Wang Jieru, Edeen Karen, Manzer Rizwan, Chang Yongsheng, Wang Shuanglin, Chen Xueni, Funk C Joel, Cosgrove Gregory P, Fang Xiaohui, Mason Robert J
Department of Medicine, National Jewish and Medical Research Center, Denver, CO 80206, USA.
Am J Respir Cell Mol Biol. 2007 Jun;36(6):661-8. doi: 10.1165/rcmb.2006-0410OC. Epub 2007 Jan 25.
Cultures of differentiating fetal human type II cells have been available for many years. However, studies with differentiated adult human type II cells are limited. We used a published method for type II cell isolation and developed primary culture systems for maintenance of differentiated adult human alveolar epithelial cells for in vitro studies. Human type II cells cultured on Matrigel (basolateral access) or a mixture of Matrigel and rat tail collagen (apical access) in the presence of keratinocyte growth factor, isobutylmethylxanthine, 8-bromo-cyclicAMP, and dexamethasone (KIAD) expressed the differentiated type II cell phenotype as measured by the expression of surfactant protein (SP)-A, SP-B, SP-C, and fatty acid synthase and their morphologic appearance. These cells contain lamellar inclusion bodies and have apical microvilli. In both systems the cells appear well differentiated. In the apical access system, type II cell differentiation markers initially decreased and then recovered over 6 d in culture. Lipid synthesis was also increased by the addition of KIAD. In contrast, type II cells cultured on rat tail collagen (or tissue culture plastic) slowly lose their lamellar inclusions and expression of the surfactant proteins and increase the expression of type I cell markers. The expression of the phenotypes is regulated by the culture conditions and is, in part, reversible in vitro.
多年来一直有可用于分化的人胎儿II型细胞的培养物。然而,对分化的成人II型细胞的研究有限。我们采用一种已发表的II型细胞分离方法,开发了原代培养系统,用于维持分化的成人肺泡上皮细胞以便进行体外研究。在角质形成细胞生长因子、异丁基甲基黄嘌呤、8-溴环磷酸腺苷和地塞米松(KIAD)存在的情况下,在基质胶(基底外侧通路)或基质胶与大鼠尾胶原的混合物(顶端通路)上培养的人II型细胞,通过表面活性蛋白(SP)-A、SP-B、SP-C和脂肪酸合酶的表达及其形态外观来衡量,表现出分化的II型细胞表型。这些细胞含有板层小体并具有顶端微绒毛。在这两种系统中,细胞看起来分化良好。在顶端通路系统中,II型细胞分化标志物最初下降,然后在培养6天内恢复。添加KIAD也增加了脂质合成。相比之下,在大鼠尾胶原(或组织培养塑料)上培养的II型细胞会慢慢失去其板层小体和表面活性蛋白的表达,并增加I型细胞标志物的表达。表型的表达受培养条件调节,并且在体外部分是可逆的。