Foxes (Vulpes vulpes) as sentinels for parasitic zoonoses, Toxoplasma gondii and Trichinella nativa, in the northeastern Canadian Arctic

Bachand, Nicholas; Ravel, André; Leighton, Patrick A.; Stephen, Craig; Iqbal, Azhar; Ndao, Momar; Konecsni, Kelly; Fernando, Champika; Jenkins, Emily J.

doi:10.1016/j.ijppaw.2018.10.003

Cited by 20 publications

(16 citation statements)

References 52 publications

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“…Since blood from marine mammals contains lipids that may interfere with the performance of agglutination assays [36], we removed lipid from seal samples using a chloroform method, re-tested using MAT, and compared serological test results with the ID Screen® Toxoplasmosis Indirect Multiple-Species ELISA kit used as per manufacturer instructions (IDVet Innovative Diagnostics, Montpellier). To ensure that lipid removal did not interfere with subsequent analyses using MAT, heart fluid from naturally-infected foxes and sera from experimentally-infected reindeer were included as positive controls, and these remained positive following lipid removal [32, 37]. ELISA results were measured as optical density percentages (OD %) as per manufacture instructions, where an OD% greater than 50% is positive, between 40–50% is ambiguous, and less than 40% is negative.…”

Section: Methodsmentioning

confidence: 99%

“…Real-time PCR amplification was done in a Bio-Rad CFX 96 DNA thermal cycler (Biorad, Hercules, California, USA) based on a published protocol for the detection of the 188 bp Toxoplasma sequence within the 529 repeat-element with the forward primer TOX 9 (5′-agg aga gat atc agg act gta g-3′) and backward primer TOX 11 (5′-gcg tcg tct cgt cta gat cg-3′) as per [28] and [38]. The final PCR assay reaction included 6.5 µl (0.5 M) of Itaq Supermix, 0.25 µl (20 µM) of TP1 probe, 1.25 µl (10 µM) of Tox 9F, 1.25 µl (10 µM) of Tox 11R, 0.5 µl (2 femtograms) of a competitive internal amplification control (CIAC), 1 µl (5 µM) of CIAC probe, 6.75 µl of PCR-grade water and 8 µl of template DNA [32]. A positive PCR reaction was defined as any reaction with a Ct-value smaller or equal to 35, a control negative PCR with a Ct-value of zero, a negative extraction control with a Ct value of zero and a control positive extraction control with a Ct-value smaller or equal to 40 [31].…”

Section: Methodsmentioning

confidence: 99%

“…Determination of the minimum number of DNA copies and tachyzoites detected by the MC-PCR technique has been described elsewhere [32]. Ct-values resulting from the amplified DNA recovered from the spiked beef samples for determining the lowest detection limit were then used to estimate the equation that predicts the log 10 (concentration) by fitting a generalized linear model in R statistical software version 3.4.4.…”

Section: Methodsmentioning

confidence: 99%

“…In Europe, the MC-PCR technique has also been used as a screening tool in food production animals for research purposes [31]. Recently, it has been used successfully in naturally-infected foxes of Nunavik [32]. There is clearly a need, and now a good method, to determine whether T. gondii DNA is present in tissues of wildlife commonly consumed by Inuit of Nunavik, and to compare these results with serological findings based on a commonly used agglutination assay.…”

Section: Introductionmentioning

confidence: 99%

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Serological and molecular detection of Toxoplasma gondii in terrestrial and marine wildlife harvested for food in Nunavik, Canada

et al. 2019

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Background Toxoplasma gondii, a zoonotic protozoan parasite, infects mammals and birds worldwide. Infection in humans is often asymptomatic, though illnesses can occur in immunocompromised hosts and the fetuses of susceptible women infected during pregnancy. In Nunavik, Canada, 60% of the Inuit population has measurable antibodies against T. gondii. Handling and consumption of wildlife have been identified as risk factors for exposure. Serological evidence of exposure has been reported for wildlife in Nunavik; however, T. gondii has not been detected in wildlife tissues commonly consumed by Inuit. Methods We used a magnetic capture DNA extraction and real-time PCR protocol to extract and amplify T. gondii DNA from large quantities of tissues (up to 100 g) of 441 individual animals in Nunavik: 166 ptarmigan ( Lagopus lagopus ), 156 geese ( Branta canadensis and Chen caerulescens ), 61 ringed seals ( Pusa hispida) , 31 caribou ( Rangifer tarandus ) and 27 walruses ( Odobenus rosmarus ). Results DNA from T. gondii was detected in 9% (95% CI: 3–15%) of geese from four communities in western and southern Nunavik, but DNA was not detected in other wildlife species including 20% (95% CI: 12–31%) of ringed seals and 26% (95% CI: 14–43%) of caribou positive on a commercial modified agglutination test (MAT) using thawed heart muscle juice. In geese, tissue parasite burden was highest in heart, followed by brain, breast muscle, liver and gizzard. Serological results did not correlate well with tissue infection status for any wildlife species. Conclusions To our knowledge, this is the first report on the detection, quantification, and characterization of DNA of T. gondii (clonal lineage II in one goose) from wildlife harvested for food in Nunavik, which supports the hypothesis that migratory geese can carry T. gondii into Nunavik where feline definitive hosts are rare. This study suggests that direct detection methods may be useful for detection of T. gondii in wildlife harvested for human consumption and provides data needed for a quantitative exposure assessment that will determine the risk of T. gondii exposure for Inuit who harvest and consume geese in Nunavik.

