Literature DB >> 2445973

An intrinsic potential-dependent inactivation mechanism associated with calcium channels in guinea-pig myocytes.

R W Hadley1, J R Hume.   

Abstract

1. Currents through Ca2+ channels of single guinea-pig ventricular myocytes were studied using patch electrodes for whole-cell recording. Currents through Na+ and K+ channels were suppressed by the application of drugs or the substitution of impermeant ions. 2. Inactivation of the Ca2+ current (ICa) was investigated using a two-pulse protocol. The amount of inactivation left behind by a pre-pulse appeared to be related to current magnitude, as others have reported. The dependence of inactivation on the pre-pulse potential was partially U-shaped, as the amount of inactivation peaked at 0 mV and then declined with more positive pre-pulses. 3. Non-specific current carried by monovalent ions through Ca2+ channels (Ins) was induced by lowering the extracellular Ca2+ concentration with EGTA. Ins peaked in an inward direction at -20 mV, reversed direction at +22 mV, and became a large outward current at more positive potentials. 4. Ins inactivated with a slow time course. The inactivation was not due to accumulation or depletion phenomena. Studies using two-pulse protocols showed that the amount of inactivation left by a pre-pulse was directly related to the pre-pulse potential. 5. The addition of micromolar amounts of free Ca2+ to the external solution induced outward rectification of Ins. Inward currents were small or absent, while larger outward currents could still be seen at very positive potentials. Ca2+-channel inactivation still occurred under these conditions, even in the absence of any significant ionic movement. 6. The time courses of Ins inactivation and recovery were studied. The half-time of Ins inactivation decreased with larger depolarizations. Recovery of Ins was very slow, but could be accounted for by changes in the surface charge of the membrane. 7. It is concluded that Ins inactivation is due solely to a voltage-dependent inactivation process which is intrinsic to myocardial Ca2+ channels. Voltage-dependent inactivation appears to account for a significant proportion of total Ca2+-channel inactivation at negative potentials, and appears to account for almost all of the inactivation at very positive potentials, even in the presence of millimolar concentration of external Ca2+.

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Year:  1987        PMID: 2445973      PMCID: PMC1192078          DOI: 10.1113/jphysiol.1987.sp016654

Source DB:  PubMed          Journal:  J Physiol        ISSN: 0022-3751            Impact factor:   5.182


  38 in total

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3.  High selectivity of calcium channels in single dialysed heart cells of the guinea-pig.

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4.  Non-selective conductance in calcium channels of frog muscle: calcium selectivity in a single-file pore.

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6.  Calcium entry leads to inactivation of calcium channel in Paramecium.

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7.  Kinetics of inactivation and recovery of the slow inward current in the mammalian ventricular myocardium.

Authors:  M Kohlhardt; H Krause; M Kübler; A Herdey
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8.  A non-selective cation conductance in frog muscle membrane blocked by micromolar external calcium ions.

Authors:  W Almers; E W McCleskey; P T Palade
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9.  The calcium and frequency dependence of the slow inward current 'staircase' in frog atrium.

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10.  Voltage-dependent inactivation of a calcium channel.

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  58 in total

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3.  Effects of magnesium on inactivation of the voltage-gated calcium current in cardiac myocytes.

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5.  Effects of the enantiomers of BayK 8644 on the charge movement of L-type Ca channels in guinea-pig ventricular myocytes.

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8.  Theoretical study of L-type Ca(2+) current inactivation kinetics during action potential repolarization and early afterdepolarizations.

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9.  Control of L-type calcium current during the action potential of guinea-pig ventricular myocytes.

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10.  The effect of a chemical phosphatase on single calcium channels and the inactivation of whole-cell calcium current from isolated guinea-pig ventricular myocytes.

Authors:  T J Allen; R A Chapman
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