首页> 外文期刊>Genes and Development: a Journal Devoted to the Molecular Analysis of Gene Expression in Eukaryotes, Prokaryotes, and Viruses >Polycistronic pre-mRNA processing in vitro: snRNP and pre-mRNA role reversal in trans-splicing.
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Polycistronic pre-mRNA processing in vitro: snRNP and pre-mRNA role reversal in trans-splicing.

机译:体外多顺反子pre-mRNA加工:snRNP和pre-mRNA在反式剪接中的作用逆转。

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Spliced leader (SL) trans-splicing in Caenorhabditis elegans attaches a 22-nucleotide (nt) exon onto the 5' end of many mRNAs. A particular class of SL, SL2, splices mRNAs of downstream operon genes. Here we use an embryonic extract-based in vitro splicing system to show that SL2 specificity information is encoded within the polycistronic pre-mRNA, and that trans-splicing specificity is recapitulated in vitro. We define an RNA sequence required for SL2 trans-splicing, the U-rich (Ur) element, through mutational analysis and bioinformatics as a short stem-loop followed by a sequence motif, UAYYUU, located approximately 50 nt upstream of the trans-splice site. Furthermore, this element is predicted in intercistronic regions of numerous operons of C. elegans and other species that use SL2 trans-splicing. We propose that the UAYYUU motif hybridizes with the 5' splice site on the SL2 RNA to recruit the SL to the pre-mRNA. In this way, the UAYYUU motif in the pre-mRNA would serve an analogous function to the similar sequence in the U1 snRNA, which binds to the 5' splice site of introns, effectively reversing the roles of snRNP and pre-mRNA in trans-splicing.
机译:秀丽隐杆线虫的剪接前导(SL)反式剪接将22个核苷酸(nt)外显子附着到许多mRNA的5'末端。一类特殊的SL,SL2,剪接下游操纵子基因的mRNA。在这里,我们使用基于胚胎提取物的体外剪接系统来显示SL2特异性信息是在多顺反子pre-mRNA内编码的,而转拼特异性在体外得到了概括。通过突变分析和生物信息学,我们将SL2反式剪接所需的RNA序列定义为U-rich(Ur)元素,将其作为短茎环,后接序列基序UAYYUU,位于反剪接上游约50 nt现场。此外,该元素在秀丽隐杆线虫和使用SL2反式剪接的其他物种的许多操纵子的顺反子区域中被预测。我们建议UAYYUU母题与SL2 RNA的5'剪接位点杂交,以将SL募集到pre-mRNA。这样,pre-mRNA中的UAYYUU基序将发挥与U1 snRNA中类似序列相似的功能,该序列与内含子的5'剪接位点结合,有效逆转了snRNP和pre-mRNA在反式中的作用。拼接。

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