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Department of Molecular Biosciences, University of California, Davis, California (G.C., W.F., E.C., I.N.P.); School of Nursing, University of Maryland, Baltimore, Maryland (C.W.W., L.M.); and Department of Anesthesiology and Perioperative and Pain Medicine, Brigham and Women's Hospital, Boston, Massachusetts (J.R.L., M.S., P.D.A.)
Received November 7, 2007; accepted December 31, 2007
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Abstract |
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 Top Abstract Materials and MethodsResults and DiscussionReferences |
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; Krause et al., 2004) and animals (Nelson, 1991; Klont et al., 1994; Bjurström and Jönsson, 1995; Roberts et al., 2001). MH is associated with acute increase in intracellular Ca2+ (Reulbach et al., 2007) resulting from exposure to volatile anesthetics and/or depolarizing muscle blockers (Ali et al., 2003; Gronert et al., 2004; Krause et al., 2004). Heat stress has also been clearly shown to trigger fulminant MH in susceptible mice (Chelu et al., 2006; Yang et al., 2006), although its etiological role in human MH and MH in other species is debated (Robinson et al., 2003). Dantrolene is also clinically useful for the treatment of spasticity or muscle spasms associated with several clinical conditions, including spinal cord injuries, stroke, multiple sclerosis, and cerebral palsy (Chou et al., 2004; Dressler and Benecke, 2005; Saulino and Jacobs, 2006; Verrotti et al., 2006). Dantrolene has been used successfully to mitigate symptoms arising from neuroleptic malignant syndrome (Lappa et al., 2002; Strawn et al., 2007), but meta-analysis of 271 case reports has indicated an over-all higher mortality rate when dantrolene monotherapy is used to treat neuroleptic malignant syndrome (Reulbach et al., 2007). The muscle relaxant properties of dantrolene have been closely correlated with its ability to both reduce basal resting free Ca2+ (López et al., 1987) and evoked increases in Ca2+ in the myoplasm, although the exact mechanisms by which dantrolene interrupts the MH episode and promotes skeletal muscle relaxation are complex (Krause et al., 2004).
Although dantrolene shows selectivity as a skeletal muscle relaxant, with little or no effect on smooth or cardiac muscle, it has relatively low apparent potency. In humans, blood concentrations of 2.8 to 4.2 mg/l (
9-13 µM) are needed to depress the response of a single muscle twitch by 70 to 75% (Flewellen et al., 1983). Recent simulations of dantrolene's pharmacokinetic profile indicate that the European recommendations for treating MH result in 24-h plasma concentrations of 14 to 18 mg/l (45-57 µM), whereas Malignant Hyperthermia Association of the United States guidelines result in plasma concentrations ranging from 7 to 23 mg/l (22.5-73 µM) (Podranski et al., 2005).
The plasma concentrations of dantrolene needed to successfully treat clinical MH (Podranski et al., 2005) and those required to attenuate contractile force (1-10 µM) (Krause et al., 2004) suggest that this drug may influence multiple homeostatic mechanisms that affect not only Ca2+ release from sarcoplasmic reticulum (SR) but also Ca2+ entry into the muscle cell. Whether all the effects of dantrolene on attenuating myoplasmic Ca2+ are mediated through a common pathway is not clear. The prevailing data support a view that ryanodine receptor type 1 (RyR1) is a direct and selective molecular target of dantrolene's muscle-relaxant action. RyR1 is the calcium-release channel of sarcoplasmic reticulum that is essential for normal excitation-contraction (EC) coupling in skeletal muscle. [3H]Dantrolene was shown to bind with high affinity (KD = 277 nM) to SR membrane preparations enriched in RyR1, and its binding site seems distinct from the site that recognizes the alkaloid ryanodine (Parness and Palnitkar, 1995; Palnitkar et al., 1997). Results from affinity-labeling studies with [3H]azido-dantrolene (Palnitkar et al., 1999; Paul-Pletzer et al., 2001) and site-directed antibodies (Paul-Pletzer