Your search keyword '"Forbes LB"' showing total 41 results

1. Trichinella Surveillance in Black Bears ( Ursus americanus ) from the Dehcho Region, Northwest Territories, Canada, 2002-15.

Author

Larter NC, Elkin BT, Forbes LB, Wagner B, and Allaire DG

Subjects

Animals, Canada, Humans, Northwest Territories, Risk, Trichinella isolation & purification, Trichinellosis veterinary, Ursidae microbiology

Abstract

We used muscle digestion to test black bears ( Ursus americanus ) from the southwestern Northwest Territories, Canada, for Trichinella. Results showed a prevalence of 4.1%. Some bears had infection intensities of more than one larva per gram of muscle tissue; this level in meat is considered to pose a human consumption safety risk.

Published

2017

2. Performance of commercial ELISA and agglutination test kits for the detection of anti-Toxoplasma gondii antibodies in serum and muscle fluid of swine infected with 100, 300, 500 or 1000 oocysts.

Author

Forbes LB, Parker SE, and Gajadhar AA

Subjects

Agglutination Tests methods, Animals, Antibodies, Protozoan analysis, Body Fluids chemistry, Enzyme-Linked Immunosorbent Assay methods, Muscle, Skeletal, Swine, Swine Diseases blood, Swine Diseases immunology, Toxoplasmosis, Animal parasitology, Agglutination Tests veterinary, Antibodies, Protozoan blood, Enzyme-Linked Immunosorbent Assay veterinary, Swine Diseases parasitology, Toxoplasma immunology, Toxoplasmosis, Animal blood

Abstract

Serum and tissue fluid samples from experimentally infected swine were tested for antibodies to Toxoplasma gondii using both an indirect ELISA and a modified agglutination test (MAT) available commercially in kit form. Ten 8-9 week-old swine were fed meatballs containing 100, 300, 500 or 1000 T. gondii oocysts and three control animals were fed meatballs with no oocysts. Post-inoculation blood samples were collected weekly until euthanasia at 35-63 days post inoculation (DPI). Tissue fluid was obtained from diaphragm, heart and sternomastoideus muscles post-mortem. By 16 DPI, nine of 10 inoculated pigs were detected serologically using ELISA at a pre-test serum dilution of 1:50 and all ten pigs were detected by the MAT at a serum dilution of 1:25. The last pig became positive on ELISA by 21 DPI and the 10 pigs maintained their serological status for the duration of the experiment. Heart muscle was the best overall source of tissue fluid for ELISA and all six pigs inoculated with either 500 or 1000 oocysts were positive using either diaphragm or heart tissue fluid samples. However, 10 of 18 fluid samples from pigs receiving ≤ 300 oocysts were not detected using ELISA, including 5 of 6 from sternomastoideus muscle. The MAT used at a 1:10 pre-test dilution of tissue fluid correctly identified all 10 inoculated pigs regardless of the source muscle. Based on these data, we conclude that either assay would be useful for herd evaluation or surveillance testing using sera, and the MAT would be a good candidate assay for testing tissue fluid for the same purposes., (Crown Copyright © 2012. Published by Elsevier B.V. All rights reserved.)

Published

2012

3. Validation of an immunohistochemical assay for bovine cysticercosis, with comparison to a standard histological method.

Author

Scandrett WB, Haines DM, Parker SE, Robinson Y, Forbes LB, Brandt J, Geerts S, Dorny P, and Gajadhar AA

Subjects

Animals, Cattle, Cattle Diseases parasitology, Cysticercosis diagnosis, Immunohistochemistry methods, Reproducibility of Results, Cattle Diseases diagnosis, Cysticercosis veterinary, Immunohistochemistry veterinary

Abstract

The larval stage (syn Cysticercus bovis) of the human tapeworm Taenia saginata causes cysticercosis in cattle, which has both aesthetic and food safety implications to consumers of beef. A monoclonal antibody-based immunohistochemical (IHC) assay developed to improve postmortem diagnosis of this parasite and a standard histological method were assessed to determine their fitness for intended use. Sections from 169 known-positive specimens of T. saginata from experimentally or naturally infected cattle, and from 30 known-negative specimens and lesions of various etiologies from non-infected cattle, were tested. The IHC assay identified significantly more known positive bovine cysticerci than the histological method (91.7% and 38.5%, respectively). Positive IHC staining occurred on sections from other cestode species, but should not affect the diagnostic specificity of this assay for bovine cysticercosis, due to the different host and/or tissue preferences amongst these parasites. Use of the IHC assay should improve the reliability of diagnosing lesions caused by degenerated cysticerci, facilitating more effective and efficient control of bovine cysticercosis., (Crown Copyright © 2011. Published by Elsevier B.V. All rights reserved.)

Published

2012

4. Prevalence of Trichinella spp. in black bears, grizzly bears, and wolves in the Dehcho Region, Northwest Territories, Canada, including the first report of T. nativa in a grizzly bear from Canada.

Author

Larter NC, Forbes LB, Elkin BT, and Allaire DG

Subjects

Animals, Female, Genotype, Humans, Male, Meat parasitology, Northwest Territories epidemiology, Prevalence, Species Specificity, Trichinella classification, Trichinella isolation & purification, Trichinellosis epidemiology, Trichinellosis transmission, Muscle, Skeletal parasitology, Trichinellosis veterinary, Ursidae parasitology, Wolves parasitology

Abstract

Samples of muscle from 120 black bears (Ursus americanus), 11 grizzly bears (Ursus arctos), and 27 wolves (Canis lupus) collected in the Dehcho Region of the Northwest Territories from 2001 to 2010 were examined for the presence of Trichinella spp. larvae using a pepsin-HCl digestion assay. Trichinella spp. larvae were found in eight of 11 (73%) grizzly bears, 14 of 27 (52%) wolves, and seven of 120 (5.8%) black bears. The average age of positive grizzly bears, black bears, and wolves was 13.5, 9.9, and approximately 4 yr, respectively. Larvae from 11 wolves, six black bears, and seven grizzly bears were genotyped. Six wolves were infected with T. nativa and five with Trichinella T6, four black bears were infected with T. nativa and two with Trichinella T6, and all seven grizzly bears were infected with Trichinella T6 and one of them had a coinfection with T. nativa. This is the first report of T. nativa in a grizzly bear from Canada. Bears have been linked to trichinellosis outbreaks in humans in Canada, and black bears are a subsistence food source for residents of the Dehcho region. In order to assess food safety risk it is important to monitor the prevalence of Trichinella spp. in both species of bear and their cohabiting mammalian food sources.

Published

2011

5. A 10-year wildlife survey of 15 species of Canadian carnivores identifies new hosts or geographic locations for Trichinella genotypes T2, T4, T5, and T6.

Author

Gajadhar AA and Forbes LB

Subjects

Animals, Canada epidemiology, Genotype, Geography, Polymerase Chain Reaction, Population Surveillance, Trichinellosis epidemiology, Animals, Wild parasitology, Carnivora parasitology, Trichinella genetics, Trichinellosis parasitology

Abstract

A survey of wild carnivores in Canada was conducted over a 10-year period to determine the prevalence and genotypes of Trichinella. Muscle samples collected from 1409 animals representing 15 hosts species were enzymatically digested to recover Trichinella larvae. Larvae were recovered from a total of 287 (20.4%) animals and PCR identified four genotypes of Trichinella. Trichinella nativa was found in 5 host species and was the most commonly found genotype. Trichinella T6 was present in 7 species of carnivores, and coyote and badger are new host records for this genotype. The recovery of T. pseudospiralis and T. murrelli from cougars is the first documentation of these species in Canada and in cougars. The cougar was also the only host species in which all four genotypes of Trichinella were identified. Black bears and walruses had the highest tissue levels of larvae in this study and are also the species most frequently associated with human trichinellosis in Canada. This work identifies additional host species and expanded geographic ranges for 4 genotypes of Trichinella in North America. Failure to demonstrate T. spiralis in wildlife and continued negative results from ongoing surveillance activities in swine provide additional evidence that T. spiralis is not present in Canada.

