Voltage-dependent calcium channels in ventricular cells of rainbow trout: effect of temperature changes in vitro

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Voltage-dependent calcium channels in ventricular cells of rainbow trout: effect of temperature changes in vitro

Catherine S. Kim¹, Mary D. Coyne², and Judith K. Gwathmey¹

¹ Institute for Cardiovascular Disease and Muscle Research, Cambridge 02138; and ² Department of Biological Sciences, Wellesley College, Wellesley, Massachusetts 02481-8203

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Voltage-dependent calcium channels (VDCC) in ventricular myocytes from rainbow trout (Oncorhynchus mykiss) were investigatedin vitro using the perforated patch-clamp technique, which maintainsthe integrity of the intracellular milieu. First, we characterizedthe current using barium as the charge carrier and establishedthe doses of various pharmacological agents to use these agentsin additional studies. Second, we examined the current at severalphysiological temperatures to determine temperature dependency.The calcium currents at 10°C (acclimation temperature) were identifiedas L-type calcium currents based on their kinetic behavior andresponse to various calcium channel agonists and antagonists.Myocytes were chilled (4°C) and warmed (18 and 22°C), and theresponse of VDCC to varying temperatures was observed. There wasno significant dependency of the current amplitude and kineticson temperature. Amplitude decreased 25-36% at 4°C (Q₁₀ ~1.89)and increased 18% at 18°C (Q₁₀ ~1.23) in control, Bay K8644 (BayK)-, and forskolin-enhanced currents. The inactivation rates ( $tau$ _i)did not demonstrate a temperature sensitivity for the VDCC (Q₁₀1.23-1.92); Bay K treatment, however, increased temperature sensitivityof $tau$ _i between 10 and 18°C (Q₁₀ 3.98). The low Q₁₀ values for VDCCare consistent with a minimal temperature sensitivity of troutmyocytes between 4 and 22°C. This low-temperature dependency mayprovide an important role for sarcolemmal calcium channels inadaptation to varying environmental temperatures introut.

cardiac myocytes; fish; perforated patch clamp; dihydropyridines

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

EXCITATION-CONTRACTION COUPLING (E-C coupling) in cardiac muscle is activated by an increase in intracellular calcium concentration([Ca²⁺]_i), which in turn is dependent on two sources: 1) internal calciummobilization from the sarcoplasmic reticulum (SR) and 2) externalcalcium influx across the sarcolemma through voltage-dependentcalcium channels (VDCC). Intracellular calcium is lowered by reuptakeinto the SR and extrusion through the sarcolemma via the Na⁺/Ca²⁺ exchanger. The magnitude of the increase in [Ca²⁺]_i depends on the contribution from each compartment, which varieswith species and temperature (11, 16). For example, fast transientincreases in intracellular calcium are seen in mammalian and avianspecies, suggesting that immediate release of calcium from theSR is the primary source of [Ca²⁺]_i (16). In contrast, in amphibians such as the salamander,the calcium transient has a more prolonged profile, suggestingthe additional contribution of [Ca²⁺]_i from another source, most likely diffusion across the sarcolemmafrom the extracellular compartment (16). At the other end ofthe spectrum, myocytes from frog ventricles have been shown torely solely on a transsarcolemmal influx of calcium (11).

To date studies in teleost cardiac myocytes have shown that E-C coupling in trout is a ryanodine-insensitive mechanism atphysiological heart rates and temperatures (10°C), implying animportant role for transsarcolemmal calcium movement. However,at higher temperatures, the reverse is true, i.e., blockage ofthe SR by ryanodine has a significant effect on cardiac musclefunction (19). This suggests that, depending on the temperature,the E-C coupling mechanism in trout hearts can vary its dependencyon calcium from the extracellular compartment or from the intracellularSR. Therefore, one might predict that the VDCC in teleost heartswould be particularly sensitive to temperaturechanges.

In these studies we identified the L-type calcium currents as the predominant calcium current in trout myocytes and characterizedtheir responsivity to various agents. This information will beused in further physiological studies on trout myocardial contractility.In addition, in contrast to hearts of other species, trout myocardiumshows little temperature dependence when subjected to warmer orcooler experimental temperatures invitro.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Cell isolation. Rainbow trout (Oncorhynchus mykiss) 8-10 inches in length were obtained from the Mohawk Trout Hatchery (Sunderland,MA). The fish were raised outdoors in open tanks maintained at10°C by a continuous flow of fresh well water and were maintainedindoors at 10°C in an aquarium containing aerated, dechlorinatedwater (pH 7.0, O₂ 7.5 parts/million) for 3-14 days untileuthanasia.

The trout were anesthetized with 3-aminobenzoic acid ethyl ester placed in an aliquot of aquarium water (0.2 g/l, pH 7.4).After excision of the heart and removal of excess tissue and bloodclots, the hearts were placed in oxygenated 0.2 mM calcium buffer(CaB) at 5°C. The heart was quickly mounted to a perfusion apparatusby inserting a cannula with an olive-shaped tip (27 gauge) throughthe bulbus arteriosus into the ventricle and tying a ligaturebetween the atria and theventricle.

