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雌激素和孕激素处理的正常人乳腺组织中I型胰岛素样生长因子受体基因的表达

Type I insulin-like growth factor receptor gene expression in normal human breast tissue treated with oestrogen and progesterone.

作者信息

Clarke R B, Howell A, Anderson E

机构信息

Clinical Research Department, Christie Hospital NHS Trust, Withington, Manchester, UK.

出版信息

Br J Cancer. 1997;75(2):251-7. doi: 10.1038/bjc.1997.41.

Abstract

The epithelial proliferation of normal human breast tissue xenografts implanted into athymic nude mice is significantly increased from basal levels by oestradiol (E2), but not progesterone (Pg) treatment at serum concentrations similar to those observed in the luteal phase of the human menstrual cycle. Type I IGF receptor (IGFR-I) mRNA and protein have been shown to be up-regulated by E2 in MCF-7 breast cancer cells in vitro in which IGF-I and E2 act synergistically to stimulate proliferation. We have investigated the expression of the IGFR-I mRNA in normal human breast xenografts treated with or without E2 or Pg alone and in combination. Northern analysis of 20 micrograms of RNA extracted from the breast xenograft samples showed no hybridization with 32P-labelled IGFR-I probe, although an 11-kb species of IGFR-I mRNA could be seen when 20 micrograms of RNA extracted from either MCF-7 breast cancer cells or human breast carcinomas was examined in this way. In order to analyse the expression of IGFR-I mRNA in breast xenografts, a quantitative reverse transcription-polymerase chain reaction (RT-PCR) was employed in which RNA loading, reverse transcription and PCR efficiencies were internally controlled. The data indicate that the IGFR-I mRNA is up-regulated by two to threefold compared with untreated levels by 7 and 14 days E2 treatment. In contrast, 7 or 14 days Pg treatment down-regulates the receptor mRNA to approximately half that of untreated levels, whereas combination E2 and Pg treatment produced a twofold increase in IGFR-I mRNA levels compared with untreated tissue. The results are consistent with the suggestion that E2 may act to stimulate proliferation indirectly via a paracrine mechanism involving IGFs in normal as well as malignant human breast epithelial cells.

摘要

将正常人类乳腺组织异种移植到无胸腺裸鼠体内,在血清浓度与人类月经周期黄体期相似的情况下,雌二醇(E2)可使上皮细胞增殖较基础水平显著增加,但孕酮(Pg)处理则无此作用。体外研究表明,在MCF-7乳腺癌细胞中,I型胰岛素样生长因子受体(IGFR-I)的mRNA和蛋白可被E2上调,其中IGF-I和E2协同作用刺激细胞增殖。我们研究了单独或联合使用E2或Pg处理的正常人类乳腺异种移植中IGFR-I mRNA的表达。对从乳腺异种移植样本中提取的20微克RNA进行Northern分析,未发现与32P标记的IGFR-I探针杂交,尽管以这种方式检测从MCF-7乳腺癌细胞或人类乳腺癌中提取的20微克RNA时,可以看到11 kb的IGFR-I mRNA条带。为了分析乳腺异种移植中IGFR-I mRNA的表达,采用了定量逆转录-聚合酶链反应(RT-PCR),其中RNA上样量、逆转录和PCR效率均进行了内部对照。数据表明,与未处理水平相比,E2处理7天和14天后,IGFR-I mRNA上调了2至3倍。相反,Pg处理7天或14天可使受体mRNA下调至未处理水平的约一半,而E2和Pg联合处理使IGFR-I mRNA水平比未处理组织增加了两倍。这些结果支持以下观点:在正常及恶性人类乳腺上皮细胞中,E2可能通过涉及IGF的旁分泌机制间接刺激细胞增殖。

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