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Yeast snoRNA accumulation relies on a cleavage-dependent/polyadenylation-independent 3′-processing apparatus

机译:酵母snoRNA积累依赖于裂解依赖性/多腺苷酸化无关的3加工设备

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摘要

In Saccharomyces cerevisiae, snoRNAs are encoded by independent genes and within introns. Despite this heterogenous organization, snoRNA biosynthesis relies on a common theme: entry sites for 5′–3′ and 3′–5′ exonucleases are created on precursor molecules allowing the release of mature snoRNAs. In independently transcribed snoRNAs, such entry sites are often produced by the Rnt1p endonuclease. In many cases, cleavage sites are absent in the 3′ portion of the pre-snoRNAs, suggesting that processing starts from the 3′ end of the primary transcript. Here we show that cleavage/polyadenylation sites driving efficient polyadenylation, such as CYC1, prevent production of mature and functional snoRNPs. With these sites, snoRNA accumulation is restored only if polyadenylation activity is inhibited. Analysis of sequences downstream of snoRNA-coding units and the use of strains carrying mutations in RNA polymerase II (polII) cleavage/polyadenylation activities allowed us to establish that formation of snoRNA mature 3′ ends requires only the cleavage activity of the polII 3′-processing machinery. These data indicate that, in vivo, uncoupling of cleavage and polyadenylation is necessary for an essential cellular biosynthesis.
机译:在酿酒酵母中,snoRNA由独立的基因和内含子编码。尽管存在这种异质性组织,但snoRNA的生物合成仍基于一个共同的主题:5'–3'和3'–5'核酸外切酶的进入位点在前体分子上产生,从而释放成熟的snoRNA。在独立转录的snoRNA中,此类进入位点通常是由Rnt1p核酸内切酶产生的。在许多情况下,pre-snoRNA的3'部分不存在切割位点,这表明加工过程是从初级转录本的3'末端开始的。在这里,我们显示驱动有效的聚腺苷酸化作用(例如CYC1)的切割/聚腺苷酸化位点阻止了成熟和功能性snoRNPs的产生。通过这些位点,只有在多腺苷酸化活性受到抑制的情况下,snoRNA的积累才能恢复。对snoRNA编码单元下游序列的分析以及使用携带有RNA聚合酶II(polII)切割/聚腺苷酸化活性突变的菌株的使用,使我们能够确定snoRNA成熟3'末端的形成仅需要polII 3'-的切割活性。加工机械。这些数据表明,在体内,裂解和聚腺苷酸化的解偶联对于必需的细胞生物合成是必需的。

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