Identification, characterization, and utilization of genome-wide simple sequence repeats to identify a QTL for acidity in apple

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Abstract

Background: Apple is an economically important fruit crop worldwide. Developing a genetic linkage map is a critical step towards mapping and cloning of genes responsible for important horticultural traits in apple. To facilitate linkage map construction, we surveyed and characterized the distribution and frequency of perfect microsatellites in assembled contig sequences of the apple genome.Results: A total of 28,538 SSRs have been identified in the apple genome, with an overall density of 40.8 SSRs per Mb. Di-nucleotide repeats are the most frequent microsatellites in the apple genome, accounting for 71.9% of all microsatellites. AT/TA repeats are the most frequent in genomic regions, accounting for 38.3% of all the G-SSRs, while AG/GA dimers prevail in transcribed sequences, and account for 59.4% of all EST-SSRs. A total set of 310 SSRs is selected to amplify eight apple genotypes. Of these, 245 (79.0%) are found to be polymorphic among cultivars and wild species tested. AG/GA motifs in genomic regions have detected more alleles and higher PIC values than AT/TA or AC/CA motifs. Moreover, AG/GA repeats are more variable than any other dimers in apple, and should be preferentially selected for studies, such as genetic diversity and linkage map construction. A total of 54 newly developed apple SSRs have been genetically mapped. Interestingly, clustering of markers with distorted segregation is observed on linkage groups 1, 2, 10, 15, and 16. A QTL responsible for malic acid content of apple fruits is detected on linkage group 8, and accounts for ~13.5% of the observed phenotypic variation.Conclusions: This study demonstrates that di-nucleotide repeats are prevalent in the apple genome and that AT/TA and AG/GA repeats are the most frequent in genomic and transcribed sequences of apple, respectively. All SSR motifs identified in this study as well as those newly mapped SSRs will serve as valuable resources for pursuing apple genetic studies, aiding the apple breeding community in marker-assisted breeding, and for performing comparative genomic studies in Rosaceae. © 2012 Zhang et al.; licensee BioMed Central Ltd.

Figures

  • Table 1 Composition and length distribution of major SSR types in the apple genome
  • Table 2 Distribution of SSR types in coding DNA sequences (CDSs), untranslated regions (UTRs), and genomic DNA of the apple genome
  • Figure 1 Distribution of dimeric SSRs in genomic DNA (A) and transcribed sequences (B) of the apple genome
  • Table 3 Average allele numbers and PIC values of SSRs in eight apple genotypes
  • Figure 2 SSR-based genetic map of apple. M: male parent (cv. ‘Golden Delicious’), F: female parent (cv. ‘Jonathan’), and LG: linkage map. The consensus map is shown in centre, and distances shown in the maps are measured in centimorgans (cM). The number of linkage groups corresponds to the number of the haploid chromosomes of the draft apple genome sequence [8]. Segregation-distorted markers clustered within the chromosomal region are indicated in gray.

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APA

Zhang, Q., Ma, B., Li, H., Chang, Y., Han, Y., Li, J., … Han, Y. (2012). Identification, characterization, and utilization of genome-wide simple sequence repeats to identify a QTL for acidity in apple. BMC Genomics, 13(1). https://doi.org/10.1186/1471-2164-13-537

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