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时间解析增强子簇揭示了单个元件的不同时间和功能贡献。

Temporal dissection of an enhancer cluster reveals distinct temporal and functional contributions of individual elements.

机构信息

Max Perutz Laboratories Vienna, University of Vienna, Vienna Biocenter, Dr Bohr Gasse 9, 1030 Vienna, Austria.

CeMM Research Center for Molecular Medicine of the Austrian Academy of Sciences, Vienna, Austria.

出版信息

Mol Cell. 2021 Mar 4;81(5):969-982.e13. doi: 10.1016/j.molcel.2020.12.047. Epub 2021 Jan 21.

Abstract

Many genes are regulated by multiple enhancers that often simultaneously activate their target gene. However, how individual enhancers collaborate to activate transcription is not well understood. Here, we dissect the functions and interdependencies of five enhancer elements that together activate Fgf5 expression during exit from naive murine pluripotency. Four intergenic elements form a super-enhancer, and most of the elements contribute to Fgf5 induction at distinct time points. A fifth, poised enhancer located in the first intron contributes to Fgf5 expression at every time point by amplifying overall Fgf5 expression levels. Despite low individual enhancer activity, together these elements strongly induce Fgf5 expression in a super-additive fashion that involves strong accumulation of RNA polymerase II at the intronic enhancer. Finally, we observe a strong anti-correlation between RNA polymerase II levels at enhancers and their distance to the closest promoter, and we identify candidate elements with properties similar to the intronic enhancer.

摘要

许多基因受到多个增强子的调控,这些增强子通常会同时激活其靶基因。然而,单个增强子如何协同激活转录尚不清楚。在这里,我们剖析了五个增强子元件的功能和相互依赖性,这些元件在退出原始小鼠多能性时共同激活 Fgf5 的表达。四个基因间元件形成一个超级增强子,并且大多数元件在不同的时间点有助于 Fgf5 的诱导。第五个位于第一内含子中的启动子元件通过放大整体 Fgf5 表达水平,在每个时间点都有助于 Fgf5 的表达。尽管单个增强子的活性较低,但这些元件共同以超加性的方式强烈诱导 Fgf5 的表达,这涉及到 RNA 聚合酶 II 在内含子增强子处的强烈积累。最后,我们观察到增强子处的 RNA 聚合酶 II 水平与它们与最近的启动子的距离之间存在很强的反相关关系,并且我们鉴定出具有与内含子增强子相似特性的候选元件。

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