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首页> 外文期刊>Theoretical and Applied Genetics: International Journal of Breeding Research and Cell Genetics >Identification, characterization and utilization of EST-derived genic microsatellite markers for genome analyses of coffee and related species
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Identification, characterization and utilization of EST-derived genic microsatellite markers for genome analyses of coffee and related species

机译:鉴定,表征和利用EST衍生基因微卫星标记进行咖啡和相关物种的基因组分析

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摘要

Genic microsatellites or EST-SSRs derived from expressed sequence tags (ESTs) are desired because these are inexpensive to develop, represent transcribed genes, and often a putative function can be assigned to them. In this study we investigated 2,553 coffee ESTs (461 from the public domain and 2,092 in-house generated ESTs) for identification and development of genic microsatellite markers. Of these, 2,458 ESTs (all > 100 bp in size) were searched for SSRs using MISA-search module followed by stackPACK clustering that revealed a total of 425 microsatellites in 331 (13.5%) non-redundant ESTs/consensus sequences suggesting an approximate frequency of 1 SSR/2.16 kb of the analysed coffee transcriptome. Identified microsatellites mainly comprised of di-/tri-nucleotide repeats, of which repeat motifs AG and AAG were the most abundant. A total of 224 primer pairs could be designed from the non-redundant SSR-positive ESTs (excluding those with only mononucleotide repeats) for possible use as potential genic markers. Of this set, a total of 24 (10%) primer pairs were tested and 18 could be validated as usable markers. Sixteen of these markers revealed moderate to high polymorphism information content (PIC) across 23 genotypes of C. arabica and C. canephora, while 2 markers were found to be monomorphic. All the markers also showed robust cross-species amplifications across 14 Coffea and 4 Psilanthus species. The apparent broad cross-species/genera transferability was further confirmed by cloning and sequencing of the amplified alleles. Thus, the study provides an insight about the frequency and distribution of SSRs in coffee transcriptome, and also demonstrates the successful development of genic-SSRs. It is expected that the potential markers described here would add to the repertoire of DNA markers needed for genetic studies in cultivated coffee and also related taxa that constitute the important secondary genepool for coffee improvement.
机译:期望从表达的序列标签(EST)衍生出的基因微卫星或EST-SSR,因为它们开发成本低,代表转录的基因,并且通常可以为它们分配推定的功能。在这项研究中,我们调查了2553个咖啡EST(来自公共领域的461个和内部生成的2092个EST),用于鉴定和开发基因微卫星标记。其中,使用MISA搜索模块搜索了2458个EST(大小均大于100 bp)的SSR,然后进行stackPACK聚类,发现331个非冗余EST /共有序列中共有425个微卫星,提示频率近似1 SSR / 2.16 kb的分析咖啡转录组。鉴定出的主要由二核苷酸/三核苷酸重复序列组成的微卫星,其中重复基序AG和AAG最丰富。可以从非冗余SSR阳性EST(不包括仅具有单核苷酸重复序列的EST)设计出总共224个引物对,以用作潜在的基因标记。在这一组中,总共测试了24个(10%)引物对,其中18个可以作为可用标记进行验证。这些标记中的十六个显示出23种阿拉伯咖啡和canephora基因型的中等至高多态性信息含量(PIC),而发现2个标记是单态的。所有标记物还显示出在14个Coffea和4个Psilanthus物种中强大的跨物种扩增。通过扩增的等位基因的克隆和测序进一步证实了明显的跨物种/属转移性。因此,该研究提供了关于咖啡转录组中SSR频率和分布的见解,并证明了基因SSR的成功开发。可以预期,此处描述的潜在标记将增加栽培咖啡和相关分类单元的遗传研究所需的DNA标记,这些构成了咖啡改良的重要二级基因库。

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