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首页> 外文期刊>Nucleic Acids Research >Identification of endoribonuclease specific cleavage positions reveals novel targets of RNase III in Streptococcus pyogenes
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Identification of endoribonuclease specific cleavage positions reveals novel targets of RNase III in Streptococcus pyogenes

机译:鉴定内衣核糖核酸酶的特异性切割位置揭示了链球菌在细菌肽中的RNase III的新靶

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A better understanding of transcriptional and post-transcriptional regulation of gene expression in bacteria relies on studying their transcriptome. RNA sequencing methods are used not only to assess RNA abundance but also the exact boundaries of primary and processed transcripts. Here, we developed a method, called identification of specific cleavage position (ISCP), which enables the identification of direct endoribonuclease targets in vivo by comparing the 5' and 3' ends of processed transcripts between wild type and RNase deficient strains. To demonstrate the ISCP method, we used as a model the double-stranded specific RNase III in the human pathogen Streptococcus pyogenes. We mapped 92 specific cleavage positions (SCPs) among which, 48 were previously described and 44 are new, with the characteristic 2 nucleotides 3' overhang of RNase III. Most SCPs were located in untranslated regions of RNAs. We screened for RNase III targets using transcriptomic differential expression analysis (DEA) and compared those with the RNase III targets identified using the ISCP method. Our study shows that in S. pyogenes, under standard growth conditions, RNase III has a limited impact both on antisense transcripts and on global gene expression with the expression of most of the affected genes being downregulated in an RNase III deletion mutant.
机译:更好地了解细菌中基因表达的转录和转录后调节依赖于研究其转录组。 RNA测序方法不仅用于评估RNA丰度,而且使用初级和加工转录物的确切边界。在此,我们开发了一种称为特异性切割位置(ISCP)的方法,其能够通过比较野生型和RNase缺乏菌株之间的5'和3'和3'末端来鉴定体内的直接内联核酸酶靶标。为了证明ISCP方法,我们用作人病原体链球菌化合物中的双链特异性RNase III的模型。我们在其中映射了92个特定的裂解位置(SCP),先前描述了48个,44个是新的,具有RNase III的特征2核苷酸3'突出。大多数SCP都位于未翻译的RNA区域。我们使用转录组差异表达分析(DEA)筛选RNase III靶标,并将那些使用ISCP方法鉴定的RNase III靶进行比较。我们的研究表明,在S. pyogenes,在标准生长条件下,RNase III对反义转录物和全局基因表达的影响有限,并且在RNase III缺失突变体中表达大多数受影响的基因的表达。

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