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piRNABank: a web resource on classified and clustered Piwi-interacting RNAs.piRNABank:一个关于分类和聚类的与Piwi相互作用RNA的网络资源。
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LongSAGE profiling of nine human embryonic stem cell lines.九种人类胚胎干细胞系的LongSAGE分析
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MiPred: classification of real and pseudo microRNA precursors using random forest prediction model with combined features.MiPred:使用具有组合特征的随机森林预测模型对真实和伪微小RNA前体进行分类。
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Redirection of silencing targets by adenosine-to-inosine editing of miRNAs.通过微小RNA的腺苷到肌苷编辑实现沉默靶点的重定向。
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大规模平行测序在人类胚胎干细胞微小RNA谱分析与发现中的应用。

Application of massively parallel sequencing to microRNA profiling and discovery in human embryonic stem cells.

作者信息

Morin Ryan D, O'Connor Michael D, Griffith Malachi, Kuchenbauer Florian, Delaney Allen, Prabhu Anna-Liisa, Zhao Yongjun, McDonald Helen, Zeng Thomas, Hirst Martin, Eaves Connie J, Marra Marco A

机构信息

Genome Sciences Centre, BC Cancer Agency, Vancouver, British Columbia V5Z 1L3, Canada.

出版信息

Genome Res. 2008 Apr;18(4):610-21. doi: 10.1101/gr.7179508. Epub 2008 Feb 19.

DOI:10.1101/gr.7179508
PMID:18285502
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2279248/
Abstract

MicroRNAs (miRNAs) are emerging as important, albeit poorly characterized, regulators of biological processes. Key to further elucidation of their roles is the generation of more complete lists of their numbers and expression changes in different cell states. Here, we report a new method for surveying the expression of small RNAs, including microRNAs, using Illumina sequencing technology. We also present a set of methods for annotating sequences deriving from known miRNAs, identifying variability in mature miRNA sequences, and identifying sequences belonging to previously unidentified miRNA genes. Application of this approach to RNA from human embryonic stem cells obtained before and after their differentiation into embryoid bodies revealed the sequences and expression levels of 334 known plus 104 novel miRNA genes. One hundred seventy-one known and 23 novel microRNA sequences exhibited significant expression differences between these two developmental states. Owing to the increased number of sequence reads, these libraries represent the deepest miRNA sampling to date, spanning nearly six orders of magnitude of expression. The predicted targets of those miRNAs enriched in either sample shared common features. Included among the high-ranked predicted gene targets are those implicated in differentiation, cell cycle control, programmed cell death, and transcriptional regulation.

摘要

微小RNA(miRNA)正逐渐成为生物过程的重要调节因子,尽管其特征尚不明确。进一步阐明其作用的关键在于生成更完整的不同细胞状态下miRNA数量及表达变化列表。在此,我们报道一种利用Illumina测序技术检测包括miRNA在内的小RNA表达的新方法。我们还展示了一套用于注释已知miRNA衍生序列、鉴定成熟miRNA序列变异性以及鉴定属于先前未鉴定miRNA基因的序列的方法。将该方法应用于人类胚胎干细胞分化为胚状体前后获得的RNA,揭示了334个已知miRNA基因和104个新miRNA基因的序列及表达水平。171个已知和23个新的微小RNA序列在这两种发育状态之间表现出显著的表达差异。由于序列读数的增加,这些文库代表了迄今为止最深层次的miRNA采样,涵盖了近六个数量级的表达水平。在任一样本中富集的那些miRNA的预测靶标具有共同特征。排名靠前的预测基因靶标包括那些与分化、细胞周期调控、程序性细胞死亡和转录调控有关的基因。