Differentiation Among Rodentibacter Species Based on 16S–23S rRNA Internal Transcribed Spacer Analysis

Author:

Benga Laurentiu1,Benten Peter M2,Engelhardt Eva2,Köhrer Karl3,Hueber Barbara4,Nicklas Werner5,Christensen Henrik6,Sager Martin2

Affiliation:

1. Central Unit for Animal Research and Animal Welfare Affairs, University Hospital, Heinrich–Heine University, Duesseldorf, Germany;, Email: Laurentiu.Benga@med.uni-duesseldorf.de

2. Central Unit for Animal Research and Animal Welfare Affairs, University Hospital, Heinrich–Heine University, Duesseldorf, Germany

3. Biological and Medical Research Center (BMFZ), Heinrich–Heine University, Duesseldorf, Germany

4. GIMmbH, Michendorf OT, Wildenbruch, Germany

5. Retired, Microbiologic Diagnostics, German Cancer Research Centre, Heidelberg, Germany

6. Department of Veterinary and Animal Science, Faculty of Health and Medical Sciences, University of Copenhagen, Denmark

Abstract

The internal transcribed spacer (ITS) regions of Rodentibacter pneumotropicus, R. heylii, R. rarus, R. ratti, and R. heidelbergensis and of a Rodentibacter- related β-hemolytic Pasteurellaceae taxon isolated from laboratory rodents were studied for their feasibility to discriminate among these species. The 6 species analyzed showed species-specific ITS patterns that were shared by the type strains and clinical isolates and that allowed their identification. Nevertheless, differentiating between the ITS band patterns of R. pneumotropicus and R. ratti is visually challenging. In all species tested, sequence analysis of the ITS fragments revealed a larger ITSile+ala, which contained the genes for tRNAIle(GAU) and tRNA Ala(UGC), and a smaller ITSglu with the tRNAGlu(UUC) gene. The ITS sequences varied among the 6 species evaluated, displaying identity levels ranging from 62% to 86% for ITSile+ala and 68% to 90% for ITSglu. Overall, ITS amplification proved to be a reliable method to differentiate among these important Pasteurellaceae species of laboratory rodents. Moreover, the ITS sequence variations recorded here might facilitate the design of probes for specific identification of these species. The ability to diagnose these organisms to the species level could increase our understanding of their clinical significance.

Publisher

American Association for Laboratory Animal Science

Subject

General Veterinary,General Biochemistry, Genetics and Molecular Biology

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