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真核转录组监测的核RNA降解密码

A nuclear RNA degradation code for eukaryotic transcriptome surveillance.

作者信息

Soles Lindsey V, Liu Liang, Zou Xudong, Yoon Yoseop, Li Shuangyu, Tian Lusong, Valdez Marielle Cárdenas, Yu Angela, Yin Hong, Li Wei, Ding Fangyuan, Seelig Georg, Li Lei, Shi Yongsheng

出版信息

bioRxiv. 2024 Jul 24:2024.07.23.604837. doi: 10.1101/2024.07.23.604837.

Abstract

The RNA exosome plays critical roles in eukaryotic RNA degradation, but it remains unclear how the exosome specifically recognizes its targets. The PAXT connection is an adaptor that recruits the exosome to polyadenylated RNAs in the nucleus, especially transcripts polyadenylated at intronic poly(A) sites. Here we show that PAXT-mediated RNA degradation is induced by the combination of a 5' splice site and a poly(A) junction, but not by either sequence alone. These sequences are bound by U1 snRNP and cleavage/polyadenylation factors, which in turn cooperatively recruit PAXT. As the 5' splice site-poly(A) junction combination is typically not found on correctly processed full-length RNAs, we propose that it functions as a "nuclear RNA degradation code" (NRDC). Importantly, disease-associated single nucleotide polymorphisms that create novel 5' splice sites in 3' untranslated regions can induce aberrant mRNA degradation via the NRDC mechanism. Together our study identified the first NRDC, revealed its recognition mechanism, and characterized its role in human diseases.

摘要

RNA外切体在真核生物RNA降解中发挥关键作用,但外切体如何特异性识别其靶标仍不清楚。PAXT连接体是一种衔接子,可将外切体招募至细胞核中的多聚腺苷酸化RNA,特别是在内含子聚腺苷酸化位点进行多聚腺苷酸化的转录本。在这里,我们表明PAXT介导的RNA降解是由5'剪接位点和多聚腺苷酸化连接的组合诱导的,而不是由单独的任何一个序列诱导的。这些序列由U1 snRNP和切割/多聚腺苷酸化因子结合,这些因子进而协同招募PAXT。由于5'剪接位点-多聚腺苷酸化连接组合通常不会出现在正确加工的全长RNA上,我们提出它作为一种“核RNA降解密码”(NRDC)发挥作用。重要的是,在3'非翻译区产生新的5'剪接位点的疾病相关单核苷酸多态性可通过NRDC机制诱导异常mRNA降解。我们的研究共同确定了首个NRDC,揭示了其识别机制,并表征了其在人类疾病中的作用。

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