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秀丽隐杆线虫反式剪接受体的功能分析

Functional analysis of a C. elegans trans-splice acceptor.

作者信息

Conrad R, Liou R F, Blumenthal T

机构信息

Department of Biology, Indiana University, Bloomington 47405.

出版信息

Nucleic Acids Res. 1993 Feb 25;21(4):913-9. doi: 10.1093/nar/21.4.913.

Abstract

The rol-6 gene is trans-spliced to the 22 nt leader, SL1, 173 nt downstream of the transcription start. We have analyzed splicing in transformants carrying extrachromosomal arrays of rol-6 with mutations in the trans-splice acceptor site. This site is a close match to the consensus, UUUCAG, that is highly conserved in both trans-splice and intron acceptor sites in C. elegans. When the trans-splice site was inactivated by mutating the perfectly-conserved AG, trans-splicing still occurred, but at a cryptic site 20 nt upstream. We tested the frequency with which splicing switched from the normal site to the cryptic site when the pyrimidines at this site were changed to A's. Since most C. elegans 3' splice sites lack an obvious polypyrimidine tract, we hypothesized that these four pyrimidines might play this role, and indeed mutation of these bases caused splicing to switch to the cryptic site. We also demonstrated that a major reason the downstream site is normally favored is because it occurs at a boundary between A+U rich and non-A+U rich RNA. When the RNA between the two splice sites was made less A+U rich, splicing occurred preferentially at the upstream site.

摘要

rol-6基因在转录起始点下游173个核苷酸处与22个核苷酸的前导序列SL1进行反式剪接。我们分析了携带rol-6染色体外阵列且反式剪接受体位点发生突变的转化体中的剪接情况。该位点与共有序列UUUCAG高度匹配,在秀丽隐杆线虫的反式剪接和内含子接受位点中都高度保守。当通过突变完全保守的AG使反式剪接位点失活时,反式剪接仍会发生,但在其上游20个核苷酸处的一个隐蔽位点。我们测试了将该位点的嘧啶突变为腺嘌呤时,剪接从正常位点切换到隐蔽位点的频率。由于大多数秀丽隐杆线虫的3'剪接位点缺乏明显的多嘧啶序列,我们推测这四个嘧啶可能起这个作用,实际上这些碱基的突变导致剪接切换到隐蔽位点。我们还证明了下游位点通常更受青睐的一个主要原因是它位于富含A+U和非富含A+U的RNA之间的边界处。当两个剪接位点之间的RNA变得不那么富含A+U时,剪接优先发生在上游位点。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8729/309224/b32713456065/nar00053-0130-a.jpg

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