摘要
目的:研究阿仑膦酸盐(ALN)对成骨细胞(OB)-破骨细胞(OC)共培养体系中破骨细胞生成、功能及相关基因表达的影响。方法:胰酶消化法培养鼠颅骨成骨细胞,并与骨髓细胞建立OB-OC共培养体系;体系中加入10-6mol/L PGE2、10-8mol/L VitD3诱导破骨细胞分化生成。实验分对照组和ALN(10-6mol/L)处理组。采用TRAP染色及扫描电镜检测破骨细胞生成及牙本质磨片吸收陷窝情况,并应用Real-time PCR检测破骨细胞相关基因NFATc1、c-Fos、RANKL、OPG的基因表达。结果:各组细胞均有TRAP阳性多核OC生成,并在牙本质磨片上形成吸收陷窝;但对照组所获TRAP阳性多核细胞数目、吸收陷窝数目及面积均显著大于ALN组。Real-time PCR检测结果显示对照组NFATc1、c-Fos、RANKL、OPG的基因表达均显著高于ALN组。结论:ALN在OB-OC共培养体系中可抑制OC的生成及其骨吸收功,并下调OC相关基因NFATc1、c-Fos、RANKL、OPG的基因表达。
Objective: To study the influence of alendronate on osteoclastogenesis, bone resorption and expression of osteoclast-as- sociated genes in an osteblast-osteoclast eo-euhure system. Methods: Mice calvarial osteoblasts were harvested by trypsin digestion and bone marrow cells were obtained. The cells were co-cultured in ct-MEM, PGEa (10-6 M) and VitD3 (10-s M) were added in the cultures to induce osteoclastogenesis. The cells treated by ALN( 10-6 mol/L) were in ALN group, and those without ALN in control group. Osteoclastogenesis and their resorption function were examined by TRAP staining and scanning electron microscope ( SEM ) observation of dentin resorption lacunaes. Gene expressions of NFATcl, c-Fos, RANKL and OPG were detected by Real-time PCR. Results: TRAP positive multinuclear cells and resorption lacunaes were observed in both groups. However, control group showed more TRAP positive multinuclear cells and more resorption lacunaes than ALN group. Real-time PCR detection showed that gene ex- pressions of NFATcl, c-Fos, RANKL and OPG were higher in control group than in ALN group. Conclusion: ALN can inhibit oste- oclastogenesis, resorption function, and gene expression of osteclast-associated genes in the osteoblast-osteoclast co-culture system.
出处
《实用口腔医学杂志》
CAS
CSCD
北大核心
2012年第6期682-685,共4页
Journal of Practical Stomatology
基金
河北省自然科学基金(编号:C2011401044)
