cAMP-activated Ca2+ signaling is required for CFTR-mediated serous cell fluid secretion in porcine and human airways
Robert J. Lee, J. Kevin Foskett
Robert J. Lee, J. Kevin Foskett
Published August 25, 2010
Citation Information: J Clin Invest. 2010;120(9):3137-3148. https://doi.org/10.1172/JCI42992.
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Research Article

cAMP-activated Ca2+ signaling is required for CFTR-mediated serous cell fluid secretion in porcine and human airways

Abstract

Cystic fibrosis (CF), which is caused by mutations in CFTR, affects many tissues, including the lung. Submucosal gland serous acinar cells are primary sites of fluid secretion and CFTR expression in the lung. Absence of CFTR in these cells may contribute to CF lung pathogenesis by disrupting fluid secretion. Here, we have isolated primary serous acinar cells from wild-type and CFTR–/– pigs and humans without CF to investigate the cellular mechanisms and regulation of fluid secretion by optical imaging. Porcine and human serous cells secrete fluid in response to vasoactive intestinal polypeptide (VIP) and other agents that raise intracellular cAMP levels; here, we have demonstrated that this requires CFTR and a cAMP-dependent rise in intracellular Ca2+ concentration ([Ca2+]i). Importantly, cAMP induced the release of Ca2+ from InsP3-sensitive Ca2+ stores also responsive to cAMP-independent agonists such as cholinergic, histaminergic, and purinergic agonists that stimulate CFTR-independent fluid secretion. This provides two types of synergism that strongly potentiated cAMP-mediated fluid secretion but differed in their CFTR dependencies. First, CFTR-dependent secretion was strongly potentiated by low VIP and carbachol concentrations that individually were unable to stimulate secretion. Second, higher VIP concentrations more strongly potentiated the [Ca2+]i responses, enabling ineffectual levels of cholinergic stimulation to strongly activate CFTR-independent fluid secretion. These results identify important molecular mechanisms of cAMP-dependent secretion, including a requirement for Ca2+ signaling, and suggest new therapeutic approaches to correct defective submucosal gland secretion in CF.

Authors

Robert J. Lee, J. Kevin Foskett

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Figure 2

VIP-activated porcine serous cell secretion requires CFTR.

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VIP-activated porcine serous cell secretion requires CFTR. (A–B) Microgr...
(AB) Micrographs showing CFTR immunostaining in WT and CFTR–/– porcine tracheal ciliated epithelial cells (A) and serous acini (B). Arrows indicate apical membrane immunofluorescence observed only in WT cells. Scale bars: 5 μm. (C and D) Representative traces showing VIP-evoked (C) and forskolin-evoked (D) volume and [Ca2+]i responses in WT, Het, and CFTR–/– cells. (E) Summary of resting and peak [Ca2+]i. (F) Summary of shrinkage (red) and time to shrinkage (gray) in WT and Het cells. VIP-stimulated shrinkage was 15% ± 1% within 196 ± 15 s (WT; n = 6) and 16% ± 1% within 218 ± 31 s (Het.; n = 6; all values NS). Forskolin-stimulated shrinkage was 16% ± 2% within 228 ± 21 s (WT; n = 14) and 15% ± 2% within 245 ± 18 s (Het.; n = 8; all values NS). (G) Bumetanide (100 μM) did not enhance VIP-evoked shrinkage in CFTR–/– cells.