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通过降低自分泌转化生长因子α的表达来抑制雌激素诱导的乳腺癌细胞增殖。

Inhibition of estrogen-induced breast cancer cell proliferation by reduction in autocrine transforming growth factor alpha expression.

作者信息

Reddy K B, Yee D, Hilsenbeck S G, Coffey R J, Osborne C K

机构信息

Department of Medicine/Medicaal Oncology, University of Texas Health Science Center at San Antonio 78284-7884.

出版信息

Cell Growth Differ. 1994 Dec;5(12):1275-82.

PMID:7696176
Abstract

Breast cancer cell lines have been shown to secrete transforming growth factor alpha (TGF alpha) and other polypeptide growth factors in response to estrogen (E2) stimulation. In this study, we investigated whether cellular-derived TGF alpha mediates the growth-stimulatory effects of E2 in ER-positive breast cancer cells. To test this hypothesis, we introduced an antisense TGF alpha mRNA expression vector under control of a human metallothionein promoter into E2-responsive T47D human breast cancer cells. In stably transfected cells, cadmium induced antisense mRNA and reduced expression of TGF alpha mRNA and protein in antisense clones (AS1). TGF alpha expression was increased in sense clones (S2), while wild-type T47D cells (W3) or pSV2 neomycin resistance-transfected cells showed no change in TGF alpha expression in response to cadmium. The basal proliferative capacity of antisense transfected cells was equivalent to that of the wild-type. E2 increased TGF alpha synthesis and cell proliferation in transfected and wild-type cells. In AS1 cells, the simultaneous addition of cadmium with E2 blocked most of the E2-induced increase in TGF alpha mRNA and protein and nearly abolished the stimulatory effects of E2 on DNA synthesis and cell number. In contrast, no reduction in cell proliferation was observed with cadmium in antisense-transfected cells with a low level of antisense expression or in the S2 or W3 cells. Our results are compatible with the hypothesis that autocrine production of TGF alpha may be an important contributor to E2-induced growth in T47D cells.

摘要

乳腺癌细胞系已被证明在雌激素(E2)刺激下会分泌转化生长因子α(TGFα)和其他多肽生长因子。在本研究中,我们调查了细胞来源的TGFα是否介导E2对雌激素受体阳性乳腺癌细胞的生长刺激作用。为了验证这一假设,我们将一个在人金属硫蛋白启动子控制下的反义TGFα mRNA表达载体导入对E2有反应的T47D人乳腺癌细胞中。在稳定转染的细胞中,镉诱导反义mRNA并降低反义克隆(AS1)中TGFα mRNA和蛋白的表达。在正义克隆(S2)中TGFα表达增加,而野生型T47D细胞(W3)或转染了pSV2新霉素抗性的细胞在镉处理后TGFα表达没有变化。反义转染细胞的基础增殖能力与野生型相当。E2增加了转染细胞和野生型细胞中TGFα的合成及细胞增殖。在AS1细胞中,镉与E2同时添加可阻断大部分E2诱导的TGFα mRNA和蛋白增加,并几乎消除E2对DNA合成和细胞数量的刺激作用。相比之下,在反义表达水平低的反义转染细胞、S2或W3细胞中,镉处理未观察到细胞增殖减少。我们的结果与以下假设相符,即TGFα的自分泌产生可能是E2诱导T47D细胞生长的一个重要因素。

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