Your search keyword '"Bosward KL"' showing total 85 results

1. Communicating the risks of handling bats: analysing approaches used by Australian stakeholders in the context of Australian bat lyssavirus

Author

Liang, BP, primary, Wingett, K, additional, Bosward, KL, additional, and Taylor, MR, additional

Published

2023

2. Canine superficial bacterial pyoderma: evaluation of skin surface sampling methods and antimicrobial susceptibility of causalStaphylococcusisolates

Author

Ravens, PA, primary, Vogelnest, LJ, additional, Ewen, E, additional, Bosward, KL, additional, and Norris, JM, additional

Published

2014

3. Erratum

Author

Lepherd, ML, primary, Canfield, PJ, additional, Hunt, GB, additional, Thomson, PC, additional, and Bosward, KL, additional

Published

2011

4. Wound healing after mulesing and other options for controlling breech flystrike in Merino lambs: quantitative and semiquantitative analysis of wound healing and wound bed contraction

Author

Lepherd, ML, primary, Canfield, PJ, additional, Hunt, GB, additional, Thomson, PC, additional, and Bosward, KL, additional

Published

2011

5. Wound healing after mulesing and other options for controlling breech flystrike in Merino lambs: observations on gross and microscopic wound healing

Author

Lepherd, ML, primary, Canfield, PJ, additional, Hunt, GB, additional, Thomson, PC, additional, and Bosward, KL, additional

Published

2011

6. Assessment of the short-term systemic effect of and acute phase response to mulesing and other options for controlling breech flystrike in Merino lambs

Author

Lepherd, ML, primary, Canfield, PJ, additional, Hunt, GB, additional, Thomson, PC, additional, and Bosward, KL, additional

Published

2011

7. Cytopathological and histopathological diagnosis of canine splenic disorders

Author

Christensen, NI, primary, Canfield, PJ, additional, Martin, PA, additional, Krockenberger, MB, additional, Spielman, DS, additional, and Bosward, KL, additional

Published

2009

8. Haematological, biochemical and selected acute phase protein reference intervals for weaned female Merino lambs

Author

Lepherd, ML, primary, Canfield, PJ, additional, Hunt, GB, additional, and Bosward, KL, additional

Published

2009

9. Elapid snake envenomation in dogs in New South Wales: a review

Author

Heller, J, primary, Mellor, DJ, additional, Hodgson, JL, additional, Reid, SWJ, additional, Hodgson, DR, additional, and Bosward, KL, additional

Published

2007

10. WHAT IS YOUR DIAGNOSIS?

Author

BOSWARD, KL, primary, RICH, S, additional, WHITE, JD, additional, MARTIN, P, additional, and MALIK, R, additional

Published

2007

11. Anuric renal failure in a dog after Red-bellied Black snake (Pseudechis porphyriacus) envenomation

Author

HELLER, J., primary, BOSWARD, KL, additional, HODGSON, DR, additional, and POTTIE, R., additional

Published

2006

12. Clinicopathological findings associated with feline infectious peritonitis in Sydney, Australia: 42 cases (1990–2002)

Author

NORRIS, JM, primary, BOSWARD, KL, additional, WHITE, JD, additional, BARAL, RM, additional, CATT, MJ, additional, and MALIK, R., additional

Published

2005

13. Snake envenomation in dogs in New South Wales

Author

HELLER, J., primary, BOSWARD, KL, additional, HODGSON, JL, additional, COLE, FL, additional, REID, SWJ, additional, HODGSON, DR, additional, and MELLOR, DJ, additional

Published

2005

14. Squamous cell carcinoma with sarcomatous stroma in the nasal cavity of a dog

Author

BOSWARD, KL, primary, KESSELL, AE, additional, and LUCY, RJ, additional

Published

2004

15. Acute febrile neutrophilic vasculitis of the skin of young Shar-Pei dogs

Author

MALIK, R, primary, FOSTER, SF, additional, MARTIN, P, additional, CANFIELD, PJ, additional, MASON, KV, additional, BOSWARD, KL, additional, GOUGH, A, additional, and RIPPON, G, additional

Published

2002

16. WHAT IS YOUR DIAGNOSIS?

Author

BOSWARD, KL, RICH, S, WHITE, JD, MARTIN, P, and MALIK, R

Published

2006

17. Engaging livestock clinical staff through research and collaboration.

Author

House JK, Rowe SM, Zadoks RN, Bosward KL, Sheehy PA, Brookes V, and Norris JM

Subjects

Animals, Livestock, Cooperative Behavior

Published

2023

18. Risk factors associated with self-reported Q fever in Australian wildlife rehabilitators: Findings from an online survey.

Author

Mathews KO, Savage C, Norris JM, Phalen D, Malikides N, Sheehy PA, and Bosward KL

Subjects

Humans, Animals, Animals, Wild, Australia epidemiology, Self Report, Cross-Sectional Studies, Surveys and Questionnaires, Ruminants, Risk Factors, Q Fever microbiology, Q Fever veterinary, Coxiella burnetii

Abstract

Australian wildlife rehabilitators (AWR) are at increased risk of developing Q fever, a serious zoonotic disease caused by the intracellular bacterium Coxiella burnetii. Previous studies have suggested that Australian wildlife may be a potential C. burnetii infection source for humans. However, a recent serological survey of AWR found no association between C. burnetii exposure and direct contact with any wildlife species. To further explore the potential risk that wildlife may pose, this study aimed to identify associations between self-reported Q fever in AWR and risk factors for exposure to C. burnetii. An online cross-sectional survey was implemented in 2018 targeting AWR nationwide. Risk factors for self-reported Q fever were determined using multivariable logistic regression. Medically diagnosed Q fever was self-reported in 4.5% (13/287) of unvaccinated respondents. Rehabilitators who self-reported medically diagnosed Q fever were significantly more likely to: primarily rehabilitate wildlife at a veterinary clinic (OR 17.87, 95% CI: 3.09-110.92), have domestic ruminants residing on the property where they rehabilitate wildlife (OR 11.75, 95% CI: 2.91-57.42), have been educated at a High School/Technical and Further Education level (OR 10.29, 95% CI: 2.13-84.03) and be aged >50 years (OR 6.61, 95% CI: 1.60-38.35). No association was found between self-reported Q fever and direct contact with wildlife. These findings support previous work suggesting that AWR are at increased risk of C. burnetii infection and may develop Q fever potentially via exposure to traditional infection sources including livestock, other domestic animals, or contaminated environments, in association with their rehabilitation practices and lifestyle. Although Q fever vaccination is recommended for AWR, vaccine uptake is low in this population. Future studies should aim to determine the level of Q fever awareness and identify barriers to Q fever vaccination in this at-risk group. The difficulty in accessing the AWR population also highlights the need for a national centralized AWR database., (© 2022 The Authors. Zoonoses and Public Health published by Wiley-VCH GmbH.)

Published

2023

19. Factors associated with Q fever vaccination in Australian wildlife rehabilitators.

Author

Mathews KO, Norris JM, Phalen D, Malikides N, Savage C, Sheehy PA, and Bosward KL

Subjects

Animals, Animals, Wild, Australia, Cross-Sectional Studies, Bacterial Vaccines, Vaccination, Q Fever prevention & control, Coxiella burnetii

Abstract

Australian wildlife rehabilitators (AWR) are at risk of contracting Q fever, a serious zoonotic disease caused by Coxiella burnetii. Despite Australian government recommendations for AWR to receive Q fever vaccination (QFV), and the availability of a safe and effective vaccine in Australia, shortfalls in vaccine uptake have been observed in AWR. This study aimed to determine factors associated with QFV status and describe AWR attitudes and potential barriers towards QFV. Data were obtained from a nationwide, online, cross-sectional survey of AWR undertaken in 2018. Approximately-three quarters (200/265; 75.5 %) of those that had heard of Q fever were also aware of the Q fever vaccine, and of those, 25.5 % (51/200) were vaccinated. Barriers to QFV, among unvaccinated respondents who had also heard of Q fever and the vaccine (149/200; 74.5 %), included concerns regarding the safety, efficacy, and importance of the Q fever vaccine. Complacency toward vaccination, convenience of vaccination, and a lack of Q fever knowledge were also notable barriers. Only 27.7 % (41/148) of respondents reported having had vaccination recommended to them. Multivariable logistic regression identified that vaccinated AWR were more likely to be aged ≤ 50 years (OR 4.51, 95 % CI: 2.14-10.11), have had a university level education (OR 2.78, 95 % CI: 1.39-5.73), have resided in New South Wales/Australian Capital Territory and Queensland than in other Australian jurisdictions (OR 2.9, 95 % CI: 1.10-8.83 and OR 4.82, 95 % CI: 1.64-16.00 respectively) and have attended an animal birth (OR 2.14, 95 % CI: 1.02-4.73). Knowledge gaps regarding Q fever and QFV in AWR demonstrated the need for interventions to raise the awareness of the potential health consequences of C. burnetii exposure and Q fever prevention. Education programs to allow AWR to develop an informed perspective of Q fever and QFV, coupled with improvements in vaccine affordability and the implementation of programs to enhance accessibility, may also increase vaccine uptake., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2022. Published by Elsevier Ltd.)

Published

2023

20. Evaluation of three immunological assays to mitigate the risk of transboundary spread of Coxiella burnetii by alpacas.

