Mao Chengjian, Patterson Nicole M, Cherian Milu T, Aninye Irene O, Zhang Chen, Montoya Jamie Bonéy, Cheng Jingwei, Putt Karson S, Hergenrother Paul J, Wilson Elizabeth M, Nardulli Ann M, Nordeen Steven K, Shapiro David J
Department of Biochemistry, and Chemistry, University of Illinois, Urbana, Illinois 61810-3602, USA.
J Biol Chem. 2008 May 9;283(19):12819-30. doi: 10.1074/jbc.M709936200. Epub 2008 Mar 12.
Estrogen receptor alpha (ERalpha) plays an important role in several human cancers. Most current ERalpha antagonists bind in the receptor ligand binding pocket and compete for binding with estrogenic ligands. Instead of the traditional approach of targeting estrogen binding to ER, we describe a strategy using a high throughput fluorescence anisotropy microplate assay to identify small molecule inhibitors of ERalpha binding to consensus estrogen response element (cERE) DNA. We identified small molecule inhibitors of ERalpha binding to the fluorescein-labeled (fl)cERE and evaluated their specificity, potency, and efficacy. One small molecule, theophylline, 8-[(benzylthio)methyl]-(7CI,8CI) (TPBM), inhibited ERalpha binding to the flcERE (IC(50) approximately 3 microm) and inhibited ERalpha-mediated transcription of a stably transfected ERE-containing reporter gene. Inhibition by TPBM was ER-specific, because progesterone and glucocorticoid receptor transcriptional activity were not significantly inhibited. In tamoxifen-resistant breast cancer cells that overexpress ERalpha, TPBM inhibited 17beta-estradiol (E(2))-ERalpha (IC(50) 9 microm) and 4-hydroxytamoxifen-ERalpha-mediated gene expression. Chromatin immunoprecipitation showed TPBM reduced E(2).ERalpha recruitment to an endogenous estrogen-responsive gene. TPBM inhibited E(2)-dependent growth of ERalpha-positive cancer cells (IC(50) of 5 microm). TPBM is not toxic to cells and does not affect estrogen-independent cell growth. TPBM acts outside of the ER ligand binding pocket, does not act by chelating the zinc in ER zinc fingers, and differs from known ERalpha inhibitors. Using a simple high throughput screen for inhibitors of ERalpha binding to the cERE, a small molecule inhibitor has been identified that selectively inhibits ERalpha-mediated gene expression and estrogen-dependent growth of cancer cells.
雌激素受体α(ERα)在多种人类癌症中发挥重要作用。目前大多数ERα拮抗剂结合于受体配体结合口袋,并与雌激素配体竞争结合。我们描述了一种策略,与传统的针对雌激素与ER结合的方法不同,该策略使用高通量荧光各向异性微孔板分析法来鉴定ERα与共有雌激素反应元件(cERE)DNA结合的小分子抑制剂。我们鉴定出了ERα与荧光素标记的(fl)cERE结合的小分子抑制剂,并评估了它们的特异性、效力和功效。一种小分子,即8 - [(苄硫基)甲基] - 茶碱(7CI,8CI)(TPBM),抑制ERα与flcERE的结合(半数抑制浓度(IC50)约为3 μM),并抑制ERα介导的稳定转染的含ERE报告基因的转录。TPBM的抑制作用具有ER特异性,因为孕酮和糖皮质激素受体的转录活性未受到显著抑制。在过表达ERα的他莫昔芬耐药乳腺癌细胞中,TPBM抑制17β - 雌二醇(E2) - ERα(IC50为9 μM)和4 - 羟基他莫昔芬 - ERα介导的基因表达。染色质免疫沉淀显示TPBM减少了E2.ERα对内源雌激素反应基因的募集。TPBM抑制ERα阳性癌细胞的E2依赖性生长(IC50为5 μM)。TPBM对细胞无毒,且不影响雌激素非依赖性细胞生长。TPBM作用于ER配体结合口袋之外,不是通过螯合ER锌指中的锌起作用,并且不同于已知的ERα抑制剂。通过对ERα与cERE结合抑制剂进行简单的高通量筛选,已鉴定出一种小分子抑制剂,其可选择性抑制ERα介导的基因表达以及癌细胞的雌激素依赖性生长。
