Percoll公司
生物
肝星状细胞
分子生物学
台盼蓝
流式细胞术
CD8型
淋巴细胞
细胞
病理
生物化学
免疫学
抗原
离心
内分泌学
医学
作者
J. Gan,Canchingre Ji,Xiaorong Mao,Jintao Wang,Chengang Lyu,Yufang Shi,Yan Liao,Yonglin He,Liuping Shu,Ling Li,Jianfeng Li
出处
期刊:PubMed
[National Institutes of Health]
日期:2023-05-20
卷期号:31 (5): 532-537
标识
DOI:10.3760/cma.j.cn501113-20220827-00433
摘要
Objective: To explore a simple and feasible method for the isolation and purification of hepatocytes, hepatic stellate cells (HSC), and lymphocytes from mice. Methods: The cell suspension was obtained from male C57bl/6 mice by hepatic perfusion through the portal vein digestion method and then isolated and purified by discontinuous Percoll gradient centrifugation. Trypan blue exclusion was used to determine cell viability. Glycogen staining, cytokeratin 18, and transmission electron microscopy were used to identify hepatic cells. Immunofluorescence was used to detect α-smooth muscle actin combined with desmin in HSCs. Flow cytometry was used to analyze lymphocyte subsets in the liver. Results: After isolation and purification, about 2.7×10(7) hepatocytes, 5.7×10(5) HSCS, and 4.6×106 hepatic mononuclear cells were obtained from the liver of mice with a body weight of about 22g. The cell survival rate in each group was > 95%. Hepatocytes were apparent in glycogen deposited purple-red granules and cytokeratin 18. Electron microscopy showed that there were abundant organelles in hepatocytes and tight junctions between cells. HSC had expressed α-smooth muscle actin and desmin. Flow cytometry showed hepatic mononuclear cells, including lymphocyte subsets such as CD4, CD8, NKs, and NKTs. Conclusion: The hepatic perfusion through the portal vein digestion method can isolate multiple primary cells from the liver of mice at once and has the features of simplicity and efficiency.
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