Vol. 273, Issue 5, H2343-H2350, November 1997
Energetics of heart muscle contraction under high K perfusion:
verapamil and Ca effects
Alicia E.
Consolini,
María T.
Márquez, and
Jorge
E.
Ponce-Hornos
Instituto de Investigaciones Cardiológicas, Facultad de
Medicina y Cátedra de Biofísica, Facultad de
Odontología, Universidad de Buenos Aires-Consejo Nacional de
Investigaciones Científicas y Técnicas, 1122 Buenos
Aires, Argentina
 |
ABSTRACT |
Tension-dependent (TDH) and tension-independent heat (TIH)
release were measured during single isovolumetric contractions in the
arterially perfused rat ventricle. Under perfusion with 7 mM K-0.5 mM
Ca, TDH showed only one component
(H3), whereas TIH could be
divided into two components (H1 and
H2) of short evolution (similar
to the classically identified activation heat) and one component
(H4) of long duration (dependent
on mitochondrial respiration). Under 25 mM K, TIH components (i.e.,
H1,
H2, and H4) increased with the increase
in extracellular Ca concentration ([Ca]o) from 0.5 to
4 mM, and H3 correlated with
pressure at all [Ca]o,
with regression parameters similar to those observed under 7 mM K. Under 25 mM K-2 mM Ca, peak pressure development (P), H1,
H2, and
H3, plotted against the number of
beats under 0.4 µM verapamil, exponentially decreased, but
H4 decreased to 5.5 ± 2.9% in
the first contraction and remained constant thereafter. Under hypoxia,
P, H1,
H2, and
H3 progressively decreased for
about six contractions, but H4 was
not detectable from the second contraction. The results suggest that
increasing extracellular K concentration decreases contractile economy
mainly by increasing energy expenditure related to a Ca-dependent
(verapamil-sensitive) mitochondrial activity that is not related to
force generation.
calorimetry; calcium; potassium; tension-independent heat; tension-dependent heat; muscle economy; mitochondria; cardioplegia; hypoxia
| |
INTRODUCTION |
AN INCREASED EXTRACELLULAR K concentration
([K]o) has been used
to prevent spontaneous contractions for the measurement of basal
metabolism (17, 29). In surgery, high
[K]o has been included
in cardioplegic solutions to safeguard the heart from damage (11). On
the other hand, it has been shown (23) that, under quiescent
conditions, increasing
[K]o increases steady
energy expenditure caused by an increase in the Na-K pump activity
(23). Therefore, it was of interest to determine whether high K
perfusion also affects the economy of a contraction. The economy of
isometric force development can be altered by affecting two major
groups of processes, namely tension-dependent and tension-independent processes (4, 12, 13). To minimize the energy contribution by
tension-dependent processes, the energy released by tension-independent processes has been classically studied by diminishing force
development. Several methods have been used to achieve that goal, such
as preshortening the resting length of the muscle (12), exposing the
muscle to a hyperosmotic medium (19), or quick-releasing the muscle
during the latency period (13). More recently, four
components of heat released (H1,
H2,
H3, and
H4) were simultaneously measured
in a single contraction (22). The most relevant aspect of these measurements is that the tension-independent heat (TIH) was evaluated simultaneously with the tension-dependent heat (TDH) component (H3) in the presence of pressure
development (22). TIH was further divided into two fractions
(H1 and
H2) of short evolution (similar to the fraction classically identified as the activation heat) and
another one of long duration
(H4) that showed a high
dependence on mitochondrial respiration (22). With the use of this
approach for simultaneous measurement of TIH and TDH, the present work shows that maintenance of isovolumic pressure development under high
[K]o perfusion induces
an overall decrease in muscle economy. The effect can be mainly
attributed to the increase in basal heat production and to an increase
in the activity of a tension-independent, oxygen-dependent mechanism
that is triggered by Ca. Furthermore, the present results also show
that, under these high K conditions, the contractile economy decreases
as [Ca]o increases.
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METHODS |
Biological preparation.
Twenty-four Wistar rats of either sex, weighing 200-250 g, were
reserpinized (5 mg/kg; Ciba Geigy) 24 h before death. The animals were
heparinized (2,000 U) and anesthetized with a pentobarbital sodium
overdose (23). The beating hearts were rapidly excised, and retrograde
perfusion by the Langendorff method was initiated with control
perfusate at room temperature (20-24°C). Both right and left
atria and right papillary muscles were dissected from the heart. Also,
a small cut in the septal wall, close to the aorta, was performed to
prevent spontaneous contractions. A latex balloon was placed into the
left ventricle, and the muscle was mounted in a Kel-F frame between two
stainless steel hooks. After cannulation and mounting, the muscle was
placed in the inner chamber of a calorimetric system. The latex balloon
was connected to a Statham P23 Db pressure transducer so that pressure
developed during isovolumic contractions could be measured. At the end
of each experiment, the tissue was removed from the calorimeter, weighed in a preweighed vial, and dried at 110°C to constant weight so that the water content could be calculated. The average water content in the present experiments was 81.7 ± 0.49%
(n = 24). Unless otherwise indicated,
results reported in the present work are quoted per gram wet weight.
