De novo assembly and characterization of the carrot transcriptome reveals novel genes, new markers, and genetic diversity

被引:152
作者
Iorizzo, Massimo [1 ]
Senalik, Douglas A. [1 ,2 ]
Grzebelus, Dariusz [3 ]
Bowman, Megan [1 ]
Cavagnaro, Pablo F. [4 ,5 ]
Matvienko, Marta [7 ]
Ashrafi, Hamid [6 ]
Van Deynze, Allen [6 ]
Simon, Philipp W. [1 ,2 ]
机构
[1] Univ Wisconsin, Dept Hort, Madison, WI 53706 USA
[2] Univ Wisconsin, USDA ARS, Vegetable Crops Res Unit, Madison, WI 53706 USA
[3] Agr Univ Krakow, Dept Genet Plant Breeding & Seed Sci, PL-31425 Krakow, Poland
[4] Consejo Nacl Invest Cient & Tecn, Mendoza, Argentina
[5] INTA EEA La Consulta, Mendoza, Argentina
[6] Univ Calif Davis, Seed Biotechnol Ctr, Davis, CA 95616 USA
[7] Univ Calif Davis, Genome Ctr, Davis, CA 95616 USA
关键词
INVERTED-REPEAT ELEMENTS; DAUCUS-CAROTA L; TRANSPOSABLE ELEMENTS; SNP DISCOVERY; SSR-MARKERS; SEQUENCE; ANNOTATION; FAMILY; EST; SUPERFAMILY;
D O I
10.1186/1471-2164-12-389
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: Among next generation sequence technologies, platforms such as Illumina and SOLiD produce short reads but with higher coverage and lower cost per sequenced nucleotide than 454 or Sanger. A challenge now is to develop efficient strategies to use short-read length platforms for de novo assembly and marker development. The scope of this study was to develop a de novo assembly of carrot ESTs from multiple genotypes using the Illumina platform, and to identify polymorphisms. Results: A de novo assembly of transcriptome sequence from four genetic backgrounds produced 58,751 contigs and singletons. Over 50% of these assembled sequences were annotated allowing detection of transposable elements and new carrot anthocyanin genes. Presence of multiple genetic backgrounds in our assembly allowed the identification of 114 computationally polymorphic SSRs, and 20,058 SNPs at a depth of coverage of 20x or more. Polymorphisms were predominantly between inbred lines except for the cultivated x wild RIL pool which had high intra-sample polymorphism. About 90% and 88% of tested SSR and SNP primers amplified a product, of which 70% and 46%, respectively, were of the expected size. Out of verified SSR and SNP markers 84% and 82% were polymorphic. About 25% of SNPs genotyped were polymorphic in two diverse mapping populations. Conclusions: This study confirmed the potential of short read platforms for de novo EST assembly and identification of genetic polymorphisms in carrot. In addition we produced the first large-scale transcriptome of carrot, a species lacking genomic resources.
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页数:14
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