Please use this identifier to cite or link to this item: https://hdl.handle.net/1959.11/14349
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dc.contributor.authorWalkden-Brown, Steve Wen
dc.contributor.authorIslam, Aminulen
dc.contributor.authorGroves, Peter Johnen
dc.contributor.authorRubite, Ambrosioen
dc.contributor.authorSharpe, Sue Men
dc.contributor.authorBurgess, Susanen
dc.date.accessioned2014-03-24T13:56:00Z-
dc.date.issued2013-
dc.identifier.citationAvian Diseases, 57(2), p. 544-554en
dc.identifier.issn1938-4351en
dc.identifier.issn0005-2086en
dc.identifier.urihttps://hdl.handle.net/1959.11/14349-
dc.description.abstractResults are presented from four studies between 2002 and 2011 into the feasibility of routinely monitoring Marek's disease virus serotype 1 (MDV-1) in broiler house dust using real-time quantitative PCR (qPCR) measurement. Study 1 on two farms showed that detection of MDV-1 occurred earlier on average in dust samples tested using qPCR than standard PCR and in spleen samples from five birds per shed assayed for MDV-1 by qPCR or standard PCR. DNA quality following extraction from dust had no effect on detection of MDV-1. Study 2 demonstrated that herpesvirus of turkeys (HVT) and MDV serotype 2 (MDV-2) in addition to MDV-1 could be readily amplified from commercial farm dust samples, often in mixtures. MDV-2 was detected in 11 of 20 samples despite the absence of vaccination with this serotype. Study 3 investigated the reproducibility and sensitivity of the qPCR test and the presence of inhibitors in the samples. Samples extracted and amplified in triplicate showed a high level of reproducibility except at very low levels of virus near the limit of detection. Mixing of samples prior to extraction provided results consistent with the proportions in the mixture. Tests for inhibition showed that if the template contained DNA in the range 0.5-20 ng/ml no inhibition of the reaction was detectable. The sensitivity of the tests in terms of viral copy number (VCN) per milligram of dust was calculated to be in the range 24-600 VCN/mg for MDV-1, 48-1200 VCN/mg for MDV-2, and 182-4560 VCN/mg for HVT. In study 4 the results of 1976 commercial tests carried out for one company were analyzed. Overall 23.1% of samples were positive for MDV-1, 26.1% in unvaccinated and 16.4% in vaccinated chickens. There was marked regional and temporal variation in the proportion of positive samples and the MDV-1 load. The tests were useful in formulating Marek's disease vaccination strategies. The number of samples submitted has increased recently, as has the incidence of positive samples. These studies provide strong evidence that detection and quantitation of MDV-1, HVT, and MDV-2 in poultry house dust using qPCR is robust, sensitive, reproducible, and meaningful, both biologically and commercially. Tactical vaccination based on monitoring of MDV-1 rather than routine vaccination may reduce selection pressure for increased virulence in MDV-1.en
dc.languageenen
dc.publisherAmerican Association of Avian Pathologists, Incen
dc.relation.ispartofAvian Diseasesen
dc.titleDevelopment, Application, and Results of Routine Monitoring of Marek's Disease Virus in Broiler House Dust Using Real-Time Quantitative PCRen
dc.typeJournal Articleen
dc.identifier.doi10.1637/10380-92112-REG.1en
dc.subject.keywordsVeterinary Virologyen
local.contributor.firstnameSteve Wen
local.contributor.firstnameAminulen
local.contributor.firstnamePeter Johnen
local.contributor.firstnameAmbrosioen
local.contributor.firstnameSue Men
local.contributor.firstnameSusanen
local.subject.for2008070712 Veterinary Virologyen
local.subject.seo2008830309 Poultryen
local.profile.schoolSchool of Environmental and Rural Scienceen
local.profile.schoolSchool of Environmental and Rural Scienceen
local.profile.schoolSchool of Environmental and Rural Scienceen
local.profile.emailswalkden@une.edu.auen
local.profile.emailpgroves2@une.edu.auen
local.profile.emailsburgess@une.edu.auen
local.output.categoryC1en
local.record.placeauen
local.record.institutionUniversity of New Englanden
local.identifier.epublicationsrecordune-20140115-092018en
local.publisher.placeUnited States of Americaen
local.identifier.runningnumbers1en
local.format.startpage544en
local.format.endpage554en
local.identifier.scopusid84879299363en
local.peerreviewedYesen
local.identifier.volume57en
local.identifier.issue2en
local.contributor.lastnameWalkden-Brownen
local.contributor.lastnameIslamen
local.contributor.lastnameGrovesen
local.contributor.lastnameRubiteen
local.contributor.lastnameSharpeen
local.contributor.lastnameBurgessen
dc.identifier.staffune-id:swalkdenen
dc.identifier.staffune-id:aislam5en
dc.identifier.staffune-id:pgroves2en
dc.identifier.staffune-id:sburgessen
local.profile.orcid0000-0002-0638-5533en
local.profile.roleauthoren
local.profile.roleauthoren
local.profile.roleauthoren
local.profile.roleauthoren
local.profile.roleauthoren
local.profile.roleauthoren
local.identifier.unepublicationidune:14564en
local.identifier.handlehttps://hdl.handle.net/1959.11/14349en
dc.identifier.academiclevelAcademicen
dc.identifier.academiclevelStudenten
dc.identifier.academiclevelAcademicen
dc.identifier.academiclevelAcademicen
dc.identifier.academiclevelAcademicen
dc.identifier.academiclevelAcademicen
local.title.maintitleDevelopment, Application, and Results of Routine Monitoring of Marek's Disease Virus in Broiler House Dust Using Real-Time Quantitative PCRen
local.output.categorydescriptionC1 Refereed Article in a Scholarly Journalen
local.search.authorWalkden-Brown, Steve Wen
local.search.authorIslam, Aminulen
local.search.authorGroves, Peter Johnen
local.search.authorRubite, Ambrosioen
local.search.authorSharpe, Sue Men
local.search.authorBurgess, Susanen
local.uneassociationYesen
local.year.published2013-
local.subject.for2020300914 Veterinary virologyen
local.subject.seo2020100411 Poultryen
Appears in Collections:Journal Article
School of Environmental and Rural Science
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