利用病毒杀灭激光处理对李斯特菌属进行噬菌体扩增检测的方法。
Bacteriophage amplification assay for detection of Listeria spp. using virucidal laser treatment.
机构信息
Departamento de Ciências da Vida, Universidade Estadual da Bahia , Salvador, BA , Brasil.
出版信息
Braz J Microbiol. 2012 Jul;43(3):1128-36. doi: 10.1590/S1517-838220120003000040. Epub 2012 Jun 1.
Abstract
A protocol for the bacteriophage amplification technique was developed for quantitative detection of viable Listeria monocytogenes cells using the A511 listeriophage with plaque formation as the end-point assay. Laser and toluidine blue O (TBO) were employed as selective virucidal treatment for destruction of exogenous bacteriophage. Laser and TBO can bring a total reduction in titer phage (ca. 10(8) pfu/mL) without affecting the viability of L. monocytogenes cells. Artificially inoculated skimmed milk revealed mean populations of the bacteria as low as between 13 cfu/mL (1.11 log cfu/mL), after a 10-h assay duration. Virucidal laser treatment demonstrated better protection of Listeria cells than the other agents previously tested. The protocol was faster and easier to perform than standard procedures. This protocol constitutes an alternative for rapid, sensitive and quantitative detection of L. monocytogenes.
摘要
建立了一种噬菌体扩增技术方案,使用 A511 噬菌体作为终点检测法,以噬菌斑形成来定量检测活菌李斯特氏菌细胞。激光和甲苯胺蓝 O(TBO)被用作选择性病毒杀灭处理,以破坏外源性噬菌体。激光和 TBO 可以使噬菌体效价(约 10(8) pfu/mL)完全降低,而不影响李斯特氏菌细胞的活力。在 10 小时的检测时间后,人工接种的脱脂乳显示细菌的平均种群数量低至 13 cfu/mL(1.11 log cfu/mL)。与之前测试的其他试剂相比,病毒杀灭激光处理对李斯特氏菌细胞的保护作用更好。该方案比标准程序更快、更容易操作。该方案为快速、灵敏和定量检测李斯特氏菌提供了一种替代方法。
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