Metzger D A, Curtis S, Korach K S
Laboratory of Reproductive and Developmental Toxicology, National Institute of Environmental Health Sciences, National Institutes of Health, Research Triangle Park, North Carolina 27709.
Endocrinology. 1991 Apr;128(4):1785-91. doi: 10.1210/endo-128-4-1785.
Estradiol (E), diethylstilbestrol (DES), and three structurally similar DES derivatives and analogs, consisting of racemic mixtures of indenestrol-A (IA; rac), indenestrol-B (IB; rac), and the Z-isomer of pseudo-DES (PD) were used as probes to determine the effect of ligand on receptor-nuclear acceptor site interactions. IA (rac), IB (rac), and Z-PD have been previously shown to interact with the mouse uterine estrogen receptor with high affinity (Kd, approximately 1.5-2.2 x 10(-10) M), occupy similar levels of receptor in the nucleus in vivo, and have nuclear retention times similar to those of E and DES. However, in spite of these similarities, they differentially stimulate estrogenic responses that were previously thought to be interrelated and obligatory for full estrogenic action. In an attempt to elucidate the mechanism of differential stimulation of estrogen-regulated responses, the temporal pattern of KCl-resistant receptor sites was examined after a single injection of E, DES, IA (rac), IB (rac), Z-PD, or saline. Z-PD displayed lower levels of KCl-resistant receptor than the other compounds, whereas IA (rac) and IB (rac) had patterns similar to those of E and DES. In cell-free binding assays, all of the different receptor-ligand complexes were equally effective at competitively inhibiting the binding of receptor-[3H]E complexes to mouse uterine nuclear matrix with a Ki of 1.1 x 10(-10) M. Direct binding analysis showed no difference in the number of nuclear binding sites (range, 40.4-63.9 fmol/100 micrograms DNA) or Kd (range, 1.3-1.8 x 10(-10) M) among the different receptor-ligand complexes. Dissociation studies performed at 4 C showed no differences among the different complexes. In contrast, Z-PD-receptor complexes dissociated much faster from matrix sites at 22 C than any of the other complexes. Significant differences were noted in the proportion of complexes that were resistant to extraction with 0.6 M KCl. Forty-three percent of receptor-E complexes and 44% of receptor-DES complexes were resistant to KCl extraction, while 61% of receptor-IA and 29% of receptor-PD complexes were resistant to extraction, paralleling their activity in eliciting some estrogenic responses. In contrast, no difference was seen by gel shift assays in the ability of the ligand-receptor complexes to bind to a specific PS2 estrogen-responsive DNA sequence. These results demonstrate that the ligand may significantly affect the interaction of the estrogen receptor with nuclear acceptor sites.
雌二醇(E)、己烯雌酚(DES)以及三种结构相似的DES衍生物和类似物,由茚满雌酚-A(IA;外消旋体)、茚满雌酚-B(IB;外消旋体)的外消旋混合物以及伪己烯雌酚(PD)的Z-异构体组成,用作探针以确定配体对受体-核受体位点相互作用的影响。IA(外消旋体)、IB(外消旋体)和Z-PD先前已被证明能与小鼠子宫雌激素受体以高亲和力相互作用(解离常数Kd约为1.5 - 2.2×10⁻¹⁰ M),在体内细胞核中占据相似水平的受体,并且其核保留时间与E和DES相似。然而,尽管有这些相似之处,它们对雌激素反应的刺激存在差异,而这些反应先前被认为是相互关联且对充分的雌激素作用必不可少的。为了阐明雌激素调节反应差异刺激的机制,在单次注射E、DES、IA(外消旋体)、IB(外消旋体)、Z-PD或生理盐水后,检测了耐KCl受体位点的时间模式。Z-PD显示出比其他化合物更低水平的耐KCl受体,而IA(外消旋体)和IB(外消旋体)具有与E和DES相似的模式。在无细胞结合试验中,所有不同的受体-配体复合物在竞争性抑制受体-[³H]E复合物与小鼠子宫核基质的结合方面同样有效,解离常数Ki为1.1×10⁻¹⁰ M。直接结合分析表明,不同的受体-配体复合物之间核结合位点数量(范围为40.4 - 63.9 fmol/100μg DNA)或Kd(范围为1.3 - 1.8×10⁻¹⁰ M)没有差异。在4℃进行的解离研究表明不同复合物之间没有差异。相反,在22℃时,Z-PD-受体复合物从基质位点的解离速度比任何其他复合物都快得多。在用0.6 M KCl提取时,耐提取的复合物比例存在显著差异。43%的受体-E复合物和44%的受体-DES复合物耐KCl提取,而61%的受体-IA复合物和29%的受体-PD复合物耐提取,这与它们在引发某些雌激素反应中的活性平行。相比之下,通过凝胶迁移试验未发现配体-受体复合物与特定的PS2雌激素反应性DNA序列结合能力的差异。这些结果表明配体可能会显著影响雌激素受体与核受体位点的相互作用。
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