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Two chromosomally located qnrB variants, qnrB6 and the new qnrB16, in Citrobacter spp. isolates causing bacteraemia  J. Sanchez-Cespedes, S. Marti, S.M.

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Presentation on theme: "Two chromosomally located qnrB variants, qnrB6 and the new qnrB16, in Citrobacter spp. isolates causing bacteraemia  J. Sanchez-Cespedes, S. Marti, S.M."— Presentation transcript:

1 Two chromosomally located qnrB variants, qnrB6 and the new qnrB16, in Citrobacter spp. isolates causing bacteraemia  J. Sanchez-Cespedes, S. Marti, S.M. Soto, V. Alba, C. Melción, M. Almela, F. Marco, J. Vila  Clinical Microbiology and Infection  Volume 15, Issue 12, Pages (December 2009) DOI: /j x Copyright © 2009 European Society of Clinical Infectious Diseases Terms and Conditions

2 FIG. 1 Pulsed-field gel electrophoresis of the three clinical Citrobacter freundii isolates. DNA was digested with XbaI. M, lambda marker; 1, C. freundii 72857; 2, C. freundii 62778; 3, C. freundii Clinical Microbiology and Infection  , DOI: ( /j x) Copyright © 2009 European Society of Clinical Infectious Diseases Terms and Conditions

3 FIG. 2 Plasmid identification in Klebsiella pneumoniae by genomic mapping with I-CeuI and digestion with SI nuclease. (a) Pulsed-field gel electrophoresis (PFGE). Lane M: lambda ladder PFGE marker. Lane 1: digestion with I-CeuI. Lane 2: digestion with SI nuclease. (b) Digestion with I-CeuI. Lane 1: hybridization with a 23S rRNA gene probe. Lane 2: hybridization with a qnrS probe. (c) Digestion with SI nuclease. Lane 1: hybridization with a 23S rRNA gene probe. Lane 2: hybridization with a qnrS probe. Arrows indicate plasmid location. Clinical Microbiology and Infection  , DOI: ( /j x) Copyright © 2009 European Society of Clinical Infectious Diseases Terms and Conditions

4 FIG. 3 Genomic localization of qnrB by genomic mapping with I-CeuI and digestion with S1 nuclease. (a) Pulsed-field gel electrophoresis (PFGE). A1, digestion with I-CeuI; A2, digestion with S1 nuclease. (b) Digestion with I-CeuI. B1, hybridization with a probe for the 23S rRNA gene; B2, hybridization with a qnrB probe. (c) Digestion with S1 nuclease. C1, hybridization with a 23S rRNA gene probe; C2, hybridization with a qnrB probe. Lane M: lambda ladder PFGE marker. Lane 1: Citrobacter freundii Lane 2: C. freundii Lane 3. C. freundii Lane 4: Citrobacter werkmanii The rectangle in A1 covers the fragments shown in Fig. 4 after changing the PFGE conditions. The arrow represents the slowest-moving band of the lambda ladder (727.5 kb). Clinical Microbiology and Infection  , DOI: ( /j x) Copyright © 2009 European Society of Clinical Infectious Diseases Terms and Conditions

5 FIG. 4 Localization of qnrB on I-CeuI-digested DNA following pulsed-field gel electrophoresis (PFGE) under the conditions described by Liu et al. [13] (a) PFGE. (b) Hybridization with a 23S rRNA gene probe. (c) Hybridization with a qnrB probe. Lane 1: Citrobacter freundii Lane 2: C. freundii Lane 3: C. freundii Lane 4: Citrobacter werkmanii The arrow indicates the position of the slowest-moving band of the lambda ladder (727.5 kb). Clinical Microbiology and Infection  , DOI: ( /j x) Copyright © 2009 European Society of Clinical Infectious Diseases Terms and Conditions

6 FIG. 5 Undigested DNA after pulsed-field gel electrophoresis (PFGE) under the conditions described by Liu et al. [13] (a) PFGE. (b) Hybridization with a qnrB probe. Lane 1: Citrobacter freundii Lane 2: Citrobacter werkmanii The arrow indicates undigested qnrB-containing DNA. Clinical Microbiology and Infection  , DOI: ( /j x) Copyright © 2009 European Society of Clinical Infectious Diseases Terms and Conditions

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