Literature DB >> 3760814

External Na-independent Ca extrusion in cultured ventricular cells. Magnitude and functional significance.

W H Barry, C A Rasmussen, H Ishida, J H Bridge.   

Abstract

The relative magnitudes and functional significance of Ca extrusion by Na-Ca exchange and by an Nao-independent mechanism were investigated in monolayer cultures of chick embryo ventricular cells. Abrupt exposure of cells in 0-Nao, nominally 0-Cao solution to 20 mM caffeine produced a large contracture (3.94 +/- 0.90 micron of cell shortening) that relaxed with a t1/2 of 8.60 +/- 1.22 s. An abrupt exposure to caffeine plus 140 mM Na resulted in a contracture that was smaller in amplitude (1.53 +/- 0.50 micron) and relaxed much more rapidly (t1/2 = 0.77 +/- 0.09 s). An abrupt exposure to caffeine in 0-Nao solutions produced an increase in 45Ca efflux that persisted for 20 s, and a net loss of Ca content, determined by atomic absorption spectroscopy (AAS), of approximately 4 nmol/mg protein, within 35 s. A comparable net loss of Ca was demonstrated in the presence of 100 microM [Ca]o. The abrupt exposure of cultured cells to 0 Nao in 1.8 mM Ca produced a Ca uptake, estimated with 45Ca, of 3.2 nmol/mg protein X 15 s, but produced no increase in cell Ca content (AAS). In cells in which a 30% increase in Nai was produced by 5 min exposure to 10(-6) M ouabain, the abrupt exposure to 0 Nao produced a Ca uptake of 6 nmol/mg protein X 15 s and an increase in Ca content (AAS) of 4 nmol/mg protein. We conclude that there is an Nao-independent mechanism for Ca extrusion in these cells, presumably a Ca-ATPase Ca pump, with a limited Ca transport capacity of no more than 2 nmol/mg protein X 15 s. This is five times smaller than the demonstrated maximum capacity of the Na-Ca exchanger in these cells. The relaxation of twitch tension in these cells seems to be dependent primarily on sarcoplasmic reticulum uptake of Ca, with a secondary role provided by the Na-Ca exchanger. The Ca pump appears to contribute little to beat-to-beat relaxation.

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Year:  1986        PMID: 3760814      PMCID: PMC2228829          DOI: 10.1085/jgp.88.3.393

Source DB:  PubMed          Journal:  J Gen Physiol        ISSN: 0022-1295            Impact factor:   4.086


  13 in total

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3.  Interaction of intracellular ion buffering with transmembrane-coupled ion transport.

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4.  Contributions of [Ca2+]i, [Pi]i, and pHi to altered diastolic myocyte tone during partial metabolic inhibition.

Authors:  H Ikenouchi; O Kohmoto; M McMillan; W H Barry
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5.  Intracellular Ca(2+) dynamics and the stability of ventricular tachycardia.

Authors:  E Chudin; J Goldhaber; A Garfinkel; J Weiss; B Kogan
Journal:  Biophys J       Date:  1999-12       Impact factor: 4.033

6.  Distinct roles of peroxynitrite and hydroxyl radical in triggering stunned myocardium-like impairment of cardiac myocytes in vitro.

Authors:  H Ishida; C Genka; Y Hirota; Y Hamasaki; H Nakazawa
Journal:  Mol Cell Biochem       Date:  1999-08       Impact factor: 3.396

7.  Alterations in cation homeostasis in cultured chick ventricular cells during and after recovery from adenosine triphosphate depletion.

Authors:  H Ishida; O Kohmoto; J H Bridge; W H Barry
Journal:  J Clin Invest       Date:  1988-04       Impact factor: 14.808

8.  Na+/H+ exchanger and reperfusion-induced ventricular arrhythmias in isolated perfused heart: possible role of amiloride.

Authors:  S Mochizuki; S Seki; M Ejima; T Onodera; M Taniguchi; S Ishikawa
Journal:  Mol Cell Biochem       Date:  1993-02-17       Impact factor: 3.396

9.  Mitochondrial and sarcolemmal Ca2+ transport reduce [Ca2+]i during caffeine contractures in rabbit cardiac myocytes.

Authors:  R A Bassani; J W Bassani; D M Bers
Journal:  J Physiol       Date:  1992       Impact factor: 5.182

10.  Intracellular Ca2+ transients during rapid cooling contractures in guinea-pig ventricular myocytes.

Authors:  D M Bers; J H Bridge; K W Spitzer
Journal:  J Physiol       Date:  1989-10       Impact factor: 5.182

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