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利用散布重复序列-PCR产物进行cDNA筛选。

Use of interspersed repetitive sequences-PCR products for cDNA selection.

作者信息

Villard L, Passage E, Colleaux L, Fontes M

机构信息

INSERM U406. 27, Marseille, France.

出版信息

Mamm Genome. 1995 Sep;6(9):617-22. doi: 10.1007/BF00352368.

Abstract

In order to increase the efficiency of cDNA selection approaches, we describe the use of interspersed repetitive sequences-PCR (IRS-PCR) products to isolate genes from large-insert genomic clones. IRS-PCR is conducted on total yeast DNA containing a YAC of interest so that there is no need to purify the starting genomic clone. This enables the production of large amounts of genomic substrate for cDNA selection and allows the use of unstable YAC clones. Moreover, the hybridization of the IRS-PCR product to the cDNA clones after selection introduces a positive selection step. We tested these PCR products from YACs for the presence of exons, using cDNAs originating from seven different genes. In each case, at least one exon was present in the IRS-PCR product. We have applied this strategy to four YAC clones originating from the human X Chromosome (Chr). All the selected cDNAs, strongly positive with the IRS-PCR product, did indeed originate from a gene in the region covered by the YAC. In all cases, the previously known genes contained in the genomic clones have been isolated. In addition, we have isolated human genes that have already been described but not assigned to any chromosomal region.

摘要

为了提高cDNA筛选方法的效率,我们描述了利用散布重复序列-PCR(IRS-PCR)产物从大插入片段基因组克隆中分离基因的方法。对含有感兴趣酵母人工染色体(YAC)的酵母总DNA进行IRS-PCR,这样就无需纯化起始基因组克隆。这能够产生大量用于cDNA筛选的基因组底物,并允许使用不稳定的YAC克隆。此外,筛选后IRS-PCR产物与cDNA克隆的杂交引入了一个阳性筛选步骤。我们使用源自七个不同基因的cDNA,测试了来自YAC的这些PCR产物中外显子的存在情况。在每种情况下,IRS-PCR产物中至少存在一个外显子。我们已将此策略应用于源自人类X染色体(Chr)的四个YAC克隆。所有与IRS-PCR产物呈强阳性反应的筛选出的cDNA确实都源自YAC所覆盖区域中的一个基因。在所有情况下,基因组克隆中包含的先前已知基因均已被分离出来。此外,我们还分离出了已被描述但尚未定位到任何染色体区域的人类基因。

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