Cardiac excitation-contraction coupling: role of membrane potential in regulation of contraction

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INVITED REVIEW
Cardiac excitation-contraction coupling: role of membrane potential in regulation of contraction

Gregory R. Ferrier and Susan E. Howlett

Cardiovascular Research Laboratories, Department of Pharmacology, Dalhousie University, Halifax, Nova Scotia, Canada B3H 4H7

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
CA²⁺-INDUCED CA²⁺ RELEASE
VOLTAGE-SENSITIVE RELEASE...
REGULATION OF VSRM BY...
CONDITIONS REQUIRED FOR...
MECHANISM OF EC COUPLING...
ROLE OF VSRM IN...
SUMMARY
REFERENCES

The steps that couple depolarization of the cardiac cell membrane to initiation of contraction remain controversial. Depolarizationtriggers a rise in intracellular free Ca²⁺ which activates contractile myofilaments. Most of this Ca²⁺ is released from the sarcoplasmic reticulum (SR). Two fundamentallydifferent mechanisms have been proposed for SR Ca²⁺ release: Ca²⁺-induced Ca²⁺ release (CICR) and a voltage-sensitive release mechanism (VSRM).Both mechanisms operate in the same cell and may contribute tocontraction. CICR couples the release of SR Ca²⁺ closely to the magnitude of the L-type Ca²⁺ current. In contrast, the VSRM is graded by membrane potentialrather than Ca²⁺ current. The electrophysiological and pharmacological characteristicsof the VSRM are strikingly different from CICR. Furthermore, theVSRM is strongly modulated by phosphorylation and provides a newregulatory mechanism for cardiac contraction. The VSRM is depressedin heart failure and may play an important role in contractiledysfunction. This review explores the operation and characteristicsof the VSRM and CICR and discusses the impact of the VSRM on ourunderstanding of cardiac excitation-contractioncoupling.

voltage-sensitive release mechanism; calcium-induced calcium release; heart failure; phosphorylation; sarcoplasmic reticulum

	INTRODUCTION

TOP ABSTRACT INTRODUCTION CA²⁺-INDUCED CA²⁺ RELEASE VOLTAGE-SENSITIVE RELEASE... REGULATION OF VSRM BY... CONDITIONS REQUIRED FOR... MECHANISM OF EC COUPLING... ROLE OF VSRM IN... SUMMARY REFERENCES

CONTRACTION IN THE HEART is initiated by a transient rise in intracellular free Ca²⁺. The cardiac action potential triggers this Ca²⁺ transient, which rapidly rises and decays with each cardiac cycle.The events that couple depolarization of the sarcolemma to elevationof Ca²⁺ and initiation of contraction are referred to as excitation-contractioncoupling (EC coupling). Several mechanisms of EC coupling havebeen proposed for cardiac muscle, and some of these are controversial.This article reviews various mechanisms of EC coupling, theircharacteristics, and evidence for their roles in ECcoupling.

	CA²⁺-INDUCED CA²⁺ RELEASE

TOP ABSTRACT INTRODUCTION CA²⁺-INDUCED CA²⁺ RELEASE VOLTAGE-SENSITIVE RELEASE... REGULATION OF VSRM BY... CONDITIONS REQUIRED FOR... MECHANISM OF EC COUPLING... ROLE OF VSRM IN... SUMMARY REFERENCES

Many studies of EC coupling conducted in the 1970s and 1980s established that depolarization of the cell membrane triggeredcardiac contraction (reviewed in Refs. 29, 36). Depolarizationalso activates inward Ca²⁺ current, and several hypotheses relating activation of Ca²⁺ current to contraction were proposed (2, 28, 53, 56).The role of Ca²⁺ influx was explored further by Fabiato (15-17) in studies thatwere conducted on "skinned" myocardial cells (i.e., cells thathave had their sarcolemma removed by mechanical or chemical means).Fabiato (15-17) showed that rapid application of Ca²⁺-containing solutions to skinned myocytes could trigger releaseof Ca²⁺ from intracellular stores. Fabiato also showed that Ca²⁺ release could be blocked by ryanodine, an agent that disruptssarcoplasmic reticulum (SR) release channels (ryanodine receptors)and that is used widely to identify involvement of SR Ca²⁺ release in contraction (3, 64, 82). These studies (15-17)showed that SR Ca²⁺ release in the heart can be triggered by a rise in Ca²⁺ concentration in the vicinity of ryanodine receptors. The processby which a small amount of Ca²⁺ triggers release of SR Ca²⁺ has been called Ca²⁺-induced Ca²⁺ release (CICR) (14).

Although Fabiato's studies showed that CICR occurred in response to application of Ca²⁺ to skinned myocytes, it was essential to determine whether CICRalso occurred in cells when the sarcolemma was intact. This wasshown in experiments on intact ventricular myocytes in which theinitial small increase in free Ca²⁺ (trigger Ca²⁺) was provided by photolysis of "caged" (chelated) Ca²⁺ (54, 86). As in skinned myocytes, this initial small risein Ca²⁺ triggered a much larger rise in intracellular free Ca²⁺, which was released from the SR. Thus CICR can initiate releaseof SR Ca²⁺ in both skinned and intact cardiacmyocytes.

Hypothetically, the source of trigger Ca²⁺ for CICR under physiological conditions could be intracellular or extracellular.Evidence for an essential role of extracellular Ca²⁺ in initiation of CICR contractions comes from a study by Nabaueret al. (52). This study demonstrated that SR Ca²⁺ release in ventricular myocytes does not occur in the absenceof extracellular Ca²⁺. This suggests either that influx of Ca²⁺ from the extracellular space may provide the trigger that activatesCICR, or that Ca²⁺ must be present at an extracellular site on the cell for initiationofcontraction.

The specific routes of Ca²⁺ entry that initiate CICR have been investigated. Many studies provide evidence that influx of Ca²⁺ through L-type Ca²⁺ channels is an important trigger for CICR. For example, voltage-clampstudies (1, 3, 4, 12, 13, 43) demonstrate thatCICR is graded by the magnitude of peak L-type Ca²⁺ current (I_Ca-L). In these studies, Ca²⁺ transients or contractions were initiated by test steps to differentmembrane potentials. The magnitudes of Ca²⁺ transients (Fig. 1A) and contractions were proportional to themagnitudes of I_Ca-L initiated by the same test steps. Therefore,the relationship between Ca²⁺ transients (or contractions) and membrane potential was bellshaped, like the current-voltage (I-V) relationship for I_Ca-L(Fig. 1B). At potentials where I_Ca-L was minimal, contractionsand transients also were negligible. In addition, Nabauer et al.(52) showed that in the absence of extracellular Ca²⁺, Na⁺ influx through Ca²⁺ channels did not initiate SR Ca²⁺ release. Because of these observations, it is generally acceptedthat I_Ca-L is the primary trigger for CICR in cardiac cells.

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Fig. 1. Ca²⁺ transients initiated by Ca²⁺-induced Ca²⁺ release (CICR) are proportional to the magnitude of inward Ca²⁺ current. A: recordings of Ca²⁺ transients (top) and verapamil-sensitive currents (bottom) initiated by steps from $-$ 40 mV to different membrane potentials in a voltage-clamped guinea pig ventricular myocyte. Voltages of the test steps are indicated below the respective current traces. B: plots of amplitudes of Ca²⁺ transients (top) and of verapamil-sensitive current (bottom) as a function of the voltage-clamp test steps. [From Beuckelmann and Wier (4)]

T-type Ca²⁺ channels provide a second route of influx of Ca²⁺ through the sarcolemma. Several studies (78, 94) demonstratethat influx of Ca²⁺ by this route also can trigger CICR. However, these studies indicatedthat T-type Ca²⁺ current is a very weak trigger for CICR and probably does notcontribute substantially to EC coupling in ventricularmyocytes.

