一种基于mRNA帽保留程序(CAPture)分离全长cDNA的有效策略。
An efficient strategy to isolate full-length cDNAs based on an mRNA cap retention procedure (CAPture).
作者信息
Edery I, Chu L L, Sonenberg N, Pelletier J
机构信息
Rutgers University, Piscataway, New Jersey 08854, USA.
出版信息
Mol Cell Biol. 1995 Jun;15(6):3363-71. doi: 10.1128/MCB.15.6.3363.
Abstract
The ability to generate cDNA libraries is one of the most fundamental procedures in contemporary molecular biology. One of the major drawbacks of current methods is that most cDNAs present in any given library are incomplete, rendering the characterization of genes an inefficient and time-consuming task. We have developed an affinity selection procedure using a fusion protein containing the murine cap-binding protein (eukaryotic initiation factor 4E), coupled to a solid support matrix, that allows for the purification of mRNAs via the 5' cap structure. When combined with a single-strand-specific RNase digestion step, specific retention of complete cDNA-RNA duplexes following first-strand synthesis is achieved. This method can be used to generate cDNA libraries in which polyadenylated and nonpolyadenylated mRNAs are equally represented and to enrich for full-length or 5'-end clones, thus facilitating cDNA cloning and promoter mapping.
摘要
生成cDNA文库的能力是当代分子生物学中最基本的操作之一。当前方法的一个主要缺点是,任何给定文库中存在的大多数cDNA都是不完整的,这使得基因表征成为一项低效且耗时的任务。我们开发了一种亲和选择程序,使用一种与固相支持基质偶联的含有鼠帽结合蛋白(真核起始因子4E)的融合蛋白,该程序允许通过5'帽结构纯化mRNA。当与单链特异性核糖核酸酶消化步骤相结合时,在第一链合成后可实现完整cDNA-RNA双链体的特异性保留。该方法可用于生成其中聚腺苷酸化和非聚腺苷酸化mRNA均得到同等代表的cDNA文库,并富集全长或5'端克隆,从而促进cDNA克隆和启动子定位。
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