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Cardiovascular Research Laboratories, Department of Pharmacology, Dalhousie University, Halifax, Nova Scotia, Canada B3H 4H7
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Control of contraction and relaxation by membrane
potential was investigated in voltage-clamped guinea pig ventricular
myocytes at 37°C. Depolarization initiated phasic contractions,
followed by sustained contractions that relaxed with repolarization.
Corresponding Ca2+ transients were observed with fura 2. Sustained responses were ryanodine sensitive and exhibited sigmoidal
activation and deactivation relations, with half-maximal voltages near
46 mV, which is characteristic of the voltage-sensitive release
mechanism (VSRM) for sarcoplasmic reticulum Ca2+.
Inactivation was not detected. Sustained responses were insensitive to
inactivation or block of L-type Ca2+ current
(ICa-L). The voltage dependence of sustained
responses was not affected by changes in intracellular or extracellular Na+ concentration. Furthermore, sustained responses were
not inhibited by 2 mM Ni2+. Thus it is improbable that
ICa-L or Na+/Ca2+ exchange
generated these sustained responses. However, rapid application of 200 µM tetracaine, which blocks the VSRM, strongly inhibited sustained
contractions. Our study indicates that the VSRM includes both a phasic
inactivating and a sustained noninactivating component. The sustained
component contributes both to initiation and relaxation of contraction.
voltage-sensitive release mechanism; calcium-induced calcium release; excitation-contraction coupling; calcium transients
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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CONTRACTION IN HEART is initiated by release of Ca2+ stores from the sarcoplasmic reticulum (SR). Two fundamentally different processes that trigger release of SR Ca2+ have been proposed. Ca2+ release can be initiated in response to influx of trigger Ca2+. This process is known as Ca2+-induced Ca2+ release (CICR; see Ref. 9) and is thought mainly to be linked to Ca2+ influx through L-type Ca2+ channels in the sarcolemma (1, 3, 6, 7, 23, 26), although Ca2+ entry via Na+/Ca2+ exchange (Na/CaEX) may contribute under some conditions (19, 21, 22, 27, 39). Contractions and Ca2+ transients initiated by this mechanism typically are proportional to the magnitude of L-type Ca2+ current (ICa-L; see Refs. 2 and 3). Our recent studies have provided evidence for a second mechanism, a voltage-sensitive release mechanism (VSRM), that links release of SR Ca2+ to depolarization of the sarcolemma (11, 13, 15, 16). The VSRM continues to operate when measurable influx of Ca2+ has been eliminated, and contractions and Ca2+ transients initiated by the VSRM are not proportional to the magnitude of ICa-L (11, 13, 15, 16). The electrophysiological characteristics of CICR and the VSRM predict that both mechanisms would be triggered by the cardiac action potential and therefore likely contribute to initiation of contraction in heart.
Relaxation of contraction takes place when free intracellular Ca2+ levels decrease. Ca2+ levels are decreased primarily by uptake of Ca2+ into the SR but also by extrusion of Ca2+ by sarcolemmal Na/CaEX, and to a lesser extent by a sarcolemmal Ca2+ ATPase (2). For Ca2+ levels to decrease, release also must terminate. It has been proposed that release of SR Ca2+ is terminated by inactivation of SR Ca2+ release channels (10, 18, 34, 37, 38). Termination of release proceeds in a time-dependent manner and is independent of the initial influx of trigger Ca2+ through the sarcolemma (18, 34, 37, 38). Thus relaxation would follow a time course determined by termination of release in combination with removal of Ca2+ from the cytosol by the SR Ca2+ ATPase, the Na+/Ca2+ exchanger, and the sarcolemmal ATPase. However, recently, we have observed that contractions and Ca2+ transients do not decline completely when depolarization of the sarcolemma is maintained in voltage-clamped cardiac myocytes (12). Sustained responses were observed under conditions that allow activation of both the VSRM and CICR. This observation led us to hypothesize that membrane potential may play a role in termination, as well as initiation of SR Ca2+ release. The objectives of this study were to explore the role of membrane potential in regulation of contraction and relaxation in cardiac ventricular cells and to determine whether sustained responses are caused by CICR or by the VSRM.
