Exercise training increases L-type calcium current density in coronary smooth muscle

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Exercise training increases L-type calcium current density in coronary smooth muscle

D. K. Bowles, Q. Hu, M. H. Laughlin, and M. Sturek

Vascular Biology Laboratory, Dalton Cardiovascular Research Center, Departments of Physiology and Veterinary Biomedical Sciences, University of Missouri, Columbia, Missouri 65211

ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Exercise training produces numerous adaptations in the coronary circulation, including an increase in coronary tone, bothin conduit and resistance arteries. On the basis of the importanceof voltage-gated Ca²⁺ channels (VGCC) in regulation of vascular tone, we hypothesizedthat exercise training would increase VGCC current density incoronary smooth muscle. To test this hypothesis, VGCC currentwas compared in smooth muscle from conduit arteries (>1.0 mm),small arteries (200-250 µm), and large arterioles (75-150 µm)from endurance-trained (Ex) or sedentary miniature swine (Sed).After 16-20 wk of treadmill training, VGCC current was determinedusing whole cell voltage-clamp techniques. In both Ex and Sed,VGCC current density was inversely related to arterial diameter,i.e., large arterioles > small arteries > conduit arteries. Exercisetraining increased peak inward currents approximately twofoldin smooth muscle from all arterial sizes compared with those fromSed (large arteriole, $-$ 12.52 ± 2.05 vs. $-$ 5.74 ± 0.99 pA/pF; smallartery, $-$ 6.20 ± 0.97 vs. $-$ 3.18 ± 0.44 pA/pF; and conduit arteries, $-$ 4.22 ± 0.30 vs. $-$ 2.41 ± 0.55 pA/pF; 10 mM Ba²⁺ external). Dihydropyridine sensitivity, voltage dependence, andinactivation kinetics identified this Ca²⁺ current to be L-type current in all arterial sizes from bothSed and Ex. Furthermore, peak VGCC current density was correlatedwith treadmill endurance in all arterial sizes. We conclude thatsmooth muscle L-type Ca²⁺ current density is increased within the coronary arterial bedby endurance exercise training. This increased VGCC density mayprovide an important mechanistic link between functional and cellularadaptations in the coronary circulation to exercisetraining.

voltage clamp; dihydropyridine; vascular smooth muscle; microcirculation; voltage-gated calcium channels; porcine

	INTRODUCTION

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ENDURANCE EXERCISE TRAINING produces numerous adaptations in the regulation of coronary arterial tone (8, 23, 30, 37).Although these adaptations appear complex and heterogeneous throughoutthe coronary circulation, in general, exercise training is associatedwith enhanced vasodilation and reduced vasoconstriction to vasoactiveagonists (23, 37). Although the cellular mechanisms underlyingthese training-induced adaptations have not been completely described,numerous studies have demonstrated a central role for dihydropyridine-sensitive,voltage-gated Ca²⁺ channels (VGCC) in the regulation of arterial tone (for review,see Ref. 33). Vasoconstrictor agonists including serotonin,endothelin, and norepinephrine increase arterial tone directlyand/or indirectly through activation of VGCC (3, 17, 18,35). Conversely, many vasodilators such as adenosine (12)decrease arterial tone, in part, through activation of K⁺ channels, which hyperpolarize the cell membrane and inactivateVGCC and Ca²⁺ influx (33). In addition, VGCC contribute significantly toboth development and maintenance of myogenic tone (20, 46).Previously, we demonstrated an enhanced myogenic response in resistance(30) and conduit (9) coronary arteries of endurance-trainedswine. Furthermore, Haskell et al. (15) provided evidence foran increased basal tone in conduit coronary arteries of endurance-trainedhumans. Thus it appears that enhanced coronary tone may be a generaladaptation to endurancetraining.

Given the central role of VGCC in the regulation of coronary arterial tone and the increase in coronary tone after exercisetraining, we hypothesized that exercise training would increaseVGCC current in coronary smooth muscle. Therefore, the presentstudy determined VGCC current densities in isolated smooth musclecells from conduit arteries (>1.0 mm), small arteries (200-250µm), and large arterioles (75-150 µm) after endurance exercisetraining. In support of our hypothesis, we found that exercisetraining increased L-type Ca²⁺ current density to a similar extent in smooth muscle from allarterialsizes.