Author

Tellis AN, Rowe SM, Coilparampil R, Jenkins C, Dart A, Zadoks RN, Regnerus CD, and Bosward KL

Subjects

Animals, Antibodies, Bacterial, Bayes Theorem, Enzyme-Linked Immunosorbent Assay methods, Enzyme-Linked Immunosorbent Assay veterinary, Seroepidemiologic Studies, Camelids, New World, Coxiella burnetii, Q Fever epidemiology, Q Fever prevention & control, Q Fever veterinary

Abstract

Coxiella burnetii causes coxiellosis in animals and Q fever in humans, a potentially debilitating zoonotic disease commonly transmitted through domestic ruminants. To prevent transboundary spread of C. burnetii, animals may be tested prior to export. In alpacas, this process is complicated by the lack of scientific evidence for C. burnetii infection in the species, and the unique composition of camelid antibodies, which may cause false-positive results in assays developed for ruminants. We evaluated a complement fixation test (CFT; currently recommended for alpacas in New Zealand), an enzyme-linked immunosorbent assay (ELISA) and an immunofluorescence assay (IFA). Positive analytical control samples were generated through vaccination of alpacas with a human Q fever vaccine, whereas negative analytical control samples were sourced from New Zealand (deemed free of C. burnetii). Immunological assays were conducted on 131 alpaca sera submitted for export testing. Test characteristics (sensitivity, specificity, positive and negative predictive values) for CFT, ELISA and IFA were determined using Bayesian latent class analysis. Due to anticomplementary activity, 37 (28.2%) of the CFT results were inconclusive, making CFT unsuitable for routine use. Of the remaining 94 samples, 10.6%, 0% and 7.4% were positive for C. burnetii antibodies based on CFT, ELISA and IFA, respectively, yielding estimated sensitivities of 58%, 26% and 78%, and estimated specificities of 95%, 98% and 95%, with the estimates for sensitivity being imprecise, as evidenced by wide 95% credible intervals. Positive predictive values were similar across assays, albeit very low at the estimated seroprevalence of 5%. Our results indicate that, of the tests available, IFA appears to be the most appropriate for use in alpacas. Higher sensitivity of antibody detection, use of antigen detection assays and availability of samples from individuals with evidence of infection could provide additional insight into the risk of transboundary spread of C. burnetii by alpacas., (© 2021 Wiley-VCH GmbH.)

Published

2022

21. Renal Crest Proliferative Lesions in Cats with Chronic Kidney Disease.

Author

White JD, Bosward KL, Norris JM, Malik R, Lindsay SA, and Canfield PJ

Subjects

Animals, Cats, Kidney, Urothelium, Carcinoma, Renal Cell veterinary, Cat Diseases, Kidney Neoplasms veterinary, Renal Insufficiency, Chronic veterinary

Abstract

In a histopathological study of the renal crest (RC) of kidneys of cats with chronic kidney disease (CKD), 58/90 (64%) had epithelial proliferation. Of these, 33 cats had hyperplasia of the collecting duct (CD) epithelium (CDH) alone, eight had hyperplasia of the urothelium covering the RC (RCUH), of which one had concurrent abaxial renal pelvic urothelial hyperplasia (UH), and eight had both CDH and RCUH. CDH or RCUH were present in five cats with marked dysplasia of the CD epithelium (CDD) and four cats with invasive carcinomas, which also had epithelial dysplasia. All nine cats with marked dysplasia or neoplasia of the RC also had substantially altered RC contours due to focal haemorrhage, papillary necrosis or fibrosis. Three of the carcinomas had a strong desmoplastic response. In control cats, both urothelial (RC and renal pelvis) and tubular (CD and distal tubular) cells were immunopositive for cytokeratin (CK; AE1/AE3), tubular epithelial cells were positive for vimentin (Vim) and aquaporin 2 (Aq2), while urothelial cells were positive for p63. PAX8 immunolabelling was difficult to validate. CD and UH labelling was similar to control tissue. While urothelial dysplasia had the same immunolabelling pattern as UH and control tissue, CDD was generally immunonegative for Aq2. As immunolabelling of the four carcinomas did not distinguish between tubular and urothelial origin, with three positive for both Vim and p63, all were broadly designated as RC carcinomas. Overall, proliferative epithelial lesions are common in cats with CKD and form a continuum from simple hyperplasia to neoplasia of the urothelium or CD of the RC., (Copyright © 2021 Elsevier Ltd. All rights reserved.)

Published

2021

22. Cat fleas ( Ctenocephalides felis clade 'Sydney') are dominant fleas on dogs and cats in New South Wales, Australia: Presence of flea-borne Rickettsia felis, Bartonella spp. but absence of Coxiella burnetii DNA.

Author

Huang HHH, Power RI, Mathews KO, Ma GC, Bosward KL, and Šlapeta J

Abstract

The cat flea ( Ctenocephalides felis ) is the most common flea species parasitising both domestic cats and dogs globally. Fleas are known vectors of zoonotic pathogens such as vector-borne Rickettsia spp. and Bartonella spp. and could theoretically transmit Coxiella burnetii , the causative agent of Q fever. A total of 107 fleas were collected from 21 cats and 14 dogs in veterinary clinics, a feline rescue organisation and a grooming salon in New South Wales, Australia, to undergo PCR detection of Bartonella spp., Rickettsia spp. and C. burnetii DNA. Morphological identification confirmed that the cat flea ( C. felis ) is the most common flea in New South Wales, Australia, with only a single stick fast flea, Echidnophaga gallinacea recorded. The examined fleas ( n  = 35) at the cox 1 locus revealed five closely related C. felis haplotypes (inter-haplotype distance < 0.5%). Multiplex TaqMan qPCR targeting the gltA ( Rickettsia spp.) and ssrA ( Bartonella spp.) genes was positive in 22.9% (95% CI: 11.8-39.3%) and 11.4% (95% CI: 3.9-26.6%) of samples, respectively. None of the DNA isolated from fleas was positive on TaqMan qPCRs targeting the C. burnetii IS 1111 , Com 1 and htp AB genes. Co-infection of C. felis with Bartonella henselae and Bartonella clarridgeiae was demonstrated using gltA and ssrA Illumina next-generation amplicon sequencing. These findings reinforce the importance of flea control on domestic dogs and cats to effectively control the transmission of Rickettsia felis and Bartonella spp. The flea, however, is unlikely to be a vector of C. burnetii between companion animals and humans., Competing Interests: The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (© 2021 The Author(s).)

Published

2021

23. Serological Evidence of Exposure to Spotted Fever Group and Typhus Group Rickettsiae in Australian Wildlife Rehabilitators.

Author

Mathews KO, Phalen D, Norris JM, Stenos J, Toribio JA, Wood N, Graves S, Sheehy PA, Nguyen C, and Bosward KL

Abstract

Rickettsioses are arthropod-borne zoonotic diseases, several of which occur in Australia. This study aimed to assess the exposure levels and risk factors for Rickettsia spp. among Australian wildlife rehabilitators (AWRs) using serology, PCR and a questionnaire. Antibody titres against Spotted Fever Group (SFG), Typhus Group (TG) and Scrub Typhus Group (STG) antigens were determined using an immunofluorescence assay. PCR targeting the gltA gene was performed on DNA extracts from whole blood and serum. Logistic regression was used to identify risk factors associated with seropositivity. Of the 27 (22.1%; 27/122) seropositive participants all were seropositive for SFG, with 5/27 (4.1%) also positive for TG. Of the 27 positive sera, 14.8% (4/27) were further classified as exposure to R. australis , 3.7% (1/27) to R. honei , 3.7% (1/27) to R. felis and 77.8% (21/27) were classified as 'indeterminate'-most of which (85.7%; 18/21) were indeterminate R. australis / R. honei exposures. Rickettsia DNA was not detected in whole blood or serum. Rehabilitators were more likely to be seropositive if more than one household member rehabilitated wildlife, were older than 50 years or had occupational animal contact. These findings suggest that AWRs are at increased risk of contracting Rickettsia -related illnesses, however the source of the increased seropositivity remains unclear.

Published

2021

24. Mycoplasma species in vaginas of dairy cows before and after exposure to bulls and their association with conception.

Author

Hazelton MS, Morton JM, Bosward KL, Sheehy PA, Parker AM, Dwyer CJ, Niven PG, and House JK

Subjects

Animals, Cattle, Cattle Diseases epidemiology, Cattle Diseases transmission, Female, Fertilization, Male, Mycoplasma classification, Mycoplasma Infections epidemiology, Mycoplasma Infections microbiology, Mycoplasma Infections transmission, Mycoplasma bovis isolation & purification, Pregnancy, Prevalence, Reproduction, Sexually Transmitted Diseases, Bacterial microbiology, Cattle Diseases microbiology, Mycoplasma isolation & purification, Mycoplasma Infections veterinary, Sexually Transmitted Diseases, Bacterial veterinary

Abstract

Mycoplasma species can colonize the urogenital tract of dairy cattle. However, interrelationships between Mycoplasma spp. and reproductive performance in dairy herds are unclear. In this study, we measured apparent prevalences of Mycoplasma spp. in the vaginas of dairy cows (n = 629) pre- and post-bull exposure in dairy herds with and without Mycoplasma bovis clinical disease (n = 5 herds), and assessed associations between variables describing reproductive performance and consequent Mycoplasma spp. isolation. Mycoplasma spp. were infrequently isolated from the vagina pre- (1.9%; 12/629) and post-bull (3.2%; 20/629) exposure. Of the mycoplasmas isolated, Mycoplasma bovigenitalium was isolated most frequently (87.5%; 28/32), followed by Mycoplasma californicum (9.3%; 3/32). Mycoplasma bovis was only isolated from one cow. We were unable to provide any evidence of venereal transmission of M. bovis in cows in M. bovis-infected herds that use natural service bulls. There was an insufficient number of cows with Mycoplasma spp. in the vagina pre-bull exposure to assess effects on subsequent reproductive performance. Cows that had not conceived before post-bull exposure sampling had much greater odds (odds ratio 14.8; 95% confidence interval 4.2 to 52.3) of having a Mycoplasma sp. isolated from the vagina at this time compared with those that had conceived. Also, within those that had conceived, delayed conception increased the odds of having a Mycoplasma spp. isolated from the vagina at the post-bull exposure sampling by a factor of 1.62 for every additional week not pregnant. The likely cause of these findings is that cows that remain not pregnant for longer are more likely to be served by a bull (likely repeatedly) and subsequently become colonized with a Mycoplasma sp. (mostly M. bovigenitalium) through venereal transmission. In dairy herds that use bulls, there is a greater chance of isolating a Mycoplasma sp. (mostly M. bovigenitalium) after a period of bull breedings from the vaginas of cows that have remained nonpregnant for longer during the bull breeding period., (© 2020, The Authors. Published by Elsevier Inc. and Fass Inc. on behalf of the American Dairy Science Association®. This is an open access article under the CC BY-NC-ND license (http://creativecommons.org/licenses/by-nc-nd/4.0/).)

