Development and validation of a reverse transcription quantitative PCR for universal detection of viral hemorrhagic septicemia virus

Garver, Kyle A.; Hawley, Laura M.; McClure, Carol; Schroeder, Tamara; Aldous, Sandra; Doig, Fiona; Snow, Michael; Edes, Sandra; Baynes, Catherine; Richard, Jon

doi:10.3354/dao02344

Cited by 68 publications

(64 citation statements)

References 47 publications

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“…Initial virus identity for isolates prior to 1998 was determined using a DNA probe (Batts et al 1993), while isolations post 1998 were confirmed via VHSV-specific reverse transcriptase polymerase chain reaction (RT-PCR) as described below. All BC VHSV isolates listed herein were cultured with the exception of the Pa cific Hake isolate which was detected via quantitative RT-PCR (RT-qPCR) (Garver et al 2011) and RT-PCR.…”

Section: Virus Isolation and Fish Lossesmentioning

confidence: 99%

Molecular epidemiology of viral haemorrhagic septicaemia virus (VHSV) in British Columbia, Canada, reveals transmission from wild to farmed fish

Garver

Traxler²,

Hawley³

et al. 2013

Dis. Aquat. Org.

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Viral haemorrhagic septicaemia virus (VHSV) is a fish pathogen found throughout the Northern Hemisphere and is capable of infecting and causing mortality in numerous marine and freshwater hosts. In the coastal waters of British Columbia, Canada, the virus has been detected for 20 yr with many occurrences of mass mortalities among populations of Pacific herring Clupea pallasii (Valenciennes) and sardine Sardinops sagax as well as detections among cultured Atlantic Salmo salar and Chinook Oncorhynchus tshawytscha salmon. We compared nucleotide sequence of the full glycoprotein (G) gene coding region (1524 nt) of 63 VHSV isolates sampled during its recorded presence from 1993 to 2011 from 6 species and a total of 29 sites. Phylogenetic analysis showed that all isolates fell into sub-lineage IVa within the major VHSV genetic group IV. Of the 63 virus isolates, there were 42 unique sequences, each of which was ephemeral, being repeatedly detected at most only 1 yr after its initial detection. Multiple sequence types were revealed during single viral outbreak events, and genetic heterogeneity was observed within isolates from individual fish. Moreover, phylogenetic analysis revealed a close genetic linkage between VHSV isolates obtained from pelagic finfish species and farmed salmonids, providing evidence for virus transmission from wild to farmed fish.

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Section: Virus Isolation and Fish Lossesmentioning

confidence: 99%

Molecular epidemiology of viral haemorrhagic septicaemia virus (VHSV) in British Columbia, Canada, reveals transmission from wild to farmed fish

Garver

Traxler²,

Hawley³

et al. 2013

Dis. Aquat. Org.

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“…For quality control purposes and to provide unambiguous definitions of positive and negative test results, both negative and positive controls should be included in each of the test runs. To show the needed information in this item, a description of the quality control samples used in a real-time RT-PCR validation study is presented in the example above (Garver et al 2011) and in Greer & Collins (2007). Authors should also specify whether or not internal and/or artificial controls are included in PCR assays to identify false-negative or falsepositive test results (Snow et al 2009, Purcell et al 2014, as well as the protocol for retesting such samples.…”

Section: Explanationmentioning

confidence: 99%

“…The challenge conditions, particularly the dose and strain of pathogen, should be reported to allow readers to evaluate how well the experimental model reflects natural exposure under field conditions. The examples by Greer & Collins (2007) and Garver et al (2011) include most of the necessary elements with the exception of Animal Ethics Committee approval of the experiment design. Research studies with amphibians and fish, but typically not molluscs and crustaceans, must be approved by the Animal Ethics Committee in most research institu-tions and should be reported as done in Purcell et al (2013), with the possible addition of approved protocol numbers (see Hyatt et al 2007).…”

Section: Explanationmentioning

confidence: 99%

“…Blinding avoids both potential bias in the interpretation of test results and overly optimistic estimates of diagnostic sensitivity and specificity or the area under the receiver-operating curve in diagnostic test evaluations. Procedures for blinding should be described as in the Garver et al (2011) example or as in Thébault et al (2005). If the joint results of the TUE and RS (positive−positive, positive−negative, negative−positive, and negative) are reviewed by testing laboratories and retesting of samples with discrepant (discordant or nonagreeing) results is done using a third test, estimates of sensitivity and specificity will change and may be inflated (Hadgu 1999).…”

Section: Explanationmentioning

confidence: 99%

“…kappa with 95% CI). For a review of methods for estimating and reporting agreement for continuous test outcomes, see for example, Barnhart et al (2007), Garver et al (2011), andOIE (2015c). Caraguel et al (2011) is a good example of reporting of more complex modelling methods to investigate the impact of sample or operational factors on test precision.…”

Section: Explanationmentioning

confidence: 99%

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Recommended reporting standards for test accuracy studies of infectious diseases of finfish, amphibians, molluscs and crustaceans: the STRADAS-aquatic checklist

Gardner¹,

Whittington²,

Caraguel³

et al. 2016

Dis. Aquat. Org.

