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哺乳动物细胞核提取物中的外显子环化

Exon circularization in mammalian nuclear extracts.

作者信息

Pasman Z, Been M D, Garcia-Blanco M A

机构信息

Department of Molecular Cancer Biology, Levine Sciences Research Center, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

RNA. 1996 Jun;2(6):603-10.

PMID:8718689
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1369399/
Abstract

Correct ligation of exons in pre-mRNA splicing requires splice site juxtaposition (splice site pairing), usually involving a 5' splice site and a downstream 3' splice site. Splicing of a 5' splice site to an upstream 3' splice site, however, is predicted to result in a circular RNA. This mode of splice site pairing across the axon has been hypothesized to account for rare RNAs containing scrambled exons (Nigro JM et al., 1991, Celt 64:607-613; Cocquerelle C et al., 1992, EMBO J 11:1 095-1098). Additionally, this mode of splice site pairing has been postulated to explain the formation of SRY circular transcripts in mouse testis (Capel B et al., 1993, Celt 73:1019- 1030). Here we show that splice site pairing across the exon can result in exon circularization in vitro. These results indicate that spliceosome-mediated axon circularization indeed can account for the formation of scrambled exons and circular RNAs. Exon circularization efficiency decreased dramatically as the length of the exon was increased from 95 nt to 274 nt. Circularization of this longer exon was restored, however, when intronic complementary sequences were included in the RNA substrate. These complementary sequences could form a stem that served to bring the splice sites into proximity and thereby promote splice site pairing. Therefore, the splicing of this structured RNA recapitulated SRY-like exon circularization in vitro.

摘要

前体mRNA剪接中外显子的正确连接需要剪接位点并列(剪接位点配对),通常涉及一个5'剪接位点和一个下游的3'剪接位点。然而,将一个5'剪接位点与一个上游的3'剪接位点进行剪接预计会产生一个环状RNA。这种跨轴突的剪接位点配对模式已被假设用于解释含有混乱外显子的罕见RNA(Nigro JM等人,1991年,《细胞》64:607 - 613;Cocquerelle C等人,1992年,《欧洲分子生物学组织杂志》11:1095 - 1098)。此外,这种剪接位点配对模式已被假定用于解释小鼠睾丸中SRY环状转录本的形成(Capel B等人,1993年,《细胞》73:1019 - 1030)。在这里,我们表明跨外显子的剪接位点配对在体外可导致外显子环化。这些结果表明,剪接体介导的轴突环化确实可以解释混乱外显子和环状RNA的形成。随着外显子长度从95个核苷酸增加到274个核苷酸,外显子环化效率急剧下降。然而,当RNA底物中包含内含子互补序列时,这个较长外显子的环化得以恢复。这些互补序列可以形成一个茎,用于使剪接位点靠近,从而促进剪接位点配对。因此,这种结构化RNA的剪接在体外重现了类似SRY的外显子环化。

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