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Serological and molecular detection of Toxoplasma gondii in terrestrial and marine wildlife harvested for food in Nunavik, Canada

et al. 2019

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“…Specifically, researchers evaluated pets as possible reservoirs of MRSA within the patient population. 164–166 Other diseases have also been examined (eg, Toxoplasmosis, Rocky Mountain Spotted Fever, and Hantavirus), 141 , 167 , 168 but many require additional research efforts to allow for extended detection and treatment in animals and humans. Recently, there has been an increased focus on carbapenem resistance and its transmission both between humans and humans and animals.…”

Section: Applications Of Veterinary Informaticsmentioning

confidence: 99%

Veterinary informatics: forging the future between veterinary medicine, human medicine, and One Health initiatives—a joint paper by the Association for Veterinary Informatics (AVI) and the CTSA One Health Alliance (COHA)

Lustgarten

Zehnder²,

Shipman

et al. 2020

JAMIA Open

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Objectives This manuscript reviews the current state of veterinary medical electronic health records and the ability to aggregate and analyze large datasets from multiple organizations and clinics. We also review analytical techniques as well as research efforts into veterinary informatics with a focus on applications relevant to human and animal medicine. Our goal is to provide references and context for these resources so that researchers can identify resources of interest and translational opportunities to advance the field. Methods and Results This review covers various methods of veterinary informatics including natural language processing and machine learning techniques in brief and various ongoing and future projects. After detailing techniques and sources of data, we describe some of the challenges and opportunities within veterinary informatics as well as providing reviews of common One Health techniques and specific applications that affect both humans and animals. Discussion Current limitations in the field of veterinary informatics include limited sources of training data for developing machine learning and artificial intelligence algorithms, siloed data between academic institutions, corporate institutions, and many small private practices, and inconsistent data formats that make many integration problems difficult. Despite those limitations, there have been significant advancements in the field in the last few years and continued development of a few, key, large data resources that are available for interested clinicians and researchers. These real-world use cases and applications show current and significant future potential as veterinary informatics grows in importance. Veterinary informatics can forge new possibilities within veterinary medicine and between veterinary medicine, human medicine, and One Health initiatives.

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A new multiplexed magnetic capture—Droplet digital PCR tool for monitoring wildlife population health and pathogen surveillance

Tschritter,

V. C. de Groot,

Branigan

et al. 2023

Ecology and Evolution

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Anthropogenic stressors are exacerbating the emergence and spread of pathogens worldwide. In regions like the Arctic, where ecosystems are particularly susceptible, marked changes are predicted in regional diversity, intensity, and patterns of infectious diseases. To understand such rapidly changing host‐pathogen dynamics and mitigate the impacts of novel pathogens, we need sensitive disease surveillance tools. We developed and validated a novel multiplexed, magnetic capture, and ddPCR tool for the surveillance of multiple pathogens in polar bears, a sentinel species that is considered susceptible to climate change and other stressors with a pan‐Arctic distribution. Through sequence‐specific magnetic capture, we concentrated five target template sequences from three zoonotic bacteria (Erysipelothrix rhusiopathiae, Francisella tularensis, and Mycobacterium tuberculosis complex) and two parasitic (Toxoplasma gondii and Trichinella spp.) pathogens from large quantities (<100 g) of host tissue. We then designed and validated two multiplexed probe‐based ddPCR assays for the amplification and detection of the low‐concentration target DNA. Validations used 48 polar bear tissues (muscle and liver). We detected 14, 1, 3, 4, and 22 tissue positives for E. rhusiopathiae, F. tularensis, M. tuberculosis complex, T. gondii, and Trichinella spp., respectively. These multiplexed assays offer a rapid, specific tool for quantifying and monitoring the changing geographical and host distributions of pathogens relevant to human and animal health.

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Foxes (Vulpes vulpes) as sentinels for parasitic zoonoses, Toxoplasma gondii and Trichinella nativa, in the northeastern Canadian Arctic

Cited by 20 publications

References 52 publications

Serological and molecular detection of Toxoplasma gondii in terrestrial and marine wildlife harvested for food in Nunavik, Canada

Serological and molecular detection of Toxoplasma gondii in terrestrial and marine wildlife harvested for food in Nunavik, Canada

Veterinary informatics: forging the future between veterinary medicine, human medicine, and One Health initiatives—a joint paper by the Association for Veterinary Informatics (AVI) and the CTSA One Health Alliance (COHA)

A new multiplexed magnetic capture—Droplet digital PCR tool for monitoring wildlife population health and pathogen surveillance

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