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METHODS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Studies were conducted within the guidelines published by the Canadian Council on Animal Care and were approved by the Dalhousie University Committee on Animal Care. Guinea pig ventricular myocytes were dissociated enzymatically, as described earlier (13, 16). Cells were superfused (3 ml/min) at 37°C with solution containing (in mM) 50 NaCl, 100 choline chloride, 2 CaCl2, 4 KCl, 1 MgCl2, 10 glucose, 10 HEPES (pH 7.4 with NaOH; gassed with 100% O2), and 250 µM lidocaine and/or 50 µM TTX to block Na+ current. In some experiments, rapid solution changes at 37°C were made within 300 ms with a computer-triggered device (15).
In most experiments, discontinuous single-electrode voltage-clamp
recordings were made with Axoclamp 2A electronics and high-resistance microelectrodes (18-24 M
filled with 2.7 M KCl). In some
experiments, discontinuous single-electrode voltage-clamp recordings
were made with Axoclamp 2A electronics and 1-3 M patch pipettes
that contained (in mM) 60 KCl, 70 potassium aspartate, 0.05 8-bromo-cAMP, 4 MgATP, 1 MgCl2, 2.5 KH2PO4, 0.12 CaCl2, 0.5 EGTA, and
10 HEPES, pH 7.2 with KOH, as described previously (13). The
free Ca2+ concentration in the pipette solution was
calculated to be 46 nM (Ecal for windows version 1.1; Biosoft, 1996).
Liquid junction potentials were compensated before data acquisition.
Unloaded cell shortening was measured with a video edge detector (11, 13, 16). Cell fluorescence was measured with a Photon Technology International DeltaRAM system (Brunswick, NJ). Cells were loaded with 1.0 µM fura 2-AM (Molecular Probes) for 20 min at room temperature. After loading, extracellular dye was eliminated by superfusion of the cells with physiological buffer solution for 20 min. The emission field was limited to the size of a single myocyte with an adjustable window. Cells were excited at 340 nm, and fluorescence emitted by the cell was recorded at 510 nm. Background fluorescence was not subtracted. Changes in intracellular Ca2+ were expressed as the ratio of peak fluorescence transient (F) over baseline fluorescence (F0). Single wavelength excitation was used, since it allowed Ca2+ transients to be displayed and recorded with pCLAMP acquisition software along with current and voltage records during the experiments. Recording times with patch pipettes were kept as short as possible to minimize washout of fura 2. Significant washout of fura 2 was not detected in experiments with high-resistance microelectrodes.
Data were acquired and analyzed with pCLAMP 6.01. Recordings were
digitized at sample rates up to 50 kHz. Voltage-clamp test steps were
preceded by 10 conditioning pulses from a holding potential of
80 to 0 mV, to provide a consistent activation history, followed by repolarization to a postconditioning potential. Further details of
specific voltage-clamp protocols are provided in the relevant sections
in RESULTS.
Data are presented as means ± SE. Differences between means were assessed with a Student's t-test (P < 0.05 was considered significant). Lidocaine, tetracaine, choline chloride, nickel chloride, and cadmium chloride were purchased from Sigma Chemical. TTX was purchased from Alomone Laboratories, and ryanodine was from Calbiochem. All drugs were dissolved in deionized water.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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In initial experiments, contractions were elicited with a voltage-clamp
protocol (Fig. 1A) that activates
the VSRM and CICR separately (11, 13, 16). This protocol elicits two
phasic contractions, the first caused by the VSRM and the second
initiated by CICR coupled to ICa-L. It is evident
in Fig. 1B that phasic contractions initiated by both
mechanisms were followed by sustained contractions that lasted for the
duration of the depolarizing steps. To determine whether sustained
contractions were caused by ICa-L, we blocked
ICa-L with rapid application of 100 µM
Cd2+. Cd2+ inhibited the CICR contraction
coupled to ICa-L but not the sustained contraction
(Fig. 1C). The phasic contraction initiated by the VSRM also
remained. Furthermore, the sustained component began with the step that
activated the VSRM, rather than the step that initiated
ICa-L. These observations indicate that it is very
unlikely that the sustained contraction was initiated by influx of
Ca2+ via ICa-L.
