文章摘要
马静波 霍静 张松 丁美玲 聂勇战.SIRT1 过表达慢病毒稳转细胞系的构建及其对脂肪合成的影响[J].,2014,14(9):1616-1621
SIRT1 过表达慢病毒稳转细胞系的构建及其对脂肪合成的影响
Construction of Stable Transfected Cell Line of SIRT1 OverexpressionLentiviral and Its Effect on Fat Synthesis
  
DOI:
中文关键词: 油红O  BODIPY  SIRT1  慢病毒  高内涵监测系统
英文关键词: Oil red O  BODIPY  SIRT1  Lentiviral  High Content Analysis
基金项目:科技部重大国际合作项目(81110200):肝脏脂质代谢障碍中SIRT1 相关分子的组学研究
作者单位
马静波 霍静 张松 丁美玲 聂勇战 第四军医大学西京消化病医院肿瘤生物学国家重点实验室 
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中文摘要:
      目的:通过油红O 及BODIPY染色选取脂肪代谢理想的细胞模型,并运用高内涵仪器检测SIRT1 高表达细胞系中脂肪的 变化。方法:在L-02、HepG2、Huh7 细胞中进行油红O 和BODIPY 染色,观察在不同油酸浓度下脂滴的生成情况;将构建成功的 SIRT1 过表达慢病毒载体GV166-SIRT1 及空载体病毒GV166-Control 感染L-02 细胞,qPCR 及Western-Blot 检测感染细胞中 SIRT1 的表达水平;高内涵系统检测L-02 SIRT1 和L-02 control细胞系产生的脂滴荧光强度,以确定油酸诱导的最佳浓度及最佳 刺激时间。结果:通过油红O 及BODIPY染色发现L-02 细胞更适宜作为脂肪代谢的细胞模型;成功构建SIRT1 过表达慢病毒载 体GV166-SIRT1 及空载体病毒GV166-Control,qPCR 及Western-Blot检测显示转染病毒后SIRT1 在细胞中的表达水平明显升 高;在油酸刺激浓度0.4mM、诱导时间12h 时,L-02 SIRT1细胞中脂滴的荧光强度明显较L-02 control 为低,且这种差异达到最大 化。结论:成功建立SIRT1过表达稳定转染细胞系,并证明高表达SIRT1 能够抑制脂肪合成。
英文摘要:
      Objective:To select a suitable cell model of fatty metabolism by oil red O staining and Bodipy staining, and detect the changes of adipose in SIRT1 overexpression cell lines by High Content Analysis.Methods:The lipid droplets generation of HepG2, Huh7 and L-02 cell lines was observed by using oil red O staining and Bodipy staining under different oleic acid stimulation concentrations; SIRT1 overexpression lentiviral vector GV166-SIRT1 and control lentiviral vector GV166-Control was constructed to infect L-02 cell line, and the expression levels of SIRT1 within infected the cells were detected by qPCR and Western-Blot ; High Content Analysis was performed to detect the fluorescence intensity of lipid droplets within L-02 SIRT1 and L-02 control cell lines in order to determine the optimal concentration of oleic acid-induced stimulation and the best time.Results:By oil red O and bodipy staining, it was found that L-02 was more suitable for a cell model of liver lipid metabolism. Lentiviral vectors GV166-SIRT1 and GV166-Control were confirmed to be successfully constructed and SIRT1 overexpression lentiviral vector was proven to be capable of raising significantly the SIRT1 expression level within the L-02 cells by qPCR and Western-Blot. When the concentration of oleic acid was 0.4mM and the treatment duration was 12h, the fluorescence intensity in L-02-sirt1 group was significantly lower than that in L-02-control group, while the difference in fluorescence intensity between the L-02-sirt1 L-02-control was largest.Conclusion:The SIRT1 overexpressing stably transfected cell lines were successful established and overexpression SIRT1 can inhibit fat synthesis.
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