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细胞周期对转录的依赖性主导基因表达中的噪声。

Cell-cycle dependence of transcription dominates noise in gene expression.

机构信息

Department of Chemical Engineering, Massachusetts Institute of Technology, Cambridge, Massachusetts, United States of America.

出版信息

PLoS Comput Biol. 2013;9(7):e1003161. doi: 10.1371/journal.pcbi.1003161. Epub 2013 Jul 25.

Abstract

The large variability in mRNA and protein levels found from both static and dynamic measurements in single cells has been largely attributed to random periods of transcription, often occurring in bursts. The cell cycle has a pronounced global role in affecting transcriptional and translational output, but how this influences transcriptional statistics from noisy promoters is unknown and generally ignored by current stochastic models. Here we show that variable transcription from the synthetic tetO promoter in S. cerevisiae is dominated by its dependence on the cell cycle. Real-time measurements of fluorescent protein at high expression levels indicate tetO promoters increase transcription rate ∼2-fold in S/G2/M similar to constitutive genes. At low expression levels, where tetO promoters are thought to generate infrequent bursts of transcription, we observe random pulses of expression restricted to S/G2/M, which are correlated between homologous promoters present in the same cell. The analysis of static, single-cell mRNA measurements at different points along the cell cycle corroborates these findings. Our results demonstrate that highly variable mRNA distributions in yeast are not solely the result of randomly switching between periods of active and inactive gene expression, but instead largely driven by differences in transcriptional activity between G1 and S/G2/M.

摘要

在单细胞中进行的静态和动态测量中发现的 mRNA 和蛋白质水平的巨大可变性在很大程度上归因于转录的随机时期,这些时期通常以爆发的形式出现。细胞周期对转录和翻译产物有显著的全局影响,但它如何影响来自嘈杂启动子的转录统计数据尚不清楚,并且通常被当前的随机模型所忽略。在这里,我们表明,来自合成 tetO 启动子的可变转录主要取决于细胞周期。在高表达水平下对荧光蛋白的实时测量表明,tetO 启动子在 S/G2/M 中增加转录速率约 2 倍,类似于组成型基因。在低表达水平下,tetO 启动子被认为产生转录的低频爆发,我们观察到表达的随机脉冲仅限于 S/G2/M,在同一细胞中存在的同源启动子之间存在相关性。在细胞周期的不同时间点对静态、单细胞 mRNA 测量的分析证实了这些发现。我们的结果表明,酵母中高度可变的 mRNA 分布不仅是主动和非活跃基因表达之间随机切换的结果,而是主要由 G1 和 S/G2/M 之间转录活性的差异驱动。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6a5c/3723585/cf68bc691e51/pcbi.1003161.g001.jpg

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