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作 者:罗文娟[1] 许文林[1] 吕旭晶[1] 邱志远[1] 陈巧云[1] 王法春[1]
机构地区:[1]江苏大学附属人民医院中心实验室,江苏镇江212002
出 处:《江苏大学学报(医学版)》2008年第3期218-222,226,共6页Journal of Jiangsu University:Medicine Edition
基 金:江苏省卫生厅重大课题资助项目(K2005017)
摘 要:目的:观察多柔比星诱导K562细胞多药耐药基因-1(mdr1)基因表达过程中Y-盒结合蛋白1(YB-1)表达和核易位的变化情况,初步探讨YB-1蛋白对mdr1基因的转录调控。方法:多柔比星间歇性长期作用于K562细胞,剂量逐渐增加。RT-PCR检测mdr1,YB-1基因表达,流式细胞仪检测mdr1基因编码的P糖蛋白(P-gp)表达,蛋白质印迹检测YB-1蛋白核易位。通过RNA干扰技术使K562细胞中YB-1基因表达沉默,多柔比星处理YB-1基因沉默细胞,RT-PCR、流式细胞仪分别检测mdr1 mRNA和P-gp的表达。结果:经多柔比星作用后K562细胞mdr1基因转录上调,P-gp表达增加,同时YB-1基因转录也增强,且出现明显的核易位。YB-1基因沉默后,mdr1基因诱导性表达减少。结论:多柔比星诱导K562细胞mdr1基因表达的过程中,YB-1对于mdr1基因的转录活化起一定的作用。Objective: To investigate the effect of YB-1 on the transcription of mdrl gene. Methods: K562 cells were treated with doxorubicin (DOX) at different concentrations and times. Expression of mdrl and YB-1 genes were examined by reverse transcription-polymerase chain reaction (RT-PCR). P-glycoprotein (P-gp) was detected by flow cytometry. Cyto/nuclear protein was extracted for Western blotting to detect YB-1. To inhibit the expression of YB-1 gene in K562 cell using RNA interference (RNAi)targeting YB-1 gene, then detect the expression of mdrl and P-gp in YB-1 gene silenced cells after treated with DOX. Resuits: When K562 cells were exposured to DOX, the mdrl gene was highly expressed as well as its corresponding protein P-gp. Further, DOX up-regulated the expression of YB-1 gene, and promoted YB-1 protein translocate to nucleus. Another, when YB-1 gene was silenced, the expression of mdrl gene and P-gp were obviously decreased in K562 cells treated with DOX. Conclusion: Doxorubicin could induce the expression of mdrl gene in K562 cells, it may be due to YB-1 activating the transcription of mdrl gene.
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