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Cytotoxic evaluation of two orthodontic silver solder materials on human periodontal ligament fibroblast cells and the effects of antioxidant and antiapoptotic reagents

机译:对人牙周韧带成纤维细胞的两种正畸银焊料的细胞毒性评价及抗氧化剂和抗透露试剂的影响

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ABSTRACT Objectives To evaluate the cytotoxicity effects of two different solder materials used for orthodontic appliances on human periodontal ligament fibroblast (HPLF) cells, and to determine whether the mechanism of toxicity may involve oxidative stress and apoptosis. Materials and Methods The silver solder samples (Leone and Summit) were soldered to orthodontic stainless steel bands and exposed to HPLF cells via cell culture inserts for 48 hours. Cytotoxicity effect of the soldered materials on HPLF cells was measured via tetrazolium salt 3-(4,5-dimethylthiazol-2-yl)-2, 5-diphenyltetrazolium bromide (MTT) colorimetric assay (n = 10/sample) and morphological observation. In addition, the mechanism of cytotoxicity of the most toxic silver solder was investigated using both a caspase inhibitor Z-VAL-Ala-Asp-flu-oromethylketone (ZVAD-fmk) and the free radical scavenger Trolox (n = 8/sample). Statistical analysis was performed using one-way analysis of variance with a Bonferroni test. P .05 was considered statistically significant. Results Compared to the control (no treatment, cells only), both silver solders were cytotoxic (P .001). The bands alone were significantly cytotoxic compared to the control. There was a significant difference in cytotoxicity between the stainless steel bands alone and the Summit silver solder (P .001), but not the Leone silver solder. The Summit silver solder was more cytotoxic than the Leone silver solder (P .05). MTT results were supported by the microscopic morphological changes of the HPLF cells. Neither ZVAD-fmk nor Trolox provided significant protection. Conclusions The two silver solder materials demonstrated different levels of cytotoxicity, and neither oxidative stress nor apoptosis is involved in the mechanism of cytotoxicity.
机译:摘要目的是评估两种不同焊料用于牙齿韧带成纤维细胞(HPLF)细胞的两种不同焊料材料的细胞毒性影响,并确定毒性机制是否可能涉及氧化应激和凋亡。材料和方法将银焊料样品(Leone和Summit)焊接到正畸不锈钢带,并通过细胞培养插入物暴露于HPLF细胞48小时。通过四唑盐3-(4,5-二甲基噻唑-2-基)-2,5-二苯基四唑溴(MTT)比色测定(N = 10 /样品)和形态学观察测量焊接材料对HPLF细胞上焊接物质的细胞毒性效应。此外,使用Caspase抑制剂Z-Val-Ala-Asp-流感 - oromethylone(ZVAD-FMK)和自由基清除剂杂志(n = 8 /样品)研究了最有毒银焊料的细胞毒性机制。使用与Bonferroni测试的单向分析进行统计分析。 P& .05被认为是统计学意义。结果与对照相比(仅处理,仅细胞),两种银焊料都是细胞毒素(P <.001)。与对照相比,单独的乐队具有显着的细胞毒性。单独的不锈钢带之间的细胞毒性和峰会银焊料(P <.001)之间存在显着差异,但不是LEONE银焊料。峰会银焊料比Leone银焊料更具细胞毒性(P <.05)。 MTT结果得到了HPLF细胞的微观形态变化的支持。 ZVAD-FMK和TROLOX都没有提供显着的保护。结论两种银焊料展示了不同水平的细胞毒性,均未参与细胞毒性机制的氧化应激。

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