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在无血清且添加激素的培养基中气管分化功能的表达

Expression of tracheal differentiated functions in serum-free hormone-supplemented medium.

作者信息

Wu R, Nolan E, Turner C

出版信息

J Cell Physiol. 1985 Nov;125(2):167-81. doi: 10.1002/jcp.1041250202.

DOI:10.1002/jcp.1041250202
PMID:4055904
Abstract

Most dissociated airway epithelial cells in culture express few of their in vivo functions and only to a limited degree. In this report, we demonstrate that hamster tracheal epithelial (HTE) cells cultured on a collagen gel substratum in a serum-free hormone-supplemented medium differentiate to cilia-beating and mucus-secreting cell types. The medium is Ham's F-12 supplemented with insulin, epidermal growth factor, transferrin, hydrocortisone, cholera toxin, bovine hypothalamus extract, and vitamin A. Under these culture conditions, HTE cells exhibit a growth rate of 24 h/population doubling and reach confluency, at a density of 2-5 X 10(4) cells/cm2, within 2 weeks. Both the collagen gel substratum and vitamin A of this culture system are important to the growth and differentiation of HTE cells in vitro. Evidence of HTE cell differentiation has been obtained at both the ultrastructural and the histochemical levels. In addition, a variety of biochemical studies (gel filtration, ion exchange column chromatography, enzyme digestion, nitrous acid treatment, and composition analysis) indicate the production of mucin-like glycoprotein in the HTE cultures. The levels of mucin-like glycoprotein were found to closely correlate with the histochemically quantitated levels of the mucous cell type. Kinetic studies demonstrate that HTE cells rapidly lose their differentiated features during the attachment stage of primary culture but redifferentiation occurs after the cultures reach confluency. The ability of HTE cells to grow and differentiate in this serum-free culture system in the absence of other cell types should greatly facilitate the study of mucociliary functions in vitro.

摘要

大多数培养的分离气道上皮细胞仅在有限程度上表达其少数体内功能。在本报告中,我们证明,在无血清、添加激素的培养基中,于胶原凝胶基质上培养的仓鼠气管上皮(HTE)细胞可分化为纤毛摆动和分泌黏液的细胞类型。该培养基是添加了胰岛素、表皮生长因子、转铁蛋白、氢化可的松、霍乱毒素、牛下丘脑提取物和维生素A的Ham's F-12培养基。在这些培养条件下,HTE细胞的生长速率为24小时/群体倍增时间,在2周内达到汇合,细胞密度为2 - 5×10⁴个细胞/cm²。该培养系统中的胶原凝胶基质和维生素A对HTE细胞的体外生长和分化均很重要。已在超微结构和组织化学水平获得了HTE细胞分化的证据。此外,各种生化研究(凝胶过滤、离子交换柱色谱、酶消化、亚硝酸处理和成分分析)表明HTE培养物中产生了黏蛋白样糖蛋白。发现黏蛋白样糖蛋白的水平与黏液细胞类型的组织化学定量水平密切相关。动力学研究表明,HTE细胞在原代培养的贴壁阶段迅速丧失其分化特征,但在培养物达到汇合后会重新分化。HTE细胞在无其他细胞类型的情况下,在这种无血清培养系统中生长和分化的能力应极大地促进体外黏液纤毛功能的研究。

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