Biocompatibility profile of aged pigmented and non‐pigmented silicone elastomer for combined maxillofacial defects

Abstract

AbstractPurposeTo assess the biocompatibility of platinum silicone elastomer A‐2000 used in combined maxillofacial defects prosthesis, after being deteriorated by an accelerated aging process resembling both the extra and intraoral environment. This assessment was done indirectly on human‐derived dermal and gingival tissues.Materials and MethodsOne hundred eight samples of room‐temperature vulcanized A‐2000 platinum silicone were equally divided into extrinsically pigmented and non‐pigmented groups to replicate combined maxillofacial defects. Accelerated aging was applied to pigmented samples to mimic extra‐ and intra‐oral conditions, while non‐aged counterparts served as controls. After isolating human cell lineages, dermal and gingival fibroblasts were indirectly exposed to silicone sample media. Cytotoxicity to cultured fibroblasts was assessed via MTT assay. Statistical significance was determined by repeated measures of one‐way ANOVA (p < 0.01), evaluating cytotoxicity on dermal and gingival fibroblasts.ResultsMTT assay showed increased cytotoxicity in pigmented silicon samples subjected to extraoral aging compared to non‐aged counterparts (p < 0.01). Non‐pigmented silicon, modeling intraoral conditions, exhibited cytotoxicity after 48 h (p < 0.05). Both aged and non‐aged silicon extracts equally sensitized gingival fibroblasts at 72 h (p < 0.001). Negative correlations between pigmented and non‐pigmented silicon were observed in dermal cell growth (p > 0.05, except at 24 h, r = 0.2), with accelerated aging showing minimal impact on the pigmentation effect (p > 0.05).ConclusionThe retrieved diminished cellular metabolic activity of platinum silicone elastomer was in an acceptable clinical range, pointing out the importance of periodic assessments of the maxillofacial prosthesis for replacement depending on aging and cytotoxic harmful cellular responses.