首页> 外文OA文献 >Roles of the three transcriptional attenuators of the Bacillus subtilis pyrimidine biosynthetic operon in the regulation of its expression.
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Roles of the three transcriptional attenuators of the Bacillus subtilis pyrimidine biosynthetic operon in the regulation of its expression.

机译:枯草芽孢杆菌嘧啶生物合成操纵子的三种转录衰减子在其表达调控中的作用。

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摘要

Expression of the Bacillus subtilis pyr operon is regulated by exogenous pyrimidines and the protein product of the first gene of the operon, PyrR. It has been proposed that PyrR mediates transcriptional attenuation at three untranslated segments of the operon (R.J. Turner, Y. Lu, and R.L. Switzer, J. Bacteriol., 176:3708-3722, 1994). In this study, transcriptional fusions of the pyr promoter followed by the pyr attenuation sequences, either individually or in tandem to a lacZ reporter gene, were used to examine the physiological functions of all three attenuators through their ability to affect beta-galactosidase expression. These fusions were studied as chromosomal integrants in various B. subtilis strains to examine the entire range of control by pyrimidines, PyrR dependence, amd developmental control of pyr gene expression. The nutritional regulation of each attenuator separately was roughly equivalent to that of the other two and was totally dependent upon PyrR, and that of tandem attenuators was cumulative. The regulation of a fusion of the spac promoter followed by the pyrP:pyrB intercistronic region to lacZ produced results similar to those obtained with the corresponding fusion containing the pyr promoter, demonstrating that attenuator-dependent regulation is independent of the promoter. Extreme pyrimidine starvation gave rise to two- to threefold-higher levels of expression of a pyr-lacZ fusion that lacked attenuators, independent of PyrR, than were obtained with cells that were not starved. Increased expression of a similar spac-lacZ fusion during pyrimidine starvation was also observed, however, indicating that attenuator-independent regulation is not a specific property of the pyr operon. Conversion of the initiator AUG codon in a small open reading frame in the pyrP:pyrB intercistronic region to UAG reduced expression by about half but did not alter regulation by pyrimidines, which excludes the possibility of a coupled transcription-translation attenuation mechanism. Developmental regulation of pyr expression during early stationary phase was found to be dependent upon the attenuators and PyrR, and the participation of SpoOA was excluded.
机译:枯草芽孢杆菌pyr operon的表达受外源嘧啶和操纵子第一个基因PyrR的蛋白质产物调节。已经提出PyrR在操纵子的三个未翻译的片段上介导转录减弱(R.J.Turner,Y.Lu,和R.L.Switzer,J.Bacteriol。,176:3708-3722,1994)。在这项研究中,通过使用pyr启动子的转录融合以及随后的pyr减毒序列,分别或与lacZ报告基因串联,通过影响β-半乳糖苷酶表达的能力来检查所有这三种减毒剂的生理功能。研究了这些融合物作为各种枯草芽孢杆菌菌株中的染色体整合体,以检查嘧啶的整个控制范围,PyrR依赖性,pyr基因表达的发育控制。每个衰减器的营养调节分别与其他两个衰减器大致相同,并且完全取决于PyrR,而串联衰减器的营养调节是累积的。调节spac启动子的融合物,然后使pyrP:pyrB顺反子区域与lacZ融合,产生的结果与相应的含有pyr启动子的融合物所获得的结果相似,这表明依赖于衰减子的调节与启动子无关。与没有饥饿的细胞相比,极端的嘧啶饥饿导致pyr-lacZ融合蛋白的表达水平提高了2-3倍,而pyr-lacZ融合蛋白缺乏与PyrR无关的衰减子。然而,在嘧啶饥饿期间,也观察到了类似的spac-lacZ融合蛋白的表达增加,这表明与衰减子无关的调控不是吡咯操纵子的特定特性。启动子AUG密码子在pyrP:pyrB顺反子区域的小的开放阅读框中转化为UAG,表达降低了约一半,但并未改变嘧啶的调控,这排除了偶联转录-翻译减弱机制的可能性。发现在静止早期早期pyr表达的发育调节取决于衰减子和PyrR,SpoOA的参与被排除在外。

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