The Na⁺/Ca²⁺ exchanger (NaCa_EX) also has been proposed as a trigger for CICR. Normally, the NaCa_EX is believed to extrude Ca²⁺ equal to the amount that enters the cell through voltage-gatedchannels during each cardiac cycle (7). However, at positivepotentials the direction of exchange can reverse, and Ca²⁺ can enter by this route and induce slow, ramplike contractions(69, 71, 83). Contractions initiated by this mechanism mayremain large or even increase in amplitude with voltage stepsto very positive potentials. These slow, ramplike contractionspersist in the presence of ryanodine, which suggests that theyare activated directly by Ca²⁺ entering through the sarcolemma rather than by release of SRCa²⁺ (69, 71). However, a number of studies (26, 38, 55,88, 89) provide evidence that Ca²⁺ influx through reverse NaCa_EX also may trigger SR Ca²⁺ release via CICR. In these studies, phasic contractions and Ca²⁺ transients attributed to CICR coupled to NaCa_EX were observedwhen reverse NaCa_EX was enhanced by high (10-20 mM) intracellularNa⁺levels.

Contractions also can be triggered by CICR in response to rapid elevation of intracellular Na⁺ following Na⁺ influx through voltage-gated Na⁺ channels (34, 35, 39). When this occurs, it is believedthat the sudden rise in intracellular Na⁺ may initiate CICR by promoting influx of Ca²⁺ via reverse NaCa_EX (34, 35, 39). However, initiation ofCa²⁺ release by this mechanism has not been observed under all experimentalconditions (6, 71, 77). These differing observations mayreflect the relative inefficiency of the NaCa_EX as a trigger forCICR (79) as well as differences in the transmembrane gradientsof Na⁺ and Ca²⁺ under different experimentalconditions.

The concept of CICR holds that influx of a small amount of Ca²⁺ will activate release of a larger quantity of Ca²⁺ by opening ryanodine receptors in the SR membrane. However, CICRis intrinsically a positive feedback system that leads to a paradox(81). It is logical that Ca²⁺ released by these ryanodine receptors would recruit other nearbyryanodine receptors, and that this secondary activation of Ca²⁺ release might become regenerative and activate even more distantryanodine receptors. This positive feedback system would be expectedto continue until all ryanodine receptors throughout the cellare activated. Thus one would predict a maximal release of SRCa²⁺ whenever depolarization initiates Ca²⁺ influx, regardless of the magnitude of the trigger. However,many studies show that the magnitude of Ca²⁺ release initiated by I_Ca-L is proportional to the peak amplitudeof this current. This paradox has led to formulation of a conceptknown as local control theory (8, 44, 81). According tothis theory, Ca²⁺ release from ryanodine receptors is controlled by Ca²⁺ influx through immediately adjacent L-channels and not by a generalizedrise in the concentration of intracellular free Ca²⁺ throughout the cytosol (9, 45, 65). Thus activation ofa single L-channel might cause a localized flux of Ca²⁺ sufficient to fully activate a group of neighboring ryanodinereceptors. However, this activation does not spread to distantryanodine receptors. Each L-channel and its functionally associatedryanodine receptors would constitute a release unit. Gradationof contraction by magnitude of whole cell I_Ca-L would reflectthe number of release units activated, rather than a change inCa²⁺ flux through individual ryanodinereceptors.

Evidence for local activation of Ca²⁺ release and release units comes from experiments with laser scanning confocal microscopyin cells loaded with Ca²⁺-sensitive fluorescent dyes. Cheng et al. (11) first demonstratedthat SR Ca²⁺ release in cardiac myocytes can occur as quanta, which they called"Ca²⁺ sparks." Sparks are discrete foci of increased fluorescence inresponse to interaction of released Ca²⁺ with fluorescent dye. Ca²⁺ sparks appear to originate near specialized Ca²⁺ release regions (junctional regions between SR and t tubules)both in cardiac myocytes (5, 59, 70) and in skeletal muscle(67). Sparks exhibit characteristic amplitudes, widths, anddurations (10, 24, 46). These properties are stochasticand therefore do not vary with the stimulus magnitude. Thus sparksmay represent the fundamental release units proposed in localcontrol theory. Ca²⁺ transients are thought to be generated by the sum of numeroussparks (8, 10, 44, 65), and the magnitude of the Ca²⁺ transient would reflect the number of release unitsactivated.

Local control theory can explain the bell-shaped dependence of contractions and Ca²⁺ transients on the magnitude of I_Ca-L at different membrane potentials(8, 44). At negative membrane potentials at which I_Ca-L andcontraction first appear, only a small number of L-channels areactivated. Therefore, only a small number of sparks, or releaseunits, will be activated and contraction will be weak (Fig. 2).As voltage steps are made progressively more positive, the numberof activated L-channels increases, and this causes correspondingincreases in the number of release units and the amplitude ofcontraction. Eventually, at more positive potentials, contractionsdecrease in amplitude, even though essentially all L-channelsare activated. This is thought to occur when the driving forcefor Ca²⁺ influx declines and the magnitude of I_Ca-L through individualchannels decreases (8, 44). As membrane potential moves towardthe reversal potential for I_Ca-L, the number of L-channels generatingcurrent sufficient to activate a release unit decreases. Therefore,there is a decrease in the number of release units activated andthe magnitude of contraction declines. Thus the bell-shaped contraction-voltagerelation for CICR coupled to I_Ca-L reflects the number of releaseunits recruited at different membrane potentials.

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Fig. 2. Relationship between the voltage dependence of Ca²⁺ sparks and local control theory. A: relationship between the number of local Ca²⁺ transients (nLCT, also called Ca²⁺ sparks) and time after initiation of voltage-clamp steps to different membrane potentials. The probability of LCT occurring was highest near the beginning of each 200-ms test step and declined markedly by the end of the step. The late LCT shown for the test step to +70 mV occurred upon repolarization. B: relationship between the peak nLCT evoked by a given step and the membrane potential (V_p) of the test step. The frequency of LCT demonstrated a bell-shaped relationship to V_p, which resembles the bell-shaped relationship between Ca²⁺ transients and test step voltage shown in Fig. 1. C: probability of a single L-channel opening resulting in a LCT. Solid line, open probability of L-type Ca²⁺ channels (P_o,L) as a function of V_p. Filled circles, relationship between peak nLCT and V_p (B) normalized to the maximum nLCT observed with V_p = +10 mV. Open squares, normalized nLCT divided by P_o,L for the corresponding V_p. This measurement is interpreted as the probability of a LCT occurring at different membrane potentials (P_i,LCT). The relationship of P_i,LCT to V_p is indicated by the broken line. Thus the probability of an L-channel opening initiating a Ca²⁺ spark is very high with test steps to negative membrane potentials, because the driving force for Ca²⁺ entry is high and the single channel current would be large. However, P_i,LCT declines with test steps to more positive membrane potentials, where the driving force for Ca²⁺ entry is small, and the current associated with L-channel opening becomes small. Reprinted with permission from: Lopez-Lopez JR, Shacklock PS, Balke CW, and Weir WG. Local calcium transients triggered by single L-type calcium channel currents in cardiac cells. [Science 268: 1042-1045, 1995 (45). Copyright 1995 American Association for the Advancement of Science]

