Transcriptome sequencing for high throughput SNP development and genetic mapping in Pea

被引:79
|
作者
Duarte, Jorge [1 ]
Riviere, Nathalie [1 ]
Baranger, Alain [2 ]
Aubert, Gregoire [4 ]
Burstin, Judith [4 ]
Cornet, Laurent [1 ]
Lavaud, Clement [2 ]
Lejeune-Henaut, Isabelle [5 ]
Martinant, Jean-Pierre [3 ]
Pichon, Jean-Philippe [1 ]
Pilet-Nayel, Marie-Laure [2 ]
Boutet, Gilles [2 ]
机构
[1] Biogemma, F-63720 Chappes, France
[2] INRA, IGEPP, UMR 1349, F-35653 Le Rheu, France
[3] Limagrain Europe, Ctr Rech, F-63720 Chappes, France
[4] INRA, UMR Agroecol 1347, F-21065 Dijon, France
[5] INRA, SADV, UMR 1281, F-80203 Peronne, France
来源
BMC GENOMICS | 2014年 / 15卷
关键词
Pisum sativum; Medicago truncatula; Next generation sequencing; Genetic diversity; Composite genetic map; Synteny; Marker assisted selection; SINGLE-NUCLEOTIDE POLYMORPHISM; QUANTITATIVE TRAIT LOCI; PISUM-SATIVUM L; PARTIAL RESISTANCE; CANDIDATE GENES; FIELD PEA; MYCOSPHAERELLA-PINODES; APHANOMYCES-EUTEICHES; MEDICAGO-TRUNCATULA; LINKAGE MAP;
D O I
10.1186/1471-2164-15-126
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
Background: Pea has a complex genome of 4.3 Gb for which only limited genomic resources are available to date. Although SNP markers are now highly valuable for research and modern breeding, only a few are described and used in pea for genetic diversity and linkage analysis. Results: We developed a large resource by cDNA sequencing of 8 genotypes representative of modern breeding material using the Roche 454 technology, combining both long reads (400 bp) and high coverage (3.8 million reads, reaching a total of 1,369 megabases). Sequencing data were assembled and generated a 68 K unigene set, from which 41 K were annotated from their best blast hit against the model species Medicago truncatula. Annotated contigs showed an even distribution along M. truncatula pseudochromosomes, suggesting a good representation of the pea genome. 10 K pea contigs were found to be polymorphic among the genetic material surveyed, corresponding to 35 K SNPs. We validated a subset of 1538 SNPs through the GoldenGate assay, proving their ability to structure a diversity panel of breeding germplasm. Among them, 1340 were genetically mapped and used to build a new consensus map comprising a total of 2070 markers. Based on blast analysis, we could establish 1252 bridges between our pea consensus map and the pseudochromosomes of M. truncatula, which provides new insight on synteny between the two species. Conclusions: Our approach created significant new resources in pea, i.e. the most comprehensive genetic map to date tightly linked to the model species M. truncatula and a large SNP resource for both academic research and breeding.
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页数:15
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