摘要
目的:探讨p38丝裂原活化蛋白激酶(p38 mitogen-activated protein kinase,p38 MAPK)在钛颗粒诱导的破骨细胞形成中的作用。方法:提取小鼠骨髓细胞,接种于24孔板后分为3组:1空白对照组;2核因子κB受体活化因子配体(receptor activator for nuclear factor-κB ligand,RANKL)组:每孔加入50 ng/ml RANKL;3钛颗粒+RANKL组:每孔加入0.01%钛颗粒悬液(0.1 mg/ml)及RANKL 50 ng/ml,抗酒石酸酸性磷酸酶(tartrate-resistant acid phosphatase,TRAP)染色鉴定和计数破骨细胞。Western blot检测p38、磷酸化p38的表达水平,通过腺病毒介导的p38 siRNA沉默p38的表达后,观察破骨细胞数目及相关蛋白RANK的变化情况。结果:各组破骨细胞计数结果分别为:空白对照组2.0±0.8,RANKL组62.8±5.6,钛颗粒+RANKL组93.0±8.8(F=235.193,P=0.000)。RANKL组高于空白对照组(P=0.000),钛颗粒+RANKL组明显高于RANKL组(P=0.000)。Western blot结果显示钛颗粒能明显提高p38的磷酸化水平(p-p38/p38相对值:空白对照组0.29±0.05,RANKL组0.64±0.05,钛颗粒+RANKL组0.87±0.05,F=106.491,P=0.000,钛颗粒+RANKL组高于空白对照组和RANKL组P1=0.000,P2=0.001)。转染腺病毒介导的p38 siRNA后,Ad-sip38干扰组RANK蛋白的表达水平低于对照组和Ad-RFP组,破骨细胞数目也明显低于对照组和Ad-RFP组(破骨细胞计数:对照组99.8±13.5,Ad-RFP组95.8±7.1,Ad-sip38组3.8±2.5,F=148.654,P=0.000,对照组与Ad-RFP组无明显差异P=0.541,Ad-sip38处理组与对照组和空白病毒组比较均P=0.000)。结论:p38 MAPK在钛颗粒诱导的破骨细胞形成中起重要的作用。
Objective:To investigate the effects of p38 mitogen-activated protein kinase on titanium(Ti)particle-induced osteoclast formation. Methods:Bone marrow cells were collected from the femur and tibiae of 4-6 week-old BALB/C mice and were divided into three groups:1control group;2receptor activator for nuclear factor-κB ligand(RANKL)treated group;3Ti particle and RANKL treated group. The numbers of osteoclasts were measured by the tartrate-resistant acid phosphatase(TRAP)staining. The expression and phosphorylation level of p38 protein were determined by Western blot. Then an adenovirus-mediated RNA interference targeting p38 was employed to knock down the expression of p38 and the numbers of osteoclasts were determined by TRAP staining;the expression of osteoclast specific gene RANK was detected using Western blot. Results:TRAP staining showed that the numbers of osteoclasts were significantly higher in Ti particle treated group than in control group with the same concentration of RANKL(blank group:2.0±0.8,RANKL group:62.8±5.6,Ti particle +RANKL group:93.0±8.8,F=235.193,P=0.000)(RANKL group vs. blank group,P=0.000;Ti particle+RANKL group vs. RANKL group,P=0.000). The relative phosphorylation level of p38 was significantly improved in Ti particle and RANKL treated group compared with that in control group and RANKL treated group(blank group:0.29±0.05,RANKL group:0.64±0.05,Ti particle+RANKL group:0.87±0.05,F=106.491,P=0.000)(Ti particle+RANKL group vs. blank group and RANKL group,P1=0.000,P2=0.001). After being treated with adenovirus-mediated p38 siRNA(Ad-sip38),the number of osteoclasts and the protein level of RANK were remarkably decreased(TRAP positive cells:control group:99.8±13.5,Ad-RFP group:95.8±7.1,Ad-sip38 group:3.8±2.5)(control group vs. Ad-RFP group,P=0.541;Ad-sip38 group vs. control group and Ad-RFP group,P1=0.000,P2=0.000). Conclusion:p38 MAPK plays an important role in the osteoclast formation induced by Ti particle.
出处
《重庆医科大学学报》
CAS
CSCD
北大核心
2015年第6期873-877,共5页
Journal of Chongqing Medical University
