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单叠氮碘化丙啶和长扩增子定量聚合酶链反应作为大肠杆菌噬菌体感染性检测方法的评估

Evaluation of propidium monoazide and long-amplicon qPCR as an infectivity assay for coliphage.

作者信息

McLellan Nicole L, Lee Hung, Habash Marc B

机构信息

School of Environmental Sciences, University of Guelph, Guelph, ON N1G 2W1, Canada.

出版信息

J Virol Methods. 2016 Dec;238:48-55. doi: 10.1016/j.jviromet.2016.10.004. Epub 2016 Oct 12.

Abstract

Standardized and rapid assays for viable viral pathogens are needed to inform human health risk assessments. Conventional qPCR is designed to enumerate the gene copies of an organism in a sample, but does not identify those that originated from a viable pathogen. This study was undertaken to evaluate modified qPCR methods as infectivity assays for the enumeration of infectious MS2 coliphage. Propidium monoazide (PMA) treatment coupled with long-amplicon qPCR assays were assessed for their ability to quantify infectious MS2 in pure cultures and following inactivation by a range of UV light exposures and chlorine doses. The qPCR results were compared to the plaque assay, which was used as the standard to indicate the level of infectious MS2 in each sample. For pure cultures, PMA-qPCR results were not significantly different from the plaque assay (p>0.05). At >4 log inactivation, combined PMA and long-amplicon qPCR assays overestimated the level of infectious MS2 remaining (p<0.05). The most accurate long-amplicon qPCR infectivity assay targeted a 624-bp region at the 5' end of the genome. Modified qPCR approaches may be useful tools to monitor the loss of infectivity as a result of disinfection processes.

摘要

需要标准化且快速的活病毒病原体检测方法,以便进行人类健康风险评估。传统的定量聚合酶链反应(qPCR)旨在对样本中生物体的基因拷贝进行计数,但无法识别那些源自活病原体的基因拷贝。本研究旨在评估改良的qPCR方法作为感染性检测方法,用于计数感染性MS2噬菌体。评估了单叠氮化丙锭(PMA)处理与长扩增子qPCR检测方法在纯培养物中以及在一系列紫外线照射和氯剂量灭活后对感染性MS2进行定量的能力。将qPCR结果与噬菌斑检测进行比较,噬菌斑检测用作指示每个样本中感染性MS2水平的标准。对于纯培养物,PMA-qPCR结果与噬菌斑检测结果无显著差异(p>0.05)。在灭活>4个对数时,PMA和长扩增子qPCR联合检测高估了剩余感染性MS2的水平(p<0.05)。最准确的长扩增子qPCR感染性检测针对基因组5'端的一个624碱基对区域。改良的qPCR方法可能是监测消毒过程导致的感染性丧失的有用工具。

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