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雌激素受体(ER)α和ERβ的共定位及配体依赖性离散分布

Colocalization and ligand-dependent discrete distribution of the estrogen receptor (ER)alpha and ERbeta.

作者信息

Matsuda Ken-ichi, Ochiai Ikuo, Nishi Mayumi, Kawata Mitsuhiro

机构信息

Department of Anatomy and Neurobiology, Kyoto Prefectural University of Medicine, Kawaramachi Hirokoji, Kamigyo-ku, Kyoto 602-8566, Japan.

出版信息

Mol Endocrinol. 2002 Oct;16(10):2215-30. doi: 10.1210/me.2002-0110.

Abstract

To investigate the relationships between the loci expressing functions of estrogen receptor (ER)alpha and that of ERbeta, we analyzed the subnuclear distribution of ERalpha and ERbeta in response to ligand in single living cells using fusion proteins labeled with different spectral variants of green fluorescent protein. Upon activation with ligand treatment, fluorescent protein-tagged (FP)-ERbeta redistributed from a diffuse to discrete pattern within the nucleus, showing a similar time course as FP-ERalpha, and colocalized with FP-ERalpha in the same discrete cluster. Analysis using deletion mutants of ERalpha suggested that the ligand-dependent redistribution of ERalpha might occur through a large part of the receptor including at least the latter part of activation function (AF)-1, the DNA binding domain, nuclear matrix binding domain, and AF-2/ligand binding domain. In addition, a single AF-1 region within ERalpha homodimer, or a single DNA binding domain as well as AF-1 region within the ERalpha/ERbeta heterodimer, could be sufficient for the cluster formation. More than half of the discrete clusters of FP-ERalpha and FP-ERbeta were colocalized with hyperacetylated histone H4 and a component of the chromatin remodeling complex, Brg-1, indicating that ERs clusters might be involved in structural changes of chromatin.

摘要

为了研究雌激素受体(ER)α和ERβ功能表达位点之间的关系,我们使用标记有绿色荧光蛋白不同光谱变体的融合蛋白,分析了单个活细胞中ERα和ERβ在配体作用下的亚核分布。在用配体处理激活后,荧光蛋白标记的(FP)-ERβ在细胞核内从弥散模式重新分布为离散模式,显示出与FP-ERα相似的时间进程,并与FP-ERα在同一离散簇中共定位。使用ERα缺失突变体的分析表明,ERα的配体依赖性重新分布可能通过受体的很大一部分发生,至少包括激活功能(AF)-1的后半部分、DNA结合结构域、核基质结合结构域和AF-2/配体结合结构域。此外,ERα同二聚体内的单个AF-1区域,或ERα/ERβ异二聚体内的单个DNA结合结构域以及AF-1区域,可能足以形成簇。超过一半的FP-ERα和FP-ERβ离散簇与高度乙酰化的组蛋白H4和染色质重塑复合物的一个组分Brg-1共定位,表明ER簇可能参与染色质的结构变化。

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