Published

2010

6. Infectivity of Toxoplasma gondii in northern traditional (country) foods prepared with meat from experimentally infected seals.

Author

Forbes LB, Measures L, and Gajadhar A

Subjects

Animals, Biological Assay, Canada, Cats, Consumer Product Safety, Humans, Risk Assessment, Time Factors, Toxoplasma growth & development, Toxoplasmosis epidemiology, Toxoplasmosis etiology, Toxoplasmosis transmission, Food Handling methods, Food Parasitology, Meat Products parasitology, Seals, Earless parasitology, Toxoplasma isolation & purification

Abstract

Serological and clinical evidence of human toxoplasmosis in the Canadian Arctic indicates a food safety risk associated with the consumption of wild game meat. Such meat often is eaten raw or partially cooked in locally prepared traditional (country) foods, but no data have been collected to describe survival of Toxoplasma gondii forms in these foods. The muscle of grey seals (Halichoerus grypus) experimentally infected with T. gondii oocysts was used to prepare three country foods: igunaq, a fermented product; nikku, a dried product; and sausage, a salted and spiced product. Igunaq and nikku were stored at 4 degrees C and bioassayed in cats at 49, 95, and 140 days postpreparation (DPP) and 41, 84, and 132 DPP, respectively. Raw and cooked sausages were stored at -20 degrees C and bioassayed at 50, 92, and 141 DPP. The source seal meat was infective for cats, but none of the foods prepared with this meat were infective for cats. Some cooked sausages did not reach internal temperatures considered lethal for T. gondii. Data from studies in domestic animals suggested that the negative results in this experiment were due to temperature and duration of storage. Because of the possibility that T. gondii of arctic origin might be more freeze tolerant than the swine-origin isolate used in this experiment, additional studies are necessary to clarify the risks of toxoplasmosis associated with consumption of arctic country foods.

Published

2009

7. Trichinella diagnostics and control: mandatory and best practices for ensuring food safety.

Author

Gajadhar AA, Pozio E, Gamble HR, Nöckler K, Maddox-Hyttel C, Forbes LB, Vallée I, Rossi P, Marinculić A, and Boireau P

Subjects

Animals, Birds parasitology, Disease Reservoirs veterinary, Global Health, Humans, Life Cycle Stages, Mammals parasitology, Muscle, Skeletal parasitology, Quality Control, Reptiles parasitology, Trichinella growth & development, Trichinellosis epidemiology, Zoonoses, Food Parasitology standards, Trichinella isolation & purification, Trichinellosis diagnosis, Trichinellosis prevention & control

Abstract

Because of its role in human disease, there are increasing global requirements for reliable diagnostic and control methods for Trichinella in food animals to ensure meat safety and to facilitate trade. Consequently, there is a need for standardization of methods, programs, and best practices used in the control of Trichinella and trichinellosis. This review article describes the biology and epidemiology of Trichinella, and describes recommended test methods as well as modified and optimized procedures that are used in meat inspection programs. The use of ELISA for monitoring animals for infection in various porcine and equine pre- and post-slaughter programs, including farm or herd certification programs is also discussed. A brief review of the effectiveness of meat processing methods, such as freezing, cooking and preserving is provided. The importance of proper quality assurance and its application in all aspects of a Trichinella diagnostic system is emphasized. It includes the use of international quality standards, test validation and standardization, critical control points, laboratory accreditation, certification of analysts and proficiency testing. Also described, are the roles and locations of international and regional reference laboratories for trichinellosis where expert advice and support on research and diagnostics are available.

Published

2009

8. Canine brucellosis in a Saskatchewan kennel.

Author

Brennan SJ, Ngeleka M, Philibert HM, Forbes LB, and Allen AL

Subjects

Abortion, Veterinary microbiology, Animals, Brucella immunology, Brucella isolation & purification, Brucellosis diagnosis, Brucellosis epidemiology, Brucellosis pathology, Dog Diseases diagnosis, Dog Diseases pathology, Dogs, Female, Fluorescent Antibody Technique, Indirect methods, Fluorescent Antibody Technique, Indirect veterinary, Immunohistochemistry veterinary, Male, Organ Specificity, Pregnancy, Saskatchewan epidemiology, Animal Husbandry methods, Antibodies, Bacterial blood, Brucellosis veterinary, Disease Outbreaks veterinary, Dog Diseases epidemiology

Abstract

Canine brucellosis is rare in Canada. This report describes an outbreak of Brucella canis infection within a kennel, emphasizing diagnostic and pathologic findings. Gender differences are described. The progestational, nongravid uterus, female spleen, and prostate gland are consistent sites of bacterial isolation.

Published

2008

9. Complete validation of a unique digestion assay to detect Trichinella larvae in horse meat demonstrates the reliability of this assay for meeting food safety and trade requirements.

Author

Forbes LB, Hill DE, Parker S, Tessaro SV, Gamble HR, and Gajadhar AA

Subjects

Animals, Consumer Product Safety, Food Handling, Horses, Humans, International Cooperation, Larva, Parasite Egg Count, Quality Control, Reproducibility of Results, Sensitivity and Specificity, Trichinella spiralis isolation & purification, Food Contamination analysis, Food Inspection standards, Food Parasitology standards, Meat parasitology, Trichinella isolation & purification

Abstract

A tissue digestion assay using a double separatory funnel procedure for the detection of Trichinella larvae in horse meat was validated for application in food safety programs and trade. The assay consisted of a pepsin-HCl digestion step to release larvae from muscle tissue and two sequential sedimentation steps in separatory funnels to recover and concentrate larvae for detection with a stereomicroscope. With defined critical control points, the assay was conducted within a quality assurance system compliant with International Organization for Standardization-International Electrotechnical Commission (ISO/IEC) 17025 guidelines. Samples used in the validation were obtained from horses experimentally infected with Trichinella spiralis to obtain a range of muscle larvae densities. One-, 5-, and 10-g samples of infected tissue were combined with 99, 95, and 90 g, respectively, of known negative horse tissue to create a 100-g sample for testing. Samples of 5 and 10 g were more likely to be positive than were 1-g samples when larval densities were less than three larvae per gram (lpg). This difference is important because ingested meat with 1 lpg is considered the threshold for clinical disease in humans. Using a 5-g sample size, all samples containing 1.3 to 2 lpg were detected, and 60 to 100% of samples with infected horse meat containing 0.1 to 0.7 lpg were detected. In this study, the double separatory funnel digestion assay was efficient and reliable for its intended use in food safety and trade. This procedure is the only digestion assay for Trichinella in horse meat that has been validated as consistent and effective at critical levels of sensitivity.