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Persistence of the sustained contraction together with the phasic VSRM
contraction during inhibition of ICa-L suggests
that the sustained contraction also may be induced by the VSRM. It was
therefore important to determine whether the magnitude of sustained
contractions varied with membrane potential and whether the voltage
dependence matched that of the VSRM. To investigate this, we used
single voltage-clamp steps to different membrane potentials (Fig.
2A). The steps initiated phasic
contractions followed by sustained contractions, both of which became
greater with progressively stronger depolarization (Fig. 2B).
Mean contraction-voltage relations for phasic and sustained components
of contraction are shown in Fig. 2C. Figure 2C shows
that the maximum amplitude of the sustained component was less than
that of phasic contractions. However, the contraction-voltage relation
for sustained contractions appeared to be negative relative to that for
phasic contractions. To more easily visualize this, contraction-voltage
relations for phasic and sustained contractions were normalized to
maximum contraction and plotted in Fig. 2D. The normalized
contraction-voltage relations were fitted by Boltzmann functions of the
following form: y = (a b)/{1 + exp[(V Vh)/k]} + b, where
a and b are the maximum and minimum contractions,
V is the test potential, Vh is the
half-maximal voltage, and k is the slope factor.
Vh for the sustained component was 47.4 ± 1.5 mV (n = 11) and was significantly more negative than
Vh for the phasic component (38.7 ± 1.3 mV, n = 11; P < 0.05).
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The occurrence of sustained contractions suggests that release of
Ca2+ from the SR also may be sustained. To determine
whether the sustained component of contraction arises from SR release
of Ca2+, we superfused myocytes with 1 µM ryanodine, an
agent that disrupts SR function (2). Sequential activation steps from
65 to 40 and 0 mV (Fig. 2E) elicited both phasic
and tonic contractions before exposure to ryanodine (Fig. 2F).
After 15 min exposure to ryanodine, both the phasic VSRM contraction
and the sustained contraction were abolished (Fig. 2F). The
contraction initiated by ICa-L also was attenuated,
although a small contraction still remained. Similar results were
observed in 12 of 12 myocytes. These observations suggest that the
sustained component of contraction is likely caused by SR
Ca2+ release.
To determine whether sustained elevation of intracellular
Ca2+ accompanies maintained depolarization, additional
experiments were conducted in cells loaded with the
Ca2+-sensitive dye fura 2. Long (1-s) voltage steps to
membrane potentials between 70 and +20 mV initiated
Ca2+ transients with prominent voltage-dependent sustained
components (Fig. 3A). These results
confirmed that the sustained component of contraction was initiated by
sustained release of SR Ca2+. The mean amplitudes of the
sustained transients (F/F0) were plotted as a function of
test step voltage and were fitted with a Boltzmann function (Fig.
3B). The mean amplitudes of sustained transients showed a
sigmoidal voltage dependence that approached a plateau near 20
mV (Fig. 3B). The voltage dependence of sustained Ca2+ transients (Fig. 3B) was virtually identical
to that shown in Fig. 2D for sustained contractions.
Furthermore, Vh for sustained transients was
essentially the same as Vh observed for sustained contractions (Fig. 2D).