Published

2020

25. Mycoplasma bovis and other Mollicutes in replacement dairy heifers from Mycoplasma bovis-infected and uninfected herds: A 2-year longitudinal study.

Author

Hazelton MS, Morton JM, Parker AM, Bosward KL, Sheehy PA, Dwyer CJ, Niven PG, and House JK

Subjects

Animals, Bacterial Shedding, Cattle, Cattle Diseases epidemiology, Colostrum, Enzyme-Linked Immunosorbent Assay veterinary, Female, Longitudinal Studies, Mycoplasma Infections epidemiology, Mycoplasma Infections microbiology, Mycoplasma bovis isolation & purification, Pregnancy, Prospective Studies, Seroepidemiologic Studies, Weaning, Cattle Diseases microbiology, Milk microbiology, Mycoplasma Infections veterinary, Mycoplasma bovis immunology, Tenericutes isolation & purification

Abstract

Replacement dairy heifers exposed to Mycoplasma bovis as calves may be at risk of future clinical disease and pathogen transmission, both within and between herds; however, little information is available about these risks. We conducted a 2-yr longitudinal (panel) study starting with 450 heifer calves reared to weaning in 8 herds (7 M. bovis infected with clinical disease, 1 uninfected) under the same ownership. After weaning, heifers were commingled and managed with non-study heifers at a single heifer rearing facility. Nose, conjunctival, and vaginal swabs were collected along with a blood sample at weaning, prebreeding, precalving, and approximately 1 mo postcalving. Additionally, a colostrum sample was collected upon calving and a composite milk sample was collected 1 mo postcalving. The swabs, colostrum, and milk samples were cultured for Mycoplasma spp., and serum from the blood was evaluated for serological evidence of exposure to M. bovis using an ELISA. Despite a high M. bovis ELISA seroprevalence at weaning in the heifers from the 7 M. bovis-infected herds with clinical disease [72% (289/400); range by herd: 28-98%], M. bovis was isolated from only 4% (16/400) of the same heifers at the same time. In heifers from the uninfected herd at weaning, M. bovis seroprevalence was 2% (1/50) and M. bovis was not detected by culture. Mycoplasma bovis was isolated from 0.5% (2/414) of heifers at prebreeding, 0% (0/374) of heifers at precalving, and 0.3% (1/356) of heifers 1 mo postcalving. The nose was the predominant anatomical site of M. bovis colonization (74%; 14/19 culture positives). A single heifer (from an M. bovis-infected herd with clinical disease) was repeatedly detected with M. bovis in its nose at weaning, prebreeding, and postcalving samplings. This demonstrates the possibility, albeit rare, of a long-term M. bovis carrier state in replacement heifers exposed to M. bovis as calves, up to at least 1 mo after entry into the milking herd. No M. bovis clinical disease was detected in any heifer from weaning through to the end of the study (approximately 1 mo after calving). Acholeplasma spp. were commonly isolated throughout the study. Mycoplasma bovigenitalium, Mycoplasma bovoculi, and Mycoplasma bovirhinis were isolated infrequently. Mycoplasma bovis seroprevalences at prebreeding, precalving, and postcalving samplings were 27% (112/414), 12% (46/374), and 18% (65/356), respectively. Overall, the results show that replacement heifers from groups exposed to M. bovis preweaning can become colonized with M. bovis and that colonization can, uncommonly, be present after their first calving. For groups of 50 or more heifers exposed to M. bovis preweaning, there is at least a nontrivial probability that the group will contain at least 1 shedding heifer postcalving., (© 2020, The Authors. Published by Elsevier Inc. and Fass Inc. on behalf of the American Dairy Science Association®. This is an open access article under the CC BY-NC-ND license (http://creativecommons.org/licenses/by-nc-nd/4.0/).)

Published

2020

26. Coxiella burnetii seroprevalence and Q fever in Australian wildlife rehabilitators.

Author

Mathews KO, Toribio JA, Norris JM, Phalen D, Wood N, Graves SR, Sheehy PA, and Bosward KL

Abstract

Coxiella burnetii is the causative bacterium of the zoonotic disease Q fever, which is recognised as a public health concern globally. Macropods have been suggested as a potential source of C. burnetii infection for humans. The aim of this cross-sectional study was to determine the prevalence of C. burnetii exposure in a cohort of Australian wildlife rehabilitators (AWRs) and assess Q fever disease and vaccination status within this population. Blood samples were collected from adult participants attending the Australian Wildlife Rehabilitation Conference in Sydney in July 2018. Participants completed a questionnaire at the time of blood collection. Antibody titres (IgG, IgA and IgM) against phase I and phase II C. burnetii antigens as determined by immunofluorescence assay, revealed that of the unvaccinated participants, 6.1% (9/147) had evidence of exposure to C. burnetii . Of the total participants, 8.1% (13/160) had received Q fever vaccination, four of whom remained seropositive at the time of blood collection. Participants reporting occupational contact with ruminants, were eight times more likely to have been vaccinated against Q fever, than those reporting no occupational animal contact (OR 8.1; 95% CI 1.85-45.08). Three AWRs (2%) reported having had medically diagnosed Q fever, two of whom remained seropositive at the time of blood collection. Despite the lack of association between macropod contacts and C. burnetii seropositivity in this cohort, these findings suggest that AWRs are approximately twice as likely to be exposed to C. burnetii , compared with the general Australian population. This provides support for the recommendation of Q fever vaccination for this potentially 'at-risk' population. The role of macropods in human Q fever disease remains unclear, and further research into C. burnetii infection in macropods including: infection rate and transmission cycles between vectors, macropods as reservoirs, other animals and humans is required., Competing Interests: The authors declare no conflict of interest (document uploaded)., (© 2020 The Authors.)

Published

2020

27. New insights on the epidemiology of Coxiella burnetii in pet dogs and cats from New South Wales, Australia.

Author

Ma GC, Norris JM, Mathews KO, Chandra S, Šlapeta J, Bosward KL, and Ward MP

Subjects

Animal Feed, Animals, Cat Diseases epidemiology, Cats, Disease Outbreaks, Dog Diseases epidemiology, Dogs, Female, Food Microbiology, Humans, Incidence, Macropodidae microbiology, Meat microbiology, New South Wales epidemiology, Prevalence, Q Fever epidemiology, Seroepidemiologic Studies, Zoonoses epidemiology, Cat Diseases microbiology, Coxiella burnetii, Dog Diseases microbiology, Q Fever veterinary

Abstract

Q fever is considered one of the most important zoonoses in Australia. Whilst ruminants are the primary reservoirs for Coxiella burnetii, and the major source of human infection, human cases have also been reported following contact with pet dogs and cats. This study aimed to estimate the prevalence of seropositivity to, and bacterial shedding of, C. burnetii by pet dogs and cats in a region with a high human Q fever incidence and explore risk factors for C. burnetii exposure. Samples (serum, whole blood, reproductive tissue, reproductive swabs) and questionnaires (completed by the pet's owner) were collected from dogs and cats from eight communities across remote New South Wales (NSW), Australia. Overall 86/330 dogs (26.1%, 95% CI 21.3-30.8%) and 19/145 cats (13.1%, 95% CI 7.6-18.6%) were seropositive to C. burnetii. Seroprevalence varied significantly between communities and was highest in communities within 150 km of a 2015 human Q fever outbreak. Feeding raw kangaroo was identified as a risk factor for seropositivity (adjusted OR 3.37, 95% CI 1.21-9.43). Coxiella burnetii DNA was not detected from any dog or cat whole blood, reproductive tissue or vaginal/preputial swab using qPCR targeting the IS1111 and com1 genes. Our findings suggest that companion animals are frequently exposed to C. burnetii in western NSW. Geographical variation in C. burnetii seroprevalence amongst companion animals - which corresponds with a human Q fever outbreak - suggests a shared environmental source of infection is likely with important consequences for public and animal health. The lack of detection of C. burnetii DNA from healthy companion animals suggests that pet dogs and cats are not an important reservoir for human Q fever infection outside a narrow periparturient window., Competing Interests: Declaration of Competing Interest The authors have no competing interests., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2020

28. Whole dairy herd sampling to detect subclinical intramammary Mycoplasma bovis infection after clinical mastitis outbreaks.

