| Literature DB >> 25144112 |
Janet V Warg1, Travis Clement, Emily R Cornwell, Angela Cruz, Rodman G Getchell, Cem Giray, Andrew E Goodwin, Geoffrey H Groocock, Mohamed Faisal, Robert Kim, Gwenn E Merry, Nicholas B D Phelps, Monica M Reising, Isaac Standish, Yan Zhang, Kathy Toohey-Kurth.
Abstract
Eight laboratories worked collectively to evaluate 4 real-time RT-PCR (rRT-PCR) protocols targeting viral hemorrhagic septicemia virus (VHSV) being considered for deployment to a USA laboratory testing network. The protocols utilized previously published primers and probe sets developed for detection and surveillance of VHSV. All participating laboratories received and followed a standard operating protocol for extraction and for each of the rRT-PCR assays. Performance measures specifically evaluated included limit of detection (defined as the smallest amount of analyte in which 95% of the samples are classified as positive), analytical specificity, assay efficiency across genotype representatives, within- and between-plate variation within a laboratory, and variation between laboratories using the same platform, between platforms, and between software versions. This evaluation clearly demonstrated that the TaqMan®-based assay developed by Jonstrup et al. (2013; J Fish Dis 36:9-23) produced the most consistent analytical performance characteristics for detecting all genotypes of VHSV across the 8 participating laboratories.Entities:
Mesh:
Year: 2014 PMID: 25144112 DOI: 10.3354/dao02753
Source DB: PubMed Journal: Dis Aquat Organ ISSN: 0177-5103 Impact factor: 1.802