Published

2008

10. Overview of food- and water-borne zoonotic parasites at the farm level.

Author

Gajadhar AA, Scandrett WB, and Forbes LB

Subjects

Animals, Commerce, Food Contamination, Humans, Life Cycle Stages, Protozoan Infections, Animal prevention & control, Protozoan Infections, Animal transmission, Consumer Product Safety, Food Handling methods, Food Parasitology, Meat parasitology, Protozoan Infections, Animal epidemiology

Abstract

Zoonotic parasites found in food animals include a wide variety of protozoa, nematodes, trematodes, and cestodes. Many of these parasites are emerging or already occur globally due to changes in farming practices and the increased movement of animals, food, and people. Some of the emerging or ubiquitous parasites, including Toxoplasma, Cryptosporidium, Trichinella, and Taenia, present enormous risks to global food production and consumer health. The parasite life cycle stages, such as eggs, oocysts, and cysts, typically resist adverse temperatures, desiccation, natural irradiation, chemicals, and disinfectants that are commonly used for controlling bacteria and viruses. Other important parasites include trematodes such as Clonorchis and Paragonimus, which are transmitted via fish or crustaceans and cause serious human disease in specific regions of the world. The potential for global occurrence of these parasites is increasing. Control of zoonotic parasites at the producer level requires education and the development and implementation of effective measures to eliminate the contamination of agricultural water and feed with viable stages of parasites. Standardisation, implementation, and documentation of control measures should increase confidence in global food trade.

Published

2006

11. A program to accredit laboratories for reliable testing of pork and horse meat for Trichinella.

Author

Forbes LB, Scandrett WB, and Gajadhar AA

Subjects

Accreditation standards, Animals, Canada, Food Inspection standards, Horses, Humans, Laboratories standards, Quality Control, Swine, Trichinellosis prevention & control, Food Inspection methods, Horse Diseases parasitology, Meat parasitology, Swine Diseases parasitology, Trichinella isolation & purification, Trichinellosis parasitology

Abstract

The Canadian Food Inspection Agency (CFIA) has developed a program to accredit external laboratories to conduct Trichinella digestion assays for export purposes. Accredited laboratories are responsible for staffing, equipment and operating test facilities under the auspices and guidance of the CFIA. The CFIA's Centre for Animal Parasitology provides training, proficiency samples, audits and other support for the accreditation process. The program has also been adapted for use in laboratories conducting Trichinella digestion tests for surveillance and food safety purposes and provides a useful template for others wishing to develop similar systems.

Published

2005

12. Comparison of synthetic tyvelose antigen with excretory-secretory antigen for the detection of trichinellosis in swine using enzyme-linked immunosorbent assay.

Author

Forbes LB, Appleyard GD, and Gajadhar AA

Subjects

Animals, Antibodies, Helminth blood, Enzyme-Linked Immunosorbent Assay methods, Female, ROC Curve, Sensitivity and Specificity, Swine, Swine Diseases immunology, Trichinella immunology, Trichinellosis diagnosis, Trichinellosis immunology, Antigens, Helminth immunology, Enzyme-Linked Immunosorbent Assay veterinary, Hexoses chemical synthesis, Hexoses immunology, Swine Diseases diagnosis, Trichinellosis veterinary

Abstract

Two enzyme-linked immunosorbent assay (ELISA) systems, one using natural excretory-secretory (ES) antigens and the other a synthetic glycan antigen (3,6-dideoxy-D-arabinohexose [tyvelose, TY]), were evaluated for the serological diagnosis of trichinellosis in swine. Sensitivity was estimated using samples (n = 113) collected 3-21 wk PI from 15 experimentally infected pigs, and specificity was estimated using samples (n = 397) from a population of Trichinella spp.-free pigs. Results were analyzed using 2 cutoff values recommended in international guidelines (Office Internationale des Epizooties [OIE]) and by the optimal cutoff level as determined by receiver-operator characteristic (ROC) analysis. The ROC-optimized TY-ELISA consistently performed better than all other combinations. None of the combinations of test and cut-off detected infected pigs sooner than 35 days; however, the ROC-optimized TY-ELISA identified 8 of 15 pigs earlier than the ES-ELISA and detected 2 pigs missed by all other tests. At 49 days PI the sensitivity and specificity of the ROC-optimized TY-ELISA were 94.3 and 96.7%, respectively, as compared with the ROC-optimized ES-ELISA at 84.9 and 96.0%, respectively. The ROC-optimized TY-ELISA was 100% specific at OIE-recommended cut-offs. This study indicates that the TY-ELISA is as good or better than the ES-ELISA for the detection of trichinellosis in swine.

Published

2004

13. A preliminary investigation on the infectivity of Trichinella larvae in traditional preparations of walrus meat.

Author

Leclair D, Forbes LB, Suppa S, Proulx JF, and Gajadhar AA

Subjects

Animals, Arctic Regions epidemiology, Disease Outbreaks, Humans, Larva pathogenicity, Quebec epidemiology, Trichinella genetics, Trichinellosis epidemiology, Meat parasitology, Trichinella isolation & purification, Trichinella pathogenicity, Walruses parasitology

Abstract

This study evaluated the infectivity of Trichinella nativa in freshly frozen walrus meat and traditionally aged walrus meat (igunaq) associated with two human outbreaks of trichinellosis in the Canadian Arctic. Trichinella larvae recovered from walrus meat stored at -20 degrees C for up to 20 months remained infective for guinea pigs inoculated with 135 or 716 larval doses. However, none of the 4-5 and 10-month-old igunaq preparations contained infective T. nativa larvae as measured by bioassays using mice and guinea pigs at inoculation doses ranging from 6 to 500 larvae. This indicates that the degradation process that occurred in the field can be sufficient to either kill Trichinella larvae or render them non-infective for mice and guinea pigs. Further research is needed to evaluate the food safety risk of traditional walrus igunaq aged under different field conditions and storage times.

Published

2004

14. Experimental Toxoplasma gondii infection in grey seals (Halichoerus grypus).

Author

Gajadhar AA, Measures L, Forbes LB, Kapel C, and Dubey JP

Subjects

Animals, Behavior, Animal, Brain parasitology, Cats, Disease Susceptibility veterinary, Feces parasitology, Female, Mice, Toxoplasmosis, Animal immunology, Toxoplasmosis, Animal physiopathology, Virulence, Seals, Earless parasitology, Toxoplasma pathogenicity, Toxoplasmosis, Animal parasitology

Abstract

Laboratory-reared animals were used to assess the susceptibility of seals (Halichoerus grypus) to Toxoplasma gondii infection. Four seals were each orally inoculated with 100 or 10,000 oocysts of T. gondii (VEG strain), and another 4 seals served as negative controls. Occasionally, mild behavioral changes were observed in all inoculated seals but not in control animals. A modified agglutination test revealed the presence of antibodies to T. gondii in sera collected from inoculated seals and mice inoculated as controls. No evidence of the parasite was found on an extensive histological examination of seal tissues, and immunohistochemical staining of tissue sections from inoculated seals revealed a single tissue cyst in only 1 seal. Control mice inoculated with 10 oocysts from the same inoculum given to seals became serologically and histologically positive for T. gondii. Cats that were fed brain or muscle tissue collected from inoculated seals passed T. gondii oocysts in feces. This study demonstrates that T. gondii oocysts can establish viable infection in seals and supports the hypothesis that toxoplasmosis in marine mammals can be acquired from oocysts in surface water runoff and sewer discharge.

