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2002 | 07 | 2B |

Tytuł artykułu

Rapid genetic mapping of ESTs using SNP pyrosequencing and indel analysis

Autorzy

Warianty tytułu

Języki publikacji

EN

Abstrakty

EN
W describe an effective systematic approach to genetic mapping of cDNA clones, including those obtained from EST sequencing. The EST of interest is first partially sequenced from the 3'-end. PCR primers which bracket the 3'-UTR segment of the cDNA are designed. The corresponding gene segment is amplified from the parents of the mapping population, using primers equipped with 3'- and 5'-extensions to facilitate direct sequencing of PCR products. Comparison of the sequences obtained from the mapping parents frequently reveals single nucleotide polymorphisms or insertion / deletion polymorphisms, which can then be genotyped in a mapping population. The genotyping of SNPs is performed by pyrosequencing, a sequencing-by-synthesis method that has been used successfully in SNP diagnostics. SNP analysis of up to 96 samples, a number required to produce meaningful genetic segregation data, can be rapidly accomplished in parallel. The parental genotype of three loci, stearoyl-ACP desaturase, nucleoside-diphosphate kinase and sucrose synthetase-1 were determined by conventional sequencing, and the polymorphism so identified were scored by the pyrosequencing of 94 individuals of a maize recombinant-inbred population. These loci were successfully placed onto chromosomes 3, 7 and 9 respectively. This method is generally applicable to most plant species, which show sufficient sequence diversity in the 3'-UTR region of genes.

Wydawca

-

Rocznik

Tom

07

Numer

2B

Opis fizyczny

p.803-810,fig.

Twórcy

autor
  • DuPont Crop Genetics, Molecular Genetics Group, 1, Innovation Way, Newark, DE 19711, USA
autor

Bibliografia

  • 1. Phillips, R. L. and Vasil, I. K. (eds.). (2001) DNA-Based markers in plants. Kluver Academic Publishers, Dordrecht.
  • 2. Henry, R. J. (ed.). (2001) Plant Genotyping. The DNA fingerprinting of plants. CABI Publishing, Wallingford, Oxon, UK.
  • 3. Rafalski, A. Applications of single nucleotide polymorphisms in crop genetics. Curr. Op. Plant Biol. 5 (2002) 94-100.
  • 4. Buckler IV, E. S. and Thornsberry, J. M. Plant molecular diversity and applications to genomics. Curr. Op. Plant Biol. 5 (2002) 107-111.
  • 5. Bhattramakki, D., Dolan, M., Hanafey, M., Wineland, R., Vaske, D., Register III, J. C., Tingey, S. V. and Rafalski, A. Insertion-deletion polymorphisms in 3' regions of maize genes occur frequently and can be used as highly informative genetic markers. Plant Mol. Biol. 48 (2002) 539-547.
  • 6. Syvanen, A. C. Accessing genetic variation: genotyping single nucleotide polymorphisms. Nat. Rev. Genet. 2 (2001) 930-942.
  • 7. Ronaghi, M., Uhlen, M. and Nyren, P. A sequencing method based on real-time pyrophosphate. Science 281 (1998) 363-365.
  • 8. Ahmadian, A., Gharizadeh, B., Gustafsson, A. C., Sterky, F., Nyren, P., Uhlen, M. and Lundeberg, J. Single-nucleotide polymorphism analysis by pyrosequencing. Anal. Biochem. 280 (2000) 103-110.
  • 9. Lander, E. S., Green, P., Abrahamson, J., Barlow, A., Daly, M. J., Lincoln, S. E. and Newburg, L. Mapmaker: An interactive computer package for constructing primary linkage maps of experimental and natural populations. Genomics 1 (1987) 174-181.
  • 10. Botstein, D., White, R. L., Skolnick, M. H. and Davis, R. W. Construction of a genetic map in man using restriction fragment length polymorphisms. Am. J. Hum. Genet. 32 (1980) 314-331.
  • 11. Konieczny, A. and Ausubel, F. M. A procedure for mapping arabidopsis mutations using co-dominant ecotype-specific PCR-based markers. Plant J. 4 (1993) 403-410.

Typ dokumentu

Bibliografia

Identyfikatory

Identyfikator YADDA

bwmeta1.element.agro-article-147ee670-74b8-49a6-9c22-b741085263e2
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