小鼠肝星状细胞分离纯化和体外培养模型的建立

目的 建立小鼠肝星状细胞(m-HSCs)分离纯化的高效稳定方案,并通过原代和传代培养观察其生物学特性.方法 依次应用预灌注液、0.1% Pronase E、0.075% Collagenase NB4G对在体肝脏原位灌注消化.肝脏离体后,在0.02%DNaseI液中磁力搅拌消化10 min,低速离心(25g,5 min)去除残余肝实质细胞,进一步用Optiprep密度梯度液获得纯化的m-HSCs.采用锥虫蓝染色法评估细胞产量及活力;采用自发荧光及油红O染色鉴定细胞纯度;采用光镜、电镜以及Desmin/α-SMA免疫荧光双染色观察细胞形态和生物学特征.结果 分离得到的原代m-HSCs数量为(1.4±0.3)×106/g肝脏,细胞活率＞95%;原代培养24 b后,细胞纯度＞90%,传1代后细胞纯度接近100%.静止期和不同活化阶段的m-HSCs在亚显微结构以及α-SMA表达强度等方面存在差异.结论 建立的m-HSCs分离和纯化方法及体外细胞培养模型具有稳定性和高纯度性及高活率性.

Abstract：

Objective To establish a high-performance and stable model for isolation and purification of mouse hepatic stellate cells, and investigate their biological phenotypes by primary culture and subculture. Methods The liver was digested by in situ perfusion of pre-perfusion solution, 0.1% pronase E and 0.075% collagenase NB4G in turn. The liver was continued to digest using 0.02% DNase Ⅰ liquid with magnetic stirring for 10 min in vitro. After low-speed centrifugation used to remove residual hepatocytes, cells were treated with Optiprep density gradient solution to obtain the purified m-HSCs. Trypan blue staining method was used to calculate cell production and viability. The cell purity was identified by mHSCs autofluorescence and oil red O staining. Light microscopy, electronic transmission microscopy and double immunofluorescence staining of Desmin and α-SMA were done to observe morphological characteristics and biological phenotypes of m-HSCs. Results The yeild rate of m-HSCs was (1.4±0.3)×106/g of liver tissue, the cell viability was more than 95%, the cell purity was more than 90% after 24 h of primary cluture and close to 100% after the first cell passage. The activated m-HSCs had different characteristics of submicroscopic structures and expression level of α-SMA. Conclusion This study established a stable model for isolation, purification and culture of m-HSCs, which obtained the high purity and high-living rate of m-HSCs.

Establishment of isolation and culture model of mouse hepatic stellate cells

Objective To establish a high-performance and stable model for isolation and purification of mouse hepatic stellate cells, and investigate their biological phenotypes by primary culture and subculture. Methods The liver was digested by in situ perfusion of pre-perfusion solution, 0.1% pronase E and 0.075% collagenase NB4G in turn. The liver was continued to digest using 0.02% DNase Ⅰ liquid with magnetic stirring for 10 min in vitro. After low-speed centrifugation used to remove residual hepatocytes, cells were treated with Optiprep density gradient solution to obtain the purified m-HSCs. Trypan blue staining method was used to calculate cell production and viability. The cell purity was identified by mHSCs autofluorescence and oil red O staining. Light microscopy, electronic transmission microscopy and double immunofluorescence staining of Desmin and α-SMA were done to observe morphological characteristics and biological phenotypes of m-HSCs. Results The yeild rate of m-HSCs was (1.4±0.3)×106/g of liver tissue, the cell viability was more than 95%, the cell purity was more than 90% after 24 h of primary cluture and close to 100% after the first cell passage. The activated m-HSCs had different characteristics of submicroscopic structures and expression level of α-SMA. Conclusion This study established a stable model for isolation, purification and culture of m-HSCs, which obtained the high purity and high-living rate of m-HSCs.