et al., 2002) identified a potential dantrolene binding site in the N-terminal region bounded by AAs 590 to 609. This region of RyR1 was used previously as a peptide to activate RyR1 and was defined by the authors as domain peptide 1 (DP1) (El-Hayek et al., 1999). One mechanism proposed for dantrolene's inhibitory activity is through the stabilization of the interactions of two RyR1 domains, AAs 590 to 609 and AAs 2442 to 2477. The second domain had also been used as a peptide to activate RyR1 and had been defined as DP4 (Yamamoto et al., 2000). Dantrolene has been shown to inhibit the ability of DP4 to enhance the binding of [3H]ryanodine to SR membranes containing RyR1 (Kobayashi et al., 2005). It has been proposed that dantrolene stabilizes DP1-DP4 interactions in a manner that prevents the "unzipping" of these domains, a process that has been theorized to be necessary for transitioning from the closed to the open channel state, thereby stabilizing the closed state of RyR1 channels (Yamamoto et al., 2000; Yamamoto and Ikemoto, 2002a,b; Kobayashi et al., 2005). MH mutations within DP1 or DP4 had been suggested to act by destabilizing the closed channel state and contribute to MH susceptibility (Murayama et al., 2007). However, no direct evidence has been presented to confirm either of these theories.
Attempts to demonstrate that the mechanism of dantrolene's action in both normal and MH muscle are solely the result of a direct and selective inhibition of RyR1 channels remains controversial. Fruen and coworkers (1997) demonstrated that dantrolene can inhibit both SR Ca2+ release and [3H]ryanodine binding to SR vesicles isolated from both normal and MH swine skeletal muscle under special experimental conditions that require the presence of AMP-PCP (a nonhydrolyzable ATP analog) and calmodulin in a buffer containing the organic anion proprionate to substitute for chloride (Fruen et al., 1997; Zhao et al., 2001). However, Szentesi and coworkers (2001) failed to inhibit the gating activity of RyR1 channels incorporated into bilayer lipid membranes (BLM) in the presence or absence of ATP (Szentesi et al., 2001). Dantrolene and its analog azumolene have been shown to reduce the resting myoplasmic free Ca2+ concentration ([Ca2+]rest) when it is administered to humans and animals in vivo when RyR1 channel activity is very low (López et al., 1985, 1987, 1990, 1992, 2000). In addition, azumolene has been shown to inhibit a specialized form of store-operated Ca2+ entry (SOCE) that is activated as a consequence of constraining an RyR1 open conformation produced by the presence of micromolar ryanodine and millimolar caffeine (Zhao et al., 2006). Whether these effects are the consequence of dantrolene modification of RyR1 conformation and Ca2+-channel gating was not demonstrated. Therefore, it seems that dantrolene may have more than one mechanism through which it can influence Ca2+ fluxes (Yang et al., 2003, 2007).
In the present study, we demonstrate for the first time that one of dantrolene's mechanisms of action is to block excitation-coupled calcium entry (ECCE) in both adult mouse flexor digitorum brevis (FDB) fibers and primary myotubes. Dantrolene's ability to block ECCE is independent of either its ability to inhibit RyR1 channel activity reconstituted in BLM or activate Ca2+ release triggered by EC coupling. The inhibitory potency of dantrolene on ECCE is consistent with the drug's clinical potency for reversing the MH syndrome, and is incomplete, as would be predicted by dantrolene's efficacy as a muscle relaxant. A second important new finding is that myotubes isolated from heterozygous and homozygous mice possessing MH missense mutation R163C-RyR1 show significantly enhanced ECCE rates that could be restored to those measured in wild-type (WT) cells after exposure to clinical concentrations of dantrolene. We propose that this gain of ECCE function is an important etiological component of MH susceptibility and possibly contributes to the MH episode. We identify inhibition of ECCE as a novel mechanism for dantrolene's clinical efficacy as a muscle relaxant.