	MATERIALS AND METHODS

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Animals. Adult female miniature swine weighing 25-40 kg were obtained from the breeder (Charles River) and housed in pens at the Collegeof Veterinary Medicine, University of Missouri, Columbia, MO.All pigs included in this study were familiarized with treadmillexercise over a 1- to 2-wk period. Treadmill performance testswere administered to each animal. Pigs were then randomly dividedinto two groups. One group (Ex, n = 9) underwent a progressivetreadmill training program used previously in our laboratory (25,30, 36). The second group of pigs was restricted to theirpens (6 × 12 ft) for 16-20 wk and served as sedentary controls(Sed, n = 10). Animal protocols were approved by the Universityof Missouri Animal Care and Use Committee in accordance with the"Principles for the Utilization and Care of Vertebrate AnimalsUsed in Testing, Research andTraining."

Training procedures. During the first week, the pigs from the Ex groups ran on the treadmill at 3 miles per hour (mph), 0% grade for 20-30 min(endurance) and at 5 mph for 15 min (sprint). The speed and durationof running were gradually increased over the first 12 wk at arate dependent on the tolerance of each pig. During the final4-8 wk of training, a typical training session consisted of thefollowing 85-min workout: 1) 5-min warm-up run at 2.5 mph, 2)15-min sprint at speeds of 5-8 mph, 3) 60-min endurance run at4-5 mph, and 4) 5-min warm-down run at 2 mph. Ranges are givenbecause the exercise training program was individualized to eachanimal's exercise ability. The pigs were given positive reinforcementfor exercise by feeding after each trainingbout.

Treadmill performance test. Efficacy of training was determined by administering treadmill performance tests before and at the completion of the training(Ex) or pen confinement (Sed). The performance tests consistedof the following four stages (performed continuously): stage 1,3.1 mph, 0% grade for 5 min; stage 2, 3.1 mph, 10% grade for 10min; stage 3, 4.3 mph, 10% grade for 10 min; and stage 4, 6 mph,10% grade until exhaustion. Typically, animals ran briefly intostage 4 before training and extended this time posttraining. Totalrunning time to exhaustion (i.e., stages 1-4) wasrecorded.

Skeletal muscle oxidative enzyme activity. At the time the animals were killed, muscle samples were taken from the lateral head of the triceps brachii and deltoid, frozenin liquid N₂, and stored until processed. Citrate synthase activitywas measured spectrophotometrically from whole muscle homogenates(40).

Preparation of coronary arteries. Pigs were anesthetized with ketamine (30 mg/kg) and pentobarbital sodium (35 mg/kg) and administered heparin. The hearts wereremoved and placed in iced (4°C) Krebs bicarbonate solution duringvessel isolation. Conduit (>1.0-mm ID) segments of right coronaryartery were trimmed of fat and connective tissue in sterile modifiedEagle's Minimal Essential Storage Media containing 20 mM HEPES(EH) plus 2% horse serum on ice. Small arteries (200- to 250-µmID) and large arterioles (75- to 150-µm ID) were dissected freefrom the subepicardial wall near the apex. Small arteries andlarge arterioles between branch points were selected. All arterieswere stored under sterile conditions in EH at 4°C untildispersion.

Cell dispersion. All experiments were performed on freshly dispersed cells using methods modified from those described previously (41-43, 45).Small arteries and large arterioles were incubated in 200 µl ofenzyme solution consisting of low-Ca²⁺ (0.5 mM) physiological solution plus 294 U/ml collagenase (CLSII, Worthington), 6.5 U/ml elastase (Worthington), 2 mg/ml bovineserum albumin (fraction V, Sigma), 1 mg/ml soybean trypsin inhibitor(type I-S, Sigma), and 0.4 mg/ml DNase I (type IV, Sigma). Cellswere enzymatically dispersed by incubation for 45-60 min in ashaking water bath at 37°C. Immediately after dispersion the enzymesolution was replaced with enzyme-free low-Ca²⁺ solution, and isolated single cells were obtained with gentletrituration by micropipette. For conduit coronary arteries, arterieswere opened longitudinally and pinned, lumen side up, onto a siliconerubber substratum in ~2 ml of low-Ca²⁺ enzyme solution. Cells were enzymatically dispersed for 45-60min in a shaking water bath at 37°C. The enzyme solution was thenreplaced with enzyme-free low-Ca²⁺ solution, and isolated single cells were obtained by repeatedlydirecting a stream of low-Ca²⁺ solution over the artery via pasteur pipette. All solutions usedfor conduit and resistance vessels were identical. Cell suspensionswere stored in low-Ca²⁺ (0.5 mM) buffer at 4°C until use (0-6h).

