A new stripe rust resistance gene, YrH52, derived from the unique Mount Hermon population of wild emmer
wheat (Triticum dicoccoides) in Israel, was previously located on chromosome 1B. The main objectives of the
present study were to increase marker density in the vicinity of the YrH52 gene using additional microsatellite
markers, and to evaluate the accuracy and efficiency of marker-assisted selection on this gene in the F2 generation.
By means of 70 additional microsatellite primer pairs, 150 individuals of the F2 mapping population were
genotyped. Among 202 marker loci, 20 were found to be linked to the YrH52 gene with log-likelihood (LOD)
scores ranging from 3.84 to 58.82, and linkage distances ranging from 0.33 to 41.39 cM. A genetic map was
constructed of chromosome 1B, consisting of 23 markers and the YrH52 gene, with a total map length of 149.5
cM. Most of the markers were located in the region close to YrH52, which was flanked by Xgwm413 and
Xgwm273a with map distances of 1.3 and 2.7 cM, respectively. The accuracy and efficiency of marker-assisted
selection were calculated as AMAS and EMAS, respectively, for homozygous resistant genotypes of YrH52 gene
in the F2 generation. AMAS and EMAS for homozygous resistant genotypes of the YrH52 gene in the F2
generation showed linear and significant negative correlation with the map distance between marker and target
gene or between the two bracketing markers. It was concluded that the YrH52 region on chromosome 1B is
significantly more enriched by microsatellite markers than the previously published map; that a single
microsatellite marker is efficient for marker-assisted selection of homozygous resistant genotypes of YrH52 gene
in the F2 generation when the map distance is <5.0 cM; and that when two markers are used AMAS can be
dramatically improved and becomes relatively stable, whereas EMAS will not be obviously improved and will still
vary linearly with map distance.