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Glycogen synthase kinase 3 promotes p53 mRNA translation via phosphorylation of RNPC1

机译:糖原合酶激酶3通过RNPC1的磷酸化促进p53 mRNA翻译

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摘要

The RNPC1 RNA-binding protein, also called Rbm38, is a target of p53 and a repressor of p53 mRNA translation. Thus, the p53-RNPC1 loop is critical for modulating p53 tumor suppression, but it is not clear how the loop is regulated. Here, we showed that RNPC1 is phosphorylated at Ser195 by glycogen synthase kinase 3 (GSK3). We also showed that GSK3 promotes p53 mRNA translation through phosphorylation of RNPC1. Interestingly, we found that the phosphor-mimetic mutant S195D and the deletion mutant Δ189-204, which lacks the GSK3 phosphorylation site, are unable to repress p53 mRNA translation due to loss of interaction with eukaryotic translation factor eIF4E on p53 mRNA. Additionally, we found that phosphorylated RNPC1, RNPC1-S195D, and RNPC1(Δ189-204) promote p53 mRNA translation through interaction with eukaryotic translation factor eIF4G, which then facilitates the assembly of the eIF4F complex on p53 mRNA. Furthermore, we showed that upon inhibition of the phosphatidylinositol 3-kinase (PI3K)-Akt pathway, GSK3 is activated, leading to increased RNPC1 phosphorylation and increased p53 expression in a RNPC1-dependent manner. Together, we postulate that the p53-RNPC1 loop can be explored to increase or decrease p53 activity for cancer therapy.
机译:RNPC1 RNA结合蛋白也称为Rbm38,是p53的靶标和p53 mRNA翻译的阻遏物。因此,p53-RNPC1回路对于调节p53肿瘤抑制至关重要,但尚不清楚该回路如何调节。在这里,我们显示RNPC1在糖原合酶激酶3(GSK3)的Ser195处被磷酸化。我们还表明,GSK3通过RNPC1的磷酸化促进p53 mRNA的翻译。有趣的是,我们发现缺少GSK3磷酸化位点的模拟荧光的突变体S195D和缺失突变体Δ189-204,由于与p53 mRNA上的真核翻译因子eIF4E的相互作用丧失而无法抑制p53 mRNA的翻译。此外,我们发现磷酸化的RNPC1,RNPC1-S195D和RNPC1(Δ189-204)通过与真核翻译因子eIF4G相互作用促进了p53 mRNA的翻译,从而促进了eIF4F复合物在p53 mRNA上的组装。此外,我们表明抑制磷脂酰肌醇3激酶(PI3K)-Akt通路后,GSK3被激活,导致RNPC1磷酸化增加,并以RNPC1依赖性方式增加p53表达。在一起,我们假设可以探索p53-RNPC1环以增加或减少p53活性用于癌症治疗。

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