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Development and validation of direct PCR and quantitative PCR assays for the rapid, sensitive, and economical detection of porcine circovirus 3.

J. Vet. Diagn. Invest.. 2018; 
FranzoGiovanni,LegnardiMatteo,CentellegheCinzia,TucciaroneClaudia M,CecchinatoMattia,CorteyMartí,SegalésJoaquim,DrigoMic
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PCR Cloning and Subcloning Because PCV-3 sequences but no isolates were available, the full genome of PCV-3 (kindly provided by Dr. B. Hause, Kansas State University, Manhattan, KS) was chemically synthesized (GenScript Biotech, Piscataway, NJ) and cloned in a pUC57-Kan plasmid. Chemically competent Escherichia coli (One Shot TOP10, Thermo Fisher Scientific, Waltham, MA) were then transformed and selected by growth in a kanamycin-enriched lysogeny broth culture medium. Get A Quote

摘要

Since the identification of species Porcine circovirus 2, the relevance of genus Circovirus has increased given its impact on the swine industry. A new species ( Porcine circovirus 3, PCV-3) has been detected in association with various clinical conditions. Consequently, there is an urgent need for reliable and widely accessible tests for both routine diagnostic and research purposes. We developed a direct PCR (requiring no DNA extraction) and a quantitative (q)PCR targeting the conserved rep gene to detect the PCV-3 genome. Test performance was assessed by testing 120 field samples within different matrices. Both methods were sensitive (detection of 10 viral genome/µL), specific, and repeatable. The... More

关键词

Direct PCR,Porcine circovirus 3,qPCR,quantification,s