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正常卵巢、卵巢浆液性囊腺癌及卵巢癌细胞系中的雌激素受体α(ER-α)和β(ER-β)mRNA:肿瘤组织中ER-β的下调

Estrogen receptor alpha (ER-alpha) and beta (ER-beta) mRNAs in normal ovary, ovarian serous cystadenocarcinoma and ovarian cancer cell lines: down-regulation of ER-beta in neoplastic tissues.

作者信息

Brandenberger A W, Tee M K, Jaffe R B

机构信息

Reproductive Endocrinology Center, University of California, San Francisco, 94143-0556, USA.

出版信息

J Clin Endocrinol Metab. 1998 Mar;83(3):1025-8. doi: 10.1210/jcem.83.3.4788.

Abstract

The prognosis in ovarian carcinoma, the most lethal of the gynecologic neoplasms, is poor and has changed little in the last three decades. Only a small number respond to antiestrogen therapy, although the classic estrogen receptor, ER-alpha, has been identified in ovarian surface epithelium, from which approximately 90% of ovarian cancers originate. We have previously shown that ER-beta mRNA is most abundant in human fetal ovaries, suggesting that it might play an important role in ovarian development. Therefore, we investigated the mRNA levels of both ERs in normal ovaries, ovarian serous cystadenocarcinomas, granulosa cells from patients undergoing in vitro fertilization (IVF), the ovarian surface epithelium cell line IOSE-Van, and the ovarian cancer cell lines SKOV3, HEY and OCC1. Northern blots of normal and neoplastic ovaries were hybridized with an ER-beta riboprobe that spans the A/B domain. We detected two major hybridizing bands at approximately 8 and 10 kb. An RNase protection assay using the same probe revealed a single band of the expected size. Hybridizing the same blot with an ER-alpha riboprobe showed a strong hybridizing band at approximately 6.5 kb. In ovarian cancer samples, ER-beta mRNA level was decreased when compared to normal ovaries. Using 25 cycles of RT-PCR followed by Southern blotting, we found equal amounts of ER-alpha and -beta mRNAs in normal ovaries in all age groups from 33 to 75 years; however, in ovarian cancer tissue, the level of ER-alpha mRNA was similar or slightly higher, comparable to 10(3) to 10(4) copies of plasmid DNA, but ER-beta mRNA levels were markedly decreased. Granulosa cells from IVF patients expressed high levels of ER-beta mRNA. The OSE cell line expressed a low level of ER-alpha, detectable after 40 cycles of RT-PCR and no ER-beta mRNA. SKOV3 showed a low level of ER-alpha and -beta mRNAs, whereas OCC1 showed a low level of ER-beta and a relatively high level of ER-alpha. HEY did not contain detectable amounts of either ER after 40 cycles of RT-PCR. We found no evidence of differential splicing or major deletions in almost the entire coding region of ER-beta in either normal ovaries or tumor samples.

摘要

卵巢癌是妇科肿瘤中最致命的一种,其预后很差,在过去三十年里变化不大。尽管经典的雌激素受体α(ER-α)已在卵巢表面上皮中被鉴定出来,而大约90%的卵巢癌起源于此,但只有少数患者对抗雌激素治疗有反应。我们之前已经表明,ER-β mRNA在人类胎儿卵巢中最为丰富,这表明它可能在卵巢发育中起重要作用。因此,我们研究了正常卵巢、卵巢浆液性囊腺癌、体外受精(IVF)患者的颗粒细胞、卵巢表面上皮细胞系IOSE-Van以及卵巢癌细胞系SKOV3、HEY和OCC1中两种雌激素受体的mRNA水平。用跨越A/B结构域的ER-β核糖探针与正常和肿瘤性卵巢的Northern印迹杂交。我们在大约8和10 kb处检测到两条主要的杂交带。使用相同探针的核糖核酸酶保护试验显示出一条预期大小的单带。用ER-α核糖探针与同一张印迹杂交,在大约6.5 kb处显示出一条强杂交带。在卵巢癌样本中,与正常卵巢相比,ER-β mRNA水平降低。通过25个循环的逆转录聚合酶链反应(RT-PCR),随后进行Southern印迹分析,我们发现在33至75岁的所有年龄组的正常卵巢中,ER-α和 -β mRNA的量相等;然而,在卵巢癌组织中,ER-α mRNA水平相似或略高,相当于10³至10⁴拷贝的质粒DNA,但ER-β mRNA水平明显降低。IVF患者的颗粒细胞表达高水平的ER-β mRNA。OSE细胞系表达低水平的ER-α,在40个循环的RT-PCR后可检测到,且没有ER-β mRNA。SKOV3显示出低水平的ER-α和 -β mRNA,而OCC1显示出低水平的ER-β和相对高水平的ER-α。在40个循环的RT-PCR后,HEY未检测到可检测量的任何一种雌激素受体。我们在正常卵巢或肿瘤样本中几乎整个ER-β编码区域都没有发现差异剪接或主要缺失的证据。

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