Solutions.
The heart muscle was perfused at a constant rate (5 ml/min) with
a solution (control) containing (in mM) 1 MgCl2, 100 NaCl, 0.5 NaH2PO4,
7 KCl, 0.5 CaCl2, 25 NaHCO3, 36 sucrose, and 6 dextrose. Sucrose was replaced by 18 mM KCl for the
high-K perfusate (25 mM K). The solutions were bubbled with 95%
O2-5%
CO2 (or 95%
N2-5% CO2 for the hypoxic experiments)
to achieve a pH of 7.3-7.4. In those experiments in which Ca
concentration in the perfusate was changed, no corrections for changes
in osmolarity or ionic strength were performed. Verapamil
(Hoescht) was diluted in Krebs solution from a 1 × 10
3 M solution the same day
of the experiment.
Mechanical and heat measurements.
The technique for on-line measurement of heat production and
mechanical activity of isolated heart muscle has been described previously in detail (10, 24). Briefly, the calorimeter was submerged
in a constant-temperature bath. The temperature of the calorimeter bath
was controlled with a cooling-heating bath (± 0.003°C) in
which the perfusate was also equilibrated. Calorimeter calibration was
accomplished by passing a 2.1-kHz sine wave through the muscle by
means of the stimulating electrodes (24). The present calorimeter uses
two insulated ceramic modules (Melchor Thermoelectrics) with a total of
254 thermosensitive junctions (22). The minimum output of the
thermosensitive units recorded in the present experiments was
>10 µV, whereas the electrical noise was 1 µV at a maximum gain
(1 µV/mm). With this method, it was possible to continuously and
simultaneously record left intraventricular pressure, its first
derivative, perfusion pressure, and rate of heat production
(
). Both mechanical and heat outputs were recorded on a Grass 5D four-channel recorder. In some experiments, heat production was also logged by an analog-to-digital converter (DT
2808, Data Translation) into an AT-386 desk computer. Data acquisition
frequency varied from 1 to 40 data points per second. The mechanical
parameters considered for this study were maximal intraventricular
pressure development (P), intraventricular pressure-time integral (PTI)
measured as the area under the pressure development signal, and maximal
rates of contraction (+
) and relaxation (
). The whole contraction was divided into three
periods as follows:
tPP, time to peak
pressure measured from the start of contraction to P;
tR1, time from P
to ; and
tR2, time from to the end of contraction.
Once the muscle was placed in the inner chamber of the calorimeter, a
60-min equilibration period with control solution was allowed to elapse
before any experimental intervention. The muscle was stimulated by 5-V,
5-ms square pulses from a Grass SD 9 stimulator in control medium and
by 
15-V, 15-ms stimulus in high-K media. The stimulus contribution to
the heat released was <1% of that released by a contraction. A
muscle was accepted for study if, during the 60-min equilibration
period under control perfusate at 25°C, a minimum of 14 mN/mm2 pressure was developed (at
0.16 Hz and a resting pressure not higher than 8 mN/mm2) and it remained
quiescent in the absence of stimulation. Reproducible P values under
control perfusate throughout the experiment were used as a measure of
muscle stability. Resting pressure was increased in steps of 1-2
mN/mm2 with the muscle stimulated
at 0.16 Hz until P reached a steady maximum value. This resting
pressure was maintained constant throughout the experiment. Once the
maximum value of P was achieved, the electrical stimulation was stopped
and resting heat rate
(r) was
recorded. The pressure and heat production from single twitches (5 min
apart) were recorded at a chart speed of 25-50 mm/s.
Heat signal analysis.
Active heat per beat (Ha; the
fraction released above
r by a
contraction) was calculated as the integral of the calorimetric output
(t) versus
time (22, 25). The various components associated with this
Ha were calculated as described
elsewhere (22). Briefly, when the power applied was either maintained constant or interrupted before the integration time of the calorimeter, t for the
period during which the power was applied can be described by the
following equation (22)
|
(1)
|
where
Ao = (µ4
2
1)0.5 tan[(µ421)0.5]; µ is the cooling rate constant of the calorimeter; is the
diffusion delay constant;
Ai = 1/{(2i + 1)2 [1 (2i + 1)2µ1]};
i = (2i + 1)2µ;
t is time; and
o represents
the applied power. On the other hand, if the released power grows for
longer periods than the integration time of the calorimeter,
o in
Eq. 1 becomes a function of time. To
test whether this time dependency could be obtained from the
calorimeter output, power was released in the calorimetric chamber
following either an exponential (4 experiments) or a linear function of
time (4 experiments). Regardless of how power was generated, each
calorimetric response was fitted by two diffusional equations similar
to Eq. 1. In one of them,
o in Eq. 1 is equal to
'o(1 e
t),
and in the other equation,
o = kt, where 
and
k are the exponential and linear rate
constants, respectively. The fitting procedure was applied
1) to the whole curve (i.e., from
the time at which power was applied to the time at which power was
switched off) and 2) to selected
periods (from time 0) of that curve.