Although sparks have been proposed as a fundamental release unit for SR Ca²⁺ release, some studies have presented evidence for Ca²⁺ transients in the absence of Ca²⁺ sparks. For example, Lipp and Niggli (40) demonstrate SR Ca²⁺ release without sparks in response to "flash-photolysis" of cagedCa²⁺ in cardiac myocytes. Lopez-Lopez et al. (45) also observedCa²⁺ transients without Ca²⁺ sparks when Ca²⁺ transients were initiated by NaCa_EX. However, this study didnot determine whether these Ca²⁺ transients involved Ca²⁺ release as well as Ca²⁺ influx. Ca²⁺ release in the absence of sparks also may play an important rolein mammalian skeletal muscle. Transients characterized by a rapiddiffuse rise in Ca²⁺ without visible sparks have been reported in adult rat skeletalmuscle (75). In amphibian skeletal muscle, Ca²⁺ sparks accompany Ca²⁺ transients; however, Ca²⁺ sparks can be abolished with tetracaine without eliminating theCa²⁺ transient (76). These observations indicate that sparks arenot required for initiation of Ca²⁺ transients in skeletal muscle. There also is evidence that quantalrelease events smaller than sparks may occur in cardiac and skeletalmuscle. Lipp and Niggli (40, 41) and Tsugorka et al. (84)measured SR Ca²⁺ release events (called "quarks"), which are 5 to 10 times smallerthan Ca²⁺ sparks in cardiac and skeletal muscles. Thus it would appearthat several fundamental release units or modes may exist, includingsparks, quarks, and even finer release units. The relationshipbetween these alternate release modes and local control theoryis unknown and will require further study with very high resolutionmeasurements.

	VOLTAGE-SENSITIVE RELEASE MECHANISM

TOP ABSTRACT INTRODUCTION CA²⁺-INDUCED CA²⁺ RELEASE VOLTAGE-SENSITIVE RELEASE... REGULATION OF VSRM BY... CONDITIONS REQUIRED FOR... MECHANISM OF EC COUPLING... ROLE OF VSRM IN... SUMMARY REFERENCES

In cardiac muscle, Ca²⁺ sparks and local control theory can explain how CICR generates contractions and Ca²⁺ transients, which are proportional to I_Ca-L. However, it hasbecome apparent that SR Ca²⁺ release and contraction are not always proportional to magnitudeof I_Ca-L. Studies in isolated cardiac myocytes demonstrate anadditional mechanism for SR Ca²⁺ release in which the magnitude of Ca²⁺ transients and contraction are graded by membrane potential ratherthan the magnitude of I_Ca-L (18, 20, 22, 29, 31, 96).This mechanism can initiate SR Ca²⁺ release and contraction when CICR coupled to I_Ca-L, Na current(I_Na), or NaCa_EX is inhibited (18, 20, 22, 27, 31, 96).Because this mechanism is graded by membrane voltage rather thancurrent, it has been named the voltage-sensitive release mechanism(VSRM) (29, 31).

Both CICR and the VSRM are triggered by depolarization. The VSRM is first activated at relatively negative membrane potentials(near $-$ 60 mV), whereas CICR coupled to I_Ca-L is first activatedwhen significant I_Ca-L appears (near $-$ 30 mV). Under physiologicalconditions, when contraction is triggered by action potentials,both mechanisms would be activated and likely contribute to initiationof contraction. However, experimentally it is possible to activateCICR and the VSRM separately with voltage-clamp techniques (18,31). Experiments in which these mechanisms are activated separatelydemonstrated that phasic contractions can be triggered by eitherCICR or the VSRM (Fig. 3). Interestingly, when cells are activatedwith long depolarizations, the VSRM also triggers sustained Ca²⁺ release and sustained contraction (20). In contrast, CICR resultsin only a phasic contraction, which terminates with a characteristictime course even if Ca²⁺ influx is prolonged (72).

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Fig. 3. Separation of voltage-sensitive release mechanism (VSRM) and CICR components of excitation-contraction coupling with voltage-clamp techniques. Top: schematic of the voltage-clamp protocol, which consisted of conditioning pulses followed by a 4-s step to a postconditioning potential of $-$ 65 mV and then two sequential test steps to $-$ 40 and 0 mV. Thick bar, period during which drugs were applied with a computer-controlled rapid solution switching device. A: phasic contractions (top trace) initiated by the VSRM and CICR were elicited by the test steps to $-$ 40 and 0 mV, respectively. L-type Ca²⁺ current (I_Ca-L) occurred with the step to 0 mV (bottom trace). B: rapid application of 100 µM Cd²⁺ abolished I_Ca-L and the CICR contraction elicited by the step to 0 mV. Both the phasic and the sustained component of the VSRM remained when CICR was inhibited with Cd²⁺. [From Ferrier et al. (20)]

The VSRM is characterized by electrophysiological and pharmacological properties that allow it to be distinguished from othermechanisms of EC coupling (18-20, 22, 27, 31, 47, 48,62, 93, 96). Voltage-clamp studies demonstrate that, incontrast to CICR coupled to I_Ca-L, the voltage dependence of theVSRM is sigmoidal (Fig. 4A). Phasic contractions and Ca²⁺ transients initiated when the VSRM is activated first appearwith voltage steps to approximately $-$ 60 mV, reach a plateau near $-$ 20 mV, and then remain relatively constant with voltage stepsas positive as +80 mV (18, 22, 31, 96). Inward Ca²⁺ current measured in the same experiments exhibits a typical bell-shapedI-V relationship, which peaks near 0 mV and declines toward zeroor reverses as voltage steps approach +60 mV (Fig. 4B). Thus themagnitude of contractions initiated by the VSRM clearly is notproportional to the amplitude of inward current, and contractionsremain maximal at membrane potentials near or beyond the reversalpotential for I_Ca-L. However, when test steps to the same voltageswere initiated from a conditioning potential of $-$ 40 mV at whichthe VSRM is inactivated, the contraction-voltage relationshipin the same cells became bell shaped and proportional to I_Ca-L(Fig. 4, A and B). These curves are typical of CICR as reportedin studies by others (Fig. 1B) (1, 4, 12, 13, 18,22, 31, 43, 96). Thus within the same cell one can demonstrateCICR, which is directly dependent on the magnitude of I_Ca-L, andthe VSRM, which is independent of the amplitude of I_Ca-L. Therefore,because these relationships to I_Ca-L are mutually exclusive, onemust postulate that CICR and the VSRM are mediated by differentmechanisms.

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Fig. 4. Activation and inactivation properties of the VSRM are distinct from those of CICR and I_Ca-L. A and B: mean contraction-voltage (A) and current-voltage relations (B) were recorded from rat ventricular myocytes voltage clamped with high-resistance microelectrodes (n = 12). Plots show magnitudes of contractions and Ca²⁺ currents activated by 200-ms depolarizing steps to different potentials from a postconditioning potential of either $-$ 40 or $-$ 65 mV. When the postconditioning potential was $-$ 40 mV the VSRM was inactivated, and the contraction-voltage relationship was bell shaped and typical of CICR. When the postconditioning potential was $-$ 65 mV, both CICR and the VSRM are available for activation, and the contraction-voltage relationship became sigmoidal. In addition, activation was shifted to more negative potentials, and the maximum amplitude of contractions increased dramatically. Current-voltage relations were affected very little by the change in postconditioning potential from $-$ 40 to $-$ 65 mV. C: schematic of the voltage-clamp protocol utilized to examine steady-state inactivation of currents or contractions. The membrane was clamped to different conditioning voltages (V_PC) between the last conditioning pulse and a test step. A test step to $-$ 35 mV was used to assess the availability of the VSRM. A test step to 0 mV was used to assess availability of I_Ca-L. D: mean steady-state inactivation curves for contractions initiated by the VSRM and inward I_Ca-L recorded in rat ventricular myocytes. The half-inactivation voltages for the VSRM ( $-$ 53.2 ± 0.4 mV) and for I_Ca-L ( $-$ 25.3 ± 0.9 mV) were significantly different (P < 0.001, n = 9). [Panel D from Howlett et al. (31)]

