首页> 美国卫生研究院文献>Nucleic Acids Research >Staufen1 and UPF1 exert opposite actions on the replacement of the nuclear cap-binding complex by eIF4E at the 5′ end of mRNAs
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Staufen1 and UPF1 exert opposite actions on the replacement of the nuclear cap-binding complex by eIF4E at the 5′ end of mRNAs

机译:Staufen1和UPF1在mRNA的5端用eIF4E替代核帽结合复合物发挥相反的作用

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摘要

Newly synthesized mRNAs are exported from the nucleus to cytoplasm with a 5′-cap structure bound by the nuclear cap-binding complex (CBC). During or after export, the CBC should be properly replaced by cytoplasmic cap-binding protein eIF4E for efficient protein synthesis. Nonetheless, little is known about how the replacement takes place. Here, we show that double-stranded RNA-binding protein staufen1 (STAU1) promotes efficient replacement by facilitating an association between the CBC–importin α complex and importin β. Our transcriptome-wide analyses and artificial tethering experiments also reveal that the replacement occurs more efficiently when an mRNA associates with STAU1. This event is inhibited by a key nonsense-mediated mRNA decay factor, UPF1, which directly interacts with STAU1. Furthermore, we find that cellular apoptosis that is induced by ionizing radiation is accompanied by inhibition of the replacement via increased association between STAU1 and hyperphosphorylated UPF1. Altogether, our data highlight the functional importance of STAU1 and UPF1 in the course of the replacement of the CBC by eIF4E, adding a previously unappreciated layer of post-transcriptional gene regulation.
机译:新合成的mRNA从细胞核输出到具有被核帽结合复合物(CBC)结合的5'-帽结构的细胞质。出口期间或之后,应使用细胞质帽结合蛋白eIF4E适当替代CBC,以实现有效的蛋白合成。但是,关于更换的方式知之甚少。在这里,我们显示双链RNA结合蛋白staufen1(STAU1)通过促进CBC-importinα复合物和importinβ之间的缔合而促进了有效置换。我们的转录组范围内的分析和人工拴系实验也表明,当mRNA与STAU1缔合时,置换更有效。该事件被关键的无意义介导的mRNA衰变因子UPF1抑制,该因子直接与STAU1相互作用。此外,我们发现电离辐射诱导的细胞凋亡伴随着通过STAU1和超磷酸化UPF1之间增加的缔合的替代抑制。总之,我们的数据强调了STAU1和UPF1在用eIF4E替代CBC的过程中的功能重要性,从而增加了转录后基因调控的先前未曾意识到的层。

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