Co-Culture of S. epidermidis and Human Osteoblasts on Implant Surfaces: An Advanced In Vitro Model for Implant-Associated Infections

Sarah Zaatreh; Katharina Wegner; Madlen Strauß; Juliane Pasold; Wolfram Mittelmeier; Andreas Podbielski; Bernd Kreikemeyer; Rainer Bader

doi:10.1371/journal.pone.0151534

Co-Culture of S. epidermidis and Human Osteoblasts on Implant Surfaces: An Advanced In Vitro Model for Implant-Associated Infections

PLoS One. 2016 Mar 16;11(3):e0151534. doi: 10.1371/journal.pone.0151534. eCollection 2016.

Authors

Sarah Zaatreh¹, Katharina Wegner¹, Madlen Strauß¹, Juliane Pasold¹, Wolfram Mittelmeier¹, Andreas Podbielski², Bernd Kreikemeyer², Rainer Bader¹

Affiliations

¹ Biomechanics and Implant Technology Research Laboratory, Department of Orthopedics, University Medicine Rostock, Rostock, Mecklenburg-Western Pomerania, Germany.
² Institute of Medical Microbiology, Virology and Hygiene, University Medicine Rostock, Rostock, Mecklenburg-Western Pomerania, Germany.

Abstract

Objectives: Total joint arthroplasty is one of the most frequent and effective surgeries today. However, despite improved surgical techniques, a significant number of implant-associated infections still occur. Suitable in vitro models are needed to test potential approaches to prevent infection. In the present study, we aimed to establish an in vitro co-culture setup of human primary osteoblasts and S. epidermidis to model the onset of implant-associated infections, and to analyze antimicrobial implant surfaces and coatings.

Materials and methods: For initial surface adhesion, human primary osteoblasts (hOB) were grown for 24 hours on test sample discs made of polystyrene, titanium alloy Ti6Al4V, bone cement PALACOS R®, and PALACOS R® loaded with antibiotics. Co-cultures were performed as a single-species infection on the osteoblasts with S. epidermidis (multiplicity of infection of 0.04), and were incubated for 2 and 7 days under aerobic conditions. Planktonic S. epidermidis was quantified by centrifugation and determination of colony-forming units (CFU). The quantification of biofilm-bound S. epidermidis on the test samples was performed by sonication and CFU counting. Quantification of adherent and vital primary osteoblasts on the test samples was performed by trypan-blue staining and counting. Scanning electron microscopy was used for evaluation of topography and composition of the species on the sample surfaces.

Results: After 2 days, we observed approximately 104 CFU/ml biofilm-bound S. epidermidis (103 CFU/ml initial population) on the antibiotics-loaded bone cement samples in the presence of hOB, while no bacteria were detected without hOB. No biofilm-bound bacteria were detectable after 7 days in either case. Similar levels of planktonic bacteria were observed on day 2 with and without hOB. After 7 days, about 105 CFU/ml planktonic bacteria were present, but only in the absence of hOB. Further, no bacteria were observed within the biofilm, while the number of hOB was decreased to 10% of its initial value compared to 150% in the mono-culture of hOB.

Conclusion: We developed a co-culture setup that serves as a more comprehensive in vitro model for the onset of implant-associated infections and provides a test method for antimicrobial implant materials and coatings. We demonstrate that observations can be made that are unavailable from mono-culture experiments.

MeSH terms

Coculture Techniques
Humans
In Vitro Techniques
Models, Biological
Osteoblasts / cytology*
Prosthesis-Related Infections / prevention & control*
Staphylococcus epidermidis / physiology*
Surface Properties

Grants and funding

The authors have no support or funding to report.