The VSRM also can be distinguished from other mechanisms of EC coupling by inactivation characteristics. Phasic contractionsinduced by the VSRM exhibit steady-state inactivation. This canbe observed when initiation of these contractions is precededby depolarization to different membrane potentials (Fig. 4, Cand D) (20, 22, 30, 31, 96). Full availability of phasicVSRM contractions is seen when activation steps are made frommembrane potentials near or negative to $-$ 65 mV, whereas completeinactivation occurs with steps near or positive to $-$ 35 mV. Thevoltage dependence of inactivation can be described by a Boltzmannfunction with a half-inactivation voltage of approximately $-$ 50mV (Fig. 4D). These inactivation properties allow the VSRM tobe distinguished from CICR coupled to I_Ca-L, because I_Ca-L exhibitsa half-inactivation potential near $-$ 25 mV (Fig. 4D) (31). Theinactivation properties of the VSRM also serve to distinguishVSRM contractions from contractions initiated by reverse NaCa_EX.NaCa_EX does not inactivate, thus contractions initiated by reverseNaCa_EX can be elicited by depolarizing steps starting from membranepotentials at which the VSRM is inactivated (37, 42, 55,88, 89).

The activation and inactivation properties of the VSRM also provide the basis for separating phasic contractions initiatedby the VSRM and CICR as shown in Fig. 3 (18, 31). When cellsare depolarized by a step from $-$ 65 mV to $-$ 40 mV, the contractionor Ca²⁺ transient that is generated is initiated almost entirely by theVSRM. This occurs because the VSRM activates at more negativemembrane potentials than CICR coupled to I_Ca-L. However, whenactivation steps are made from $-$ 40 to 0 mV, the VSRM is largelyinactivated, whereas I_Ca-L is inactivated only slightly. Thusactivation steps initiated from a membrane potential of $-$ 40 mVelicit phasic contractions or Ca²⁺ transients generated almost entirely byCICR.

The VSRM also initiates a sustained component of Ca²⁺ release and contraction. Although the sustained component is typicallysmaller than the phasic component of the VSRM, it shows a sigmoidalvoltage dependence similar to the phasic component and remainsmaximal positive to $-$ 20 mV (Fig. 5, A and B) (20). In contrastto phasic VSRM contractions and transients, sustained responsespersist as long as depolarization is maintained, even for depolarizationslasting many seconds. Thus the sustained component does not showinactivation in response to maintained depolarization. Sustainedcontractions and transients terminate promptly on repolarizationto potentials near the resting membrane potential. If cells arenot repolarized abruptly, but stepwise, the sustained componentalso declines in a stepwise manner (Fig. 5, C and D). The declineof the sustained component shows a voltage dependence that isidentical to the voltage dependence of activation (20). Thusthe sustained component of the VSRM exhibits activation and deactivationthat follow the same relationship with membrane potential (Fig.5, B and D). The voltage dependence of the sustained componentof the VSRM allows the VSRM to grade sustained Ca²⁺ release and contraction reversibly between $-$ 80 and $-$ 20 mV. Becausedeactivation of the sustained component of the VSRM is gradedby membrane potential, changes in action potential duration couldaffect the time course of relaxation. Furthermore, full relaxationmay be prevented if the cell does not fully repolarize.

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Fig. 5. VSRM generates sustained Ca²⁺ transients that show activation and deactivation with identical voltage dependence. Sequence of voltage steps is in the direction of the arrows (A, C). A: guinea pig ventricular myocytes were depolarized to different potentials with the voltage-clamp protocol (top). Ca²⁺ transients were detected with fura-2. Progressively more positive activation steps elicited sustained Ca²⁺ transients (middle), which increased in amplitude until a maximum was reached. Currents are shown at bottom. B: activation curve derived by plotting mean amplitudes of sustained Ca²⁺ transients as a function of test potential. F, peak fluorescence; F₀ baseline fluorescence. C: voltage-clamp protocol used to investigate deactivation (top). Ca²⁺ transients and currents elicited by this protocol are shown by the middle and bottom traces. D: deactivation curve derived by plotting the amplitude of the sustained Ca²⁺ transient as a function of the repolarization voltage. The deactivation curve was very similar to the activation curve shown in B. The half-maximal voltage (V_h) was determined from Boltzmann fits and was similar for activation and deactivation of the sustained component of the VSRM. [Adapted from Ferrier et al. (20)]

Pharmacological characteristics also distinguish the VSRM from other mechanisms of EC coupling. Much of the pharmacologicalprofile for the VSRM has emerged from experiments designed toexplore how the VSRM functions. Many of these studies comparedeffects of different agents on the VSRM and CICR in experimentsin which both of these mechanisms were activated sequentially.Contractions and transients initiated by CICR are inhibited byagents that block I_Ca-L (Fig. 3) (20, 22, 27, 30, 31,47, 96). In contrast, VSRM contractions and/or transientsstill can be elicited when CICR is blocked by Cd²⁺, Ni²⁺, or nifedipine (20, 22, 27, 30, 31, 47, 96). BecauseNi²⁺ also blocks the T-type Ca²⁺ current (49, 85), persistence of the VSRM in the presenceof Ni²⁺ also indicates that the T-type Ca²⁺ current does not trigger the VSRM (20, 27). Further evidenceexcluding the T-type current comes from studies in adult rat ventricularmyocytes, in which T-type Ca²⁺ current cannot be detected (85), but in which VSRM contractionscan be observed (27, 31). The lack of inhibition of the VSRMby Ni²⁺ also serves to distinguish the VSRM from NaCa_EX. VSRM Ca²⁺ transients can be elicited in the presence of 2-5 mM Ni²⁺ and/or 0 mM intracellular Na⁺ (20, 27, 96), both of which inhibit contractions and transientsinitiated by NaCa_EX (32, 37, 55, 71, 88).

Inward Na⁺ or Ca²⁺ current carried by Na⁺ channels also can initiate CICR under certain conditions (34, 66). However, theVSRM is not inhibited by substitution of extracellular Na⁺ with choline or sucrose, or by block of I_Na with tetrodotoxinor lidocaine (18, 31, 47), which would block CICR secondaryto Na⁺ or Ca²⁺ influx through Na⁺ channels (34, 66). These findings demonstrate that VSRM contractionsand Ca²⁺ transients are not initiated by ion fluxes through Na⁺channels.

Although, the VSRM is not inhibited when I_Na is blocked by lidocaine or tetrodotoxin, or when cells are exposed to Na⁺-free solutions, the VSRM is inhibited by the local anesthetictetracaine (47). This effect can be observed in myocytes inwhich I_Na already has been inhibited either by lidocaine and/orby tetrodotoxin (20, 47, 96). Thus the effect of tetracaineappears not to be related to its ability to block Na⁺ channels. Tetracaine also is believed to act on ryanodine receptors(57, 58), and it is possible that tetracaine may inhibit theVSRM by an action at this site. When tetracaine is applied witha rapid solution changing device, it selectively blocks the VSRMwithout blocking CICR (47). The selective block of the VSRMby tetracaine can be used to evaluate the contribution of theVSRM to contractions initiated by voltage steps that recruit bothCICR and the VSRM. Inhibition of the VSRM with tetracaine reducesthe magnitude of contraction by ~50% at voltages that would maximallyactivate both CICR and the VSRM (Fig. 6). At more positive potentials,corresponding to the overshoot and plateau of the action potential,the fraction of contraction inhibited by tetracaine is even larger.Thus the component of the contraction-voltage relationship inhibitedby tetracaine appears to be identical to that removed by voltageinactivation of the VSRM (Fig. 4). These observations indicatethat the VSRM contributes substantially to EC coupling, even inthe presence of CICR.