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Materials and Methods |
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TopAbstractMaterials and MethodsResults and DiscussionReferences |
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) as described previously (Rando and Blau, 1997; Cherednichenko at al., 2004; Hurne et al., 2005). The myoblasts were expanded in 10-cm cell culture-treated Corning dishes coated with collagen (Calbiochem, Richmond, CA) and were plated onto 96-well µ-clear plates (Greiner Bio-One, Longwood, FL) coated with MATRIGEL (BD Biosciences, San Jose, CA) for Ca2+-imaging studies. Upon reaching 80% confluence, growth factors were withdrawn, and the cells were allowed to differentiate into myotubes over a period of 3 days.
Preparation of FDB Fibers. FDB muscles were dissected from adult mice (C57/B6), and single intact FDB myofibers were enzymatically isolated as described previously (Brown et al., 2007). After isolation, FDBs were plated on ECM (Sigma, St. Louis, MO)-coated glass-bottomed imaging dishes (Matek Corporation Ashland, MD) and maintained in Dulbecco's modified Eagle's medium (Invitrogen, Carlsbad, CA) supplemented with 0.2% bovine serum albumin and 100 mM gentamicin (Sigma). Fibers were kept overnight in a 5% CO2 incubator, and experiments were conducted within 12 to 24 h of plating. Dishes of myofibers were randomized to control treatment (0.1% dimethyl sulfoxide), ryanodine (Calbiochem) treatment (250 µM, 1 h), or ryanodine treatment followed by a 10-min application of dantrolene (10 µM).
Ca2+ and Mn2+ Imaging. Differentiated primary myotubes were loaded with 5 µM Fura-2-AM to measure the rate of dye quench by Mn2+ entry or Fluo-4-AM to measure Ca2+ transients (Invitrogen) at 37°C for 20 min in imaging buffer (125 mM NaCl, 5 mM KCl, 2 mM CaCl2, 1.2 mM MgSO4, 6 mM dextrose, and 25 mM HEPES, pH 7.4 supplemented with 0.05% bovine serum albumin). The cells were then washed three times with imaging buffer and transferred to the stage of a Nikon Diaphot inverted microscope (Nikon, Tokyo, Japan) and illuminated at the isosbestic wavelength for Fura-2 or 494 nm for Fluo-4 with a Delta Ram excitation source (Photon Technology International, Lawrenceville, NJ). Fluorescence emission at 510 nm was captured from regions of interest within each myotube from 3 to 10 individual cells at five frames per second using an Olympus 40x oil numerical aperture 1.3 objective, IC-300 intensified charge-coupled device camera and digitized and analyzed with ImageMaster software (Photon Technology International). When used, electrical field stimuli were applied using two platinum electrodes fixed to opposite sides of the well and connected to an A.M.P.I. Master 8 stimulator set at 3-V, 25-ms bipolar pulse duration over a range of frequencies (0.05-20 Hz; 40-s pulse train duration). Alternatively, higher-frequency stimuli were applied to the cells at 30 Hz for 1.5 s (7 V, 1-ms bipolar pulse duration) as described above, and Fluo-4 fluorescence emission from individual cells was measured at 100 Hz using photometry (Photon Technology International). In some experiments, KCl was focally applied for 2 s to depolarize the cells using Multivalve Perfusion System (Automate Scientific Inc., Oakland, CA). When K+ (40 mM) was applied, the concentration of Na+ was lowered accordingly to preserve osmolarity in the external medium.
Mn2+ influx into myotubes was measured as described previously or with minor modification (Clementi et al., 1992; Fessenden et al., 2000). A final concentration of 500 µM MnCl2 was added to a nominally Ca2+-free (7 µM free Ca2+) external solution to measure Mn2+ entry rates in response to depolarization. Independent experiments were performed with the external solution containing 300 µM Ca2+ to determine whether competition between Mn2+ and Ca2+ affected the rates of Mn2+ quench attributed to ECCE. Cells were stimulated by electrical field or with focal application of K+ or as described above.
