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一项遗传编码交联筛选发现 SERBP1 是 PKCε 的底物,影响翻译和细胞分裂。

A genetically-encoded crosslinker screen identifies SERBP1 as a PKCε substrate influencing translation and cell division.

机构信息

Protein Phosphorylation Laboratory, The Francis Crick Institute, London, UK.

RNA Network Laboratory, The Francis Crick Institute, London, UK.

出版信息

Nat Commun. 2021 Nov 26;12(1):6934. doi: 10.1038/s41467-021-27189-5.

Abstract

The PKCε-regulated genome protective pathway provides transformed cells a failsafe to successfully complete mitosis. Despite the necessary role for Aurora B in this programme, it is unclear whether its requirement is sufficient or if other PKCε cell cycle targets are involved. To address this, we developed a trapping strategy using UV-photocrosslinkable amino acids encoded in the PKCε kinase domain. The validation of the mRNA binding protein SERBP1 as a PKCε substrate revealed a series of mitotic events controlled by the catalytic form of PKCε. PKCε represses protein translation, altering SERBP1 binding to the 40 S ribosomal subunit and promoting the assembly of ribonucleoprotein granules containing SERBP1, termed M-bodies. Independent of Aurora B, SERBP1 is shown to be necessary for chromosome segregation and successful cell division, correlating with M-body formation. This requirement for SERBP1 demonstrates that Aurora B acts in concert with translational regulation in the PKCε-controlled pathway exerting genome protection.

摘要

PKCε 调控的基因组保护途径为转化细胞提供了成功完成有丝分裂的安全保障。尽管 Aurora B 在这个程序中起着必要的作用,但尚不清楚其需求是否足够,或者是否涉及其他 PKCε 细胞周期靶标。为了解决这个问题,我们开发了一种使用 PKCε 激酶结构域中编码的可光交联氨基酸的捕获策略。PKCε 底物 mRNA 结合蛋白 SERBP1 的验证揭示了一系列由 PKCε 催化形式控制的有丝分裂事件。PKCε 抑制蛋白质翻译,改变 SERBP1 与 40S 核糖体亚基的结合,并促进包含 SERBP1 的核糖核蛋白颗粒的组装,称为 M 体。SERBP1 的分离与 Aurora B 无关,对于染色体分离和成功的细胞分裂是必需的,与 M 体的形成相关。SERBP1 的这种需求表明,Aurora B 与 PKCε 控制的途径中的翻译调节协同作用,发挥基因组保护作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/84a8/8626422/9df0c24271ba/41467_2021_27189_Fig1_HTML.jpg

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