牙科修复材料的体外胚胎毒性评估

In vitro embryotoxicity assessment with dental restorative materials.

作者信息

Schwengberg S, Bohlen H, Kleinsasser N, Kehe K, Seiss M, Walther U I, Hickel R, Reichl F X

机构信息

Axiogenesis AG, Joseph-Stelzmann-Str. 50, 50931 Köln, Germany.

出版信息

J Dent. 2005 Jan;33(1):49-55. doi: 10.1016/j.jdent.2004.08.001.

DOI:10.1016/j.jdent.2004.08.001

PMID:15652168

Abstract

OBJECTIVES

Resin (co)monomers may be released from restorative dental materials and can diffuse into the tooth pulp or the gingiva, and can reach the saliva and the circulating blood. Genotoxic potential of some dental composite components has been clearly documented. The genotoxic effects of xenobiotics can represent a possible step in tumor initiation and/or embryotoxicity/teratogenesis. A modified fluorescent mouse embryonic stem cell test (R.E.Tox) was used to test the embryotoxic potential of following dental restorative materials: Bisphenol A glycidylmethacrylate (BisGMA), urethanedimethacrylate (UDMA), hydroxyethylmethacrylate (HEMA), and triethyleneglycoldimethacrylate (TEGDMA), as well as some of their metabolic intermediates 2,3-epoxy-2-methyl-propionicacid-methylester (EMPME), methacrylic acid (MA), and 2,3-epoxy-2-methylpropionic acid (EMPA).

METHODS

Mouse embryonic stem (ES) cells stably transfected with a vector containing the gene for the green fluorescent protein under control of the cardiac alpha-myosin heavy chain promoter were differentiated in the presence of various concentrations of the test compounds for 12 days. Fluorescence was measured using the TECAN Safire and values were expressed as percent of control values. To distinguish between cytotoxic and embryotoxic effects, all compounds were tested in a standard MTT assay.

RESULTS

HEMA, TEGDMA and EMPME did not influence the differentiation process of ES cells towards cardiac myocytes. No cytotoxic effects were observed at any of the concentration levels tested. Exposure to BisGMA resulted in a 50% decrease in cell survival and a very strong inhibition of cell differentiation at 10(-5)M (p<0.01). Embryotoxic effects were also present at 10(-6) and 10(-7)M (p<0.05). EMPA induced a decrease in ES cell differentiation at 10(-5)M (p<0.01) without cytotoxic effects. No embryotoxic effects were induced at lower concentrations. Exposure to UDMA resulted in a slight decrease of cell differentiation at 10(-5)M (p<0.05). Exposure of cells to MA resulted in an increase of cardiac differentiation up to 150% (p<0.05) at 10(-5)M without cytotoxic effects.

CONCLUSIONS

BisGMA induced a significant high embryotoxic/teratogenic effect over a large range of concentration. Therefore attention should be focused on this dental monomer, which should be investigated further by in vivo experiments.

摘要

目的

树脂（共）单体可能从牙科修复材料中释放出来，扩散到牙髓或牙龈中，并进入唾液和循环血液。一些牙科复合材料成分的遗传毒性潜力已有明确记录。外源性物质的遗传毒性作用可能是肿瘤发生和/或胚胎毒性/致畸作用的一个可能步骤。采用改良的荧光小鼠胚胎干细胞试验（R.E.Tox）来检测以下牙科修复材料的胚胎毒性潜力：双酚A甲基丙烯酸缩水甘油酯（BisGMA）、二甲基丙烯酸聚氨酯（UDMA）、甲基丙烯酸羟乙酯（HEMA）和三乙二醇二甲基丙烯酸酯（TEGDMA），以及它们的一些代谢中间体2,3-环氧-2-甲基丙酸甲酯（EMPME）、甲基丙烯酸（MA）和2,3-环氧-2-甲基丙酸（EMPA）。

方法

将稳定转染了含有在心脏α-肌球蛋白重链启动子控制下的绿色荧光蛋白基因的载体的小鼠胚胎干细胞（ES细胞）在存在不同浓度测试化合物的情况下分化12天。使用TECAN Safire测量荧光，并将值表示为对照值的百分比。为了区分细胞毒性和胚胎毒性作用，所有化合物都在标准MTT试验中进行了测试。

结果

HEMA、TEGDMA和EMPME不影响ES细胞向心肌细胞的分化过程。在任何测试浓度水平下均未观察到细胞毒性作用。暴露于BisGMA导致细胞存活率降低50%，并且在10⁻⁵M时对细胞分化有非常强烈的抑制作用（p<0.01）。在10⁻⁶和10⁻⁷M时也存在胚胎毒性作用（p<0.05）。EMPA在10⁻⁵M时诱导ES细胞分化降低（p<0.01），但无细胞毒性作用。在较低浓度下未诱导胚胎毒性作用。暴露于UDMA导致在10⁻⁵M时细胞分化略有降低（p<0.05）。细胞暴露于MA导致在10⁻⁵M时心脏分化增加至150%（p<0.05），且无细胞毒性作用。