The fitted parameters remained constant only if the curve was fitted with the function under which power was applied. When an exponential fit was used for data produced by a linear growing process, a systematic deviation between the parameter obtained for the whole curve
and that from the selected period was observed. The same type of
deviation was found when the linear fit was used for the exponentially
growing process. The parameters obtained from the whole curve in each
case were not statistically different from the known parameters (mean
differences:
'o,
95 ± 109 µW; , 0.0047 ± 0.002 s1; and
k, 0.156 ± 0.258 µW/s).
Initial values for the fitting procedure during the experiments were
easily obtained by dividing data from calorimetric output (after 60 s)
by the diffusional term of Eq. 1.
Statistical analysis.
Data are presented as means ± SE, and statistical significance was
settled at P < 0.05. For a
comparison between two samples, the
t-test was used. For multiple
comparisons, a one-way analysis of variance test followed by a
nonparametric Mann-Whitney ranking test was applied (27). Regression
analysis was performed with the use of a nonlinear regression technique
running on an AT-386-compatible desk computer (22). The difference
between the estimated and the hypothetical value (i.e., estimated slope
against 1, correlation coefficients, and zero abscissae values against
0) was analyzed as described elsewhere (9), and the statistical
significance was settled at P < 0.05. Systematic deviations of the fitted curve from the data points
were studied with the sign test (9). Statistical significance between
two different correlation coefficients was estimated as described
elsewhere (9). The comparison between fitted curves obtained with
different numbers of terms (for a given set of data points) was
performed with the Fisher's test (9).
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RESULTS |
Under control perfusion (7 mM K-0.5 mM Ca), resting heat production
averaged 4.16 ± 0.15 mW/g. Figure 1
shows that, after 5-min periods of quiescence, maximal pressure
development (P) averaged 42.5 ± 2.9 mN/mm2 and active heat
(Ha) averaged 31.6 ± 3.6 mJ/g
(n = 14). In all experiments, the
power curve obtained under control perfusate was fitted to four heat
components (Fig.
2A). The
mean values obtained were 2.2 ± 0.3, 2.3 ± 0.3, and 16.9 ± 1.8 mJ/g for the TIH components
(H1,
H2, and
H4, respectively) and 8.9 ± 0.7 mJ/g for the TDH release
(H3).
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Fig. 1.
Effects of 25 mM K and different
[Ca]o on active heat
per beat (Ha) and peak pressure
development (P) of rat ventricle single contractions. Bars indicate
means ± SE of data under perfusion with 7 mM K-0.5 mM Ca (control;
n = 14) and 25 mM K and different
[Ca]o (0.5, 1, 2, and
4 mM Ca; n = 8, 11, 14, and 11, respectively). P < 0.01 for both
parameters by analysis of variance (ANOVA).
* P < 0.05 compared with
respective control value by Mann-Whitney ranking test. Note that
recovery of P under 25 mM K by increasing
[Ca]o was accompanied
by an increase in associated Ha of
10 times that obtained under 7 mM K.
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Fig. 2.
Typical digitized records of heat production () from
single contractions obtained under perfusion with 7 mM K-0.5 mM Ca
(A), 25 mM K-0.5 mM Ca
(B), or 25 mM K-4 mM Ca
(C). Dashed lines represent various
energy components (H1,
H2,
H3, and
H4 in accord with their times to
peak), and continuous curves show linear combinations of all energy
components. Note that whereas only 3 components are shown in
B, the magnitude of
H4 in
C is 15 times that shown in
A.
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Effects of 25 mM K.
As previously described (23), changing the perfusate from 7 mM K-0.5 mM
Ca to 25 mM K-0.5 mM Ca induced a transitory increase in
r (+1.46 ± 0.42 mW/g). This increase was followed by a decrease in resting heat
values to a new steady level that remained higher (+1.17 ± 0.33 mW/g; n = 14;
P < 0.01) than control resting heat (4.16 ± 0.15 mW/g). Under this new resting condition, P and
Ha decreased to ~20% of their
respective values under control perfusate (Fig. 1). Maximum rate of
contraction (+) and relaxation
() also decreased. To investigate
whether the decrease in + and were associated with the decrease in P, the
ratios between + or and P
were studied. Whereas the +-to-P ratio remained unchanged (8.7 ± 0.6 vs. 9.7 ± 0.9 s1;
n = 8; not significant), the
-to-P ratio significantly increased from 3.1 ± 0.3 to 4.7 ± 0.7 s1
(P < 0.05). Neither time to peak
pressure (tPP) nor
the last part of the relaxation period
(tR2) changed with
the increase in [K]o.
On the other hand, the first period of relaxation
(tR1) significantly
decreased from 0.26 ± 0.02 to 0.15 ± 0.02 s
(P < 0.01). The energy released by a
contraction under 25 mM K-0.5 mM Ca perfusate was always decomposed
into only three components (H1,
H2, and
H3). As shown in Figs.
