PCR-based ORF typing of Klebsiella pneumoniae for rapid identification of global clones and transmission events

Author:

Nonogaki Rina1,Iijima Anna1,Kawamura Kumiko1,Kayama Shizuo23,Sugai Motoyuki23,Yagi Tetsuya4,Arakawa Yoshichika56,Doi Yohei789,Suzuki Masahiro7ORCID

Affiliation:

1. Department of Integrated Health Sciences Nagoya University Graduate School of Medicine Aichi Japan

2. Antimicrobial Resistance Research Center National Institute of Infectious Diseases Tokyo Japan

3. Department of Antimicrobial Resistance Hiroshima University Graduate School of Biomedical and Health Sciences Hiroshima Japan

4. Department of Infectious Diseases Nagoya University Graduate School of Medicine Japan

5. Department of Bacteriology Nagoya University Graduate School of Medicine Aichi Japan

6. Laboratory of Microbiology, Department of Medical Technology, Faculty of Medical Sciences Shubun University Ichinomiya Aichi Japan

7. Department of Microbiology Fujita Health University School of Medicine Aichi Japan

8. Department of Infectious Diseases Fujita Health University School of Medicine Aichi Japan

9. Division of Infectious Diseases University of Pittsburgh School of Medicine Pittsburgh Pennsylvania USA

Abstract

Abstract Aims Klebsiella pneumoniae is a major cause of healthcare-associated infections. In this study, we aimed to develop a rapid and simple genotyping method that can characterize strains causing nosocomial infections. Methods and results The PCR-based open reading frame (ORF) typing (POT) method consists of two multiplex PCR reactions that were designed to detect 25 ORFs specific to bacterial genetic lineages, species, antimicrobial-resistant genes (blaCTX-M group-1, blaCTX-M group-9, blaIMP and blaKPC), a capsular K1-specific gene and a virulence factor gene (rmpA/A2). The electrophoresis results are then digitized. A total of 192 strains (136 clinical and 8 reference strains of K. pneumoniae, 33 clinical and 1 reference strains of K. variicola and 14 clinical strains of K. quasipneumoniae) were classified into 95, 26 and 11 POT values, respectively. The distribution patterns of ORFs among K. pneumoniae correlated well with multilocus sequence typing (MLST). Furthermore, closely related species could be distinguished and key antimicrobial resistance and hypervirulence genes were identified as part of POT. Conclusions The POT method was developed and validated for K. pneumoniae. In comparison to MLST, the POT method is a rapid and easy genotyping method for monitoring transmission events by K. pneumoniae in clinical microbiology laboratories. Significance and Impact of the Study The POT method supplies clear and informative molecular typing results for K. pneumoniae. The method would facilitate molecular epidemiological analysis in infection control and hospital epidemiology investigations.

Funder

Japan Agency for Medical Research and Development

Publisher

Oxford University Press (OUP)

Subject

Applied Microbiology and Biotechnology,General Medicine,Biotechnology

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