Genetic mapping and a new PCR-based marker linked to a dwarfing gene in oat (Avena sativa L.)

Author:

Zhao Jun1,Tang Xueqin12,Wight Charlene P.3,Tinker Nicholas A.3,Jiang Yunfeng1,Yan Honghai13,Ma Jian1,Lan Xiujin1,Wei Yuming1,Ren Changzhong4,Chen Guoyue1,Peng Yuanying1

Affiliation:

1. Triticeae Research Institute, Sichuan Agricultural University, Wenjiang District, 211 Huimin Road, Chengdu 611130, Sichuan, China.

2. Agricultural Bureau of Xingwen County, Yibin 644400, Sichuan, China.

3. Ottawa Research and Development Centre, Agriculture & Agri-Food Canada, Ottawa, ON K1A 0C6, Canada.

4. Baicheng Academy of Agricultural Sciences, Baicheng 137000, Jilin, China.

Abstract

Short straw is a desired trait in cultivated hexaploid oat (Avena sativa L.) for some production environments. Marker-assisted selection, a key tool for achieving this objective, is limited by a lack of mapping data and available markers. Here, bulked-segregant analysis was used to identify PCR-based markers associated with a dwarfing gene. Genetic analysis identified a monogenic dominant inheritance of one dwarfing gene from WAOAT2132, temporarily designated DwWA. A simple sequence repeat (SSR) marker (AME117) that was already available and a new codominant PCR-based marker (bi17) developed by homologous cloning in the present study were both associated with the dwarfing gene. The two markers were located 21 and 1.2 cM from DwWA, respectively. The bi17 marker was mapped to neighboring SNP markers on chromosome 18D of the oat consensus map. Since Dw6 was previously mapped on chromosome 18, and since our new marker bi17 is also diagnostic for NILs generated for Dw6, there is strong evidence that the dwarfing gene identified in WAOAT2132 is Dw6. The newly developed markers could find applications in the identification of this gene in oat germplasm and in the fine mapping or positional cloning of the gene.

Publisher

Canadian Science Publishing

Subject

Genetics,Molecular Biology,General Medicine,Biotechnology

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