一种寻找组织特异性选择性腺苷脱氨基新位点的方法。

A method to find tissue-specific novel sites of selective adenosine deamination.

作者信息

Ohlson Johan, Ensterö Mats, Sjöberg Britt-Marie, Ohman Marie

机构信息

Department of Molecular Biology and Functional Genomics, Stockholm University, S-106 91 Stockholm, Sweden.

出版信息

Nucleic Acids Res. 2005 Oct 27;33(19):e167. doi: 10.1093/nar/gni169.

DOI:10.1093/nar/gni169

PMID:16257978

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1275595/

Abstract

Site-selective adenosine (A) to inosine (I) RNA editing by the ADAR enzymes has been found in a variety of metazoan from fly to human. Here we describe a method to detect novel site-selective A to I editing that can be used on various tissues as well as species. We have shown previously that there is a preference for ADAR2-binding to selectively edited sites over non-specific interactions with random sequences of double-stranded RNA. The method utilizes immunoprecipitation (IP) of intrinsic RNA-protein complexes to extract substrates subjected to site-selective editing in vivo, in combination with microarray analyses of the captured RNAs. We show that known single sites of A to I editing can be detected after IP using an antibody against the ADAR2 protein. The RNA substrates were verified by RT-PCR, RNase protection and microarray. Using this method it is possible to uniquely identify novel single sites of selective A to I editing.

摘要

在从果蝇到人类的多种后生动物中都发现了ADAR酶介导的位点选择性腺苷（A）到肌苷（I）的RNA编辑。在此，我们描述了一种检测新型位点选择性A到I编辑的方法，该方法可用于各种组织和物种。我们之前已经表明，相较于与双链RNA随机序列的非特异性相互作用，ADAR2更倾向于结合到选择性编辑的位点。该方法利用体内经过位点选择性编辑的内在RNA-蛋白质复合物的免疫沉淀（IP）来提取底物，并结合对捕获RNA的微阵列分析。我们表明，使用针对ADAR2蛋白的抗体进行IP后，可以检测到已知的A到I编辑单一位点。RNA底物通过逆转录聚合酶链反应（RT-PCR）、核糖核酸酶保护和微阵列进行了验证。使用这种方法可以唯一地识别新型的选择性A到I编辑单一位点。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/fc8f/1275595/6d3ba3232231/gni169f1.jpg

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一种寻找组织特异性选择性腺苷脱氨基新位点的方法。

A method to find tissue-specific novel sites of selective adenosine deamination.

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