β-防御素3调节人牙龈成纤维细胞分泌MMP-1及PGE_2的信号通路研究

目的:研究β-防御素3(HBD3)调节人牙龈成纤维细胞(HGFs)分泌MMP-1和PGE2的信号通路。方法:取P5代HGFs接种于96孔板,并随机分为1个对照组(HBD3)和7个实验组(HBD3+antiTLR2、HBD3+anti-TLR4、HBD3+SB203580、HBD3+PD98059、HBD3+SP600125、HBD3+LY294002、HBD3+SC3060)。各实验组分别以相应的信号通路抑制剂anti-TLR2、anti-TLR4预处理30 min,SB203580、PD98059、SP600125、LY294002、SC3060预处理60min,然后各组再加入100μL浓度为1μg/mL的HBD3进行培养,12h后收集各组培养上清液,ELISA法检测MMP-1及PGE2浓度。结果:信号通路抑制剂SB203580、PD98059、SC3060、anti-TLR2各组MMP-1的浓度(ng/mL)分别为3.660±0.286、3.410±0.554、4.435±0.235、3.995±0.612,低于对照组(5.128±0.256)ng/mL(P<0.05);信号通路抑制剂SP600125、SC3060两组PGE2浓度(pg/mL)分别为146.518±15.800和180.349±5.490,低于对照组(209.213±7.284)pg/mL(P<0.05)。结论:HBD3调节HGFs分泌MMP-1涉及TLR2、P38、ERK、NF-κB信号途径;调节PGE2分泌涉及JNK和NF-κB信号途径。

EXPRESSION OF HUMAN BETA-DEFENSIN 3 IN COS-7 CELL

To establish a cell line for stable expression of human beta-defensin 3 (hBD3). Methods Full length cDNA of hBD3 was isolated from previously constructed pGEM-hBD3 and then inserted into pcDNA3. The recombinant vector identified carrying hBD3 with right direction was introduced into COS-7 cells by Lipofe-ctamine. Cell clones survived in G418-rich medium and with stable expression of hBD3 in both mRNA and protein levels were identified by RT-PCR and Western blot respectively. Genomic integration of the hBD3 gene with the COS-7 cells was confirmed by Southern dot blot and primary analysis. The antimicrobial activity of the secreted hBD3 was also evaluated. Results COS-7 cells transfected with pcDNA3-hBD3 expressed hBD3 stably in mRNA and protein level. Southern dot blot analysis showed successful integration of the hBD3 gene into the genome of COS-7 cell and the hBD-3 protein secreted into the culture medium showed antimicrobial activity. Conclusion We successfully established a hBD3-expressing cell line.