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作者	单位
严俊，杨足君，程剑平	（1．贵州大学生命科学院，贵州贵阳 550025； 2. 贵州大学农学院，贵州贵阳 550025； 3．海法大学进化研究所,以色列海法 31905； 4．电子科技大学生命科学与技术学院，四川成都 610054）

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中文摘要:

为开发与野生二粒小麦抗条锈病基因YrH52紧密连锁的分子标记，并为该基因的克隆及应用奠定基础，运用RGA (Resistance gene analog) 分子标记法，以 YrH52定位作图F₂群体形成的F₄抗性和感病基因池（Gene pool）及其亲本（抗病材料H52与感病材料Ldn）进行多态性筛选分析，共获得17个RGA分子标记。使用已有的遗传图并进行MultiPoint分析，构建了由与抗性（H）和感病(L) 两个亲本对应的显性位点组成的两个遗传图，即H遗传图和L遗传图。在H图中， YrH52与10个RGA标记，即 X_uhw3, X_uhw17, X_uhw18, X_uhw23, X_uhw36, X_uhw38, X_uhw46, X_uhw59, X_uhw62 和 X_uhw73 紧密连锁, 其中 X_uhw23 标记为共显性分子标记，连锁距离为1.0 cM。在L图中，发现 X_uhw57, X_uhw68, X_uhw189, X_uhw192及其 X_uhw23与 YrH52 相聚成簇（Cluster）。本研究结果说明RGA分子标记结合集群分离分析法（Bulked segregant analysis，BSA）是一种快速开发与小麦抗病基因紧密连锁标记的有效方法，对小麦抗条锈病分子育种和抗病基因的克隆具有促进作用。

英文摘要:

The wheat stripe rust resistance geneYrH52, derived from wild emmer wheat,Triticum dicoccoides, was previously mapped on chromosome 1BS.The aim of the present study was to develop resistance gene analog (RGA) markers linked toYrH52 for future marker assisted selection in wheat and cloning of the resistance geneYrH52.The bulked segregate analysis (BSA) was used to screen DNA pools of resistant vs.susceptible progenies, and 17 RGA markers linked toYrH52 were obtained.Two versions of genetic maps were constructed with skeleton and added markers by MultiPoint based on the previous linkage map of T.dicoccoides, respectively.As added markers in the H version map, theYrH52 and 10 RGA markers (X_uhw3, X_uhw17, X_uhw18, X_uhw23, X_uhw36, X_uhw38, X_uhw46, X_uhw59, X_uhw62 and X_uhw73) were linked tightly together within genetic distance of 1.0 cM.In the L version map, four RGA markers, X_uhw57, X_uhw68, X_uhw189, X_uhw192 and also X_uhw23 were clustered withYrH52.These results demonstrate the RGA sequences combination with BSA, was a useful method for rapidly generating markers tightly linked to resistance loci in wheat.The RGA approach will greatly benefit the marker assisted selection in wheat and cloning of the resistance geneYrH52.

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