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The utility of high-resolution melting analysis of SNP nucleated PCR amplicons-an MLST based Staphylococcus aureus typing scheme

机译:SNP有核PCR扩增子的高分辨率熔解分析的实用性-基于MLST的金黄色葡萄球菌分型方案

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摘要

High resolution melting (HRM) analysis is gaining prominence as a method for discriminating DNA sequence variants. Its advantage is that it is performed in a real-time PCR device, and the PCR amplification and HRM analysis are closed tube, and effectively single step. We have developed an HRM-based method for Staphylococcus aureus genotyping. Eight single nucleotide polymorphisms (SNPs) were derived from the S. aureus multi-locus sequence typing (MLST) database on the basis of maximized Simpson’s Index of Diversity. Only G«A, G«T, C«A, C«T SNPs were considered for inclusion, to facilitate allele discrimination by HRM. In silico experiments revealed that DNA fragments incorporating the SNPs give much higher resolving power than randomly selected fragments. It was shown that the predicted optimum fragment size for HRM analysis was 200 bp, and that other SNPs within the fragments contribute to the resolving power. Six DNA fragments ranging from 83 bp to 219 bp, incorporating the resolution optimized SNPs were designed. HRM analysis of these fragments using 94 diverse S. aureus isolates of known sequence type or clonal complex (CC) revealed that sequence variants are resolved largely in accordance with G+C content. A combination of experimental results and in silico prediction indicates that HRM analysis resolves S. aureus into 268 ‘‘melt types’’ (MelTs), and provides a Simpson’s Index of Diversity of 0.978 with respect to MLST. There is a high concordance between HRM analysis and the MLST defined CCs. We have generated a Microsoft Excel key which facilitates data interpretation and translation between MelT and MLST data. The potential of this approach for genotyping other bacterial pathogens was investigated using a computerized approach to estimate the densities of SNPs with unlinked allelic states. The MLST databases for all species tested contained abundant unlinked SNPs, thus suggesting that high resolving power is not dependent upon large numbers of SNPs.
机译:作为分辨DNA序列变异的一种方法,高分辨率熔解(HRM)分析正日益受到重视。它的优点是它是在实时PCR设备中执行的,并且PCR扩增和HRM分析是封闭的,有效的一步。我们已经开发了一种基于HRM的金黄色葡萄球菌基因分型方法。在最大化的辛普森多样性指数的基础上,从金黄色葡萄球菌多基因座序列类型(MLST)数据库中获得了八个单核苷酸多态性(SNP)。仅考虑将G«A,G«T,C«A,C«T SNP包括在内,以利于HRM识别等位基因。在计算机实验中发现,掺入SNP的DNA片段比随机选择的片段具有更高的分辨能力。结果表明,HRM分析的预测最佳片段大小为200 bp,片段中的其他SNP有助于分辨能力。设计了六个DNA片段,范围从83 bp到219 bp,并结合了分辨率优化的SNP。使用已知序列类型或克隆复合物(CC)的94种不同的金黄色葡萄球菌分离物对这些片段进行HRM分析,结果表明,序列变异很大程度上取决于G + C含量。实验结果和计算机模拟的结合表明,HRM分析将金黄色葡萄球菌解析为268种“熔体类型”(MelTs),相对于MLST,辛普森多样性指数为0.978。 HRM分析与MLST定义的CC之间具有高度的一致性。我们已经生成了一个Microsoft Excel密钥,该密钥便于在MelT和MLST数据之间进行数据解释和转换。使用计算机化方法评估具有未关联等位基因状态的SNP的密度,研究了该方法对其他细菌病原体进行基因分型的潜力。所测所有物种的MLST数据库均包含大量未连接的SNP,因此表明高分辨力不依赖于大量SNP。

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