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Comparison of promoter-specific events during transcription initiation in mycobacteria

机译:分枝杆菌转录起始期间的启动子特异性事件的比较

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DNA–protein interactions that occur during transcription initiation play an important role in regulating gene expression. To initiate transcription, RNA polymerase (RNAP) binds to promoters in a sequence-specific fashion. This is followed by a series of steps governed by the equilibrium binding and kinetic rate constants, which in turn determine the overall efficiency of the transcription process. We present here the first detailed kinetic analysis of promoter–RNAP interactions during transcription initiation in the σA-dependent promoters PrrnAPCL1, PrrnBand Pgyrof Mycobacterium smegmatis. The promoters show comparable equilibrium binding affinity but differ significantly in open complex formation, kinetics of isomerization and promoter clearance. Furthermore, the two rrn promoters exhibit varied kinetic properties during transcription initiation and appear to be subjected to different modes of regulation. In addition to distinct kinetic patterns, each one of the housekeeping promoters studied has its own rate-limiting step in the initiation pathway, indicating the differences in their regulation.
机译:转录起始期间发生的DNA-蛋白质相互作用在调节基因表达中起重要作用。引发转录,RNA聚合酶(RNAP)以序列特异性方式与启动子结合。接下来是由平衡结合和动力速率常数治理的一系列步骤,这反过来决定了转录过程的整体效率。我们在这里介绍了在ΣA依赖于促进剂PRRNAPCL1中转录起始期间启动子RNAP相互作用的第一个详细的动力学分析PRRNAPCL1,PRRNBAND PGYROF分枝杆菌浓缩术。该启动子表现出可比的平衡结合亲和力,但在开放复杂的形成中显着差异,异构化和启动子间隙的动力学。此外,两个RRN启动子在转录开始期间表现出变化的动力学性质,似乎受到不同的调节模式。除了不同的动力学模式之外,所研究的每一个内政局促进剂在起始途径中有自己的速率限制步骤,表明其调节的差异。

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