"Spotting" Mycobacterium bovis infection in leopards (Panthera pardus) - novel application of diagnostic tools

Rachiel Gumbo; Wynand J Goosen; Peter E Buss; Lin-Mari de Klerk-Lorist; Konstantin Lyashchenko; Robin M Warren; Paul D van Helden; Michele A Miller; Tanya J Kerr

doi:10.3389/fimmu.2023.1216262

"Spotting" Mycobacterium bovis infection in leopards (Panthera pardus) - novel application of diagnostic tools

Front Immunol. 2023 Sep 1:14:1216262. doi: 10.3389/fimmu.2023.1216262. eCollection 2023.

Authors

Rachiel Gumbo¹, Wynand J Goosen¹, Peter E Buss², Lin-Mari de Klerk-Lorist³, Konstantin Lyashchenko⁴, Robin M Warren¹, Paul D van Helden¹, Michele A Miller¹, Tanya J Kerr¹

Affiliations

¹ DSI-NRF Centre of Excellence for Biomedical Tuberculosis Research, SAMRC Centre for Tuberculosis Research, Division of Molecular Biology and Human Genetics, Faculty of Medicine and Health Sciences, Stellenbosch University, Cape Town, South Africa.
² South African National Parks, Veterinary Wildlife Services, Kruger National Park, Skukuza, South Africa.
³ Skukuza State Veterinary Office, Department of Agriculture, Land Reform and Rural Development, Skukuza, South Africa.
⁴ Chembio Diagnostic Systems, Inc., Medford, New York, NY, United States.

Abstract

Background: Mycobacterium bovis (M. bovis) is the causative agent of animal tuberculosis (TB) which poses a threat to many of South Africa's most iconic wildlife species, including leopards (Panthera pardus). Due to limited tests for wildlife, the development of accurate ante-mortem tests for TB diagnosis in African big cat populations is urgently required. The aim of this study was to evaluate currently available immunological assays for their ability to detect M. bovis infection in leopards.

Methods: Leopard whole blood (n=19) was stimulated using the QuantiFERON Gold Plus In-Tube System (QFT) to evaluate cytokine gene expression and protein production, along with serological assays. The GeneXpert^® MTB/RIF Ultra (GXU^®) qPCR assay, mycobacterial culture, and speciation by genomic regions of difference PCR, was used to confirm M. bovis infection in leopards.

Results: Mycobacterium bovis infection was confirmed in six leopards and individuals that were tuberculin skin test (TST) negative were used for comparison. The GXU^® assay was positive using all available tissue homogenates (n=5) from M. bovis culture positive animals. Mycobacterium bovis culture-confirmed leopards had greater antigen-specific responses, in the QFT interferon gamma release assay, CXCL9 and CXCL10 gene expression assays, compared to TST-negative individuals. One M. bovis culture-confirmed leopard had detectable antibodies using the DPP^® Vet TB assay.

Conclusion: Preliminary results demonstrated that immunoassays and TST may be potential tools to identify M. bovis-infected leopards. The GXU^® assay provided rapid direct detection of infected leopards. Further studies should aim to improve TB diagnosis in wild felids, which will facilitate disease surveillance and screening.

Keywords: DPP® Vet TB assay; GeneXpert® MTB/RIF Ultra qPCR assay; Mycobacterium bovis; Panthera pardus; gene expression assay; interferon-gamma release assay; leopard; tuberculin skin test.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Animals, Wild
Antibodies
Cats
Mycobacterium Infections*
Mycobacterium bovis*
Panthera*

Substances

Antibodies

Grants and funding

This research was funded by the South African Medical Research Council (SAMRC) Centre for Tuberculosis Research, National Research Foundation (NRF) South African Research Chair Initiative (SARChI grant 86949), American Association of Zoo Veterinarians (AAZV) Wild Animal Health Fund (WAHF) (AAZV WAHF Grant 2020 #4) and The Harry Crossley Foundation. Funding to RG was provided through a Stellenbosch University (SU) Postgraduate Scholarship (2021) and German Academic Exchange Service (DAAD) In-Region Scholarship SUN MBHG South Africa (2022-2023). Funding to TK was provided through DSI-NRF PDP Fellowship within the SAMRC Centre for Tuberculosis Research.