Whole cell voltage clamp. Whole cell currents were determined with a standard whole cell voltage-clamp technique as used routinely (42-44). Cells wereinitially superfused with physiological saline solution (PSS)containing (in mM) 2 CaCl₂, 138 NaCl, 1 MgCl₂, 5 KCl, 10 HEPES,and 10 glucose, pH 7.4, during gigaseal formation. After wholecell configuration, the superfusate was switched to PSS with tetraethylammoniumchloride (TEACl) substituted for NaCl and either 2 mM Ca²⁺ or 10 mM Ba²⁺ as the charge carrier. The pipette solution contained (in mM)120 CsCl, 10 TEACl, 1 MgCl₂, 20 HEPES, 2 Na₂ATP, 0.5 Tris-GTP,5 EGTA, and 0.2 fura 2 pentapotassium salt, pH 7.1. Fura 2 wasincluded in the pipette to verify whole cell dialysis. Ionic currentswere amplified by a List EPC-7 patch-clamp amplifier with a 0.5-50G $Omega$ variable feedback resistance head stage. Whole cell currentswere filtered through an eight-pole low-pass filter with a cutofffrequency of 400 Hz, digitized at 495-µs intervals, and storedon computer. Current densities (pA/pF) were obtained for eachcell by normalization of whole cell current to cell capacitanceto account for differences in cell membrane surface area. Capacitycurrents were measured for each cell during 10-ms pulses froma holding potential of $-$ 80 mV to a test potential of $-$ 70 mV. Capacitycurrents were filtered at a low-pass cut-off frequency of 8.4kHz and digitized at 25-µs intervals. Leak subtraction was notperformed. Data acquisition and analysis were accomplished usinga Labmaster analog-to-digital converter and microcomputer equippedwith AxoBASIC 1.0 data acquisition software (Axon Instruments).All experiments were conducted at room temperature (22-25°C).Cells were continually superfused under gravity flow. Stock solutionsof nifedipine were dissolved in 100% ethanol and diluted 1,000-foldfor finalsolutions.

Statistics. Data are expressed as means ± SE with data from each animal averaged and counted as one observation (n). The data presentedfor sedentary controls represent a subset of previously publisheddata demonstrating an inverse relationship between coronary arterialdiameter and smooth muscle VGCC density in sedentary swine (6).For the purposes of the present investigation, data obtained oncells from sedentary animals whose time of death correspondedwith the exercise-trained group were analyzed on a per-animalbasis (i.e., all cells for each vessel category for each animalwere averaged and counted as 1 observation). There was no significantdifference between the sedentary animals or cells from the previousstudy and the subset utilized in the present investigation. Datapresented for exercise-trained animals have been previously publishedonly as an abstract (7). ANOVA was used for comparisons betweengroups with unpaired t-test used for post hoc analysis. A P value<0.05 was set as the criterion for significance in allcomparisons.

	RESULTS

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Efficacy of exercise training. Consistent with previous reports using the treadmill-trained miniature swine model (23, 25, 30, 36), the exercise-trainedanimals in the current study demonstrated marked training adaptationsincluding a 33% increase in citrate synthase activity in the lateralhead of the triceps brachii (Sed 13.81 ± 0.76 vs. Ex 18.32 ± 1.34µmol · min¹ · g¹; P < 0.05), a 39% increase in citrate synthase activity in thedeltoid (Sed 16.15 ± 1.24 vs. Ex 22.49 ± 1.51 µmol · min¹ · g¹; P < 0.05), an increased heart weight-to-body weight ratio (Sed4.49 ± 0.13 vs. Ex 5.35 ± 0.15 g/kg; P < 0.05), and a 42 ± 6%increase in treadmill endurance time (Fig. 1).

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Fig. 1. Increased treadmill endurance time with training. Total treadmill endurance time before (Pre) and after (Post) 16-20 wk of treadmill training (Ex) or sedentary confinement (Sed) is shown. Group data are plotted as means ± SE, in addition to individual animal Pre and Post values. Exercise training produced a significant increase in endurance exercise capacity. Significant individual variation was observed in training response for animals in Ex group. Sedentary pen confinement had no effect on exercise capacity. * P < 0.05 vs. Sed.

