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首页> 外文期刊>Molecular and Cellular Biology >Processing of the Intron-Encoded U18 Small Nucleolar RNA in the Yeast Saccharomyces cerevisiaeRelies on Both Exo- and Endonucleolytic Activities
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Processing of the Intron-Encoded U18 Small Nucleolar RNA in the Yeast Saccharomyces cerevisiaeRelies on Both Exo- and Endonucleolytic Activities

机译:酵母酵母中内含子编码的U18小核仁RNA的加工依赖于核酸外切和核酸内切活性

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Many small nucleolar RNAs (snoRNAs) are encoded within introns of protein-encoding genes and are released by processing of their host pre-mRNA. We have investigated the mechanism of processing of the yeast U18 snoRNA, which is found in the intron of the gene coding for translational elongation factor EF-1β. We have focused our analysis on the relationship between splicing of the EF-1β pre-mRNA and production of the mature snoRNA. Mutations inhibiting splicing of the EF-1β pre-mRNA have been shown to produce normal U18 snoRNA levels together with the accumulation of intermediates deriving from the pre-mRNA, thus indicating that the precursor is an efficient processing substrate. Inhibition of 5′→3′ exonucleases obtained by insertion of G cassettes or by the use of a rat1-1 xrn1Δ mutant strain does not impair U18 release. In the Exo? strain, 3′ cutoff products, diagnostic of an endonuclease-mediated processing pathway, were detected. Our data indicate that biosynthesis of the yeast U18 snoRNA relies on two different pathways, depending on both exonucleolytic and endonucleolytic activities: a major processing pathway based on conversion of the debranched intron and a minor one acting by endonucleolytic cleavage of the pre-mRNA.
机译:许多小核仁RNA(snoRNA)在蛋白质编码基因的内含子中编码,并通过加工其宿主前体mRNA释放。我们研究了酵母U18 snoRNA的加工机制,该机制在编码翻译延伸因子EF-1β的基因的内含子中发现。我们将分析的重点放在EF-1βpre-mRNA的剪接与成熟snoRNA的产生之间的关系上。已显示出抑制EF-1β前mRNA剪接的突变会产生正常的U18 snoRNA水平,以及源自前mRNA的中间体的积累,因此表明该前体是有效的加工底物。通过插入G盒或使用 rat1-1 xrn1 Δ突变株获得的5'→3'核酸外切酶的抑制不会损害U18的释放。在Exo ?菌株中,检测到3'截断产物,可诊断核酸内切酶介导的加工途径。我们的数据表明,酵母U18 snoRNA的生物合成依赖于两种不同的途径,具体取决于外切核酸和内切核酸活性:一种主要的加工途径是基于脱支内含子的转化,另一部分是通过前mRNA的内切核酸酶的作用。

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