Development and test of 21 multiplex PCRs composed of SSRs spanning most of the apple genome

被引:51
作者
Patocchi, A. [1 ]
Fernandez-Fernandez, F. [2 ]
Evans, K. [2 ]
Gobbin, D. [1 ]
Rezzonico, F. [1 ]
Boudichevskaia, A. [3 ]
Dunemann, F. [3 ]
Stankiewicz-Kosyl, M. [4 ]
Mathis-Jeanneteau, F. [5 ]
Durel, C. E. [5 ]
Gianfranceschi, L. [6 ]
Costa, F. [7 ]
Toller, C. [8 ]
Cova, V. [8 ]
Mott, D. [8 ]
Komjanc, M. [8 ]
Barbaro, E. [8 ]
Kodde, L. [9 ]
Rikkerink, E. [10 ]
Gessler, C. [1 ]
van de Weg, W. E. [9 ]
机构
[1] ETH, Inst Integrat Biol IBZ, Plant Pathol, CH-8092 Zurich, Switzerland
[2] E Malling Res, E Malling ME19 6BJ, Kent, England
[3] JKI, Bundesforschungsinst Kulturpflanzen, D-01326 Dresden, Germany
[4] Agr Univ Warsaw, Lab Basic Res Hort, Fac Hort & Landscape Architecture, PL-02787 Warsaw, Poland
[5] INRA, UMR Genet & Hort 1259, F-49071 Beaucouze, France
[6] Univ Milan, Dept Biomol Sci & Biotechnol, I-20133 Milan, Italy
[7] Univ Bologna, Dept Fruit Tree & Woody Plant Sci, I-40127 Bologna, Italy
[8] Ist Agr San Michele All Adige, I-38010 San Michele All Adige, Trento, Italy
[9] Plant Res Int, Dept Biodivers & Breeding, NL-6700 AA Wageningen, Netherlands
[10] Hort & Food Res Inst New Zealand Ltd, Mt Albert Res Ctr, Auckland 92169, New Zealand
关键词
SSR; Multiplex PCR; Genotyping; Malus; MICROSATELLITE MARKERS; MALUS; POLYMORPHISM; RESISTANCE; JAPANESE; QTL;
D O I
10.1007/s11295-008-0176-7
中图分类号
S7 [林业];
学科分类号
0829 ; 0907 ;
摘要
A series of 21 multiplex (MP) polymerase chain reactions containing simple sequence repeat (SSR) markers spanning most of the apple genome has been developed. Eighty-eight SSR markers, well distributed over all 17 linkage groups (LGs), have been selected. Eighty-four of them were included in 21 different MPs while four could not be included in any MPs. The 21 MPs were then used to genotype approximately 2,000 DNA samples from the European High-quality Disease-Resistant Apples for a Sustainable agriculture project. Two SSRs (CH01d03 and NZAL08) were discarded at an early stage as they did not produce stable amplifications in the MPs, while the scoring of the multilocus (ML) SSR Hi07d11 and CN44794 was too complex for large-scale genotyping. The testing of the remaining 80 SSRs over a large number of different genotypes allowed: (1) a better estimation of their level of polymorphism; as well as of (2) the size range of the alleles amplified; (3) the identification of additional unmapped loci of some ML SSRs; (4) the development of methods to assign alleles to the different loci of ML SSRs and (5) conditions at which an SSR previously described as ML would amplify alleles of a single locus to be determined. These data resulted in the selection of 75 SSRs out of the 80 that are well suited and recommended for large genotyping projects.
引用
收藏
页码:211 / 223
页数:13
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