2-4, all three components of heat
released under 25 mM K-0.5 mM Ca were smaller than those obtained under
control perfusate.
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Fig. 3.
Tension-independent heat components
H1 and
H2
(A) and
H4
(B) obtained from single
contractions under 25 mM K and different
[Ca]o. Bars indicate
means ± SE from 8, 11, 14, and 11 contractions obtained for 0.5, 1, 2, and 4 mM Ca, respectively. P < 0.01 for H1,
H2, and
H4, respectively, by ANOVA.
* P < 0.05 compared with
respective value at 0.5 mM Ca by Mann-Whitney ranking test. Note that
whereas H1 and
H2 (i.e., fraction classically
identified as activation heat) reached values either similar to control
value (H1) or 1.73 times
control value (H2),
H4 (a tension-independent,
oxygen-dependent fraction of heat released increased ~15 times above
control value.
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Effects of increasing [Ca]o
under 25 mM K.
To compensate for the negative inotropic effect of 25 mM K,
[Ca]o was increased
from 0.5 mM to 4.0 mM. The experimental sequence of altered
[Ca]o was 0.5, 1.0, 2.0, and 4.0 mM. As shown in Fig. 1, increasing
[Ca]o under 25 mM K
perfusate increased P (up to 85% of control values) and
Ha (up to 830% of control, under
4 mM Ca). The +-to-P ratios at 1, 2, and 4 mM Ca did not change with the changes in
[Ca]o, and the pooled
data (n = 36) averaged 9.6 ± 0.5 s1. The
-to-P ratio (which was increased by 25 mM
K-0.5 mM Ca) was not altered by increasing
[Ca]o, and the pooled
data for 1, 2, and 4 mM Ca averaged 4.5 ± 0.3 s1. Similarly, under 25 mM
K, tR1 remained
unchanged with changes in
[Ca]o (pooled data
average: 0.14 ± 0.01 s; n = 36),
but it was shorter (P < 0.05) than
the tR1 observed under
7 mM K (0.26 ± 0.02 s; n = 14).
The second period of relaxation
(tR2) was
significantly prolonged only under 25 mM K-4 mM Ca (1.44 ± 0.26 vs.
0.53 ± 0.05 s for 25 mM K-4 mM Ca and 7 mM K-0.5 mM Ca,
respectively; P < 0.01). This
prolonged relaxation was not enough to significantly increase PTI when
[Ca]o was increased
from 2 to 4 mM Ca.
The increase in [Ca]o
under 25 mM K increased all four components of heat production (Figs.
2-4).
H1 significantly increased when
[Ca]o was raised from
0.5 to 1 mM under 25 mM K media and remained unchanged and similar to
the control (2.2 ± 0.3 mJ/g) between 1 and 4 mM Ca (Fig.
3A).
H2 significantly increased from 0.5 to 4 mM Ca (Fig. 3A), reaching a
value (4.0 ± 0.5 mJ/g) higher (P < 0.001) than that measured under control perfusate (2.3 ± 0.3 mJ/g). As reported for 7 mM K (22),
H3 varied proportionally with P
and PTI. Because at the various
[Ca]o no significant
differences among their slopes were found, the data were pooled. The
correlation for 44 data points yielded a straight relationship with
r > 0.74 (P < 0.001) (Fig. 4). The
tension-independent, oxygen-dependent heat component
H4 was absent at 0.5 mM Ca-25 mM K
conditions (see Fig. 2B). On the
other hand, it significantly increased as
[Ca]o was raised (Fig.
3B), reaching a value (253 ± 36 mJ/g) of ~15 times that observed under 7 mM K-0.5 mM Ca (16.9 ± 1.8 mJ/g). Under 1 mM Ca, H4
showed similar magnitude and kinetic characteristics to those observed
under control perfusate. At 2 and 4 mM Ca,
H4 increased exponentially for
>80 s after the mechanical event was over (Fig.
2C). The exponential increase in
H4 under 2 or 4 mM Ca25 mM K
was further supported by the fact that when data from the calorimetric
output (observed after 60 s of contraction) were divided by the
diffusional term of Eq. 1, an exponential function was consistently
observed.
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Fig. 4.
Energy released by H3 plotted
against P (A) and pressure-time
integral (PTI; B) from single
contractions under 25 mM K and different
[Ca]o. Linear
correlation between H3 and P
yielded a slope of 0.23 ± 0.03 mJ · mN1 · mm2 · g1
and an intercept of 1.1 ± 2.8 mJ/g
(P < 0.001). Linear
correlation between H3 and PTI
yielded a slope of 0.66 ± 0.08 mW · mN1 · mm2 · g1
and an intercept of 1.8 ± 2.6 mJ/g
(P < 0.001).
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Effects of verapamil under 25 mM K-2 mM Ca.
