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Influence of the GCGC discriminator motif introduced into the ribosomal RNA P2- and tac promoter on growth-rate control and stringent sensitivity.

机译:引入核糖体RNA P2-和tac启动子的GCGC鉴别子基序对生长速率控制和严格敏感性的影响。

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摘要

The synthesis of stable RNA in bacteria is known to be regulated by a stringent control mechanism. Characteristic of stringent-regulated promoters, all ribosomal RNA promoters P1, but not P2, contain a GC-rich discriminator sequence assumed to be important for such a control. Using site-directed mutagenesis we have altered both the rrnB P2 and the synthetic tac promoter to the consensus GCGC discriminator motif. The modified promoters were placed upstream of the structural gene encoding the chloramphenicol acetyltransferase. The response of the modified promoters to amino acid starvation, changes in the growth rate or differences in the basal level of guanosine tetraphosphate (ppGpp) were determined in vivo. The results clearly show, that the discriminator motif is sufficient to convert the ribosomal RNA promoter P2 to a stringent, as well as growth-rate regulated, promoter. By contrast, the same discriminator sequence linked to the synthetic tac promoter does not convert this promoter to either stringency or growth-rate regulation. Finally, the results presented in this study reinforce the view that stringent and growth-rate regulation utilize the same mechanism, with ppGpp being the common mediator.
机译:已知细菌中稳定RNA的合成受到严格控制机制的调控。严格调节的启动子的特征是,所有核糖体RNA启动子P1,而不是P2,都包含富含GC的鉴别序列,该序列被认为对这种控制至关重要。使用定点诱变,我们已经将rrnB P2和合成tac启动子都改变为共有的GCGC鉴别子基序。将修饰的启动子置于编码氯霉素乙酰转移酶的结构基因的上游。在体内确定了修饰的启动子对氨基酸饥饿,生长速度的变化或鸟嘌呤四磷酸鸟苷(ppGpp)的基础水平的差异的响应。结果清楚地表明,鉴别基序足以将核糖体RNA启动子P2转化为严格的,以及受生长速率调节的启动子。相比之下,连接至合成tac启动子的相同鉴别子序列不会将该启动子转化为严格性或生长速率调节。最后,本研究提出的结果强化了这样的观点,即严格的调控和增长率调控利用相同的机制,而ppGpp是共同的媒介。

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