首页> 外文期刊>Molecular and Cellular Probes: The Location, Diagnosis and Monitoring of Disease by Specific Molecules and Cell Lines >A multiplexed PCR-coupled liquid bead array for the simultaneous detection of four biothreat agents.
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A multiplexed PCR-coupled liquid bead array for the simultaneous detection of four biothreat agents.

机译:用于同时检测四种生物威胁剂的多重PCR偶联液珠阵列。

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摘要

We have developed a 10-plexed PCR assay coupled to a 12-plexed liquid bead array to rapidly screen environmental samples for B. anthracis, Y. pestis, F. tularensis, and B. melitensis. Highly validated species-specific primer sets were used to simultaneously amplify multiple diagnostic regions unique to each individual pathogen. Resolution of the mix of amplified products was achieved by PCR product hybridization to corresponding probe sequences, attached to unique sets of fluorescent beads. The hybridized beads were processed through a flow cytometer, which detected presence and quantity of each PCR product. The assay was optimized to allow for maximum sensitivity in a multiplexed format. A high-throughput demonstration was performed where 384 simulated environmental samples were spiked with different amounts of B. thuringensis spores and pathogen DNA. The samples were robotically processed to extract DNA and arrayed for multiplexed PCR-liquid bead detection. The assay correctly identified the presenceor absence of each pathogen and collected over 3000 individual data points within a single 8-h shift for approximately Dollars 4.00 material costs per environmental sample in a 10-plexed assay.
机译:我们已经开发了一种10重PCR方法,结合了12重液珠阵列,可以快速筛选环境样品中的炭疽芽孢杆菌,鼠疫耶尔森氏菌,土拉弗朗西斯霉和B. melitensis。高度验证的物种特异性引物组用于同时扩增每种病原体特有的多个诊断区域。通过将PCR产物与相应的探针序列杂交(与独特的荧光珠组相连),可以实现扩增产物混合物的分离。通过流式细胞仪处理杂交的珠,该流式细胞仪检测每种PCR产物的存在和数量。对测定进行了优化,以允许以多重形式获得最大灵敏度。进行了高通量论证,其中向384个模拟环境样品中掺入了不同数量的苏云金芽孢杆菌孢子和病原体DNA。对样品进行自动处理,以提取DNA并进行阵列,以进行多重PCR-液珠检测。该测定法正确地鉴定出每种病原体的存在或不存在,并在一次10小时检测中,在一次8小时的班次中收集了3000多个单独的数据点,每个环境样品的材料成本约为4.00美元。

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