Abstract
BackgroundFeline panleukopenia virus (FPV) is an etiologic pathogen of feline panleukopenia that infects all members of Felidae including tigers (Panthera tigris). Vaccinations against FPV among wild felid species have long been practiced in zoos worldwide. However, few studies have assessed the tiger immune response post-vaccination due to the absence of a serological diagnostic tool. To address these limitations, this study aimed to develop an in-house indirect enzyme-linked immunosorbent assay (ELISA) for the monitoring of tiger antibody levels against the feline panleukopenia vaccine by employing the synthesized subunit capsid protein VP2. An in-house horseradish peroxidase (HRP) conjugated rabbit anti-tiger immunoglobulin G (IgG) polyclonal antibody (HRP-anti-tiger IgG) was produced in this study and employed in the assay. It was then compared to a commercial HRP-conjugated goat anti-cat IgG (HRP-anti-cat IgG). Sensitivity and specificity were evaluated using the Bayesian model with preferential conditional dependence between HRP-conjugated antibody-based ELISAs and hemagglutination-inhibition (HI) tests.ResultsThe posterior estimates for sensitivity and specificity of two indirect ELISA HRP-conjugated antibodies were higher than those of the HI test. The sensitivity and specificity of the indirect ELISA for HRP-anti-tiger IgG and HRP-anti-cat IgG were 86.5, 57.2 and 86.7%, 64.6%, respectively, while the results of the HI test were 79.1 and 54.1%. In applications, 89.6% (198/221) and 89.1% (197/221) of the tiger serum samples were determined to be seropositive by indirect ELISA testing against HRP-anti-tiger and HRP-anti-cat, respectively.ConclusionTo the best of our knowledge, the specific serology assays for the detection of the tiger IgG antibody have not yet been established. The HRP-anti-tiger IgG has been produced for the purpose of developing the specific immunoassays for tigers. Remarkably, an in-house indirect ELISA based on VP2 subunit antigen has been successfully developed in this study, providing a potentially valuable serological tool for the effective detection of tiger antibodies.
Highlights
Feline panleukopenia virus (FPV) is an etiologic pathogen of feline panleukopenia that infects all members of Felidae including tigers (Panthera tigris)
Generation and binding capability of horseradish peroxidase (HRP)-conjugated rabbit anti-tiger immunoglobulin G (IgG) antibody The purified rabbit anti-tiger IgG was conjugated with HRP
2.651 2.283 2.000 1.582 1.637 a Represents suitable signal to noise (S/N) ratio obtained from this study at 1:20, the seropositive value of tiger antibodies against FPV vaccine was 80% (178/221)
Summary
Feline panleukopenia virus (FPV) is an etiologic pathogen of feline panleukopenia that infects all members of Felidae including tigers (Panthera tigris). Dissanayake et al (2017) [7] reported on the death of an unvaccinated Bengal tiger cub (Panthera tigris tigris) and severe illness in an unvaccinated leopard cub (Panthera pardus) at a zoological garden in Sri Lanka, both of which were caused by FPV. These incidences indicated that tigers, which are the largest known cat species, appear to be susceptible to FPV infection. Feline panleukopenia in tigers should be of significant concern because tigers are an endangered species according to the International Union for Conservation of Nature’s (IUCN) Red List of Threatened Species [8]
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