Published

2004

15. Experimental Brucella abortus infection in wolves.

Author

Tessaro SV and Forbes LB

Subjects

Animals, Antibodies, Bacterial blood, Bison microbiology, Brucellosis epidemiology, Brucellosis pathology, Brucellosis transmission, Feces microbiology, Lymph Nodes microbiology, Lymph Nodes pathology, Male, Random Allocation, Saskatchewan, Time Factors, Brucella abortus isolation & purification, Brucella abortus pathogenicity, Brucellosis veterinary, Wolves

Abstract

Four juvenile male wolves (Canis lupus) each received an oral dose of 1.6-1.7 x 10(12) colony-forming units of Brucella abortus biovar 1 isolated from a bison (Bison bison) in Wood Buffalo National Park (Canada), and two others served as negative controls. Infected wolves did not show clinical signs of disease but did develop high Brucella antibody titers. Small numbers of B. abortus were excreted sporadically in feces until day 50 postinoculation (PI). Very small numbers of the bacterium were isolated from urine of only one wolf late on the same day that it was infected, and very small numbers of colonies of B. abortus were obtained from buccal swabs of three wolves for up to 48 hr PI. Two infected wolves euthanized 6 mo after the start of the experiment had no lesions, and colonies of B. abortus were isolated from thymus and most major lymph nodes. The other two infected wolves euthanized 12 mo after the start of the experiment had no lesions, and smaller numbers of brucellae were recovered from fewer lymph nodes compared with the wolves killed 6 mo earlier. The sporadic excretion of very small numbers of brucellae by the wolves was insignificant when compared with the infective dose for cattle. Brucella abortus, brucellosis, Canis lupus, pathogenesis, serology, wolf.

Published

2004

16. Infectivity of Trichinella nativa in traditional northern (country) foods prepared with meat from experimentally infected seals.

Author

Forbes LB, Measures L, Gajadhar A, and Kapel C

Subjects

Animals, Canada, Cats, Female, Food Parasitology, Humans, Larva, Male, Meat Products parasitology, Mice, Specific Pathogen-Free Organisms, Temperature, Time Factors, Trichinellosis transmission, Consumer Product Safety, Food Handling methods, Meat parasitology, Seals, Earless parasitology, Trichinella isolation & purification, Trichinella pathogenicity, Trichinellosis parasitology

Abstract

The infectivity of Trichinella nativa larvae in three traditional northern (country) foods was assessed. Foods were prepared with meat from seals experimentally infected with Trichinella nativa and evaluated over a 317-day period during which this food was fed directly to cats while mice were orally inoculated with larvae recovered following the digestion of the food in a solution containing 1% pepsin and 1% HCl at 37 degrees C. Foods examined were igunaq (meat and blubber placed in a seal skin bag and allowed to ferment), nikku (air-dried meat), and sausage (meat, fillers, salt, and spices). Sausage was examined both in a raw state and after partial cooking. Infective T. nativa larvae survived in igunaq, nikku, raw frozen sausage, and poorly cooked sausage for at least 5 months under controlled laboratory conditions. Core temperatures of partially cooked sausage never exceeded 50 degrees C. Caution should be exercised in using these data to establish guidelines for the consumption of raw products, since the survival of infective larvae could be unpredictably extended under field conditions. These data indicate significant food safety risks associated with igunaq, nikku, and sausage prepared with Trichinella-infected meat and provide information for use in risk management and in directing future research.

Published

2003

17. Comparison of a modified digestion assay with trichinoscopy for the detection of Trichinella larvae in pork.

Author

Forbes LB, Parker S, and Scandrett WB

Subjects

Animals, Muscles parasitology, Quality Control, Reproducibility of Results, Sensitivity and Specificity, Swine, Food Inspection methods, Food Parasitology, Meat parasitology, Trichinella isolation & purification

Abstract

A pepsin-HCl digestion assay and two compressorium techniques (trichinoscopy) for the identification of swine muscle tissue containing low levels of Trichinella larvae were compared as part of the test validation process for quality assurance purposes. Compressoria read with a stereomicroscope detected more larvae (P < 0.0001, n = 57) and more tissues (P = 0.0047, n = 57) than did compressoria read with a projection microscope (trichinoscope). The digestion assay evaluated was 3.2 times as likely as the best compressorium technique to identify a positive tissue when these procedures were used to test 1 g of infected muscle (P < 0.001; 95% confidence interval for the odds ratio, 2.0 to 5.4; n = 161 and n = 189, respectively). Detection by trichinoscopy improved as the number of larvae in tissues increased to > 2 larvae per g, but trichinoscopy was less sensitive than the digestion assay regardless of the tissue larval load. These data indicate that the quality controlled digestion assay used in this study is more sensitive than trichinoscopic techniques in the detection of tissues containing low levels of Trichinella larvae.

Published

2003

18. Evaluation of cattle for experimental infection with and transmission of Brucella suis biovar 4.

Author

Forbes LB and Tessaro SV

Subjects

Agglutination Tests veterinary, Animals, Antibodies, Bacterial blood, Brucella suis immunology, Brucellosis, Bovine blood, Brucellosis, Bovine microbiology, Cattle, Complement Fixation Tests veterinary, Diagnosis, Differential, Enzyme-Linked Immunosorbent Assay veterinary, Female, Male, Pregnancy, Brucella suis isolation & purification, Brucellosis, Bovine diagnosis, Brucellosis, Bovine transmission, Disease Transmission, Infectious veterinary, Infectious Disease Transmission, Vertical veterinary

Abstract

Objective: To determine whether cattle can become persistently infected with Brucella suis biovar 4, whether the organism can be transmitted vertically or horizontally, and whether tests for bovine brucellosis are diagnostic., Design: Observational study., Animals: 24 pregnant cows and their calves and 6 bulls., Procedure: Cows and bulls were housed separately in groups of 6 with each group consisting of 3 cattle experimentally infected with B suis biovar 4 and 3 naïve animals. Cattle were observed for clinical signs daily; blood samples were collected weekly. Clotted blood from each sample was submitted for bacterial culture. Serum was tested with an indirect ELISA and the standard tube agglutination test (STAT), buffered plate agglutination test, brucellosis card test (BCT), and complemen't fixation test (CFT). Tissues collected at necropsy were submitted for bacterial culture and histologic examination., Results: All 15 inoculated cattle seroconverted on 2 or more serologic tests, and bacteria were isolated from 4 inoculated cows at necropsy. There was no bacteriologic evidence of vertical or horizontal transmission, and none of the cattle developed clinical abnormalities or gross or histologic lesions. Results of the indirect ELISA were positive for all inoculated cattle. The other tests gave variable results; the CFT, STAT, and BCT yielded negative results for at least 1 of the 4 cattle from which the organism was isolated., Conclusions and Clinical Relevance: Results suggest that cattle-to-cattle transmission of B suis biovar 4 is unlikely. Serologic tests for bovine brucellosis should be used cautiously when attempting to identify cattle with rangiferine brucellosis, as they do not discriminate between the 2 diseases and vary in their ability to detect exposed cattle.

Published

2003

19. Evaluation of a digestion assay and determination of sample size and tissue for the reliable detection of Trichinella larvae in walrus meat.

Author

Leclair D, Forbes LB, Suppa S, and Gajadhar AA

Subjects

Animals, Diaphragm parasitology, Larva, Muscle, Skeletal parasitology, Sample Size, Tongue parasitology, Trichinellosis diagnosis, Trichinellosis veterinary, Food Parasitology, Meat parasitology, Trichinella isolation & purification, Walruses parasitology

Abstract

A digestion assay was validated for the detection of Trichinella larvae in walrus (Odobenus rosmarus) meat, and appropriate samples for testing were determined using tissues from infected walruses harvested for food. Examination of muscles from 3 walruses showed that the tongue consistently contained approximately 2-6 times more larvae than the pectoral and intercostal muscles. Comparison of numbers of larvae in the root, body, and apex of the tongue from 3 walruses failed to identify a predilection site within the tongue, but the apex was considered an optimal tissue because of the high larval density within the tongue and the ease of collection. All 31 spiked samples weighing 50 g each and containing between 0.1 and 0.4 larvae per gram (lpg) were correctly identified as infected, indicating that the sensitivity of this procedure is adequate for diagnostic use. A sample size of 10 g consistently detected larvae in 2 walrus tongues containing > or = 0.3 lpg (n = 40), and until additional data are available, sample sizes from individual walrus tongues should be a minimum of 10 g. This study provides the preliminary data that were used for the development of a food safety analytical protocol for the detection of Trichinella in walrus meat in arctic communities.