The cell isolation procedure was modified from that of Mitra and Morad (29) and Karttunen and Tirri (20). Solutions forisolation were as follows: standard buffer (SB) contained (inmM) 137 NaCl, 4.6 KCl, 1.2 MgCl₂, 3.5 NaH₂PO₄ · H₂O, 11 glucose,and 10 HEPES, pH to 7.4 with 1 M NaOH. CaB contained SB with 0.2mM CaCl₂. Enzyme buffer was composed of 50 ml CaB, 0.033 g collagenase(type 1), and 0.025 g BSA (fraction V). The heart was perfusedfor 20 min with calcium-free SB and then with enzyme buffer containingcollagenase (type 1, 300 U/mg) and 0.2 mM Ca²⁺ for 20 min. After digestion, the heart was perfused with 0.2mM CaB for 10 min to wash out the enzyme solution. All solutionswere oxygenated at room temperature. The heart was then placedinto CaB, atria and bulbus arteriosus were excised, and the remainingtissue was teased apart into small pieces and triturated withfresh CaB. The cells in CaB were oxygenated and stored at 2-8°Cuntiluse.

Chemicals. The following stock solutions were kept frozen in aliquots and thawed and diluted just before use: Bay K8644 1,10, and 100 µM {Bay K; 1,4-dihydro-2,6-dimethyl-5-nitro-4-[2-(trifluoromethyl)phenyl]pyridine-3-carboxylic acid methyl ester} in DMSO, a giftof Dr. A. Scriabine (Miles Laboratories; New Haven, CT); nifedipine100 µM in DMSO; 8-bromoadenosine 3',5'-cyclic monophosphate (8-BrcAMP)0.058 M. The following stock solutions were refrigerated (2-4°C)until used: FPL-64176 100 µM {FPL; 2,5-dimethyl-4-[2-(phenylmethyl)benzoyl]-1H-pyrrole-3-carboxlicacid methyl ester} (Research Biochemicals International; Natick,MA) and 1 mM nicardipine. A stock solution of isoproterenol HCl(1 mM) was kept in a dark bottle at room temperature and was dilutedbefore use. Unless indicated otherwise, chemicals were obtainedfrom Sigma (St. Louis, MO) and were of the highest analyticgrade.

Electrophysiology. Currents were recorded using the perforated patch-clamp version of the original patch-clamp technique (32).Myocytes were plated on 35-mm tissue culture dishes pretreatedwith 10% poly-L-lysine solution. The composition of the extracellular(bath) solution and the pipette solution was designed to minimizecurrents through Na⁺ and K⁺ channels. Tetrodotoxin (TTX, 1-2 µM) was applied to the bathto block Na⁺ channels. The predominant use of barium as the charge carrierand Cs⁺ in the pipette solution blocked K⁺ currents. Barium or calcium was used as the charge carrier inthe bath solution, which contained (in mM) 138 NaCl, 5 BaCl₂,1 MgCl₂, 10 glucose, 10 HEPES with 1 M NaOH or 115.5 NaCl, 20CaCl_2, 1 MgCl₂, 10 glucose, and 10 HEPES. The pH was set to 7.3with 1 M NaOH at room temperature and varied from 7.2 to 7.4 overthe experimental temperature range (4-22°C). These pH ranges reflectthose used for catfish (7.3) (26), perch (7.4) (20), and frogand shark (7.2) (29) myocardium and myocytes. The pipette solutioncontained (in mM) 123 Cs-glutamate, 20 tetraethylammonium chloride,2 CaCl₂, 1 MgCl₂, 10 glucose, 10 HEPES, pH to 7.3 with 1 M CsOH.All solutions were passed through a 0.2-µm filter before use.Amphotericin B for the perforated patch was made fresh daily (30mg/ml DMSO). The final concentration was 240 µg/ml in the pipettesolution.

For perforated patch recording, the tip of the pipette was filled with amphotericin B-free pipette solution and was backfilledwith the amphotericin B solution. Electrode resistance variedfrom 2-5 M $Omega$ . The liquid junction potential was adjusted beforeseal formation, and capacitive transients were compensated afterseal formation but not after perforation. Once an electrical continuitywas established, the currents were stable for up to 2 h. Datawere filtered at 5 kHz using an Axopatch 200A patch-clamp amplifier(Axon Instruments; Foster City, CA), collected on a Gateway 20004DX2-50 computer, and analyzed using pCLAMP software (version5.5, Axon Instruments). Patch electrodes were made from soft glasshematocrit tubes (Drummond Scientific; Broomall, PA; 100 µl) witha double pull (David Kopf Instruments; Tujunga, CA) coated withSylgard (Dow Corning; Midland, MI) and fire-polished on a home-mademicroforge (36).

Under voltage clamp conditions, the cells (n = 57) were held at $-$ 100 or $-$ 50 mV and stepped in 10-mV increments to differentpotentials for 300 ms. Voltage-dependent activation was takenas the average response of cells held at $-$ 100 mV and stepped tovoltages between $-$ 40 to +20 mV. For steady-state inactivation,cells were held at a given voltage for 1.5 s before stepping to20 mV for 300 ms. Linear leakage current was determined at thedifferent potentials and subtracted from the individual records.The temperature was set during the experiments with a heatingand cooling temperature controller (TC-10, Dagan; Minneapolis,MN) with a stability of ±0.1°C. The cooling apparatus surroundedthe culture dish containing the cells, which were brought to temperatureover a 10-min period and then held at each temperature for atleast 5 min before testing. The cells were perfused by gravityflow except during the equilibration and test periods. All drugs,including TTX, were added directly to the bath during the testperiod. The temperature probe was resin-coated so metal was notin contact with the bathsolution.

