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Direct effects of 9-anthracene compounds on cystic fibrosis transmembrane conductance regulator gating
Authors:Tomohiko Ai  Silvia G. Bompadre  Yoshiro Sohma  Xiaohui Wang  Min Li  Tzyh-Chang Hwang
Affiliation:(1) Department of Medical Pharmacology and Physiology, Dalton Cardiovascular Research Center, University of Missouri-Columbia, MO 65211, USA;(2) Department of Physiology, Osaka Medical College, Takatsuki, 569-0081 Osaka, Japan;(3) Cardiac Electrophysiology Research Laboratory, Texas Heart Institute, St Luke"rsquo"s Episcopal Hospital, Houston, TX 77030, USA
Abstract:
Anthracene-9-carboxylic acid (9-AC) has been reported to show both potentiation and inhibitory effects on guinea-pig cardiac cAMP-activated chloride channels via two different binding sites, and inhibition of Mg2+-sensitive protein phosphatases has been proposed for the mechanism of 9-AC potentiation effect. In this study, we examined the effects of 9-AC on wild-type and mutant human cystic fibrosis transmembrane conductance regulator (CFTR) chloride channels expressed in NIH3T3 or CHO cells. 9-AC inhibits whole-cell CFTR current in a voltage-dependent manner, whereas the potentiation effect is not affected by membrane potentials. Anthracene-9-methanol, an electro-neutral 9-AC analog, fails to block CFTR, but shows a nearly identical potentiation effect, corroborating the idea that two chemically distinct sites are responsible, respectively, for potentiation and inhibitory actions of 9-AC. 9-AC also enhances the activity of DeltaR-CFTR, a constitutively active CFTR mutant whose R-domain is removed. In excised inside-out patches, 9-AC increases Po by prolonging the mean burst durations and shortening the interburst durations. We therefore conclude that two different 9-AC binding sites for potentiation and inhibitory effects on CFTR channels are located outside of the R-domain. We also speculate that 9-AC potentiates CFTR activity by directly affecting CFTR gating.
Keywords:Chloride channel  Cystic fibrosis  Patch clamp  Single channel
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