Please use this identifier to cite or link to this item: https://ir.swu.ac.th/jspui/handle/123456789/15071
Title: Target for standard Thai PCR assay identical in 12 white spot syndrome virus (WSSV) types that differ in DNA multiple repeat length
Authors: Kiatpathomchai W.
Taweetungtragoon A.
Jittivadhana K.
Wongteerasupaya C.
Boonsaeng V.
Flegel T.W.
Keywords: virus DNA
agricultural worker
article
controlled study
gene sequence
genetic variability
laboratory diagnosis
nonhuman
nucleotide repeat
nucleotide sequence
open reading frame
polymerase chain reaction
priority journal
sample size
sensitivity analysis
validation process
virus
virus detection
virus gene
virus strain
White spot syndrome virus
Animals
Base Sequence
DNA, Viral
Molecular Sequence Data
Open Reading Frames
Penaeidae
Polymerase Chain Reaction
Sequence Analysis, DNA
Thailand
White spot syndrome virus 1
Decapoda (Crustacea)
DNA viruses
Shrimp white spot syndrome virus
Issue Date: 2005
Abstract: A Thai PCR detection method (WSSV-232) yielding a 232 bp amplicon has been used for detection of white spot syndrome virus (WSSV) since 1996. It targets ORF 91 in the full sequence of the only Thai WSSV isolate at GenBank (AF369029). At the beginning of 2002, some Thai shrimp farmers complained that ponds stocked with WSSV-232 PCR negative post-larvae (PL) later suffered WSSV disease outbreaks. Although these outbreaks may have resulted from horizontal transmission of WSSV after stocking, it was also possible that they resulted from false negative PCR test results due to genetic changes at the PCR-assay target after the first appearance of WSSV in Thailand in 1995. Indeed, recent results have revealed at least 12 WSSV variants in Thailand that can be distinguished based on differences in DNA multiple repeat lengths in ORF 94 (GenBank AF369029). To test for variation in the WSSV-232 target sequence in ORF 91, 20 DNA extracts derived from field samples and representing 9 of the WSSV DNA multiple repeat groups were subjected to PCR amplification and sequencing using primers that generated a 403 bp amplicon covering the target for the WSSV-232 assay. An additional three repeat types were included from archived material. Analysis revealed that the 232 bp target sequence in ORF 91 was unchanged in all of the 12 types tested and that the original WSSV-232 detection system was still valid. Thus, any false negative PCR test results leading to farmer complaints would probably have arisen from small sample sizes and low sensitivity of the single-step PCR assay. If so, false negative results could be reduced by the use of nested PCR assays with larger PL sample sizes. © 2005 Elsevier B.V. All rights reserved.
URI: https://ir.swu.ac.th/jspui/handle/123456789/15071
https://www.scopus.com/inward/record.uri?eid=2-s2.0-27744481024&doi=10.1016%2fj.jviromet.2005.06.006&partnerID=40&md5=6f5d3c3809a31b86e69e38b13670f797
ISSN: 1660934
Appears in Collections:Scopus 1983-2021

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