In Vivo Transfer and Microevolution of Avian Native IncA/C2blaNDM-1-Carrying Plasmid pRH-1238 during a Broiler Chicken Infection Study

Sead Hadziabdic; Jennie Fischer; Burkhard Malorny; Maria Borowiak; Beatriz Guerra; Annemarie Kaesbohrer; Bruno Gonzalez-Zorn; Istvan Szabo

doi:10.1128/AAC.02128-17

In Vivo Transfer and Microevolution of Avian Native IncA/C₂bla_NDM-1-Carrying Plasmid pRH-1238 during a Broiler Chicken Infection Study

Antimicrob Agents Chemother. 2018 Mar 27;62(4):e02128-17. doi: 10.1128/AAC.02128-17. Print 2018 Apr.

Authors

Sead Hadziabdic¹, Jennie Fischer¹, Burkhard Malorny¹, Maria Borowiak¹, Beatriz Guerra¹, Annemarie Kaesbohrer¹, Bruno Gonzalez-Zorn², Istvan Szabo³

Affiliations

¹ German Federal Institute for Risk Assessment (BfR), Department for Biological Safety, Berlin, Germany.
² Departamento de Sanidad Animal and Centro de Vigilancia Sanitaria Veterinaria, Facultad de Veterinaria, Universidad Complutense de Madrid, Madrid, Spain.
³ German Federal Institute for Risk Assessment (BfR), Department for Biological Safety, Berlin, Germany istvan.szabo@bfr.bund.de.

Abstract

The emergence and spread of carbapenemase-producing Enterobacteriaceae (CPE) in wildlife and livestock animals pose an important safety concern for public health. With our in vivo broiler chicken infection study, we investigated the transfer and experimental microevolution of the bla_NDM-1-carrying IncA/C₂ plasmid (pRH-1238) introduced by avian native Salmonella enterica subsp. enterica serovar Corvallis without inducing antibiotic selection pressure. We evaluated the dependency of the time point of inoculation on donor (S Corvallis [12-SA01738]) and plasmid-free Salmonella recipient [d-tartrate-fermenting (d-Ta⁺) S Paratyphi B (13-SA01617), referred to here as S Paratyphi B (d-Ta⁺)] excretion by quantifying their excretion dynamics. Using plasmid profiling by S1 nuclease-restricted pulsed-field gel electrophoresis, we gained insight into the variability of the native plasmid content among S Corvallis reisolates as well as plasmid acquisition in S Paratyphi B (d-Ta⁺) and the enterobacterial gut microflora. Whole-genome sequencing enabled us to gain an in-depth insight into the microevolution of plasmid pRH-1238 in S Corvallis and enterobacterial recipient isolates. Our study revealed that the fecal excretion of avian native carbapenemase-producing S Corvallis is significantly higher than that of S Paratyphi (d-Ta⁺) and is not hampered by S Paratyphi (d-Ta⁺). Acquisition of pRH-1238 in other Enterobacteriaceae and several events of plasmid pRH-1238 transfer to different Escherichia coli sequence types and Klebsiella pneumoniae demonstrated an interspecies broad host range. Regardless of the microevolutionary structural deletions in pRH-1238, the single carbapenem resistance marker bla_NDM-1 was maintained on pRH-1238 throughout the trial. Furthermore, we showed the importance of the gut E. coli population as a vector of pRH-1238. In a potential scenario of the introduction of NDM-1-producing S Corvallis into a broiler flock, the pRH-1238 plasmid could persist and spread to a broad host range even in the absence of antibiotic pressure.

Keywords: Enterobacteriaceae; NDM-1 carbapenemase; Salmonella; antimicrobial resistance; broiler chickens; in vivo transfer; microevolution.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Anti-Bacterial Agents / pharmacology
Bacterial Proteins / genetics
Chickens
Electrophoresis, Gel, Pulsed-Field
Enterobacteriaceae / drug effects
Enterobacteriaceae / genetics*
Klebsiella pneumoniae / drug effects
Klebsiella pneumoniae / genetics
Salmonella enterica / drug effects
Salmonella enterica / genetics*
beta-Lactamases / genetics

Substances

Anti-Bacterial Agents
Bacterial Proteins
beta-Lactamases
beta-lactamase NDM-1
carbapenemase