Author

Hazelton MS, Morton JM, Parker AM, Sheehy PA, Bosward KL, Malmo J, and House JK

Subjects

Animals, Asymptomatic Infections, Cattle, Dairying, Female, Milk microbiology, Mycoplasma Infections epidemiology, Sampling Studies, Seroepidemiologic Studies, Tasmania epidemiology, Victoria epidemiology, Disease Outbreaks veterinary, Mastitis, Bovine epidemiology, Mastitis, Bovine microbiology, Mycoplasma Infections diagnosis, Mycoplasma Infections veterinary, Mycoplasma bovis isolation & purification

Abstract

After clinical Mycoplasma bovis mastitis outbreaks in dairy herds, M. bovis can persist as subclinical intramammary infections. Identification and culling of sub-clinically infected cows may be warranted to reduce future pathogen transmission and disease. In this study, apparent cow-level prevalences of M. bovis intramammary infection within 4 milking herds immediately following outbreaks of clinical disease due to M. bovis were determined utilising PCR and culture. All clinically affected M. bovis cows had been culled from the herds prior to herd sampling. Composite milk samples were collected once from each cow (n = 2,258) using a routine milk recording sampling technique. These samples were pooled for PCR screening; positive pools were analysed in different sized pools as needed from large to small, until individual PCR-positive animals could be identified. Despite M. bovis seroprevalences of 76% (herd 1), 40% (herd 2), 20% (herd 3) and 16% (herd 4), apparent prevalences of intramammary infection in the main milking group based on PCR in herds 1 to 4 were 0.2% (1/497), 0.0% (0/475), 0.1% (1/816) and 0.0% (0/444), respectively. Due to the low apparent prevalences of subclinical intramammary mycoplasma infections in these herds and the high expense associated with milk sample collection and testing, the return on diagnostic investment was very limited, particularly considering that additional cows are likely to have been colonised with mycoplasma in other anatomical sites. The results of this study suggest that pursuing identification of cows with subclinical intramammary mycoplasma infections following resolution of clinical M. bovis disease outbreaks in dairy herds may be of minimal benefit in programs designed to control or eradicate M. bovis., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2020

29. Coxiella burnetii seroprevalence in unvaccinated veterinary workers in Australia: Evidence to support Q fever vaccination.

Author

Sellens E, Bosward KL, Norris JM, Wood N, Heller J, Graves S, and Gidding HF

Subjects

Adolescent, Adult, Aged, Aged, 80 and over, Animals, Australia epidemiology, Female, Humans, Male, Middle Aged, Seroepidemiologic Studies, Surveys and Questionnaires, Veterinarians, Young Adult, Zoonoses, Animal Technicians, Bacterial Vaccines immunology, Q Fever epidemiology, Q Fever prevention & control

Abstract

Q fever (caused by Coxiella burnetii) is a serious zoonotic disease that occurs almost worldwide. Occupational contact with animals increases the risk of exposure, and Q fever vaccination is recommended for veterinary workers in Australia. This study aimed to investigate C. burnetii seroprevalence among unvaccinated veterinary workers in Australia and determine factors associated with a positive serological result. During 2014 and 2015, convenience sampling at veterinary conferences and workplace vaccination clinics was undertaken. Participants completed a questionnaire and provided a blood sample for C. burnetii serology. Participants were predominantly veterinarians (77%), but veterinary support staff, animal scientists, and administration workers also participated. Blood samples (n = 192) were analysed by an immunofluorescence assay and considered positive where the phase I or phase II IgG titre was ≥1/50. Seroprevalence was 19% (36/192; 95% CI 14%-25%). A positive serological result was significantly associated with (a) working in outer regional/remote areas (odds ratio [OR] 6.2; 95% CI 1.9-20.8; reference = major cities; p = .009) and (b) having spent more than 50% of total career working with ruminants (OR 4.8; 95% CI 1.7-13.5; reference = <15% of career; p = .025). These findings confirm an increased risk of exposure to C. burnetii compared to the general population, providing new evidence to support Q fever vaccination of veterinary workers in Australia., (© 2019 Blackwell Verlag GmbH.)

Published

2020

30. Frequency of Adverse Events Following Q Fever Immunisation in Young Adults.

Author

Sellens E, Bosward KL, Willis S, Heller J, Cobbold R, Comeau JL, Norris JM, Dhand NK, and Wood N

Abstract

Q fever is a zoonosis of concern in many countries. Vaccination is the most effective means of prevention, and since 1989, Australia has had a licensed Q fever vaccine, Q-VAX ® . This vaccine was also used in the Netherlands in 2011 following the largest recorded Q fever outbreak globally. There is a paucity of available data regarding adverse events following immunisation (AEFI) for young adult females. Such data are important for informing future vaccination recommendations both within Australia and internationally. This study collected Q fever vaccine (Q-VAX ® ) AEFI data in veterinary and animal science students at Australian universities. Students were enrolled at the time of vaccination and were emailed a link to an online AEFI survey one week later. Of the 60% (499/827) that responded, 85% were female and the median age was 18 years. Local injection site reactions (ISRs) occurred in 98% (95%; CI 96⁻99%) of respondents, of which 30% (95% CI 24⁻32%) were severe. Systemic AEFI occurred in 60% (95%; CI 55⁻64%) of respondents within the seven days following immunisation. Medical attention was sought by 19/499 (3.8%) respondents, of whom one sought treatment at a hospital emergency department. Females were more likely than males to experience any local ISR (odds ratio [OR] 9.3; 95% CI 2.5⁻33.8; p < 0.001), ISRs of greater severity (OR 2.5; 95% CI 1.5⁻4.2; p < 0.001), and any systemic AEFI (OR 1.9; 95% CI 1.1⁻3.1; p = 0.016). These safety data suggest that a high frequency of adverse events following immunisation should be expected in young adults, particularly females. However, the consequences of Q fever disease are potentially far more debilitating.

Published

2018

31. Isolation of Mycoplasma spp. and serological responses in bulls prior to and following their introduction into Mycoplasma bovis-infected dairy herds.

Author

Hazelton MS, Morton JM, Bosward KL, Sheehy PA, Parker AM, Dwyer CJ, Niven PG, and House JK

Subjects

Animals, Cattle, Male, Mycoplasma Infections epidemiology, Semen Analysis, Seroepidemiologic Studies, Sperm Motility, Antibodies, Bacterial blood, Cattle Diseases epidemiology, Mycoplasma Infections veterinary, Mycoplasma bovis immunology

Abstract

With the common use of bulls for breeding following a period of artificial insemination in seasonally bred dairy herds, it is important to consider the potential role of the bull in transmission of Mycoplasma spp. within and between herds. This study aimed to assess the prevalence of Mycoplasma spp. in a population of bulls before and after use in Mycoplasma bovis-infected herds. The frequency of subclinical infection was also measured serologically postbreeding, and the association of Mycoplasma spp. on semen quality was evaluated. Mycoplasma bovis was isolated from 4 of 118 bulls after use in 4 herds infected with M. bovis. In the bulls, M. bovis seroprevalence increased from 9% prebreeding to 46% postbreeding with a total seroconversion rate of 44% across the 4 herds, with no evidence of clinical disease. There was no association of Mycoplasma spp. in the bulls' semen and abnormal palpation characteristics (enlarged or nodular) of seminal vesicular glands or poor semen quality attributes such as semen mass activity, sperm motility, and morphology. These results demonstrate a high degree of subclinical exposure of the bulls to M. bovis in infected herds and highlight the potential for bulls to be mycoplasma carriers within and between herds. Herd biosecurity protocols and control programs should take into account the potential role of bulls in the introduction and spread of Mycoplasma spp., (Copyright © 2018 American Dairy Science Association. Published by Elsevier Inc. All rights reserved.)

Published

2018

32. Willingness of veterinarians in Australia to recommend Q fever vaccination in veterinary personnel: Implications for workplace health and safety compliance.

Author

Sellens E, Norris JM, Dhand NK, Heller J, Hayes L, Gidding HF, Willaby H, Wood N, and Bosward KL

Subjects

Adult, Animals, Bacterial Vaccines immunology, Coxiella burnetii immunology, Coxiella burnetii pathogenicity, Cross-Sectional Studies, Humans, Logistic Models, Middle Aged, Q Fever microbiology, Surveys and Questionnaires, Vaccination, Workplace, Animal Technicians psychology, Attitude to Health, Occupational Health, Q Fever prevention & control, Veterinarians psychology

Abstract

Q fever vaccine uptake among veterinary nurses in Australia is low, suggesting veterinarians are not recommending the vaccination to veterinary personnel. This study aimed to determine the willingness of veterinarians to recommend Q fever vaccination to veterinary personnel and to identify factors influencing Q fever vaccine uptake by veterinary nurses in Australia. An online cross sectional survey targeted veterinarians and veterinary nurses in Australia in 2014. Responses were analysed using multivariable logistic regression. Factors significantly (p<0.05) associated with a willingness to recommend the vaccination, expressed by 35% (95% CI 31-38%) of veterinarians (n = 828), were (1) being very concerned for colleagues regarding Coxiella burnetii (OR 4.73), (2) disagreeing the vaccine is harmful (OR 3.80), (3) high Q fever knowledge (OR 2.27), (4) working within small animal practice (OR 1.67), (5) disagreeing the vaccine is expensive (OR 1.55), and (6) age, with veterinarians under 39 years most likely to recommend vaccination. Of the veterinary nursing cohort who reported a known Q fever vaccination status (n = 688), 29% (95% CI 26-33%) had sought vaccination. This was significantly (p<0.05) associated with (1) agreeing the vaccine is important (OR 8.34), (2) moderate/high Q fever knowledge (OR 5.51), (3) working in Queensland (OR 4.00), (4) working within livestock/mixed animal practice (OR 3.24), (5) disagreeing the vaccine is expensive (OR 1.86), (6) strong reliance on work culture for biosecurity information (OR 2.5), (7) perceiving personal exposure to Coxiella burnetii to be at least low/moderate (OR 2.14), and (8) both agreeing the vaccine is safe and working within a corporate practice structure (OR 4.28). The study identified the need for veterinarians to take greater responsibility for workplace health and safety promotion, and calls for better education of veterinary personnel to raise awareness of the potential for occupational exposure to C. burnetii and improve the perception of the Q fever vaccine as being important, safe and cost-effective., Competing Interests: The authors have declared that no competing interests exist.

Published

2018

33. One health in our backyard: Design and evaluation of an experiential learning experience for veterinary medical students.

