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首页> 外文期刊>Breeding science >Selection criteria for SNP loci to maximize robustness of high-resolution melting analysis for plant breeding
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Selection criteria for SNP loci to maximize robustness of high-resolution melting analysis for plant breeding

机译:SNP基因座的选择标准最大限度地提高植物育种高分辨率熔化分析的鲁棒性

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摘要

DNA markers are useful for identifying genes and developing new genetic materials for breeding and genetic research. High-resolution melting (HRM) analysis can detect a single nucleotide polymorphism (SNP) in two polymerase chain reaction (PCR) fragments as a melting temperature (Tm) difference without additional experimental steps, such as gel electrophoresis. To design a method for developing reliable HRM markers that discriminate between homozygous alleles containing SNPs, we tested new evaluation indexes related to the thermodynamics of double-stranded DNA to find one that maximizes the difference in Tm values between PCR fragments. We found that differences in the change in Gibbs free energy (Delta G degrees) correlated with actual differences in Tm values. Optimization of the nearest neighboring nucleotide (NNN) of a SNP by nucleotide substitution in the primer and reducing the size of the PCR fragment both enlarged the actual differences in Tm. The genetic DNA markers we developed by NNN substitution, termed NNNs-HRM markers, could be precisely mapped within soybean chromosomes by linkage analysis. We developed a Perl script pipeline to enable the automatic design of a massive number of NNNs-HRM markers; these scripts are freely available and would be useful for practical breeding programs for other plant species.
机译:DNA标记可用于鉴定基因和开发用于育种和遗传研究的新型遗传物质。高分辨率熔融(HRM)分析可以在两种聚合酶链反应(PCR)片段中检测单个核苷酸多态性(SNP),作为熔化温度(TM)差,而无需额外的实验步骤,例如凝胶电泳。设计一种用于开发可靠的HRM标记的方法,以区分含有SNP的纯合等位基因,我们测试了与双链DNA热力学相关的新评估指标,以找到一种最大化PCR片段之间的TM值差异的索引。我们发现Gibbs自由能量(Delta G度)的变化的差异与TM值的实际差异相关。底漆中核苷酸取代的核苷酸取代并降低PCR片段的尺寸的优化均扩大了TM的实际差异。我们通过NNNS-HRM标记替代的NNNS-HRM标记开发的遗传DNA标志物可以通过连杆分析精确地映射在大豆染色体内。我们开发了一个Perl脚本流水线,以启用大量NNNS-HRM标记的自动设计;这些脚本可自由可用,可用于其他植物物种的实用育种计划。

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