As shown in Effects of increasing
[Ca]o under 25 mM
K, all four heat components released under high-K
perfusate were dependent on
[Ca]o. To
investigate the relationship of the heat components with Ca influx via
Ca channels, five experiments were done in which the effect of 0.4 µM
verapamil was tested during 25 mM K-2 mM Ca perfusion. Verapamil was
added during quiescence in the presence of 25 mM K-2 mM Ca. About 2 min
later, two or three electrical stimuli (5 min apart) were applied to
each muscle. Verapamil induced a decrease in P which was dependent on
the period elapsed in the presence of the drug under 25 mM K (Fig.
5D). It
is of interest that the effects of verapamil were independent of the
number of isolated contractions performed (Fig. 5). No changes were
found in resting pressure or +- or
-to-P ratios. When P,
H1,
H2, and
H3 values obtained in the presence
of verapamil were plotted against time, all three heat components
exponentially decreased with similar time constants (Fig. 5). On the
other hand, H4 decreased with
verapamil treatment to 6.7 ± 3.2%
(n = 12, P < 0.05 against 0) of the value
under 25 mM K-2 mM Ca perfusate independent of the duration of the
verapamil treatment.
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Fig. 5.
Effect of 0.4 µM verapamil on
H1,
H2, and
H3 energies
(A-C,
respectively) and P (D) of single
contractions obtained from 5 muscles under 25 mM K-2 mM Ca perfusion as
a function of time of treatment with Ca blocker. Values are expressed
as percentages of those obtained in absence of drug. Data points
correspond to first ( ), second ( ), and third beats ( ) of each
muscle under verapamil treatment. Note similarity of rate constants for
all four parameters.
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Severe hypoxia under 25 mM K-2 mM Ca.
It has been suggested (22) that under control perfusate,
H4 was associated with
mitochondrial activity. To test whether the magnitude of
H4 observed under high
[K]o perfusion was
also oxygen-dependent, in five experiments (after at least 30 min under 25 mM K-2 mM Ca-perfusion) the oxygen of the perfusate was removed by
switching to a 95% N2-5%
CO2 perfusate. Three minutes after the hypoxic perfusate was started, five or six pulses separated by
intervals of ~5 min were applied and their mechanical and heat outputs recorded. As shown in Fig. 6, the
decrease in Ha through the
successive hypoxic contractions was mostly caused by a decrease in
H4 (which fell to 30% of its
original value in the first hypoxic beat and disappeared in the second
beat). In contrast, the decreases in P,
H1,
H2, and
H3 with the successive hypoxic
beats were similar. As shown in Fig. 6,
A and
B, these components remained present in each muscle for at least five contractions. The energy released as
H3 was linearly correlated with P
under hypoxic conditions (slope: 0.17 ± 0.02 mJ · mN1 · mm2 · g1;
intercept not different from zero: 0.55 ± 1.2 mJ/g;
r= 0.7988). The slope for
H3 versus P in hypoxia was about
80% of that observed for aerobic conditions under 25 mM K-2 mM Ca
perfusion (slope: 0.21 ± 0.06 mJ · mN1 · mm2 · g1).
The paired differences between the
H3-to-P ratios in hypoxic and
aerobic conditions averaged 0.024 ± 0.009 mJ · mN1 · mm2 · g1
(n = 28, P < 0.01). No changes were found in
resting intraventricular pressure or in +- or
-to-P ratios during the hypoxic period studied
(<35 min).
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Fig. 6.
Effect of severe hypoxia (N2
perfusate) on heat components and P of single contractions from rat
ventricles in 25 mM K-2 mM Ca. Bars indicate means ± SE from 5 muscles (6 hypoxic single contractions were done in each muscle).
P < 0.01 for P,
H1,
H2,
H3, and
H4, respectively, by ANOVA.
* P < 0.05 compared with
respective O2 value by ranking
test. Note that whereas P (A) and tension-dependent heat
(H3) and two fractions associated with activation heat
(H1 and H2) (B) decreased very
slowly under N2 perfusate,
H4 values (A) beginning
with second contraction were not different from 0.