Author

Mor SM, Norris JM, Bosward KL, Toribio JLML, Ward MP, Gongora J, Vost M, Higgins PC, McGreevy PD, White PJ, and Zaki S

Abstract

Background: New educational approaches are needed to improve student understanding of the wider sociological and ecological determinants of health as well as professional responsibilities in related areas. Field trips allow students to observe interaction between plant, animal and human communities, making them an ideal tool for teaching One Health concepts., Methods: Veterinary medical students participated in a field trip to a local parklands area, frequented by humans, dogs, horses, and wildlife. Students rotated through 5 learning activities ('stations') that focused on: (1) response to exotic animal disease incursion (equine influenza); (2) impact of cultures and belief systems on professional practice; (3) management of dangerous dogs; (4) land use change, biodiversity and emerging infectious disease; and (5) management of environmentally-acquired zoonoses (botulism). Intended learning outcomes were for students to: evaluate the various roles and responsibilities of veterinarians in society; compare the benefits and risks associated with human-animal and animal-animal interactions; and evaluate the contributions made by various professionals in safeguarding the health and welfare of animals, humans and the environment. Following the field trip, students participated in a debrief exercise and completed an online survey on their experiences., Results: Feedback from students collected in 2016/2017 (n = 211) was overwhelmingly positive. The learning experience at each station was rated as 4 ('Good') or 5 ('Very Good') out of 5 by 82-96% of students. Responses to closed- and open-ended questions - as well as outputs generated in the debrief session - indicated that students achieved the learning outcomes. Overall, 94% of students agreed or strongly agreed that they had a better understanding of One Health because of the field trip., Conclusions: Field trips to local parklands are effective in promoting learning about One Health and can be incorporated into the core curriculum to maximize student exposure at relatively low cost.

Published

2018

34. A review of mycoplasma diagnostics in cattle.

Author

Parker AM, Sheehy PA, Hazelton MS, Bosward KL, and House JK

Subjects

Animals, Cattle, Cattle Diseases microbiology, Milk microbiology, Mycoplasma, Mycoplasma Infections diagnosis, Mycoplasma bovis, Polymerase Chain Reaction methods, Polymerase Chain Reaction veterinary, Serologic Tests methods, Serologic Tests veterinary, Cattle Diseases diagnosis, Mycoplasma Infections veterinary

Abstract

Mycoplasma species have a global distribution causing serious diseases in cattle worldwide including mastitis, arthritis, pneumonia, otitis media and reproductive disorders. Mycoplasma species are typically highly contagious, are capable of causing severe disease, and are difficult infections to resolve requiring rapid and accurate diagnosis to prevent and control disease outbreaks. This review discusses the development and use of different diagnostic methods to identify Mycoplasma species relevant to cattle, with a particular focus on Mycoplasma bovis. Traditionally, the identification and diagnosis of mycoplasma has been performed via microbial culture. More recently, the use of polymerase chain reaction to detect Mycoplasma species from various bovine samples has increased. Polymerase chain reaction has a higher efficiency, specificity, and sensitivity for laboratory diagnosis when compared with conventional culture-based methods. Several tools are now available for typing Mycoplasma spp. isolates, allowing for genetic characterization in disease outbreak investigations. Serological diagnosis through the use of indirect ELISA allows the detection of antimycoplasma antibodies in sera and milk, with their use demonstrated on individual animal samples as well as BTM samples. While each testing method has strengths and limitations, their combined use provides complementary information, which when interpreted in conjunction with clinical signs and herd history, facilitates pathogen detection, and characterization of the disease status of cattle populations., (Copyright © 2018 The Authors. Journal of Veterinary Internal Medicine published by Wiley Periodicals, Inc. on behalf of the American College of Veterinary Internal Medicine.)

Published

2018

35. Short communication: Shedding of Mycoplasma bovis and antibody responses in cows recently diagnosed with clinical infection.

Author

Hazelton MS, Sheehy PA, Bosward KL, Parker AM, Morton JM, Dwyer CJ, Niven PG, and House JK

Subjects

Animals, Antibody Formation, Bacterial Shedding, Cattle, Enzyme-Linked Immunosorbent Assay veterinary, Female, Lactation, Mastitis, Bovine diagnosis, Mycoplasma Infections diagnosis, Mycoplasma Infections microbiology, Mycoplasma bovis isolation & purification, Mycoplasma bovis physiology, Sensitivity and Specificity, Mastitis, Bovine microbiology, Milk microbiology, Mycoplasma Infections veterinary, Mycoplasma bovis immunology

Abstract

Mycoplasma bovis can have significant consequences when introduced into immunologically naïve dairy herds. Subclinically infected carrier animals are the most common way that M. bovis is introduced into herds. Although M. bovis udder infections can be detected by milk sampling lactating animals before their introduction, currently, no definitive way of identifying M. bovis carrier animals that are nonlactating (i.e., calves, heifers, dry cows, or bulls) is available. Understanding the prevalence of M. bovis shedding from various body sites in clinically infected animals could inform strategies for the detection of subclinical infection in nonlactating stock. The mucosal surfaces of the nose, eye, and vagina of 16 cows with recent clinical mastitis caused by M. bovis were examined for the presence of M. bovis shedding. Blood was collected for serological evaluation by a commercially available ELISA. Mycoplasma bovis was isolated from the vagina of only 3 (18.8%) of the cows and was not detected from the noses or eyes of any of the cows. Fifteen of the 16 (93.8%) cows were seropositive to the ELISA. With such low prevalence of detection of M. bovis from the vagina and no detections from the noses or eyes of recently clinically infected animals, it is very likely that sampling these sites would be ineffective for detecting subclinical infection in cattle. Serology using the ELISA may have some use when screening animals for biosecurity risk assessment. However, more information regarding time to seroconversion, antibody longevity, and test diagnostic sensitivity and specificity are required to define the appropriate use of this ELISA for biosecurity purposes., (Copyright © 2018 American Dairy Science Association. Published by Elsevier Inc. All rights reserved.)

Published

2018

36. Bulk tank milk antibody ELISA as a biosecurity tool for detecting dairy herds with past exposure to Mycoplasma bovis.

Author

Parker AM, House JK, Hazelton MS, Bosward KL, Morton JM, and Sheehy PA

Subjects

Animals, Australia, Belgium, Cattle, Cattle Diseases immunology, Cattle Diseases transmission, Female, Lactation, Milk microbiology, Mycoplasma Infections diagnosis, Mycoplasma Infections immunology, Mycoplasma Infections transmission, Seroepidemiologic Studies, Antibodies, Bacterial analysis, Cattle Diseases diagnosis, Enzyme-Linked Immunosorbent Assay veterinary, Milk immunology, Mycoplasma Infections veterinary, Mycoplasma bovis immunology, Security Measures

Abstract

In Australia, one of the biosecurity recommendations to help prevent the introduction of Mycoplasma bovis into a dairy herd is to use a PCR assay on bulk tank milk (BTM) samples to evaluate the M. bovis infection status of potential source herds. An alternative approach is to assess the immunological status of the herd with respect to previous exposure to M. bovis via the use of an ELISA that is commercially available for use on cattle milk and serum. The objectives of this study were to (1) evaluate factors potentially associated with variation in the ELISA BTM optical density coefficient (ODC%) in previously exposed herds, (2) evaluate the association between the proportion of cows that are ELISA positive and the BTM ELISA ODC%, (3) assess agreement between the BTM ELISA and PCR and culture, and (4) compare BTM ELISA ODC% between the "hospital" herd and the main lactating herd on the same farm. Bulk tank milk samples (n = 192) were collected from 19 dairy herds with a history of clinical M. bovis disease and from 6 control herds (herds with no known clinical cases of mycoplasmosis). For 28 of the BTM samples collected, blood was also collected from 50 lactating cows contributing to that bulk tank sample. From 1 herd, concurrent paired BTM samples were collected from the main herd and the hospital herd on 16 occasions. All BTM samples were analyzed by ELISA (Bio-X Bio K 302, Bio-X Diagnostics, Rochefort, Belgium), PCR, and culture. The BTM ELISA ODC% was associated with time since initial M. bovis outbreak and time since the start of the herd's calving period. Following an initial outbreak of M. bovis, the BTM ELISA ODC% was highest in the first 8 mo. In split- and seasonal-calving herds, significantly higher BTM ELISA ODC% results were observed 5 to 8 wk after the commencement of the calving period. A significant association was observed between the within-herd seroprevalence for the lactating herd and BTM ELISA ODC%, but within-herd seroprevalence explained little of the variation in BTM ELISA ODC%. When comparing the BTM ELISA with a multiplex probe PCR and culture followed by 16S to 23S rRNA sequencing, there was virtually no agreement above that expected by chance; prevalence-adjusted bias-adjusted kappa values were 0.22 and 0.25 for ELISA category versus PCR category and culture, respectively. Finally, the hospital herd BTM ELISA ODC% mirrored that for the main herd BTM but was significantly higher. This study demonstrates that this commercially available ELISA used on BTM samples may complement the use of BTM PCR or culture in identifying herds from which purchase of animals may pose a higher biosecurity risk for introduction of M. bovis into noninfected herds., (Copyright © 2017 American Dairy Science Association. Published by Elsevier Inc. All rights reserved.)

