Uji sitotoksisitas mikrofiber PMMA dan PMMA-Silika wetspinning pada kultur sel primer L-929 sebagai aplikasi penguat jembatan gigi direkCytotoxicity test of PMMA and PMMA-Silica wet spinning microfibers in L-929 primary cell culture as a direct dental bridge reinforcement application

N. Djustiana, Yanwar Faza, A. Hardiansyah
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Abstract

Introduction: Direct dental bridge consists of a fiber reinforcement component and a composite resin matrix component. The use of target cells for the cytotoxicity test of dental fiber materials is generally performed by experimental in-vitro tests to determine the clinical relevance of the test. This study was aimed to examine the cytotoxicity of PMMA and PMMA-silica wet spinning microfibers with different parameters on the primary cell culture (cell line) of L-929 fibroblasts. Methods: The research design was descriptive qualitative. Primary L-929 fibroblast cells were exposed to PMMA and PMMA-silica microfibers consecutively for 1, 4, and 7 days. Cytotoxicity test was performed using the MTT Assay. Parameters of PMMA and PMMA-silica microfibers used were concentration and flow rate, then divided into several research groups and named as follows: PMMA microfiber vertical system 250ml/hour with a concentration in %: 0.75(A); 1(B); 1.25(C); PMMA-silica microfiber vertical system with the speed of 200 ml/hour (D), 250 ml/hour (E), 300 ml/hour (F) and PMMA microfiber with rotation system 200 ml/ hour with a concentration in % 0.75(G );1(H), 1,25(I); PMMA-silica microfiber rotation system with concentrations of 200ml/hour (J), 250ml/hour (K), and 300 ml/hour (L). Results: In-vitro test of the L-929 cell picture showed no primary fibroblast cells that died. The cell line growth curve of each microfiber parameter shows that the cells can proliferate during the incubation period and show a positive trend of cell growth. Conclusions: PMMA and MMAsilica wet spinning microfibers did not show any toxicity to the growth of the L-929 fibroblast cell line, so they have potential as reinforcement applications for direct dental bridges.
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简介:直接牙桥由纤维增强部件和复合树脂基部件组成。使用靶细胞进行牙纤维材料的细胞毒性试验通常是通过实验性体外试验来确定试验的临床相关性。研究不同参数的PMMA和PMMA-二氧化硅湿纺微纤维对L-929成纤维细胞原代培养(细胞系)的细胞毒性。方法:采用描述性定性设计。将原代L-929成纤维细胞连续暴露于PMMA和PMMA-二氧化硅微纤维中1,4,7天。采用MTT法进行细胞毒性试验。采用PMMA和PMMA-二氧化硅微纤维的参数为浓度和流速,分为几个研究组命名为:PMMA微纤维垂直体系250ml/h,浓度为%:0.75(a);1 (B);1.25 (C);PMMA-二氧化硅微纤维垂直系统,速度为200 ml/小时(D), 250 ml/小时(E), 300 ml/小时(F), PMMA微纤维旋转系统,浓度为% 0.75(G), 1(H), 1,25(I);pmma -二氧化硅微纤维旋转体系,浓度分别为200ml/h (J)、250ml/h (K)和300ml /h (L)。结果:L-929细胞图体外测试未见原代成纤维细胞死亡。各微纤维参数的细胞系生长曲线显示,细胞在孵育期间均能增殖,细胞生长呈正向趋势。结论:PMMA和MMAsilica湿纺丝微纤维对L-929成纤维细胞系生长无明显毒性,具有作为直接牙桥加固材料的应用潜力。
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