首页> 美国卫生研究院文献>Comparative and Functional Genomics >Characterization and Development of EST-SSRs by Deep Transcriptome Sequencing in Chinese Cabbage (Brassica rapa L. ssp. pekinensis)
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Characterization and Development of EST-SSRs by Deep Transcriptome Sequencing in Chinese Cabbage (Brassica rapa L. ssp. pekinensis)

机译:大白菜深转录组测序技术对EST-SSRs的鉴定和发育

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摘要

Simple sequence repeats (SSRs) are among the most important markers for population analysis and have been widely used in plant genetic mapping and molecular breeding. Expressed sequence tag-SSR (EST-SSR) markers, located in the coding regions, are potentially more efficient for QTL mapping, gene targeting, and marker-assisted breeding. In this study, we investigated 51,694 nonredundant unigenes, assembled from clean reads from deep transcriptome sequencing with a Solexa/Illumina platform, for identification and development of EST-SSRs in Chinese cabbage. In total, 10,420 EST-SSRs with over 12 bp were identified and characterized, among which 2744 EST-SSRs are new and 2317 are known ones showing polymorphism with previously reported SSRs. A total of 7877 PCR primer pairs for 1561 EST-SSR loci were designed, and primer pairs for twenty-four EST-SSRs were selected for primer evaluation. In nineteen EST-SSR loci (79.2%), amplicons were successfully generated with high quality. Seventeen (89.5%) showed polymorphism in twenty-four cultivars of Chinese cabbage. The polymorphic alleles of each polymorphic locus were sequenced, and the results showed that most polymorphisms were due to variations of SSR repeat motifs. The EST-SSRs identified and characterized in this study have important implications for developing new tools for genetics and molecular breeding in Chinese cabbage.
机译:简单序列重复(SSR)是种群分析中最重要的标记之一,已被广泛用于植物遗传图谱和分子育种。位于编码区的表达序列标签SSR(EST-SSR)标记对于QTL定位,基因靶向和标记辅助育种可能更有效。在这项研究中,我们调查了51694个非冗余单基因,这些基因是用Solexa / Illumina平台从深度转录组测序的纯净读数中组装而成的,用于鉴定和开发大白菜中的EST-SSR。总共鉴定并鉴定了10,420个12bp以上的EST-SSR,其中2744个EST-SSR是新的,已知2317个EST-SSR具有以前报道的SSR的多态性。总共设计了用于1561个EST-SSR基因座的7877个PCR引物对,并选择了二十四个EST-SSR的引物对进行引物评估。在19个EST-SSR位点(占79.2%)中,成功地高质量产生了扩增子。在二十四个白菜品种中有十七个(89.5%)表现出多态性。对每个多态性位点的多态性等位基因进行了测序,结果表明大多数多态性是由于SSR重复基序的变异所致。在这项研究中鉴定和鉴定的EST-SSRs对开发用于大白菜遗传和分子育种的新工具具有重要意义。

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