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首页> 外文期刊>Comptes rendus. Biologies >Multiplex SSR-PCR approaches for semi-automated genotyping and characterization of loci linked to blast disease resistance genes in rice
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Multiplex SSR-PCR approaches for semi-automated genotyping and characterization of loci linked to blast disease resistance genes in rice

机译:多重SSR-PCR方法可对水稻中与稻瘟病抗性基因相关的基因座进行半自动基因分型和鉴定

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In the present study, 63 polymorphic microsatellite markers related to rice blast resistance genes were fluorescently labelled at the 5'-end with either 6-FAM or HEX using the G5 dye set and incorporated into a multiplex SSR-PCR for the detection of fragments using an automated system. For rice F-3 families obtained from crosses between Pongsu Seribu 2 (Malaysian blast resistant cultivar) and Mahsuri (a susceptible rice cultivar), the genotypes for 13 designated multiplex SSR panels were determined. The genotyping assays were performed using a capillary-based ABIPRISM 3100 genetic analyser. The sizes of the SSRs alleles observed in the range from 79 to 324 bp. The observed marker segregation data were analysed using the Chi(2) test. A genetic linkage map covering ten chromosomes and comprising 63 polymorphic SSR markers was constructed, and the distorted loci were localised to linkage groups. The results indicated that distorted loci are presented on eight chromosomes. (C) 2015 Academie des sciences. Published by Elsevier Masson SAS. All rights reserved.
机译:在本研究中,使用G5染料在6'FAM或HEX的5'末端用荧光标记了与稻瘟病抗性基因相关的63个多态性微卫星标记,并掺入了多重SSR-PCR中,使用以下方法检测片段自动化系统。对于从Pongsu Seribu 2(马来西亚抗病品种)和Mahsuri(易感水稻品种)之间杂交获得的水稻F-3家族,确定了13个指定的多重SSR面板的基因型。使用基于毛细管的ABIPRISM 3100遗传分析仪进行基因分型测定。观察到的SSRs等位基因的大小在79至324 bp之间。使用Chi(2)测试分析观察到的标记偏析数据。构建了涵盖10条染色体并包含63个多态性SSR标记的遗传连锁图谱,并将扭曲的基因座定位于连锁群。结果表明畸变的基因座出现在八个染色体上。 (C)2015年科学研究院。由Elsevier Masson SAS发布。版权所有。

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