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首页> 外文期刊>Horticulture,Environment,and Biotechnology >Development of SNP markers for marker-assisted breeding in Chinese cabbage using Fluidigm genotyping assays
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Development of SNP markers for marker-assisted breeding in Chinese cabbage using Fluidigm genotyping assays

机译:使用Fluidigm基因分型测定的大白菜中标记辅助育种的SNP标记

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Traditional breeding methods usually involve field tests carried out by experienced breeders. However, such methods are costly and time-consuming. Recently, with the development of Next-Generation Sequencing (NGS) technology, molecular markers are being utilized for selection processes in breeding. To implement a high-throughput system using molecular markers in Chinese cabbage (Brassica rapa subsp. pekinensis) breeding, we developed single nucleotide polymorphism (SNP) marker sets for background selection and testing F-1 purity using Fluidigm genotyping assays. SNPs were generated using NGS technology on 209 varieties of Chinese cabbage collected from around the world. Those with minor allele frequency >= 5% and polymorphism information content >= 0.3 were screened, and then based on the physical distribution among the 10 chromosomes, 177 SNPs were selected and synthesized for testing. To obtain marker sets with high selection efficiency, we tested 192 SNPs on 45 types of inbred lines and 29 types of F-1 hybrids. Among the 192 SNPs, we selected 96 markers sets for background selection and 24 marker sets for F-1 purity testing according to the following criteria; the genotype of the parents was homozygous, and the F-1 follows the parents' genotypes. These SNP sets are suitable for high-throughput systems using the 96.96 and 192.24 integrated fluidic circuit platforms of Fluidigm genotyping assays. These SNP marker sets are not only efficient for selecting of early fixed lines as background selection but are also useful for testing the purity of F-1 hybrids.
机译:传统育种方法通常涉及经验丰富的育种者进行的现场测试。然而,这些方法昂贵且耗时。最近,随着下一代测序(NGS)技术的发展,分子标记用于育种过程中的选择方法。利用大白菜(Brassica Rapa Subsp.Pekinensis)繁殖的分子标记实施高通量系统,我们开发了用于背景选择的单核苷酸多态性(SNP)标记组,并使用Fluidigm基因分型测定测试F-1纯度。在来自世界各地的209种大白菜中,使用NGS技术产生了SNP。具有次要等位基因频率> = 5%的那些,并且筛选多态性信息含量> = 0.3,然后基于10染色体中的物理分布,选择177个SNP并合成测试。为了获得具有高选择效率的标记集,我们在45种自交系和29种F-1杂种类型中测试了192个SNP。在192个SNP中,我们选择了96个标记为背景选择和24个标记组,用于根据以下标准进行F-1纯度测试;父母的基因型是纯合的,F-1跟随父母的基因型。这些SNP组适用于使用96.96和192.24综合流体基因分型测定的高通量系统。这些SNP标记集不仅有效地选择早期的固定线作为背景选择,而且对于测试F-1杂种的纯度也是有用的。

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