Kh. Nielsen et al., IMPROVED COMPETITIVE ENZYME-IMMUNOASSAY FOR THE DIAGNOSIS OF BOVINE BRUCELLOSIS, Veterinary immunology and immunopathology, 46(3-4), 1995, pp. 285-291
A modification of the competitive enzyme-linked immunosorbent assay (C
-ELISA) for differentiating the antibody response of cattle vaccinated
with Brucella abortus strain 19 and B. abortus infected cattle is des
cribed. This assay utilizes lipopolysaccharide as the antigen, immobil
ized on a polystyrene matrix, and a monoclonal antibody (M84) with spe
cificity for an epitope of the O-polysaccharide. A goat anti-mouse IgG
antibody-enzyme conjugate is used for detection. The specificity of t
he modified assay was 99.7% when 1446 sera from brucellosis free herds
were tested and it correctly identified 636 sera from B. abortus infe
cted cattle as positive, using a cut-off of 30% inhibition, for a sens
itivity estimate of 100%. No reactions were noted among 261 sera from
vaccinated cattle. However, in testing 1147 sera that gave positive re
actions in the buffered plate antigen test, the indirect ELISA, the co
mplement fixation test or a combination of these tests from the serum
bank, 31 gave positive reactions. Twenty-seven of the 31 sera originat
ed from recently vaccinated cattle. The overall specificity for sera f
rom vaccinated cattle was 97.3%. Because of the sensitivity and specif
icity of this procedure and its ease of performance, it would be a rea
sonable alternative as a single assay for serological diagnosis of bru
cellosis.