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Fig. 6. Selective block of the VSRM with tetracaine demonstrates the contribution of the VSRM to the contraction-voltage relationship. Tetracaine was applied rapidly, 3 s in advance of test steps to avoid effects on sarcoplasmic reticulum (SR) Ca²⁺ content. Na currents were blocked with lidocaine throughout the experiments. A: contraction-voltage relationships before and after application of tetracaine. In the presence of tetracaine, the contraction-voltage relationship became bell shaped and proportional to inward Ca²⁺ current (B). In addition, tetracaine reduced the maximum peak contraction and shifted the activation curve in the positive direction. * Significantly different from control (P < 0.05). B: current-voltage (I-V) relationships in the absence and presence of tetracaine. Tetracaine had little effect on the I-V relationship. [From Mason and Ferrier (47)]

Contractions and transients can be initiated by the VSRM when I_Ca-L is blocked. This suggests that the Ca²⁺ transient likely originates entirely from release of intracellularstores of Ca²⁺. Release of SR Ca²⁺ through ryanodine receptors can be assessed with ryanodine. Atlow concentrations (micromolar), ryanodine is believed to renderthe SR leaky, thereby depleting SR Ca²⁺ stores (50, 64, 73). However, experiments with ryanodinedemonstrated that unexpectedly low concentrations of ryanodine(30 nM) blocked the VSRM (18). Furthermore, block of the VSRMoccurred at concentrations that did not deplete the SR of Ca²⁺ and that had little or no effect on contractions initiated byCICR coupled to I_Ca-L (48). These observations confirmed thatryanodine receptors are essential for the operation of the VSRMand also indicated that a high affinity binding site for ryanodinemay be associated with this mechanism. Selective blockade of theVSRM by very low concentrations of ryanodine also raises an intriguingpossibility that the VSRM and CICR utilize separate populationsof ryanodinereceptors.

The preceding discussion focuses on characteristics of phasic VSRM contractions and transients. Sustained transients and contractionsinitiated by the VSRM show the same pharmacology as phasic VSRMcontractions and are inhibited by tetracaine and ryanodine, butnot by Cd²⁺, Ni²⁺, tetrodotoxin, or lidocaine (Figs. 3 and 7) (20). These electrophysiologicaland pharmacological properties add further evidence that the VSRMand CICR are different and distinct mechanisms for EC coupling.

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Fig. 7. Sustained component of the VSRM shows the same pharmacological properties as the phasic component of the VSRM. A: effects of ryanodine (1 µM) on contractions elicited by sequential steps to $-$ 40 and 0 mV (voltage-clamp protocol at left). Ryanodine abolished both the phasic and sustained contractions elicited by the VSRM but had much less effect on the CICR contraction. B: sustained component of the VSRM is not inhibited by 2 mM Ni²⁺. Inset: voltage-clamp protocol. [Adapted from Ferrier et al. (20)]

	REGULATION OF VSRM BY PHOSPHORYLATION

TOP ABSTRACT INTRODUCTION CA²⁺-INDUCED CA²⁺ RELEASE VOLTAGE-SENSITIVE RELEASE... REGULATION OF VSRM BY... CONDITIONS REQUIRED FOR... MECHANISM OF EC COUPLING... ROLE OF VSRM IN... SUMMARY REFERENCES

Phosphorylation pathways play a major role in regulation of the strength of cardiac contraction. The VSRM is a target forphosphorylation by at least two major routes: the adenylyl cyclase-proteinkinase A (AC/PKA) pathway and the Ca²⁺-calmodulin-dependent kinase (CaM kinase) pathway. Therefore,phosphorylation of the VSRM may play a role in regulation of cardiacstrength.

The importance of phosphorylation in activation of the VSRM first was recognized in experiments with patch pipettes (22,96). The VSRM is readily demonstrable when cells are studiedwith high-resistance microelectrodes, which minimize intracellulardialysis with electrode solution. However, when cells were dialyzedwith conventional intracellular patch pipette solutions, the VSRMwas not observed (22, 27, 96). Under these conditions, contraction-voltagerelations were bell shaped as expected for CICR, even when activationsteps were made from near the resting membrane potential to ensurethat the VSRM was not inactivated. Subsequent experiments demonstratedthat addition of either 8-bromo-cAMP or calmodulin (Fig. 8) tothe pipette solution restored activation of the VSRM (22, 27,96).

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Fig. 8. Calmodulin (CaM) restores activation of the VSRM in experiments with patch pipettes. A: voltage-clamp protocol. B: only the CICR contraction was demonstrable in cells dialyzed with standard potassium-based patch pipette solution. C: addition of CaM to the patch pipette solution allowed activation of the VSRM in addition to CICR. D: effect of CaM was prevented by KN-62, a specific inhibitor of CaM kinase. [From Zhu and Ferrier (96)]

The component of EC coupling activated by these agents was identified as the VSRM by its electrophysiological and pharmacologicalproperties. Responses that appeared in the presence of calmodulinor 8-bromo-cAMP exhibited half-inactivation voltages typical ofthe VSRM (approximately $-$ 50 mV) were resistant to blockade ofI_Ca-L by Cd²⁺ and were inhibited by tetracaine (22, 96). Furthermore, thepresence of either 8-bromo-cAMP or calmodulin in the intracellularsolution resulted in sigmoidal contraction-voltage (Fig. 9) orCa²⁺ transient-voltage relations (22, 96). Activation of the VSRMby either agent also increased the maximum amplitude of contractionsor Ca²⁺ transients at membrane potentials corresponding to the overshootand plateau of the action potential. Thus the component of ECcoupling supported by 8-bromo-cAMP or calmodulin had characteristicsidentical to the VSRM in myocytes studied with high-resistancemicroelectrodes.

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Fig. 9. Addition of 8-bromo-cAMP (8-Br-cAMP) to patch pipette solutions dramatically enhances the contribution of the VSRM to contraction but causes only modest stimulation of CICR contractions. A: contraction-voltage relationships determined when the VSRM was available for activation (postconditioning potential $-$ 65 mV). In the absence of 8-Br-cAMP, the contraction-voltage relationship was bell shaped. Inclusion of 8-Br-cAMP in the pipette solution resulted in a contraction-voltage relationship characteristic of the VSMR. 8-Br-cAMP caused the contraction-voltage relationship to become sigmoidal, markedly increased the amplitudes of contractions, and shifted activation negatively. B: inclusion of 8-Br-cAMP in the pipette increased I_Ca-L primarily near the peak of the I-V relationship. C: relationship between contraction and current determined from a postconditioning potential of $-$ 65 mV in the absence of 8-Br-cAMP was similar to those in F. However, addition of 8-Br-cAMP eliminated the proportionality between contraction and current. D: effects of 8-Br-cAMP on contraction-voltage relations elicited when the VSRM was inactivated (postconditioning potential $-$ 40 mV). Contraction-voltage relations were bell shaped and increased modestly when 8-Br-cAMP was included in the pipette. E: I-V relations corresponding to experiments illustrated in D. F: plot of contraction amplitudes as a function of corresponding currents. The relationship between contraction and current was not changed by addition of 8-Br-cAMP to the pipette solution. Thus CICR contractions remained proportional to magnitude of current and there was no evidence for a significant change in gain. [Adapted from Ferrier et al. (22)]