Data analysis. Curve fitting to data was accomplished using Sigma Plot Scientific Graphing Software (Jandel Scientific; CorteMadera, CA). The half-maximum activation and inactivation of thebarium currents were obtained by fitting the data to the Boltzmannequation for activation or for inactivation (15). The time constants( $tau$ _i) for the inactivation of the barium currents were determinedusing pCLAMP software. Inactivation was fit with a single or adouble exponential. An R value of 0.97 or greater determined thebest fit. The value for Q₁₀ for the temperature analyses was determinedwith the equation

log Q10 = (10/(t2 − t1))(log <IT>X</IT>t1 − log <IT>X</IT>t2)

where t₂ and t₁ represent the temperatures at which the parameters (X) were measured (e.g., peak current amplitude, rateof inactivation) (26).

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

All experiments were conducted at 10°C, the acclimated body temperature of the fish, unless otherwise noted. Freshly isolatedrainbow trout ventricular myocytes were narrow, elongated, andstriated. Two inward currents were expressed in myocytes, a low-threshold,voltage-dependent Na⁺ current as well as a high-threshold, voltage-dependent calciumcurrent. The Na⁺ current activated between $-$ 30 and $-$ 40 mV and was blocked with1-2 µM TTX, which did not affect the remaining inward current(data not shown). The inward high-voltage activating calcium currentwas present in all cells tested (n = 57) and was investigatedin the presence of TTX at 10°C.

Calcium and barium were compared as charge carriers by holding the potential of the cell at $-$ 50 mV and stepping to voltagesfrom $-$ 60 to +70 mV in 10-mV increments for 300 ms. Figure 1 showscurrent traces with the two different carriers recorded from twodifferent cells. At 10°C, the calcium current (Fig. 1A) was smalleven with 20 mM Ca²⁺ and inactivated rapidly [ $tau$ _i 52.10 ms at voltage step (V_s) +50mV]. The peak current with 20 mM Ca²⁺ was at 50 mV. In contrast, with barium as the charge carrier(Fig. 1B), the amplitude of the inward current was larger anddid not completely inactivate during the depolarizing step ( $tau$ _i80.52 ms at V_s 20 mV). The faster inactivation with calcium asthe charge carrier could be due to calcium-dependent inactivationof L-type calcium channels. The peak current was shifted to amore hyperpolarized voltage (+20 mV) with barium. The larger current,slower inactivation, and shift of peak voltage is characteristicof an L-type calcium current seen in mammalian cells with bariumas a charge carrier vs. calcium (12, 18). Because barium provideda larger current in these cells, it was used as the charge carrierin subsequent experiments.

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Fig. 1. Calcium and barium currents in trout ventricular myocytes under perforated patch-clamp conditions (PPCC). Example of peak current amplitude and inactivation at 10°C with 20 mM calcium or 5 mM barium. Data are taken from 2 different cells and are representative of currents seen. Note difference in scaling. Dotted line indicates zero current levels in this and all subsequent figures. A: 20 mM CaCl₂. B: 5 mM BaCl₂.

Voltage-dependent kinetics. Figure 2A shows a family of barium currents obtained under perforated patch-clamp conditions.Cells were held at $-$ 100 mV with 10-mV steps between $-$ 10 and 40mV. As the cell was depolarized by increasing voltage steps, thevoltage-dependent current demonstrated an increased amplitudeand increased rate of inactivation up to the peak voltages. Asseen in Fig. 2B, activation occurred at voltages more positivethan $-$ 20 mV. The mean voltage eliciting a peak current was 10mV, although with barium it varied between 10 and 20 mV for anygiven cell. This may be due to the normal variability from cellto cell because the perforated patch maintains cellular integrity.

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Fig. 2. Barium currents in trout myocytes using PPCC. A: family of inward barium (5 mM) currents at 10°C. Voltage steps are shown to left of each trace. B: current-voltage relationships of inward barium current; mean of 4 cells ± SE. Peak current values in each cell were normalized to maximum current and plotted against voltage step. C: plot of voltage dependence of inactivation as time constant ( $tau$ _i) of single exponential decay of current taken from traces in A. Inset: single exponential fit (white line) to trace [holding potential (V_h) $-$ 100 mV, voltage step (V_s) 20 mV]. I/I_max, current amplitude/maximum current.

The time course of the current decay during depolarization at 10°C was best fit with a single exponential function at allvoltages tested. The time constants for inactivation of the currentsshown in Fig 2A are plotted in Fig 2C where the value decreasedfrom 589 ms at V_s 10 mV to about 70-75 ms between V_s 20 and 40mV. The fast inactivation at the peak voltage was not due to calcium-inducedinactivation because barium was used as the charge carrier. Althoughthe rate of decay for L-type channels is much slower in many tissues,generally moderately fast inactivation is characteristic of L-typecurrent in ventricular myocytes (18).

