Anti-Salmonella lipopolysaccharide monoclonal antibodies: characterization of Salmonella BO-, CO-, DO-, and EO-specific clones and their diagnostic usefulness.

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J Clin Microbiol. 1991 November; 29(11): 2424-2433

Anti-Salmonella lipopolysaccharide monoclonal antibodies: characterization of Salmonella BO-, CO-, DO-, and EO-specific clones and their diagnostic usefulness.

J M Luk and A A Lindberg

Department of Clinical Bacteriology, Karolinska Institute, Huddinge Hospital, Stockholm, Sweden.

ABSTRACT

To facilitate the identification and serotyping of Salmonellaspecies, we established a wide variety of murine monoclonalantibodies (MAbs) that were reactive with the lipopolysaccharides(LPSs) of Salmonella serogroups B to E. An effective approachfor generating LPS-reactive hybridomas was used; this requiredimmunization of mice with LPS-coated bacteria. To screen fordiagnostically useful MAbs, the MAbs were tested by enzyme-linkedimmunosorbent assay against a set of purified LPSs from smoothand rough Salmonella strains. At least four major groups ofantibody specificities were identified: Salmonella (i) BO specific,(ii) CO specific, (iii) DO specific, and (iv) EO specific. Fora more detailed epitope analysis, a panel of eight differentserogroup-specific MAbs which were shown to bind the O-antigenicpolysaccharide chains, yielding characteristic ladder patternsin Western blots (immunoblots) against the LPS of Salmonellaserogroups B to E, were selected. The availability of variouschemically defined LPS structures and Salmonella O-antigen glycoconjugatespermitted the definition of O-antigenic polysaccharide epitopesrecognized by each MAb that serologically corresponded to factorsO3, O4, O5, O6, O7, O8, O9, and O10 on the basis of the Kauffmann-Whitescheme for Salmonella classification. The diagnostic accuracyof these immunochemically defined O-specific MAbs for Salmonellaserotyping was demonstrated by correct identification of all167 salmonellae (including 72 serotypes from serogroups B toE) among the 294 bacterial strains in a slide agglutinationtest. No false-positive reactions were detected.

J Clin Microbiol. 1991 November; 29(11): 2424-2433

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