Coagulase-negative staphylococcal bloodstream and prosthetic-device-associated infections: the role of biofilm formation and distribution of adhesin and toxin genes

Nikolaos Giormezis, Fevronia Kolonitsiou, Antigoni Foka, Eleanna Drougka, Apostolos Liakopoulos, Antonia Makri, Anastasios D. Papanastasiou, Aliki Vogiatzi, Gabriel Dimitriou, Markos Marangos, Myrto Christofidou, Evangelos D. Anastassiou, Efthimia Petinaki, Iris Spiliopoulou

¹Department of Microbiology, School of Medicine, University of Patras, Greece

²National Reference Laboratory for Staphylococci, Patras, Greece

³Department of Microbiology, School of Medicine, University of Thessaly, Larissa, Greece

⁴Laboratory of Microbiology, General Children Hospital Pentelis, Athens, Greece

⁵Department of Biology, School of Medicine, University of Patras, Greece

⁶Neonatal Intensive Care Unit, Department of Paediatrics, School of Medicine, University of Patras, Greece

⁷Division of Infectious Diseases, Department of Internal Medicine, School of Medicine, University of Patras, Greece

Correspondence
Iris Spiliopoulou spiliopl{at}upatras.gr

Journal of Medical Microbiology 2014; 63(Pt 11):1500–1508 · https://doi.org/10.1099/jmm.0.075259-0

Abstract

Coagulase-negative staphylococci (CNS), especially Staphylococcus epidermidis and Staphylococcus haemolyticus, have emerged as opportunistic pathogens in immunocompromised patients and those with indwelling medical devices. In this study, CNS recovered from patients with bloodstream infections (BSIs) or prosthetic-device-associated infections (PDAIs) were compared in terms of biofilm formation, antimicrobial resistance, clonal distribution, and carriage of adhesin and toxin genes. A total of 226 CNS isolates (168 S. epidermidis and 58 S. haemolyticus) recovered from hospital inpatients with BSIs (100 isolates) or PDAIs (126 isolates) were tested for biofilm formation, antimicrobial susceptibility, and mecA, ica operon, adhesin (aap, bap, fnbA, atlE, fbe) and toxin (tst, sea, sec) genes. The selected CNS were classified into pulsotypes by PFGE and assigned to sequence types by multilocus sequence typing. In total, 106/226 isolates (46.9 %) produced biofilm, whereas 150 (66.4 %) carried the ica operon. Most isolates carried mecA and were multidrug resistant (90.7 %). CNS recovered from BSIs were significantly more likely to produce biofilm (P = 0.003), be resistant to antimicrobials and carry mecA (P<0.001), as compared with isolates derived from PDAIs. CNS from PDAIs were more likely to carry the aap and bap genes (P = 0.006 and P = 0.045, respectively). No significant differences in the carriage of toxin genes were identified (P>0.05). Although PFGE revealed genetic diversity, especially among S. epidermidis, analysis of representative strains from the main PFGE types by multilocus sequence typing revealed three major clones (ST2, ST5 and ST16). A clonal relationship was found with respect to antimicrobial susceptibility and ica and aap gene carriage, reinforcing the premise of clonal expansion in hospital settings. The results of this study suggest that the pathogenesis of BSIs is associated with biofilm formation and high-level antimicrobial resistance, whereas PDAIs are related to the adhesion capabilities of S. epidermidis and S. haemolyticus strains.