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利用聚合酶链反应和序列特异性DNA引物检测黑麦2R染色体

Detection of rye chromosome 2R using the polymerase chain reaction and sequence-specific DNA primers.

作者信息

Lee J H, Graybosch R A, Lee D J

机构信息

Department of Agronomy, University of Nebraska, Lincoln 68583.

出版信息

Genome. 1994 Feb;37(1):19-22. doi: 10.1139/g94-003.

Abstract

Sequences derived from a rye gamma secalin gene were used as primers in polymerase chain reactions using DNA obtained from a series of wheat and triticale genetic stocks. A 473-bp fragment, the predicted size based on the distance between the selected primers, was found only in rye, triticales, and wheat lines carrying rye chromosome 2RS. Use of triticale lines with various wheat chromosome substitutions confirmed the chromosomal origin of the rye-specific marker. The presence of the 473-bp PCR product was always associated with the production of 75K secalins in grain samples. Thus, the primer sequences, and the clone of origin (pSC503), were both derived from the SEC-2 locus of rye chromosome 2RS.

摘要

来自黑麦γ-黑麦碱基因的序列被用作聚合酶链反应的引物,该反应使用从一系列小麦和小黑麦遗传材料中获得的DNA。一个473bp的片段,其大小是根据所选引物之间的距离预测的,仅在黑麦、小黑麦以及携带黑麦2RS染色体的小麦品系中发现。使用具有各种小麦染色体替换的小黑麦品系证实了黑麦特异性标记的染色体起源。473bp PCR产物的存在总是与谷物样品中75K黑麦碱的产生相关。因此,引物序列和原始克隆(pSC503)均来自黑麦2RS染色体的SEC-2位点。

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