DNA Stability, Regeneration Capacity, and Mucociliary Differentiation of Human Nasal Mucosa Cells in Tissue Systems

Pascal Ickrath; Katrin Ickrath; Maria Steinke; Agmal Scherzad; Norbert Kleinsasser; Nina Lodes; Maximilian Bregenzer; Rudolf Hagen; Stephan Hackenberg

doi:10.1089/ten.TEA.2020.0089

DNA Stability, Regeneration Capacity, and Mucociliary Differentiation of Human Nasal Mucosa Cells in Tissue Systems

Tissue Eng Part A. 2020 Nov;26(21-22):1199-1208. doi: 10.1089/ten.TEA.2020.0089. Epub 2020 Jul 28.

Authors

Pascal Ickrath¹, Katrin Ickrath¹, Maria Steinke², Agmal Scherzad¹, Norbert Kleinsasser³, Nina Lodes², Maximilian Bregenzer¹, Rudolf Hagen¹, Stephan Hackenberg¹

Affiliations

¹ Department of Oto-Rhino-Laryngology, Plastic, Aesthetic and Reconstructive Head and Neck Surgery, University of Würzburg, Würzburg, Germany.
² Chair of Tissue Engineering and Regenerative Medicine, University Hospital Wuerzburg, Würzburg, Germany.
³ Department of Otorhinolaryngology, Head and Neck Surgery, Kepler University Hospital, Linz, Austria.

PMID: 32524916
DOI: 10.1089/ten.TEA.2020.0089

Abstract

For culture models of primary cells of the human nasal mucosa, monocultures with epithelial cells (ECs) are used as well as cocultures with ECs and fibroblasts (FBs). Well-differentiated models of the respiratory nasal epithelium can be used for ecogenotoxicological assessments, for experiments on host/pathogen interactions, or tissue engineering. However, long-term cultivation and repeated passaging may induce a loss of DNA integrity or cell functionality. The aim of this study was to evaluate these parameters in test systems created from primary nasal mucosa cells. Enzymatic and sequential cell isolation from nasal tissue was performed. EC monocultures and compartment-separated EC-FB cocultures were cultivated over three passages under air/liquid interface conditions. DNA stability and regenerative capacity at the DNA and chromosomal level as well as proliferation and cell differentiation were examined. Both methods showed equivalent levels of DNA stability and regenerative capacity over all passages. Sequential growth of the coculture provided higher cell purity, while enzymatic cell harvest was associated with FB contamination in EC culture. Mucociliary differentiation was verified with electron microscopy in both methods. Functionality measured by lipopolysaccharide stimulation of interleukins was constant over long-term cultivation. Our data confirm DNA stability in long-term cell cultivation as well as functional integrity in both culture methods. Sequential cell isolation should be favored over enzymatic isolation due to higher culture purity. Impact statement Cell culture models are frequently used for ecogenotoxicological assessments, for experiments on host/pathogen interactions, or tissue engineering. However, DNA stability and functional integrity after long-term cultivation in such tissue models have not been investigated, yet. This study is the first showing systematic and evident data on DNA damage and functional aspects in primary human cell culture models of nasal epithelium.

Keywords: DNA stability; coculture; epithelial cell models; human nasal mucosa; tissue system.

MeSH terms

Cell Culture Techniques
Cell Differentiation
Cells, Cultured
DNA Damage*
Epithelial Cells / cytology*
Humans
Nasal Mucosa* / cytology
Regeneration