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DISCUSSION |
It has been shown that the energy released by a single contraction can
be decomposed into TDH (H3) and
TIH components (22). Two of the TIH components
(H1 and
H2) were related to a fraction classically identified as activation heat (mainly myofilament calcium-binding and calcium-removal processes, respectively). Because
of its oxygen dependency, a third fraction of TIH was associated with
the mitochondria (22). Increasing
[K]o induced a
caffeine-sensitive transitory increase in
r (23). It was suggested that the high
[K]o could be
depleting the sarcoplasmic reticulum (SR), leaving less Ca available
for the twitch (23). This suggestion agrees with the observed fall in P
under 25 mM K-0.5 mM Ca perfusate and with the decreased
H1. Because high [K]o perfusion induces
an increase in the Na-K pump activity (23), a decrease in intracellular
Na and an activation of Ca removal by the Na/Ca exchanger would be
expected. An increase in Na/Ca-exchange activity (in the Ca efflux
mode) could explain the relative increase in the
-to-P ratio observed at all
[Ca]o under high K. On
the other hand, the prolongation (+0.91 s) of the last part of
relaxation (tR2;
observed at 4 mM Ca-25 mM K perfusate) could be an indication of an
impairment of Ca removal, at least for a period in which the Na/Ca
exchanger would be less active. Such a situation can also be explained
by an impairment of the SR to keep Ca loaded under 25 mM K (23). In
this regard, Meyer et al. (18) suggested a low SR Ca content of
myocytes perfused under 20 mM K. In accord with this hypothesis is the
fact that H2 [which is a
fraction of energy attributed to Ca removal (22)] grows more than
H1 (which would represent, to some
extent, the amount of Ca to be removed) compared with control
conditions (22). In fact, because the energetic cost for Ca removal is
one ATP per Ca removed via the Na/Ca exchanger (because of the 1 Ca:3
Na stoichiometry of the Na/Ca exchanger and the one ATP hydrolyzed for
every three Na removed via the Na-K pump) and two Ca per ATP via the SR
Ca pump (6, 21), an increase of the activity of Na/Ca exchanger over
the SR Ca pump should result in an increase in energy
expenditure.
Because H3 is the only
pressure-dependent energy release component of the contraction, the
ratio between P and H3 can be used as a measure of the isometric economy (22). When both P and H3 are expressed in the same units
[using 1.05 as the density of the muscle (15)], the ratio
between them is dimensionless. This ratio would be a measure of the
isometric heat coefficient, which is a useful index of contraction
economy (4, 19). Under 25 mM K perfusate, the
P-to-H3 ratio (~4.3) calculated
from the inverse of the slope of the plot shown in Fig.
4A was independent of changes in
[Ca]o. Furthermore, it
was similar to that calculated from single contractions under 7 mM
K-0.5 mM Ca perfusate (~3.9). The
P-to-H3 (~4.3) and
PTI-to-H3 (~1.44
s1) ratios under 25 mM K
were similar to those reported for rat ventricles perfused under 7 mM
K-0.5 mM Ca (~4.2 and 1.5 s1, respectively) (22). The
P-to-H3 ratio was also similar to that calculated from the TDH of rabbit myocardium (~3.6) (19). The
absence of changes in these ratios would indicate that varying [K]o and
[Ca]o does not affect
the economy of force development or that of force maintenance. Hypoxia
also increased the P-to-H3 ratio
(to 5.6) under 25 mM K conditions, indicating as previously suggested
under 7 mM K (22) the existence of a heat fraction related to recovery
metabolism in H3.
It is clear from Fig. 3 that the increased
Ha is mainly caused by an
increased H4. As previously shown
for 7 mM K (22), under 25 mM K perfusate
H4 is a pressure-independent and
oxygen-dependent fraction of energy. The fact that under
O2 deprivation
H4 disappeared even under
conditions in which P was scarcely affected (see the second hypoxic
beat in Fig. 6) indicates that H4
should be coupled to mitochondrial respiration. A range of evidence
indicates that whereas P and H4
are both related to
[Ca]o under 25 mM K,
there seems to be no direct relationship between them. For instance, whereas P was saturated at 2 mM Ca,
H4 increased with a further increase in [Ca]o to 4 mM (see Fig. 3B). In addition, the
fact that under 25 mM K-0.5 mM Ca
H4 could not be detected suggests that the processes associated with
H4 might have a higher Ca
threshold than P. Furthermore, whereas
H4 was strongly inhibited by
verapamil in a time-independent fashion, the effects of verapamil on P, H1,
H2, and
H3 were time dependent and all
four parameters were affected with a similar time constant (see Fig.
6). These results suggest that whereas P,
H1,
H2, and
H3 might have a common dependence on Ca channels, H4 could be
related to another verapamil-sensitive site. In this connection, it has
been shown that verapamil inhibits the mitochondrial Na/Ca exchanger
(7, 30), which participates in the mitochondrial Ca transport cycle (8,
14). The differential sensitivity of
H4 to verapamil and the fact that
it is altered by changes in
[Ca]o and is coupled
to mitochondrial respiration suggest a Ca-related mitochondrial
activity. Furthermore, the time course of
H4 (developed for >80 s after
the twitch) indicates that this process is active even after the
contraction-relaxation cycle has finished. In this connection, it is
known that cytosolic Ca could trigger either an increase of oxidative
phosphorylation in response to ATP-consuming processes (5) or a Ca
cycling through mitochondrial membrane coupled to respiration (6, 8, 14, 16). Therefore, the presence of
H4 (even under control perfusate)
suggests that the mitochondria participate in the homeostasis of a Ca
fraction in response to a contraction but that this Ca fraction is
different from that involved in the development of pressure.
