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Literature DB >> 10200424

One calcium ion may suffice to open the tetrameric cardiac ryanodine receptor in rat ventricular myocytes.

Abstract

1. The release of Ca2+ from sarcoplasmic reticulum in response to Ca2+ entering through L-type Ca2+ channels was studied in isolated voltage clamped rat ventricular myocytes at room temperature using the fluorescent Ca2+ indicators fluo-3 and Oregon Green 488 Bapta 5N. 2. Depolarizations to positive potentials elicited fluo-3 Ca2+ transients with rates of rise that were linearly related to the magnitude of the peak measured Ca2+ current in the presence of Cs+-containing pipette solutions. 3. Further experiments utilizing prepulses to preactivate a constant number of channels also revealed a linear relationship between the Ca2+ transient rate of rise and the magnitude of entering Ca2+ current at positive potentials. Under these conditions as well, the maximal rates of rise of global myoplasmic Ca2+ transients were due primarily to Ca2+ release from the sarcoplasmic reticulum as revealed by effects of ryanodine and caffeine on the Ca2+ transients. Using such prepulses, linearity between the Ca2+ transient rate of rise and the magnitude of the peak Ca2+ current was found under a variety of pulse protocols. 4. Using one such pulse protocol, linearity between the Ca2+ transient rate of rise and the magnitude of the peak Ca2+ current was also found when Ca2+ currents assessed at one potential were reduced in magnitude during the onset of block by application of Co2+. Using the same pulse protocol, linearity between the Ca2+ transient rate of rise and the magnitude of the peak Ca2+ current was also found when use of Cs+ was avoided by blocking K+ currents with extracellular TEA and 4-aminopyridine. Linearity in the relationship between the Ca2+ transient rate of rise and the magnitude of the peak Ca2+ current was also found when Ca2+ transients were measured using the low affinity Ca2+ indicator Oregon Green 488 Bapta 5N in place of fluo-3. 5. These results appear to indicate that the cardiac ryanodine receptor is capable of being activated by only one calcium ion. Alternative interpretations of the data are discussed.

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Year: 1999 PMID： 10200424 PMCID： PMC2269301 DOI： 10.1111/j.1469-7793.1999.0769u.x

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

32 in total

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Journal: Biophys J Date: 1992-08 Impact factor: 4.033

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Journal: Pflugers Arch Date: 1982-10 Impact factor: 3.657

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Journal: J Physiol Date: 1988-11 Impact factor: 5.182

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Journal: Biophys J Date: 1992-05 Impact factor: 4.033

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Journal: J Biol Chem Date: 1987-03-05 Impact factor: 5.157

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Journal: J Cell Biol Date: 1988-12 Impact factor: 10.539

5 in total

1. A model of the L-type Ca2+ channel in rat ventricular myocytes: ion selectivity and inactivation mechanisms.

Authors: L Sun; J S Fan; J W Clark; P T Palade
Journal: J Physiol Date: 2000-11-15 Impact factor: 5.182

2. Effects of FPL 64176 on Ca transients in voltage-clamped rat ventricular myocytes.

Authors: Jing-Song Fan; Philip Palade
Journal: Br J Pharmacol Date: 2002-03 Impact factor: 8.739

3. Modeling CICR in rat ventricular myocytes: voltage clamp studies.

Authors: Abhilash Krishna; Liang Sun; Miguel Valderrábano; Philip T Palade; John W Clark
Journal: Theor Biol Med Model Date: 2010-11-10 Impact factor: 2.432

Review 4. Chemical calcium indicators.

Authors: R Madelaine Paredes; Julie C Etzler; Lora Talley Watts; Wei Zheng; James D Lechleiter
Journal: Methods Date: 2008-10-16 Impact factor: 3.608

5. Voltage-dependent Ca2+ release from the SR of feline ventricular myocytes is explained by Ca2+-induced Ca2+ release.

Authors: V Piacentino; K Dipla; J P Gaughan; S R Houser
Journal: J Physiol Date: 2000-03-15 Impact factor: 5.182

5 in total