摘要
本文采用ELISA方法检测培养的人脐静脉内皮细胞(HUVEC)表面玻璃连接蛋白受体(VitronectinreceptorVnR即整合素家庭的α_vβ_3)的表达改变;用(51)Cr-标记血小板((51)Cr-platelete,(51)Cr-pL)检测HUvEc的粘附功能;Fura-2/Am负载EC,测定HUVEC胞内游离钙离子浓度([Ca(2+)]),观察了高糖、肿瘤坏死因子-α(Tumornecrosisfactor-α,TNF-α)对EC粘附功能的影响。结果表明:①高糖(30mmol/L)可明显促进EC与PL的粘附(CPM值:361±2l.93VS2l9.67±16.26,n=6P<0.01),抗β3亚单位单抗(β3McAb)可部分阻断EC与PL粘附。TNF-α(1000μ/m1)也有相同作用(CPM值:4l0.7±17.6VS219.67±16.261n=6P<0.01),β3McAb也部分阻断TNF-α诱导的EC-PL间的粘附。②不同浓度高糖和TNF-α不同时间可影响EC表面的α_vβ_3表达,并且在一定范围内有浓度和时间依赖性。③高糖和TNF-α可明显增加EC的[Ca(2+)]i,上述资料提示?
his study was performed on the cultured endothelial cells(EC)to observe the promoting effect oftumor necrosis factor-α(TNF-α) and high glucose (HG) on the expression of integrin-αvβ3 on the surfaceof EC, It was found that TNF-αand HG enhanced obviously the expression of αvβ3, and the adhessivefunction of EC to platelet (PL). With ELIsA, we found that different concentration of TNF-αand HGcould increase the expression of αvβ3 In the same concentration group, the expressiozi of αvβ3 showed aup-tendency with the stimulated time prolonged. In addition, TNF-αand HG can induce the increase of[Ca2+]i remarkably, Our results suggested that TNF-α and HG could strengthen the expression of αvβ3and increase the adhesive function of ECs to Pls。αvβ3was a important mediator in the adhesion of PL-EC。Meanwhile,[Ca2+]i also played a important role in mediating adhesion between ECs and PLs as asecond-messeger。
出处
《解剖科学进展》
CAS
1996年第4期370-376,共7页
Progress of Anatomical Sciences