Data from multiple cells for voltage-dependent activation and steady-state inactivation were normalized to the maximum currentand the means ± SE were plotted as current amplitude/maximum current(I/I_max) vs. the holding potential (Fig. 3). Both sets of datawere fit with the appropriate form of the Boltzmann equation,which is shown as a smooth line. The inward barium current activatedat voltages greater than $-$ 20 mV with a peak at 10 mV and a midpointpotential (V_1/2) for activation at $-$ 8.05 mV, slope parameter (k)4.37. Steady-state inactivation began around $-$ 30 mV with completeinactivation at 5-10 mV; V_1/2 for inactivation was $-$ 14.11 mV,k 5.16. Our values, however, for V_1/2 for steady-state inactivationare about 12 mV more depolarized than those values for rainbowtrout under whole cell patch clamp (40). A similar shift hasbeen reported for calcium currents in Y1 adrenal cells when theperforated patch clamp was used compared with whole cell patch-clampconditions (9)

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Fig. 3. Mean activation and steady-state inactivation curves for the inward barium (5 mM) current in trout ventricular myocytes at 10°C; error bars are SE and are sometimes smaller than symbols.

, activation; $open circle$ , inactivation. Peak current amplitudes were normalized to maximum current and plotted against holding potential. Data were fit (solid line) using appropriate form of Boltzmann equation (see METHODS). With barium as charge carrier, currents activated at voltages more positive than $-$ 20 mV, midpoint potential (V_1/2) $-$ 8.05 mV, slope (k) 4.37, n = 6. Inactivation began around $-$ 30 mV, V_1/2 $-$ 14.11, k 5.16, n = 4.

The steady-state inactivation curve shows that the inward current was not inactivated at $-$ 50 mV. This is also illustratedin Fig. 4 where no difference was observed in the amplitude orcharacteristic shape of the inward current when myocytes wereheld at $-$ 100 or at $-$ 50 mV (V_s 20 mV). The consistency of thisresponse suggests that only one type of inward calcium currentis present in teleost ventricular myocytes.

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Fig. 4. Current traces for inward barium current at 10°C from V_h of $-$ 100 (A) and $-$ 50 mV (B) with V_s to 20 mV. There was no change in amplitude or voltage-dependent kinetics at 2 different V_h values.

Dihydropyridine sensitivity. Myocytes (~70%) tended to have very small inward currents under control conditions at 10°C comparedwith those seen by Vornanen (40) in trout that were studiedat 22°C using the whole cell patch clamp. This response raisedthe question of whether calcium channels in these trout ventricularmyocytes were inactive because of either the low temperature (10°Ccompared with 22°C) (40) or the patch-clamp conditions vs. wholecell. Bay K, a dihydropyridine (DHP) calcium channel agonist,which enhances open time of L-type channels (18), was appliedto the myocytes to expose latent L-type calcium channels. As seenin a typical cell in Fig. 5A, a much larger current was expressedafter application of 20 nM Bay K. The calcium channels in troutmyocytes were very sensitive to Bay K, showing a response to dosesas small as 5 nM. Figure 5A shows that at holding potential (V_h) $-$ 100 mV and V_s 0 mV, the barium currents were enhanced with increasingdoses of Bay K from 5 nM up to a concentration of 20 nM Bay K;no significant change in the current amplitude was observed beyondthis concentration. The inward barium current was also sensitiveto nifedipine, a DHP calcium channel antagonist, as illustratedin Fig. 5B.

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Fig. 5. Effect of dihydropyridines on barium currents in trout ventricular myocytes at 10°C. A: current traces of inward barium current enhanced with the L-type calcium channel agonist Bay K8644 (Bay K). Doses ranged from 5 to 20 nM. The drug elicited a positive response beginning at 5 nM with maximum fivefold increase in current amplitude at 20 nM. B: current traces of inward barium current in response to L-type calcium channel antagonist nifedipine (nif) from 200 nM to 1 µM. Bay K (80 nM) was applied initially to enhance current. A 12-fold increase in nifedipine (1 µM compared with 80 nM Bay K) suppressed ~62% of Bay K-enhanced current at V_h $-$ 100 mV.

To see inhibition with DHP antagonists, we first generated a larger current with 80 nM Bay K. Increasing doses of the antagonistnifedipine were then used to block the Bay K effects, but theconcentrations necessary were substantially higher than expected.At V_h $-$ 100 mV, 1 µM nifedipine (12.5 times greater concentrationthan Bay K) suppressed only 62% of the Bay K-enhanced current(Fig. 5B); at V_h $-$ 50 mV, however, 86% of the current was suppressed(data not shown). The greater effectiveness of nifedipine at V_h $-$ 50 mV is most likely due to the fact that DHP binding is greatestat more depolarized holding potentials (4). We approached theproblem another way by increasing the current using forskolin,which increases phosphorylation of L-type calcium channels bydirectly activating adenylate cyclase. Forskolin activation ofthe current eliminated binding competition between two DHPs, andin addition, we used a more potent DHP antagonist, nicardipine.At 4°C and V_h $-$ 100 mV, 6 µM nicardipine, but not 3 µM, blockedthe inward current by 87.9% (Fig 6D). At V_h $-$ 50 mV, however, 92.9%of the current was suppressed by nicardipine. In summary, theinward current in trout myocytes was as sensitive to DHP agonistsas cardiac cells in other species (3, 30, 31) but demonstratedless sensitivity to antagonists as reported earlier in carp andtrout myocytes (39, 40).

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Fig. 6. Effects of other agonists and inhibitors. A: non-dihydropyridine agonist FPL-64176 (FPL). FPL (60 nM) increased barium current more than ninefold. Barium 20 mM. B: cadmium (250 µM) completely suppressed Bay K-enhanced current (100 nM). C: cadmium (250 µM) also suppressed current enhanced by FPL (60 nM). Barium 20 mM. $open circle$ , control;

, treatment. D: blockage of inward current by nicardipine. Current was stimulated with 10 µM forskolin (4°C). Nicardipine (6 µM) suppressed 87.9% of inward forskolin-activated current.