Mn2+ influx into FDBs was performed using dishes of adhered FDBs loaded with Fura-2-AM (5 µM; 20 min) in normal mouse Ringer solution containing (146 mM NaCl, 4.7 mM KCl, 0.6 mM MgSO4, 1.6 mM Na2CO3, 0.13 mM NaH2PO4, 7.8 mM glucose, 20 mM HEPES, and 1.8 mM CaCl2). Fura-2 fluorescence was imaged on an inverted microscope (Olympus IX-50; 40x H2O objective, 1.15 numerical aperture; Olympus, Tokyo, Japan) equipped for fluorescence excitation (
DG-4) and coupled to a charge-coupled device-based imaging system (CoolSnap HQ charge-coupled device camera) all controlled by IP Lab 4.0 (BD Biosciences). During the study, the myofibers were excited at the isosbestic wavelength of Fura-2 (360 ± 7 nm) (Klein et al., 1988), and images of emission intensity (510 nm) were sampled for 50 ms at a rate of 1 Hz for 3 to 5 min. During the imaging period, the myofibers were continuously superfused (2 ml/min) first with normal mouse Ringer solution followed by perfusion with manganese-containing Ringer (Mn-R) solution in which Ca2+ (1.8 mM) was replaced with equimolar [Mn2+]). After a 1-min application of Mn-R, fibers were superfused with Mn-R solution containing 40 mM K+ (adjusted for ionic balance by lowering Na+ in the buffer).
The rate of and extent of changes in Ca2+ measured with Fluo-4 and the quench rate of Fura-2 fluorescence measured in both myotube and myofiber preparations were determined by linear least-squares regression (OriginLab 7.5; OriginLab Corp, Northampton, MA) and expressed as mean ± S.E.M. Statistical analysis was performed in SigmaStat (version 3.1; SPSS Inc., Chicago, IL) using one-way analysis of variance and Tukey's post hoc to establish significance (p < 0.05).
Preparation of SR Membranes and Purified RyR1. Junctional SR membranes enriched in RyR1 were prepared from skeletal muscle of New Zealand White rabbits and stored in 10% sucrose, 10 mM HEPES, pH 7.4, at -80°C until needed for solubilization in CHAPS detergent as described previously (Pessah et al., 1986). RyR1 was purified from the CHAPS-solubilized proteins by column chromatography through Sephacryl S-300 HR (GE Healthcare, Chalfont St. Giles, Buckinghamshire, UK), and the RyR1 peak was further purified on a 5 to 20% (w/v) linear sucrose gradient. The 30S fraction containing enriched RyR1 was then concentrated on a HiTrap Heparin HP column (GE Healthcare) (Samso et al., 2005). Purity of RyR1 was assessed by SDS-PAGE and silver stain. For preparation of the RyR1-FKBP12 complex, purified RyR1 was supplemented with an 8-fold molar excess of recombinant FKBP12 (Sigma-Aldrich, St. Louis, MO) immediately before channel reconstitution experiments.
Measurement and Analysis of Purified RyR1 Single-Channel Reconstituted in Planar Lipid Bilayer. Bilayers were composed of phosphatidylethanolamine/phosphatidylserine/phosphatidylcholine (5:3:2 w/w; Avanti Polar Lipids, Alabaster, AL) dissolved in decane at a final concentration of 30 mg/ml across a 200-µm aperture on a polysulfone cup (Warner Instruments, Hamden, CT). The bilayer partitioned two chambers (cis and trans) with buffer solution containing 500 mM CsCl, defined free Ca2+ (buffered by certain EGTA calculated according to the software Bound and Determined) and 20 HEPES-Tris, pH 7.4, on cis, 500 or 50 CsCl and 20 HEPES-Tris, pH 7.4, on trans. The addition of protein was made to the cis solution that was held at the virtual ground, whereas the trans solution was connected to the head stage input of an amplifier (Bilayer Clamp BC 525C; Warner Instruments). BLM-TC Planar Lipid Bilayer Thermocycler (Warner Instruments) was used to control the recording temperature throughout the experiment at a setting of either 25 or 35°C. After supplementation of purified RyR1 with a molar excess of FKPB12, single channels were reconstituted by introducing the FKBP12-RyR1 protein preparation in the cis chamber. Single-channel gating was monitored and recorded at a holding potential of -40 mV (applied to the trans side). The sidedness (cytosolic) of the channel was verified by the positive response to addition of micromolar Ca2+ once the channel was reconstituted. In addition, the response of most channels to 2 µM ryanodine or ruthenium red was tested at the end of the experiment. The amplified current signals, filtered at 1 kHz (Low-Pass Bessel Filter 8 Pole; Warner Instruments) were digitized and acquired at a sampling rate of 10 kHz (Digidata 1320A, Axon-Molecular Devices, Sunnyvale, CA). All of the recordings were made for at least 2 to 10 min under each defined experimental condition. The channel open probability (Po), mean open-, and mean closed-dwell times (
o and c) were obtained by using Clampfit, pClamp software 9.0 without further filtration (Axon-Molecular Devices).
