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secretion in
cystic fibrosis epithelial cells by an analog of squalamine
1 Genzyme Corporation, Framingham 01701-9322; and 2 Department of Medicine, Beth Israel Deaconess Medical Center, Harvard Medical School, Boston, Massachusetts 02215
Defective
cystic fibrosis (CF) transmembrane conductance regulator
(CFTR)-mediated Cl
transport across the apical membrane
of airway epithelial cells is implicated in the pathophysiology of CF
lungs. A strategy to compensate for this loss is to augment
Cl
transport through alternative pathways. We report here
that partial correction of this defect could be attained through the
incorporation of artificial anion channels into the CF cells.
Introduction of GL-172, a synthetic analog of squalamine, into CFT1
cells increased cell membrane halide permeability. Furthermore, when a
Cl
gradient was generated across polarized monolayers of
primary human airway or Fischer rat thyroid cells in an Ussing chamber, addition of GL-172 caused an increase in the equivalent short-circuit current. The magnitude of this change in short-circuit current was
~30% of that attained when CFTR was maximally stimulated with cAMP
agonists. Patch-clamp studies showed that addition of GL-172 to CFT1
cells also increased whole cell Cl
currents. These
currents displayed a linear current-voltage relationship and no time
dependence. Additionally, administration of GL-172 to the nasal
epithelium of transgenic CF mice induced a hyperpolarization response
to perfusion with a low-Cl
solution, indicating
restoration of Cl
secretion. Together, these
results demonstrate that in CF airway epithelial cells, administration
of GL-172 is capable of partially correcting the defective
Cl
secretion.
cystic fibrosis transmembrane conductance regulator; nasal potential difference; Ussing chamber; whole cell patch clamp; chloride ion
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