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FAX-RIC enables robust profiling of dynamic RNP complex formation in multicellular organisms

机译:Fax-RIC使多细胞生物体中动态RNP复合物形成的强大分析

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摘要

RNA–protein interaction is central to post-transcriptional gene regulation. Identification of RNA-binding proteins relies mainly on UV-induced crosslinking (UVX) followed by the enrichment of RNA–protein conjugates and LC-MS/MS analysis. However, UVX has limited applicability in tissues of multicellular organisms due to its low penetration depth. Here, we introduce formaldehyde crosslinking (FAX) as an alternative chemical crosslinking for RNA interactome capture (RIC). Mild FAX captures RNA–protein interaction with high specificity and efficiency in cell culture. Unlike UVX-RIC, FAX-RIC robustly detects proteins that bind to structured RNAs or uracil-poor RNAs (e.g. AGO1, STAU1, UPF1, NCBP2, EIF4E, YTHDF proteins and PABP), broadening the coverage. Applied to Xenopus laevis oocytes and embryos, FAX-RIC provided comprehensive and unbiased RNA interactome, revealing dynamic remodeling of RNA–protein complexes. Notably, translation machinery changes during oocyte-to-embryo transition, for instance, from canonical eIF4E to noncanonical eIF4E3. Furthermore, using Mus musculus liver, we demonstrate that FAX-RIC is applicable to mammalian tissue samples. Taken together, we report that FAX can extend the RNA interactome profiling into multicellular organisms.
机译:RNA-蛋白质相互作用是转录后基因调控的核心。 RNA结合蛋白的鉴定主要依赖于UV诱导的交联(UVX),然后富集RNA-蛋白缀合物和LC-MS / MS分析。然而,由于其渗透深度低,UVX在多细胞生物组织中具有有限的适用性。在这里,我们将甲醛交联(传真)引入RNA互乱捕获(RIC)的替代化学交联。轻度传真在细胞培养的高特异性和效率中捕获RNA蛋白质相互作用。与UVX-RIC不同,FAX-RIC鲁棒地检测与结构化RNA或URACIL-POSRNAS(例如1,Stau1,UPF1,NCBP2,EIF4E,YTHDF蛋白和PABP)结合的蛋白质,扩大覆盖率。应用于Xenopus Laevis卵母细胞和胚胎,Fax-Ric提供了综合和无偏的RNA互蛋白,揭示了RNA蛋白复合物的动态重塑。值得注意的是,在卵母细胞到胚胎转换期间改变的翻译机械改变,例如,从规范EIF4E到非甘露透化的EIF4E3。此外,使用Mus Musculus肝脏,我们证明Fax-Ric适用于哺乳动物组织样品。我们一起携带,我们报告传真可以将RNA互乱的谱分析扩展到多细胞生物中。

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