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Growth and differentiation of primary and passaged equine bronchial epithelial cells under conventional and air-liquid-interface culture conditions

机译:在常规和气液界面培养条件下原代和传代马的支气管上皮细胞的生长和分化

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Background Horses develop recurrent airway obstruction (RAO) that resembles human bronchial asthma. Differentiated primary equine bronchial epithelial cells (EBEC) in culture that closely mimic the airway cells in vivo would be useful to investigate the contribution of bronchial epithelium in inflammation of airway diseases. However, because isolation and characterization of EBEC cultures has been limited, we modified and optimized techniques of generating and culturing EBECs from healthy horses to mimic in vivo conditions. Results Large numbers of EBEC were obtained by trypsin digestion and successfully grown for up to 2 passages with or without serum. However, serum or ultroser G proved to be essential for EBEC differentiation on membrane inserts at ALI. A pseudo-stratified muco-ciliary epithelium with basal cells was observed at differentiation. Further, transepithelial resistance (TEER) was more consistent and higher in P1 cultures compared to P0 cultures while ciliation was delayed in P1 cultures. Conclusions This study provides an efficient method for obtaining a high-yield of EBECs and for generating highly differentiated cultures. These EBEC cultures can be used to study the formation of tight junction or to identify epithelial-derived inflammatory factors that contribute to lung diseases such as asthma.
机译:背景技术马会出现类似于人支气管哮喘的反复气道阻塞(RAO)。体内紧密模拟气道细胞的培养中分化的初级马匹支气管上皮细胞(EBEC)将有助于研究支气管上皮在气道疾病炎症中的作用。但是,由于EBEC培养物的分离和表征受到限制,我们修改并优化了从健康马匹生成和培养EBEC的技术,以模仿体内条件。结果通过胰蛋白酶消化获得了大量的EBEC,无论有无血清,EBEC都能成功生长2代。然而,在ALI膜插入物上,血清或ulturer G被证明对EBEC的分化至关重要。在分化时观察到具有基底细胞的伪分层的粘膜纤毛上皮。此外,与P 0 培养相比,P 1 培养中的跨上皮抵抗(TEER)更一致且更高,而P 1 培养中的纤毛延迟。 。结论这项研究为获得高产量的EBEC和产生高度分化的培养物提供了一种有效的方法。这些EBEC培养物可用于研究紧密连接的形成或鉴定上皮来源的炎性因子,这些因子会导致肺部疾病,例如哮喘。

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