Peer-reviewed veterinary case report
Development of a multiplex TaqMan probe-based real-time PCR for discrimination of variant and classical porcine epidemic diarrhea virus.
- Journal:
- Journal of virological methods
- Year:
- 2014
- Authors:
- Zhao, Pan-deng et al.
- Affiliation:
- College of Veterinary Medicine · China
Plain-English summary
Since October 2010, there have been widespread outbreaks of diarrhea in piglets in China, leading to significant losses. A new strain of the porcine epidemic diarrhea virus (PEDV), which has some genetic changes compared to the older strain, has been identified as the cause of these outbreaks. Researchers developed a special test called multiplex TaqMan probe-based real-time PCR that can detect both the new and old strains of the virus in pig samples. In tests of 42 samples from pigs with severe diarrhea, they found that the new strain was much more common. This new testing method should help in measuring the amount of virus present and distinguishing between the two strains of PEDV.
Abstract
Since October 2010, porcine diarrhea outbreaks have occurred widely, resulting in major losses in suckling piglets in China. A variant porcine epidemic diarrhea virus (PEDV), characterized by base deletion and insertion in the S gene, compared to classical PEDV CV777, was shown to be responsible for this outbreak. In this study, a multiplex TaqMan probe-based real-time PCR was developed for detecting PEDV and differentiating the variant from classical PEDV, by using two sets of primers and probes based on the S gene of PEDV. The limits of detection of both variant and classical PEDV were 5×10(2) DNA copies. Specificity was determined using eight other viral pathogens of swine. Reproducibility was evaluated using standard dilutions, with coefficients of variation <1.4%. Standard dilutions included in each test allowed quantification of the amount of PEDV. Among 42 intestinal samples from pigs with severe watery diarrhea, 36 variant PEDV and three classical PEDV samples were detected, with viral loads of 10(2)-10(8) copies/μl and 10(3)-10(5) copies/μl, respectively, which suggested that the variant PEDV was prevalent in China. The multiplex TaqMan probe-based real-time PCR should be a useful tool for quantifying viral load, detecting PEDV, and differentiating variant from classical PEDV.
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Search related cases →Original publication: https://pubmed.ncbi.nlm.nih.gov/24928691/