Response to other agonists and inhibitors. A non-DHP agonist for the L-type calcium channel FPL was also tested in trout cardiacmyocytes with 20 mM barium in the bath. A dose of 30 nM FPL wasineffective, but 60 nM produced a large current similar to theresponse seen with Bay K but with considerably slower rates ofactivation, inactivation, and deactivation (Fig. 6A; V_h $-$ 100 mV,V_s 30 mV). FPL also shifted the voltage peak of the inward bariumcurrent to a relatively more depolarized voltage (30 mV). Similardifferences in the three rates in response to Bay K and FPL havebeen demonstrated in rat and guinea pig ventricular myocytes (33,34).

Calcium channels are differentially blocked by specific inorganic ions. Cadmium has a potent inhibitory effect on VDCC. Asseen in Fig. 6B, 250 µM Cd²⁺ completely suppressed the Bay K-enhanced barium current in troutmyocytes (V_h $-$ 100 mV, V_s 10 mV). This is similar to the effectof cadmium observed in frog (3, 13), carp (39), and rat(22) myocardium. In trout myocytes, with an FPL-enhanced bariumcurrent, 250 µM Cd²⁺ also completely blocked the inward current (Fig. 6C).

Isoproterenol, a potent stimulator of cardiac contraction, acts by phosphorylating L-type calcium channels via a cAMP-dependentkinase. The inward current in trout ventricular myocytes exhibiteda positive response to isoproterenol at 30 nM with a maximum 10-foldincrease in current at 300 nM (Fig. 7A; V_h $-$ 100 mV, V_s 0 mV) withan EC₅₀ of approximately 60 nM (Fig. 7B). Although the magnitudeof the response to isoproterenol was greater than that previouslyreported for trout and carp (40), the sensitivity appeared tobe somewhat less than that reported, although the full range ofdoses was not tested in earlier reports (40).

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Fig. 7. $beta$ -Adrenergic agonist. A: traces of inward barium current (5 mM) at 10°C in response to increasing doses of isoproterenol from 30 to 300 nM. B: dose-response curve to isoproterenol with current amplitudes normalized to maximum current. Current amplitude reached maximum at 300 nM with an EC₅₀ of ~60 nM.

8-BrcAMP, which easily penetrates the cell membrane and is not degraded, was added to the bath solution to bypass the receptor-adenylatecyclase complex and to directly stimulate protein kinase A forchannel phosphorylation. At 10°C 8-BrcAMP (100 µM) elicited apositive response from trout ventricular myocytes (Fig. 8A; V_h $-$ 100 mV, V_s 10 mV). The amplitude of the inward current increasedprogressively with additional 8-BrcAMP, reaching an eightfoldincrease at 1 mM. With these data EC₅₀ was ~250 µM (Fig. 8B).

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Fig. 8. Channel phosphorylation. 8-Bromoadenosine 3',5'-cyclic monophosphate (8-BrcAMP) was used to promote calcium channel phosphorylation. A: traces of inward barium current (5 mM) at 10°C in response to increasing doses of 8-BrcAMP from 0.1 to 1 mM. B: dose-response to 8-BrcAMP with current amplitudes normalized to maximum current. Current amplitude reached maximum at 1 mM with EC₅₀ of ~250 µM.

We noticed that there were differences in the time course of the inward barium current inactivation with isoproterenol and8-BrcAMP stimulation compared with Bay K. Isoproterenol and 8-BrcAMPpromoted increases in channel phosphorylation and hence currentamplitude, with nominal inactivation during the 300-ms depolarization,whereas the current in the presence of Bay K, which also increasedin amplitude, had a comparatively rapid rate ofinactivation.

Temperature effects on current amplitude. The effect of temperature on barium currents in trout ventricular myocytes was testedin vitro in ventricular myocytes from trout kept at their standardenvironmental temperature of 10°C. The myocytes were held at thefollowing temperatures within their physiologically relevant temperaturerange: 10°C (control, acclimation temperature) and 4, 18, and22°C, with 22°C being considered a stress temperature. Each cellwas tested at two to four different temperatures: 10°C and then4, 10, 18, and 22°C, except for the control cell in Fig. 9A, whichwas tested in the following sequence: 22°C and then 18, 10, and4°C. No difference in the results was noted with the order oftemperatures studied. Figure 9A demonstrates traces obtained froma cell stepped to 20 mV from a holding potential of $-$ 100 mV. Fromthe current-voltage plot shown in Fig. 9B, there was a significantdecrease (32%) in current amplitude at 4°C compared with the currentat 10°C (Table 1). This difference also held true in subsequentexperiments when the cell was first held at 10°C and then changedto 4°C. The amplitude of the currents at 18 and 22°C was not significantlydifferent from the control at 10°C. The average Q₁₀ for changein amplitude of the peak current from 10 to 4°C was 1.73 ± 0.30(n = 4). This is less than that seen in mammalian cardiac ventricularmyocytes, which have Q₁₀ values between 2.4-3.0 at temperaturesbetween 22 and 37°C (26), but comparable to the Q₁₀ for peakcurrent between 10 and 20°C in frog skeletal muscle (1.6) (7).

