Since ancient Eygypt, various dental materials were used for lost teeth including gold. The key point of this materials were nontoxic to human body. Since early of 1990's, dental implant was done for recovery of maxillofacial defects. From middle of 1970's, osseointergation concept of implant was introduced and performed in dental field. Biocompatibility of titanium showed good effect for osseointergration but had some problems (Galvance current and toxic corrosion) with suprastructures such as gold crowns. This study was performed to make safe dental implants which have reduced Galvanic currents and corrosion. 3 kind of dental casting gold alloys (different Gold contents, 1㎝×1㎝×0.1㎝ plates.) were used as experimental group, while Titanium were used as control group. Normal human osteoblasts(NHOsts)were cultured during 1-4weeks for histologic study. For analysing the calcium(Ca), Phosphorus(P) and alkaline phosphatase(ALP), NHosts were cultred during 2-23days. After experiments, histologic finding were observed by LSM and SEM. Ca, P, ALP concentration by automatic biochemical analyzer were analyzed by ANOVA test and linear regression method. The results were as follows. Biocompatibility of dental casting gold alloys were similar to titianium alloys histolgically. Biochemical analysis of dental casting gold alloys had no significant difference to titianium alloy except AIGIS-Fine. We could conclude that biocompatibility of dental casting gold alloys with high contents of gold were superior to that of low contents and alloys with high contents of gold had no significant difference from titanium on NHost culture. Gold dental implant might be better than titanium implant due to similar biocompatibility and no galvanic currency.

The aim of this study was to investigate the cytotoxicity of dental casting gold alloys. Recently, "biocompatability" is considered the most important requirement of dental materials. Dental metals and alloys were estimated by quantity of released ions, which had influenced to living tissues. The requirement of using normal human cells for cytoxicity strudy were abruptly increased. We used the cultured normal human gingival fibroblasts to estimate the cytotoxicity of dental casting gold alloys. The product of S company(Korea, AIGIS-SOFT, AIGIS-PLUS, AIGIS-A, AIGIS-PT, experimental group) and D company's (German, Biocclus inlay, Biolor SG, Stabilor NF Ⅳ, Degulor B, control group) dental casting gold alloys were used. The morphological investigation, hemolysis test, MTT assay and SRB assay were done in vitro. In vivo, inflammatory reaction in rat was examined for 2 weeks. 1. In the result of cytotoxicity assay, there were some differences but was no significancy among the results between two group's hemolysis, MTT and SRB assay. 2. The gingival fibroblasts attached to the surface of dental casting gold alloy showed various features and increased in number as the time had passed. 3. In vivo, chronic inflammatory cell infiltration was prominent from 3 days to 1 week and inflammation was reduced as time had gone. From the aboving results, there were no significant differences in cytoxicity depending on the ratio of gold content, but showed differences depending on the ratio of total precious and non-precious metal content between two groups. In vitro study showed few differences in inflamation reaction.