Exercise training and cell size. Exercise training had no effect on whole cell membrane capacitance in cells from conduit arteries, small arteries, or largearterioles, indicating a similar cell surface area in coronarysmooth muscle cells from Sed and Ex (Table 1). In both groups,mean cell membrane surface area decreased as arterial diameterdecreased, demonstrating an overall tendency for smooth musclecell size to decrease with arterial size; however, the differencebetween cells from small arteries and large arterioles was notsignificant in Ex. Series resistance during voltage clamp wassimilar in all arterial groups (Table 1).

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Table 1. Coronary smooth muscle cell characteristics

VGCC in coronary smooth muscle. Figure 2 shows a representative family of currents obtained under the experimental conditions described using 10 mM externalBa²⁺ as the charge carrier. Successive depolarization steps from aholding potential of $-$ 80 mV to a final test potential of +50 mVin 10-mV increments produced inward currents showing a peak near+10 mV and slow inactivation. With Ca²⁺ as the external charge carrier, the time for the sustained currentto decay to one-half peak amplitude at a test potential of 0 mVwas similar in conduit arteries, small arteries, and large arterioles(200 ± 22, 203 ± 25, and 212 ± 11 ms, respectively) and was unaffectedby exercise training (191 ± 25, 180 ± 13, and 206 ± 12 ms, respectively).These values for current inactivation are similar to those previouslyreported for L-type current in smooth muscle and are ~15-foldgreater than those for T-type current (44). Thus the whole cellcurrents measured in the present study demonstrated current-voltage(I-V) relationships and slow inactivation characteristics consistentwith L-type Ca²⁺ current (2, 5, 26, 44).

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Fig. 2. Voltage-gated Ca²⁺ channel (VGCC) current in coronary smooth muscle. Representative family of current traces for voltage-gated Ca²⁺ current in coronary smooth muscle cells is shown. Currents were elicited by 260-ms step depolarizations from holding potential (HP) of $-$ 80 mV to test potentials (TP) of $-$ 80 to +50 mV in 10-mV increments with 10 mM external Ba²⁺ as charge carrier (selected test potentials shown). Displayed currents were obtained with a coronary myocyte from a large arteriole (117 µm) of a sedentary animal. Depolarizations positive to $-$ 40 elicited a sustained, slowly inactivating inward current that was maximal near +10 mV. Further depolarization reduced inward current. Dotted line, zero-current level. Capacitance transients are eliminated for clarity.

Exercise training and VGCC density. Figure 3 shows representative current traces comparing voltage-gated Ca²⁺ current in smooth muscle from conduits (Fig. 3A), small arteries(Fig. 3B), and large arterioles (Fig. 3C) from sedentary and exercise-trainedanimals. The magnitude of both the peak and sustained inward currentwas increased in cells from trained animals in all arterial sizes.The effect of exercise training on I-V relationships for coronarymyocytes from conduit arteries, small arteries, and large arteriolesis shown using either 10 mM external Ba²⁺ (Fig. 4A) or 2 mM external Ca²⁺ (Fig. 4B) as the charge carrier. Exercise training increasedpeak VGCC density approximately twofold in all arteries. In bothgroups, VGCC density increased as arterial diameter decreased,indicating a heterogeneous distribution of VGCC within the coronaryarterial network as previously reported (6). Voltage-dependentactivation was not affected by exercise training in any arterialsize (Fig. 5). Membrane potential producing half-maximal activationtended to be more positive in arteries from exercise-trained animals;however, this difference was not significant (conduit, $-$ 1.63 ±0.76 vs. 1.38 ± 0.31 mV; small artery, $-$ 0.60 ± 0.75 vs. 1.57 ±0.62 mV; and large arteriole, $-$ 3.78 ± 0.99 vs. $-$ 1.29 ± 0.31 mV;Sed vs. Ex, respectively).

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Fig. 3. Exercise training increases VGCC current. Representative current traces comparing peak voltage-gated inward Ca²⁺ current in smooth muscle cells from conduit arteries (A), small arteries (B), and large arterioles (C) from Sed and Ex animals. Currents were elicited by 260-ms step depolarizations to +10 mV from HP of $-$ 80 mV with 10 mM Ba²⁺ as external charge carrier. Peak and sustained inward currents were increased in Ex compared with Sed. Membrane capacitance was 25 and 23 pF (A), 16 and 12 pF (B), and 13 and 12 pF (C) for Sed and Ex, respectively. Capacitance transients are eliminated for clarity. Dotted line, zero-current level.

