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Differentiated human alveolar epithelial cells and reversibility of their phenotype in vitro
被引:119
作者:
Wang, Jieru
Edeen, Karen
Manzer, Rizwan
Chang, Yongsheng
Wang, Shuanglin
Chen, Xueni
Funk, C. Joel
Cosgrove, Gregory P.
Fang, Xiaohui
Mason, Robert J.
机构:
[1] Natl Jewish & Med Res Ctr, Dept Med, Denver, CO 80206 USA
[2] Univ Calif San Francisco, Dept Med, Cardiovasc Res Inst, San Francisco, CA 94143 USA
关键词:
type I cell;
type II cell;
surfactant;
lipogenesis;
II CELLS;
MAINTENANCE;
SECRETION;
MARKER;
D O I:
10.1165/rcmb.2006-0410OC
中图分类号:
Q5 [生物化学];
Q7 [分子生物学];
学科分类号:
071010 ;
081704 ;
摘要:
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.
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页码:661 / 668
页数:8
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