It is well known that hypoxia decreases mechanical activity in general
and P in particular. The decrease in P has been attributed to a number
of processes such as 1) a decrease
in ATP or creatine phosphate content (20, 26);
2) intracellular acidosis caused by
glycolytic lactate and H+
accumulation (2); or 3) a decrease
in Ca influx or Ca release (1, 20). The effects of
hypoxia on P, H1,
H2, and
H3 under 25 mM K perfusate
observed in the present work were more marked than under control
perfusate (22). Nevertheless, resting pressure and relaxation times
were not altered by hypoxia, suggesting that at least ATP levels near
the myofilaments and Ca pumps were not significantly affected. It has
been shown that acidosis by itself does not reduce the cytosolic peak
of aequorin (3), indicating that the amount of Ca released should
remain approximately constant. In line with this finding is the fact
that H1 and
H2 reportedly (22) did not
decrease during the fall in P observed under hypoxic control perfusion.
On the other hand, under 25 mM K conditions, the progressive fall in
H1 and
H2 suggests that hypoxia could have decreased the availability of Ca for myofilaments, which in turn
could have a further effect on P. Therefore, whereas the negative
inotropism found under control perfusion could be ascribed to acidosis,
the larger decrease in P observed under high-K media might be related
to an additional effect on cytosolic Ca. This interpretation is also
supported by the fact that a decreased 47Ca uptake has been found in
rabbit intraventricular septum during hypoxia (20) and that a
shortening in action potential duration is induced by anoxia in rat
ventricular myocytes (28). Because high K perfusion induces a Ca
depletion from SR (18, 23), P should be more dependent on Ca influx
under high K than under 7 mM K. Consequently, an effect of hypoxia on
Ca current should be more noticeable on cytosolic Ca and P under 25 mM
K than under 7 mM K conditions. In summary, increasing
[K]o decreases
contractile economy mainly by increasing energy expenditure related to
a long-duration, Ca-dependent, and verapamil-sensitive mitochondrial
activity different from that related to force generation. Therefore,
the increase in energy expenditure is pressure independent and likely
caused by an increase in the energy expenditure for Ca sequestration and for a Ca-dependent increase in mitochondrial activity.
| |
ACKNOWLEDGEMENTS |
This work was supported by the University of Buenos Aires Grants
OD-009 and OD-022 UBACYT República Argentina.
| |
FOOTNOTES |
M. T. Márquez and J. E. Ponce-Hornos are Established
Investigators of the Consejo Nacional de Investigaciones
Científicas y Técnicas (CONICET), and A. E. Consolini is
a Postdoctoral Fellow of CONICET.
Address for reprint requests: J. E. Ponce-Hornos, Instituto de
Investigaciones Cardiológicas, Fac. de Medicina, Univ. de Buenos
Aires, Marcelo T. de Alvear 2270, 1122 Buenos Aires, Argentina.
Received 28 January 1997; accepted in final form 10 June 1997.
| |
REFERENCES |
1.
Allen, D. G.,
and
C. H. Orchard.
Intracellular calcium concentration during hypoxia and metabolic inhibition in mammalian ventricular muscle.
J. Physiol. (Lond.)
339:
107-122,
1983[Abstract/Free Full Text].
2.
Allen, D. G.,
and
C. H. Orchard.
The effect of pH on intracellular calcium transients in mammalian heart muscle.
J. Physiol. (Lond.)
335:
555-567,
1983[Abstract/Free Full Text].
3.
Allen, D. G.,
and
C. H. Orchard.
Measurements of intracellular calcium concentration in heart muscle: the effects of inotropic interventions and hypoxia.
J. Mol. Cell. Cardiol.
16:
117-128,
1984[Medline].
4.
Alpert, N. R.,
and
L. A. Mulieri.
Increased myothermal economy of isometric force generation in compensated cardiac hypertrophy induced by pulmonary artery constriction in the rabbit.
Circ. Res.
50:
491-500,
1982[Free Full Text].
5.
Balaban, R. S.,
and
F. W. Heineman.
Control of mitochondrial respiration in the heart in vivo.
Mol. Cell. Biochem.
89:
191-197,
1989[Medline].
6.
Carafoli, E.
The homeostasis of calcium in heart cells.
J. Mol. Cell. Cardiol.
17:
203-212,
1985[Medline].
7.
Cox, D. A.,
and
M. A. Matlib.
Modulation of intramitochondrial free Ca2+ concentration by antagonists of Na+-Ca2+ exchange.
Trends Pharmacol. Sci.
14:
408-413,
1993[Medline].
8.
Crompton, M.
The role of Ca2+ in the function and dysfunction of heart mitochondria.
In: Calcium and the Heart, edited by G. A. Langer. New York: Raven, 1990, p. 167-198.
9.
Documenta Geigy.
Scientific Tables (6th ed.), edited by K. Diem. New York: Geigy Chemical Corporation, 1962.
10.
Dominguez-Mon, M.,
J. E. Ponce-Hornos,
R. Gómez,
M. A. Cannata,
and
A. C. Taquini.
Energetic, metabolic and contractile effects of vasopressin in mammalian heart.
Methods Find. Exp. Clin. Pharmacol.
6:
373-378,
1984[Medline].
11.
