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首页> 外文期刊>Biophysical Journal >Probing Mechanisms of Transcription Elongation Through Cell-to-Cell Variability of RNA Polymerase
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Probing Mechanisms of Transcription Elongation Through Cell-to-Cell Variability of RNA Polymerase

机译:通过RNA聚合酶细胞对细胞变异性转录伸长率的探测机制

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The process of transcription initiation and elongation are primary points of control in the regulation of gene expression. Although biochemical studies have uncovered the mechanisms involved in controlling transcription at each step, how these mechanisms manifest in vivo at the level of individual genes is still unclear. Recent experimental advances have enabled single-cell measurements of RNA polymerase (RNAP) molecules engaged in the process of transcribing a gene of interest. In this article, we use Gillespie simulations to show that measurements of cell-to-cell variability of RNAP numbers and interpolymerase distances can reveal the prevailing mode of regulation of a given gene. Mechanisms of regulation at each step, from initiation to elongation dynamics, produce qualitatively distinct signatures, which can further be used to discern between them. Most intriguingly, depending on the initiation kinetics, stochastic elongation can either enhance or suppress cell-to-cell variability at the RNAP level. To demonstrate the value of this framework, we analyze RNAP number distribution data for ribosomal genes in Saccharomyces cerevisiae from three previously published studies and show that this approach provides crucial mechanistic insights into the transcriptional regulation of these genes.
机译:转录起始和伸长率的过程是基因表达调控中的主要控制点。虽然生化研究已经未覆盖在每个步骤中控制转录的机制,但这些机制如何在单个基因的体内表现出来尚不清楚。最近的实验进展使得在转录感兴趣基因的过程中的RNA聚合酶(RNAP)分子的单细胞测量能够。在本文中,我们使用Gillespie模拟来表明RNAP数和互聚物酶距离的细胞对细胞变异性的测量可以揭示给定基因的普遍调节模式。每个步骤的调节机制,从启动到伸长动态,产生定性不同的签名,这可以进一步用于辨别它们。根据引发动力学,大多数有趣的是,随机伸长率可以增强或抑制RNAP水平的细胞对细胞变异性。为了证明该框架的价值,我们从三个先前公布的研究中分析综合症酿酒酵母中核糖瘤基因的RNAP数分布数据,并表明这种方法为这些基因的转录调节提供了重要的机制见解。

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