Evaluation of ELISA and PCR in parallel to single intradermal cervical tuberculin test (SICT) for diagnosis of tuberculosis in buffaloes

被引:0
作者
Bincy Joseph
Amit Kumar Pandey
Ashok Kumar
Dushyant Kumar Sharma
Ajay Kumar Yadav
Bablu Kumar
Vishal Abhishek
Gaurav Kumar Chander
Ajay Pratap Sharma
Chandan Singh
机构
[1] RAJUVAS,Department of Veterinary Microbiology, Postgraduate Institute of Veterinary Education and Research
[2] RAJUVAS,Department of Veterinary Biochemistry, College of Veterinary and Animal Science
[3] ICAR-Central Sheep and Wool Research Institute,Division of Animal Reproduction
[4] ICAR-Central Sheep and Wool Research Institute,Division of Animal Health
[5] ICAR-Indian Veterinary Research Institute,Division of Biological Products
[6] ICAR-Indian Veterinary Research Institute,Division of Bacteriology and Mycology
[7] ICAR-Indian Veterinary Research Institute,Centre for Animal Research and Diagnosis
[8] DUVASU,Division of Veterinary Microbiology, College of Veterinary Science
来源
Tropical Animal Health and Production | 2021年 / 53卷
关键词
Skin test (SICT); Tuberculosis; Buffaloes; ELISA; PCR;
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摘要
Bovine tuberculosis is an economically important disease with very high zoonotic potential. Single intradermal cervical tuberculin test (SICT) is considered a gold standard assay for the diagnosis of bovine tuberculosis. However, bovines especially buffaloes may produce a false negative result when the animal becomes cell-mediated immune (CMI) anergic in the advanced stage of the disease. In the present study, ELISA and PCR assays were successfully demonstrated to be useful in diagnosing tuberculosis especially in the CMI anergic buffaloes infected with Mycobacterium bovis. ELISA and PCR assays are able to detect 8.94% and 8.13%, respectively, more animals as positive in comparison to standard SICT assay in a selected population of 123 buffaloes. The moderate agreement between SICT and ELISA (k: 0.528; 0.249–0.807), a substantial agreement between SICT and PCR (k: 0.648; 0.364–0.931), and high agreement between ELISA and PCR (k: 0.856; 0.697–1.0) highlight that ELISA and PCR, if used in parallel with SICT, will provide better sensitivity over single assay. Reduction of false negative reactors may help in minimizing the zoonotic threat from bovine tuberculosis especially in disease endemic region where human and livestock interface is quite high.
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