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Novel DNA Chip Based on a Modified DigiTag2 Assay for High-Throughput Species Identification and Genotyping of Mycobacterium tuberculosis Complex Isolates

机译:基于改良的DigiTag2分析的新型DNA芯片用于高通量物种鉴定和结核分枝杆菌复合物分离物的基因分型

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摘要

A multipurpose high-throughput genotyping tool for the assessment of recent epidemiological data and evolutional pattern in Mycobacterium tuberculosis complex (MTBC) clinical isolates was developed in this study. To facilitate processing, 51 highly informative single nucleotide polymorphisms (SNPs) were selected for discriminating the clinically most relevant MTBC species and genotyping M. tuberculosis into its principle genetic groups (PGGs) and SNP cluster groups (SCGs). Because of the high flexibility of the DigiTag2 assay, the identical protocol and DNA array containing the identical set of probes were applied to the highly GC-rich mycobacterial genome. The specific primers with multiplex amplification and hybridization conditions based on the DigiTag2 principle were optimized and evaluated with 14 MTBC reference strains, 4 nontuberculous mycobacteria (NTM) isolates, and 322 characterized M. tuberculosis clinical isolates. The DNA chip that was developed revealed a 99.85% call rate, a 100% conversion rate, and 99.75% reproducibility. For the accuracy rate, 98.94% of positive calls were consistent with previous molecular characterizations. Our cost-effective technology was capable of simultaneously identifying the MTBC species and the genotypes of 96 M. tuberculosis clinical isolates within 6 h using only simple instruments, such as a thermal cycler, a hybridization oven, and a DNA chip scanner, and less technician skill was required than for other techniques. We demonstrate this approach's potential as a simple, flexible, and rapid tool for providing clearer information regarding circulating MTBC isolates.
机译:在这项研究中开发了一种多功能的高通量基因分型工具,用于评估结核分枝杆菌复合体(MTBC)临床分离株的近期流行病学数据和进化模式。为了促进加工,选择了51个高度信息化的单核苷酸多态性(SNP),以区分临床上最相关的MTBC物种,并对结核分枝杆菌进行基因分型,使其成为主要的遗传组(PGG)和SNP簇组(SCG)。由于DigiTag2测定的高度灵活性,因此将相同的方案和包含相同探针组的DNA阵列应用于富含GC的高度分枝杆菌基因组。基于DigiTag2原理对具有多重扩增和杂交条件的特定引物进行了优化,并用14个MTBC参考菌株,4个非结核分枝杆菌(NTM)分离株和322个特征性结核分枝杆菌临床分离株进行了评估。所开发的DNA芯片显示出99.85%的回收率,100%的转化率和99.75%的再现性。对于准确率,98.94%的阳性应答与以前的分子表征一致。我们具有成本效益的技术能够仅使用简单的仪器(例如热循环仪,杂交箱和DNA芯片扫描仪)在6 h内同时鉴定96种结核分枝杆菌临床分离株的MTBC种类和基因型,而技术人员较少比其他技术更需要技能。我们展示了这种方法作为一种简单,灵活且快速的工具的潜力,可提供有关循环MTBC分离物的更清晰信息。

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