The observation that dialysis of myocytes with patch pipettes inhibits the VSRM unless 8-bromo-cAMP or calmodulin are addedto the intracellular solution suggests that dialysis can disruptphosphorylation pathways essential for activation of the VSRM.Evidence supporting this interpretation comes from experimentswith specific kinase inhibitors (e.g., Fig. 8D). When the VSRMis supported by calmodulin, the CaM kinase inhibitor KN-62 abolishesVSRM responses; however, the PKA inhibitor H-89 is without effect(96). In contrast, when the VSRM is supported by addition of8-bromo-cAMP to the patch pipette solution, H-89 inhibits theresponses (22), whereas KN-62 is without effect (96). Theseobservations suggest that calmodulin and 8-bromo-cAMP restoreactivation of the VSRM by activation of the CaM kinase and PKApathways, respectively. Evidence that these pathways normallyregulate activation of the VSRM comes from experiments with nondialyzedcells studied with high-resistance microelectrodes (96). Inthese experiments, inhibition of either PKA or CaM kinase individuallyresulted in about 50% inhibition of the VSRM. Simultaneous superfusionof the myocytes with both H-89 and KN-62 virtually abolished theVSRM. These observations indicate that these phosphorylation pathwaysplay a critical role in regulation of the VSRM in cardiacmuscle.

Although 8-bromo-cAMP and calmodulin both activated the VSRM, they had very different effects on maximum inward I_Ca-L. Theeffects of 8-bromo-cAMP were accompanied by an increase in maximumpeak inward I_Ca-L (22). In contrast, calmodulin increased VSRMcontractions and transients without increasing the magnitude ofI_Ca-L or contractions initiated by CICR (96). In either case,block of I_Ca-L eliminated CICR contractions but had virtuallyno effect on the amplitude of contractions activated by the VSRM.Thus activation of the VSRM by these agents was independent ofeffects on I_Ca-L.

In the absence of 8-bromo-cAMP, when the conditioning potential was $-$ 65 mV to allow activation of the VSRM, both the I-V relationshipfor I_Ca-L and the contraction-voltage relationship were bell shaped(Fig. 9, A and B). When contraction amplitude is plotted as afunction of magnitude of I_Ca-L, it is clear that contraction isproportional to the magnitude of I_Ca-L (Fig. 9C). However, additionof 8-bromo-cAMP to the patch pipette solution caused an increasein the amplitude of contraction, and the contraction-voltage relationshipbecame sigmoidal (Fig. 9A). In contrast, the I-V relationshipfor I_Ca-L remained bell shaped, although the amplitude of currentwas increased by 8-bromo-cAMP (Fig. 9B). If one plots the amplitudeof contraction as a function of magnitude of I_Ca-L, it is apparentthat amplitude of contraction is unrelated to magnitude of I_Ca-Lin the presence of 8-bromo-cAMP when the VSRM is available (Fig.9C).

When the VSRM was inactivated by a conditioning potential of $-$ 40 mV, a different picture emerged. Although addition of 8-bromo-cAMPto patch pipette solutions increased the amplitude of I_Ca-L andCICR contractions, CICR contractions remained proportional tothe magnitude of current and still exhibited bell-shaped contraction-voltagerelationships (Fig. 9, D and E). The increase in CICR contractionsappeared to be related directly to the increased magnitude ofI_Ca-L, because the relationship between the amplitudes of contractionand current (gain) was unchanged by 8-bromo-cAMP (Fig. 9F) (22).Thus activation of the VSRM by 8-bromo-cAMP occurred without disruptionof the graded relationship between CICR contractions and I_Ca-Lin the same cells. Therefore, activation of the VSRM in responseto inclusion of 8-bromo-cAMP in the intracellular solution cannotbe explained by a marked increase in gain of CICR resulting ina "hair-trigger" for contraction (91).

Experiments that demonstrated that cAMP could restore VSRM contractions and Ca²⁺ transients in dialyzed myocytes utilized 8-bromo-cAMP. This analogof cAMP is resistant to hydrolysis by phosphodiesterases (51).A recent study concluded that there was no evidence for the VSRMin myocytes dialyzed with pipette solutions containing Tris-cAMP(60). Tris-cAMP is readily hydrolyzable by phosphodiesterases(51). We hypothesized that Tris-cAMP was ineffective in activatingthe VSRM because it would be rapidly broken down by phosphodiesterases.In experiments to examine whether different analogs of cAMP wouldsupport the VSRM, we found that two phosphodiesterase-resistantanalogs, 8-bromo- and dibutyryl-cAMP, activated the VSRM (21).However, unsubstituted cAMP (Tris- or Na-salt), which is hydrolyzableby phosphodiesterase, was ineffective in activating the VSRM (21).To confirm the role of phosphodiesterase in these observations,the effect of 3-isobutyl-1-methylxanthine (IBMX), a nonspecificphosphodiesterase inhibitor was examined (21). In myocytes dialyzedwith standard intracellular solutions not containing either cAMPor calmodulin, IBMX allowed activation of the VSRM (21). Therefore,it would appear that phosphodiesterase plays an important rolein regulating activation of theVSRM.

	CONDITIONS REQUIRED FOR ACTIVATION OF VSRM

TOP ABSTRACT INTRODUCTION CA²⁺-INDUCED CA²⁺ RELEASE VOLTAGE-SENSITIVE RELEASE... REGULATION OF VSRM BY... CONDITIONS REQUIRED FOR... MECHANISM OF EC COUPLING... ROLE OF VSRM IN... SUMMARY REFERENCES

The VSRM is demonstrable in cells from different species, including guinea pigs, rats, hamsters, rabbits, and humans (18,25, 27, 30, 31, 87). Furthermore, the characteristicsof the VSRM are essentially identical in these studies, despitethe use of different myocyte isolation procedures in differentlaboratories (18, 25, 27, 30, 31, 87). Early studiesin multicellular preparations at body temperature also reportedinitiation of contraction at membrane potentials negative to thoseat which significant I_Ca-L is activated (e.g., 2, 23; and reviewedin 29, 36). Contractions initiated in these studies may have includedactivation of the VSRM; however, the mechanism of these contractionswas not clearly identified. Subsequent to these studies in multicellularpreparations, isolated myocytes became available for experimentation.However, evidence for the VSRM was not observed in these earlystudies in isolated myocytes. The properties of the VSRM describedin this review likely explain why this mechanism was not detectedin older studies in myocytes. In the past, EC coupling studiestypically were conducted at room temperature with patch pipettesand with protocols in which holding or conditioning potentialsnear $-$ 40 mV were utilized (29). Clearly experiments conductedwith patch pipettes, in the absence of calmodulin or a nonhydrolyzableanalog of cAMP, would not have activated this mechanism. The VSRMalso is inhibited in experiments conducted at room temperature(19, 29). Similarly, the VSRM would be inactivated in experimentsthat utilized holding or conditioning potentials near $-$ 40 mV,because of the steady-state inactivation properties of phasicVSRM contractions. In addition, the VSRM is much more sensitiveto conditioning pulses (amplitude and frequency) than CICR (31,62, 95). Thus it has become clear from recent studies that,to study the VSRM, one must avoid inactivation with depolarizedconditioning potentials, use physiological temperature (37°C),provide a substrate for phosphorylation when experiments are conductedwith patch pipettes, and precede test steps with conditioningpulses of sufficient amplitudes and durations to activate theVSRM. The use of high-resistance electrodes minimizes cell dialysiswith electrode solution and eliminates the need for exogenouscAMP or calmodulin required with patchpipettes.

