Oral Keratinocyte Responses to Nickel-based Dental Casting Alloys In Vitro

Abstract

Adverse reactions of oral mucosa to nickel-based dental casting alloys are probably due to corrosion metal ion release. We exposed H400 oral keratinocytes to two Ni-based dental alloys (Matchmate and Dsign10) as well as NiCl₂ (1—40 μg/mL Ni²⁺). Alloy derived Ni²⁺ media concentrations were determined. Direct culture on both alloys resulted in inhibited growth with a greater effect observed for Dsign10 (higher ion release). Indirect exposure of cells to conditioned media from Dsign10 negatively affected cell numbers (~64% of control by 6 days) and morphology while Matchmate-derived media did not. Exposure to increasing NiCl₂ negatively affected cell growth and morphology, and the Granulocyte-macrophage colony-stimulating factor (GM-CSF) transcript was significantly up-regulated in cells following direct and indirect exposure to Dsign10. NiCl₂ exposure up-regulated all cytokine transcripts at 1 day. At day 6, IL-1β and IL-8 transcripts were suppressed while GM-CSF and IL-11 increased with Ni²⁺ dose. Accumulation of Ni²⁺ ions from alloys in oral tissues may affect keratinocyte viability and chronic inflammation.

Keywords

cell viability dental alloy gene expression inflammation metal ion release metal ion toxicity.

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