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Fig. 4. Effect of exercise training on VGCC current-voltage (I-V) relationship. I-V relationships for whole cell VGCC current in coronary myocytes from conduit arteries (a), small arteries (b), and large arterioles (c) from Ex and Sed animals are shown. Currents were obtained using either 10 mM Ba²⁺ (I_Ba; A) or 2 mM Ca²⁺ (I_Ca; B) as external charge carrier. Current is plotted as peak inward current measured during a 260-ms step depolarization to membrane potential (V_m) indicated from HP of $-$ 80 mV. Current is normalized to cell membrane capacitance (pA/pF). Data are means ± SE; n values as in Table 1, average of 2-5 cells/artery/animal. * P < 0.05, Sed vs. Ex.

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Fig. 5. Exercise training does not alter voltage-dependent activation. Voltage-dependent activation (d $infinity$ ) in smooth muscle cells from conduit arteries (A), small arteries (B), and large arterioles (C) from Ex and Sed animals. Data are means ± SE (n values as in Table 1), where d $infinity$ = peak I_Ba/[g_Ba (V $-$ E_rev)], g_Ba is maximal conductance obtained from linear regression of positive limb of I-V relationship through apparent reversal potential (E_rev), and I_Ba was obtained from I-V relationship. Activation data were fit to a conventional Boltzmann distribution equation, d $infinity$ = 1/{1 + exp[(V_0.5 $-$ V)]/k}, where V_0.5 is membrane potential producing half-maximal activation and k is slope factor. Exercise training had no effect on activation curves for any arterial size.

Endurance capacity and VGCC density. As demonstrated in Fig. 1, the individual responsiveness to training among animals, as indicated by treadmill endurance tests,was quite variable. This variation stimulated an examination ofthe relationship between training status and coronary smooth muscleVGCC density (Fig. 6). With data from both groups combined, asignificant correlation was found between treadmill endurancetime and peak VGCC density in conduit arteries, small arteries,and large arterioles, suggesting a direct association betweenendurance capacity and VGCC density. Approximately 45-65% of thevariation in VGCC density could be accounted for by differencesin endurance capacity, with the strongest correlation found inthe large arterioles. In fact, when data from large arteriolesof trained animals were analyzed separately, over 90% of the variationin VGCC density was accounted for by the response to training(r² = 0.93).

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Fig. 6. Relationship of endurance capacity and VGCC current density. Relationship of endurance capacity, as assessed by treadmill endurance time, vs. peak VGCC density (I_{Ba max}) in coronary smooth muscle from conduit arteries (A), small arteries (B), and large arterioles (C). Individual animal values are plotted ( $open circle$ , Sed; $bullet$ , Ex). Correlation analysis for all animals showed significant positive correlation between treadmill endurance time and peak VGCC density for all arterial sizes, especially for large arterioles. Separate correlation analysis on large arteriole data from Ex group alone revealed greater correlation coefficient (r = 0.96), indicating that >90% of variation in peak VGCC density in large arterioles after training could be accounted for by variation in endurance capacity.

