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J Appl Physiol 98: 1712-1719, 2005. First published January 7, 2005; doi:10.1152/japplphysiol.00630.2004
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Artifactual contractions triggered by field stimulation of cardiomyocytes

Janny Bøkenes,1 Ivar Sjaastad,1,2 and Ole M. Sejersted1,3

1Institute for Experimental Medical Research, and 2Department of Cardiology, Ullevaal University Hospital, and 3Center of Heart Failure Research, University of Oslo, N-0407 Oslo, Norway

Submitted 21 June 2004 ; accepted in final form 29 December 2004

Although cell shortening in patch-clamped cells (current-clamp mode) is triggered by an ordinary action potential, the trigger mechanism in field-stimulated cells is not so obvious. The contraction characteristics of the two methods differ, and we, therefore, examined the triggering sequence in field-stimulated cells. Isolated rat cardiomyocytes were plated on laminin-coated coverslips that were mounted on an inverted light microscope and superfused with HEPES-Tyrode buffer (pH 7.4; 37°C). The cells were stimulated to contract either by a 0.5-ms current injection (CC cells) through high-resistance electrodes or a 5-ms biphasic field-stimulation pulse (FS cells), and drugs were added to block sarcolemmal proteins involved in excitation-contraction coupling. Time to peak contraction (TTP) was significantly longer in FS cells and was not affected by the polarity or the length of the stimulus pulse. Tetrodotoxin (TTX; 20 µM) blocked cell shortening in CC cells but not in FS cells. Ni2+ (5 mM) blocked cell shortening in FS cells, whereas KB-R7943 (KB; 5 µM) had no effect either on cell shortening or TTP. In FS cells, nifedipine (Nif; 100 µM) and Cd2+ (300 µM) reduced fractional shortening by 34 and 63%, respectively, but only Cd2+ affected TTP (reduced by 48%). A combination of Nif and KB reduced cell shortening by 50%, whereas a combination of Cd2+ and KB almost abolished cell shortening. We conclude that field stimulation per se prolongs TTP and that cell shortening in FS cells is not dependent on Na+ current but is triggered by a combination of L-type Ca2+ current and reverse mode Na+/Ca2+ exchange.

excitation-contraction coupling; rat; L-type Ca2+ channel; Na+/Ca2+ exchanger



Address for reprint requests and other correspondence: J. Bøkenes, Institute for Experimental Medical Research, Univ. of Oslo, N-0407 Oslo, Norway (E-mail: janny.bokenes{at}medisin.uio.no)




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