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使用无预扩增定向RNA测序方法从小规模样本中检测双向启动子衍生的长链非编码RNA

Detection of Bidirectional Promoter-Derived lncRNAs from Small-Scale Samples Using Pre-Amplification-Free Directional RNA-seq Method.

作者信息

Hamazaki Nobuhiko, Nakashima Kinichi, Hayashi Katsuhiko, Imamura Takuya

机构信息

Department of Stem Cell Biology and Medicine, Graduate School of Medical Sciences, Kyushu University, Maidashi 3-1-1, Fukuoka 812-8582, Japan.

出版信息

Methods Mol Biol. 2017;1605:83-103. doi: 10.1007/978-1-4939-6988-3_6.

DOI:10.1007/978-1-4939-6988-3_6
PMID:28456959
Abstract

Development of high-throughput sequencing technologies has uncovered the immensity of the long noncoding RNA (lncRNA) world. Divergently transcribed lncRNAs from bidirectional gene promoters, called promoter-associated noncoding RNAs (pancRNAs), account for ~20% of the total number of lncRNAs, and this major fraction is involved in many biological processes, such as development and cancer formation. Recently, we have found that the pancRNAs activate their partner genes, as represented by the fact that pancIl17d, a pancRNA that is transcribed from the antisense strand of the promoter region of Interleukin 17d (Il17d) at the onset of zygotic gene activation (ZGA), is essential for mouse preimplantation development through Il17d upregulation. The discovery of the expression of a specific set of pancRNAs during ZGA was achieved by using a method that generates directional RNA-seq libraries from small-scale samples. Although there are several methods available for small-scale samples, most of them require a pre-amplification procedure that frequently generates some amplification biases toward a subset of transcripts. We provide here a highly sensitive and reproducible method based on the preparation of directional RNA-seq libraries from as little as 100 mouse oocytes or embryos without pre-amplification for the quantification of lncRNAs as well as mRNAs.

摘要

高通量测序技术的发展揭示了长链非编码RNA(lncRNA)世界的广阔性。从双向基因启动子反向转录的lncRNA,称为启动子相关非编码RNA(pancRNA),占lncRNA总数的约20%,并且这一主要部分参与了许多生物学过程,如发育和癌症形成。最近,我们发现pancRNA激活其伙伴基因,例如pancIl17d,它是在合子基因激活(ZGA)开始时从白细胞介素17d(Il17d)启动子区域的反义链转录的一种pancRNA,通过上调Il17d对小鼠植入前发育至关重要。通过使用一种从小规模样本生成定向RNA-seq文库的方法,实现了在ZGA期间一组特定pancRNA表达的发现。虽然有几种方法可用于小规模样本,但大多数方法都需要预扩增程序,这经常会对一部分转录本产生一些扩增偏差。我们在此提供一种高度灵敏且可重复的方法,该方法基于从低至100个小鼠卵母细胞或胚胎制备定向RNA-seq文库,无需预扩增即可对lncRNA和mRNA进行定量。

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