Published

2017

37. Vector-borne and zoonotic diseases of dogs in North-west New South Wales and the Northern Territory, Australia.

Author

Shapiro AJ, Brown G, Norris JM, Bosward KL, Marriot DJ, Balakrishnan N, Breitschwerdt EB, and Malik R

Subjects

Anaplasma isolation & purification, Anemia veterinary, Animals, Babesia isolation & purification, Coxiella burnetii isolation & purification, DNA, Bacterial, DNA, Protozoan, Dog Diseases microbiology, Dog Diseases parasitology, Dogs, Humans, Mycoplasma isolation & purification, New South Wales epidemiology, Northern Territory epidemiology, Protozoan Infections, Animal epidemiology, Real-Time Polymerase Chain Reaction, Thrombocytopenia veterinary, Zoonoses microbiology, Zoonoses parasitology, Dog Diseases epidemiology, Zoonoses epidemiology

Abstract

Background: Vector-borne diseases of dogs in Australian Aboriginal communities are relatively unexplored. These dogs represent a unique group with variable ecto- and endo-parasitic burdens, nutritional stresses and a general lack of veterinary intervention. We investigated haemoprotozoal and bacterial pathogen prevalences in relation to erythrocyte and platelet numbers in dogs from North-West New South Wales (N-W NSW) and the Northern Territory (NT; Central Australia)., Methods: Real-time PCR (qPCR) amplification of Anaplasma platys, Babesia vogeli, Mycoplasma haemocanis, Candidatus Mycoplasma haematoparvum and Bartonella spp., serological screening for Coxiella burnetii, and Bartonella spp. and haematological analyses were performed on dogs from the two cohorts (96 dogs in total). Brucella suis serology was determined additionally for the N-W NSW cohort., Results: Anaplasma platys (n = 26 dogs), Babesia vogeli (n = 7), Candidatus Mycoplasma haematoparvum (n = 10 dogs), and Mycoplasma haemocanis (n = 14) were detected in the sample population (n = 96) using qPCR. There were significant associations between (i) A. platys and anaemia (OR 8.7, CI 2.4-31.7; P < 0.001), thrombocytopenia (OR 12.1, CI 3.4-43.2; P < 0.001) and breed (OR 16.1, CI 2.1-121.5; P = 0.007), and (ii) between B. vogeli and anaemia (OR 11.8, CI 2.3-61.6; P = 0.003). Neither protozoal nor bacterial DNA loads, estimated using qPCR, were positively correlated with anaemia or thrombocytopenia. Haemotropic mycoplasmas were not associated with any haematologic abnormality. Four dogs from the NT were seropositive for Coxiella burnetii, while no dogs were seropositive for Brucella suis or to a panel of Bartonella spp. antigens. Despite directed efforts, Bartonella DNA was not detected in blood from any of the cohorts studied. A sample of dogs from the NT recruited specifically for Bartonella α-proteobacteria growth medium enrichment blood culture were also Bartonella PCR negative., Conclusions: Vector-borne pathogens occur in dogs free ranging near Aboriginal communities, with higher detection rates in NT than N-W NSW. The preponderant haematologic abnormalities were anaemia and thrombocytopenia, likely attributable to A. platys and B. vogeli infections, but also probably affected by nutritional, parasitic, lactational and environmental stressors. The absence of Bartonella spp. is of importance to the Australian setting, and work needs to be extended to tropical coastal communities where fleas are present as well as ticks. Dogs living in and around Aboriginal communities may provide valuable sentinel information on disease infection status of human public health significance.

Published

2017

38. Q Fever (Coxiella burnetii) Knowledge and Attitudes of Australian Cat Breeders and Their Husbandry Practices.

Author

Shapiro AJ, Norris JM, Bosward KL, and Heller J

Subjects

Animals, Australia epidemiology, Cat Diseases epidemiology, Cats, Humans, Q Fever epidemiology, Q Fever microbiology, Animal Husbandry, Cat Diseases microbiology, Coxiella burnetii physiology, Health Knowledge, Attitudes, Practice, Q Fever veterinary, Zoonoses

Abstract

A Q fever outbreak in a small animal veterinary hospital, associated with a cat caesarean section, initiated a cat seroprevalence study (n = 712) that found circulating antibodies to Coxiella burnetii was highest in cattery-confined breeding cats (9.3%). These findings stimulated interest about potential sources of C. burnetii infection for cats and humans associated with cats. Cat breeders are potentially a group at increased risk of C. burnetii infection, and this study sought to identify potential risk factors. A cross-sectional online survey was conducted targeting all domestic cat breeders registered with an affiliate member body in Australia in 2015. Responses from 177 cat breeders across Australia were analysed. Forty per cent of responding cat breeders had not heard of Q fever. Raw meat was fed as an integral constituent of the diet by 89% of respondents. Eighty per cent of respondents allowed queens access to the home for parturition, and assistance of queens and resuscitation of kittens at the time of birth were reported by 97% of respondents. Respondents who perceived some level of exposure to Q fever through their breeding activities were three times less likely to perform mouth-to-snout resuscitation (OR 0.3 95% CI 0.1-0.9; P = 0.034) than those who did not perceive a risk of exposure. Similarly, respondents who perceived Q fever as a risk through breeding activities were close to eight times more likely to use personal protective equipment during parturition (OR 7.7 95% CI 1.5-39.9; P = 0.015) than those who did not. Husbandry practices of cat breeders that may increase the risk of C. burnetii transmission require further targeted investigations to assess the contribution of these risk factors to the acquisition of disease. Concurrent education forums are recommended to inform Australian cat breeders of the aetiopathogenesis of Q fever., (© 2016 Blackwell Verlag GmbH.)

Published

2017

39. Comparison of culture and a multiplex probe PCR for identifying Mycoplasma species in bovine milk, semen and swab samples.

Author

Parker AM, House JK, Hazelton MS, Bosward KL, and Sheehy PA

Subjects

Animals, Cattle, Female, Male, Sensitivity and Specificity, Milk microbiology, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction standards, Mycoplasma genetics, Semen microbiology

Abstract

Mycoplasma spp. are a major cause of mastitis, arthritis and pneumonia in cattle, and have been associated with reproductive disorders in cows. While culture is the traditional method of identification the use of PCR has become more common. Several investigators have developed PCR protocols to detect M. bovis in milk, yet few studies have evaluated other sample types or other important Mycoplasma species. Therefore the objective of this study was to develop a multiplex PCR assay to detect M. bovis, M. californicum and M. bovigenitalium, and evaluate its analytical performance against traditional culture of bovine milk, semen and swab samples. The PCR specificity was determined and the limit of detection evaluated in spiked milk, semen and swabs. The PCR was then compared to culture on 474 field samples from individual milk, bulk tank milk (BTM), semen and swab (vaginal, preputial, nose and eye) samples. Specificity analysis produced appropriate amplification for all M. bovis, M. californicum and M. bovigenitalium isolates. Amplification was not seen for any of the other Mollicutes or eubacterial isolates. The limit of detection of the PCR was best in milk, followed by semen and swabs. When all three Mycoplasma species were present in a sample, the limit of detection increased. When comparing culture and PCR, overall there was no significant difference in the proportion of culture and PCR positive samples. Culture could detect significantly more positive swab samples. No significant differences were identified for semen, individual milk or BTM samples. PCR identified five samples with two species present. Culture followed by 16S-23S rRNA sequencing did not enable identification of more than one species. Therefore, the superior method for identification of M. bovis, M. californicum and M. bovigenitalium may be dependent on the sample type being analysed, and whether the identification of multiple target species is required.

Published

2017

40. Milk acidification to control the growth of Mycoplasma bovis and Salmonella Dublin in contaminated milk.

Author

Parker AM, House JK, Hazelton MS, Bosward KL, Mohler VL, Maunsell FP, and Sheehy PA

Subjects

Animals, Cattle, Cattle Diseases microbiology, Female, Ovum, Milk microbiology, Mycoplasma bovis growth & development, Salmonella enterica growth & development

Abstract

Bacterial contamination of milk fed to calves compromises calf health. Several bacterial pathogens that infect cows, including Mycoplasma bovis and Salmonella enterica ssp. enterica serovar Dublin, are shed in milk, providing a possible route of transmission to calves. Milk acidification lowers the milk pH so that it is unsuitable for bacterial growth and survival. The objectives of this study were to (1) determine the growth of M. bovis and Salmonella Dublin in milk, and (2) evaluate the efficacy of milk acidification using a commercially available acidification agent (Salstop, Impextraco, Heist-op-den-Berg, Belgium) to control M. bovis and Salmonella Dublin survival in milk. For the first objective, 3 treatments and a positive control were prepared in 10 mL of milk and broth, respectively, and inoculated with M. bovis or Salmonella Dublin to an approximate concentration of 10 4 cfu/mL. Each treatment was retained at 5, 23, or 37°C with the positive control at 37°C. Aliquots were taken at 4, 8, 24, 28, 32, 48, 52, and 56 h after inoculation and transferred onto agar medium in triplicate following a 10-fold dilution series in sterile phosphate-buffered saline. All plates were incubated and colonies counted. For the second objective, 4 treatments and a positive control were prepared with 100 mL of milk and inoculated with M. bovis or Salmonella Dublin to an approximate concentration of 10 6 cfu/mL. With the use of Salstop, treatments were adjusted to an approximate pH of 6, 5, 4, or 3.5. The positive control was left untreated. At 1, 2, 4, 6, 8, and 24 h after treatment, triplicate aliquots were taken, the pH measured, and then the aliquots were transferred onto agar medium and into broth for enrichment. Following incubation, agar colonies were counted, while broths were plated and incubated prior to colonies being counted. All trials were repeated. Mycoplasma bovis did not grow in milk, but Salmonella Dublin proliferated. The pH of all acidification treatments remained stable for 24 h. No viable M. bovis organisms were detected at 1 h of exposure to pH 3.5 and 4 or at 8 h of exposure to pH 5. Following 24 h of exposure to pH 6 M. bovis remained viable. No viable Salmonella Dublin organisms were detected at 2 and 6 h of exposure to pH 3.5 and 4, respectively. Salmonella Dublin remained viable following 24 h of exposure to pH 5 and 6. These results demonstrate that milk acidification using Salstop is effective at eliminating viable M. bovis and Salmonella Dublin organisms in milk if the appropriate pH and exposure time are maintained., (Copyright © 2016 American Dairy Science Association. Published by Elsevier Inc. All rights reserved.)

