摘要
目的:探讨钙通道拮抗剂—维拉帕米(verapamil,Ver)对体外培养的人视网膜色素上皮(humanretinalpigmentepithelium,hRPE)细胞凋亡诱导作用及凋亡过程中细胞内钙浓度[Ca2+]i的变化。方法:应用80mg/L的Ver作用体外培养hRPE细胞12,24及48h,采用吖叮橙(AO)荧光染色法、透射电镜、流式细胞术观察hRPE细胞凋亡;Fluo-3/AM负载技术,观察凋亡过程中细胞[Ca2+]i的变化。结果:一定浓度Ver可诱导hRPE细胞凋亡,荧光显微镜及电镜观察hRPE细胞具有早期凋亡特征:核荧光呈黄绿色,电镜下核染色质浓染、边集。流式细胞术显示,Ver作用后的hRPE细胞凋亡百分率增加(F=12.3415,P<0.05)。Ver作用的hRPE细胞内钙浓度([Ca2+]i)呈下降趋势(F=23.607,P<0.01)。结论Ver能诱导体外培养的hRPE细胞凋亡,细胞内[Ca2+]i浓度的变化可能是诱导hRPE凋亡的机制之一。
AIM: To explore the effect of calcium channel antagonist, verapamil on inducing hRPE apoptosis and the changes of intracellular free [Ca^2+]i.
METHODS: Cultured hRPE cells were added 80mg/L verapamil for 12, 24 and 48h. AO fluorescence staining, transmission electron microscopy and flow cytometer were used to determine the effect of verapamil on hRPE cells. Fluo-3/AM load technique was used to observed the changes of hRPE intracellular free [Ca^2+]i.
RESULTS: Verapamil can induce apoptosis of hRPE. Apoptosis features were observed by AO staining with fluorescence microscope: nucleolus fluorescence was kelly. Under transmission electron microscope, nucleolus chromatin concentrated and dyed black. Flow cytometer displayed the apoptosis rate increased (F =12.3415, P 〈 0.05). hRPE cells intracellular free [Ca^2+]i decreased gradually (F =23.607, P〈0.01).
CONCLUSION: Verapamil may induce the apoptosis of cultured hRPE in vitro. The change of [Ca^2+]i may be the one of important mechanisms of apoptosis of hRPE cells.
出处
《国际眼科杂志》
CAS
2006年第2期324-327,共4页
International Eye Science
基金
中国国家自然科学基金资助(No.30471865)~~
