Effects of temperature on intracellular [Ca2+] in trout atrial myocytes
Holly A. Shiels1,*,
Matti Vornanen2 and
Anthony P. Farrell1
1 Simon Fraser University, Biological Sciences, Burnaby, British Columbia,
V5A 1S6, Canada
2 University of Joensuu, Department of Biology, PO Box 111, 80101 Joensuu,
Finland
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Fig. 4. This figure is an example of a recording for a single myocyte at 21°C.
Part (A) shows intracellular Ca2+ concentration
([Ca2+]i) and part (B) shows the corresponding L-type
Ca2+ channel current (ICa) at each stimulus change. Each
panel is marked according to the frequency and waveform used to elicit
currents and transients. The first five transients at each temperature were
elicited by square pulses at 0.2 Hz (SQ0.2Hz). The middle five
transients were elicited by SQ pulses applied at a physiologically relevant
frequency for the test temperature (SQ1.4Hz), but with a long pulse
duration (500ms). Together these factors contribute to the dramatic rise in
diastolic Ca2+ levels. The last five transients were elicited by
temperature- and frequency-dependent action potentials (AP1.4Hz).
The dotted line in the lower panel indicates 0mV. Leakage correction was
employed at SQ0.2Hz, but not at SQ1.4Hz or
AP1.4Hz.
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Fig. 2. The effect of temperature on intracellular Ca2+ concentration
([Ca2+]i) and L-type Ca2+ channel current
(ICa) in trout atrial myocytes. (A) The effect of temperature on
[Ca2+]i during SQ0.2Hz, SQphysiol
and APphysiol (the physiological frequencies were: 0.6 Hz at
7°C, 1.0 Hz at 14°C and 1.4 Hz at 21°C). The increase in the
resting level of the transient at SQphysiol reflects the increase
in diastolic Ca2+ concentration (see
Fig. 4,
Table 3). (B) Current
recordings of ICa under the same conditions. Peak current amplitude
was calculated as the difference between the peak inward current and the
current recorded at the end of the depolarizing pulse. The currents elicited
at SQ0.2Hz were leakage corrected using the P/N procedure of the
software (Clampex, Axon Instruments). Leakage correction was not employed at
SQphysiol or APphysiol. Mean data and statistical
analysis is given in Tables
1,2,3
and in Fig. 3.
SQ0.2Hz, square pulses at a frequency of 0.2 Hz;
SQphysiol, square pulses at physiological frequency;
APphysiol, action potential at physiological frequency.
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Fig. 3. The effect of temperature and stimulus change on (A) the peak current
density of L-type Ca2+ channel current (ICa) and (B) the
charge density of ICa in trout atrial myocytes. Dissimilar letters
indicate significant effects of temperature within each stimulus treatment
(analysis of variance, Student—Newman—Keuls test). *
indicates a significant decrease in ICa during AP stimulation at
all temperatures and with each successive stimulus protocol at 21°C.
 indicates greater ICa charge density at 7°C
during AP stimulation compared with SQ stimulation. Values are means ±
S.E.M.; N=7 for 7°C and 21°C, and N=8 for
14°C.
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© The Company of Biologists Ltd 2002
