Mobile insertion cassette elements found in small non-transmissible plasmids in Proteeae may explain qnrD mobilization.

qnrD is a plasmid mediated quinolone resistance gene from unknown origin, recently described in Enterobacteriaceae. It encodes a pentapeptide repeat protein 36-60% different from the other Qnr (A, B, C, S and VC). Since most qnrD-positive strains were described as strains belonging to Proteus or Pro...

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Main Authors: Thomas Guillard, Antoine Grillon, Christophe de Champs, Céline Cartier, Janick Madoux, Béatrice Berçot, Anne-Laure Lebreil, Alain Lozniewski, Jacques Riahi, Véronique Vernet-Garnier, Emmanuelle Cambau
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2014-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC3913671?pdf=render
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spelling doaj-812b5efcdb7e4053aae38250f644f1312020-11-25T01:52:45ZengPublic Library of Science (PLoS)PLoS ONE1932-62032014-01-0192e8780110.1371/journal.pone.0087801Mobile insertion cassette elements found in small non-transmissible plasmids in Proteeae may explain qnrD mobilization.Thomas GuillardAntoine GrillonChristophe de ChampsCéline CartierJanick MadouxBéatrice BerçotAnne-Laure LebreilAlain LozniewskiJacques RiahiVéronique Vernet-GarnierEmmanuelle CambauqnrD is a plasmid mediated quinolone resistance gene from unknown origin, recently described in Enterobacteriaceae. It encodes a pentapeptide repeat protein 36-60% different from the other Qnr (A, B, C, S and VC). Since most qnrD-positive strains were described as strains belonging to Proteus or Providencia genera, we hypothesized that qnrD originated in Proteeae before disseminating to other enterobacterial species. We screened 317 strains of Proteeae for qnrD and its genetic support by PCR. For all the seven qnrD-positive strains (4 Proteus mirabilis, 1 Proteus vulgaris and 2 Providencia rettgeri) the gene was carried onto a small non-transmissible plasmid, contrarily to other qnr genes that are usually carried onto large multi-resistant plasmids. Nucleotide sequences of the qnrD-bearing plasmids were 96% identical. Plasmids contained 3 ORFs apart from qnrD and belonged to an undescribed incompatibility group. Only one plasmid, in P. vulgaris, was slightly different with a 1,568-bp insertion between qnrD and its promoter, leading to absence of quinolone resistance. We sought for similar plasmids in 15 reference strains of Proteeae, but which were tested negative for qnrD, and found a 48% identical plasmid (pVERM) in Providencia vermicola. In order to explain how qnrD could have been inserted into such native plasmid, we sought for gene mobilization structures. qnrD was found to be located within a mobile insertion cassette (mic) element which sequences are similar to one mic also found in pVERM. Our conclusions are that (i) the small non-transmissible qnrD-plasmids described here may result from the recombination between an as-yet-unknown progenitor of qnrD and pVERM, (ii) these plasmids are maintained in Proteeae being a qnrD reservoir (iii) the mic element may explain qnrD mobilization from non-transmissible plasmids to mobilizable or conjugative plasmids from other Enterobacteriaceae, (iv) they can recombined with larger multiresistant plasmids conjugated in Proteeae.http://europepmc.org/articles/PMC3913671?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Thomas Guillard
Antoine Grillon
Christophe de Champs
Céline Cartier
Janick Madoux
Béatrice Berçot
Anne-Laure Lebreil
Alain Lozniewski
Jacques Riahi
Véronique Vernet-Garnier
Emmanuelle Cambau
spellingShingle Thomas Guillard
Antoine Grillon
Christophe de Champs
Céline Cartier
Janick Madoux
Béatrice Berçot
Anne-Laure Lebreil
Alain Lozniewski
Jacques Riahi
Véronique Vernet-Garnier
Emmanuelle Cambau
Mobile insertion cassette elements found in small non-transmissible plasmids in Proteeae may explain qnrD mobilization.
PLoS ONE
author_facet Thomas Guillard
Antoine Grillon
Christophe de Champs
Céline Cartier
Janick Madoux
Béatrice Berçot
Anne-Laure Lebreil
Alain Lozniewski
Jacques Riahi
Véronique Vernet-Garnier
Emmanuelle Cambau
author_sort Thomas Guillard
title Mobile insertion cassette elements found in small non-transmissible plasmids in Proteeae may explain qnrD mobilization.
title_short Mobile insertion cassette elements found in small non-transmissible plasmids in Proteeae may explain qnrD mobilization.
title_full Mobile insertion cassette elements found in small non-transmissible plasmids in Proteeae may explain qnrD mobilization.
title_fullStr Mobile insertion cassette elements found in small non-transmissible plasmids in Proteeae may explain qnrD mobilization.
title_full_unstemmed Mobile insertion cassette elements found in small non-transmissible plasmids in Proteeae may explain qnrD mobilization.
title_sort mobile insertion cassette elements found in small non-transmissible plasmids in proteeae may explain qnrd mobilization.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2014-01-01
description qnrD is a plasmid mediated quinolone resistance gene from unknown origin, recently described in Enterobacteriaceae. It encodes a pentapeptide repeat protein 36-60% different from the other Qnr (A, B, C, S and VC). Since most qnrD-positive strains were described as strains belonging to Proteus or Providencia genera, we hypothesized that qnrD originated in Proteeae before disseminating to other enterobacterial species. We screened 317 strains of Proteeae for qnrD and its genetic support by PCR. For all the seven qnrD-positive strains (4 Proteus mirabilis, 1 Proteus vulgaris and 2 Providencia rettgeri) the gene was carried onto a small non-transmissible plasmid, contrarily to other qnr genes that are usually carried onto large multi-resistant plasmids. Nucleotide sequences of the qnrD-bearing plasmids were 96% identical. Plasmids contained 3 ORFs apart from qnrD and belonged to an undescribed incompatibility group. Only one plasmid, in P. vulgaris, was slightly different with a 1,568-bp insertion between qnrD and its promoter, leading to absence of quinolone resistance. We sought for similar plasmids in 15 reference strains of Proteeae, but which were tested negative for qnrD, and found a 48% identical plasmid (pVERM) in Providencia vermicola. In order to explain how qnrD could have been inserted into such native plasmid, we sought for gene mobilization structures. qnrD was found to be located within a mobile insertion cassette (mic) element which sequences are similar to one mic also found in pVERM. Our conclusions are that (i) the small non-transmissible qnrD-plasmids described here may result from the recombination between an as-yet-unknown progenitor of qnrD and pVERM, (ii) these plasmids are maintained in Proteeae being a qnrD reservoir (iii) the mic element may explain qnrD mobilization from non-transmissible plasmids to mobilizable or conjugative plasmids from other Enterobacteriaceae, (iv) they can recombined with larger multiresistant plasmids conjugated in Proteeae.
url http://europepmc.org/articles/PMC3913671?pdf=render
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