Reagents. Dantrolene sodium, calmodulin, and FKBP12 were obtained from Sigma-Aldrich. Fura-2 AM and Fluo-4 AM were obtained from Invitrogen. Dantrolene was dissolved in dried dimethyl sulfoxide (high-performance liquid chromatography grade). All other reagents were of the highest purity commercially available.
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Results and Discussion |
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TopAbstractMaterials and MethodsResults and DiscussionReferences |
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; Paul-Pletzer et al., 2001, 2002). However, given dantrolene's relatively low (micromolar) potency for attenuating Ca2+ transient amplitude and contractility, its pharmacological activity could be the result of additional yet undiscovered mechanisms, and these were further investigated.
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To directly assess the possible inhibition of RyR1 activation by dantrolene, we therefore reconstituted purified RyR1/FKBP12 complexes in BLM and directly studied the effects of dantrolene on single-channel gating kinetics. Figure 2A shows the high molecular band of solubilized RyR1 protomer purified by column chromatography and visualized by SDS-PAGE and silver stain. Purified RyR1 was incubated with recombinant FKBP12 before reconstitution in BLM and recording of channel gating activity. The first trace of Fig. 2B shows the activity of a representative RyR1 channel in the presence of CaM (2 µM), ATP (2 mM), and Ca2+ (10 µM) on the cytoplasmic (cis) side at 25°C. The addition of 10 µM dantrolene to the cis chamber did not change gating parameters, including channel Po or open and closed dwell time constants (o and c, respectively) over a 10-min recording period (trace 2 shows gating parameters for >50 s of continuous recording). Dantrolene was then increased to 20 µM in the cis solution of the BLM chamber, at which time the addition of 10 µM dantrolene was made to the trans (lumenal) side, but the drug failed to affect changes in channel gating parameters over an additional 10 min of recording (Fig. 2B, third trace). RyR1 channel activity was also studied under conditions in which the BLM solutions were equilibrated at 35°C to test the possible temperature dependence of dantrolene inhibition of RyR1 (Fruen et al., 1997). The fourth and fifth traces in Fig. 2B showed that, under these conditions, the addition of CaM (1 µM) to the cis chamber rapidly enhanced channel Po as a result of prolonging o1 and shortening c (traces 4 and 5). Subsequent addition of 10 and 20 µM dantrolene to the cis chamber failed to diminish channel gating parameters over the 20 min of recording (traces 6 and 7), although the channel remained responsive to the addition of ryanodine and ruthenium red to the cis chamber (Fig. 2B, bottom traces).
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) who failed to identify detectable inhibition of ATP-activated RyR1 channels reconstituted in BLM. Zhang and coworkers (2005) reported that although dantrolene's structural analog azumolene depressed spark frequency in permeabilized frog skeletal muscle fibers, it did not significantly alter the properties of individual spark events. Compounds known to directly bind to RyR1 or affect channel activity through their influences on protein-protein interactions known to occur within the triadic complex have been shown to alter the intensity and spatial spread of individual sparks in addition to their frequency in a manner consistent with their influence on single RyR1 channel kinetics (González et al., 2000). Because we failed to demonstrate a direct action of dantrolene on the functioning FKBP12-RyR1-CaM channel complex, we therefore examined the possible influence of dantrolene on two different forms of Ca2+ entry, SOCE and ECCE, as possible mechanisms contributing to dantrolene's pharmacological activity as a muscle relaxant.
