一种改进的大鼠肝星状细胞分离方法  被引量：8

作　　者：舒建昌[1] 赵景润[1] 杨冬华[2] 沈雁[1] 钟灿灿[1] 

机构地区：[1]暨南大学医学院附属广州红十字会医院,广州510220 [2]暨南大学医学院附属第一医院

出　　处：《中华肝脏病杂志》2004年第6期353-355,共3页Chinese Journal of Hepatology

基　　金：广东省中医药局科研基金(10220);广州市卫生局科研基金(200226)

摘　　要：目的改进大鼠肝星状细胞的分离方法,提高肝星状细胞分离的纯度和活力.方法 SD大鼠在静脉注射1 m1含二氯亚甲基二磷酸盐的脂质体3d后,用含100U/ml肝素的D-H anks液灌注肝脏l0～l5min,改用含0.05%胶原酶溶液的D-Hanks液灌注25～30min,将肝脏细胞悬液置于0.025%胶原酶、0.005%DNase Ⅰ的溶液中振荡消化30 min,细胞悬液过200目筛网,50×g离心2 min去除肝细胞,300×g离心10 min得到肝脏非实质细胞沉淀,将细胞悬浮于Nycodenz使终浓度为11.5%,1400×g离心17mmin,吸取Nycodenz上层的细胞即为肝星状细胞.台盼蓝拒染实验鉴定细胞活力,自发荧光、D esmin免疫细胞化学染色鉴定细胞纯度,内源性过氧化物酶染色检测库普弗细胞.结果肝星状细胞得率每只大鼠约3×107个,细胞活力在95%以上,初分离的肝星状细胞在328 nm激发光下自发蓝绿色荧光,De smin免疫细胞化学染色鉴定纯度达到90%,未检测到内源性过氧化物酶阳性细胞.结论建立了一种无库普弗细胞混杂的大鼠肝星状细胞分离方法,可以用于原代肝星状细胞的生物学行为的研究.Objective To present an improved method to obtain pure, viable, freshly isolated hepatic stellate cells. Methods Adult male SD rats were used. All procedures were performed with the animals under sodium pentobarbital anesthesia. Three days after the single intravenous administration of 1 ml liposome-encapsulated CL2MDP, which has selective cytotoxicity of Kupffer cells, livers were perfused with D-Hank's solution containing 100 U/ml heparin for 10 to 15 minutes, and then with 0.05% collagenase dissolved in D-Hank's solution for 25 to 30 minutes. The liver was then gently homogenized and further incubated in 0.025% collagenase, and 0.005% DNAase I for 30 minutes at 37℃ under constant stirring. This suspension was filtered through stainless steel gauze and centrifuged for 2 minutes at 50×g to remove parenchymal cells. Sinusoidal cells in the supernatant were recovered by centrifugation for 10 minutes at 300× g. The cells were resuspended in the presence of 28.7% Nycodenz stock solution. The final concentration of Nycodenz at this stage was 11.5%. Following centrifugation for 17 minutes at 1400×g, The cells at the top of this Nycodenz solution were collected. Cells were resuspended in Dulbecco's modified Eagle medium supplemented with 10% fetal calf serum, The cells were seeded in 50 ml culture flask at a density of 500 000 cells/ml, The cell viability was determined by trypan blue exclusion staining, the purity of hepatic stellate cells was identified by the expression of Desmin using immunocytochemistry method. Endogenous peroxidase staining was used to detect Kupffer cells. Results The yield rate of hepatic stellate cells was 3×10~7 per rat, the cell viability was more than 95%, the desmin positive cell rate was 90%, no endogenous peroxidase positive cells were detected. Conclusion The method for the isolation of hepatic stellate cells was developed without kupffer

关 键 词：大鼠 肝星状细胞 细胞分离 二氯亚甲基二磷酸盐 库普弗细胞 肝纤维化 

分 类 号：R575.2[医药卫生—消化系统]