The use of a modified bulk segregant analysis to identify a molecular marker linked to a scab resistance gene in apple

被引:0
|
作者
Hong Y. Yang
Schuyler S. Korban
Jutta Krüger
Hanna Schmidt
机构
[1] University of Illinois,Department of Natural Resources and Environmental Sciences
[2] Institute for Ornamental Plant Breeding,Federal Centre for Breeding Research on Cultivated Plants
来源
Euphytica | 1997年 / 94卷
关键词
Malus; apple; apple scab resistance; Venturia inaequalis; V; gene; bulked segregant analysis; RAPDs; SCAR;
D O I
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中图分类号
学科分类号
摘要
Almost two-hundred random sequence decamer-primers were used to screen a pair of bulked samples and the donor parent Malus floribunda clone 821 for markers linked to the Vf gene conferring resistance to apple scab (Venturia inaequalis (Cke.) Wint.). A single primer was identified which generated a PCR fragment, OPK16/1300, from the donor parent M. floribunda clone 821 and the scab-resistant selections/cultivars bulk, but not from the scab-susceptible recurrent parent bulk. Co-segregation analysis using a segregating apple progeny and polymorphism analysis of individual scab-resistant Coop selections/cultivars confirmed that this marker was linked to the scab-resistance gene Vf with a recombination frequency of 4.3%. OPK16/1300 was then cloned and sequenced. Sequence-specific primers of 25 oligonucleotides based on the marker were synthesized, and used in turn to screen M. floribunda clone 821, scab-susceptible apple cultivars, scab-resistant apple cultivars, and scab-resistant Coop selections. A pair of sequence-specific primers of clone OPK16/1300 amplified a distinct single band of the same size as the RAPD clone. Thus, a sequence characterized amplified region (SCAR) marker was developed which can be used to identify polymorphisms of OPK16/1300 based on the presence or absence of a single band.
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页码:175 / 182
页数:7
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