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首页> 外文期刊>Theoretical and Applied Genetics: International Journal of Breeding Research and Cell Genetics >Rapid development of molecular markers by next-generation sequencing linked to a gene conferring phomopsis stem blight disease resistance for marker-assisted selection in lupin (Lupinus angustifolius L.) breeding.
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Rapid development of molecular markers by next-generation sequencing linked to a gene conferring phomopsis stem blight disease resistance for marker-assisted selection in lupin (Lupinus angustifolius L.) breeding.

机译:通过下一代测序技术快速开发分子标记,该测序与赋予磷光病枯萎病抗性的基因相关联,用于羽扇豆(Lupinus angustifolius L.)育种中的标记辅助选择。

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Selection for phomopsis stem blight disease (PSB) resistance is one of the key objectives in lupin (Lupinus angustifolius L.) breeding programs. A cross was made between cultivar Tanjil (resistant to PSB) and Unicrop (susceptible). The progeny was advanced into F8 recombinant inbred lines (RILs). The RIL population was phenotyped for PSB disease resistance. Twenty plants from the RIL population representing disease resistance and susceptibility was subjected to next-generation sequencing (NGS)-based restriction site-associated DNA sequencing on the NGS platform Solexa HiSeq2000, which generated 7,241 single nucleotide polymorphisms (SNPs). Thirty-three SNP markers showed the correlation between the marker genotypes and the PSB disease phenotype on the 20 representative plants, which were considered as candidate markers linked to a putative R gene for PSB resistance. Seven candidate markers were converted into sequence-specific PCR markers, which were designated as PhtjM1, PhtjM2, PhtjM3, PhtjM4, PhtjM5, PhtjM6 and PhtjM7. Linkage analysis of the disease phenotyping data and marker genotyping data on a F8 population containing 187 RILs confirmed that all the seven converted markers were associated with the putative R gene within the genetic distance of 2.1 CentiMorgan (cM). One of the PCR markers, PhtjM3, co-segregated with the R gene. The seven established PCR markers were tested in the 26 historical and current commercial cultivars released in Australia. The numbers of "false positives" (showing the resistance marker allele band but lack of the putative R gene) for each of the seven PCR markers ranged from nil to eight. Markers PhtjM4 and PhtjM7 are recommended in marker-assisted selection for PSB resistance in the Australian national lupin breeding program due to its wide applicability on breeding germplasm and close linkage to the putative R gene. The results demonstrated that application of NGS technology is a rapid and cost-effective approach in development of markers for molecular plant breeding.
机译:拟南芥枯萎病(PSB)抗性的选择是羽扇豆(Lupinus angustifolius L.)育种计划的主要目标之一。品种Tanjil(抗PSB)和Unicrop(易感)杂交。后代被推进到F8重组近交系(RIL)。对RIL人群进行PSB疾病抗性表型分析。在NGS平台Solexa HiSeq2000上,对来自RIL群体的20株代表疾病抗性和敏感性的植物进行了基于下一代测序(NGS)的限制性位点相关的DNA测序,产生了7,241个单核苷酸多态性(SNP)。 33个SNP标记在20个代表性植物上显示了标记基因型与PSB病表型之间的相关性,这被认为是与推定的PSB抗性R基因相关的候选标记。将七个候选标记转化为序列特异性PCR标记,分别称为PhtjM1,PhtjM2,PhtjM3,PhtjM4,PhtjM5,PhtjM6和PhtjM7。对包含187个RIL的F 8 群体的疾病表型数据和标记基因分型数据的连锁分析,证实了所有七个转化标记均与2.1 CentiMorgan(cM)的遗传距离内的推定R基因相关。 。 PCR标记之一PhtjM3与R基因共分离。在澳大利亚发布的26个历史和当前商业品种中测试了这七个已建立的PCR标记。七个PCR标记的每一个的“假阳性”(显示抗性标记等位基因带,但缺少推定的R基因)的数量在零到八个之间。在澳大利亚国家羽扇豆育种计划中,标记PhtjM4和PhtjM7被推荐用于PSB抗性的标记辅助选择,因为它在育种种质中具有广泛的适用性并与推定的R基因密切相关。结果表明,NGS技术的应用是开发分子植物育种标记的快速且经济高效的方法。

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