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Fig. 9. Response to in vitro changes in temperature. Recordings were taken in following temperature sequence: A and B: 22, 18, 10, 4°C. C and D: 10, 4, 18, 22°C. A and B: untreated cell. A: traces at 4 temperatures. B: current-voltage plot at 4 temperatures. C and D: cell exposed to 100 nM Bay K8644. C: traces at 4 temperatures. D: current-voltage plot at 4 temperatures.

, 4°C;

, 10°C; $black-diamond$ , 18°C; $triangle$ , 22°C.

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Table 1. Effects of temperature on amplitude of barium currents and related Q₁₀ values from representative cells

Bay K (100 nM) was added to prolong the open state of L-type calcium channels to see whether the changes in current at thedifferent temperatures remained. As expected the current was significantlyenhanced with Bay K. The temperature effects, nevertheless, werestill present. At 4°C, the current was reduced by 36% comparedwith the control at 10°C (Fig. 9C; V_h $-$ 100 mV, V_s 10 mV; Table1); this was similar to the depression in amplitude expressedin the control cell (Fig. 9A). The magnitude of the current at22°C was similar to that at 10°C, and a small increase in thebarium current occurred at 18°C (Fig. 9D).

$beta$ -Agonists act by a cAMP-dependent phosphorylation of L-type channels, which is a result of the sequential activation of adenylatecyclase and protein kinase A. Forskolin was added to bypass the $beta$ -adrenergic receptor and to stimulate cAMP production via directactivation of adenylate cyclase. This treatment should providea large population of phosphorylated L-type calcium channels.At 10°C 10 µM forskolin significantly enhanced the inward currentand displayed a noninactivating current characteristic of phosphorylatedchannels (V_h -80 mV, V_s 10 mV) (Fig. 10A). At 4°C, the currentwas again suppressed by 25% compared with that seen at 10°C (Table1) but its profile was not changed (Fig 10A). At 18°C, the forskolin-stimulatedcurrent was increased by 23% (V_s 10 mV) as seen in the current-voltageplot (Fig. 10B). The Q₁₀ values remained similar to that seen withprimarily unphosphorylated control cells.

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Fig. 10. Activation of adenylate cyclase. Forskolin was used to directly activate adenylate cyclase in these cells. A: 10 µM forskolin significantly stimulated inward barium current at 10°C. At 4°C current was reduced by 25% compared with that at 10°C. Shifting to 18°C increased amplitude of current by 21%. B: current-voltage relationship of forskolin-stimulated current at 3 temperatures.

, 4°C;

, 10°C; $black-diamond$ , 18°C.

In summary, the colder temperature resulted in a suppression of the peak current by about 28%, whereas the warmer temperatureyielded an average increment of 23% and the Q₁₀ values indicateminimal temperature sensitivity beyond that of diffusionalone.

Voltage-dependent kinetics at different temperatures. To determine whether the calcium channel kinetics as well as currentamplitude were altered by the change in temperature, we lookedat $tau$ _i at the experimental temperatures. This parameter has beenexamined in other species, that is, in rat (26, 28) and guineapig hearts (2, 6, 17, 23), as well as frog skeletalmuscle (7) and is particularly sensitive to temperature changes.We looked at this same parameter to compare the responses of thetrout with otherspecies.

Inactivation of the barium current was easily quantitated and was best fit to a single exponential in the control and forskolin-treatedgroups. At the acclimation temperature of 10°C, the inactivationrate in both the control and Bay K-enhanced currents were similar.As temperature warmed, $tau$ _i became longer in untreated control cellsand was the reverse direction of change expected with an increasein temperature. Conversely, Bay K had a shorter $tau$ _i, indicatingan increased rate of decay with increasing temperature. Unlikethe other curve fits for $tau$ _i, inactivation in the presence of BayK at the higher temperatures was best fit with a double exponentialcurve, suggesting two components of the current under these conditions,a slower and faster phase. When the current was enhanced by phosphorylation,i.e., forskolin treatment (Fig. 10), there was very little decayduring the depolarizing step. However, by estimating the slopeof a line, a slight increase in the $tau$ _i was apparent at the highertemperatures (Q₁₀ 1.3, Table 2). All temperature-related changesin the untreated control and forskolin-treated cells had Q₁₀ between1.2 and 1.4 (Table 2), implying that both unphosphorylated andphosporylated L-type channels did not show any temperature dependencebeyond that resulting from thermal effect on ion diffusion. Inthe presence of Bay K between 10 and 22°C, the values for Q₁₀were higher (>3) than between 4 and 10°C. It is important to notethat the rate of inactivation in phosphorylated or unphosphorylatedL-type calcium currents, which are very sensitive to temperaturechange in other species (Q₁₀ >3), do not display this temperaturedependence in trout cardiac myocytes.

