Intraspecies Biodiversity of the Genetically Homologous Species Brucella microti

Author:

Al Dahouk Sascha12,Hofer Erwin3,Tomaso Herbert4,Vergnaud Gilles567,Le Flèche Philippe568,Cloeckaert Axel9,Koylass Mark S.10,Whatmore Adrian M.10,Nöckler Karsten1,Scholz Holger C.11

Affiliation:

1. Federal Institute for Risk Assessment, Berlin, Germany

2. RWTH Aachen University, Department of Internal Medicine III, Aachen, Germany

3. Austrian Agency for Health and Food Safety, Mödling, Austria

4. Friedrich Loeffler Institute, Institute of Bacterial Infections and Zoonoses, Jena, Germany

5. Université Paris Sud, Institut de Génétique et Microbiologie, UMR 8621, Orsay, France

6. Centre National de la Recherche Scientifique (CNRS), Orsay, France

7. Mission pour la Recherche et l'Innovation Scientifique (DGA/MRIS), Bagneux, France

8. Centre d'Etudes du Bouchet, Division of Analytical Microbiology, Vert le Petit, France

9. Institut National de la Recherche Agronomique (INRA), UR1282, Infectiologie Animale et Santé Publique (IASP), Nouzilly, France

10. Animal Health and Veterinary Laboratories Agency (AHVLA), Department of Bacteriology, New Haw, United Kingdom

11. Bundeswehr Institute of Microbiology, Department of Bacteriology, Munich, Germany

Abstract

ABSTRACT Brucellosis is one of the major bacterial zoonoses worldwide. In the past decade, an increasing number of atypical Brucella strains and species have been described. Brucella microti in particular has attracted attention, because this species not only infects mammalian hosts but also persists in soil. An environmental reservoir may pose a new public health risk, leading to the reemergence of brucellosis. In a polyphasic approach, comprising conventional microbiological techniques and extensive biochemical and molecular techniques, all currently available Brucella microti strains were characterized. While differing in their natural habitats and host preferences, B. microti isolates were found to possess identical 16S rRNA, recA , omp2a , and omp2b gene sequences and identical multilocus sequence analysis (MLSA) profiles at 21 different genomic loci. Only highly variable microsatellite markers of multiple-locus variable-number tandem repeat (VNTR) analysis comprising 16 loci (MLVA-16) showed intraspecies discriminatory power. In contrast, biotyping demonstrated striking differences within the genetically homologous species. The majority of the mammalian isolates agglutinated only with monospecific anti-M serum, whereas soil isolates agglutinated with anti-A, anti-M, and anti-R sera. Bacteria isolated from animal sources were lysed by phages F1, F25, Tb, BK2, Iz, and Wb, whereas soil isolates usually were not. Rough strains of environmental origin were lysed only by phage R/C. B. microti exhibited high metabolic activities similar to those of closely related soil organisms, such as Ochrobactrum spp. Each strain was tested with 93 different substrates and showed an individual metabolic profile. In summary, the adaptation of Brucella microti to a specific habitat or host seems to be a matter of gene regulation rather than a matter of gene configuration.

Publisher

American Society for Microbiology

Subject

Ecology,Applied Microbiology and Biotechnology,Food Science,Biotechnology

Reference38 articles.

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