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Literature DB >> 1335510

Phosphorylation restores activity of L-type calcium channels after rundown in inside-out patches from rabbit cardiac cells.

Abstract

1. Rundown of L-type calcium channels was studied in inside-out patches made from single isolated rabbit ventricular myocytes, using barium as the charge carrier. 2. In the cell-attached patches single-channel activity was stable for more than 15 min after the patch pipette sealed. beta-Receptor stimulation by isoprenaline caused a characteristic increase in opening probability and the appearance of prolonged openings. When the patch was excised to the inside-out configuration and exposed to a simple ionic solution, channel activity disappeared within 1-2 min and never reappeared spontaneously. 3. After rundown of L-type channel activity in the excised patch, exposure of the inside face of the patch to MgATP and the catalytic subunit of the cyclic AMP-dependent protein kinase (PKAc) resulted in recovery of Ca2+ channel activity. Under these conditions channel activity could be even greater than under control cell-attached conditions, resembling channel activity after exposure to isoprenaline. This recovery of activity persisted many minutes, usually until the patch was lost. Addition of MgATP alone caused a small transient increase in channel activity in some patches. 4. Recovery of activity by MgATP and PKAc could be prevented by prior exposure of the excised patch to protein kinase inhibitor (PKI), or it could be abruptly terminated by exposure to PKI after recovery of activity. Addition to the pipette solution of okadaic acid, a protein phosphatase inhibitor, greatly slowed rundown. These findings support the proposal that dephosphorylation is an important component of rundown, and that phosphorylation is needed for channel opening activity. 5. Single-channel conductance was not altered by patch excision, but it was reduced after exposure of the excised patch to MgATP and PKAc. Mg2+ was responsible for this effect, probably by direct channel block from the inside, and Mg2+ also caused a negative shift in the channel activation, as expected from shielding of inside fixed negative charges.

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Year: 1992 PMID： 1335510 PMCID： PMC1175627 DOI： 10.1113/jphysiol.1992.sp019286

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

35 in total

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

Authors: H C Hartzell; R E White
Journal: J Gen Physiol Date: 1989-10 Impact factor: 4.086

2. Alpha-subunit of Gs directly activates cardiac calcium channels in lipid bilayers.

Authors: Y Imoto; A Yatani; J P Reeves; J Codina; L Birnbaumer; A M Brown
Journal: Am J Physiol Date: 1988-10

Review 3. Calcium channel.

Authors: S Hagiwara; L Byerly
Journal: Annu Rev Neurosci Date: 1981 Impact factor: 12.449

4. Effects of a protein phosphatase inhibitor, okadaic acid, on membrane currents of isolated guinea-pig cardiac myocytes.

Authors: J Hescheler; G Mieskes; J C Rüegg; A Takai; W Trautwein
Journal: Pflugers Arch Date: 1988-08 Impact factor: 3.657

5. The kinetics of transport of lactate and pyruvate into isolated cardiac myocytes from guinea pig. Kinetic evidence for the presence of a carrier distinct from that in erythrocytes and hepatocytes.

Authors: R C Poole; A P Halestrap; S J Price; A J Levi
Journal: Biochem J Date: 1989-12-01 Impact factor: 3.857

6. Regulation of Ca2+-dependent K+-channel activity in tracheal myocytes by phosphorylation.

Authors: H Kume; A Takai; H Tokuno; T Tomita
Journal: Nature Date: 1989-09-14 Impact factor: 49.962

7. Localization of beta adrenergic receptors, and effects of noradrenaline and cyclic nucleotides on action potentials, ionic currents and tension in mammalian cardiac muscle.

Authors: H Reuter
Journal: J Physiol Date: 1974-10 Impact factor: 5.182

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
Journal: Pflugers Arch Date: 1995-05 Impact factor: 3.657

Phosphorylation restores activity of L-type calcium channels after rundown in inside-out patches from rabbit cardiac cells.

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

2. Alpha-subunit of Gs directly activates cardiac calcium channels in lipid bilayers.

Review 3. Calcium channel.

4. Effects of a protein phosphatase inhibitor, okadaic acid, on membrane currents of isolated guinea-pig cardiac myocytes.

5. The kinetics of transport of lactate and pyruvate into isolated cardiac myocytes from guinea pig. Kinetic evidence for the presence of a carrier distinct from that in erythrocytes and hepatocytes.

6. Regulation of Ca2+-dependent K+-channel activity in tracheal myocytes by phosphorylation.

7. Localization of beta adrenergic receptors, and effects of noradrenaline and cyclic nucleotides on action potentials, ionic currents and tension in mammalian cardiac muscle.

8. Inhibition of the calcium channel by intracellular protons in single ventricular myocytes of the guinea-pig.

9. Effects of membrane surface charge and calcium on the gating of rat brain sodium channels in planar bilayers.

10. Ionic blockage of sodium channels in nerve.

1. Molecular determinant for run-down of L-type Ca2+ channels localized in the carboxyl terminus of the 1C subunit.

2. Ion concentration-dependence of rat cardiac unitary L-type calcium channel conductance.

3. Mechanosensitivity of N-type calcium channel currents.

4. Slow deactivation and U-shaped inactivation properties in cloned Cav1.2b channels in Chinese hamster ovary cells.

Review 5. Regulation of L-type Ca2+ channels in the heart: overview of recent advances.

6. A single amino acid mutation attenuates rundown of voltage-gated calcium channels.

7. Phosphatidylinositol 4,5-bisphosphate (PIP₂) and Ca²⁺ are both required to open the Cl^- channel TMEM16A.

8. Regulation of the calcium slow channel by cyclic GMP dependent protein kinase in chick heart cells.

9. Role of calmodulin in the activation of carbachol-activated cationic current in guinea-pig gastric antral myocytes.

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.