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Figure 3A also shows that sustained transients declined only
when myocytes were repolarized. To determine whether this decrease in
the transient also was graded by membrane potential, we modified the
voltage-clamp protocol so that an initial activation step to 0 mV was
followed by repolarization to different potentials between +20 and
90 mV (Fig. 4A). With this
protocol, the initial activation step always initiated a similar phasic
transient. However, this was followed by sustained transients with
amplitudes that varied with repolarization to different potentials
(Fig. 4A). The amplitudes of the sustained transients were
plotted as a function of the voltage of the repolarization step and
were fitted with a Boltzmann function (Fig. 4B). The voltage
dependence of the sustained transients observed with repolarizing steps
was sigmoidal (Fig. 4B) and was virtually identical to that
observed with activation steps (Fig. 3B). This observation
suggests that sustained transients show deactivation with the same
voltage dependence as activation.
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It is unlikely that ICa-L contributes to sustained
transients initiated with the protocol shown in Fig. 4A, as
ICa-L should inactivate during the initial
depolarizing step and should remain inactivated during maintained
depolarizations. To test this, we interpolated an activation step to 0 mV at the end of the repolarization steps as shown in Fig.
5A. The activation step to 0 mV was
preceded by a 3-ms return to 70 mV to provide a constant
activation step. The magnitude of ICa-L elicited by
the test step varied in response to changes in preceding potential
(Fig. 5A, bottom). Peak inward current was plotted as a
function of the preceding conditioning potential in Fig. 5B. A
Boltzmann function fitted to these mean data had a
Vh of 33.6 mV. The relation between
magnitude of peak inward current and the preceding potential
demonstrated that ICa-L was inactivated at
potentials that elicited maximal sustained transients and was only
fully available at potentials where sustained transients were minimal
(Fig. 5B). Thus the curve describing the voltage dependence of
availability of ICa-L (Fig. 5B) was
opposite to the curve exhibited by sustained transients (Figs.
3B and 4B), which further indicates that a role for
ICa-L in sustained transients is highly unlikely.
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To evaluate a possible role of Na/CaEX in sustained
transients, we used several approaches. First, we determined the
voltage dependence of deactivation in cells superfused with
extracellular solution that contained 50 or 100 mM extracellular
Na+. If sustained transients are caused by
Na/CaEX, the voltage dependence of the transient-voltage
relation should shift in response to a twofold change in extracellular
Na+ concentration (4, 8, 17). Figure
6A shows plots of mean amplitudes
of sustained Ca2+ transients recorded with the deactivation
protocol shown in Fig. 4A. Curves recorded in 50 or 100 mM
extracellular Na+ were superimposable.
Vh for deactivation in 100 mM Na+ was
43.0 mV (n = 4) and was not significantly different from Vh of 44.8 mV determined in 50 mM
Na+ (n = 11). The absence of an effect of doubling
of Na+ concentration on deactivation indicates that it is
unlikely that Na/CaEX contributed to these transients.
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A second approach to evaluate the role of Na/CaEX in sustained transients was to determine whether sustained transients were present in myocytes dialyzed with 0 mM Na+, which has been shown to prevent contractions initiated by reverse Na/CaEX (20, 27, 39). Figure 6B, inset, shows that a sustained Ca2+ transient was still present in a representative experiment conducted with patch pipettes that contained 0 mM Na+. Figure 6B also shows a plot of mean amplitudes of sustained transients, recorded from cells dialyzed with 0 mM Na+, as a function of repolarization potential. The protocol used was identical to that shown in Fig. 4A. The deactivation curve (Fig. 6B) exhibited a value of Vh very similar to that determined in undialyzed cells (Figs. 3B, 4B, and 6A). Thus experimental manipulation of intracellular Na+ also indicates it is very unlikely that Na/CaEX generated these sustained transients.
A third approach to evaluate a possible role of Na/CaEX in
sustained responses was to compare effects of agents known to inhibit either Na/CaEX or the VSRM. Effects of Ni2+ and
tetracaine were examined on sustained contractions initiated by the
voltage-clamp protocol shown in Fig.
