文章摘要
丁美玲 冯文强 张 松 曹海超 聂勇战.RNA 特异腺苷脱氨酶 1( p150 亚型)抑制肝细胞脂质合成[J].,2015,15(5):829-833
RNA 特异腺苷脱氨酶 1( p150 亚型)抑制肝细胞脂质合成
RNA-specific Adenosine Deaminase 1 p150 Isoform Inhibits Lipid Synthesisin Hepatocytes
  
DOI:
中文关键词: ADAR1 -p150  脂质合成  高内 涵筛选系统
英文关键词: ADAR1 -p150  Lipid synthesis  High content screening system
基金项目:科技部重大国际合作项目( 811 10200)
作者单位
丁美玲 冯文强 张 松 曹海超 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 
摘要点击次数: 1077
全文下载次数: 1114
中文摘要:
      目 的: 在油酸诱导的肝细胞脂肪变模型中,检测 RNA 特异腺苷脱氨酶 1 p1 50亚型( ADAR1-p1 50)高表达细胞系中脂肪合成 的变化。方法: 利用 本课题组前期摸索的油酸刺激人胚胎肝细胞 L-02 细胞系脂肪变的条件, qRT-PCR 和 Western-Blot 检测油酸刺 激组和对照 组 ADAR1 -p150表达变 化; 将构 建成功 的 ADAR1 -p150过表达慢病毒载体 GV166-ADAR1 -p150及空 载体病毒 GV166-control 感染 L-02 细胞, 检测感染细胞中 ADAR1 -p150的 mRNA 和蛋白 表达水平; 通过油红 O 染色和 BODIPY 染色观察 L-02 ADAR1-p150和 L-02 control 细胞中脂滴形成, 并进一步利用 高内 涵系统检测其荧光强度,对脂滴合成作定量分析。 结果: L-02 细胞在 油酸刺 激 后 ADAR1 -p150 的 mRNA 和蛋白 水平 降低;成 功 构建 ADAR1 -p150 过表达 慢 病毒载体 GV166- ADAR1 -p150及空 载体病毒 GV1 66-control, qRT-PCR 及 Western-Blot 检测 显示病毒转染 GV1 66- ADAR1 -p1 50后 ADAR1 -p150 在细胞中的表达水平显著升高;油红 O 染色和 BODIPY 染色发现 L-02 ADAR1 -p150较 L-02 control 细胞胞质中脂滴数量减少。 高 内 涵筛选系统检测提示 L-02 ADAR1-p1 50组中脂滴的荧光强度明显较 L-02 control 组低。 结论: 成功构建 ADAR1-p1 50过表达稳 定转染 L-02 细胞系, 并证实高表达 ADAR1 -p150能够抑制脂肪合成。
英文摘要:
      Objective:To investigate the regulatory effect of RNA-specific adenosine deaminase 1 p150 isoform (ADAR1 -p150) on fat synthesis in oleic acid-induced hepatic steatosis cell model.Methods:Oleic acid stimulated steatosis model in human embryonic liver cell line L-02 cells was constructed according to our previously reported protocols. ADAR1 -p150 expression was analyzed by qRT-PCR and Western-Blot in both control group and oleic acid (OA) group. ADAR1-p1 50 overexpression lentiviral vector GV166-ADAR1 -p150 and control lentiviral vector GV166-control were constructed to infect L-02 cell line, the mRNA and protein expression levels of ADAR1 -p150 were detected by qRT-PCR and Western-Blot. The lipid droplets formation of L-02 ADAR1 -p150 and L-02 control cell lines was observed by oil red O staining and BODIPY staining. High Content Screening system was performed to detect the average fluorescence intensity of lipid droplets.Results:The mRNA and protein expression levels of ADAR1-p1 50 were down-regulated in OA group as compared with that in control group. ADAR1-p1 50 overexpression lentiviral vector GV1 66- ADAR1 -p150 and empty vector virus GV166-control were successfully constructed. qRT-PCR and Western-Blot analysis showed that ADAR1 -p150 expression significantly increased in GV166- ADAR1 -p150 treated cells. Oil Red O staining and BODIPY staining revealed that the number of lipid droplets in L-02 ADAR1 -p150 cells was less than that in L-02 control cells. High content screening system demonstrated that the lipid droplets fluorescence intensity of L-02 ADAR1-p1 50 cells was significantly lower than that of L-02 control cells.Conclusion:Stable ADAR1 -p150 overexpressing cell line was successfully established. More importantly, high expression of ADAR1-p1 50 was capable of inhibiting fat synthesis in L-02 cells.
查看全文   查看/发表评论  下载PDF阅读器
关闭