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Address correspondence to Michael D. Cahalan, Department of Physiology and Biophysics, University of California, Irvine, CA 92697-4561. Fax: 949-824-3143; E-mail: mcahalan{at}uci.edu
In rat basophilic leukemia (RBL) cells and Jurkat T cells, Ca2+ releaseactivated Ca2+ (CRAC) channels open in response to passive Ca2+ store depletion. Inwardly rectifying CRAC channels admit monovalent cations when external divalent ions are removed. Removal of internal Mg2+ exposes an outwardly rectifying current (Mg2+-inhibited cation [MIC]) that also admits monovalent cations when external divalent ions are removed. Here we demonstrate that CRAC and MIC currents are separable by ion selectivity and rectification properties: by kinetics of activation and susceptibility to run-down and by pharmacological sensitivity to external Mg2+, spermine, and SKF-96365. Importantly, selective run-down of MIC current allowed CRAC and MIC current to be characterized under identical ionic conditions with low internal Mg2+. Removal of internal Mg2+ induced MIC current despite widely varying Ca2+ and EGTA levels, suggesting that Ca2+-store depletion is not involved in activation of MIC channels. Increasing internal Mg2+ from submicromolar to millimolar levels decreased MIC currents without affecting rectification but did not alter CRAC current rectification or amplitudes. External Mg2+ and Cs+ carried current through MIC but not CRAC channels. SKF-96365 blocked CRAC current reversibly but inhibited MIC current irreversibly. At micromolar concentrations, both spermine and extracellular Mg2+ blocked monovalent MIC current reversibly but not monovalent CRAC current. The biophysical characteristics of MIC current match well with cloned and expressed TRPM7 channels. Previous results are reevaluated in terms of separate CRAC and MIC channels.
Key Words: store-operated channel CRAC channel Ca2+ channel TRPM7 cation channel
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