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Strain discrimination of Yersinia pestis using a SERS-based electrochemically driven melting curve analysis of variable number tandem repeat sequences

机译:基于可变数目串联重复序列的基于SERS的电化学驱动熔解曲线分析来鉴定鼠疫耶尔森菌

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Strain discrimination within genetically highly similar bacteria is critical for epidemiological studies and forensic applications. An electrochemically driven melting curve analysis monitored by SERS has been utilised to reliably discriminate strains of the bacterial pathogen Yersinia pestis, the causative agent of plague. DNA amplicons containing Variable Number Tandem Repeats (VNTRs) were generated from three strains of Y. pestis: CO92, Harbin 35 and Kim. These amplicons contained a 10 base pair VNTR repeated 6, 5, and 4 times in CO92, Harbin 35 and Kim respectively. The assay also included a blocker oligonucleotide comprising 3 repeats of the 10-mer VNTR sequence. The use of the blocker reduced the effective length of the target sequence available to bind to the surface bound probe and significantly improved the sensitivity of the discrimination. The results were consistent during three replicates that were carried out on different days, using different batches of PCR product and different SERS sphere segment void (SSV) substrate. This methodology which combines low cost, speed and sensitivity is a promising alternative to the time consuming current electrophoretic methods.
机译:遗传上高度相似的细菌中的菌株区分对于流行病学研究和法医学应用至关重要。利用SERS监测的电化学驱动的熔解曲线分析已可可靠地区分鼠疫病原菌细菌鼠疫耶尔森菌。含有可变数目串联重复序列(VNTR)的DNA扩增子是从三株 Y菌株中产生的。鼠疫:CO92,哈尔滨35和金。这些扩增子包含在CO92,哈尔滨35和Kim中分别重复6、5和4次的10个碱基对的VNTR。该测定还包括包含10-mer VNTR序列的3个重复的阻断剂寡核苷酸。阻断剂的使用减少了可用于结合表面结合探针的靶序列的有效长度,并显着提高了区分的灵敏度。使用不同批次的PCR产物和不同的SERS球体区段空隙(SSV)底物,在不同天进行的三个重复实验中,结果是一致的。这种结合了低成本,快速和灵敏性的方法是一种费时的电流电泳方法的有前途的替代方法。

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