Intracellular Transposition of Mobile Genetic Elements Associated with the Colistin Resistance Gene mcr-1

Richard N Goodman; Supathep Tansirichaiya; Michael S M Brouwer; Adam P Roberts

doi:10.1128/spectrum.03278-22

Intracellular Transposition of Mobile Genetic Elements Associated with the Colistin Resistance Gene mcr-1

Microbiol Spectr. 2023 Feb 14;11(1):e0327822. doi: 10.1128/spectrum.03278-22. Epub 2022 Dec 13.

Authors

Richard N Goodman¹, Supathep Tansirichaiya², Michael S M Brouwer³, Adam P Roberts¹

Affiliations

¹ Department of Tropical Disease Biology, Liverpool School of Tropical Medicine, Liverpool, United Kingdom.
² Department of Microbiology, Faculty of Medicine Siriraj Hospital, Mahidol University, Bangkok, Thailand.
³ Wageningen Bioveterinary Research, Lelystad, The Netherlands.

Abstract

Mobile colistin resistance (mcr) genes are often located on conjugative plasmids, where their association with insertion sequences enables intercellular and intracellular dissemination throughout bacterial replicons and populations. Multiple mcr genes have been discovered in every habitable continent, in many bacterial species, on both plasmids and integrated into the chromosome. Previously, we showed the intercellular transfer of mcr-1 on an IncI1 plasmid, pMCR-E2899, between strains of Escherichia coli. Characterizing the intracellular dynamics of mcr-1 transposition and recombination would further our understanding of how these important genes move through bacterial populations and whether interventions can be put in place to stop their spread. In this study, we aimed to characterize transfer events from the mcr-1-containing transposon Tn7511 (ISApl1-mcr-1-pap2-ISApl1), located on plasmid pMCR-E2899, using the pBACpAK entrapment vector. Following the transformation of pBACpAK into our DH5α-Azi^r/pMCR-E2899 transconjugant, we captured ISApl1 in pBACpAK multiple times and, for the first time, observed the ISApl1-mediated transfer of the mcr-1 transposon (Tn7511) into the chromosome of E. coli DH5α. Whole-genome sequencing allowed us to determine consensus insertion sites of ISApl1 and Tn7511 in this strain, and comparison of these sites allowed us to explain the transposition events observed. These observations reveal the consequences of ISApl1 transposition within and between multiple replicons of the same cell and show mcr-1 transposition within the cell as part of the novel transposon Tn7511. IMPORTANCE By analyzing the intracellular transfer of clinically relevant transposons, we can understand the dissemination and evolution of drug resistance conferring mobile genetic elements (MGEs) once a plasmid enters a cell following conjugation. This knowledge will help further our understanding of how these important genes move through bacterial populations. Utilizing the pBACpAK entrapment vector has allowed us to determine the mobility of the novel mcr-1-containing transposon Tn7511.

Keywords: ISApl1; Tn7511; antimicrobial resistance; entrapment vector; insertion sequence; plasmid; target site.

Publication types

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

MeSH terms

Anti-Bacterial Agents / pharmacology
Bacteria / genetics
Colistin* / pharmacology
DNA Transposable Elements
Drug Resistance, Bacterial / genetics
Escherichia coli / genetics
Escherichia coli Proteins* / genetics
Microbial Sensitivity Tests
Plasmids / genetics

Substances

Colistin
Anti-Bacterial Agents
DNA Transposable Elements
Escherichia coli Proteins
MCR-1 protein, E coli

Abstract

Publication types

MeSH terms

Substances

Grants and funding