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通过差异cDNA文库筛选策略分离大量新的哺乳动物基因。

Isolation of a large number of novel mammalian genes by a differential cDNA library screening strategy.

作者信息

Höög C

机构信息

Department of Molecular Genetics, Karolinska Institutet, Stockholm, Sweden.

出版信息

Nucleic Acids Res. 1991 Nov 25;19(22):6123-7. doi: 10.1093/nar/19.22.6123.

Abstract

As part of the ongoing human and mouse genome projects, the aim of this study was to isolate novel, previously uncharacterized, genes from mouse testis. Two approaches were compared for their effectiveness in isolating novel genes: random, vs differential, complementary DNA (cDNA) cloning methods. In the differential approach, only the cDNA clones containing rare sequences (as determined by preliminary clone hybridization) are further analyzed; in the random approach, cDNA clones are isolated at random from the cDNA library. More than two hundred cDNA clones altogether were analyzed, using a PCR-mediated amplification and sequencing strategy. A comparison of these sequences to nucleic acid and protein sequence databases, revealed that 84% of the isolated rare cDNA clones represented new, previously uncharacterized mouse genes. In contrast, less than 63% of the cDNA clones isolated at random from cDNA libraries, contained novel genes. Thus, the probability of isolating new, previously uncharacterized, mammalian genes from cDNA libraries can be markedly improved by focusing efforts on clones containing rare sequences.

摘要

作为正在进行的人类和小鼠基因组计划的一部分,本研究的目的是从小鼠睾丸中分离新的、以前未被表征的基因。比较了两种方法在分离新基因方面的有效性:随机互补DNA(cDNA)克隆方法和差异cDNA克隆方法。在差异方法中,仅进一步分析含有稀有序列的cDNA克隆(通过初步克隆杂交确定);在随机方法中,从cDNA文库中随机分离cDNA克隆。使用PCR介导的扩增和测序策略总共分析了两百多个cDNA克隆。将这些序列与核酸和蛋白质序列数据库进行比较,发现84%的分离出的稀有cDNA克隆代表新的、以前未被表征的小鼠基因。相比之下,从cDNA文库中随机分离的cDNA克隆中,含有新基因的不到63%。因此,通过集中精力于含有稀有序列的克隆,可以显著提高从cDNA文库中分离新的、以前未被表征的哺乳动物基因的概率。

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