The role of PRP8 protein in nuclear pre-mRNA splicing in yeast.

J D Beggs, S Teigelkamp, A J Newman
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引用次数: 25

Abstract

The removal of introns from precursor messenger RNAs occurs in a large complex, the spliceosome, that contains many proteins and five small nuclear RNAs (snRNAs). The snRNAs interact with the intron-containing substrate RNA and with each other to form a dynamic network of RNA interactions that define the intron and promote splicing. There is evidence that protein splicing factors play important roles in regulating RNA interactions in the spliceosome. PRP8 is a highly conserved protein that is associated in particles with the U5 snRNA and directly binds the substrate RNA in spliceosomes. UV crosslinking has been used to map the binding sites, and shows extensive interaction between PRP8 protein and the 5' exon prior to the first step of splicing and with the 3' splice site region subsequently. It is proposed that PRP8 protein may stabilize fragile interactions between the U5 snRNA and exon sequences at the splice sites, to anchor and align them in the catalytic centre of the spliceosome.

PRP8蛋白在酵母核前mrna剪接中的作用。
从前体信使rna中去除内含子发生在一个大的复合体中,剪接体包含许多蛋白质和5个小核rna (snrna)。snrna与内含子的底物RNA相互作用,并相互作用形成一个动态的RNA相互作用网络,定义内含子并促进剪接。有证据表明,蛋白质剪接因子在调节剪接体中RNA的相互作用中起着重要作用。PRP8是一种高度保守的蛋白,在颗粒中与U5 snRNA结合,并在剪接体中直接结合底物RNA。UV交联已被用于定位结合位点,并显示PRP8蛋白在剪接的第一步之前与5'外显子以及随后与3'剪接位点区域之间存在广泛的相互作用。PRP8蛋白可能稳定了U5 snRNA与剪接位点外显子序列之间脆弱的相互作用,将它们锚定并排列在剪接体的催化中心。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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