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Dantrolene Suppresses ECCE Elicited by Electrical Pulse Trains or KCl Depolarization. Because dantrolene failed to have a measurable effect on the gating activity of purified reconstituted FKBP12-RyR1-CaM channels or on SR depletion-activated SOCE, we next tested whether or not dantrolene may inhibit ECCE. Using the Mn2+ quench technique with Fura-2-loaded WT myotubes, the quench of Fura-2 fluorescence was measured before (Fig. 4 trace "Ctrl") and during electrical stimulation with 20-Hz electrical pulse trains lasting 40 s in a nominally Ca2+-free external buffer containing 500 µM Mn2+. Under these assay conditions, electrical stimulation of the cells resulted in rapid enhancement of the rate of Mn2+ quench of Fura-2 that we attribute to ECCE (Fig. 4A). If cells were preincubated with 10 µM dantrolene for 10 min before applying the electrical pulse train, the initial rate of Mn2+ quench was reduced by 72 ± 4% (p < 0.001).
Ryanodine has been shown previously to transiently activate and then persistently block RyR1 channel activity in a concentration- and time-dependent manner (Pessah and Zimányi, 1991). Pretreatment of RyR1 with ryanodine in intact myotubes has been shown to accentuate ECCE by slowing its inactivation/deactivation (Cherednichenko at al., 2004; Hurne et al., 2005). In the present study, we pretreated myotubes with 500 µM ryanodine for 30 min. Under these conditions, the cells failed to respond to 20 mM caffeine (data not shown), indicating that ryanodine blocked RyR1 activity. Nevertheless, stimulation of the same cells with a 20-Hz pulse train resulted in a large Ca2+ transient, which we attributed to the rapid entry of extracellular Ca2+ into the cells via ECCE (Fig. 5A). Dantrolene inhibited ECCE in ryanodine-pretreated myotubes in a dose-dependent manner with an IC50 value of 4.2 ± 1.9 µM but failed to completely inhibit ECCE, reaching a maximum inhibition of 69% of the control rate between 10 and 50 µM dantrolene (Fig. 5A, inset). Dantrolene also inhibited the rate of Mn2+ quench triggered by electrical pulse trains delivered to cells not pretreated with ryanodine in an external medium containing 500 µM Mn2+ and nominally free of Ca2+ with a dose-response characteristic similar to that of ryanodine-pretreated cells tested for ECCE (Fig. 5, B versus A, respectively).
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Enhanced ECCE in Myotubes Expressing R163C-RyR1 Is Restored by Dantrolene. To determine whether or not dantrolene's effects on ECCE were relevant to its ability to prevent or treat MH, myotubes prepared from WT, HET, and HOM R163C-RyR1 mice were tested for their rates of Mn2+ quench elicited by 20-Hz electrical pulses described above and the effects of dantrolene on these quench rates. In these experiments, the extracellular Mn2+ was set at 500 µM, but instead of the nominally Ca2+-free external solution used in experiments shown in Figs. 4 and 5B, external Ca2+ was set to 300 µM Ca2+. Under these experimental conditions (500 µM Mn2+ + 300 µM Ca2+), the Mn2+ quench rates triggered by 20-Hz pulse trains were approximately 50% of those measured in nominally Ca2+-free solutions. Figure 7 shows that the rate of Mn2+ quench elicited by this stimulus protocol was enhanced 1.8- and 2-fold for HET and HOM R163C-RyR1 myotubes compared with WT (p < 0.0001). When the myotubes were pretreated with 10 µM dantrolene 10 min before measuring quench rates using solvent as a control, it had profound effects on ECCE similar to what we observed in WT myotubes. Figure 8 shows that dantrolene reduced ECCE rates (measured as the rate of Mn2+ entry elicited by a 20-Hz electrical train, 40 s in duration) to 60 to 70% of the respective control rate irrespective of genotype. In this regard, dantrolene was able to lower ECCE rates in HET and HOM myotubes to less than those measured in WT myotubes in the absence of dantrolene (Fig. 8) but was not able to lower them to the rate of dantrolene-treated WT cells, suggesting that additional mechanisms might also be important in the actions of dantrolene.
