Zhang Ying-yi, Tian Wei-ping, Mei Mei
Zhongguo Ying Yong Sheng Li Xue Za Zhi. 2015 May;31(3):220-4.
To determine the interaction between miR-21 and DNA methylation in different breast cancer cells.
Fluorescence tagged miR-21 inhibitor and its negative control (NC) were transient transfected into MCF-7 and MDA-MB-231 cell, the transfection efficiency was observed using fluorescence microscopy, and the miR-21 expression level and genome DNA methylation status before and after transfection were assessed by real-time PCR and bisulfite-qMSP respectively. To investigate the regulation effect of DNA methylation on miR-21, cells were treated with 5-AZA (2.5 µmol/L) for 72 h, with dimethyl sulfoxide (DMSO) treatment as its negative control (NC), and the expression level of phosphatase and tensin homolog deleted on chromosome ten (PTEN) and AKT(also known as Protein Kinase B), two downstream genes of miR-21 were detected by Western blot.
The expression of miR-21 in MCF-7 cell was significantly knocked down (P < 0.01) by miR-21 inhibitor, with the genome DNA methylation level (P < 0.05) and all the three Dnmts: Dnmt1, Dnmt3a, and Dnmt3b unregulated. In contrast, the miR-21 expression in MDA-MB-231 cell was elevated ( P < 0.01) by miR-21 inhibitor, meanwhile, down- regulated of genome DNA methylation (P < 0.05) and Dnmt3b expression, upregulation of Dnmt3a were also observed. In addition, treated with 5-AZA resulted in significant increases of miR-21 expression in both MCF-7 and MDA-MB-231 cells (P < 0.01), with the protein level of PTEN increased in MCF-7 cell, which was further involved in the downregulation of AKT.
The regulation effects of DNA methylation by transient transfection of miR-21 in MCF-7 and MDA-MB-231 cells are almost opposite, whilst the expression of miR-21 in two cell lines were all upregulated by decreased DNA methylation level and our results may provide some experimental evidences for the future development of rational therapy for different breast cancer.
确定miR-21与不同乳腺癌细胞中DNA甲基化之间的相互作用。
将荧光标记的miR-21抑制剂及其阴性对照(NC)瞬时转染至MCF-7和MDA-MB-231细胞中,使用荧光显微镜观察转染效率,并分别通过实时PCR和亚硫酸氢盐-qMSP评估转染前后miR-21的表达水平和基因组DNA甲基化状态。为了研究DNA甲基化对miR-21的调控作用,用5-AZA(2.5 µmol/L)处理细胞72小时,以二甲基亚砜(DMSO)处理作为阴性对照(NC),并通过蛋白质免疫印迹法检测miR-21的两个下游基因,即第10号染色体缺失的磷酸酶和张力蛋白同源物(PTEN)以及AKT(也称为蛋白激酶B)的表达水平。
miR-21抑制剂显著降低了MCF-7细胞中miR-21的表达(P < 0.01),基因组DNA甲基化水平(P < 0.05)以及所有三种DNA甲基转移酶(Dnmt):Dnmt1、Dnmt3a和Dnmt3b均未受调控。相反,miR-21抑制剂使MDA-MB-231细胞中miR-21的表达升高(P < 0.01),同时观察到基因组DNA甲基化下调(P < 0.05)和Dnmt3b表达下调,Dnmt3a表达上调。此外,用5-AZA处理导致MCF-7和MDA-MB-231细胞中miR-21的表达均显著增加(P < 0.01),MCF-7细胞中PTEN的蛋白水平增加,这进一步参与了AKT的下调。
在MCF-7和MDA-MB-231细胞中,通过瞬时转染miR-21对DNA甲基化的调控作用几乎相反,而两种细胞系中miR-21的表达均因DNA甲基化水平降低而上调,我们的结果可能为未来不同乳腺癌合理治疗的发展提供一些实验证据。
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