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MBC in Press, published online ahead of print February 16, 2005
Mol. Biol. Cell 10.1091/mbc.E04-11-1010

A more recent version of this article appeared on May 1, 2005
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Submitted on November 17, 2004
Revised on January 31, 2005
Accepted on February 9, 2005

Characterization of Wild-Type and {Delta}F508 Cystic Fibrosis Transmembrane Regulator in Human Respiratory Epithelia

Silvia M. Kreda,* Marcus Mall,* April Mengos,{dagger} Lori Rochelle,* James Yankaskas,* John R. Riordan,{dagger}{ddagger} and Richard C. Boucher*{ddagger}

*Cystic Fibrosis/Pulmonary Research and Treatment Center, School of Medicine, The University of North Carolina at Chapel Hill, Chapel Hill, NC 27599-7248; {dagger}Mayo Foundation, S. C. Johnson Medical Research Center, Mayo Clinic Scottsdale, Scottsdale, AZ 85259

Monitoring Editor: Keith Mostov

Previous studies in native tissues have produced conflicting data on the localization and metabolic fate of WT and {Delta}F508 cystic fibrosis transmembrane regulator (CFTR) in the lung. Combining immunocytochemical and biochemical studies utilizing new high-affinity CFTR mAbs with ion transport assays, we examined both (1) the cell type and region specific expression of CFTR in normal airways and (2) the metabolic fate of {Delta}F508 CFTR and associated ERM proteins in the cystic fibrosis lung. Studies of lungs from a large number of normal subjects revealed that WT CFTR protein localized to the apical membrane of ciliated cells within the superficial epithelium and gland ducts. In contrast, other cell types in the superficial, gland acinar, and alveolar epithelia expressed little WT CFTR protein. No {Delta}F508 CFTR mature protein or function could be detected in airway specimens freshly excised from a large number of {Delta}F508 homozygous subjects, despite an intact ERM complex. In sum, our data demonstrate that WT CFTR is predominantly expressed in ciliated cells, and {Delta}F508 CFTR pathogenesis in native tissues, like heterologous cells, reflects loss of normal protein processing.


{ddagger}These authors contributed equally to this work.

Address correspondence to: Silvia M. Kreda (silkre{at}med.unc.edu)




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