基础医学与临床 ›› 2011, Vol. 31 ›› Issue (11): 1278-1282.

• 技术与方法 • 上一篇    下一篇

简易高效分离培养鼠胸主动脉血管内皮细胞方法的建立

韩松1,曲彦明1,李俊发2   

  1. 1. 首都医科大学神经生物学系
    2. 首都医科大学
  • 收稿日期:2011-02-18 修回日期:2011-04-20 出版日期:2011-11-05 发布日期:2011-11-02
  • 通讯作者: 李俊发 E-mail:junfali@ccmu.edu.cn
  • 基金资助:
    国家自然科学基金;国家重点基础性研究项目;北京市教育委员会科技计划重点项目;北京市属高等院校人才强教计划项目;北京市新世纪百千万人才工程培养经费;教育部高等学校博士点科研基金

Establishment of a simple and efficient method for isolating and culturing vascular endothelial cells of rat thoracic aorta

  • Received:2011-02-18 Revised:2011-04-20 Online:2011-11-05 Published:2011-11-02
  • Contact: Jun-fa LI E-mail:junfali@ccmu.edu.cn

摘要: 摘要:目的 建立一种建议高效分离、培养大鼠胸主动脉血管内皮细胞的方法。方法 实验用健康雄性Wistar大鼠(200~250g),无菌条件下开胸并取胸主动脉,去除血管外膜,制备长约1.0~1.5mm动脉环。将血管环垂直置于干燥的培养皿中,并向血管环内加入含有10%胎牛血清的DMEM/ F12培养液、静止培养;24h血管环贴壁后,加入培养液;3~4d 内皮细胞长出,弃血管环,并经0.25%胰酶消化传代。应用形态学、免疫细胞化学及流式细胞分析等方法,鉴定血管内皮细胞标志物,即vWF的表达情况。结果 培养3~4d 时有细胞自主动脉环内迁移出并贴壁生长,细胞汇合后呈现典型的“铺路石”样内皮细胞特征;免疫组化和流式细胞分析结果示,vWF表达阳性率可高达( 98.3±0.2)%。结论 本实验采用改良的植块培养方法,不需要胶原及内皮细胞生长补充物,较传统酶消化法更为经济、高效,且简便易行,适用于细小血管内皮细胞的分离与培养。

关键词: 关键词:内皮细胞, 胸主动脉, 大鼠

Abstract: Abstract: Objective To establish a simple and efficient method for isolating and culturing vascular endothelial cells of rat thoracic aorta. Methods Under aseptic condition, the thoracic aorta was harvested from healthy male Wistar rat. After stripping off the adventitia, the thoracic aorta were cut into vessel rings with length of 1.0~1.5mm. The vessel rings were placed on culture dish vertically and filled with the culture medium DMEM/ F12 containing 10 % fetal bovine serum; After 24h, the vessel rings had attached on the culture dish firmly and some new culture medium were added; 3~4d later, the thoracic aorta was discarded and the new culture medium was added into the culture dish. The migrating cells were digested by 0.25 % pancreatic enzyme for serial subcultivation. The endothelial cells were identified by morphological, immunohistochemical and flow-cytometry methods with anti-vWF antibody, which was regarded as the marker of endothelial cells. Results A amount of cells migrated from the aorta and adhered to the bottom of culture dish 3~4d after cultivation. The confluent cells grew rapidly after being digested with 0.25% pancreatic enzyme and showed the typical cobblestone appearance. The cells were identified as endothelial cells, its positive ratio was (98.3±0.2)% by using immunostaining and flow-cytometry with vWF. Conclusion The modified explanting cultivation method for isolating and culturing was established in the this study. This method is simple, easy to handle and more economical and applicable as does not need collagen and endothelial cell growth promoting substrate. In addition, this modified method is especially suitable for isolation and cultivation of vascular endothelial cells from small arteries.

Key words: Key words: endothelial cells, thoracic aorta, rats