Development of PCR Assays for Species- and Type-Specific Identification of Pasteurella multocida Isolates

Author:

Townsend Kirsty M.1,Frost Alan J.1,Lee Chiang W.1,Papadimitriou John M.2,Dawkins Hugh J. S.3

Affiliation:

1. Division of Veterinary Pathobiology, University of Queensland, Brisbane 4072 Queensland,1 Australia

2. University of Western Australia Department of Pathology2 and

3. Urological Research Centre,3 Queen Elizabeth II Medical Centre, Nedlands 6009 Western Australia, and

Abstract

ABSTRACT Genomic subtractive hybridization of closely related Pasteurella multocida isolates has generated clones useful in distinguishing hemorrhagic septicemia-causing type B strains from other P. multocida serotypes. Oligonucleotide primers designed during the sequencing of these clones have proved valuable in the development of PCR assays for rapid species- and type-specific detection of P. multocida and of type B:2 in particular. This study demonstrated that the primer pair designed from the sequence of the clone 6b (KTT72 and KTSP61) specifically amplified a DNA fragment from types B:2, B:5, and B:2,5 P. multocida and that the primers KMT1T7 and KMT1SP6 produced an amplification product unique to all P. multocida isolates analyzed. It was also shown that PCR amplification performed directly on bacterial colonies or cultures represents an extremely rapid, sensitive method of P. multocida identification.

Publisher

American Society for Microbiology

Subject

Microbiology (medical)

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