MiR-224-5p靶向沉默前蛋白转化酶枯草溶菌素9影响HepG2细胞脂质摄取与蓄积

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MiR-224-5p靶向沉默前蛋白转化酶枯草溶菌素9影响HepG2细胞脂质摄取与蓄积
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作者单位:(1.南华大学附属第一医院心内科,湖南省衡阳市 421001;2.岳阳市第二人民医院病理科,湖南省岳阳市 414000)
作者简介:何倩,硕士研究生,研究方向为心血管基础与临床,E-mail为570694833@qq.com。通信作者唐惠芳,博士,教授,硕士研究生导师,研究方向为心血管基础与临床,E-mail为1132226235@qq.com。
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MiR-224-5p affects lipid uptake and accumulation in HepG2 cells by targeting silence of proprotein convertase subtilisin/kexin type 9

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1.Department of Cardiology, the First Affiliated Hospital, University of South China, Hengyang, Hunan 421001, China;2.Department of Pathology, the Second People's Hospital of Yueyang, Yueyang, Hunan 414000, China)

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目的探讨miR-224-5p对前蛋白转化酶枯草溶菌素9(PCSK9)表达及对HepG2细胞摄脂能力的影响。方法运用生物信息学方法对miR-224-5p基因位置、保守性、种子序列进行分析。在Targetscan、miRanda、miRDB、RNAhybrid等多个数据库分析miR-224-5p与PCSK9结合位点及结合自由能。双荧光素酶报告基因验证miR-224-5p与PCSK9 mRNA 3′UTR直接靶向结合。Western blot检测miR-224-5p模拟物和miR-224-5p抑制剂对PCSK9和低密度脂蛋白受体(LDLR)蛋白的影响。细胞免疫荧光直接观察细胞膜上的LDLR。油红O染色和DiI-LDL分别观察miR-224-5p对HepG2细胞脂滴含量和脂质摄取能力的影响。结果生物信息学分析发现人的miR-224-5p基因定位于Xq28,不同物种间高度保守。miR-224-5p与PCSK9 mRNA 3′UTR存在靶向结合的基础,结合自由能较低。双荧光素酶报告基因显示,miR-224-5p模拟物能抑制PCSK9-WT 3′UTR荧光素酶活性,而对PCSK9-Mut 3′UTR没有抑制作用,表明PCSK9 mRNA 3′UTR是miR-224-5p的靶点。进一步实验发现miR-224-5p模拟物能够明显抑制PCSK9蛋白表达,增加LDLR蛋白含量。miR-224-5p下调后则表现为PCSK9表达增加,细胞LDLR水平降低。此外,油红O染色可见miR-224-5p模拟物组HepG2细胞内的脂滴明显减少,而miR-224-5p抑制剂组HepG2细胞内的脂滴明显增多。miR-224-5p高表达后明显促进HepG2细胞对LDLC的摄取。结论 miR-224-5p靶向结合PCSK9 mRNA 3′UTR,抑制PCSK9表达,进而降低HepG2细胞内脂滴含量,增加HepG2细胞对脂质的摄取。

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Aim To investigate the effect of miR-224-5p on the expression of proprotein convertase subtilisin/kexin type 9 (PCSK9) and the lipid uptake of HepG2 cells. Methods The position, conservativeness and seed sequence of miR-224-5p gene were analyzed by bioinformatics method. The binding sites and binding free energies of miR-224-5p to PCSK9 were analyzed in databases such as Targetscan, miRanda, miRDB and RNAhybrid. Direct targeted binding of miR-224-5p to PCSK9 mRNA 3′UTR was verified by double luciferase reporter gene. Western blot was used to detect the effects of miR-224-5p mimic and miR-224-5p inhibitor on PCSK9 and low density lipoprotein receptor (LDLR) proteins. LDLR on the cell membrane was directly observed with cellular immunofluorescence. Oil red O staining and DiI-LDL were respectively used to observe the effects of miR-224-5p on lipid droplet content and lipid uptake in HepG2 cells. Results Bioinformatics analysis revealed that the human miR-224-5p gene was located in Xq28 and highly conserved among different species. MiR-224-5p and PCSK9 mRNA 3′UTR had the basis of targeted binding, and the binding free energy was low. The double luciferase reporter gene assay showed that miR-224-5p mimic could inhibit the luciferase activity of PCSK9-WT 3′UTR, but not PCSK9-Mut 3′UTR, suggesting that the PCSK9 mRNA 3′UTR was the target of miR-224-5p. Further experiments showed that the miR-224-5p mimic could significantly inhibit the expression of PCSK9 protein and increase the content of LDLR protein. The expression of PCSK9 increased and the level of LDLR decreased after the down-regulation of miR-224-5p. In addition, oil red O staining showed that lipid droplets in HepG2 cells decreased significantly in the miR-224-5p mimic group, while lipid droplets in HepG2 cells increased significantly in the miR-224-5p inhibitor group. High expression of miR-224-5p significantly promoted LDLC uptake by HepG2 cells. Conclusion miR-224-5p targeting PCSK9 mRNA 3′UTR inhibits the expression of PCSK9, thereby reducing the content of lipid droplets in HepG2 cells and increasing the uptake of lipid by HepG2 cells.

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何倩,高亚,唐惠芳. MiR-224-5p靶向沉默前蛋白转化酶枯草溶菌素9影响HepG2细胞脂质摄取与蓄积[J].中国动脉硬化杂志,2019,27(5):401~409.

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收稿日期:2019-01-16
最后修改日期:2019-03-06
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在线发布日期: 2019-04-08

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