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; Hurne et al., 2005). Here, we provide the first evidence that ECCE is also operant in mature adult skeletal muscle fibers (i.e., FDBs) and implicates a potential physiological role for ECCE in adult skeletal muscle. A defining characteristic of ECCE seen in both FDBs and myotubes is that the magnitude of ECCE (defined by the rate of Mn2+ quench triggered by addition of K+ to the external medium) is greatly enhanced when measured after blocking RyR1 with micromolar ryanodine, a concentration sufficient to eliminate responses to caffeine.
It is well established that exposure of mice to ryanodine and its derivatives triggers hypercontraction of skeletal muscle with rapid onset that is invariably lethal (Waterhouse et al., 1987). To date, skeletal muscle hypercontraction elicited by ryanodine has been interpreted as being solely the result of stabilizing a persistent open state of RyR1 (Meissner, 2002). However, ryanodine has been shown to stabilize multiple RyR1 channel conductance states, and predominating among them is a highly stable fully closed state (Zimányi et al., 1992; Buck et al., 1997; Bidasee et al., 2003). The novel observation reported here is that the ryanodine-modified RyR1 state in which ryanodine completely locks the RyR1 channel in a nonconducting conformation greatly enhances ECCE in myotubes and adult fibers, suggesting a potentially important role for Ca2+ entry in the etiology of ryanodine-induced hypercontraction. In support of this hypothesis, the actions of ryanodine have been documented to be dependent on the activity of the EC coupling elicited by transverse tubule depolarization (Procita, 1956, 1958; Hillyard and Procita, 1959). Moreover, evidence for the role of ECCE in normal use-dependent physiology and pathophysiology of adult skeletal muscles may have been described in earlier studies but were underappreciated. For example, the rate of relaxation of contractures after prolonged applications of extracellular K+ was faster in the absence of extracellular Ca2+ than in its presence (Caputo and Gimenez, 1967), whereas brief depolarization in Ca2+-free solutions was not different from the response in Ca2+-replete external medium (Caputo and Gimenez, 1967; Grabowski et al., 1972). More recently, age-related denervation of fast skeletal muscle was found in senescent mice, and muscle fibers isolated from them were found to show dependence on extracellular Ca2+ to maintain tetanic force (Payne et al., 2007).
Results from the present study also identify ECCE as a target of dantrolene's pharmacological actions in both FDBs and myotubes prepared from WT mice. The potency (IC50 = 4 µM) and limited maximum efficacy (60-70% diminution) of dantrolene toward attenuating ECCE is consistent with its pharmacological activity as a muscle relaxant. The efficacy of 10 µM dantrolene toward attenuating ECCE is similar in naive and ryanodine-exposed preparations in both models, suggesting that a common mechanism is involved. Together, these results confirm that myotubes represent a predictive and useful model of adult fibers in which to study physiological, pathophysiological, and pharmacological processes associated with ECCE. Dantrolene's inhibitory activity could be measured in both native and ryanodine-treated myotubes by monitoring either Mn2+ (Figs. 4 and 5B) or Ca2+ (Fig. 5A) entry. In this regard, Mn2+ and Ca2+ seem to compete for a common ECCE influx pathway because the rate of Mn2+ quench of Fura-2 is reduced by approximately 2-fold when the Ca2+ concentration in the external buffer is increased from nominally free Ca2+ (Fig. 4) to one that contains 300 µM Ca2+ (Figs. 7 and 8). As a skeletal muscle relaxant, dantrolene is active in the dose range of 1 to 10 µM, and it produces a maximum of 60 to 70% attenuation of contractile force (Gronert et al., 2004; Krause et al., 2004).
