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Nucleotide-binding site (NBS) profiling of genetic diversity in durum wheat.

机译:硬粒小麦遗传多样性的核苷酸结合位点(NBS)分析。

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摘要

Molecular markers are effective tools to investigate genetic diversity for resistance to pathogens. NBS (nucleotide-binding site) profiling is a PCR (polymerase chain reaction)-based approach to studying genetic variability that specifically targets chromosome regions containing R-genes and R-gene analogues. We used NBS profiling to measure genetic diversity among 58 accessions of durum wheat. Mean polymorphism rates detected using MseI and AluI as restriction enzymes were 34 and 22%, respectively. The mean number of polymorphisms per enzyme-primer combination was equal to 23.8+or-5.9, ranging from 13 to 31 polymorphic bands. In total, 96 markers over 190 indicated a good capacity to discriminate between accessions (the polymorphic index content ranging from 0.30 to 0.50). The results obtained with NBS profiling were compared with simple sequence repeat (SSR) and amplified fragment length polymorphism (AFLP) data of the same set of accessions. The genetic distances computed with 190 NBS profiling markers were in close agreement with those obtained with AFLP and SSR markers (r=0.73 and 0.76, respectively). Our results indicate that NBS profiling provides an effective means to investigate genetic diversity in durum wheat..
机译:分子标记是研究遗传多样性对病原体抗性的有效工具。 NBS(核苷酸结合位点)分析是一种基于PCR(聚合酶链反应)的方法,用于研究遗传变异性,该变异性专门针对包含R基因和R基因类似物的染色体区域。我们使用NBS分析对58个硬粒小麦品种的遗传多样性进行了测量。使用MseI和AluI作为限制酶检测到的平均多态性率分别为34%和22%。每个酶-引物组合的平均多态性数目等于23.8+或-5.9,范围为13至31个多态性条带。总共有190个以上的96个标记表明了对种质进行区分的良好能力(多态性指数含量在0.30至0.50之间)。将使用NBS分析获得的结果与同一保藏组的简单序列重复(SSR)和扩增片段长度多态性(AFLP)数据进行比较。用190个NBS分布标记计算的遗传距离与用AFLP和SSR标记获得的遗传距离非常接近(分别为r = 0.73和0.76)。我们的结果表明,国家统计局的概况分析提供了一种有效的手段来研究硬粒小麦的遗传多样性。

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