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农学学报

农学学报 ›› 2013, Vol. 3 ›› Issue (5): 8-11.

所属专题: 小麦

• 农艺科学 作物遗传育种 生理生化 • 上一篇    下一篇

小麦优质Ax1/Ax2*和Dx5亚基的二重AS-PCR分子鉴定

孙宪印 吴科 钱兆国 米勇 牟秋焕 郭营 李斯深   

  • 收稿日期:2013-03-19 修回日期:2013-04-02 出版日期:2013-05-20 发布日期:2013-05-20
  • 基金资助:
    国家现代农业产业技术体系项目;泰安市科技发展计划项目

Identification of Ax1/Ax2* and Dx5 Subunit of Wheat HMW Glutenin By Duplex AS-PCR

  • Received:2013-03-19 Revised:2013-04-02 Online:2013-05-20 Published:2013-05-20

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摘要: 为了提高小麦Glu-A1位点Ax1/Ax2*亚基和Glu-D1位点Dx5亚基分子标记鉴定效率,方便小麦分子水平的辅助选择及品种评价,建立了小麦高分子量谷蛋白Ax1/Ax2*亚基及Dx5亚基基因的二重AS-PCR反应体系。结果表明,PCR鉴定结果与SDS-PAGE电泳结果一致。利用建立的二重AS-PCR稳定扩增体系鉴定了21份外引小麦品种系的谷蛋白Glu-A1及Glu-D1位点,有7个品种扩增出1500 bp特异片段,表明具有Ax1/Ax2*亚基;有11个品种扩增出478 bp特异片段,表明具有Dx5亚基;小麦优质Ax1/Ax2*亚基和Dx5亚基出现百分率分别为33.3%和52.4%。该反应体系扩增稳定,可同时鉴定Ax1/Ax2*亚基及Dx5亚基,适用于优质小麦新品种的辅助选择。

关键词: 河北省, 河北省, 蛴螬, 金针虫, 地下害虫, 农作物田

Abstract: It has been demonstrated that Ax1/Ax2* and Dx5 are normally associated with wheat flour superior end-use quality, especially dough strength. This paper was designed to improve the molecular marker identification efficiency by the duplex allele-specific polymerase chain reaction (Duplex AS-PCR). In distinguishing the high molecular weight glutenin subunit, the results of sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) proved that the established duplex AS-PCR was credible. The genes of Ax1/Ax2* and Dx5 could be identified simultaneously in this polymerase chain reaction system. The presence of 1500 bp and 478 bp bands showed Ax1/Ax2* and Dx5 genes, respectively. A total of 21 wheat cultivars abroad were tested by the duplex allele-specific PCR-based assay and the frequencies of Ax1/Ax2* and Dx5 were 33.3% and 52.4%, respectively. In conclusion, the amplification reaction system was stable, and it could be used to simultaneously identify Ax1/Ax2* and Dx5 subunits, so it would be very helpful for marker-assisted selection of new wheat varieties with high quality.