Please use this identifier to cite or link to this item: http://hdl.handle.net/1893/18247
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dc.contributor.authorDalvin, Sussieen_UK
dc.contributor.authorGlover, Kevin Aen_UK
dc.contributor.authorSorvik, Anne G Een_UK
dc.contributor.authorSeliussen, Bjorghild Ben_UK
dc.contributor.authorTaggart, Johnen_UK
dc.date.accessioned2017-08-25T01:08:03Z-
dc.date.available2017-08-25T01:08:03Z-
dc.date.issued2010-11en_UK
dc.identifier.other12en_UK
dc.identifier.urihttp://hdl.handle.net/1893/18247-
dc.description.abstractBackground: Aquaculture is a globally important and rapidly growing industry. It contributes positively to the economy and sustainability of coastal communities, but it is not without regulatory challenges. These challenges are diverse, and may include identification of fish discarded in an illegal manner, biological discharge from fish ensilage tanks, and partially destroyed or processed tissues. Robust genetic tools are required by management authorities to address these challenges. In this paper, we describe nine species-specific primer sets amplifying very short DNA fragments within the mitochondrial DNA cytochrome c oxidase (COI) gene, which were designed to permit diagnostic identification of degraded DNA from two of the most commonly farmed salmonids in Europe and North America. Results: Of the nine designed primer sets, six were found to be species-specific (four Atlantic salmon, two rainbow trout), whereas the remaining three sets (two Atlantic salmon, one rainbow trout) also amplified a product from other, closely related, salmonid DNA templates. Screening of DNA templates from 11 other non-salmonid native fish species did not produce PCR products with any of the primer sets. Specific tests confirmed the ability of these markers to identify Atlantic salmon and rainbow trout tissues in treated food products, chemically treated ensilage waste and fillets left to degrade in saltwater for up to 31 days at 15°C. Importantly, these markers provided diagnostic identification in cases where other genetic methods failed because of degraded DNA quality. Conclusions: Results from this study demonstrate that amplification of very short DNA fragments using species-specific primers represents a robust and versatile method to create cheap and efficient genetic tests that can be implemented in a range of forensic applications. These markers will provide fishery, aquaculture and food regulatory authorities with a method to investigate and enforce regulations within these industries.en_UK
dc.language.isoenen_UK
dc.publisherBioMed Centralen_UK
dc.relationDalvin S, Glover KA, Sorvik AGE, Seliussen BB & Taggart J (2010) Forensic identification of severely degraded Atlantic salmon (Salmo salar) and rainbow trout (Oncorhynchus mykiss) tissues. Investigative Genetics, 1 (1), Art. No.: 12. https://doi.org/10.1186/2041-2223-1-12en_UK
dc.rights© Dalvin et al. 2010This article is published under license to BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.10.1186/2041-2223-1-12en_UK
dc.rights.urihttp://creativecommons.org/licenses/by/2.0/en_UK
dc.titleForensic identification of severely degraded Atlantic salmon (Salmo salar) and rainbow trout (Oncorhynchus mykiss) tissuesen_UK
dc.typeJournal Articleen_UK
dc.identifier.doi10.1186/2041-2223-1-12en_UK
dc.citation.jtitleInvestigative Geneticsen_UK
dc.citation.issn2041-2223en_UK
dc.citation.volume1en_UK
dc.citation.issue1en_UK
dc.citation.publicationstatusPublisheden_UK
dc.citation.peerreviewedRefereeden_UK
dc.type.statusVoR - Version of Recorden_UK
dc.author.emailj.b.taggart@stir.ac.uken_UK
dc.contributor.affiliationNorwegian Institute of Marine Researchen_UK
dc.contributor.affiliationNorwegian Institute of Marine Researchen_UK
dc.contributor.affiliationNorwegian Institute of Marine Researchen_UK
dc.contributor.affiliationNorwegian Institute of Marine Researchen_UK
dc.contributor.affiliationInstitute of Aquacultureen_UK
dc.identifier.scopusid2-s2.0-79953890867en_UK
dc.identifier.wtid659695en_UK
dc.contributor.orcid0000-0002-3843-9663en_UK
dcterms.dateAccepted2010-11-30en_UK
dc.date.filedepositdate2014-01-10en_UK
rioxxterms.typeJournal Article/Reviewen_UK
rioxxterms.versionVoRen_UK
local.rioxx.authorDalvin, Sussie|en_UK
local.rioxx.authorGlover, Kevin A|en_UK
local.rioxx.authorSorvik, Anne G E|en_UK
local.rioxx.authorSeliussen, Bjorghild B|en_UK
local.rioxx.authorTaggart, John|0000-0002-3843-9663en_UK
local.rioxx.projectInternal Project|University of Stirling|https://isni.org/isni/0000000122484331en_UK
local.rioxx.freetoreaddate2014-01-10en_UK
local.rioxx.licencehttp://creativecommons.org/licenses/by/2.0/|2014-01-10|en_UK
local.rioxx.filenameInvestigative Genetics 2010.pdfen_UK
local.rioxx.filecount1en_UK
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