EphB-EphrinB相互作用通过氢氧化钙控制牙源性/成骨分化。
EphB-EphrinB interaction controls odontogenic/osteogenic differentiation with calcium hydroxide.
作者信息
Wang Xiaozhe, Jong George, Lin Louis M, Shimizu Emi
机构信息
Department of Basic Science and Craniofacial Biology, New York University College of Dentistry, New York, New York; Department of Preventive Dentistry, Peking University School and Hospital of Stomatology, Beijing, China.
出版信息
J Endod. 2013 Oct;39(10):1256-60. doi: 10.1016/j.joen.2013.06.016. Epub 2013 Aug 27.
INTRODUCTION
Calcium hydroxide is used in direct pulp capping of uncontaminated exposed vital pulps caused by mechanical or traumatic injury. Calcium hydroxide creates a high alkaline pH environment and initiates a mineralized tissue formation in the pulp. The exact mechanism by which calcium hydroxide induces the reparative dentin formation is unknown. Because Eph receptors and ephrin ligands play a role in pulp stem cell migration and proliferation, our hypothesis is that calcium hydroxide-related odontogenic/osteogenic differentiation may be associated with Eph-ephrin interaction. The aim of this study was to investigate whether Eph-ephrin interaction regulates odontogenic/osteogenic differentiation with calcium hydroxide.
METHODS
Primary pulp cells were harvested from the molars of C57BL/6 mice. The cells were treated with calcium hydroxide. Immunofluorescence was used to detect protein expression. A knockout of the ephrinB1 or EphB2 gene was performed with short hairpin RNAs. Cell migration, proliferation, and gene expression were then analyzed.
RESULTS
Calcium hydroxide stimulated EphB2 gene expression but suppressed ephrinB1 gene expression at the proliferation stage. However, calcium hydroxide stimulated both ephrinB1 and EphB2 gene expression at the differentiation stage. In addition, EphB2 localized at ephrinB1-positive cells at the area of Dentin sialoprotein (DSP) staining, which increased with calcium hydroxide treatment. Knockdown of ephrinB1-EphB2 significantly suppressed cell proliferation. Additionally, knockdown of the ephrinB1 gene caused cell migration, whereas a lack of the EphB2 gene suppressed calcium hydroxide-induced mineralization from primary pulp cells.
CONCLUSIONS
EphrinB1-EphB2 interaction contributes to calcium hydroxide-induced odontogenic/osteogenic differentiation. This observation is the first finding of the mechanism of calcium hydroxide-induced odontogenic/osteogenic differentiation.
引言
氢氧化钙用于对因机械或外伤导致的未受污染的暴露活髓进行直接盖髓。氢氧化钙可营造高碱性pH环境,并启动牙髓中矿化组织的形成。氢氧化钙诱导修复性牙本质形成的确切机制尚不清楚。由于Eph受体和ephrin配体在牙髓干细胞迁移和增殖中发挥作用,我们的假设是氢氧化钙相关的成牙/成骨分化可能与Eph-ephrin相互作用有关。本研究的目的是调查Eph-ephrin相互作用是否通过氢氧化钙调节成牙/成骨分化。
方法
从C57BL/6小鼠的磨牙中获取原代牙髓细胞。用氢氧化钙处理这些细胞。采用免疫荧光法检测蛋白表达。利用短发夹RNA对ephrinB1或EphB2基因进行敲除。然后分析细胞迁移、增殖和基因表达情况。
结果
在增殖阶段,氢氧化钙刺激EphB2基因表达,但抑制ephrinB1基因表达。然而,在分化阶段,氢氧化钙刺激ephrinB1和EphB2基因表达。此外,在牙本质涎蛋白(DSP)染色区域,EphB2定位于ephrinB1阳性细胞,且随着氢氧化钙处理而增加。敲低ephrinB1-EphB2可显著抑制细胞增殖。此外,敲低ephrinB1基因导致细胞迁移,而缺乏EphB2基因则抑制了氢氧化钙诱导的原代牙髓细胞矿化。
结论
EphrinB1-EphB2相互作用有助于氢氧化钙诱导的成牙/成骨分化。这一观察结果是氢氧化钙诱导成牙/成骨分化机制的首次发现。
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