2016
DOI: 10.1007/s00122-016-2720-4
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A saturated SNP linkage map for the orange wheat blossom midge resistance gene Sm1

Abstract: SNP markers were developed for the OWBM resistance gene Sm1 that will be useful for MAS. The wheat Sm1 region is collinear with an inverted syntenic interval in B. distachyon. Orange wheat blossom midge (OWBM, Sitodiplosis mosellana Géhin) is an important insect pest of wheat (Triticum aestivum) in many growing regions. Sm1 is the only described OWBM resistance gene and is the foundation of managing OWBM through host genetics. Sm1 was previously mapped to wheat chromosome arm 2BS relative to simple sequence re… Show more

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Cited by 18 publications
(13 citation statements)
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“…3a). Sm1 is the only gene in wheat known to provide resistance to OWBM 6 . CDC Landmark, Robigus and Paragon are all resistant to the OWBM, and all three carry the same 7.3-Mb haplotype within the Sm1 locus on chromosome 2B (Fig.…”
Section: Haplotype-based Gene Mappingmentioning
confidence: 99%
See 3 more Smart Citations
“…3a). Sm1 is the only gene in wheat known to provide resistance to OWBM 6 . CDC Landmark, Robigus and Paragon are all resistant to the OWBM, and all three carry the same 7.3-Mb haplotype within the Sm1 locus on chromosome 2B (Fig.…”
Section: Haplotype-based Gene Mappingmentioning
confidence: 99%
“…Characterization of Sm1. Sm1-linked markers 6 were located in RQAs using BLAST v.2.8.0. Two high-resolution mapping populations were developed, 99B60-EJ2D/Thatcher and 99B60-EJ2G/Infinity.…”
Section: Articlementioning
confidence: 99%
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“…Marker saturation in the vicinity of the target resistance gene is a critical step for mapped-based or positional cloning of R-genes which results in the development of diagnostic markers [20]. RGAs-based marker development strategies have been successfully applied for the development of diagnostic markers for orange wheat blossom midge and wheat stem rust resistance genes [21, 22]. This strategy involves four iterative steps: (1) identification of genome-wide RGAs, (2) identification of potential RGA candidates in the vicinity of the target resistance gene using comparative genomics analysis, (3) design of SNP markers for candidate RGAs, and (4) marker evaluation using biparental genetic populations and/or association panels.…”
Section: Introductionmentioning
confidence: 99%