4.1 Article

Determinants of culture success in an airway epithelium sampling program of young children with cystic fibrosis

Journal

EXPERIMENTAL LUNG RESEARCH
Volume 40, Issue 9, Pages 447-459

Publisher

TAYLOR & FRANCIS INC
DOI: 10.3109/01902148.2014.946631

Keywords

airway; bronchial brushing; cell culture; cystic fibrosis; epithelium

Funding

  1. Cystic Fibrosis Foundation Therapeutics [SLY04A0, STICK09A0]
  2. National Health and Medical Research Council (Australia) (Centres of Research Excellence) [1000896]
  3. National Health and Medical Research Council (Australia)
  4. Cystic Fibrosis Australia
  5. Australian Respiratory Council
  6. University of Western Australia

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Aim of the study: The bronchial brushing technique presents an opportunity to establish a gold standard in vitro model of Cystic Fibrosis (CF) airway disease. However, unique obstacles exist when establishing CF airway epithelial cells (pAEC(CF)). We aimed to identify determinants of culture success through retrospective analysis of a program of routinely brushing children with CF. Materials and methods: Anaesthetised children (CF and non-CF) had airway samples taken which were immediately processed for cell culture. Airway data for the CF cohort was obtained from clinical records and the AREST CF database. Results: Of 260 brushings processed for culture, 114 (43.8%) pAECCF successfully cultured to passage one (P1) and 63 (24.2% of total) progressed to passage two (P2). However, >80% of non-CF specimens (pAEC(non-CF)) cultured to P2 from similar cell numbers. Within the CF cohort, specimens successfully cultured to P2 had a higher initial cell count and lower proportion of severe CF mutation phenotype than those that did not proliferate beyond initial seeding. Elevated airway IL-8 concentration was also negatively associated with culture establishment. Contamination by opportunistic pathogens was observed in 81 (31.2% of total) cultures and brushings from children with lower respiratory tract infections were more likely to co-culture contaminating flora. Conclusions: Lower passage rates of pAEC(CF) cultures uniquely contrasts with pAEC(non-CF) despite similar cell numbers. An equivalent establishment rate of CF nasal epithelium reported elsewhere, significant associations to CFTR mutation phenotype, elevated airway IL-8 and opportunistic pathogens all suggest this is likely related to the CF disease milieu.

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