Measurements of RyR1 channel gating kinetics in the BLM preparation previously have failed to support (Szentesi et al., 2001) the biochemical evidence that is the basis for the hypothesis that the muscle relaxant properties of dantrolene result from a direct interaction with RyR1 domains that stabilize the closed conformation of the channel (Palnitkar et al., 1997, 1999; Paul-Pletzer et al., 2001, 2002; Kobayashi et al., 2005). Several prominent methodological differences between studies of single channels reconstituted in BLM and previous biochemical and biophysical studies could account for the discrepancy. For example, Fruen and colleagues (1997) demonstrated the importance of CaM, ATP, and temperature to measure dantrolene's inhibition of [3H]ryanodine binding to skeletal muscle membranes and enhanced SR Ca2+ mobilization from SR vesicles elicited by the addition of caffeine (Zhao et al., 2001). However, despite the fact that the conditions used in our BLM studies closely mimicked those used by Fruen and coworkers, they still do not support a direct mechanism by which dantrolene promotes channel closure at 35°C in the presence of CaM and ATP. Moreover, the RyR1 channels remained responsive to ryanodine even in the presence of dantrolene. Although the present results do not refute the presence of [3H]dantrolene or [3H]azido-dantrolene binding sites on RyR1, they do not support the interpretation that the occupation of these sites suppresses SR Ca2+ release from a given Ca2+ release unit or that it interferes with the gating activity of RyR1 channels. Our results do support the concept that dantrolene binding to the RyR1 complex could weaken its functional coupling to ECCE in native or ryanodine-modified states without affecting its inherent channel activity. It is important to note that attenuation of ECCE in intact skeletal muscle cells represents the first evidence of a pharmacologically relevant mechanism by which dantrolene suppresses sarcolemmal Ca2+ entry in response to a physiologically relevant trigger (i.e., membrane depolarization). In contrast, its proposed inhibition of a specific type of SOCE could only be demonstrated when stores were depleted by caffeine in combination with a ryanodine-modified RyR1 (Zhao et al., 2006).
We have shown previously that point mutations C4958S and C4961S change in the conformation of these Ca2+ channels to a persistent inactive state that can in turn influence ECCE inactivation/deactivation (Hurne et al., 2005). Similar influences on ECCE were reported in ryanodine-pretreated myotubes (Cherednichenko et al., 2004). In the present article, we demonstrate enhanced ECCE in R163C HET and HOM myotubes that could be reduced by 10 µM dantrolene to a rate similar to that seen in naive WT cells. It remains to be seen whether enhanced rates of ECCE in MH myotubes could represent a risk factor for triggering clinical MH with halogenated general anesthetics and whether triggering agents further exacerbate the rate of ECCE in MH muscles to that observed with ryanodine-modified channels. A role for ECCE in MH susceptibility, clinical MH, and possibly other disorders of skeletal muscle deserves further attention.
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Footnotes |
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ABBREVIATIONS: MH, malignant hyperthermia; BLM, bilayer lipid membrane; EC, excitation-contraction; ECCE, excitation coupled calcium entry; FDB, flexor digitorum brevis; FKBP12, FK506 binding protein 12 kDa; RyR1, ryanodine receptor type 1; SR, sarcoplasmic reticulum; SOCE, store-operated calcium entry; c, mean closed-dwell time; o, mean open-dwell time; ES, electrical stimulation; WT, wild type; DP1, domain peptide 1; AA, amino acid; HET, heterozygous; HOM, homozygous; AM, acetoxymethyl ester; Mn-R, manganese-containing Ringer; CHAPS, 3-[(3-cholamidopropyl)dimethylammonio]propanesulfonate; PAGE, polyacrylamide gel electrophoresis; Ry, ryanodine.
Address correspondence to: Dr. Isaac N. Pessah, Department of Molecular Biosciences, School of Veterinary Medicine, One Shields Avenue, University of California, Davis, CA 95616, E-mail: inpessah{at}ucdavis.edu
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10 min; depletion phase not shown), 
