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Direct detection of Listeria monocytogenes from milk by magnetic based DNA isolation and PCR

机译:磁性DNA分离和PCR直接检测牛奶中的李斯特菌

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摘要

Two nucleic acid-based methods for rapid and sensitive detection of the foodborne pathogen Listeria monocytogenes in milk were developed in this study. These methods rely on paramagnetic nanoparticle-based isolation of bacterial DNA directly from milk and subsequent PCR with selective primers for the listeriolysin O (hlyA) gene. The hlyA specific product was reproducibly detected and showed a sensitivity of 10 cfu ml~(-1). The magnetic-based system had a sensitivity 10-fold higher than that of commercially available column devices. The detection limit of both methods is sufficient for direct detection of L. monocytogenes DNA in milk avoiding the enrichment culturing step, reducing the time necessary to obtain results from samples to 7 h rather than the 5-day minimum required for the standard procedure. The methods developed are suitable for automation.
机译:本研究开发了两种基于核酸的方法,用于快速灵敏地检测牛奶中的食源性单核细胞增生李斯特氏菌。这些方法依赖于直接从牛奶中基于顺磁性纳米颗粒的细菌DNA分离,以及随后使用针对李斯特菌溶血素O(hlyA)基因的选择性引物进行的PCR。可检测到hlyA特异产物,灵敏度为10 cfu ml〜(-1)。基于磁性的系统的灵敏度比市售色谱柱设备高10倍。两种方法的检出限足以直接检测牛奶中的单核细胞增生李斯特氏菌DNA,而无需进行富集培养步骤,从而将从样品中获得结果所需的时间减少到7小时,而不是标准程序所需的最少5天。开发的方法适用于自动化。

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