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Complete and transparent reporting of key elements of diagnostic accuracy studies for infectious diseases in cultured and wild aquatic animals benefits end-users of these tests, enabling the rational design of surveillance programs, the assessment of test results from clinical cases and comparisons of diagnostic test performance. Based on deficiencies in the Standards for Reporting of Diagnostic Accuracy (STARD) guidelines identified in a prior finfish study (Gardner et al. 2014), we adapted the Standards for Reporting of Animal Diagnostic Accuracy Studiesparatuberculosis (STRADAS-paraTB) checklist of 25 reporting items to increase their relevance to finfish, amphibians, molluscs, and crustaceans and provided examples and explanations for each item. The checklist, known as STRADAS-aquatic, was developed and refined by an expert group of 14 transdisciplinary scientists with experience in test evaluation studies using field and experimental samples, in operation of reference laboratories for aquatic animal pathogens, and in development of international aquatic animal health policy. The main changes to the STRADAS-paraTB checklist were to nomenclature related to the species, the addition of guidelines for experimental challenge studies, and the designation of some items as relevant only to experimental studies and ante-mortem tests. We believe that adoption of these guidelines will improve reporting of primary studies of test accuracy for aquatic animal diseases and facilitate assessment of their fitness-forpurpose. Given the importance of diagnostic tests to underpin the Sanitary and Phytosanitary agreement of the World Trade Organization, the principles outlined in this paper should be applied to other World Organisation for Animal Health (OIE)-relevant species.

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A Comparison of Nonlethal and Destructive Methods for Broad‐Based Infectious Agent Screening of Chinook Salmon Using High‐Throughput qPCR

Teffer

Miller

2019

J Aqua Anim Hlth

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Molecular tools, such as high-throughput quantitative polymerase chain reaction (HT-qPCR), are useful for monitoring multiple infectious agents in wild animal populations (i.e., broad-based screening). If destructive tissue samples cannot be obtained due to experimental design requirements (e.g., bio-telemetry; holding with repeated biopsy) or the conservation status of host species, then nonlethally sampled tissues can be substituted. However, infection profiles have been found to differ between nonlethally and destructively sampled tissues. We present a comparative analysis of nonlethal (gill and blood) and destructive (pool of internal and external tissue) approaches for broad-based infectious agent screening of adult Chinook Salmon Oncorhynchus tshawytscha. Of a possible 47 agents, 16 were detected overall by nonlethal and destructive methods. Our results indicated moderate differences in infection profiles among tissues, with limitations of each tissue type dependent on the ecology of each agent. The gill was the most comprehensive screening tissue, as more infectious agents were detected overall in gill (n = 16) than in blood (n = 12) or multi-tissue pools (n = 15). The agreement in the estimated agent prevalence between tissue types ranged from poor to excellent, while overall agent community structure (the combined prevalence of all agents) showed low agreement between tissue types. Two agents occurred at 100% prevalence in all tissue types. Nine agents, including types of bacteria and gill parasites, were more prevalent in gill than in blood, while five agents, including one virus and several microparasites, were more prevalent in blood. Future studies should pair microscopy and histopathology with HT-qPCR to better characterize host health and disease development relative to molecular detection of agents across tissue types.

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Development and validation of a reverse transcription quantitative PCR for universal detection of viral hemorrhagic septicemia virus

Cited by 68 publications

References 47 publications

Molecular epidemiology of viral haemorrhagic septicaemia virus (VHSV) in British Columbia, Canada, reveals transmission from wild to farmed fish

Molecular epidemiology of viral haemorrhagic septicaemia virus (VHSV) in British Columbia, Canada, reveals transmission from wild to farmed fish

Recommended reporting standards for test accuracy studies of infectious diseases of finfish, amphibians, molluscs and crustaceans: the STRADAS-aquatic checklist

A Comparison of Nonlethal and Destructive Methods for Broad‐Based Infectious Agent Screening of Chinook Salmon Using High‐Throughput qPCR

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