Published

2016

41. Genetic characterization of Australian Mycoplasma bovis isolates through whole genome sequencing analysis.

Author

Parker AM, Shukla A, House JK, Hazelton MS, Bosward KL, Kokotovic B, and Sheehy PA

Subjects

Animals, Australia, Bacterial Proteins genetics, Cattle, Female, Genomics, Lipoproteins genetics, Mycoplasma Infections microbiology, Mycoplasma bovis isolation & purification, Virulence Factors genetics, Genetic Variation, Genome, Bacterial genetics, Mastitis, Bovine microbiology, Mycoplasma Infections veterinary, Mycoplasma bovis genetics

Abstract

Mycoplasma bovis is a major pathogen in cattle causing mastitis, arthritis and pneumonia. First isolated in Australian cattle in 1970, M. bovis has persisted causing serious disease in infected herds. To date, genetic analysis of Australian M. bovis isolates has not been performed. With whole genome sequencing (WGS) becoming a common tool for genetic characterization, this method was utilized to determine the degree of genetic diversity among Australian M. bovis isolates collected over a nine year period (2006-2015) from various geographical locations, anatomical sites, and from clinically affected and non-clinical carrier animals. Eighty-two M. bovis isolates underwent WGS from which single nucleotide polymorphism (SNP) analysis, comparative genomics and analysis of virulence genes was completed. SNP analysis identified a single M. bovis strain circulating throughout Australia with marked genomic similarity. Comparative genomics suggested minimal variation in gene content between isolates from clinical and carrier animals, and between isolates recovered from different anatomical sites. A total of 50 virulence genes from the virulence factors database (VFDB) were identified as highly similar in the Australian isolates, while the presence of variable surface lipoprotein (vsp) genes was greatly reduced compared to reference strain M. bovis PG45. These results highlight that, while the introduction of multiple M. bovis strains has been prevented, elimination of the current strain has not been successful. The persistence of this strain may be due to the significant role that carrier animals play in harboring the pathogen. The similarity of clinical and non-clinical isolates suggests host and environmental factors play a significant role in determining host pathogen outcomes., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published

2016

42. Seroprevalence of Coxiella burnetii in Australian dogs.

Author

Shapiro AJ, Norris JM, Heller J, Brown G, Malik R, and Bosward KL

Subjects

Aging, Animals, Antibodies, Bacterial blood, Australia epidemiology, Dog Diseases blood, Dog Diseases epidemiology, Dogs, Female, Male, Q Fever blood, Q Fever epidemiology, Seroepidemiologic Studies, Coxiella burnetii, Dog Diseases microbiology, Q Fever veterinary

Abstract

The role of dogs in the transmission of Coxiella burnetii to humans is uncertain, and extensive seroprevalence studies of dogs have not been previously conducted in Australia. This study determined C. burnetii exposure in four diverse canine subpopulations by adapting, verifying and comparing an indirect immunofluoresence assay (IFA) and an enzyme-linked immunosorbent assay (ELISA) used to detect anti-C. burnetii antibodies in humans. Canine serum samples (n = 1223) were tested with IFA from four subpopulations [breeding establishments; household pets; free-roaming dogs in Aboriginal communities; shelter dogs]. The proportions of seropositive dogs were as follows: breeding (7/309, 2.3%), household pets (10/328, 3%), Aboriginal communities (21/321, 6.5%) and shelters (5/265, 1.9%). Dogs from Aboriginal communities were 2.8 times (CI 1.5-5.1; P < 0.001) more likely to be seropositive than dogs from other populations. The ELISA was used on 86 of 1223 sera tested with IFA, and a Cohen's Kappa coefficient of 0.60 (CI 0.43-0.78) indicated good agreement between the two assays. This study has established that Australian dogs within all four subpopulations have been exposed to C. burnetii and that a higher seroprevalence was observed amongst free-roaming dogs associated with Aboriginal communities. As C. burnetii recrudesces during pregnancy and birth products contain the highest concentration of organism, individuals assisting at the time of parturition, those handling pups shortly after birth as well as those residing in the vicinity of whelping dogs are potentially at risk of developing Q fever. However, the identification of active antigen shed in excreta from seropositive dogs is required in order to accurately define and quantify the public health risk., (© 2016 Blackwell Verlag GmbH.)

Published

2016

43. Development of a loop-mediated isothermal amplification assay for the detection of Streptococcus agalactiae in bovine milk.

Author

Bosward KL, House JK, Deveridge A, Mathews K, and Sheehy PA

Subjects

Animals, Cattle, Female, Food Contamination analysis, Food Microbiology, Mastitis, Bovine microbiology, Polymerase Chain Reaction veterinary, Sensitivity and Specificity, Streptococcus agalactiae genetics, DNA, Bacterial isolation & purification, Milk microbiology, Streptococcus agalactiae isolation & purification

Abstract

Streptococcus agalactiae is a well-characterized bovine mastitis pathogen that is known to be highly contagious and capable of spreading rapidly in affected dairy herds. Loop-mediated isothermal amplification (LAMP) is a novel molecular diagnostic method that has the capability to provide rapid, cost-effective screening for pathogens to support on-farm disease control and eradication programs. In the current study, a LAMP test was developed to detect S. agalactiae in milk. The assay was validated on a bank of existing clinical mastitis milk samples that had previously been identified as S. agalactiae positive via traditional microbiological culture techniques and PCR. The LAMP assay was conducted on bacterial colonies and DNA extracted from milk in tube- and plate-based formats using multiple detection platforms. The 1-h assay conducted at 64 °C exhibited repeatability (coefficient of variation) of 2.07% (tube) and 8.3% (plate), sensitivity to ~20 pg of extracted DNA/reaction, and specificity against a panel of known bacterial mastitis pathogens. Of the 109 known S. agalactiae isolates assessed by LAMP directly from bacterial cells in culture, 108 were identified as positive, in accordance with PCR analysis. The LAMP analysis from the corresponding milk samples indicated that 104 of these milks exhibited a positive amplification curve. Although exhibiting some limitations, this assay provides an opportunity for rapid screening of milk samples to facilitate on-farm management of this pathogen., (Copyright © 2016 American Dairy Science Association. Published by Elsevier Inc. All rights reserved.)

Published

2016

44. Q Fever Knowledge, Attitudes and Vaccination Status of Australia's Veterinary Workforce in 2014.

Author

Sellens E, Norris JM, Dhand NK, Heller J, Hayes L, Gidding HF, Willaby H, Wood N, and Bosward KL

Subjects

Adult, Aged, Aged, 80 and over, Australia, Coxiella burnetii immunology, Demography, Female, Humans, Logistic Models, Male, Middle Aged, Nurses, Occupational Exposure, Risk Factors, Young Adult, Health Knowledge, Attitudes, Practice, Q Fever immunology, Q Fever prevention & control, Vaccination, Veterinarians

Abstract

Q fever, caused by Coxiella burnetii, is a serious zoonotic disease in humans with a worldwide distribution. Many species of animals are capable of transmitting C. burnetii, and consequently all veterinary workers are at risk for this disease. An effective Q fever vaccine has been readily available and used in Australia for many years in at-risk groups, and the European Centre for Disease Prevention and Control has recently also called for the use of this vaccine among at-risk groups in Europe. Little is known about attitudes towards this vaccine and vaccine uptake in veterinary workers. This study aimed to determine the Q fever vaccination status of veterinarians and veterinary nurses in Australia and to assess and compare the knowledge and attitudes towards Q fever disease and vaccination of each cohort. An online cross-sectional survey performed in 2014 targeted all veterinarians and veterinary nurses in Australia. Responses from 890 veterinarians and 852 veterinary nurses were obtained. Binary, ordinal and multinomial logistic regression were used to make comparisons between the two cohorts. The results showed that 74% of veterinarians had sought vaccination compared to only 29% of veterinary nurses. Barriers to vaccination among those not vaccinated did not differ between cohorts, and included a lack of perceived risk, financial expense, time constraints, and difficulty in finding a vaccine provider. Poor knowledge and awareness of Q fever disease and vaccination were additional and notable barriers for the veterinary nursing cohort, suggesting veterinary clinics and veterinarians may not be meeting their legal responsibility to educate staff about risks and risk prevention. Further evaluation is needed to identify the drivers behind seeking and recommending vaccination so that recommendations can be made to improve vaccine uptake.