7A, inset. An initial test
step from 65 to 0 mV was followed by a 7-s maintained
repolarization step to 20 mV. This resulted in a rapid phasic
contraction followed by a sustained contraction (Fig. 7A). Test
agents were applied with the rapid solution changer during the step to
20 mV. Application of 2 mM Ni2+, an inhibitor of
Na/CaEX (17), had little effect on sustained contractions
(Fig. 7A). In contrast, application of 200 µM tetracaine (Fig. 7B), which does not block Na/CaEX (28, 29)
but which inhibits the VSRM (24), caused a prompt but reversible
inhibition of the sustained contraction. These results in combination
demonstrate that sustained responses are not caused by
Na/CaEX but are likely caused by the VSRM.
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One new characteristic not previously reported for the VSRM is the
ability to maintain continuous release of Ca2+. Our
previous studies showed that phasic VSRM contractions are subject to
steady-state inactivation (13, 16). The existence of sustained
contractions and Ca2+ transients, however, suggests that
there is a noninactivating component of the VSRM. We therefore compared
the role of inactivation in determining the magnitude of sustained and
phasic VSRM contractions with the protocol shown in Fig.
8A, inset. Here we used an
activation step to 35 mV to elicit VSRM contractions selectively
(13, 16). To evaluate inactivation, the test step was preceded by conditioning steps to potentials between 30 and 105 mV.
The test steps elicited phasic contractions (b) superimposed
upon sustained contractions (c) (Fig. 8A). The
amplitudes of the phasic contractions varied with preceding
conditioning potential, whereas the amplitude of the sustained
component was constant (Fig. 8A). The mean amplitudes of phasic
contractions (b-c) are plotted as a function of preceding
conditioning potential in Fig. 8B. This plot shows that phasic
contractions exhibited steady-state inactivation and approached a
minimum with conditioning potentials near 30 mV (Fig.
8B). The representative recordings shown in Fig. 8A
show that cell length preceding phasic contractions (a) also
changed in response to conditioning potential. These changes in cell
length (a) measured with respect to a constant
reference at d were plotted as a function of conditioning
potential in Fig. 8C. The contraction-voltage relation for cell
length followed the same activation-deactivation relation as that
described for Ca2+ transients (Fig. 4B).
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Developed contraction normally is measured as the difference between peak contraction and preceding diastolic length. In the present experiment, this would correspond to the difference between b and a (Fig. 8A), which is plotted as a function of preceding conditioning potential in Fig. 8D. The resulting curve is identical to the steady-state inactivation curve previously described for the VSRM (13, 16). However, here we show that the magnitude of developed contraction initiated by the VSRM is determined by a combination of inactivation of the phasic component of the VSRM and voltage-dependent changes in diastolic length regulated by the activation/deactivation properties of the sustained component.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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The objectives of this study were to determine whether sustained contractions represent a component of excitation-contraction coupling, which contributes to initiation and/or relaxation of contraction in cardiac myocytes, and to determine whether sustained responses are caused by CICR or the VSRM. Our results indicate that maintained depolarization causes sustained Ca2+ transients and contractions, and that relaxation of these sustained responses occurs only upon repolarization to membrane potentials near the normal resting membrane potential of ventricular myocytes. Our experiments indicate that the sustained component represents maintained SR Ca2+ release. Furthermore, our observations indicate that it is improbable that CICR coupled to ICa-L or Na/CaEX initiates these sustained responses. Instead, our observations indicate that sustained responses represent a component of the VSRM. The contribution of the VSRM to initiation of contraction likely involves both phasic and sustained components. Although relaxation of the phasic component of VSRM contraction proceeds independently of membrane potential, relaxation of the sustained component is controlled by membrane potential.
