4.6 Article

The development and characterization of in vivo-like three-dimensional models of bronchial epithelial cell lines

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DOI: 10.1016/j.ejps.2023.106567

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Three-dimensional cell culture models; Bronchial epithelial cells; Rotating wall vessel bioreactor; Organotypic; Differentiation; Cystic fibrosis

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In vitro models of differentiated respiratory epithelium are crucial for exploring new therapeutics for chronic respiratory diseases. This study developed three-dimensional models of bronchial epithelial cell lines that closely resemble the in vivo tissue. The models were compared to traditional two-dimensional cultures and air-liquid interface cultures, and showed promising potential as an alternative for in vivo studies.
In vitro models of differentiated respiratory epithelium that allow high-throughput screening are an important tool to explore new therapeutics for chronic respiratory diseases. In the present study, we developed in vivo-like three-dimensional (3-D) models of bronchial epithelial cell lines that are commonly used to study chronic lung disease (16HBE14o , CFBE41o  and CFBE41o  6.2 WT-CFTR). To this end, cells were cultured on porous microcarrier beads in the rotating wall vessel (RWV) bioreactor, an optimized suspension culture method that allows higher throughput experimentation than other physiologically relevant models. Cell differentiation was compared to conventional two-dimensional (2-D) monolayer cultures and to the current gold standard in the respiratory field, i.e. air-liquid interface (ALI) cultures. Cellular differentiation was assessed in the three model systems by evaluating the expression and localization of markers that reflect the formation of tight junctions (zonula occludens 1), cell polarity (intercellular adhesion molecule 1 at the apical side and collagen IV expression at the basal cell side), multicellular complexity (acetylated & alpha;-tubulin for ciliated cells, CC10 for club cells, keratin-5 for basal cells) and mucus production (MUC5AC) through immunostaining and confocal laser scanning microscopy. Results were validated using Western Blot analysis. We found that tight junctions were expressed in 2-D monolayers, ALI cultures and 3-D models for all three cell lines. All tested bronchial epithelial cell lines showed polarization in ALI and 3-D cultures, but not in 2-D monolayers. Mucus secreting goblet-like cells were present in ALI and 3-D cultures of CFBE41o  and CFBE41o  6.2 WT-CFTR cells, but not in 16HBE14o  cells. For all cell lines, there were no ciliated cells, basal cells, or club cells found in any of the model systems. In conclusion, we developed RWV-derived 3-D models of commonly used bronchial epithelial cell lines and showed that these models are a valuable alternative to ALI cultures, as they recapitulate similar key aspects of the in vivo parental tissue.

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