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Circulation Research. 1997;80:720-729

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(Circulation Research. 1997;80:720-729.)
© 1997 American Heart Association, Inc.


Articles

C2 Region–Derived Peptides of ß-Protein Kinase C Regulate Cardiac Ca2+ Channels

Zhi-Hao Zhang, John A. Johnson, Long Chen, Nabil El-Sherif, Daria Mochly-Rosen, , Mohamed Boutjdir

From the Cardiology Division (Z.-H.Z., L.C., N.E.-S., M.B.), Department of Medicine, State University of New York, Health Science Center, and the Veterans Administration Medical Center, Brooklyn, New York, and the Department of Molecular Pharmacology (J.A.J., D.M.-R.), Stanford (Calif) University School of Medicine.

Correspondence to Dr Mohamed Boutjdir, Cardiology Division (IIIA), VA Medical Center, 800 Poly Place, Brooklyn, NY 11209. E-mail boutjdir.mohamed{at}brooklyn.va.gov

Abstract We have previously shown that {alpha}1-adrenergic activation inhibited ß-adrenergic–stimulated L-type Ca2+ current (ICa). To determine the role of protein kinase C (PKC) in this regulation, the inositol trisphosphate pathway was bypassed by direct activation of PKC with 4ß-phorbol 12-myristate 13-acetate (PMA). To minimize Ca2+-induced Ca2+ inactivation, Ba2+ current (IBa) was recorded through Ca2+ channels in adult rat ventricular myocytes. We found that PMA (0.1 µmol/L) consistently inhibited basal IBa by 40.5±7.4% and isoproterenol (ISO, 0.1 µmol/L)–stimulated IBa by 48.9±7.8%. These inhibitory effects were not observed with the inactive phorbol ester analogue {alpha}-phorbol 12,13-didecanoate (0.1 µmol/L). To identify the PKC isozymes that mediate these PMA effects, we intracellularly applied peptide inhibitors of a subclass of PKC isozymes, the C2-containing cPKCs. These peptides (ßC2-2 and ßC2-4) specifically inhibit the translocation and function of C2-containing isozymes ({alpha}-PKC, ßI-PKC, and ßII-PKC), but not the C2-less isozymes ({delta}-PKC and {epsilon}-PKC). We first used the pseudosubstrate peptide (0.1 µmol/L in the pipette), which inhibits the catalytic activity of all the PKC isozymes, and found that PMA-induced inhibition of ISO-stimulated IBa was reduced to 16.8±7.4% but was not affected by the scrambled pseudosubstrate peptide. The effects of PMA on basal and ISO-stimulated IBa were then determined in the presence of C2-derived peptides or control peptides. When the pipette contained 0.1 µmol/L of ßC2-2 or ßC2-4, PMA-induced inhibition of basal IBa was 26.1±4.5% and 23.6±2.2%, respectively. Similarly, ISO-stimulated IBa was inhibited by 29.9±6.6% and 29.3±7.8% in the presence of ßC2-2 and ßC2-4, respectively. In contrast, there was no significant change in the effect of PMA in the presence of control peptides, scrambled ßC2-4, or pentalysine. Finally, PMA-induced inhibition of basal and ISO-stimulated IBa was almost completely abolished in cells dialyzed with both ßC2-2 and ßC2-4. Together, these data suggest a role for C2-containing isozymes in mediating PMA-induced inhibition of L-type Ca2+ channel activity.


Key Words: Ca2+ current • receptor • phorbol ester • protein kinase C isozyme • cardiac myocyte




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