Published

2003

20. National serologic survey for trichinellosis in sows in Canada 1996-1997.

Author

Appleyard GD, Forbes LB, and Gajadhar AA

Subjects

Animals, Antibodies, Helminth blood, Canada epidemiology, Enzyme-Linked Immunosorbent Assay veterinary, Female, Prevalence, Seroepidemiologic Studies, Swine, Swine Diseases blood, Swine Diseases diagnosis, Trichinella immunology, Trichinella isolation & purification, Trichinellosis blood, Trichinellosis diagnosis, Trichinellosis epidemiology, Swine Diseases epidemiology, Trichinellosis veterinary

Abstract

Sera from 14,408 market sows from the Canadian domestic swine herd were tested for trichinellosis using an indirect-ELISA as a screening test and a competitive ELISA for confirmatory testing. Three sera (0.02%) gave low level reactions on the competitive ELISA. These reactions were considered nonspecific, and this designation was supported by data from previous and subsequent national surveys, in which serologic, trichinoscopic, and digestion test methodologies was used. This study provides additional evidence that Canada is free of trichinellosis in domestic swine.

Published

2002

21. An internationally recognized quality assurance system for diagnostic parasitology in animal health and food safety, with example data on trichinellosis.

Author

Gajadhar AA and Forbes LB

Subjects

Animal Welfare, Animals, Feces parasitology, Food Handling standards, Horses, International Cooperation, Meat standards, Quality Control, Reproducibility of Results, Safety, Swine, Trichinella isolation & purification, Trichinellosis diagnosis, Food Inspection standards, Food Parasitology standards, Meat parasitology, Trichinellosis veterinary

Abstract

A quality assurance (QA) system was developed for diagnostic parasitology and implemented for several diagnostic assays including fecal flotation and sedimentation assays, trichomonad culture assay, and the testing of pork and horse meat for Trichinella to facilitate consistently reliable results. The system consisted of a validated test method, procedures to confirm laboratory capability, and protocols for documentation, reporting, and monitoring. Specific system components included a quality assurance manual, training program, proficiency panels, inter-laboratory check-sample exchange program, assay critical control points, controls, and audits. The quality assurance system of the diagnostic laboratory was audited according to ISO/IEC Standard 17025 by an international third party accrediting body and accredited as a testing laboratory for the specific parasitology tests. Test results generated from the laboratory were reliable and scientifically defensible according to the defined parameters of the tests and were therefore valid for a variety of purposes, including food safety, international trade, and declaration of disease status in an animal, herd, farm, or region. The system was applicable to various test methods for the detection of parasites in feces or other samples, and a digestion test system developed for Trichinella was used as an example. A modified tissue digestion assay was developed, validated, and implemented by the Canadian Food Inspection Agency's Centre for Animal Parasitology for efficiency and quality assurance. The details of the method were properly documented for routine testing and consisted of a homogenization process, an incubation at 45+/-2 degrees C, and two sequential sedimentations in separatory funnels to concentrate and clarify final aliquots for microscopic examination. To facilitate consistently reliable test results, 14 critical control points were identified and monitored, analysts were certified, and the test system verified through the use of validation data, proficiency samples, and training modules.

Published

2002

22. The occurrence and ecology of Trichinella in marine mammals.

Author

Forbes LB

Subjects

Animals, Caniformia parasitology, Ecology, Food Parasitology, Humans, Meat parasitology, Trichinella, Trichinellosis epidemiology, Ursidae parasitology, Mammals parasitology, Trichinellosis veterinary

Abstract

Trichinella in marine mammals has a circumpolar arctic distribution and a narrow range of host species. It is commonly found in polar bears (Ursus maritimus), and increasingly in walruses (Odobenus rosmarus) where it presents a significant zoonotic hazard. This has resulted in the implementation of food safety programs in some arctic communities to test harvested walrus meat for Trichinella larvae prior to consumption. Trichinella has been reported infrequently in bearded seals (Erignathus barbatus) and ringed seals (Phoca hispida), and was once observed in a Beluga whale (Delphinapterus leucas). Cannibalism is probably the most important factor in maintaining a Trichinella cycle in polar bears. Arctic carnivores such as polar bears, arctic foxes (Alopex lagopus) and domestic dogs (Canis familiaris) have a high prevalence of Trichinella infection and the carcasses of at least some of these animals are deposited in the ocean. Scavenging of these carcasses by walruses probably occurs, but may not account for the high prevalence the parasite seen in this host species. Predation, carrion feeding and cannibalism have been documented for walruses and a sylvatic cycle similar to that of bears may exist in walrus populations. Seals and whales are likely infected through infrequent exposure to infected carcasses, either directly by scavenging or indirectly by consuming amphipods or fish that have fed on infected carcasses. The inefficiency of this mechanism may account for the low prevalence of Trichinella in seals and whales. It is known that isolates from marine mammals are cold tolerant, and infectious for man, and have been identified as Trichinella nativa (T2). Molecular and other phylogenetic studies would be useful to facilitate studies on the inter-relationship of Trichinella cycles involving marine and terrestrial mammals in the arctic and subarctic, and in the investigation of human outbreaks of trichinellosis in these areas.

Published

2000

23. Brucellosis in ringed seals and harp seals from Canada. lforbes@em.agr.ca.

Author

Forbes LB, Nielsen O, Measures L, and Ewalt DR

Subjects

Animals, Arctic Regions epidemiology, Brucella classification, Brucellosis epidemiology, Canada epidemiology, Lymph Nodes microbiology, Brucella isolation & purification, Brucellosis veterinary, Seals, Earless

Abstract

A novel Brucella sp. was isolated from lymph nodes of four ringed seals (Phoca hispida) collected near Pangnirtung (Baffin Island, Canada) in January and February 1995 and in one harp seal (Phoca groenlandica) collected near the Magdalen Islands (Gulf of St. Lawrence, Canada) in March 1996. Bacteriological characteristics were the same for all five isolates. The colonies were typical of Brucella spp., but took 2 to 5 days longer than the traditional species to appear on primary isolation media. Biotyping results did not match any of the known biovars of Brucella, but were similar to isolates of the genus Brucella previously reported from marine mammals inhabiting other areas of the northern hemisphere. This is the first confirmed report of brucellosis in marine mammals from Canada, and the first report of this organism in ringed and harp seals.

Published

2000

24. A validated Trichinella digestion assay and an associated sampling and quality assurance system for use in testing pork and horse meat.

