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首页> 外文期刊>The Prostate >DNA methylation in the androgen receptor gene promoter region in rat prostate cancers.
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DNA methylation in the androgen receptor gene promoter region in rat prostate cancers.

机译:大鼠前列腺癌中雄激素受体基因启动子区域的DNA甲基化。

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BACKGROUNDInvasive adenocarcinomas developing in the rat dorsolateral prostate on combined treatment with 3,2'-dimethyl-4-aminobiphenyl (DMAB) and testosterone propionate (TP) are biologically androgen-independent and lacking androgen receptor protein (AR) expression. The present study was conducted to assess the mechanisms underlying this loss of AR expression in rat prostate cancer.METHODSThe methylation status of the AR gene promoter region in rat prostate cancer and cell lines (PLS10, 20, and 30) was examined by Southern blotting, methylation-specific polymerase chain reaction, and methylation-sensitive single-strand conformation analysis (MS-SSCA).RESULTSAR mRNA expression was not detected in any of the rat prostate cancers or cancer cell lines tested by Northern blot analysis. Higher levels of methylated CpGs were observed in PLS20 than PLS10 or 30. Demethylation treatment by 5-aza-2'-deoxycytidine restored AR mRNA expression in PLS20. The CpGs suggested to be responsible for AR expression in rat prostate cancer were found to be located -9 and -1 nucleotides upstream of the transcriptional initiation site. All of the examined rat prostate and seminal vesicle cancers demonstrated hypermethylation at these CpG sites.CONCLUSIONSThese data clearly demonstrate that aberrant hypermethylation in the AR promoter region may play a critical role in AR expression in rat prostate cancers. Prostate 52: 82-88, 2002.
机译:背景技术与3,2'-二甲基-4-氨基联苯(DMAB)和丙酸睾丸酮(TP)联合治疗在大鼠背外侧前列腺中发展的浸润性腺癌在生物学上不依赖雄激素并且缺乏雄激素受体蛋白(AR)表达。本研究旨在评估大鼠前列腺癌中AR表达缺失的机制。方法通过Southern印迹法检测大鼠前列腺癌和细胞系(PLS10、20和30)中AR基因启动子区域的甲基化状态,甲基化特异性聚合酶链反应和甲基化敏感的单链构象分析(MS-SSCA)。在通过Northern blot分析测试的任何大鼠前列腺癌或癌细胞系中均未检测到RESULTSAR mRNA表达。在PLS20中观察到的甲基化CpGs水平高于PLS10或30。通过5-氮杂2'-脱氧胞苷进行的脱甲基处理恢复了PLS20中AR mRNA的表达。发现负责大鼠前列腺癌中AR表达的CpG位于转录起始位点上游的-9和-1核苷酸。所有检查的大鼠前列腺癌和精囊癌在这些CpG位点均显示出高甲基化。结论这些数据清楚地表明,AR启动子区域异常的甲基化可能在大鼠前列腺癌的AR表达中起关键作用。前列腺52:82-88,2002年。

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