerase activity depend on the intracellular concentration of guanosine tetraphosphate, whereas the altered chain elongation rate and stability of rRNA are temperature or amino acid starvation effects, respectively, without involvement of relA function.

摘要

在含有温度敏感型缬氨酰 - tRNA合成酶的大肠杆菌relA +和relA - 同基因菌株对中,将温度从30℃转移至42℃后,测量了与RNA合成相关的参数。获得了以下结果:(i) 两种菌株中rRNA链生长速率均增加了2倍;(ii) 两种菌株中新合成的rRNA均变得不稳定;(iii) 稳定RNA基因活性(rRNA和tRNA,以相对于RNA合成总瞬时速率的稳定RNA合成速率衡量)在relA +菌株中降低了1.7倍,而在relA突变体中增加了1.9倍;以及(iv) RNA聚合酶活性(通过在任何时刻转录中活性的总RNA聚合酶酶的百分比衡量)在relA +菌株中从20%降至3.6%,而在relA突变体中保持不变(或最多增加至22%)。有人提出,rRNA基因活性和RNA聚合酶活性均取决于鸟苷四磷酸的细胞内浓度,而rRNA链伸长速率和稳定性的改变分别是温度或氨基酸饥饿效应,与relA功能无关。

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