Relative contribution of L-type Ca²⁺ current. Smooth muscle has been reported to contain both T-type and L-type Ca²⁺ channels (44). L-type Ca²⁺ channels are highly sensitive to block by dihydropyridines suchas nifedipine, whereas T-type channels are insensitive to thisclass of drugs (2). To determine the relative contributionof dihydropyridine-sensitive L-type Ca²⁺ channels to whole cell VGCC current, inhibition of whole cellVGCC current by nifedipine was examined. Sensitivity of wholecell VGCC to nifedipine in porcine coronary smooth muscle cellsis shown in Fig. 7. With a holding potential of $-$ 80 mV, peak inwardcurrent at +10 mV was inhibited in a concentration-dependent fashion(IC₅₀ $approx$ 32 nM). Although L-type Ca²⁺ channels are highly sensitive to nifedipine, this sensitivityis highly voltage dependent. The holding potential of $-$ 80 mV usedin the present study (chosen to avoid possible differences ininactivation characteristics between groups) is relatively hyperpolarized,necessitating a higher dihydropyridine concentration to producemaximal inhibition. In addition, a maximally effective concentrationof nifedipine avoids possible differences in dihydropyridine sensitivitybetween groups. Therefore, a maximally effective concentrationof nifedipine (3 µM) was used for comparison between groups. Figure8 shows the effect of 3 µM nifedipine on Ca²⁺ current in smooth muscle cells from conduit arteries (Fig. 8,A and D), small arteries (Fig. 8, B and E), and large arterioles(Fig. 8, C and F) from both sedentary (Fig. 8, A-C) and exercise-trained(Fig. 8, D-F) animals. Peak inward current at +10 mV in the presenceof 3 µM nifedipine was effectively abolished in cells from allarterial sizes from both trained and sedentary animals (% inhibition:Sed, 96 ± 2, 98 ± 2, and 91 ± 4; Ex, 99 ± 2, 98 ± 2, and 103 ±11 for conduit, small artery, and larger arterioles, respectively).Thus dihydropyridine-sensitive L-type Ca²⁺ current appears to be the dominant VGCC current in coronary smoothmuscle of all arterial sizes, supporting previous studies showinga predominance of L-type Ca²⁺ current in most vascular smooth muscle (6, 19, 26, 28).To further test the relative contribution of L-type Ca²⁺ current in coronary arterial myocytes, we examined the effectof steady-state depolarization on the I-V relationship. Currentsderived from T-type and L-type voltage-gated Ca²⁺ channels in smooth muscle can be separated by holding potential(2, 19, 44). Compared with L-type channels, T-type channelsactivate and peak at more negative membrane potentials and areinactivated by steady holding potentials less than $-$ 40 mV (2,44). Thus the presence of two types of voltage-gated Ca²⁺ channels can be discerned by a positive shift in the I-V relationshipwhen the holding potential is increased (44). Normalized I-Vrelationships obtained at holding potentials of $-$ 80 mV and $-$ 30mV were superimposable in arteries of all sizes and were unaffectedby training (Fig. 9). The lack of a positive shift in the I-Vrelationship with sustained depolarization to $-$ 30 mV confirmsthe absence of a significant T-type Ca²⁺ current and supports a predominance of L-type Ca²⁺ current in coronary arteries from both trained and sedentaryanimals.

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Fig. 7. Dihydropyridine inhibition of VGCC current. A: inhibition of normalized Ba²⁺ current (I_Ba/I_{Ba max}) by 0.1 (top) and 1.0 (bottom) µM nifedipine (Nif). Effect of 0.01 µM nifedipine is shown for comparison. After whole cell access (time 0), I_Ba elicited by depolarization to +10 mV from HP of $-$ 80 mV increased to a steady-state plateau, which was unaffected by 0.01 µM nifedipine. Subsequent application of either 0.1 or 1.0 µM nifedipine resulted in reversible inhibition. B: VGCC current was inhibited by nifedipine in a concentration-dependent manner. Data were fitted with a sigmoidal curve (IC₅₀ $approx$ 32 nM). Data are expressed as means ± SE; n = 3 cells/concentration, obtained from conduit arteries of sedentary control animal.

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Fig. 8. Similar efficacy of dihydropyridine inhibition across arterial size and training status. Typical experimental tracings showing block of inward current by the dihydropyridine nifedipine (3 µM) are given. Step depolarizations to +10 mV from HP of $-$ 80 mV before ( $open circle$ ) and after ( $bullet$ ) nifedipine are shown for cells from conduit arteries (A and D), small arteries (B and E), and large arterioles (C and F) from Sed (A-C) and Ex (D-F) animals. Nifedipine completely abolished inward current at +10 mV in all arteries from both groups, demonstrating predominance of dihydropyridine-sensitive Ca²⁺ channel current (L-type) in coronary smooth muscle in arteries from both Sed and Ex animals. Similar inhibition was seen at all membrane potentials (data not shown). Capacitance transients are eliminated for clarity. Dotted line, zero-current level.

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Fig. 9. Effect of sustained depolarization on VGCC I-V relationship. I-V relationships for VGCC obtained by 10-mV step depolarizations to from $-$ 60 mV to +50 mV from HP of $-$ 80 ( $bullet$ ) or $-$ 30 ( $open circle$ ) mV are shown. Normalized I-V relationships are shown for cells from conduit arteries (A and D), small arteries (B and E), and large arterioles (C and F) from Sed (A-C) and Ex (D-F) animals. Currents were normalized to peak inward current for each cell at each HP. I-V relationships obtained at each HP were superimposable in all arteries. Lack of a shift in I-V relationship with sustained depolarization indicates lack of T-type VGCC current and predominance of L-type VGCC current in all arteries from both Sed and Ex groups.

