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  3. Characterization of pediatric cystic fibrosis airway epithelial cell cultures at the air-liquid interface obtained by non-invasive nasal cytology brush sampling.
 

Characterization of pediatric cystic fibrosis airway epithelial cell cultures at the air-liquid interface obtained by non-invasive nasal cytology brush sampling.

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BORIS DOI
10.7892/boris.108529
Date of Publication
December 28, 2017
Publication Type
Article
Division/Institute

Department for BioMed...

Institut für Anatomie...

Universitätsklinik fü...

Department of Infecti...

Department for BioMed...

Author
Schögler, Aline
Blank, Fabian
Department for BioMedical Research, Live Cell Imaging (LCI)
Brügger, Melanie
Beyeler, Seraina Martina
Department for BioMedical Research, Forschungsgruppe Pneumologie (Erwachsene)
Universitätsklinik für Pneumologie
Tschanz, Stefan A.orcid-logo
Institut für Anatomie
Regamey, Nicolas
Casaulta, Carmenorcid-logo
Universitätsklinik für Kinderheilkunde
Geiser, Thomas
Department for BioMedical Research, Forschungsgruppe Pneumologie (Erwachsene)
Universitätsklinik für Pneumologie
Alves, Marco
Department of Infectious Diseases and Pathobiology (DIP)
Subject(s)

600 - Technology::630...

600 - Technology::610...

Series
Respiratory research
ISSN or ISBN (if monograph)
1465-9921
Publisher
BioMed Central
Language
English
Publisher DOI
10.1186/s12931-017-0706-7
PubMed ID
29282053
Uncontrolled Keywords

Air-liquid interface ...

Description
BACKGROUND

In vitro systems of primary cystic fibrosis (CF) airway epithelial cells are an important tool to study molecular and functional features of the native respiratory epithelium. However, undifferentiated CF airway cell cultures grown under submerged conditions do not appropriately represent the physiological situation. A more advanced CF cell culture system based on airway epithelial cells grown at the air-liquid interface (ALI) recapitulates most of the in vivo-like properties but requires the use of invasive sampling methods. In this study, we describe a detailed characterization of fully differentiated primary CF airway epithelial cells obtained by non-invasive nasal brushing of pediatric patients.

METHODS

Differentiated cell cultures were evaluated with immunolabelling of markers for ciliated, mucus-secreting and basal cells, and tight junction and CFTR proteins. Epithelial morphology and ultrastructure was examined by histology and transmission electron microscopy. Ciliary beat frequency was investigated by a video-microscopy approach and trans-epithelial electrical resistance was assessed with an epithelial Volt-Ohm meter system. Finally, epithelial permeability was analysed by using a cell layer integrity test and baseline cytokine levels where measured by an enzyme-linked immunosorbent assay.

RESULTS

Pediatric CF nasal cultures grown at the ALI showed a differentiation into a pseudostratified epithelium with a mucociliary phenotype. Also, immunofluorescence analysis revealed the presence of ciliated, mucus-secreting and basal cells and tight junctions. CFTR protein expression was observed in CF (F508del/F508del) and healthy cultures and baseline interleukin (IL)-8 and IL-6 release were similar in control and CF ALI cultures. The ciliary beat frequency was 9.67 Hz and the differentiated pediatric CF epithelium was found to be functionally tight.

CONCLUSION

In summary, primary pediatric CF nasal epithelial cell cultures grown at the ALI showed full differentiation into ciliated, mucus-producing and basal cells, which adequately reflect the in vivo properties of the human respiratory epithelium.
Handle
https://boris-portal.unibe.ch/handle/20.500.12422/199630
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s12931-017-0706-7.pdftextAdobe PDF3.23 MBpublishedOpen
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