Minor Nucleotide Substitutions in the omp31 Gene of Brucella ovis Result in Antigenic Differences in the Major Outer Membrane Protein That It Encodes Compared to Those of the Other Brucella Species

Author:

Vizcaı́no Nieves1,Kittelberger Reinhold2,Cloeckaert Axel3,Marı́n Clara M.4,Fernández-Lago Luis1

Affiliation:

1. Departamento de Microbiologı́a y Genética, Edificio Departmental, Universidad de Salamanca, 37007 Salamanca,1 and

2. National Centre for Disease Investigation, Ministry of Agriculture and Forestry, Upper Hutt, New Zealand,2; and

3. Station de Pathologie Aviaire et Parasitologie, Institut National de la Recherche Agronomique, Centre de Tours, 37380 Nouzilly, France3

4. Unidad de Sanidad Animal, Servicio de Investigación Agroalimentaria, Diputación General de Aragón, 50080 Zaragoza,4 Spain;

Abstract

ABSTRACT The gene coding for the major outer membrane protein Omp31 was sequenced in five Brucella species and their biovars. Although the omp31 genes appeared to be highly conserved in the genus Brucella , nine nucleotide substitutions were detected in the gene of Brucella ovis compared to that of Brucella melitensis . As shown by differential binding properties of monoclonal antibodies (MAbs) to the two Brucella species, these nucleotide substitutions result in different antigenic properties of Omp31. The antigenic differences were also evidenced when sera from B. ovis -infected rams were tested by Western blotting with the recombinant B. melitensis or B. ovis Omp31 proteins. Twelve available sera reacted with recombinant B. ovis Omp31, but only four of them reacted with recombinant B. melitensis Omp31. These results validate previous evidence for the potential of Omp31 as a diagnostic antigen for B. ovis infection in rams and demonstrate that B. ovis Omp31, instead of B. melitensis Omp31, should be used to evaluate this point. The antigenic differences between the B. melitensis and B. ovis Omp31 proteins should also be taken into account when Omp31 is evaluated as a candidate for the development of subcellular vaccines against B. ovis infection. No reactivity against recombinant B. melitensis Omp31 was detected, by Western blotting, with sera from B. melitensis -infected sheep. Accordingly, Omp31 does not seem to be a good diagnostic antigen for B. melitensis infections in sheep. Two immunodominant regions were identified on the B. ovis Omp31 protein by using recombinant DNA techniques and specific MAbs. Sera from B. ovis -infected rams that reacted with the recombinant protein were tested by Western blotting against one of these immunodominant regions shown to be exposed at the bacterial surface. Only 4 of the 12 sera reacted, but with strong intensity.

Publisher

American Society for Microbiology

Subject

Infectious Diseases,Immunology,Microbiology,Parasitology

Reference37 articles.

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3. Blasco J. M. Brucella ovis Animal brucellosis. Nielsen K. Duncan J. R. 1990 157 167 CRC Press Boca Raton Fla

4. Surface exposure of outer membrane protein and lipopolysaccharide epitopes in Brucella species studied by enzyme-linked immunosorbent assay and flow cytometry

5. Outer-membrane protein- and rough lipopolysaccharide-specific monoclonal antibodies protect mice against Brucella ovis;Bowden R. A.;J. Med. Microbiol.,1995

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