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中介亚基 MED1 调节甲状腺激素受体的核内动力学。

Mediator subunit MED1 modulates intranuclear dynamics of the thyroid hormone receptor.

机构信息

Department of Biology, William and Mary, Williamsburg, Viginia.

出版信息

J Cell Biochem. 2020 Apr;121(4):2909-2926. doi: 10.1002/jcb.29532. Epub 2019 Nov 6.

Abstract

The thyroid hormone receptors (TRs) mediate thyroid hormone (T )-dependent gene expression. The nuclear import and export signals that direct TR shuttling are well characterized, but little is known about factors modulating nuclear retention. We used fluorescence-based nucleocytoplasmic scoring and fluorescence recovery after photobleaching in transfected cells to investigate whether Mediator subunits MED1 and MED13 play a role in nuclear retention of TR. When MED1 was overexpressed, there was a striking shift towards a greater nuclear localization of TRβ1 and the oncoprotein v-ErbA, subtypes with cytosolic populations at steady-state, and TRβ1 intranuclear mobility was reduced. For TRα1, there was no observable change in its predominantly nuclear distribution pattern or mobility. Consistent with a role for MED1 in nuclear retention, the cytosolic TRα1 and TRβ1 population were significantly greater in MED1 cells, compared with MED1 cells. Exposure to T and epidermal growth factor, which induces MED1 phosphorylation, also altered TR intranuclear dynamics. Overexpression of miR-208a, which downregulates MED13, led to a more cytosolic distribution of nuclear-localized TRα1; however, overexpression of MED13 had no effect on TRβ1 localization. The known binding site of MED1 overlaps with a transactivation domain and nuclear export signal in helix 12 of TR's ligand-binding domain (LBD). Coimmunoprecipitation assays demonstrated that TR's LBD interacts directly with exportins 5 and 7, suggesting that binding of exportins and MED1 to TR may be mutually exclusive. Collectively, our data provide evidence that MED1 promotes nuclear retention of TR, and highlight the dual functionality of helix 12 in TR transactivation and nuclear export.

摘要

甲状腺激素受体 (TRs) 介导甲状腺激素 (T) 依赖性基因表达。指导 TR 穿梭的核输入和输出信号已得到很好的描述,但对于调节核保留的因素知之甚少。我们使用基于荧光的核质评分和转染细胞中的荧光恢复后光漂白来研究 Mediator 亚基 MED1 和 MED13 是否在 TR 的核保留中发挥作用。当 MED1 过表达时,TRβ1 和致癌蛋白 v-ErbA 的核定位明显增加,这些亚型在稳态时有细胞质群体,并且 TRβ1 的核内迁移性降低。对于 TRα1,其主要位于核内的分布模式或迁移性没有观察到变化。与 MED1 在核保留中的作用一致,与 MED1 细胞相比,Mediator1 细胞中的细胞质 TRα1 和 TRβ1 群体显著增加。暴露于 T 和表皮生长因子(诱导 MED1 磷酸化)也改变了 TR 核内动力学。下调 MED13 的 miR-208a 的过表达导致核定位的 TRα1 更偏向细胞质分布;然而,MED13 的过表达对 TRβ1 定位没有影响。已知的 MED1 结合位点与 TR 配体结合域 (LBD) 中螺旋 12 的转录激活域和核输出信号重叠。共免疫沉淀测定表明 TR 的 LBD 与输出蛋白 5 和 7 直接相互作用,这表明输出蛋白和 MED1 与 TR 的结合可能是相互排斥的。总之,我们的数据提供了证据表明 MED1 促进了 TR 的核保留,并强调了 TR 转录激活和核输出中螺旋 12 的双重功能。

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