A multicentre hospital outbreak in Sweden caused by introduction of a vanB2 transposon into a stably maintained pRUM-plasmid in an Enterococcus faecium ST192 clone.
Permanent lenke
https://hdl.handle.net/10037/6730Dato
2014Type
Journal articleTidsskriftartikkel
Peer reviewed
Forfatter
Sivertsen, Audun; Billström, Hanna; Melefors, Öjar; Liljequist, Barbro Olsson; Wisell, Karin Tegmark; Ullberg, Måns; Özenci, Volkan; Sundsfjord, Arnfinn; Hegstad, KristinSammendrag
The clonal dissemination of VanB-type vancomycin-resistant Enterococcus faecium (VREfm) strains in three Swedish hospitals
between 2007 and 2011 prompted further analysis to reveal the possible origin and molecular characteristics of the
outbreak strain. A representative subset of VREfm isolates (n = 18) and vancomycin-susceptible E. faecium (VSEfm, n = 2)
reflecting the spread in time and location was approached by an array of methods including: selective whole genome
sequencing (WGS; n = 3), multi locus sequence typing (MLST), antimicrobial susceptibility testing, virulence gene profiling,
identification of mobile genetic elements conferring glycopeptide resistance and their ability to support glycopeptide
resistance transfer. In addition, a single VREfm strain with an unrelated PFGE pattern collected prior to the outbreak was
examined by WGS. MLST revealed a predominance of ST192, belonging to a hospital adapted high-risk lineage harbouring
several known virulence determinants (n$10). The VREfm outbreak strain was resistant to ampicillin, gentamicin,
ciprofloxacin and vancomycin, and susceptible to teicoplanin. Consistently, a vanB2-subtype as part of Tn1549/Tn5382 with
a unique genetic signature was identified in the VREfm outbreak strains. Moreover, Southern blot hybridisation analyses of
PFGE separated S1 nuclease-restricted total DNAs and filter mating experiments showed that vanB2-Tn1549/Tn5382 was
located in a 70-kb sized rep17/pRUM plasmid readily transferable between E. faecium. This plasmid contained an axe-txe toxinantitoxin
module associated with stable maintenance. The two clonally related VSEfm harboured a 40 kb rep17/pRUM plasmid
absent of the 30 kb vanB2-Tn1549/Tn5382 gene complex. Otherwise, these two isolates were similar to the VREfm outbreak
strain in virulence- and resistance profile. In conclusion, our observations support that the origin of the multicentre outbreak
was caused by an introduction of vanB2-Tn1549/Tn5382 into a rep17/pRUM plasmid harboured in a pre-existing high-risk E.
faecium ST192 clone. The subsequent dissemination of VREfm to other centres was primarily caused by clonal spread rather
than plasmid transfer to pre-existing high-risk clones.
Forlag
Public Library of Science (PLoS)Sitering
PLoS ONE (2014), vol. 9(8): e103274.Metadata
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