Effect of ProRoot ® MTA mixed with chlorhexidine on apoptosis and cell cycle of fibroblasts and macrophages in vitro *

Aim  To compare the percentage of apoptotic cells and the cell cycle profile of fibroblasts and macrophages exposed to either ProRoot ® mineral trioxide aggregate (MTA) mixed with chlorhexidine (CHX), or exposed to ProRoot ® MTA mixed with sterile water. Methodology  Mouse gingival fibroblasts or mouse macrophages were seeded in six‐well plates and allowed to attach overnight. Freshly mixed or set (allowed to dry for 24 h) specimens of tooth‐coloured (white) ProRoot ® MTA were prepared with 0.12% CHX gluconate (MTA/CHX) or with sterile water (MTA/H 2 O). The cells were exposed for 24 h to the MTA specimens, which were placed over permeable membrane inserts to avoid direct contact with the cells. Untreated cells served as controls. Propidium iodide staining followed by flow cytometry was used to evaluate the effects of ProRoot ® MTA on cell apoptosis and cell cycle. Statistical analyses were performed by one‐way anova followed by post‐hoc tests with the use of the SigmaStat 2.0 software, and significance was determined at P  ≤ 0.05. Results  MTA specimens containing CHX induced apoptosis of macrophages and fibroblasts ( P  < 0.05). In contrast, no change in the proportion of apoptotic cells was observed when sterile water was used to prepare the specimens ( P  > 0.05). Cell cycle analysis showed that exposure to MTA/CHX decreased the percentage of fibroblasts and macrophages in S phase (DNA synthesis) as compared with exposure to MTA/H 2 O ( P  < 0.05). Conclusion  This in vitro study demonstrated that the substitution of CHX for sterile water in MTA increases its cytotoxicity. This suggests that the potentially beneficial antimicrobial effect of CHX may be accompanied by an increase in the cytotoxicity of the resulting MTA‐based material.