Most early studies in isolated myocytes were conducted under conditions that would not allow activation of the VSRM. Therefore,early studies with isolated myocytes only investigated CICR andconcluded that this was the only mechanism for cardiac EC coupling.Because of this, the existence of the VSRM is controversial. Itis extremely important that attempts to verify the existence ofthe VSRM are conducted under conditions that have been demonstratedto allow its activation. A recent study by Piacentino et al. (60)concluded that the VSRM could be explained by CICR in feline ventricularmyocytes. However, there is no evidence in this study that themechanism which we have identified as the VSRM was ever activated.Piacentino et al. (60) conducted their study two ways. In onecase, cells were dialyzed with patch pipettes containing Tris-cAMP,which is a hydrolyzable analog of cAMP. Ferrier et al. (21)demonstrate that hydrolyzable analogs will not activate the VSRM.Thus the VSRM would not have been activated under these conditions.In other experiments, Piacentino et al. (60) voltage-clampedmyocytes with patch pipettes that did not contain cAMP. Extracellularapplication of 50 nM isoproterenol was used in an attempt to activatethe VSRM. However, the contraction-voltage relations remainedbell shaped and were very sensitive to Cd²⁺, as expected for CICR. Thus it is doubtful that the VSRM wasactivated under the experimental conditions employed by Piacentinoet al. (60). Because there was no evidence that the VSRM wasactivated in this study, it is not clear how one can concludethat the VSRM can be explained byCICR.

	MECHANISM OF EC COUPLING FOR VSRM

TOP ABSTRACT INTRODUCTION CA²⁺-INDUCED CA²⁺ RELEASE VOLTAGE-SENSITIVE RELEASE... REGULATION OF VSRM BY... CONDITIONS REQUIRED FOR... MECHANISM OF EC COUPLING... ROLE OF VSRM IN... SUMMARY REFERENCES

The mechanism by which the VSRM is coupled to membrane potential is not clear. Although VSRM contractions are not proportionalto I_Ca-L, activation of the VSRM requires extracellular Ca²⁺ (18). However, the VSRM can be activated in the presence ofas little as 50 µM extracellular Ca²⁺ (18). Thus it is not known whether Ca²⁺ entry is required for activation of the VSRM, or alternatively,whether Ca²⁺ is necessary at some extracellular binding site. If Ca²⁺ influx is required to trigger the VSRM, this mechanism must bedifferent from, and coexist with, conventional CICR. The influxmust be extremely small, and there can be little, if any, proportionalitybetween the magnitude of Ca²⁺ entry and the magnitude of contractions or Ca²⁺ transients. If this Ca²⁺ entry occurs through voltage-gated channel openings, it cannotbe the same as or as large as that entering through L-channels,because summation of L-channel openings gives rise to whole cellI_Ca-L. This is precluded because the VSRM is independent of themagnitude of I_Ca-L and persists when the I_Ca-L is blocked by Cd²⁺. Furthermore, this conductance must be inactivated with a conditioningpotential of $-$ 40 mV, despite the fact that I_Ca-L and CICR persistfrom this potential. This hypothetical explanation for the VSRMwould require the operation of two mechanisms for CICR in thesame cell at the same time: one with ultra-high gain for the VSRM,and one with low gain for conventional CICR graded by I_Ca-L. Topostulate that CICR can activate the VSRM, it will be necessaryto address these paradoxesexperimentally.

The sustained component of the VSRM also is difficult to explain by conventional CICR. Phasic CICR contractions terminatewith a characteristic time course, even when inactivation of I_Ca-Lis slowed greatly by a Ca²⁺ channel agonist (72). This observation has led to the hypothesisthat ryanodine receptors enter a refractory or inactivated state,during which CICR is no longer possible. This property of CICRis not compatible with the occurrence of sustained Ca²⁺ release observed with the VSRM. This problem also would needto be resolved to explain the VSRM in terms ofCICR.

Alternatively, Ca²⁺ influx may not be required for activation of the VSRM. In this case, one must propose that the VSRM is coupledto changes in membrane potential through some voltage-dependentevent separate from Ca²⁺ permeation. This might be gating charge movement of a channelmoiety, as in skeletal muscle (33), or it could be a biochemicallink such as release of a second messenger or activation of aphosphorylation step (61, 92). It is not clear whether onewould expect a biochemical link to show a voltage dependence,which is described by a Boltzmann function, like that of the VSRM.However, charge movement in voltage-gated ion channels, includingthe voltage sensor for EC coupling in skeletal muscle, does followa Boltzmann distribution and would be compatible with the voltagedependence of theVSRM.

Ca²⁺ transients initiated by the VSRM resemble those observed in skeletal muscle (63, 74). Skeletal muscle transients arecharacterized by an initial rapid phase, which exhibits inactivation,followed by a sustained component, which does not inactivate (Fig.10) (68, 74). The configuration of these transients is similarto that of transients observed in cardiac myocytes when the VSRMis available (Fig. 5A). The configurations of the Ca²⁺ transients in skeletal muscle are believed to reflect changesin efflux of Ca²⁺ from the SR (Fig. 10). The sustained component of skeletal muscleresponses is believed to reflect opening of ryanodine receptorsby a voltage sensor. The initial phasic component occurs in responseto recruitment of adjacent ryanodine receptors through intracellularCICR (63). Thus CICR provides a multiplier or amplificationsystem for the voltage sensor component and causes a phasic Ca²⁺ release that terminates with a time course that is independentof the sustained component (63, 68). One may speculate thatsimilar mechanisms may account for phasic and sustained componentsof the VSRM observed in cardiac myocytes. Clearly additional studieswill be required to test this possibility.

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Fig. 10. Phasic and sustained components of Ca²⁺ release in frog and rat skeletal muscles resembles that observed in cardiac myocytes. Ca²⁺ was detected with antipyrylazo III. A: representative recordings of Ca²⁺ transients in frog semitendinosus (left) and rat extensor digitorum longus muscles (right). Transients were initiated by voltage steps from the holding potential to different more positive potentials as indicated in the figure. The transients show a phasic component followed by a sustained component, which terminates promptly with repolarization. B: release flux calculated from the time derivative of the Ca²⁺ transients in frog (left) and rat (right) muscles. The removal flux was determined from fits to a removal model; (see Ref. 74 for details). Ca²⁺ flux in both species demonstrated an initial phasic rise followed by a decrease to a constant lower flux. [Reproduced from The Journal of General Physiology, 1996, vol. 107, pp. 1-18 by copyright permission of The Rockefeller University Press (74)]

	ROLE OF VSRM IN HEART DISEASE

TOP ABSTRACT INTRODUCTION CA²⁺-INDUCED CA²⁺ RELEASE VOLTAGE-SENSITIVE RELEASE... REGULATION OF VSRM BY... CONDITIONS REQUIRED FOR... MECHANISM OF EC COUPLING... ROLE OF VSRM IN... SUMMARY REFERENCES

The VSRM contributes substantially to contraction in myocytes from normal hearts. However, the VSRM appears to be attenuatedin myocytes from two different animal models of congestive heartfailure: cardiomyopathic hamsters and rats with heart failuresecondary to myocardial infarction. The VSRM contributes substantiallyto contractile function in myocytes from normal hamsters, muchas observed in other species (30). In contrast, contractionsinitiated by the VSRM are depressed selectively in myocytes fromhamsters with a cardiomyopathic genotype, with virtually no changein contractions triggered by CICR (Fig. 11) (30). In rats withheart failure secondary to coronary ligation, the VSRM also isdepressed significantly with virtually no change in CICR (80).These studies demonstrate that defects in the VSRM are largelyresponsible for the decrease in contractile function observedin these two animal models of heart failure. Thus the relativecontributions of the VSRM and CICR to EC coupling may be alteredin heart diseases characterized by contractile dysfunction.

