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荚膜红细菌中小RNA的全基因组鉴定与特征分析以及受应答调节因子CtrA缺失影响的小RNA的鉴定

Genome-wide identification and characterization of small RNAs in Rhodobacter capsulatus and identification of small RNAs affected by loss of the response regulator CtrA.

作者信息

Grüll Marc P, Peña-Castillo Lourdes, Mulligan Martin E, Lang Andrew S

机构信息

a Department of Biology , Memorial University of Newfoundland , St. John's , NL , Canada.

b Department of Computer Science , Memorial University of Newfoundland , St. John's , NL , Canada.

出版信息

RNA Biol. 2017 Jul 3;14(7):914-925. doi: 10.1080/15476286.2017.1306175. Epub 2017 Mar 15.

Abstract

Small non-coding RNAs (sRNAs) are involved in the control of numerous cellular processes through various regulatory mechanisms, and in the past decade many studies have identified sRNAs in a multitude of bacterial species using RNA sequencing (RNA-seq). Here, we present the first genome-wide analysis of sRNA sequencing data in Rhodobacter capsulatus, a purple nonsulfur photosynthetic alphaproteobacterium. Using a recently developed bioinformatics approach, sRNA-Detect, we detected 422 putative sRNAs from R. capsulatus RNA-seq data. Based on their sequence similarity to sRNAs in a sRNA collection, consisting of published putative sRNAs from 23 additional bacterial species, and RNA databases, the sequences of 124 putative sRNAs were conserved in at least one other bacterial species; and, 19 putative sRNAs were assigned a predicted function. We bioinformatically characterized all putative sRNAs and applied machine learning approaches to calculate the probability of a nucleotide sequence to be a bona fide sRNA. The resulting quantitative model was able to correctly classify 95.2% of sequences in a validation set. We found that putative cis-targets for antisense and partially overlapping sRNAs were enriched with protein-coding genes involved in primary metabolic processes, photosynthesis, compound binding, and with genes forming part of macromolecular complexes. We performed differential expression analysis to compare the wild type strain to a mutant lacking the response regulator CtrA, an important regulator of gene expression in R. capsulatus, and identified 18 putative sRNAs with differing levels in the two strains. Finally, we validated the existence and expression patterns of four novel sRNAs by Northern blot analysis.

摘要

小非编码RNA(sRNA)通过多种调控机制参与众多细胞过程的控制,在过去十年中,许多研究利用RNA测序(RNA-seq)在多种细菌物种中鉴定出了sRNA。在此,我们首次对紫色非硫光合α-变形菌荚膜红细菌的sRNA测序数据进行了全基因组分析。使用最近开发的生物信息学方法sRNA-Detect,我们从荚膜红细菌的RNA-seq数据中检测到422个假定的sRNA。基于它们与sRNA集合(由来自另外23种细菌物种的已发表假定sRNA组成)和RNA数据库中sRNA的序列相似性,124个假定sRNA的序列在至少一种其他细菌物种中是保守的;并且,19个假定sRNA被赋予了预测功能。我们对所有假定的sRNA进行了生物信息学表征,并应用机器学习方法来计算核苷酸序列成为真正sRNA的概率。所得的定量模型能够正确分类验证集中95.2%的序列。我们发现反义sRNA和部分重叠sRNA的假定顺式靶标富含参与初级代谢过程、光合作用、化合物结合的蛋白质编码基因,以及构成大分子复合物一部分的基因。我们进行了差异表达分析,以将野生型菌株与缺乏应答调节因子CtrA(荚膜红细菌中基因表达的重要调节因子)的突变体进行比较,并鉴定出两种菌株中水平不同的18个假定sRNA。最后,我们通过Northern印迹分析验证了四种新型sRNA的存在和表达模式。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/fab9/5546546/c6ba69425719/krnb-14-07-1306175-g001.jpg

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