摘要
目的:探索建立稳定有效的脐静脉内皮细胞体外培养方法。方法:用0.1%II型胶原酶消化分离人脐静脉肉皮细胞,加入含内皮细胞生长因子的M199完全培养液中培养,用胰蛋白酶-EDTA进行消化传代培养,用光镜和免疫组化方法对培养的细胞进行形态观察和鉴定。结果:原代培养的内皮细胞在接种后24h后完全贴壁生长,第445天后融合呈铺路石样镶嵌排列,免疫组化可见胞浆中第Ⅷ因子相关抗原呈阳性反应,证实培养的细胞为内皮细胞。结论:脐静脉灌注II型胶原酶消化法配合M199完全培养液可获得高纯度的内皮细胞,细胞可传代5—6次,但细胞产出量不高,不能传10代以上,5代以后细胞形态变化较大,对于复杂的基础研究应用受限。
Objective: To investigate a stable way to culture the human umbilical vein endothelial cells(HUVECs). Methods: HU- VECs were obtained from human umbilical vein, digested with 0.1% coUagenase type II and cultivated in M 199 culture medium containing 20μg/mL ECGF. Subculture was attained with trypsin/EDTA solution when cells were 90% confluent. The cells were detected under a fluorescence microscope with immunohistochemical method. Results: The primary cells could adhere to the plate completely within 24 hours and grow to a monolayer in 4-5 days. Confluent cells exhibited the characteristic "cobblestone" morphology in culture and were positively immunostained with antibodies against von Willeband factor(vWF), which proved that the cultured cells were endothetial cells. Conclusion: Highly purified primary HUVECs can be acquired by digestion of collagenase type II and cultivation of M199 complete culture medium. Further subculture beyond passage 5 is not advisable since the cell growth rate may decline and phenotypic changes become evident which may limit its application in complicated basic research.
出处
《现代生物医学进展》
CAS
2013年第28期5438-5441,共4页
Progress in Modern Biomedicine
基金
云南省教育厅科学研究基金项目(08Y0222)
关键词
人脐静脉内皮细胞
细胞培养
鉴定
Human umbilical vein endothelial cells (HUVECs)
Culture
Characterization