Published

2016

45. Seroprevalence of Coxiella burnetii in domesticated and feral cats in eastern Australia.

Author

Shapiro AJ, Bosward KL, Heller J, and Norris JM

Subjects

Animals, Antibodies, Bacterial blood, Australia epidemiology, Enzyme-Linked Immunosorbent Assay veterinary, Female, Humans, Pregnancy, Q Fever epidemiology, Q Fever microbiology, Seroepidemiologic Studies, Cat Diseases epidemiology, Cat Diseases microbiology, Cats, Coxiella burnetii immunology, Q Fever veterinary

Abstract

The seroprevalence of Coxiella burnetii (C. burnetii) in cats in eastern Australia is unknown, and the risk of transmission from cats to humans is undetermined. This study aimed to determine the exposure of cats to C. burnetii in four distinct cat subpopulations. An indirect immunofluoresence assay (IFA) and an Enzyme-linked immunosorbent assay (ELISA) used for detection of anti-C. burnetii antibodies in humans were adapted, verified for use on feline serum, and compared. Cat serum samples (n=712) were tested with IFA from four subpopulations [cattery-confined breeding cats, pet cats, feral cats and shelter cats]. The proportions of seropositive cats were; cattery-confined breeding cats (35/376, 9.3%), pets (2/198, 1%), feral cats (0/50), shelter cats (0/88). The significant variables in C. burnetii seropositivity were cattery-confined breeding cat subpopulation and sterilisation status, with infected cats 17.1 (CI 4.2-70.2; P<0.001) times more likely to be cattery-confined breeding cats and 6.00 (CI 2.13-16.89; P<0.001) times more likely to be entire than sterilised. ELISA was used on 143 of 712 sera tested with IFA, and the Cohen's Kappa coefficient of 0.75 indicated 92.2% agreement between the two assays. These results confirm that Australian cats have been exposed to C. burnetii and that a higher seroprevalence of C. burnetii is seen amongst cattery-confined breeding cats. Cat breeders and veterinary personnel involved in feline reproductive procedures may be at higher risk of exposure to C. burnetii., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2015

46. Investigating Coxiella burnetii infection in a breeding cattery at the centre of a Q fever outbreak.

Author

Kopecny L, Bosward KL, Shapiro A, and Norris JM

Subjects

Animals, Anti-Bacterial Agents therapeutic use, Australia epidemiology, Cat Diseases drug therapy, Cat Diseases mortality, Cats, Female, Male, Q Fever drug therapy, Q Fever epidemiology, Q Fever microbiology, Q Fever mortality, Serologic Tests, Cat Diseases microbiology, Coxiella burnetii isolation & purification, Disease Outbreaks veterinary, Q Fever veterinary

Abstract

The potential role of cats in transmitting Coxiella burnetii to humans was highlighted in a Q fever outbreak, linked to a caesarean section in a breeding queen, in an Australian small animal veterinary hospital. The objectives of this study were to evaluate the C burnetii seroreactivity of the breeding queen and other cats residing at the same breeding cattery (n = 27) and to evaluate C burnetii infection of the breeding queen by molecular and histological methods. Three assays [complement fixation test (CFT), indirect immunofluorescence assay (IFA) and enzyme-linked immunosorbent assay (ELISA)] were used for serological evaluation. Additionally, uterine and ovarian samples collected from the breeding queen 11 weeks post-parturition were assessed by routine and specialised histological methods and polymerase chain reaction. The breeding queen showed strong seropositivity using CFT (titre 1/32), IFA (titre phase I 1/8192 and phase II 1/8192) and ELISA; however, the reproductive tract showed no evidence of pathology or C burnetii infection. A number of cattery-confined cats were identified as seropositive to phase II and/or phase I C burnetii. Serological detection of C burnetii in a breeding cattery linked to a Q fever outbreak indicates likely infection by this bacterium in Australian feline populations, re-confirming the relevance of this zoonosis.

Published

2013

47. Optimization of a whole blood gamma interferon assay for the detection of sheep infected with Mycobacterium avium subspecies paratuberculosis.

Author

Bosward KL, Dhand NK, Begg DJ, Thomson PC, Emery DL, and Whittington RJ

Subjects

Animals, Anticoagulants, Bacteriological Techniques, Blood Cell Count, Enzyme-Linked Immunosorbent Assay veterinary, Leukocytes, Paratuberculosis blood, Sheep, Specimen Handling veterinary, Temperature, Interferon-gamma blood, Mycobacterium avium subsp. paratuberculosis, Paratuberculosis diagnosis, Sheep Diseases diagnosis

Abstract

The capacity of a commercially available gamma interferon (IFNgamma) assay to detect infected sheep early in the pathogenesis of Johne's disease enables the removal of such animals from the flock before bacterial shedding and pasture contamination. However, nonspecific IFNgamma responses in the assay have meant that to achieve high-test specificity, there has been a reduction in sensitivity. Although the optimal conditions for the use of the assay in cattle have been well documented, there have been few studies optimizing the assay for use in sheep. The current study details the effect of anticoagulant, duration of incubation, cell concentration, blood storage temperature, time of stimulation of cells with antigen relative to time of sample collection, and temperatures during transit on IFNgamma synthesis. Maximal IFNgamma synthesis occurred with incubation periods of 48 hr in blood collected into heparinized tubes. Decreasing the leukocyte population by diluting the total peripheral blood leukocyte concentration was associated with a decreasing IFNgamma response. Conversely, concentrating the peripheral blood concentration 2-fold resulted in an increase in the IFNgamma production. In field studies, immediate incubation of blood samples with antigen at 37 degrees C resulted in larger IFNgamma responses; however, significantly lower IFNgamma values were obtained if the samples were transported at ambient temperature. The results of this study indicate that optimization of the IFNgamma assay may enable increased synthesis of IFNgamma during the stimulation phase of the assay and that future work may determine whether this translates to increased sensitivity of the assay in detecting early infections in sheep.

Published

2010

48. Immunohistological evaluation of feline herpesvirus-1 infection in feline eosinophilic dermatoses or stomatitis.

Author

Lee M, Bosward KL, and Norris JM

Subjects

Alphaherpesvirinae immunology, Alphaherpesvirinae isolation & purification, Animals, Cats, Eosinophilic Granuloma pathology, Female, Herpesviridae Infections pathology, Immunohistochemistry veterinary, Male, Skin Diseases pathology, Stomatitis pathology, Cat Diseases pathology, Eosinophilic Granuloma veterinary, Herpesviridae Infections veterinary, Skin Diseases veterinary, Stomatitis veterinary

Abstract

This study used immunohistochemistry (IHC) and histopathology to evaluate the presence of feline herpesvirus-1 (FHV-1) in feline cases of 'eosinophilic granuloma complex' (EGC) or other eosinophilic dermatoses or stomatitis, diagnosed at the Veterinary Pathology Diagnostic Service, University of Sydney between January 1996 and June 2008. Two of the 30 cases (6.6%) examined showed positive immunoreactivity to FHV-1 using IHC. Intranuclear inclusion bodies were also detected on histopathological examination of haematoxylin and eosin stained sections of both cases but were very difficult to find. Therefore, FHV-1 is uncommonly associated with EGC or other eosinophilic dermatoses or stomatitis in Sydney. However, misdiagnosis as an EGC lesion or other eosinophilic dermatoses may occur if inclusion bodies are overlooked or absent on histopathology and this may significantly decrease the chance of a favourable treatment outcome. FHV-1 should be considered in cats with severe ulcerative cutaneous or oral lesions, unresponsive to corticosteroid treatment, with or without concurrent or historical signs of upper respiratory tract or ocular disease more typical of FHV-1. IHC may be helpful in differentiating FHV-1 dermatitis or stomatitis from other eosinophilic lesions, which is of vital clinical and therapeutic importance., (Crown Copyright 2009. Published by Elsevier Ltd. All rights reserved.)

Published

2010

49. Persistent haematuria and proteinuria due to glomerular disease in related Abyssinian cats.

Author

White JD, Norris JM, Bosward KL, Fleay R, Lauer C, and Malik R

Subjects

Animals, Disease Progression, Female, Glomerulonephritis complications, Hematuria etiology, Kidney Glomerulus pathology, Male, Proteinuria etiology, Species Specificity, Cat Diseases diagnosis, Cats classification, Glomerulonephritis veterinary, Hematuria veterinary, Proteinuria veterinary

Abstract

Eight cases of glomerular disease in young, related Abyssinian cats are described. Haematuria was the most consistent feature. Six cats developed the nephrotic syndrome. The short-term prognosis was good for cats with haematuria and fair for cats with the nephrotic syndrome as oedema resolved in three of the six cats. Light microscopic examination of renal biopsies from three cats was considered normal or revealed only mild abnormalities. In the three cases subjected to necropsy, histological abnormalities included mild mesangial hypercellularity and adhesions between the glomerular tuft and Bowman's capsule consistent with a focal proliferative glomerulopathy. Further investigation into this glomerulopathy will require ultrastructural and immunohistochemical studies to characterise the glomerular abnormality and genetic analyses to investigate its potential to be an inherited disease. Glomerular disease, potentially a familial one, should be considered in the investigation of persistent haematuria or proteinuria in Abyssinian and related cats.

Published

2008

50. Integrated Case-Based Applied Pathology (ICAP): a diagnostic-approach model for the learning and teaching of veterinary pathology.

Author

Krockenberger MB, Bosward KL, and Canfield PJ

Subjects

Animals, Australia, Case-Control Studies, Diagnosis, Differential, Education, Distance, Humans, Internet, Problem-Based Learning, Education, Veterinary methods, Education, Veterinary standards, Learning physiology, Pathology, Veterinary education, Pathology, Veterinary standards, Teaching methods

Abstract

Integrative Case-Based Applied Pathology (ICAP) cases form one component of learning and understanding the role of pathology in the veterinary diagnostic process at the Faculty of Veterinary Science, University of Sydney. It is a strategy that focuses on student-centered learning in a problem-solving context in the year 3 curriculum. Learning exercises use real case material and are primarily delivered online, providing flexibility for students with differing learning needs, who are supported by online, peer, and tutor support. The strategy relies heavily on the integration of pre-clinical and para-clinical information with the introduction of clinical material for the purposes of a logical three-level, problem-oriented approach to the diagnosis of disease. The focus is on logical diagnostic problem solving, primarily using gross pathology and histopathological material, with the inclusion of microbiological, parasitological, and clinical pathological data. The ICAP approach is linked to and congruent with the problem-oriented approach adopted in veterinary medicine and the case-based format used by one of the authors (PJC) for the teaching and learning of veterinary clinical pathology in year 4. Additionally, final-year students have the opportunity, during a diagnostic pathology rotation, to assist in the development and refinement of further ICAPs, which reinforces the importance of pathology in the veterinary diagnostic process. Evidence of the impact of the ICAP approach, based primarily on student surveys and staff peer feedback collected over five years, shows that discipline-specific learning, vertical and horizontal integration, alignment of learning outcomes and assessment, and both veterinary and generic graduate attributes were enhanced. Areas for improvement were identified in the approach, most specifically related to assistance in the development of generic teamwork skills.

Published

2007