Human airway epithelia (HAE) cells (Lonza; cat# CC-2540S) are available in our laboratory and routinely cultured in air–liquid interface (ALI) as described (15 (link), 35 (link)). Briefly, cells were cultured in a T75 flask using Pneuma Cult Ex Plus medium (Stemcell; cat# 05040) supplemented with hydrocortisone (Stemcell; cat# 07980) for 2–4 d until they reached 80% confluence. The cells were dissociated with an Animal Component-Free Cell Dissociation Kit (Stemcell; cat# 05426) and seeded onto collagen-coated 0.33 cm2 porous (0.4 µm) polyester membrane inserts with a seeding density of 1 × 105 cells per Transwell. The cells were grown to near confluence in submerged culture for 2–3 d in Pneuma Cult Ex Plus medium supplemented with hydrocortisone. Cultures were maintained in a humidified atmosphere with 5% CO2 at 37°C and then transferred to ALI culture. The epithelium was expanded and differentiated using Pneuma Cult ALI medium (Stemcell; cat# 05021) supplemented with hydrocortisone and 0.2% heparin solution (Provitro; cat#0863). The number of days in development was designated relative to initiation of ALI culture, corresponding to day 0.
Hae cells
Manufactured by Lonza
HAE) cells are a type of human airway epithelial cell line used in laboratory research. They are primary cells derived from the human airway epithelium and are commonly used as an in vitro model for studying various respiratory functions and processes.
Automatically generated - may contain errors
2 protocols using hae cells
1
Human Airway Epithelial (HAE) Cell Culture Protocol
2
Human Airway Epithelial (HAE) Cell Culture Protocol
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Human airway epithelia (HAE) cells (Lonza; cat# CC-2540S) are available in our laboratory and routinely cultured in air–liquid interface (ALI) as described (15 (link), 35 (link)). Briefly, cells were cultured in a T75 flask using Pneuma Cult Ex Plus medium (Stemcell; cat# 05040) supplemented with hydrocortisone (Stemcell; cat# 07980) for 2–4 d until they reached 80% confluence. The cells were dissociated with an Animal Component-Free Cell Dissociation Kit (Stemcell; cat# 05426) and seeded onto collagen-coated 0.33 cm2 porous (0.4 µm) polyester membrane inserts with a seeding density of 1 × 105 cells per Transwell. The cells were grown to near confluence in submerged culture for 2–3 d in Pneuma Cult Ex Plus medium supplemented with hydrocortisone. Cultures were maintained in a humidified atmosphere with 5% CO2 at 37°C and then transferred to ALI culture. The epithelium was expanded and differentiated using Pneuma Cult ALI medium (Stemcell; cat# 05021) supplemented with hydrocortisone and 0.2% heparin solution (Provitro; cat#0863). The number of days in development was designated relative to initiation of ALI culture, corresponding to day 0.
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