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首页> 外文期刊>Genes and Development: a Journal Devoted to the Molecular Analysis of Gene Expression in Eukaryotes, Prokaryotes, and Viruses >Reduced capacity of alternative sigmas to melt promoters ensures stringent promoter recognition.
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Reduced capacity of alternative sigmas to melt promoters ensures stringent promoter recognition.

机译:替代sigma融化启动子的能力降低,从而确保了严格的启动子识别。

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摘要

In bacteria, multiple sigmas direct RNA polymerase to distinct sets of promoters. Housekeeping sigmas direct transcription from thousands of promoters, whereas most alternative sigmas are more selective, recognizing more highly conserved promoter motifs. For sigma(32) and sigma(28), two Escherichia coli Group 3 sigmas, altering a few residues in Region 2.3, the portion of sigma implicated in promoter melting, to those universally conserved in housekeeping sigmas relaxed their stringent promoter requirements and significantly enhanced melting of suboptimal promoters. All Group 3 sigmas and the more divergent Group 4 sigmas have nonconserved amino acids at these positions and rarely transcribe >100 promoters. We suggest that the balance of "melting" and "recognition" functions of sigmas is critical to setting the stringency of promoter recognition. Divergent sigmas may generally use a nonoptimal Region 2.3 to increase promoter stringency, enabling them to mount a focused response to altered conditions.
机译:在细菌中,多个sigma将RNA聚合酶引导至不同的启动子集。管家西格玛直接从数千个启动子转录,而大多数替代西格玛则更具选择性,可以识别更多高度保守的启动子基序。对于sigma(32)和sigma(28),两个大肠埃希菌3组sigma,改变了2.3区的一些残基,即部分与启动子融化有关的sigma部分,到普遍在管家sigma中保守的那些部分放宽了对严格启动子的要求,并显着提高了次佳启动子融化。所有第3组sigma和差异更大的第4组sigma在这些位置均具有非保守氨基酸,很少转录> 100个启动子。我们建议,sigma的“融化”和“识别”功能之间的平衡对于设定启动子识别的严格性至关重要。发散的sigma通常可能会使用非最佳区域2.3来增加启动子严格性,从而使它们能够针对变化的条件进行集中响应。

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