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Alu剪接聚合酶链反应:一种从克隆的人类基因组DNA中分离含外显子片段的简单方法。

Alu-splice PCR: a simple method to isolate exon-containing fragments from cloned human genomic DNA.

作者信息

Fuentes J J, Pucharcós C, Pritchard M, Estivill X

机构信息

Medical and Molecular Genetics Center-IRO, L'Hospitalet de Llobregat, Barcelona, Spain.

出版信息

Hum Genet. 1997 Dec;101(3):346-50. doi: 10.1007/s004390050639.

Abstract

We have developed a simple, straightforward procedure to isolate exons from cloned human genomic DNA. The method is PCR based and relies upon the conservation of splice-site sequences and the frequency of Alu repeat elements in the genome to capture coding sequences. We designed two different sets of primers: a primer from each end of the Alu element and primers with the 5' or 3' splice-site consensus sequences. Putative exons were amplified by PCR using YAC DNA as starting material. We applied Alu-splice PCR to two overlapping YACs, 72H9 and 860G11, from human chromosome 21. Sequence and northern analysis of 37 initial clones resulted in the identification of five novel exons.

摘要

我们开发了一种简单、直接的方法,用于从克隆的人类基因组DNA中分离外显子。该方法基于聚合酶链反应(PCR),并依赖于剪接位点序列的保守性以及基因组中Alu重复元件的频率来捕获编码序列。我们设计了两组不同的引物:一组来自Alu元件两端的引物,另一组带有5'或3'剪接位点共有序列的引物。以酵母人工染色体(YAC)DNA作为起始材料,通过PCR扩增推定的外显子。我们将Alu - 剪接PCR应用于来自人类21号染色体的两个重叠YAC,即72H9和860G11。对37个初始克隆进行序列和Northern分析后,鉴定出了5个新的外显子。

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