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通过B1重复序列代表性差异分析分离48个适合近交系大鼠品系高通量基因分型的遗传标记。

Isolation of 48 genetic markers appropriate for high throughput genotyping of inbred rat strains by B1 repetitive sequence-representational difference analysis.

作者信息

Ushijima T, Nomoto T, Sugimura T, Housman D E, Nagao M

机构信息

Carcinogenesis Division, National Cancer Center Research Institute, 1-1 Tsukiji 5-chome, Chuo-ku, Tokyo 104-0045, Japan.

出版信息

Mamm Genome. 1998 Dec;9(12):1008-12. doi: 10.1007/s003359900916.

Abstract

Mapping of genetic suppressors, modifiers, and quantitative trait loci (QTLs) requires genetic markers that can be efficiently and inexpensively genotyped for a large number of individuals. To isolate rat genetic markers suitable for this purpose, representational difference analysis (RDA) was performed with amplicons prepared by PCR with the B1 repetitive sequence used as the primer (B1-amplicons). In total, 48 polymorphic DNA fragments were isolated by five series of RDA, subtracting the B1-amplicons prepared from an ACI/N (ACI) rat from those prepared from BUF/Nac (BUF), and vice versa. All the polymorphic fragments detected "presence-or-absence" polymorphisms with B1-amplicons prepared from ACI, BUF, and their F2 progeny, and each fragment was linkage mapped. Dot-blotting amplicons onto filters at a high density and hybridization of the filters with these B1-RDA markers made it possible to genotype a large number of rats simultaneously for multiple loci. These B1-RDA markers were polymorphic between two given inbred strains of rat at frequencies between 30% and 70%. This is the first report on the isolation of B1-RDA markers among inbred strains of rats.

摘要

基因抑制因子、修饰因子和数量性状基因座(QTL)的定位需要能够对大量个体进行高效且低成本基因分型的遗传标记。为了分离适用于此目的的大鼠遗传标记,使用以B1重复序列作为引物通过PCR制备的扩增子(B1-扩增子)进行了代表性差异分析(RDA)。总共通过五轮RDA分离出48个多态性DNA片段,将从ACI/N(ACI)大鼠制备的B1-扩增子与从BUF/Nac(BUF)大鼠制备的B1-扩增子相减,反之亦然。所有检测到的多态性片段与从ACI、BUF及其F2后代制备的B1-扩增子呈现“存在或缺失”多态性,并且每个片段都进行了连锁定位。将扩增子高密度点样到滤膜上,并使滤膜与这些B1-RDA标记杂交,从而能够同时对大量大鼠的多个基因座进行基因分型。这些B1-RDA标记在两种给定的大鼠近交系之间的多态性频率在30%至70%之间。这是关于在大鼠近交系中分离B1-RDA标记的首次报道。

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