摘要
目的通过表观遗传学干预,研究p33ING1b启动子甲基化和组蛋白乙酰化状态、基因和蛋白的表达及其细胞增殖能力的改变,探讨结直肠癌中p33ING1b转录抑制的表观遗传机制。方法通过曲古抑菌素A及5-氮-2′-脱氧胞苷,对结直肠癌细胞株HT29、LOVO、HCT116和COLO205行恢复乙酰化和去甲基化干预,分单独用药组和联合用药组。RT-PCR结合Real-time qPCR方法检测其p33ING1bmRNA表达的变化,nMSP法分析其p33ING1b启动子甲基化状态的改变,ChIP法检测其p33ING1b乙酰化状态的改变,蛋白质印迹法检测p33ING1b蛋白的表达,MTT法检测细胞的增殖能力。结果曲古抑菌素A及5-氮-2′-脱氧胞苷可逆转结直肠癌细胞株的甲基化及乙酰化状况。2种药物干预后,4种结直肠癌细胞株各组间p33ING1bmRNA表达,差异有统计学意义,HCT116:F=1 690.446,P<0.001;HT29:F=284.474,P<0.001;LOVO:F=2 930.284,P<0.001;COLO205:F=33.540,P<0.001;p33ING1bmRNA蛋白表达差异有统计学意义,HCT116:F=32.606,P<0.001;HT29:F=33.422,P<0.001;LOVO:F=13.975,P<0.01;COLO205:F=7.119,P<0.05,细胞增殖能力差异有统计学意义,HCT116:F=7.327,P<0.05;HT29:F=17.642,P<0.001;LOVO:F=7.035,P<0.05;COLO205:F=9.008,P<0.01。联合使用两种药物对p33ING1bmRNA的表达具有协同作用。结论 p33ING1b基因甲基化和去乙酰化可抑制抑癌基因p33ING1b转录,使用甲基化抑制剂及去乙酰化抑制剂可逆转这一效应,且两者具有协同作用,这为表观基因治疗提供了新的思路。
OBJECTIVE To investigate the epigenetic mechanism of the p33iN1b transcription inhibition through epi- genetic intervention and analyze the change of epigenetic pattern, genetic expression in p33INGlb promoter,protein expres- sion of p33ING1b and proliferation of colorectal cancer cells. METHODS Colorectal cancer cell lines were cultured in vitro and divided into four groups:control group treated without any drug, and the other three experimental groups treated with TSA(TSA group), 5-Aza-2'-dc (Aza group), 5-Aza-2'-dc + TSA(Aza+ TSA group) separately. The expressions of p33IN6~b mRNA were detected by real-time quantitative RT-PCR. The patterns of p33~N^IB promoter methylation were ana- lyzed by nMSP. Acetylation levels of p33INGIB fragment 1 and 2 were estimated by CHIP. p33ING1b protein expression was detected by Western Blot. The biological behaviors of the colorectal cancer cells were investigated by MTT. RESULTS TSA and 5-Aza-2Cdc can rerevse methglation and acetylation status of the colorectal cancer lines. After the intervention of TSA and 5-Aza-2Cdc,the differences of p33ING1bmRNA expression in four cell lines were significant(HCTl16:F= 1 690. 446, P〈 0. 001 ; HT29 : F= 284. 474,P〈0. 001 ; LOVO: F= 2 930. 284,P〈0. 001 ; COLO205 : F= 33. 540, P〈0. 001) ; The differences of p33tNc^b mRNA protein expression were significant ( HCT116 : F= 32. 606, P〈 0. 001 ; HT29 : F = 33. 422, P〈0. 001 ; LOVO: F = 13.975, P〈0. 01 ; COLO205 : F= 7. 119, P〈 0.05 ). The proliferation of colorectal cancer ceils were significant ( HCT116 : F = 7. 327, P〈0. 05 ; HT29 : F = 17. 642, P〈 0. 001 ; LOVO: F = 7. 035, P〈 0. 05 ; COLO205 : F = 9. 008, P〈0. 01 ). There was a synergistic effect with the combination of the two drugs. CONCLUSIONS Methylation and deacetylation inhibit the transcription of p33INGlb , 5-Aza-2'-dc and TSA can reverse the efficacy and exhibite obvious synergistic effect. It will provide a novel approach to epigenetic therapy.
出处
《中华肿瘤防治杂志》
CAS
北大核心
2015年第2期81-85,90,共6页
Chinese Journal of Cancer Prevention and Treatment
基金
国家自然科学基金(30760246)