Author

Forbes LB and Gajadhar AA

Subjects

Animals, Horses, Larva, Quality Control, Swine, Food Handling standards, Food Parasitology, Meat parasitology, Trichinella isolation & purification

Abstract

A revised digestion method, developed for efficiency and quality assurance, was validated for the detection of Trichinella larvae in pork and horse meat to meet requirements for food safety testing and facilitate access to international markets. The method consisted of a tissue homogenization step and a spin bar digestion procedure conducted at 45 degrees C to free larvae from muscle tissue, followed by two sequential separatory funnel steps to concentrate the larvae for detection using a stereomicroscope. Critical control points were determined for the method and monitored during testing. Under conditions of a defined protocol, test capacity was suitable for industrial applications, since multiples of up to 100 g of tissue could be analyzed at one time. The overall sensitivity of the test system depended on the size and origin of the sample taken from individual infected carcasses. Data from swine indicated that the currently accepted sample size of 1 g from individual carcasses consistently detected larval loads of > or =3 larvae per gram. Larval loads of 1.0 to 1.9 larvae per gram required 3- to 5-g samples of muscle tissue for reliable detection. Five-gram samples were considered optimal, because they consistently detected more tissues than 3-g samples, although the difference was not statistically significant. Tissue localization studies in experimental pigs indicated that the tongue and diaphragm were the tissues of choice for the most sensitive larval recovery. A system of analyst training, laboratory certification based on ISO guide 25, and on-site proficiency panel testing was used to ensure that external laboratories would consistently produce reliable test results. The system developed for pork was successfully modified for the testing of horse meat.

Published

1999

25. Proficiency samples for quality assurance in Trichinella digestion tests.

Author

Forbes LB, Rajic A, and Gajadhar AA

Subjects

Animals, Cattle, Meat standards, Meat Products standards, Quality Control, Rats, Swine parasitology, Trichinella spiralis growth & development, Food Inspection standards, Food Parasitology standards, Meat parasitology, Meat Products parasitology, Trichinella spiralis isolation & purification

Abstract

A reliable method to produce proficiency samples containing known numbers of Trichinella spiralis cysts for use in quality assurance systems for Trichinella digestion tests was developed and validated. A filtrate containing Trichinella cysts was produced by homogenizing and filtering the muscles of an experimentally infected rat. Using a stereomicroscope and micropipette, intact cysts were removed from the filtrate and were transferred onto an agar substrate to allow accurate counting and subsequent transfer into a sample matrix. The proficiency sample matrix consisted of 20-g balls of lean ground beef and was combined with 80 g of a Trichinella-free muscle tissue to obtain the required 100-g sample weight for the assay. The mean overall larval recovery from 404 proficiency samples was 93.0%. Larval recoveries > or = 95, 85, and 75% occurred in 52.4, 84.4, and 94.3%, respectively, of the 404 samples tested. Results indicated that, after a short training period, technicians with no prior experience in digestion techniques performed as well as experienced technicians. The maximum shelf life of proficiency samples was not determined but was at least 3 weeks. Validation data were used to develop panels composed of proficiency samples prepared as described above and to establish guidelines for the interpretation of proficiency panel results.

Published

1998

26. Infection of cattle with Brucella abortus biovar 1 isolated from a bison in Wood Buffalo National Park.

Author

Forbes LB and Tessaro SV

Subjects

Animals, Brucellosis epidemiology, Brucellosis etiology, Cattle Diseases epidemiology, Female, Pregnancy, Saskatchewan epidemiology, Bison microbiology, Brucella abortus isolation & purification, Brucellosis veterinary, Cattle microbiology, Cattle Diseases etiology

Abstract

An experiment was conducted to determine if cattle could be infected with a strain of Brucella abortus biovar 1 isolated from a bison in Wood Buffalo National Park. Three pregnant cows inoculated conjunctivally with 5.7 x 10(8) cfu of the bacterium, and their subsequent calves, showed seroconversion on standard serological tests for bovine brucellosis, and large numbers of the bacterium were isolated from numerous tissues at necropsy. A 4th cow that was moved into the pen that previously contained the inoculated cows subsequently showed seroconversion, and the same strain of B. abortus biovar 1 was isolated from numerous tissues. Although this strain from bison in Wood Buffalo National Park has existed in isolation from cattle for over 60 years, it remains infectious and contagious for cattle.

Published

1996

27. Experimental studies on Brucella abortus in moose (Alces alces).

Author

Forbes LB, Tessaro SV, and Lees W

Subjects

Agglutination Tests veterinary, Animals, Antibodies, Bacterial blood, Blood Cell Count veterinary, Blood Chemical Analysis veterinary, Brucella abortus immunology, Brucellosis immunology, Brucellosis pathology, Complement Fixation Tests veterinary, Disease Susceptibility, Female, Joints pathology, Liver pathology, Lymph Nodes pathology, Male, Brucella abortus pathogenicity, Brucellosis veterinary, Deer

Abstract

Four moose (Alces alces) were inoculated conjunctivally with B. abortus biovar 1 to determine their susceptibility to brucellosis, and to describe the serology, bacteriology, hematology, clinical chemistry, and pathology associated with infection. All moose became infected. Two moose were killed at day 70 post-exposure, one (83F) died acutely at day 85, and one was killed at day 166. None of the moose had clinical signs, except for 83F immediately before death. Infected moose were readily detected serologically by the buffered antigen plate test, Brewer card test, standard tube agglutination test, and complement fixation test as used for brucellosis in cattle. With the exception of samples from 83F taken 24 hours before death, clinical chemistry, and hematology results were stable for all moose, and similar to normal values seen in cattle. Lesions seen in all moose were indicative of endotoxemia, and moose 83F died of acute endotoxic shock. Brucella abortus biovar 1 was isolated from several tissues in all moose, most notably from lymph nodes where counts often exceeded 4 x 10(4) colony forming units per g of tissue. Thus infection with B. abortus will kill moose, and progression of the disease is likely rapid under field conditions. Moose appear to be a dead-end host for brucellosis.

Published

1996

28. The brucellosis and tuberculosis status of wood bison in the Mackenzie Bison Sanctuary, Northwest Territories, Canada.

Author

Tessaro SV, Gates CC, and Forbes LB

Subjects

Animals, Brucellosis epidemiology, Female, Likelihood Functions, Male, Northwest Territories epidemiology, Pregnancy, Pregnancy Complications, Infectious epidemiology, Prevalence, Tuberculosis epidemiology, Bison, Brucellosis veterinary, Pregnancy Complications, Infectious veterinary, Tuberculosis veterinary

Abstract

Postmortem examinations were done on 51 wood bison (Bison bison athabascae) killed as part of a multidisciplinary research project in the Mackenzie Bison Sanctuary, Northwest Territories, Canada, between 1986 and 1988. There was no gross, histological or bacteriological evidence of brucellosis or tuberculosis in these bison. Traumatic lesions were seen in one calf that had been attacked by wolves and a second calf that had been gored. Antibody titers to Brucella abortus were not found in sera from these 51 animals or an additional 112 wood bison that were chemically-immobilized or killed in the Sanctuary between 1986 and 1990. The combined prevalence of the diseases in the population could not have exceeded 5.95% for the necropsy survey to have missed finding at least one infected animal, and the prevalence of brucellosis in the population would have had to be less than 1.95% for the broader serological survey to have failed to find at least one reactor animal on the battery of tests. These results, and the cumulative epidemiological information on brucellosis and tuberculosis in bison, indicate that bovine brucellosis and tuberculosis are not enzootic in the wood bison population in and around the Mackenzie Bison Sanctuary, and suggest that the population is free of these diseases. However, this expanding population is at risk of contracting both diseases from the infected bison population in and around nearby Wood Buffalo National Park.

