Development and validation of a TaqMan PCR assay for the Australian abalone herpes-like virus

The recent emergence of a herpes-like virus in both farmed and wild populations of abalone in Victoria, Australia, has been associated with high mortality rates in animals of all ages. Based on viral genome sequence information, a virus-specific real-time TaqMan assay was developed for detection and...

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Veröffentlicht in:Diseases of aquatic organisms 2010-10, Vol.92 (1), p.1-10
Hauptverfasser: Corbeil, Serge, Colling, Axel, Williams, Lynette M, Wong, Frank Y K, Savin, Keith, Warner, Simone, Murdoch, Bronwyn, Cogan, Noel O I, Sawbridge, Timothy I, Fegan, Mark, Mohammad, Ilhan, Sunarto, Agus, Handlinger, Judith, Pyecroft, Stephen, Douglas, Marianne, Changs, Pen H, Crane, Mark St J
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container_end_page 10
container_issue 1
container_start_page 1
container_title Diseases of aquatic organisms
container_volume 92
creator Corbeil, Serge
Colling, Axel
Williams, Lynette M
Wong, Frank Y K
Savin, Keith
Warner, Simone
Murdoch, Bronwyn
Cogan, Noel O I
Sawbridge, Timothy I
Fegan, Mark
Mohammad, Ilhan
Sunarto, Agus
Handlinger, Judith
Pyecroft, Stephen
Douglas, Marianne
Changs, Pen H
Crane, Mark St J
description The recent emergence of a herpes-like virus in both farmed and wild populations of abalone in Victoria, Australia, has been associated with high mortality rates in animals of all ages. Based on viral genome sequence information, a virus-specific real-time TaqMan assay was developed for detection and identification of the abalone herpes-like virus (AbHV). The assay was shown to be specific as it did not detect other viruses from either the Herpesvirales or the Iridovirales orders which have genome sequence similarities. However, the TaqMan assay was able to detect DNA from the Taiwanese abalone herpes-like virus, suggesting a relationship between the Taiwanese and Australian viruses. In addition, the assay detected < 300 copies of recombinant plasmid DNA per reaction. Performance characteristics for the AbHV TaqMan assay were established using 1673 samples from different abalone populations in Victoria and Tasmania. The highest diagnostic sensitivity and specificity were 96.7 (95% CI: 82.7 to 99.4) and 99.7 (95% CI: 99.3 to 99.9), respectively, at a threshold cycle (C(T)) value of 35.8. The results from 2 separate laboratories indicated good repeatability and reproducibility. This molecular assay has already proven useful in confirming presumptive diagnosis (based on the presence of ganglioneuritis) of diseased abalone in Victorian waters as well as being a tool for surveillance of wild abalone stocks in other parts of Australia.
doi_str_mv 10.3354/dao02277
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The results from 2 separate laboratories indicated good repeatability and reproducibility. 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The results from 2 separate laboratories indicated good repeatability and reproducibility. 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subjects Animals
Australia
DNA, Viral - genetics
DNA, Viral - isolation & purification
Haliotis
Herpes-like virus
Herpesviridae - isolation & purification
Mollusca - virology
Polymerase Chain Reaction - methods
Reproducibility of Results
Sensitivity and Specificity
title Development and validation of a TaqMan PCR assay for the Australian abalone herpes-like virus
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