Competitive ELISA for Serodiagnosis of Bluetongue: Evaluation of Group-Specific Monoclonal Antibodies and Expressed VP7 Antigen

Author:

Afshar Ahmad1,Eaton Bryan T.2,Wright Peter F.3,Pearson James E.4,Anderson John5,Jeggo Martyn3,Trotter Holly C.1

Affiliation:

1. Animal Diseases Research Institute, Agriculture Canada, PO Box 11300, Station H, Nepean, Ontario K2H 8P9, Canada

2. Australian Animal Health Laboratories, PO Bags 24, Geelong, Victoria 3220, Australia

3. International Atomic Energy Agency, Wagramerstrasse 5, PO Box 100, A-1400 Vienna, Austria

4. National Veterinary Services Laboratories, USDA-APHIS, PO Box 844, Ames, IA 50010, USA

5. Institute for Animal Health, Pirbright Laboratory, Ash Road, Pirbright, Woking GU24 ONF, UK

Abstract

The performance of 2 competitive enzyme-linked immunosorbent assays (C-ELISA) was compared with the reference C-ELISA I for the detection of antibodies to bluetongue virus (BTV). One of the assays (C-ELISA II) used a group-specific monoclonal antibody (MAb) to BTV, obtained from the American Type Culture Collection (8A3B-6) and tissue culture (TC)-derived BTV antigen (Ag), and the other assay (C-ELISA III) used BTV core protein VP7 (expressed in yeast) and the reference MAb (Pirbright Laboratory, 3–17-A3). Test sera were obtained by sequential blood samples from 22 calves, each inoculated with a different serotype (T) of BTV (South African [SA] T-1-T-16 and T-18-T-20 and USA T-11, T-13, and T-1 7). Sera were also obtained from 4 calves and 4 sheep inoculated with USA BTV T-10 and from several groups of calves exposed to single or multiple doses of epizootic hemorrhagic disease virus (EHDV) T-1-T-4 grown in TC (BHK-21) or suckling mouse brain (SMB). A total of 618 bovine and ovine field sera collected from BT-free and BT-endemic areas were also tested. The C-ELISA III was more sensitive than the C-ELISA II in the detection of anti-BTV antibody in sera from cattle and sheep early after infection with BTV. Seroconversion was demonstrated by the 3 C-ELISAs in all animals inoculated with BTV by 20 days postinfection (DPI), except in calves that received SA T-3 or USA T-13, which became positive at 40 DPI. Unlike with the immunodiffusion test, reaction was not generally seen between BTV TC-derived or VP7 antigens and sera from calves exposed to a single dose of EHDV T-1, T-2, T-3, or T-4 or from calves that received TC-derived EHDV T-1 or T-2 initially and were then challenged with the heterologous EHDVs. Postchallenge samples from calves inoculated and challenged with SMB-derived EHDV T-2 and T-1, respectively, resulted in false reactions in all the C-ELISAs. Relative to the reference C-ELISA I results, the C-ELISA II and C-ELISA III results for the field sera demonstrated lower levels of agreement for bovine samples (97.8% and 96.5%, respectively) than for ovine sera (99.3% and 98.2%, respectively). The overall results suggest that both MAb 8A3B-6 and yeast-expressed VP7 may be suitable as diagnostic reagents in C-ELISA for the detection of anti-BTV group-specific antibodies.

Publisher

SAGE Publications

Subject

General Veterinary

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