Knockdown of TRPM2 promotes osteogenic differentiation of human periodontal ligament stem cells by modulating NF-κB/NLRP3 pathway

被引:2
作者
Xiang, Xiaosong [1 ]
Hu, Yongxin [2 ]
Song, Zhiqiang [3 ]
Wang, Chunlin [4 ,5 ]
机构
[1] Guangzhou Med Univ, Affiliated Stomatol Hosp, Guangdong Engn Res Ctr Oral Restorat & Reconstruct, Dept Orthodont,Guangzhou Key Lab Basic & Appl Res, Guangzhou 510182, Guangdong, Peoples R China
[2] Guangzhou Med Univ, Affiliated Stomatol Hosp, Guangdong Engn Res Ctr Oral Restorat & Reconstruct, Dept Oral & Maxillofacial Surg,Guangzhou Key Lab B, Guangzhou 510182, Guangdong, Peoples R China
[3] Guangzhou Med Univ, Affiliated Stomatol Hosp, Guangdong Engn Res Ctr Oral Restorat & Reconstruct, Dept Temporomandibular Joint,Guangzhou Key Lab Bas, Guangzhou 510182, Guangdong, Peoples R China
[4] Southern Med Univ, Stomatol Hosp, Sch Stomatol, Dept Orthodont, Guangzhou 510280, Guangdong, Peoples R China
[5] Southern Med Univ, Stomatol Hosp, Sch Stomatol, Dept Orthodont, 366 Jiangnan Da Dao South Haizhu Dist, Guangzhou 510280, Guangdong, Peoples R China
关键词
TRPM2; HPDLSC; NF-kappa B; NLRP3; Periodontitis; INFLAMMATION; ACTIVATION; VS;
D O I
10.1016/j.tice.2023.102184
中图分类号
R602 [外科病理学、解剖学]; R32 [人体形态学];
学科分类号
100101 ;
摘要
Periodontitis is characterized by periodontal destruction triggered by chronic inflammation. The optimal treatment for periodontitis is to improve the periodontal microenvironment, reduce inflammation and achieve periodontal regeneration. Recently, the role of TRPM2 in inflammatory diseases has been reported. However, the function of TRPM2 in periodontal disease and the biological mechanism remain elusive. Therefore, this study aimed to identify the role and explore the underlying mechanisms of TRPM2 in periodontal disease. Here, we first identified the characterization of human periodontal ligament stem cells (PDLSCs). Oil Red O Staining and Alizarin Red mineralized matrix were used to evaluate the multi-differentiation capacity of cells. Flow cytometry was employed to detect MSC-specific surface markers of hPDLSCs. hPDLSCs were treated with 0, 5, 10 or 40 mu g/mL of TNF-alpha for 72 h. Western blot assay were performed to examine the expression of Transient receptor potential cation channel, subfamily M, member 2 (TRPM2) in hPDLSCs. CCK8 and colony formation assays were used to detect the cell viability and proliferation of hPDLSCs, which revealed that TRPM2 knockdown promoted hPDLSCs proliferation. Then, ALP activity in hPDLSCs was detected by ALP activity detection kit. Next, the expression of ALP and Runx2 in hPDLSCs was detected by immunofluorescence staining. The result showed that TRPM2 knockdown promoted osteogenic differentiation and affected the genes expression of osteogenic. Finally, the expressions of p-p65, p65, p-I kappa B alpha, I kappa B alpha and NLRP3 in hPDLSCs were detected by western blot assay. Together, these results suggested that knockdown of TRPM2 accelerated osteogenic differentiation of hPDLSCs through mediating NF-kappa B /NLRP3 pathway.
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页数:7
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