A major finding in this study was that cardiac myocytes exhibit a component of contraction that is maintained at potentials positive to the resting membrane potential. The voltage dependence of these contractions or transients is described by a Boltzmann function, as would be predicted for a phenomenon that is regulated by charge movement in a voltage sensor (14). The voltage dependence of sustained transients was the same regardless of the direction of membrane potential change. This suggests that sustained transients are regulated by a mechanism that exhibits activation and deactivation with virtually identical voltage dependencies. Furthermore, no evidence of inactivation was observed with sustained responses up to 7 s in duration.
In theory, several mechanisms might be responsible for generation of sustained Ca2+ transients and contractions; these include CICR coupled to ICa-L, Na+ current, or Na/CaEX , or alternatively, the VSRM. It is unlikely that ICa-L causes the sustained phenomena, since sustained contractions persisted in the presence of ICa-L blockade with Cd2+ or when ICa-L was inactivated by sustained depolarization. In fact, sustained Ca2+ transients were maximal at membrane potentials that strongly inactivated ICa-L. Also, sustained contractions and Ca2+ transients appeared at membrane potentials more negative to those at which ICa-L is significantly activated (25). The activation-deactivation curve for sustained transients was similar to the voltage dependence of the VSRM described previously (11, 13, 16).
Our results also suggest that it is unlikely that the sustained responses are initiated by mechanisms of excitation-contraction coupling linked to activation of Na+ channels. Ca2+ influx through Na+ channels has been reported to initiate cardiac contraction in isolated myocytes treated with isoproterenol or ouabain (31). In addition, Na+ influx through Na+ channels may initiate CICR by causing Ca2+ influx via reverse-mode Na/CaEX (19, 22 but also see 5, 33, 36). Both of these mechanisms for initiation of contraction are blocked by Na+ channel blockers. However, the sustained responses in the present study could not have been initiated by either of these mechanisms, since they were not affected by Na+ channel blockade with either lidocaine or TTX.
Our observations also indicate that it is highly unlikely that CICR coupled to influx of Ca2+ through Na/CaEX initiates the sustained contractions and transients described in this study. The voltage dependence of activation-deactivation was independent of changes in concentration of extracellular Na+, which have been shown to shift the voltage dependence of the exchanger (4, 8, 17). Also, sustained transients with an identical voltage dependence were demonstrated in experiments in which cells were dialyzed with patch pipette solution with 0 mM Na+ to inhibit reverse-mode Na/CaEX (20, 27, 39). Furthermore, sustained contractions were not affected by 2 mM Ni2+, which significantly inhibits Na/CaEX (17). In contrast, 200 µM tetracaine, which inhibits the VSRM (24) but not Na/CaEX (28, 29), strongly inhibited sustained contractions.
The sustained components of contractions and Ca2+ transients described in this study exhibit properties that are characteristic of the VSRM. Sustained responses exhibited a sigmoidal voltage dependence that was well described by a Boltzmann function with a Vh identical to that described for the VSRM (13, 16). The sustained responses, like the VSRM, were not inhibited by agents or conditions that inhibit contractions and transients initiated by ICa-L, Na/CaEX, or Na+ current. Although sustained contractions and transients were insensitive to Cd2+ and Ni2+, they were strongly inhibited by tetracaine, a known blocker of the VSRM (24). These similarities indicate that the phasic and sustained components are most likely initiated by the same event. However, one striking difference between these two phases is that the phasic component exhibits inactivation, whereas the sustained component does not. This difference is reminiscent of the properties of two components of Ca2+ release described for skeletal muscle excitation-contraction coupling. Indeed, the VSRM transients observed in the present study bear a striking resemblance to Ca2+ transients recorded from skeletal muscle (30, 35). Transients in skeletal muscle exhibit an initial rapid phase, which inactivates, followed by a noninactivating sustained component (32, 35). In skeletal muscle, the sustained component is believed to represent activation of ryanodine receptors by the voltage sensor. It has been suggested that the initial phasic component is large because Ca2+ released by ryanodine receptors coupled to voltage sensors recruits adjacent ryanodine receptors through CICR (30). This results in a multiplier or amplification system that exhibits inactivation, possibly through a Ca2+-dependent mechanism (30, 32). One may speculate that similar mechanisms are responsible for the phasic and sustained components of Ca2+ release observed in cardiac myocytes. Clearly, additional studies will be required to test this possibility.
