Objective: To analyze the effect of DNA hypermethylation on NOR1 promoter activity and expression.Methods: NOR1 promoter plasmids were treated with SssI methyltransferase. The plasmids were modified by sodium bisulfite and purified. Sodium bisulfite-modified plasmids were subjected to PCR with primers designed to analyze the methylation status of 26 CpG sites in a 311-bp region of the NOR! promoter. Cells were transfected by methylated or mock-methylated promoter plasmids. The promoter activities were assessed by the luciferase levels of cell lysates or by directly observing GFP expression under fluorescence microscope. HL60 cells were treated with different concentrations of 5-aza-dC. Total RNA was isolated from harvested cells. Real-time RT-PCR was used to measure the expression level of NOR1 mRNA.Results: Bisulfite sequencing confirmed that SssI methyltransferase treatment successfully resulted in intensive hypermethylation of the NOR1 promoter plasmids. The promoter activity of NOR1 promoter plasmids was totally blocked by SssI methyltransferase treatment. NOR1 expression levels in HL60 cells were restored by 5-aza-dC treatment.Conclusion: NOR1 promoter plasmids are intensively hypermethylated by SssI methyltransferase treatment. The promoter activity of NOR1 promoter plasmids are totally blocked by SssI methyltransferase treatment. The 5-aza-dC treatment may restore the endogenous NOR1 mRNA level in HL60 cells.%目的:研究DNA甲基化对NOR1基因启动子活性和表达的影响.方法:采用SssI甲基转移酶处理NOR1基因启动子报告载体,经重亚硫酸钠修饰后测序检测报告载体甲基化水平.未经SssI处理和经SssI处理的NOR1基因启动子报告载体分别转染细胞,检测荧光素酶活性或GFP表达.采用去甲基化药物5-氮杂-2’-脱氧胞苷处理白血病细胞系HL60细胞,抽提RNA,Real-time RT-PCR检测NOR1 mRNA表达水平.结果:重亚硫酸钠测序表明SssI甲基转移酶体外处理导致NOR1启动子CpG岛CG位点完全甲基化.体外甲基化的NOR1启动子活性完全丧失.去甲基化药物5-氮杂-2' -脱氧胞苷连续处理3d后,白血病细胞系HL60细胞中内源性NOR1 mRNA表达水平显著增加.结论:SssI甲基转移酶可用于体外甲基化修饰NOR1基因启动子报告载体.甲基化修饰导致NOR1启动子活性丧失.去甲基化药物5-氮杂-2’-脱氧胞苷处理恢复NOR1 mRNA表达.
展开▼