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Fig. 11. Contractile dysfunction in ventricular myocytes from cardiomyopathic hamsters is caused by selective depression of the VSRM. A: contraction-voltage relationships recorded from normal and cardiomyopathic myocytes when the VSRM was inactivated (postconditioning potential $-$ 40 mV) were virtually identical. B: I-V relationships determined from $-$ 40 mV also were identical in normal and cardiomyopathic cells. C: contraction-voltage relationships recorded when the VSRM was not inactivated (postconditioning potential $-$ 60 mV). The contraction-voltage relationship from cardiomyopathic hamsters was significantly depressed relative to the corresponding curve for normal hamsters. * Significantly different from normal (P < 0.05). D: I-V relationships recorded from $-$ 60 mV were identical in the two groups. [Adapted from Howlett et al. (30)]

The role of the sustained component of the VSRM in heart disease has not been investigated. Because the sustained componentis reversibly graded by voltage, it may alter function in conditionswhere membrane potential is abnormal. For example, the sustainedcomponent of the VSRM might delay relaxation in conditions wherethe action potential is significantly prolonged, such as cardiachypertrophy or heart failure (90). In addition, the sustainedcomponent might prevent full relaxation in disease conditions,which result in incompleterepolarization.

	SUMMARY

TOP ABSTRACT INTRODUCTION CA²⁺-INDUCED CA²⁺ RELEASE VOLTAGE-SENSITIVE RELEASE... REGULATION OF VSRM BY... CONDITIONS REQUIRED FOR... MECHANISM OF EC COUPLING... ROLE OF VSRM IN... SUMMARY REFERENCES

There is increasing evidence that the VSRM and CICR represent two different mechanisms for EC coupling in the heart. We illustratethis possibility in Fig. 12. Both mechanisms likely contributeto initiation of cardiac contraction. These two mechanisms havedistinct electrophysiological and pharmacological characteristicsthat allow them to be distinguished from each other in the samecell. Because of the mutually exclusive nature of many of thesecharacteristics, the VSRM and CICR cannot be explained by a singlemechanism. Thus we indicate the VSRM and CICR as two independentmechanisms for release of SR Ca²⁺ (Fig. 12). However, it is unclear whether the VSRM operates aseparate population of ryanodine receptors or opens the same populationof release channels as CICR. The functional characteristics ofthe VSRM resemble characteristics associated with Ca²⁺ release coupled to gating charge in skeletal muscle. Therefore,we have indicated a physical link between a channel moiety, functioningas a voltage sensor in the sarcolemma, and the Ca²⁺ release channel in the SR (Fig. 12). However, the molecular identityof the VSRM is not yet known and other mechanisms must be considered.Phosphorylation plays a major role in activation of the VSRM andmay allow the VSRM to serve as a major regulatory mechanism forcardiac contraction in normal heart. As suggested in Fig. 12, phosphorylationsites for PKA and CaM kinase may be located on one or more componentsof the VSRM. At present it would be speculative to suggest whatsites would regulate the VSRM. If the VSRM and CICR are separateparallel mechanisms, this allows for separate alterations of eithermechanism in disease states. Indeed, the VSRM plays a major rolein contractile dysfunction in several models of heart failureand may contribute to impaired contractile performance in heartdisease. As our information about the VSRM accumulates, it isbecoming clear that this important trigger for cardiac contractionplays a central role in regulation of cardiac contraction in normaland diseased myocardium.

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Fig. 12. Schematic illustrating a possible relationship between the VSRM and CICR in cardiac myocytes. The VSRM and CICR are depicted as independent mechanisms, which operate to release Ca²⁺ from a common Ca²⁺ store within the SR. CICR is shown with Ca²⁺ influx occurring through an L-type Ca²⁺ channel. Incoming Ca²⁺ binds to an activation site on Ca²⁺ release channels, which causes these channels to open and release Ca²⁺. The VSRM is shown as a voltage sensor, based on a channel moiety, which signals Ca²⁺ release channels to open through a physical link. AC, adenylyl cyclase, which is coupled to various receptors (R) through a stimulatory G protein (G_s). Some possible regulatory phosphorylation sites for protein kinase A (PKA) and CaM kinse (CamK) are indicated on proteins involved in SR Ca²⁺ release. See text for discussion.

	ACKNOWLEDGEMENTS

We thank Peter Nicholl and Dr. Jiequan Zhu for assistance in preparation ofillustrations.

	FOOTNOTES

This work was supported in part by grants from the Heart and Stroke Foundation of Nova Scotia and from The Canadian Institutesfor HealthResearch.

Address for reprint requests and other correspondence: G. R. Ferrier and S. E. Howlett, Dept. of Pharmacology, Sir CharlesTupper Medical Bldg., Dalhousie Univ., Halifax, Nova Scotia, CanadaB3H 4H7 (E-mail: Gregory.Ferrier{at}dal.ca and Susan.Howlett{at}dal.ca).

REFERENCES

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ABSTRACT
INTRODUCTION
CA²⁺-INDUCED CA²⁺ RELEASE
VOLTAGE-SENSITIVE RELEASE...
REGULATION OF VSRM BY...
CONDITIONS REQUIRED FOR...
MECHANISM OF EC COUPLING...
ROLE OF VSRM IN...
SUMMARY
REFERENCES

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19. Ferrier, GR, and Redondo IM. Low temperature inhibits cardiac contractions initiated by the voltage-sensitive release mechanism (Abstract). J Mol Cell Cardiol 28: A180, 1996.

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				J. M. Cordeiro, L. Greene, C. Heilmann, D. Antzelevitch, and C. Antzelevitch Transmural heterogeneity of calcium activity and mechanical function in the canine left ventricle Am J Physiol Heart Circ Physiol, April 1, 2004; 286(4): H1471 - H1479. [Abstract] [Full Text] [PDF]

				F. Brette, J.-Y. Le Guennec, and I. Findlay Low-voltage triggering of Ca2+ release from the sarcoplasmic reticulum in cardiac muscle cells Am J Physiol Cell Physiol, December 1, 2003; 285(6): C1544 - C1552. [Abstract] [Full Text] [PDF]

				H. Griffiths and K.T. MacLeod The Voltage-sensitive Release Mechanism of Excitation Contraction Coupling in Rabbit Cardiac Muscle Is Explained by Calcium-induced Calcium Release J. Gen. Physiol., April 28, 2003; 121(5): 353 - 373. [Abstract] [Full Text] [PDF]

				W. E. Louch, G. R. Ferrier, and S. E. Howlett Changes in excitation-contraction coupling in an isolated ventricular myocyte model of cardiac stunning Am J Physiol Heart Circ Physiol, August 1, 2002; 283(2): H800 - H810. [Abstract] [Full Text] [PDF]

				W. Xiong, H. M. Moore, S. E. Howlett, and G. R. Ferrier In Contrast to Forskolin and 3-Isobutyl-1-methylxanthine, Amrinone Stimulates the Cardiac Voltage-Sensitive Release Mechanism without Increasing Calcium-Induced Calcium Release J. Pharmacol. Exp. Ther., September 1, 2001; 298(3): 954 - 963. [Abstract] [Full Text]

				V. Piacentino III, J. P. Gaughan, and S. R. Houser L-Type Ca2+ Currents Overlapping Threshold Na+ Currents: Could They Be Responsible for the "Slip-Mode" Phenomenon in Cardiac Myocytes? Circ. Res., March 8, 2002; 90(4): 435 - 442. [Abstract] [Full Text] [PDF]

INVITED REVIEW Cardiac excitation-contraction coupling: role of membrane potential in regulation of contraction

INVITED REVIEW
Cardiac excitation-contraction coupling: role of membrane potential in regulation of contraction