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Table 2. Current inactivation rate and Q₁₀ values for unphosphorylated (untreated) and phosphorylated (treated with 10 µM forskolin) channels

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Characterization of L-type current in fish. A high-voltage activating current was found in trout ventricular myocytes, whichis an L-type calcium current based on its kinetic behavior andresponse to various calcium channel agonists and antagonists.Similar currents have been reported in both carp and trout (39,40), but there are some differences in the characteristics ofthe current that require further comment with regard to the currentamplitude, sensitivity to DHP, and current decay after phosphorylation.The current amplitude in control cells using either calcium orbarium as the charge carrier is substantially smaller in thisreport compared with that reported earlier for trout and carpunder whole cell patch-clamp conditions (39, 40). The smallcurrent under perforated patch-clamp conditions might suggesta lesser density of channels, but when the population of L-typechannels was fully activated by either Bay K or forskolin, thecurrents increased substantially. The low activity of VDCC atrest in the trout myocytes in the present study, in comparisonto the stimulatory response seen with isoproterenol, cAMP, andforskolin, could be due to multiple controls on the phosphorylationof VDCC. For example, in rat ventricular myocytes, $beta$ ₂-receptorscouple to a G protein. The adenylate cyclase system has both astimulatory (G_s) and inhibitory (G_i) control, as shown by pertussistoxin inhibition of G_i (41). If the G_i system predominates inresting conditions, which are more likely to be seen with useof the perforated patch technique, then a smaller proportion ofthe population of L-type channels would be active. However, with $beta$ -adrenergic stimulation using isoproterenol and subsequentlyactivation of the G_s pathway, VDCC would be significantly increasedas more channels were phosphorylated. This hypothesis needs tobe testedfurther.

There also appears to be a large discrepancy in trout cells in their comparable sensitivity to DHP agonists and antagonists.The sensitivity to Bay K was in the nanomolar range, similar tothat found in both mammalian cardiac and skeletal muscle cells(14). The antagonists, however, appeared to have a reduced effectivenessin trout cardiac cells. We found that concentrations greater than1-6 µM were required for suppression of the current, whereas theusual dissociation constants are in the nanomolar range (14).Even though it has been reported that DHP antagonists are lesseffective on barium currents (24), similar µM doses of nifedipinewere needed to inhibit calcium currents in carp as well as introut myocytes (39, 40).

Phosphorylation of the L-type calcium channels in trout with either isoproterenol, cAMP, or forskolin not only increased currentamplitude but also reduced current decay during the depolarizingstep. These responses are characteristic of phosphorylated channels,whether from mammals or amphibians (25, 38). Although thesechanges in VDCC were seen in trout ventricular myocytes usingthe perforated patch, the slower current inactivation was notvisually observed in current traces of carp or trout myocytesunder whole cell conditions using either isoproterenol or forskolin,as reported by Vornanen (40). This may reflect differences inexperimental techniques, i.e., whole cell vs. perforatedpatch.

Temperature responses. Cardiac tissue in mammals is very sensitive to a fall in body temperature, which results in an increasedrisk of cardiac failure. However, poikilotherms, such as trout,may experience a range of body temperatures otherwise found onlyin hibernating animals (17) and yet are able to maintain adequatecardiac function. In this study, we attempted to explore the adaptabilityof VDCC in trout ventricular cells to changes in temperature.There are two ways to approach this problem: 1) acute studiesin vitro and 2) long-term adaptive studies in vivo. We began bytaking the former approach and determined that in the temperaturerange for trout from 4 to 22°C, their ventricular cells did notdemonstrate temperature sensitivity beyond that which could beattributed to thermal effect on iondiffusion.

The first parameter measured in trout ventricular myocytes was amplitude of the inward barium current. The amplitude decreasedas conditions shifted from the control acclimation temperatureof 10°C to cooler conditions. Because of the detrimental effectsof higher temperatures on the trout myocardium we were not ableto do a complete range of temperatures for an Arrhenius plot.However, we estimated Q₁₀ using a calculation that has been utilizedto assess temperature effects on calcium currents in rat ventriculartissue (26). With use of this method, the estimated Q₁₀ forcurrent amplitude with cooling was only 1.73, whereas the Q₁₀found in mammalian ventricular cells is usually between 2 and3 (17, 26), indicating a more temperature-sensitive response.Conversely, as the temperature was raised to 18 or 22°C, the amplitudeincreased, again with a low value for the Q₁₀. It appears thatusing the perforated patch clamp, the change in amplitude in responseto temperature shifts is not much greater than the Q₁₀ for thediffusion of ions (~1.3-1.6) (18) and implies a low sensitivityof trout myocardial cells to changes in temperature within theenvironmentalrange.

In addition to amplitude, we measured rates of inactivation in trout myocytes because this parameter is particularly sensitiveto temperature variation with reported Q₁₀ of 3 or greater (17,26). Inactivation rates were quantitated in all three groups(untreated, forskolin, and Bay K) and demonstrated low valuesfor Q₁₀. This indicates that although there were modificationsin inactivation of VDCC in trout with temperature, the changesdid not have a Q₁₀ large enough to indicate an enhanced sensitivityto temperature. These data in trout are contrary to those seenin other species. In addition, inactivation of calcium uptakeby cardiac SR in crucian carp and rainbow trout has been shownto express an insensitivity to temperature as well (1). Inthe hearts of other species, even in hibernators (7, 17,26, 28), however, the rate of current decay of L-type currentis the one response that is consistently temperature sensitive.Therefore, trout appear to be a specialcase.

We next asked whether the amplitude changes would still be present if the currents were enhanced with Bay K to prolong theopen time of the L-type channels. We saw an increase in overallcurrent amplitude as would be expected with longer open timesin the presence of the agonist. Inactivation kinetics in the presenceof Bay K was the one situation in which a temperature change (from10 to 18 or 22°C) exaggerated the response. At 18 and 22°C $tau$ _iwas fit with a double exponential curve rather than a single.The faster time constant for inactivation had a Q₁₀ of ~3, suggestingthat Bay K increased the sensitivity of inactivation at the highertemperatures, but the mechanism for this change is unknown andcontrary to what we found for trout myocytes in untreated andforskolin-treatedgroups.