In previous studies, we have focused on the phasic component of the VSRM. However, evidence for the sustained component can be found in many of our figures published earlier [e.g., Fig. 10 (11); Figs. 3 and 5 (15); Fig. 10 (16)]. In other examples, the existence of the sustained component was obscured by use of less negative postconditioning potentials and recording windows that did not include sufficient baseline recording both before and after the contractions and transients. In the present study, we have used techniques to clearly show the relation of the contractions and Ca2+ transients to the diastolic levels before and after the events. With this approach, the sustained component is very evident.
Interestingly, sustained VSRM contractions and transients were normally very stable and did not exhibit oscillatory behavior. Our observations with ryanodine indicate that sustained VSRM contractions are generated by release of SR stores of Ca2+. Thus our observations suggest that it is likely that released Ca2+ is taken back up by the SR and rereleased. These considerations suggest that, under the conditions of our experiments, Ca2+ release, uptake, and rerelease must reach a stable equilibrium that does not spontaneously oscillate.
In contrast to earlier concepts of excitation-contraction coupling in heart, our results demonstrate that sustained release of Ca2+ can be regulated by membrane potential through the VSRM. Through voltage-dependent activation and deactivation, membrane potential adjusts release of Ca2+ stores and determines contraction and relaxation of the cardiac cell. Activation of contraction by the VSRM includes activation of both sustained and phasic components of Ca2+ release. Relaxation of the phasic component of contraction occurs even when the cell membrane remains depolarized. However, termination of sustained Ca2+ release requires repolarization. Thus the VSRM is a mechanism of excitation-contraction coupling that actively controls both contraction and relaxation in cardiac myocytes. Our study demonstrates that we must revise our concepts of excitation-contraction coupling in heart to include an important contribution of Ca2+ release linked to membrane potential, in addition to CICR coupled to Ca2+ influx.
Because the sustained component of the VSRM is graded by voltage, this component might delay relaxation in cardiac hypertrophy or failure where the action potential is significantly prolonged (40). Furthermore, sustained Ca2+ release graded by the VSRM may alter diastolic compliance, especially in disease conditions that result in reduction of membrane potential. Thus our observations have important implications for regulation of contraction in diseased and normal hearts.
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ACKNOWLEDGEMENTS |
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We thank J. Q. Zhu, Peter Nicholl, and Claire Guyette for technical assistance.
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FOOTNOTES |
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This work was supported by the Medical Research Council of Canada and by the Heart and Stroke Foundation of Nova Scotia.
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. §1734 solely to indicate this fact.
Address for reprint requests and other correspondence: G. R. Ferrier and S. E. Howlett, Dept. of Pharmacology, Sir Charles Tupper Medical Bldg., Dalhousie Univ., Halifax, Nova Scotia, Canada B3H 4H7 (E-mail: Gregory.Ferrier{at}dal.ca and Susan.Howlett{at}dal.ca).
Received 9 July 1999; accepted in final form 2 December 1999.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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) and sustained (
) components, both of which increased
with depolarization. C: mean contraction-voltage curves for
phasic and sustained components of contraction. D: normalized
contraction-voltage relations for phasic and sustained contractions
were fitted by Boltzmann functions. Half-maximal voltage
(Vh) for the sustained component was 
f, Change in fluorescence. B:
amplitudes of the sustained transients [peak fluorescence
transient (F)/baseline fluorescence (F0)] showed a
sigmoidal dependence on membrane potential, which was fit with a
Boltzmann function (n = 11).
