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原代仓鼠气管气道上皮细胞的分化培养物。

Differentiated cultures of primary hamster tracheal airway epithelial cells.

作者信息

Rowe Regina K, Brody Steven L, Pekosz Andrew

机构信息

Molecular Microbiology and Microbial Pathogenesis Graduate Program, Washington University School of Medicine, St. Louis, Missouri 63110, USA.

出版信息

In Vitro Cell Dev Biol Anim. 2004 Nov-Dec;40(10):303-11. doi: 10.1290/0408056.1.

Abstract

Primary airway epithelial cell cultures can provide a faithful representation of the in vivo airway while allowing for a controlled nutrient source and isolation from other tissues or immune cells. The methods used have significant differences based on tissue source, cell isolation, culture conditions, and assessment of culture purity. We modified and optimized a method for generating tracheal epithelial cultures from Syrian golden hamsters and characterized the cultures for cell composition and function. Soon after initial plating, the epithelial cells reached a high transepithelial resistance and formed tight junctions. The cells differentiated into a heterogeneous, multicellular culture containing ciliated, secretory, and basal cells after culture at an air-liquid interface (ALI). The secretory cell populations initially consisted of MUC5AC-positive goblet cells and MUC5AC/CCSP double-positive cells, but the makeup changed to predominantly Clara cell secretory protein (CCSP)-positive Clara cells after 14 d. The ciliated cell populations differentiated rapidly after ALI, as judged by the appearance of beta tubulin IV-positive cells. The cultures produced mucus, CCSP, and trypsin-like proteases and were capable of wound repair as judged by increased expression of matrilysin. Our method provides an efficient, high-yield protocol for producing differentiated hamster tracheal epithelial cells that can be used for a variety of in vitro studies including tracheal cell differentiation, airway disease mechanisms, and pathogen-host interactions.

摘要

原代气道上皮细胞培养可以在提供可控营养来源并与其他组织或免疫细胞分离的同时,忠实地呈现体内气道的情况。所使用的方法在组织来源、细胞分离、培养条件以及培养纯度评估方面存在显著差异。我们改进并优化了一种从叙利亚金黄地鼠生成气管上皮培养物的方法,并对培养物的细胞组成和功能进行了表征。初次接种后不久,上皮细胞就达到了较高的跨上皮电阻并形成了紧密连接。在气液界面(ALI)培养后,这些细胞分化为包含纤毛细胞、分泌细胞和基底细胞的异质性多细胞培养物。分泌细胞群体最初由MUC5AC阳性杯状细胞和MUC5AC/CCSP双阳性细胞组成,但在14天后,其组成转变为主要是Clara细胞分泌蛋白(CCSP)阳性的Clara细胞。根据β微管蛋白IV阳性细胞的出现判断,ALI后纤毛细胞群体迅速分化。这些培养物产生黏液、CCSP和胰蛋白酶样蛋白酶,并且根据基质溶素表达的增加判断能够进行伤口修复。我们的方法为生成可用于多种体外研究(包括气管细胞分化、气道疾病机制和病原体-宿主相互作用)的分化仓鼠气管上皮细胞提供了一种高效、高产的方案。

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