	DISCUSSION

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Substantial evidence exists supporting the role of chronic exercise in reducing the incidence and severity of coronary vasculardisease (1, 13). Although recent studies have greatly expandedour understanding of the impact of exercise on coronary arterialregulation, relatively little is known about the intrinsic cellularchanges within the coronary vasculature associated with thesefunctional adaptations. The present study provides novel evidencethat endurance exercise training increases voltage-gated Ca²⁺ channel current density in coronary arterial smooth muscle. Inlight of the well-documented importance of voltage-gated Ca²⁺ channels in regulation of vascular tone in both normal and diseasestates (27, 33), this information could provide a vital mechanisticlink between exercise training and associated functional adaptationswithin the coronarycirculation.

Arterial tone, via control of vascular resistance, is the major determinant of total blood flow and distribution within thecoronary circulation. Various vasoactive stimuli including norepinephrine(32), serotonin (14), endothelin (17) and pressure (22,27) increase arterial smooth muscle tone through depolarizationand activation, directly or indirectly, of VGCC. In addition,vasodilators such as endothelium-dependent hyperpolarizing factor(11), nitric oxide (4), and adenosine (12) have been shownto activate K⁺ channels, resulting in hyperpolarization, inactivation of VGCC,and vasodilation. Thus the relative activation of VGCC can affectboth vasoconstriction and vasodilation. The present study foundan approximately twofold increase in peak voltage-gated Ca²⁺ current density in coronary smooth muscle after exercise training.This training-induced increase was similar in magnitude in conduitarteries, small arteries, and largearterioles.

Although the training-induced increase was most apparent at membrane potentials positive to the reported physiological rangefor vascular smooth muscle, i.e., $-$ 60 to $-$ 30 mV (33, 34),it is important to note that apparent thresholds for Ca²⁺ current activation in whole cell voltage-clamp configurationsare really detection thresholds. VGCC activity is a continuousfunction of membrane potential, with no true threshold (16,33). Therefore, it is probable that the training-induced differencesin whole cell Ca²⁺ current can be extrapolated to more negative membrane potentials.Furthermore, important physiological vasoconstrictors such asnorepinephrine and serotonin shift the voltage dependence foractivation of VGCC to more negative membrane potentials (33,35). On the basis of these findings, we predict an enhancedrole of VGCC in regulation of coronary vascular tone after enduranceexercise training. Although numerous physiological stimuli associatedwith acute exercise and exercise training could be responsiblefor the increase in VGCC density, it is interesting to note thatdihydropyridine-sensitive VGCC number has been reported to beincreased by $beta$ -adrenergic stimulation (39). The increased sympatheticactivation and circulating catecholamines associated with exercisemay be a contributing stimulus for training-induced increasesin VGCC current. This training-induced increase in VGCC currentdensity may be specific for coronary smooth muscle, because endurancetraining did not alter VGCC current in rat cardiac myocytes (29).

Smooth muscle contains two distinct types of voltage-gated Ca²⁺ current (2, 5, 44). The channel subtype responsible forwhole cell currents can be distinguished by several characteristicsincluding dihydropyridine sensitivity and time- and depolarization-dependentinactivation characteristics. L-type channels are highly sensitiveto inhibition by dihydropyridines (2, 33), whereas T-typechannels are insensitive to this class of drugs (16, 33).Furthermore, T-type channels are activated by small depolarizationsand inactivate quickly, whereas L-type channels require greaterdepolarization for activation and inactivate slowly (5). Thewhole cell currents in all arterial sizes in the present studywere abolished by the dihydropyridine nifedipine and showed characteristicL-type voltage dependence of activation and slow inactivation(2, 33, 44). These characteristics are strongly indicativeof L-type Ca²⁺ channels being the predominant channel type in smooth muscleof all coronary arterial sizes. This conclusion is in agreementwith other studies showing a predominance of L-type Ca²⁺ channels in most vascular smooth muscle (2, 6, 19, 28)including coronary myocytes (26). Exercise training had no effecton either current characteristics or sensitivity to nifedipine,indicating a similar predominance of L-type channels in arteriesfrom trained and sedentaryanimals.

