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Dynamic profiling of mRNA turnover reveals gene-specific and system-wide regulation of mRNA decay

机译:mRNA周转量的动态分析揭示了mRNA衰减的基因特异性和系统范围的调节

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摘要

RNA levels are determined by the rates of both transcription and decay, and a mechanistic understanding of the complex networks regulating gene expression requires methods that allow dynamic measurements of transcription and decay in living cells with minimal perturbation. Here, we describe a metabolic pulse-chase labeling protocol using 4-thiouracil combined with large-scale RNA sequencing to determine decay rates of all mRNAs in Saccharomyces cerevisiae. Profiling in various growth and stress conditions reveals that mRNA turnover is highly regulated both for specific groups of transcripts and at the system-wide level. For example, acute glucose starvation induces global mRNA stabilization but increases the degradation of all 132 detected ribosomal protein mRNAs. This effect is transient and can be mimicked by inhibiting the target-of-rapamycin kinase. Half-lives of mRNAs critical for galactose (GAL) metabolism are also highly sensitive to changes in carbon source. The fast reduction of GAL transcripts in glucose requires their dramatically enhanced turnover, highlighting the importance of mRNA decay in the control of gene expression. The approach described here provides a general platform for the global analysis of mRNA turnover and transcription and can be applied to dissect gene expression programs in a wide range of organisms and conditions.
机译:RNA的水平由转录和衰变的速率决定,对调节基因表达的复杂网络的机械理解要求采用允许动态测量活细胞转录和衰变的方法,且干扰最小。在这里,我们描述了使用4-巯基尿嘧啶与大规模RNA测序相结合来确定酿酒酵母中所有mRNA的衰减率的代谢脉冲追踪标签协议。在各种生长和胁迫条件下进行的分析表明,对于特定的转录本组以及在整个系统范围内,mRNA转换都受到高度调节。例如,急性葡萄糖饥饿诱导整体mRNA稳定,但增加了所有132种检测到的核糖体蛋白mRNA的降解。这种作用是短暂的,可以通过抑制雷帕霉素靶蛋白来模仿。对半乳糖(GAL)代谢至关重要的mRNA的半衰期也对碳源的变化高度敏感。葡萄糖中GAL转录物的快速减少需要其转录显着增强,从而突显了mRNA衰减在控制基因表达中的重要性。此处描述的方法提供了一个全面的平台,可对mRNA的营业额和转录进行全局分析,并可用于剖析各种生物和条件下的基因表达程序。

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