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Application of High-Resolution Melting for Genotyping Bovine Mitochondrial DNA

机译:高分辨率熔解在牛线粒体DNA基因分型中的应用

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Recent studies have demonstrated that mitochondrial DNA (mtDNA) haplotype has a significant impact on the efficiency of bovine somatic cell nuclear transfer. Conventional methods for detecting mtDNA variations and haplotypes, such as restriction fragment length polymorphism (RFLP), temporal temperature gradient gel electrophoresis, dHPLC and sequencing, are labor intensive or expensive and have low sensitivity. High-resolution melting (HRM) analysis is a new technique for mutation detection and has the advantages of speed, cost, and accuracy. Here, we describe the genotyping of bovine mtDNA using HRM analysis. DNA samples containing mtDNA were extracted from 75 Holstein cows and subjected to rapid-cycle (<20 min) PCR of small amplicons (<120 bp) using specific primer sets. Capillaries containing the PCR products were then subjected to HRM analysis; data were acquired in 2 min and analyzed using the instrument's software. Five common bovine mtDNA single nucleotide polymorphisms were identified: 9602 G>A, 169 A>G, 166A>G with 173A>G, and 363C>G. These results agree with both sequencing and RFLP analysis. In addition, a very small amount of heteroplasmic variants (<5%) was sufficiently to be distinguished by HRM analysis that would be very useful to differentiate heteroplasmy vs. homoplasmy. HRM analysis-thus provides a new approach to genotyping bovine mtDNA sequence variations and has many advantages over other methods, including speed of analysis, cost, and accuracy. We believe this will be a valuable technique for determining the efficiency of nuclear transfer in cloned embryos and for studying maternal effects on nuclear-cytoplasm interactions.
机译:最近的研究表明,线粒体DNA(mtDNA)单倍型对牛体细胞核转移的效率有重大影响。用于检测mtDNA变异和单倍型的常规方法(如限制性片段长度多态性(RFLP),瞬时温度梯度凝胶电泳,dHPLC和测序)是劳动密集型或昂贵的且灵敏度低。高分辨率熔解(HRM)分析是一种用于突变检测的新技术,具有速度快,成本高和准确性高的优点。在这里,我们描述了使用HRM分析牛mtDNA的基因型。从75头荷斯坦奶牛中提取含有mtDNA的DNA样品,并使用特异性引物对小扩增子(<120 bp)进行快速循环(<20分钟)PCR。然后将含有PCR产物的毛细管进行HRM分析;在2分钟内获取数据并使用仪器的软件进行分析。鉴定了五个常见的牛mtDNA单核苷酸多态性:9602 G> A,169 A> G,166A> G,其中173A> G和363C> G。这些结果与测序和RFLP分析一致。此外,非常少量的异质变体(<5%)足以通过HRM分析加以区分,这对于区分异质性还是同质性非常有用。因此,HRM分析提供了一种对牛mtDNA序列变异进行基因分型的新方法,与其他方法相比,具有许多优势,包括分析速度,成本和准确性。我们相信这将是确定克隆胚胎中核转移效率和研究母体对核质相互作用的有价值的技术。

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