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一种新型雌激素受体-β亚型的功能分析

Functional analysis of a novel estrogen receptor-beta isoform.

作者信息

Hanstein B, Liu H, Yancisin M C, Brown M

机构信息

Department of Adult Oncology, Dana-Farber Cancer Institute, Boston, Massachusetts 02115, USA.

出版信息

Mol Endocrinol. 1999 Jan;13(1):129-37. doi: 10.1210/mend.13.1.0234.

DOI:10.1210/mend.13.1.0234
PMID:9892018
Abstract

A new level of complexity has recently been added to estrogen signaling with the identification of a second estrogen receptor, ERbeta. By screening a rat prostate cDNA library, we detected ERbeta as well as a novel isoform that we termed ERbeta2. ERbeta2 contains an in-frame inserted exon of 54 nucleotides that results in the predicted insertion of 18 amino acids within the ERbeta hormone-binding domain. We also have evidence for the expression of both ERbeta1 and ERbeta2 in human cell lines. Competition ligand binding analysis of bacterially expressed fusion proteins revealed an 8-fold lower affinity of ERbeta2 for 17beta-estradiol (E2) [dissociation constant (Kd approximately 8 nM)] as compared with ERbeta1 (Kd approximately 1 nM). In vitro transcribed and translated ERbeta1 and ERbeta2 bind specifically to a consensus estrogen responsive element in a gel mobility shift assay. Furthermore, we show heterodimerization of ERbeta1 and ERbeta2 with each other as well as with ERalpha. In affinity interaction assays for proteins that associate specifically with the hormone-binding domain of these receptors, we demonstrate that the steroid receptor coactivator SRC-1 interacts in an estrogen-dependent manner with ERalpha and ERbeta1, but not with ERbeta2. In cotransfection experiments with expression plasmids for ERalpha, ERbeta1, and ERbeta2 and an estrogen-responsive element-containing luciferase reporter, the dose response of ERbeta1 to E2 was similar to that of ERalpha although the maximal stimulation was approximately 50%. In contrast, ERbeta2 required 100- to 1000-fold greater E2 concentrations for maximal activation. Thus, ERbeta2 adds yet another facet to the possible cellular responses to estrogen.

摘要

随着第二种雌激素受体ERβ的发现,雌激素信号传导最近又增加了一个新的复杂层面。通过筛选大鼠前列腺cDNA文库,我们检测到了ERβ以及一种新的亚型,我们将其命名为ERβ2。ERβ2包含一个54个核苷酸的框内插入外显子,这导致在ERβ激素结合域内预测插入18个氨基酸。我们也有证据表明ERβ1和ERβ2在人类细胞系中均有表达。对细菌表达的融合蛋白进行的竞争配体结合分析显示,与ERβ1(解离常数Kd约为1 nM)相比,ERβ2对17β-雌二醇(E2)的亲和力低8倍(Kd约为8 nM)。在凝胶迁移率变动分析中,体外转录和翻译的ERβ1和ERβ2特异性结合一致的雌激素反应元件。此外,我们展示了ERβ1和ERβ2之间以及它们与ERα之间的异源二聚化。在针对与这些受体的激素结合域特异性结合的蛋白质的亲和相互作用分析中,我们证明类固醇受体辅激活因子SRC-1以雌激素依赖的方式与ERα和ERβ1相互作用,但不与ERβ2相互作用。在用ERα、ERβ1和ERβ2的表达质粒以及含雌激素反应元件的荧光素酶报告基因进行的共转染实验中,ERβ1对E2的剂量反应与ERα相似,尽管最大刺激约为50%。相比之下,ERβ2需要高100至1000倍的E2浓度才能达到最大激活。因此,ERβ2为细胞对雌激素的可能反应又增添了一个新层面。

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