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甲状腺激素通过激活人肝癌细胞系中的弗林蛋白酶表达促进细胞侵袭。

Thyroid hormone promotes cell invasion through activation of furin expression in human hepatoma cell lines.

作者信息

Chen Ruey-Nan, Huang Ya-Hui, Lin Ya-Chu, Yeh Chau-Ting, Liang Ying, Chen Shen-Liang, Lin Kwang-Huei

机构信息

Department of Biochemistry, Chang-Gung University, 259 Wen-hwa 1 Road, Taoyuan 333, Taiwan, Republic of China.

出版信息

Endocrinology. 2008 Aug;149(8):3817-31. doi: 10.1210/en.2007-0989. Epub 2008 May 8.

Abstract

The objective of this study was to identify genes regulated by thyroid hormone (T(3)) and associated with tumor invasion. The gene encoding furin, as previously identified by cDNA microarray, is known to be up-regulated by T(3) treatment, and stimulated furin production occurs in thyroidectomized rats after administration of T(3). Presently, by using serial deletion of the promoter and EMSAs, the T(3) response element on the furin promoter was localized to the -6317/-6302 region. T(3)-mediated furin up-regulation was cooperative with TGF-beta because T(3) induction increased after Smad3/4 addition. Furthermore, the invasiveness of HepG2-thyroid hormone receptor (TR) cells was significantly increased by T(3) treatment, perhaps due to furin processing of matrix metalloproteinase-2 and -9. In addition, furin up-regulation either by stable overexpression or T(3) and/or TGF-beta induction was evident in severe-combined immune-deficient mice inoculated with HepG2-TRalpha1 cells. The HepG2-furin mice displayed a higher metastasis index and tumor size than HepG2-neo mice. Notably, the increased liver and lung tumor number or size in the hyperthyroid severe-combined immune-deficient mice as well as TGF-beta mice was attributed specifically to furin overexpression in the HepG2-TRalpha1 cells. Furthermore, this study demonstrated that furin overexpression in some types of hepatocellular carcinomas is TR dependent and might play a crucial role in the development of hepatocellular carcinoma. Thus, T(3) regulates furin gene expression via a novel mechanism or in cooperation with TGF-beta to enhance tumor metastasis in vitro and in vivo.

摘要

本研究的目的是鉴定受甲状腺激素(T3)调控并与肿瘤侵袭相关的基因。如先前通过cDNA微阵列鉴定的那样,编码弗林蛋白酶的基因已知在T3处理后会上调,并且在给予T3后,甲状腺切除的大鼠中会出现弗林蛋白酶产生增加的情况。目前,通过使用启动子的系列缺失和电泳迁移率变动分析(EMSA),弗林蛋白酶启动子上的T3反应元件定位于-6317 / -6302区域。T3介导的弗林蛋白酶上调与转化生长因子-β(TGF-β)协同作用,因为添加Smad3/4后T3诱导增加。此外,T3处理显著增加了HepG2-甲状腺激素受体(TR)细胞的侵袭性,这可能是由于基质金属蛋白酶-2和-9的弗林蛋白酶加工所致。此外,在接种了HepG2-TRα1细胞的严重联合免疫缺陷小鼠中,通过稳定过表达或T3和/或TGF-β诱导导致的弗林蛋白酶上调是明显的。与HepG2-neo小鼠相比,HepG2-弗林蛋白酶小鼠表现出更高的转移指数和肿瘤大小。值得注意的是,甲状腺功能亢进的严重联合免疫缺陷小鼠以及TGF-β小鼠中肝脏和肺部肿瘤数量或大小的增加具体归因于HepG2-TRα1细胞中弗林蛋白酶的过表达。此外,本研究表明,某些类型肝细胞癌中弗林蛋白酶的过表达是TR依赖性的,并且可能在肝细胞癌的发展中起关键作用。因此,T3通过一种新机制或与TGF-β协同作用来调节弗林蛋白酶基因表达,以增强体外和体内的肿瘤转移。

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