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Endogenous RNAi pathway evolutionarily shapes the destiny of the antisense lncRNAs transcriptome

机译:内源性RNAi途径进化形成反义lncRNA转录组的命运

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摘要

Antisense long noncoding (aslnc)RNAs are extensively degraded by the nuclear exosome and the cytoplasmic exoribonuclease Xrn1 in the budding yeast Saccharomyces cerevisiae, lacking RNAi. Whether the ribonuclease III Dicer affects aslncRNAs in close RNAi-capable relatives remains unknown. Using genome-wide RNA profiling, here we show that aslncRNAs are primarily targeted by the exosome and Xrn1 in the RNAi-capable budding yeast Naumovozyma castellii, Dicer only affecting Xrn1-sensitive aslncRNAs levels in Xrn1-deficient cells. The dcr1 and xrn1 mutants display synergic growth defects, indicating that Dicer becomes critical in the absence of Xrn1. Small RNA sequencing showed that Dicer processes aslncRNAs into small RNAs, with a preference for Xrn1-sensitive aslncRNAs. Consistently, Dicer localizes into the cytoplasm. Finally, we observed an expansion of the exosome-sensitive antisense transcriptome in N. castellii compared with S. cerevisiae, suggesting that the presence of cytoplasmic RNAi has reinforced the nuclear RNA surveillance machinery to temper aslncRNAs expression. Our data provide fundamental insights into aslncRNAs metabolism and open perspectives into the possible evolutionary contribution of RNAi in shaping the aslncRNAs transcriptome.
机译:反义的长非编码(aslnc)RNA被核外泌体和缺少RNAi的酿酒酵母中的胞质外核糖核酸酶Xrn1广泛降解。核糖核酸酶III Dicer是否会影响具有RNAi能力的近亲中的aslncRNA,尚不清楚。使用全基因组的RNA分析,在这里我们显示aslncRNAs主要是由具有RNAi能力的发芽酵母Naumovozyma castellii中的外泌体和Xrn1靶向的,Dicer仅影响Xrn1缺陷细胞中对Xrn1敏感的aslncRNAs水平。 dcr1和xrn1突变体显示协同生长缺陷,表明Dicer在缺少Xrn1的情况下变得至关重要。小RNA测序显示Dicer将aslncRNA加工成小RNA,优先选择对Xrn1敏感的aslncRNA。一致地,切丁机定位于细胞质中。最后,我们观察到与啤酒糖酵母相比,在卡氏猪笼草中外泌体敏感的反义转录组有所扩展,这表明细胞质RNAi的存在增强了核RNA监测机制,以调节aslncRNAs的表达。我们的数据为aslncRNA的代谢提供了基本见识,并为RNAi在塑造aslncRNA转录组中可能的进化贡献提供了开阔的视野。

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