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人卵巢表面上皮在组织培养中的连续传代

Serial propagation of human ovarian surface epithelium in tissue culture.

作者信息

Siemens C H, Auersperg N

机构信息

Department of Anatomy, University of British Columbia, Vancouver.

出版信息

J Cell Physiol. 1988 Mar;134(3):347-56. doi: 10.1002/jcp.1041340305.

DOI:10.1002/jcp.1041340305
PMID:2450877
Abstract

Most human ovarian cancers are thought to arise in the ovarian surface epithelium (OSE). The precise role of OSE in carcinogenesis has not been defined because no appropriate animal models for the study of this tissue exist and culture of human OSE has been limited to primary outgrowths. In this report, we describe conditions for serial cultivation of normal human OSE. Premenopausal ovarian tissue was obtained at surgery. OSE growth was compared in media MCDB 202, 199 and Waymouth's 752/1 (WM) supplemented with 5, 15, or 25% fetal bovine serum (FBS), with/without 20 ng/ml epidermal growth factor (EGF) and 0.4 micrograms/ml hydrocortisone (HC). The rate and extent of OSE outgrowths from explants in primary culture were greatest in either WM or 199/202 (1:1), supplemented with 15% FBS/EGF/HC. In early passage cultures, cell proliferation was most rapid and extensive in 199/202 with 15% FBS, EGF, and HC. In this medium, OSE cells were subcultured up to 10 times and underwent 20-25 population doublings over 5 weeks. The population doubling time during rapid growth was approximately 48 h. Seeding efficiencies of up to 53% and cloning efficiencies of up to 13% were obtained. Early passage OSE cells reversibly modulated from a slow growing, epithelial, intensely keratin-positive form in 199/202 medium lacking EGF/HC, to a rapidly proliferating, elongate, less keratin-positive form in medium with EGF/HC. OSE cells grown in WM/5-15% FBS were epithelial and near-stationary. Thus, culture conditions have been defined for ovarian carcinogen assays requiring either proliferating or stationary cell populations, and for further studies of the role of OSE in ovarian biology.

摘要

大多数人类卵巢癌被认为起源于卵巢表面上皮(OSE)。由于不存在用于研究该组织的合适动物模型,且人类OSE的培养仅限于原代生长,因此OSE在致癌作用中的精确作用尚未明确。在本报告中,我们描述了正常人OSE连续培养的条件。在手术中获取绝经前卵巢组织。比较了在添加5%、15%或25%胎牛血清(FBS)、有/无20 ng/ml表皮生长因子(EGF)和0.4 μg/ml氢化可的松(HC)的MCDB 202、199和Waymouth's 752/1(WM)培养基中OSE的生长情况。原代培养中外植体OSE生长的速率和程度在添加15% FBS/EGF/HC的WM或199/202(1:1)中最大。在早期传代培养中,添加15% FBS、EGF和HC的199/202培养基中细胞增殖最为迅速和广泛。在此培养基中,OSE细胞可传代培养达10次,并在5周内经历20 - 25次群体倍增。快速生长期间群体倍增时间约为48小时。获得了高达53%的接种效率和高达13%的克隆效率。早期传代的OSE细胞在缺乏EGF/HC的199/202培养基中可逆地从生长缓慢、上皮样、角蛋白强阳性形态,转变为添加EGF/HC的培养基中快速增殖、细长、角蛋白阳性较弱的形态。在WM/5 - 15% FBS中生长的OSE细胞呈上皮样且接近静止状态。因此,已经确定了用于需要增殖或静止细胞群体的卵巢致癌物检测以及进一步研究OSE在卵巢生物学中作用的培养条件。

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