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TAIL-seq:全基因组测定多聚(A)尾长度和 3'末端修饰。

TAIL-seq: genome-wide determination of poly(A) tail length and 3' end modifications.

机构信息

Center for RNA Research, Institute for Basic Science, Seoul 151-742, Korea; School of Biological Sciences, Seoul National University, Seoul 151-742, Korea.

Center for RNA Research, Institute for Basic Science, Seoul 151-742, Korea; School of Biological Sciences, Seoul National University, Seoul 151-742, Korea.

出版信息

Mol Cell. 2014 Mar 20;53(6):1044-52. doi: 10.1016/j.molcel.2014.02.007. Epub 2014 Feb 27.

Abstract

Global investigation of the 3' extremity of mRNA (3'-terminome), despite its importance in gene regulation, has not been feasible due to technical challenges associated with homopolymeric sequences and relative paucity of mRNA. We here develop a method, TAIL-seq, to sequence the very end of mRNA molecules. TAIL-seq allows us to measure poly(A) tail length at the genomic scale. Median poly(A) length is 50-100 nt in HeLa and NIH 3T3 cells. Poly(A) length correlates with mRNA half-life, but not with translational efficiency. Surprisingly, we discover widespread uridylation and guanylation at the downstream of poly(A) tail. The U tails are generally attached to short poly(A) tails (<25 nt), while the G tails are found mainly on longer poly(A) tails (>40 nt), implicating their generic roles in mRNA stability control. TAIL-seq is a potent tool to dissect dynamic control of mRNA turnover and translational control, and to discover unforeseen features of RNA cleavage and tailing.

摘要

尽管 3' 末端(3'-terminome)在基因调控中非常重要,但由于与同聚序列相关的技术挑战以及相对较少的 mRNA,对其进行全球研究一直不可行。我们在这里开发了一种方法 TAIL-seq,用于对 mRNA 分子的末端进行测序。TAIL-seq 使我们能够在基因组范围内测量 poly(A) 尾的长度。在 HeLa 和 NIH 3T3 细胞中,poly(A) 长度的中位数为 50-100 nt。poly(A) 长度与 mRNA 半衰期相关,但与翻译效率无关。令人惊讶的是,我们发现 poly(A) 尾下游存在广泛的尿嘧啶化和鸟嘌呤化。U 尾通常附着在短的 poly(A) 尾部(<25 nt),而 G 尾主要存在于较长的 poly(A) 尾部(>40 nt)上,这表明它们在 mRNA 稳定性控制中具有通用作用。TAIL-seq 是一种强大的工具,可以剖析 mRNA 周转和翻译控制的动态,以及发现 RNA 切割和加尾的意外特征。

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