Differences in the form of the salt-transformed estrogen receptor when bound by estrogen versus antiestrogen

Journal of steroid biochemistry Pub Date : 1990-08-28 DOI:10.1016/0022-4731(90)90166-P

Mary F. Ruh, Jane W. Turner, Christine M. Paulson, Thomas S. Ruh

{"title":"Differences in the form of the salt-transformed estrogen receptor when bound by estrogen versus antiestrogen","authors":"Mary F. Ruh, Jane W. Turner, Christine M. Paulson, Thomas S. Ruh","doi":"10.1016/0022-4731(90)90166-P","DOIUrl":null,"url":null,"abstract":"<div><p>Our laboratory has previously reported that antiestrogen binding to molybdate-stabilized non-transformed estrogen receptor results in a larger form of the receptor in 0.3 M KCl when compared with estrogen bound receptor. Estradiol promoted the formation of monomers in the presence of 0.3 M KC1 whereas antiestrogen appeared to promote dimer formation. We have extended these studies examining the rabbit uterine salt-transformed estrogen receptor partially purified by DEAE-cellulose chromatography. We previously demonstrated that estrogen receptor prepared in this way bound to different sites on partially deproteinized chromatin subfractions or reconstituted chromosomal protein/DNA fractions when the receptor was complexed with estrogen vs antiestrogen. Analysis of these receptor preparations indicated that DEAE-cellulose step-elution resulted in a peak fraction which sedimented as a single 5.9S peak in 5–20% sucrose density gradients containing 0.3 M KCl for receptor bound by the antiestrogens H1285 and <em>trans</em>-hydroxytamoxifen. However, receptor bound by estradiol sedimented as 4.5S. These receptor complexes bound DNA-cellulose indicating that these partially purified receptors were transformed. DEAE rechromatography or agarose gel filtration of the partially purified antiestrogen-receptor complexes resulted in significant dissociation of the larger complex into monomers. Incubations of 5.9S antiestrogen-receptor complexes with antibodies against nontransformed steroid receptor-associated proteins (the 59 and 90 kDa proteins) did not result in the interaction of this larger antiestrogen-receptor complex with these antibodies (obtained from L.E. Faber and D.O. Toft, respectively). Our results support the concept that antiestrogen binding induces a different receptor conformation which could affect monomer-dimer equilibrium, thus rendering the antiestrogen-receptor complex incapable of inducing complete estrogenic responses in target tissues.</p></div>","PeriodicalId":17138,"journal":{"name":"Journal of steroid biochemistry","volume":null,"pages":null},"PeriodicalIF":0.0000,"publicationDate":"1990-08-28","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://sci-hub-pdf.com/10.1016/0022-4731(90)90166-P","citationCount":"18","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"Journal of steroid biochemistry","FirstCategoryId":"1085","ListUrlMain":"https://www.sciencedirect.com/science/article/pii/002247319090166P","RegionNum":0,"RegionCategory":null,"ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"","JCRName":"","Score":null,"Total":0}

引用次数: 18

Abstract

Our laboratory has previously reported that antiestrogen binding to molybdate-stabilized non-transformed estrogen receptor results in a larger form of the receptor in 0.3 M KCl when compared with estrogen bound receptor. Estradiol promoted the formation of monomers in the presence of 0.3 M KC1 whereas antiestrogen appeared to promote dimer formation. We have extended these studies examining the rabbit uterine salt-transformed estrogen receptor partially purified by DEAE-cellulose chromatography. We previously demonstrated that estrogen receptor prepared in this way bound to different sites on partially deproteinized chromatin subfractions or reconstituted chromosomal protein/DNA fractions when the receptor was complexed with estrogen vs antiestrogen. Analysis of these receptor preparations indicated that DEAE-cellulose step-elution resulted in a peak fraction which sedimented as a single 5.9S peak in 5–20% sucrose density gradients containing 0.3 M KCl for receptor bound by the antiestrogens H1285 and trans-hydroxytamoxifen. However, receptor bound by estradiol sedimented as 4.5S. These receptor complexes bound DNA-cellulose indicating that these partially purified receptors were transformed. DEAE rechromatography or agarose gel filtration of the partially purified antiestrogen-receptor complexes resulted in significant dissociation of the larger complex into monomers. Incubations of 5.9S antiestrogen-receptor complexes with antibodies against nontransformed steroid receptor-associated proteins (the 59 and 90 kDa proteins) did not result in the interaction of this larger antiestrogen-receptor complex with these antibodies (obtained from L.E. Faber and D.O. Toft, respectively). Our results support the concept that antiestrogen binding induces a different receptor conformation which could affect monomer-dimer equilibrium, thus rendering the antiestrogen-receptor complex incapable of inducing complete estrogenic responses in target tissues.

查看原文

微信好友朋友圈 QQ好友复制链接

本刊更多论文

雌激素与抗雌激素结合时盐转化雌激素受体形式的差异

我们的实验室之前报道过，与雌激素结合的受体相比，抗雌激素结合钼酸盐稳定的非转化雌激素受体在0.3 M KCl中产生更大的受体形式。雌二醇在0.3 M KC1存在时促进单体的形成，而抗雌激素似乎促进二聚体的形成。我们扩展了这些研究，检测了用deae -纤维素层析部分纯化的兔子宫盐转化雌激素受体。我们之前已经证明，当雌激素受体与雌激素或抗雌激素络合时，以这种方式制备的雌激素受体结合在部分去蛋白的染色质亚段或重组的染色体蛋白/DNA部分的不同位点上。对这些受体制备的分析表明，deae -纤维素阶梯式洗脱在含有0.3 M KCl的5-20%蔗糖密度梯度下，受体与抗雌激素H1285和反式羟他莫昔芬结合，形成5.9S的单峰。雌二醇结合受体沉淀为4.5S。这些受体复合物结合dna -纤维素表明这些部分纯化的受体被转化了。DEAE重层析或琼脂糖凝胶过滤部分纯化的抗雌激素受体复合物导致较大的复合物解离成单体。5.9S抗雌激素受体复合物与针对非转化类固醇受体相关蛋白(59和90 kDa蛋白)的抗体孵育，不会导致这种较大的抗雌激素受体复合物与这些抗体相互作用(分别来自L.E. Faber和D.O. Toft)。我们的研究结果支持了一个概念，即抗雌激素结合诱导不同的受体构象，这可能会影响单体-二聚体的平衡，从而使抗雌激素受体复合物无法在靶组织中诱导完全的雌激素反应。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

求助全文

约1分钟内获得全文去求助

来源期刊

Journal of steroid biochemistry

自引率

0.00%

发文量

期刊最新文献

Editorial Announcement Insulin-like growth factor I (IGF I) induces cortisol production in bovine adrenocortical cells in primary culture Steroid biosynthesis by zona glomerulosa-fasciculata cells in primary culture of guinea-pig adrenals Immunological measurement of human 17β-hydroxysteroid dehydrogenase