首页> 外文期刊>Journal of Endodontics: Official Journal of American Association of Endodontists >Mineral trioxide aggregate induces bone morphogenetic protein-2 expression and calcification in human periodontal ligament cells.
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Mineral trioxide aggregate induces bone morphogenetic protein-2 expression and calcification in human periodontal ligament cells.

机译:三氧化二铁矿物质诱导人牙周膜细胞中骨形态发生蛋白2的表达和钙化。

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INTRODUCTION: Mineral trioxide aggregate (MTA) is a therapeutic, endodontic repair material that is reported to exhibit calcified tissue-conductive activity although the mechanisms remain unclear. We hypothesize that the dissolution of calcium from MTA into the surrounding environment may play an important role in the osteoblastic/cementoblastic differentiation of human periodontal ligament cells (HPLCs). METHODS: Two populations of HPLCs were obtained from two patients, respectively, and were cultured in the presence or absence of MTA discs and/or CaCl(2) in order to investigate calcium release, calcification activity, calcium-sensing receptor (CaSR) gene expression and bone morphogenetic protein-2 (BMP-2), and BMP-2 receptor protein and gene expression. RESULTS: MTA released a substantial accumulation of calcium (4 mmol/L) within 14 days into culture media. After 4 weeks, the two populations of HPLCs independently exhibited calcification as well as BMP-2 distribution in the vicinity of MTA. HPLCs inherently expressed genes encoding for the CaSR and BMP-2 receptors. Exogenous CaCl(2) media supplementation induced CaSR gene expression in HPLCs and calcification and BMP-2 synthesis throughout the entire HPLC cultures, whereas MgCl(2) had no effect. Both MTA and CaCl(2) stimulated BMP-2 gene expression above that of baseline levels. CONCLUSION: Here we show the first report showing that HPLCs cocultured directly with MTA up-regulated BMP2 expression and calcification. These results may be through CaSR interactions that were potentially activated by the release of calcium from MTA into the culture environment.
机译:简介:三氧化二矿骨料(MTA)是一种治疗性牙髓修复材料,据报道其具有钙化的组织传导活性,尽管其机理尚不清楚。我们假设钙从MTA溶解到周围环境中可能在人牙周膜细胞(HPLC)的成骨/胶质母细胞分化中起重要作用。方法:分别从两名患者中获得两个HPLC种群,并在存在或不存在MTA盘片和/或CaCl(2)的情况下进行培养,以研究钙的释放,钙化活性,钙敏感受体(CaSR)基因骨形态发生蛋白2(BMP-2)的表达以及BMP-2受体蛋白和基因的表达。结果:MTA在14天内向培养基中释放了大量钙(4 mmol / L)。 4周后,这两个HPLC群体在MTA附近独立显示钙化以及BMP-2分布。 HPLC固有地表达编码CaSR和BMP-2受体的基因。外源CaCl(2)培养基诱导在整个HPLC文化中的HPLC中钙化和BMP-2合成的CaSR基因表达,而MgCl(2)没有作用。 MTA和CaCl(2)都刺激BMP-2基因表达高于基线水平。结论:在这里我们显示了第一个报告,表明与MTA直接共培养的HPLC上调了BMP2的表达和钙化。这些结果可能是通过CaSR相互作用引起的,该相互作用可能是由MTA中的钙释放到培养环境中而潜在激活的。

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