Literature DB >> 11158165

Allosteric regulation of Na/Ca exchange current by cytosolic Ca in intact cardiac myocytes.

C R Weber1, K S Ginsburg, K D Philipson, T R Shannon, D M Bers.   

Abstract

The cardiac sarcolemmal Na-Ca exchanger (NCX) is allosterically regulated by [Ca](i) such that when [Ca](i) is low, NCX current (I(NCX)) deactivates. In this study, we used membrane potential (E(m)) and I(NCX) to control Ca entry into and Ca efflux from intact cardiac myocytes to investigate whether this allosteric regulation (Ca activation) occurs with [Ca](i) in the physiological range. In the absence of Ca activation, the electrochemical effect of increasing [Ca](i) would be to increase inward I(NCX) (Ca efflux) and to decrease outward I(NCX). On the other hand, Ca activation would increase I(NCX) in both directions. Thus, we attributed [Ca](i)-dependent increases in outward I(NCX) to allosteric regulation. Ca activation of I(NCX) was observed in ferret myocytes but not in wild-type mouse myocytes, suggesting that Ca regulation of NCX may be species dependent. We also studied transgenic mouse myocytes overexpressing either normal canine NCX or this same canine NCX lacking Ca regulation (Delta680-685). Animals with the normal canine NCX transgene showed Ca activation, whereas animals with the mutant transgene did not, confirming the role of this region in the process. In native ferret cells and in mice with expressed canine NCX, allosteric regulation by Ca occurs under physiological conditions (K(mCaAct) = 125 +/- 16 nM SEM approximately resting [Ca](i)). This, along with the observation that no delay was observed between measured [Ca](i) and activation of I(NCX) under our conditions, suggests that beat to beat changes in NCX function can occur in vivo. These changes in the I(NCX) activation state may influence SR Ca load and resting [Ca](i), helping to fine tune Ca influx and efflux from cells under both normal and pathophysiological conditions. Our failure to observe Ca activation in mouse myocytes may be due to either the extent of Ca regulation or to a difference in K(mCaAct) from other species. Model predictions for Ca activation, on which our estimates of K(mCaAct) are based, confirm that Ca activation strongly influences outward I(NCX), explaining why it increases rather than declines with increasing [Ca](i).

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Year:  2001        PMID: 11158165      PMCID: PMC2217247          DOI: 10.1085/jgp.117.2.119

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


  46 in total

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  59 in total

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2.  A mathematical treatment of integrated Ca dynamics within the ventricular myocyte.

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3.  Data-based theoretical identification of subcellular calcium compartments and estimation of calcium dynamics in cardiac myocytes.

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5.  Rate dependence and regulation of action potential and calcium transient in a canine cardiac ventricular cell model.

Authors:  Thomas J Hund; Yoram Rudy
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Review 6.  Excitation-contraction coupling and mitochondrial energetics.

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Journal:  Basic Res Cardiol       Date:  2007-07-27       Impact factor: 17.165

7.  Steady-state coupling of plasma membrane calcium entry to extrusion revealed by novel L-type calcium channel block.

Authors:  William C Lester; Elizabeth A Schroder; Don E Burgess; Doug Yozwiak; Douglas A Andres; Jonathan Satin
Journal:  Cell Calcium       Date:  2008-10       Impact factor: 6.817

8.  Calcium clearance mechanisms of mouse sperm.

Authors:  Gunther Wennemuth; Donner F Babcock; Bertil Hille
Journal:  J Gen Physiol       Date:  2003-07       Impact factor: 4.086

9.  Imatinib activates pathological hypertrophy by altering myocyte calcium regulation.

Authors:  Larry A Barr; Catherine A Makarewich; Remus M Berretta; Hui Gao; Constantine D Troupes; Felix Woitek; Fabio Recchia; Hajime Kubo; Thomas Force; Steven R Houser
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10.  NCLX: the mitochondrial sodium calcium exchanger.

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