Gay, W. A., Jr.
Potassium-induced cardioplegia: evolution and present status.
Ann. Thorac. Surg.
48:
441-443,
1989[Abstract].
12.
Gibbs, C. L.,
and
J. B. Chapman.
Cardiac energetics.
In: Handbook of Physiology. The Cardiovascular System. The Heart. Bethesda, MD: Am. Physiol. Soc., 1979, sect. 2, vol. I, chapt. 22, p. 775-804.
13.
Gibbs, C. L.,
D. S. Loiselle,
and
I. R. Wendt.
Activation heat in rabbit cardiac muscle.
J. Physiol. (Lond.)
395:
115-130,
1988[Abstract/Free Full Text].
14.
Gunter, T. E.,
K. K. Gunter,
S. S. Sheu,
and
C. E. Gavin.
Mitochondrial calcium transport: physiological and pathological relevance.
Am. J. Physiol.
267 (Cell Physiol. 36):
C313-C339,
1994[Abstract/Free Full Text].
15.
Hill, A. V.
Trails and Trials in Physiology. London: Arnold, 1965.
16.
Lehninger, A. L.
Role of phosphate and other proton-donating anions in respiration-coupled transport of Ca2+ by mitochondria.
Proc. Natl. Acad. Sci. USA
71:
1520-1524,
1974[Abstract/Free Full Text].
17.
Lochner, W., G. Arnold, and E. R. Muller-Ruchholtz.
Metabolism of the artificially arrested heart and of the
gas-perfused heart. Am. J. Cardiol. 22: 299-311.
18.
Meyer, R.,
H. G. Haas,
and
J. Wiemer.
Excitation-contraction coupling in voltage-clamped cardiac myocytes.
Basic Res. Cardiol.
84:
136-148,
1989[Medline].
19.
Mulieri, L. A.,
and
N. R. Alpert.
Activation heat and latency relaxation in relation to calcium movement in skeletal and cardiac muscle.
Can. J. Physiol. Pharmacol.
60:
529-541,
1982[Medline].
20.
Nayler, W. G.,
P. A. Poole-Wilson,
and
A. Williams.
Hypoxia and calcium.
J. Mol. Cell. Cardiol.
11:
683-706,
1979[Medline].
21.
Ponce-Hornos, J. E.
Energetics of calcium movements.
In: Calcium and the Heart, edited by G. A. Langer. New York: Raven, 1990, p. 269-298.
22.
Ponce-Hornos, J. E.,
P. Bonazzola,
F. D. Marengo,
A. E. Consolini,
and
M. T. Márquez.
Tension-dependent and tension-independent energy components of heart contraction.
Pflügers Arch.
429:
841-851,
1995[Medline].
23.
Ponce-Hornos, J. E.,
M. T. Márquez,
and
P. Bonazzola.
Influence of extracellular potassium on energetics of resting heart muscle.
Am. J. Physiol.
262 (Heart Circ. Physiol. 31):
H1081-H1087,
1992[Abstract/Free Full Text].
24.
Ponce-Hornos, J. E.,
N. V. Ricchiuti,
and
G. A. Langer.
On-line calorimetry in the arterially perfused rabbit interventricular septum.
Am. J. Physiol.
243 (Heart Circ. Physiol. 12):
H289-H295,
1982.
25.
Ponce-Hornos, J. E.,
and
A. C. Taquini.
Calcium effects on contractility and heat production in mammalian myocardium.
Am. J. Physiol.
251 (Heart Circ. Physiol. 20):
H127-H132,
1986.
26.
Poole, P. E.,
J. W. Covell,
C. A. Chidsey,
and
E. Braunwald.
Myocardial high energy phosphate stores in acutely induced hypoxic heart failure.
Circ. Res.
19:
221-229,
1966[Abstract/Free Full Text].
27.
Siegel, S.
Estadística no Parametrica. Mexico: Editorial Trillas, 1970.
28.
Stern, M. D.,
H. S. Silverman,
S. R. Houser,
R. A. Josephson,
M. C. Capogrossi,
C. G. Nichols,
W. J. Lederer,
and
E. G. Lakatta.
Anoxic contractile failure in rat heart myocytes is caused by failure of intracellular calcium release due to alteration of the action potential.
Proc. Natl. Acad. Sci. USA
85:
6954-6958,
1988[Abstract/Free Full Text].
29.
Suga, H.,
R. Hisano,
Y. Goto,
O. Yamada,
and
Y. Igarashi.
Effects of positive inotropic agents on the relation between oxygen consumption and systolic pressure volume area in canine left ventricle.
Circ. Res.
53:
306-318,
1983[Abstract/Free Full Text].
30.
Vaghy, P. L.,
J. D. Johnson,
M. A. Matlib,
T. Wang,
and
A. Schwartz.
Selective inhibition of Na-induced Ca release from heart mitochondria by diltiazem and certain other Ca antagonist drugs.
J. Biol. Chem.
257:
6000-6002,
1982[Abstract/Free Full Text].
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