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Characterization and enrichment of hepatic progenitor cells in adult rat liver

机译:成年大鼠肝脏中肝祖细胞的表征和富集

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AIM: To detect the markers of oval cells in adult rat liver and to enrich them for further analysis of characterization in vitro. METHODS: Rat model for hepatic oval cell proliferation was established with 2-acetylaminofluorene and two third partial hepatectomy (2-AAF/PH). Paraffin embedded rat liver sections from model (11 d after hepatectomy) and control groups were stained with HE and OV6, cytokeratin19 (CK19), albumin, alpha fetoprotein (AFP), connexin43, and c-kit antibodies by immunohistochemistry. Oval cell proliferation was measured with BrdU incorporation test. C-kit positive oval cells were enriched by using magnetic activated cell sorting (MACS) The sorted oval cells were cultured in a low density to observe colony formation and to examine their characterization in vitro by immunocytochemistry and RT-PCR. RESULTS: A 2-AAF/PH model was successfully established to activate the oval cell compartment in rat liver. BrdU incorporation test of oval cell was positive. The hepatic oval cells coexpressed oval cell specific marker OV6, hepatocyte-marker albumin and cholangiocyte-marker CK19. They also expressed AFP and connexin 43. C-kit, one hematopoietic stem cell receptor, was expressed in hepatic oval cells at high levels. By using c-kit antibody in conjunction with MACS, we developed a rapid oval cell isolation protocol. The sorted cells formed colony when cultured in vitro. Cells in the colony expressed albumin or CK19 or coexpressed both and BrdU incorporation test was positive. RT-PCR on colony showed expression of albumin and CK19 gene. CONCLUSION: Hepatic oval cells in the 2-AAF/PH model had the properties of hepatic stem/progenitor cells. Using MACS, we established a method to isolate oval cells. The sorted hepatic oval cells can form colony in vitro which expresses different combinations of phenotypic markers and genes from both hepatocytes and cholangiocyte lineage.
机译:目的:检测成年大鼠肝脏中卵圆细胞的标志物,并对其进行富集,以进一步进行体外特征分析。方法:用2-乙酰氨基芴和二分之三肝切除术(2-AAF / PH)建立大鼠肝卵圆细胞增殖模型。通过免疫组织化学,用HE和OV6,细胞角蛋白19(CK19),白蛋白,甲胎蛋白(AFP),连接蛋白43和c-kit抗体对来自模型(肝切除术后11天)和对照组的石蜡包埋的大鼠肝脏切片进行染色。用BrdU掺入测试测量卵形细胞的增殖。通过使用磁激活细胞分选术(MACS)富集C-kit阳性椭圆形细胞。将分选的椭圆形细胞以低密度培养,以观察菌落形成并通过免疫细胞化学和RT-PCR体外检查其特征。结果:成功建立了2-AAF / PH模型以激活大鼠肝脏的卵圆细胞室。卵圆细胞BrdU掺入试验阳性。肝卵圆形细胞共表达卵圆形细胞特异性标记OV6,肝细胞标记白蛋白和胆管细胞标记CK19。他们还表达了AFP和连接蛋白43。C-kit是一种造血干细胞受体,在肝卵圆形细胞中高水平表达。通过将c-kit抗体与MACS结合使用,我们开发了一种快速的椭圆形细胞分离方案。体外培养时,分选的细胞形成菌落。菌落中的细胞表达白蛋白或CK19或两者共表达,且BrdU掺入试验为阳性。菌落RT-PCR显示白蛋白和CK19基因表达。结论:2-AAF / PH模型中的肝卵圆形细胞具有肝干/祖细胞的特性。使用MACS,我们建立了一种分离椭圆形细胞的方法。分选的肝卵圆形细胞可以在体外形成集落,其表达来自肝细胞和胆管细胞谱系的表型标记和基因的不同组合。

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