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RPL30 剪接调控揭示了 Cbp80 在 U1 和 U2 snRNP 共转录募集中的不同作用。

RPL30 regulation of splicing reveals distinct roles for Cbp80 in U1 and U2 snRNP cotranscriptional recruitment.

机构信息

Centre de Regulació Genòmica, Barcelona, Spain.

出版信息

RNA. 2010 Oct;16(10):2033-41. doi: 10.1261/rna.2366310. Epub 2010 Aug 27.

Abstract

Pre-mRNA splicing is catalyzed by the spliceosome, and its control is essential for correct gene expression. While splicing repressors typically interfere with transcript recognition by spliceosomal components, the yeast protein L30 blocks spliceosomal rearrangements required for the engagement of U2 snRNP (small ribonucleoprotein particle) to its own transcript RPL30. Using a mutation in the RPL30 binding site that disrupts this repression, we have taken a genetic approach to reveal that regulation of splicing is restored in this mutant by deletion of the cap-binding complex (CBC) component Cbp80. Indeed, our data indicate that Cbp80 plays distinct roles in the recognition of the intron by U1 and U2 snRNP. It promotes the initial 5' splice site recognition by U1 and, independently, facilitates U2 recruitment, depending on sequences located in the vicinity of the 5' splice site. These results reveal a novel function for CBC in splicing and imply that these molecular events can be the target of a splicing regulator.

摘要

前体 mRNA 剪接由剪接体催化,其调控对于正确的基因表达至关重要。虽然剪接抑制剂通常干扰剪接体成分对转录本的识别,但酵母蛋白 L30 阻止了 U2 snRNP(小核糖核蛋白颗粒)与其自身转录本 RPL30 结合所需的剪接体重排。我们利用 RPL30 结合位点的突变,该突变破坏了这种抑制作用,通过删除帽结合复合物(CBC)成分 Cbp80 ,采用遗传方法揭示了这种突变体中剪接的调控得以恢复。事实上,我们的数据表明 Cbp80 在 U1 和 U2 snRNP 对内含子的识别中发挥不同的作用。它促进了 U1 对 5' 剪接位点的初始识别,并且独立地促进 U2 的募集,这取决于位于 5' 剪接位点附近的序列。这些结果揭示了 CBC 在剪接中的新功能,并暗示这些分子事件可以成为剪接调节剂的靶标。

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