Published

1993

29. Transmission of brucellosis from reindeer to cattle.

Author

Forbes LB and Tessaro SV

Subjects

Abortion, Veterinary etiology, Animals, Antibodies, Bacterial blood, Brucella immunology, Brucella isolation & purification, Brucellosis transmission, Cattle, Female, Male, Pregnancy, Pregnancy Complications, Infectious, Brucellosis veterinary, Brucellosis, Bovine etiology, Reindeer

Abstract

Sixteen reindeer (Rangifer tarandus tarandus) naturally infected with Brucella suis biovar 4 were penned with 6 male and 2 female cattle for 30 days, then removed and euthanatized. During this period, 5 reindeer had fawns, and 2 reindeer aborted. Brucella suis biovar 4 was recovered from all adult reindeer at necropsy. Nine reindeer had B suis biovar 4 in uterus, udder, and/or milk. The cattle were euthanatized 2 months after the reindeer were removed. Clinical or pathologic signs of disease were not observed in the cattle. Brucella suis biovar 4 was isolated from 2 male and from both female cattle at necropsy. The female cattle had positive reactions on the buffered plate antigen test, brucellosis card test, tube agglutination test, complement fixation test, and indirect enzyme immunoassay for most of the experiment, but the males had inconsistent reactions on these tests. The indirect enzyme immunoassay was the only test to detect all cattle from which bacteria were cultured. This study revealed that caution is warranted before moving reindeer or caribou into areas of traditional agriculture.

Published

1993

30. Isolates of Brucella suis biovar 4 from animals and humans in Canada, 1982-1990.

Author

Forbes LB

Published

1991

31. Brucella abortus infection in 14 farm dogs.

Author

Forbes LB

Subjects

Agglutination Tests veterinary, Animals, Brucella abortus classification, Brucellosis transmission, Dog Diseases immunology, Dogs, Female, Male, Serotyping veterinary, Time Factors, Brucella abortus isolation & purification, Brucellosis veterinary, Disease Vectors, Dog Diseases transmission

Abstract

Fourteen dogs were obtained from 10 farms with Brucella-infected cattle and were studied for periods ranging from 2 to 81 days. At necropsy, Brucella abortus biovar 4 was isolated from all 14 dogs. Mandibular, medial retropharyngeal, tracheobronchial, and mesenteric lymph nodes yielded the highest rate of recovery. Urogenital infection with active shedding was seen in a single aged bitch. Fecal samples (291 from 13 dogs) were B abortus culture negative. Ten dogs monitored serologically over time had standard tube agglutination test titers that fluctuated between 1:50 with incomplete reaction and greater than or equal to 1:200 with positive reaction. At necropsy, the magnitude of seroconversion was not directly related to the number of culture-positive tissues. The maximal duration of infection, based on the time interval between the last possible exposure to infected cattle and recovery of the organism at necropsy, was 464 days. If it were assumed that infection occurred at about the same time as seroconversion in the cattle herd of origin, maximal observed duration of infection was 539 days. The actual maximal duration of infection could not be determined from this study, but would have exceeded the values reported here. The data indicate that dogs have the potential to infect cattle and could pose a threat for longer duration of disease transmission than had previously been assumed. Although the risk of transmission appears small, infection of human beings or cattle associated with Brucella-infected dogs would cause unfavorable political and economic consequences, particularly in low-incidence areas. Removal of contact dogs from infected herds should prevent such transmission.

Published

1990

32. A survey of brucellosis and tuberculosis in bison in and around Wood Buffalo National Park, Canada.

Author

Tessaro SV, Forbes LB, and Turcotte C

Abstract

Examinations of complete or partial remains of 72 bison found dead in and around Wood Buffalo National Park, Canada, revealed evidence of brucellosis in 18 (25%) and tuberculosis in 15 (21%), with a combined prevalence of 42%. Urease-positive and ureasenegative strains of Brucella abortus biovar 1, and strains of biovar 2, were isolated from tissues of bison, including synovium and exudate from severe arthritic lesions. Mycobacterium bovis was isolated from a range of granulomatous lesions that were similar to those reported in tuberculous cattle. Diseased bison had a broad geographical distribution, and were found outside the park on at least three natural corridors. The diseases have a deleterious effect on this population of bison, and pose a health risk to other bison herds, livestock, and native hunters in the region.

Published

1990

33. Atypical isolates of Brucella abortus from Canada and the United States characterized as dye sensitive with M antigen dominant.

Author

Ewalt DR and Forbes LB

Subjects

Animals, Antigens, Bacterial analysis, Brucella abortus immunology, Brucella abortus isolation & purification, Brucella abortus pathogenicity, Canada, Cattle, Coloring Agents pharmacology, Guinea Pigs, Male, United States, Virulence, Brucella abortus classification, Brucellosis, Bovine microbiology

Abstract

A total of 41 Brucella isolates, examined by standard biotyping procedures, were found to be similar to Brucella abortus biovar 2 in dye sensitivity but had a dominant M antigen. Oxidative metabolic tests performed on 39 of the isolates confirmed them as B. abortus. Additional biochemical and bacteriophage susceptibility studies were performed on 35 of the isolates. The isolates had identical reactions in the various tests, except for one isolate which was resistant to lysis by all phage strains used. Two isolates were injected into guinea pigs and shown to be virulent. The isolates described in this study appear similar to atypical Brucella isolates previously reported in the United Kingdom and the United States and may form the basis of a new biovar, B. abortus biovar 10.

Published

1987

34. Brucella canis Isolates from Canadian Dogs.

Author

Forbes LB and Pantekoek JF

Abstract

Eleven Brucella canis isolates from Canadian dogs were characterized by dye and antibiotic sensitivity, phage susceptibility, urease and H(2)S production, CO(2) requirement, and reaction with monospecific A,M, and R anti-Brucella antiserum. The isolates could be separated into two distinct groups. One group had a sensitivity pattern similar to that seen with the American type strain RM666, while the other group had a pattern identical to that of a Mexican strain, Mex 51. Epidemiological studies supported contraction of infections in the United States and Mexico respectively. The characteristics of all isolates were stable after repeated subculture indicating that strain differences could serve as useful epidemiological markers and supporting division of the species into two biovars.

Published

1988

35. A comparison of five serological tests for bovine brucellosis.

Author

Dohoo IR, Wright PF, Ruckerbauer GM, Samagh BS, Robertson FJ, and Forbes LB

Subjects

Agglutination Tests, Animals, Cattle, Complement Fixation Tests, False Positive Reactions, Hemolytic Plaque Technique, Immunoenzyme Techniques, Predictive Value of Tests, Brucellosis, Bovine diagnosis

Abstract

Five serological assays: the buffered plate antigen test, the standard tube agglutination test, the complement fixation test, the hemolysis-in-gel test and the indirect enzyme immunoassay were diagnostically evaluated. Test data consisted of results from 1208 cattle in brucellosis-free herds, 1578 cattle in reactor herds of unknown infection status and 174 cattle from which Brucella abortus had been cultured. The complement fixation test had the highest specificity in both nonvaccinated and vaccinated cattle. The indirect enzyme immunoassay, if interpreted at a high threshold, also exhibited a high specificity in both groups of cattle. The hemolysis-in-gel test had a very high specificity when used in nonvaccinated cattle but quite a low specificity among vaccinates. With the exception of the complement fixation test, all tests had high sensitivities if interpreted at the minimum threshold. However, the sensitivities of the standard tube agglutination test and indirect enzyme immunoassay, when interpreted at high thresholds were comparable to that of the complement fixation test. A kappa statistic was used to measure the agreement between the various tests. In general the kappa statistics were quite low, suggesting that the various tests may detect different antibody isotypes. There was however, good agreement between the buffered plate antigen test and standard tube agglutination test (the two agglutination tests evaluated) and between the complement fixation test and the indirect enzyme immunoassay when interpreted at a high threshold. With the exception of the buffered plate antigen test, all tests were evaluated as confirmatory tests by estimating their specificity and sensitivity on screening-test positive samples.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1986