Although not directly addressed in this study, the expected physiological consequence of this training-induced increase inL-type VGCC current would be an overall increase in contractileresponse to the numerous vasoconstrictor stimuli that activateVGCC. Exercise training was shown to increase myogenic tone inresistance arteries similar in size to the large arterioles ofthe present study (30), and dihydropyridine-sensitive Ca²⁺ channels are required for development and maintenance of myogenictone (20, 46). Therefore, the increased myogenic responseof resistance arteries after exercise training may be caused,in part, by an enhanced VGCC current. The strong correlation betweentraining status and VGCC density in the large arterioles (Fig.6C) supports the hypothesis that training-induced increases inVGCC density contribute to the previously reported enhanced myogenictone in these arteries (30). Similarly, exercise training hasbeen shown to increase basal tone in conduit coronary arteriesof miniature swine in vitro (9), and Haskell et al. (15)concluded that basal tone in conduit arteries of endurance athletesis also increased in vivo. The finding that training increasedVGCC density in smooth muscle cells from conduit arteries as wellas smaller resistance arteries supports an overall direct associationbetween a training-induced increase in coronary tone and VGCCcurrent density. Although this is intriguing, it must be emphasizedthat these correlations do not provide direct evidence linkingenhanced myogenic tone and increased VGCC current density in responseto training. Further studies will be needed to directly test thishypothesis.

Aside from increases in basal coronary tone, the overall functional adaptation of the coronary circulation to exercise traininghas been generalized as reduced vasoconstriction and enhancedvasodilation to various vasoactive agents (23, 24, 37).After exercise training, in vitro studies showed reduced contractileresponses in coronary arteries to norepinephrine (36) and endothelin(8), both of which are known to activate VGCC (21). Thesefindings appear difficult to reconcile with the increase in VGCCdensity found in the present study. However, recent studies ofvascular smooth muscle are uncovering a role for intracellularCa²⁺ not exclusively in vasoconstriction but, under certain conditions,as a mechanism for vasodilation (10, 31, 47). By compartmentalizingintracellular Ca²⁺ into restricted subcellular spaces, i.e., the subsarcolemmalspace, and away from the Ca²⁺-dependent contractile apparatus, localized increases in Ca²⁺ can activate Ca²⁺-activated K⁺ (K_Ca) channels to limit depolarization and vasoconstriction orproduce vasodilation. Thus, under certain conditions, increasingCa²⁺ influx could be a mechanism to limit vasoconstriction or inducevasodilation. Several lines of evidence support such a model fortraining-induced adaptations in coronary smooth muscle. With theuse of simultaneous intracellular Ca²⁺ and contractile techniques, we previously reported a reducedaveraged myoplasmic Ca²⁺ (Ca_m) and contractile response to endothelin after exercise training(8). Paradoxically, although contraction and bulk Ca_m werereduced by training, Ca²⁺ influx was dramatically increased, providing indirect evidencefor increased sarcolemmal Ca²⁺ cycling after exercise training. As proposed by Rasmussen etal. (38), sarcolemmal Ca²⁺ cycling produces a high subsarcolemmal Ca²⁺ (Ca_s) concentration without a substantial increase in Ca_m. Theresulting increase in Ca_s could, therefore, limit contractionby activation of K_Ca channels, which hyperpolarize the membraneand limit contraction (10). Recently, a similar role for sarcoplasmicreticulum (SR) Ca²⁺ release, i.e., Ca²⁺ sparks, in limiting depolarization and vasoconstriction by activationof K_Ca channels has been proposed (31). Sturek and colleagues(41, 42) found that exercise training increased slow SR Ca²⁺ release, i.e., SR Ca²⁺ unloading, in coronary smooth muscle, which can produce increasedCa_s and K_Ca channel activation (43). Together, these data supporta model for limiting contraction and/or enhancing vasodilationby increasing Ca²⁺ influx. The increased VGCC density in smooth muscle after trainingdescribed in the present study fits well within such amodel.

In conclusion, the current study provides direct electrophysiological evidence that endurance exercise training increasesL-type VGCC current density in coronary smooth muscle. This trainingadaptation was similar in coronary myocytes from conduit arteries(>1.0 mm), small arteries (200-250 µm), and large arterioles (75-150µm). Furthermore, L-type Ca²⁺ current density was directly correlated with endurance capacity.In light of the importance of VGCC in regulation of coronary arterialtone and, consequently, total and regional blood flow, these findingsshould provide an important mechanistic link between cellularand functional adaptations of the coronary circulation to exercisetraining.

	ACKNOWLEDGEMENTS

The authors thank Pam Thorne and Tammy Strawn for invaluable assistance in thisproject.

	FOOTNOTES

This work was supported by National Heart, Lung, and Blood Institute Grants HL-52490 (M. H. Laughlin, M. Sturek, and D. K.Bowles), HL-41033 (M. Sturek), and HL-02872 (M.Sturek).

Address for reprint requests: D. K. Bowles, E102 Veterinary Medicine, Univ. of Missouri, Columbia, MO 65211.

Received 17 November 1997; accepted in final form 31 August 1998.

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