Chen Theresa L, Shen Wen-Jun, Qiu Xin-Wen, Li Tao, Hoffman Andrew R, Kraemer Fredric B
Veterans Affairs, Palo Alto Health Care System, Palo Alto, CA 94304, USA.
Stem Cells Dev. 2007 Jun;16(3):371-80. doi: 10.1089/scd.2006.0037.
Here we show a simplified and improved method to produce large quantities of evenly distributed monolayer cultures that display major characteristics of adipocytes. These cultures are applicable for quantitative analysis for biochemical and molecular events in adipogenesis during development and may provide a useful system for high-throughput drug screening assays of antiobesity drugs. In our method, we treated embryoid bodies (EBs) with all-trans retinoic acid (ATRA) for 3 days, 1 day after they attached to the gelatin-coated culture plates without further transfer. The cells were maintained in insulin and trioiodothyronine (T(3))-containing medium until day 12, when they were dispersed by enzymatic digestion and replated onto multiple culture plates. Two days later, adipocyte induction factors were added for 6 days and examined 6 days later. The amount of lipid droplet-laden adipocytes in the culture reached approximately 80%, with a nearly five-fold increase in GPDH activity. The cells expressed high levels of adipose-specific proteins (adipocyte markers), including PPARgamma2, ALBP, LPL, HSL, perilipin, and DGAT1. The adipocytes are functionally active, as evidenced by their response to lipolytic agents, such as forskolin, Bt2-cAMP, and isoproterenol, with more than 20-fold increases in glycerol release.
在此,我们展示了一种简化且改进的方法,用于大量生产具有脂肪细胞主要特征的均匀分布的单层培养物。这些培养物适用于对发育过程中脂肪生成的生化和分子事件进行定量分析,并且可能为抗肥胖药物的高通量药物筛选试验提供一个有用的系统。在我们的方法中,我们在胚状体(EBs)附着于明胶包被的培养板1天后,用全反式维甲酸(ATRA)处理3天,无需进一步传代。细胞在含胰岛素和三碘甲状腺原氨酸(T(3))的培养基中培养至第12天,此时通过酶消化将其分散并重新接种到多个培养板上。两天后,添加脂肪细胞诱导因子6天,并在6天后进行检测。培养物中充满脂滴的脂肪细胞数量达到约80%,甘油磷酸脱氢酶(GPDH)活性增加近五倍。细胞表达高水平的脂肪特异性蛋白(脂肪细胞标志物),包括过氧化物酶体增殖物激活受体γ2(PPARγ2)、脂肪酸结合蛋白(ALBP)、脂蛋白脂肪酶(LPL)、激素敏感性脂肪酶(HSL)、围脂滴蛋白和二酰甘油酰基转移酶1(DGAT1)。这些脂肪细胞功能活跃,对脂解剂如福斯高林、Bt2 - cAMP和异丙肾上腺素的反应证明了这一点,甘油释放增加超过20倍。