Assessment of current amplitude in phosphorylated channels is simpler compared with the previous experiments because the currentis uncontaminated by an inactivation process. The peak of thecurrents in forskolin-treated cells exhibited similar directionalchanges in current amplitude to that of previous groups, i.e.,increasing with a rise in temperature with Q₁₀ values between1.27 and 1.85. This is in contrast to guinea pig ventricular cellsin which the Q₁₀ for changes in amplitude shifts from 2.57 to1.85 after phosphorylation (2). The Q₁₀ value for $tau$ _i in forskolin-treatedcells did not show a temperature dependency beyond that whichmight reflect changes in ionicflow.

The identification of calcium permeable stretch-sensitive cation channels (35) raises the question of whether such channelsare present in the trout ventricle. Moreover, could such currentsbe activated by a potential change in cell volume at differenttemperatures? These mechanosensitive channels do not appear tobe responsible for the inward currents in trout ventricular cellsthat we observed in response to temperature, because the changein cell volume (increasing at lower temperatures) varied inverselywith the magnitude of the current rather than thereverse.

What does this apparent temperature independence of cardiac VDCC mean to the fish? At decreased temperatures the metabolicneeds of the organism may be less, but blood pressure must bemaintained to adequately perfuse the tissues. Heart rate usuallydecreases with temperature, which would decrease cardiac output(10). Therefore, to maintain blood flow, stroke volume wouldneed to increase. This latter response would require an increasein [Ca²⁺]_i, which in turn is dependent on release of calcium from theSR or entry via VDCC. We have demonstrated that VDCC show minimaltemperature sensitivity so that the decrease in calcium currentand channel kinetics would be small with falling temperatures.This would allow the fish to adapt to the oscillating environmentaltemperatures with only a small change in the activity of the channelsand influx of calcium. In addition, if norepinephrine were released,phosphorylated channels would further increase calcium influx.Because the activity of Ca²⁺-ATPase in trout SR is not significantly altered at lower temperatures,reuptake of calcium would remain relatively stable (1). However,there may be less release of calcium from the SR since cardiaccontraction in teleosts is ryanodine-insensitive at low temperatures(19, 21), implying that calcium release from the SR is notcentral to E-C coupling at low temperatures. In this case then,maintenance of calcium influx via VDCC becomes an important mechanismin trout cardiac function at low temperatures. Lowered temperaturesmight also decrease the activity of the Na⁺-K⁺-ATPase, leading to an increase in intracellular Na⁺. The elevated Na⁺ could in turn promote further calcium influx via the reverseactivity of the Na⁺/Ca²⁺ exchanger as has been shown in guinea pig myocytes (5, 37).Ultimately, the total influx of calcium per given unit of timeand the chances of overloading the cell with calcium would dependon the heart rate and phosphorylation state of the channels. Ifthe actin-myosin-troponin complex remained sensitive to [Ca²⁺]_i (27) then we could predict the maintenance or even enhancementof the stroke volume at lower temperatures sustaining adequatecardiacoutput.

Perspectives

Factors that need to be considered in evaluating the physiological response of ventricular muscle at different temperatureswould include heart rate, the state of E-C coupling, potentialrelease of norepinephrine under stress and hence channel phosphorylation,calcium reuptake by the SR, calcium extrusion via sarcolemmalNa⁺/Ca²⁺ exchanger, Ca²⁺-ATPase, binding of calcium to calsequestrin in the SR, and thesensitivity of the actin-myosin-troponin complex to calcium signaling.Of all these parameters the availability of calcium plays a pivotalrole in ventricular contraction. In contrast to mammalian hearts,which are severely impaired at lower temperatures, the abilityof teleosts to maintain [Ca²⁺]_i may be an important mechanism in their ability to adapt tothe cold. Part of the adaptive response appears to be an abilityto maintain calcium entry via VDCC at lower temperatures, whichmay compensate for the declining availability of calcium influxfrom intracellular stores. Clearly, plasma membrane calcium channelsmay be an important consideration in adaptation of cardiac functionto changes in temperature in teleosts. However, studies on thefunction of trout VDCC in the cold need to be coupled with additionalexperiments on cardiac function at different temperatures whencalcium channel activity has been modified. These responses aredemonstrated in the companion study (8), which investigatesthe contractile function of trout hearts in the cold in the presenceof modulators of VDCCactivity.

	ACKNOWLEDGEMENTS

We thank Dr. John S. Cameron for advice and assistance on trout myocyte isolation and for use of the TC-10 temperature regulatorand cell isolationequipment.

	FOOTNOTES

Preliminary results were presented at the 42nd Annual Meeting of the Biophysical Society; Kansas City, MO; February 22-26,1998.

This work was supported by the National Science Foundation Grant IBN-9601434 to J. K.Gwathmey.

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.§1734 solely to indicate thisfact.

Address for reprint requests and other correspondence: M. D. Coyne, Dept. of Biological Sciences, Wellesley College, 106 Central St., Wellesley, MA 02481-8203 (E-mail: mcoyne{at}wellesley.edu).

Received 9 June 1999; accepted in final form 16 December 1999.

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