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Published ahead of print on November 7, 2007, doi:10.1165/rcmb.2007-0177OC

Am. J. Respir. Cell Mol. Biol., Volume 38, Number 4, April 2008, 423-434

A more recent version of this article appeared on April 1, 2008
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Submitted on May 17, 2007
Revised on October 25, 2007

Modelling Dysregulated Na+ Absorption in Airway Epithelial Cells with Mucosal Nystatin Treatment

Alessandra Livraghi1*, Marcus Mall2, Anthony M Paradiso1, Richard C Boucher3, and Carla M Pedrosa Ribeiro3

1 The University of North Carolina at Chapel Hill, Cystic Fibrosis/Pulmonary Research and Treatment Center, Chapel Hill, NC, USA, 2 Department of Pediatrics III, University of Heidelberg, Pediatric Pulmonology and Cystic Fibrosis Center, Heidelberg, Germany, 3 The University of North Carolina at Chapel Hill, Cystic Fibrosis/Pulmonary Research and Treatment Center, Chapel Hill, NC, USA; Department of Medicine, University of North Carolina at Chapel Hill, Chapel Hill, NC, USA

* To whom correspondence should be addressed. E-mail: alessandra_livraghi{at}med.unc.edu.

In cystic fibrosis (CF), the absence of functional CFTR leads to dysregulated Na+ absorption across airway epithelia. We established an in vitro model of dysregulated Na+ absorption by treating polarized normal human bronchial epithelial cells (HBEs) with nystatin (Nys), a polyene antibiotic that enables monovalent cations to permeate biological membranes. Acute mucosal Nys produced a rapid increase in short circuit current (Isc) that reflected increased transepithelial Na+ absorption and required Na+/K+ATPase activity. The acute increase in Isc was associated with increased mucosal liquid absorption. Prolonged mucosal Nys treatment resulted in sustained Na+ hyperabsorption, associated with increased mucosal liquid absorption in comparison to naive (non-treated, kept under air-liquid interface conditions) or vehicle-treated cultures. Nys treatment was not toxic. Increased lactate accumulation in Nys-treated culture media suggested a higher metabolic rate associated with the higher energy demand for Na+ transport. After chronic Nys treatment, the increased Isc was rapidly lost when the cultures where mounted in Ussing chambers, indicating that Nys could be rapidly removed from the apical membrane. Importantly, chronic Nys treatment promoted sustained mucosal liquid depletion and caused mucus dehydration, compaction and adhesion to the apical surface of Nys-treated cultures. We conclude that mucosal Nys treatment of HBEs provides a simple in vitro model to recapitulate the Na+ and volume hyperabsorptive features of CF airway epithelia.




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