牙龈卟啉单胞菌外膜囊泡携带脂多糖激活Toll样受体2促进破骨细胞分化的研究  

作　　者：邹捷康 曹宇蒙 田义 李璇 吴瑞鑫 田蓓敏 孙海花 陈发明 贺小涛 Zou Jiekang;Cao Yumeng;Tian Yi;Li Xuan;Wu Ruixin;Tian Beimin;Sun Haihua;Chen Faming;He Xiaotao(Department of Periodontology,School of Stomatology,The Fourth Military Medical University,State Key Laboratory of Oral&Maxillofacial Reconstruction and Regeneration,National Clinical Research Center for Oral Diseases,Shaanxi International Joint Research Center for Oral Diseases,Xi′an 710032,China;College of Life Sciences,Northwest University,Xi′an 710069,China;Department of General Dentistry&Emergency,School of Stomatology,The Fourth Military Medical University,State Key Laboratory of Oral&Maxillofacial Reconstruction and Regeneration,National Clinical Research Center for Oral Diseases,Shaanxi International Joint Research Center for Oral Diseases,Xi'an 710032,China)

机构地区：[1]第四军医大学口腔医院牙周病科、口颌系统重建与再生全国重点实验室、国家口腔疾病临床医学研究中心、陕西省口腔疾病国际联合研究中心,西安710032 [2]西北大学生命科学学院,西安710069 [3]第四军医大学口腔医院急诊与综合临床科、口颌系统重建与再生全国重点实验室、国家口腔疾病临床医学研究中心、陕西省口腔疾病国际联合研究中心,西安710032

出　　处：《中华口腔医学杂志》2024年第3期237-246,共10页Chinese Journal of Stomatology

基　　金：国家自然科学基金(82371010,82301079,82101013)。

摘　　要：目的探索牙龈卟啉单胞菌(Pg)来源的外膜囊泡(OMV)对巨噬细胞破骨分化的影响及其作用机制。方法使用透射电镜和纳米颗粒追踪分析仪对Pg OMV进行鉴定和表征;使用1、3和10 mg/L的Pg OMV处理破骨前体细胞,分别为1、3和10 mg/L OMV处理组,磷酸盐缓冲液处理破骨前体细胞为对照组,通过抗酒石酸酸性磷酸酶(TRAP)染色、F-肌动蛋白(F-actin)染色和实时荧光定量PCR技术检测破骨细胞形成和破骨相关基因FBJ骨肉瘤癌基因(Fos)和基质金属蛋白酶9(MMP9)的表达;利用多黏菌素B(PMB)封闭脂多糖(LPS)后的Pg OMV处理破骨前体细胞(PMB-OMV处理组),OMV单独处理为对照,通过TRAP和F-actin染色观察破骨细胞及肌动蛋白环的形成情况;使用蛋白质印迹法检测Pg OMV对破骨前体细胞Toll样受体(TLR)2和TLR4表达水平的影响;利用10、50、100和200μmol/L TLR2抑制剂C29预处理破骨前体细胞后,使用Pg OMV处理破骨前体细胞,分别为OMV+10μmol/L、OMV+50μmol/L、OMV+100μmol/L和OMV+200μmol/L C29处理组,未使用C29预处理的OMV处理组为对照,通过TRAP和F-actin染色观察破骨细胞和肌动蛋白环形成情况;使用OMV和PMB孵育的OMV处理破骨前体细胞,分别为OMV处理组和PMB-OMV处理组,通过蛋白质印迹法检测破骨前体细胞TLR2蛋白表达水平。结果Pg OMV的平均粒径为179.2 nm,具有典型的囊泡结构;3和10 mg/L OMV处理组中可见大量肌动蛋白环形成,TRAP阳性破骨细胞面积占比[分别为(22.6±2.1)%、(32.0±2.3)%]均显著高于对照组[(4.9±0.5)%](P<0.001),3和10 mg/L OMV处理组Fos mRNA表达量(1.491±0.114、1.726±0.254)均显著高于对照组(1.000±0.029)(P=0.013,P=0.001),10 mg/L OMV处理组MMP9 mRNA表达量(2.232±0.097)显著高于对照组(1.007±0.148)(P<0.001);PMB-OMV处理组中肌动蛋白环形成少于OMV处理组,PMB-OMV处理组TRAP阳性破骨细胞面积占比[(14.8±3.8)%]显著低于OMV处理组[(31.5±6.7)%](P=0.004);OMV处理组TLR2表达水平(1.359±0.ObjectiveTo investigate the effects of Porphyromonas gingivalis derived outer membrane vesicles(Pg OMV)on osteoclast differentiation of macrophages and its underlying mechanisms.MethodsThe morphology and the size distribution of Pg OMV were analyzed by transmission electron microscopy and nanoparticle tracing analysis,respectively.The osteoclast precursors were treated with 1,3 and 10 mg/L Pg OMV(1,3 and 10 mg/L OMV treatment group)or phosphate buffer solution(PBS)(control group).The formation of osteoclasts was analyzed by tartrate-resistant acid phosphase(TRAP)staining and F-actin staining and real-time quantitative PCR(RT-qPCR)were used to detect the expression of Fos and matrix metallopeptidase 9(MMP9).Polymyxin B(PMB)was used to block lipopolysaccharide(LPS)and then Pg OMV was used to treat osteoclast precursor(PMB-OMV treatment group),and OMV treatment group was used as control.TRAP and F-actin staining were used to observe the formation of osteoclasts and actin rings.The effect of Pg OMV on the expression of Toll-like receptor(TLR)2 and TLR4 in preosteoclasts was detected by Western blotting.The osteoclast precursors were pretreated with 10,50,100 and 200μmol/L C29,an inhibitor of TLR2,and then treated with Pg OMV(OMV+10,50,100 and 200μmol/L C29 treatment group)and OMV treatment group without C29 pretreatment was control.TRAP and F-actin staining were used to observe the formation of osteoclasts and actin rings.The osteoclast precursor cells were treated with OMV(OMV treatment group)and OMV incubated with PMB(PMB-OMV treatment group)and the expression of TLR2 in osteoclast precursor was detected by Western blotting.ResultsPg OMV showed classical vesicular structures,and the average particle size of Pg OMV were 179.2 nm.A large number of actin rings were observed in the 3 and 10 mg/L OMV treatment groups.The percentages of TRAP-positive osteoclast area in 3 mg/L OMV treatment group[(22.6±2.1)%]and 10 mg/L OMV treatment group[(32.0±2.3)%]were significantly increased compared with control group[(4.9±0.5)

关 键 词：牙周炎 紫单胞菌 龈 外膜囊泡 破骨细胞 TOLL样受体2 

分 类 号：R781.42[医药卫生—口腔医学]