a Area de Bioquímica y Biología Molecular, Universidad de La Rioja, Logroño; b Servicio de Microbiología, Hospital Ramón y Cajal, Ctra Colmenar Viejo Km 9.1, 28034 Madrid; c Departamento de Microbiología, Universidad Zaragoza, Zaragoza, Spain
Sir,
Vancomycin-resistant enterococci constitute an increasing clinical problem in the USA, and clonal dissemination of vancomycin-resistant isolates among hospitals, especially Enterococcus faecium, has been described.1 In Europe, detection of vanA enterococci in the clinical setting is less frequently reported and few reports exist of clonal dissemination of resistant isolates among different hospitals.2 This study examines eight vanA-containing Enterococcus faecalis clinical isolates (blood and exudates) from hospitals in four different Spanish regions: Aragón (AR721), Asturias (AS215 and AS237), Cataluña (CT715, CT716, CT718 and CT719) and La Rioja (LR337). Antibiotic resistance phenotype was determined by the agar dilution method of the NCCLS.3 The putative presence of vanR, vanS, vanH, vanA, vanY, vanX, vanZ, aac(6')-aph(2"),aph(3'), and erm(B) genes was examined by PCR, using specific primers. Aminoglycoside-modifying enzymes were determined in extracts of resistant Enterococcus isolates obtained by ultrasonic disruption, using the phosphocellulose paper binding assay as described previously.4 Clonal identity was studied by analysing the genomic DNA of vanA isolates digested with SmaI by pulsed-field gel electrophoresis (PFGE) as described previously.5 Isolates were classified as indistinguishable, closely related, possible related or unrelated according to published criteria.6
All eight vanA E. faecalis isolates were resistant to vancomycin and teicoplanin (MIC ranges 256512 mg/L and 64256 mg/L, respectively) as well as to erythromycin (MIC > 128 mg/L), but were susceptible to ampicillin (MIC < 4 mg/L). Seven isolates showed high-level resistance (HLR) to kanamycin (>2000 mg/L) and streptomycin (>1000 mg/L); one (AS237) also showed HLR to gentamicin (>1000 mg/L) and one (CT718) showed HLR only to streptomycin. In E. faecalis strains that showed HLR to kanamycin APH (3') activity was detected by the radioenzymic assay and the presence of the aph3'-III gene was confirmed by PCR amplification. No streptomycin-modifying enzyme was detected in high-level streptomycin-resistant isolates. APH(2")-AAC(6') activity was detected in the E. faecalis strain that showed HLR to gentamicin, and the presence of the aac6-aph2 gene was confirmed by PCR. Positive PCR amplifications were obtained in all eight isolates for all genes of the vanA operon (vanR, vanS, vanH, vanA, vanX, vanY and vanZ) and also for the erm(B) gene.
All E. faecalis isolates carried a high molecular weight plasmid (c. 60 kb) that was transferred to the recipient E. faecalis JH2-2 strain by filter mating. Both donors and transconjugants also showed a positive hybridization pattern with a vanA probe in the chromosome. The same hybridization pattern was obtained when genomic DNA was digested with EcoRI, transferred to a nylon membrane and hybridized with the vanA probe.
Five unrelated patterns were found by SmaIPFGE among the eight E. faecalis isolates. Four vanA-carrying E. faecalis isolates from three geographically distant hospitals showed an indistinguishable PFGE pattern (E. faecalis CT716, CT719, LR337 and AS215) (Figure). These four isolates were also further characterized as bacteriocin producers with a broad spectrum of activity,7 similar in all four strains. The other four E. faecalis isolates (CT715, CT718, AR721 and AS237) showed unrelated PFGE patterns; from these, one strain was a non-bacteriocin producer, and the other three produced possibly different antibacterial substances.
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Acknowledgements
We are grateful to M. Lantero, J. Castillo, C. Rubio, F. Marco and A. Fleites for submitting the E. faecalis vanA isolates. R.d.C. was supported by a grant from the Diputación General de Aragón (project P94/97). This work has been supported in part by a grant from the Fondo de Investigaciones Sanitarias (00/0545), Spain.
Notes
* Corresponding author. Tel: +34-91-336-8330; Fax: +34-91-336-8809; E-mail: rcampo{at}hrc.insalud.es
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