36. Characterization of an atypical biotype of Brucella abortus.

Author

Garcia MM, Brooks BW, Ruckerbauer GM, Rigby CE, and Forbes LB

Subjects

Animals, Bacterial Proteins analysis, Bacterial Typing Techniques, Brucella abortus analysis, Brucella abortus growth & development, Brucella abortus immunology, Cattle, Electrophoresis, Polyacrylamide Gel, Immunoblotting, Milk microbiology, Brucella abortus classification, Brucellosis, Bovine microbiology

Abstract

Brucella abortus strains were isolated from bovine tissue and milk samples from seven Ontario herds. The isolates were characterized by colonial morphology, requirement of CO2 for growth, lysis by Tbilisi phage, biochemical tests and agglutination in monospecific sera. They resembled B. abortus biotype 2 (on the basis of sensitivity to thionin and basic fuchsin) and biotype 4 (on the basis of agglutination with anti-Brucella "M" but not anti-Brucella "A" absorbed sera). Sodium dodecyl sulphate-polyacrylamide gel electrophoresis of these isolates and B. abortus biotypes 1, 2 and 4 showed similar profiles. Immunoblots with anti-A and anti-M absorbed sera showed different antigenic regions reacting with the specific sera and also confirmed that the atypical B. abortus isolates were serologically similar to biotype 4.

Published

1988

37. A comparison of standard serological tests for the diagnosis of bovine brucellosis in Canada.

Author

Stemshorn BW, Forbes LB, Eaglesome MD, Nielsen KH, Robertson FJ, and Samagh BS

Subjects

Animals, Canada, Cattle, Diagnostic Errors, Evaluation Studies as Topic, Serologic Tests, Agglutination Tests veterinary, Brucellosis, Bovine diagnosis, Complement Fixation Tests veterinary

Abstract

Six agglutination and two complement fixation tests were compared with respect to specificity, sensitivity and relative sensitivity for the serodiagnosis of bovine brucellosis. Based on 1051 sera from brucellosis free herds, the specificity of the tests was 98.9% for the buffered plate antigen test (BPAT), 99.2% and 99.3% for the standard tube and plate agglutination tests (STAT and SPAT), respectively, and 99.8% for the 2-mercaptoethanol test (2MET). On this small sample, the rose bengal plate test (RBPT), card test (CARD) and the complement fixation test (CFT) correctly classed all sera as negative. On a sample of 167 culture positive cattle, the sensitivities of the tests were CFT: 79.0%, BPAT: 75.4, RBPT: 74.9%, CARD: 74.3%, SPAT: 73.1%, STAT: 68.9%, and 2MET: 59.9%. All tests combined detected only 82% of these infected cattle. Analysis of the relative sensitivity of the six agglutination tests gave the following ranking: BPAT greater than RBPT greater than CARD greater than SPAT greater than STAT. The 2MET ranked between the BPAT and RBPT or between the RBPT and CARD depending on the analysis used. The use of the BPAT as a screening test is recommended provided that a test of high specificity and sensitivity such as the CFT is used to confirm screening test reactions.

Published

1985

38. Brucella suis biotype 4: a case of granulomatous nephritis in a barren ground caribou (Rangifer tarandus groenlandicus L.) with a review of the distribution of rangiferine brucellosis in Canada.

Author

Tessaro SV and Forbes LB

Subjects

Animals, Brucella classification, Brucella isolation & purification, Brucellosis epidemiology, Brucellosis pathology, Canada, Nephritis microbiology, Nephritis pathology, Brucellosis veterinary, Nephritis veterinary, Reindeer microbiology

Abstract

Severe granulomatous nephritis caused by Brucella suis biotype 4 was found in a barren ground caribou (Rangifer tarandus groenlandicus) from Northwest Territories, Canada. A review of the distribution of human and animal cases of brucellosis in northern Canada indicated that B. suis biotype 4 is distributed widely and is probably enzootic in most Canadian caribou herds.

Published

1986

39. Evaluation of an enzyme-labeled antiglobulin test for anti-Brucella immunoglobulin G among 3 cattle populations.

Author

Stemshorn BW, Nielsen KH, Samagh BS, Forbes LB, and Ingram DG

Subjects

Agglutination Tests, Animals, Brucellosis, Bovine immunology, Complement Fixation Tests, Brucella abortus immunology, Cattle immunology, Coombs Test, Immunoenzyme Techniques, Immunoglobulin G analysis

Abstract

Antibody to smooth Brucella abortus lipopolysaccharide antigen on the surface of polystyrene tubes was detected with peroxidase-labeled antibody against bovine immunoglobulin G. The enzyme-labeled antiglobulin test (ELAT) activity of samples was expressed in arbitrary units/0.01 ml by reference to a standard curve based on tests of dilutions of a positive serum pool. Reactions greater than 3.0 U/0.01 ml were classified positive because specificity at this level was 99.8% (417/418 samples correctly classified negative) with agglutination test-negative sera from 33 Brucella-free herds. Results of the ELAT were compared with results of agglutination tests and the complement-fixation test (CFT), using 430 sera from cattle in 7 infected herds. Activity of greater than 5.0 ELAT U/0.01 ml was detected in all 54 sera classified as positive (titer greater than 1:10) by the CFT, including 5 sera classified as negative by the tube agglutination test. Sera from 8 nonvaccinated cows in the infected herds reacted only by the ELAT, whereas reactions were obtained with 25 and 5 sera by only agglutination tests and the CFT, respectively. The ELAT and CFT results were in agreement for 25 of 26 sera from agglutination test-reactor cattle in herds of unknown status. Comparisons of milk ring and whey agglutination tests with the whey ELAT on 146 quarter samples from cows in an infected herd revealed no ELAT activity greater than or equal to 1.0 U/0.01 ml in the 73 samples considered negative by the 2 other tests. Samples (n = 47) that contained greater than or equal to 1.0 ELAT U/0.01 ml included all (n = 40) samples with milk ring or whey agglutination titers greater than or equal to 1:16 and greater than or equal to 32, respectively, and 7 samples that gave weaker reactions to the latter tests.

Published

1980

40. An outbreak of Brucella abortus biovar 2 in Canadian cattle.

Author

Forbes LB and Steele TB

Abstract

An outbreak of brucellosis caused by Brucella abortus biovar 2 was identified in cattle in Alberta in December 1986. This was the only clinical infection discovered since the national cattle herd was declared brucellosisfree in 1985. It was the first report of B. abortus biovar 2 in Canadian cattle. The outbreak, involving three herds containing purebred Hereford cattle, was spread by the private treaty sale of untested cattle, and was identified following investigation of an abortion. The source of infection for the outbreak was not established, but several possibilities were identified including infected herds present in the area during the mid-1970's, latent infection originating in a Saskatchewan herd during the early 1960's, American cattle imported during the early 1970's, and brucellosis-infected bison in Wood Buffalo National Park. The containment and elimination of this nidus of infection appears to have been successful, and the national cattle herd at the time of writing is free of the disease.

Published

1989

41. Rangiferine brucellosis in a Muskox, Ovibos moschatus moschatus (Zimmermann).

Author

Gates CC, Wobeser G, and Forbes LB

Subjects

Animals, Animals, Wild, Brucellosis diagnosis, Brucellosis transmission, Canada, Male, Species Specificity, Artiodactyla, Brucella isolation & purification, Brucellosis veterinary

Published

1984