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1 Laboratory of Heart Electrophysiology, Institute of Experimental Cardiology, Cardiology Research Center, Moscow 121552, Russia; and 2 Laboratory of Cardiovascular Science, Gerontology Research Center, National Institute on Aging, National Institutes of Health, Baltimore, Maryland 21224
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ABSTRACT |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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With the whole cell patch-clamp technique, we studied the effects of the n-3 and n-6 polyunsaturated fatty acids (PUFAs), linoleic (C18:2n-6), eicosapentaenoic (C20:4n-3), docosahexaenoic (C22:5n-3), and arachidonic (AA; C20:4n-6) acids, on K+ currents in rat ventricular myocytes. At low concentrations (5-10 µM) all PUFAs except AA inhibited, by ~40%, the transient outward current (Ito) without affecting other K+ currents and markedly prolonged the action potential (AP). AA inhibited Ito but also augmented a sustained depolarization-induced outward K+ current (Isus); the latter effect did not occur in the presence of 4-aminopyridine or with eicosatetraynoic acid, a nonmetabolizable analog of AA. Higher concentrations of PUFAs (20-50 µM) further inhibited Ito and also inhibited Isus. Thus, at high concentrations, PUFAs have a nonspecific effect on several K+ channels; at low concentrations, PUFAs preferentially inhibit Ito and prolong the AP.
linoleic acid; eicosapentaenoic acid; fish oil; arachidonic acid; potassium currents
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INTRODUCTION |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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THE VITAL IMPORTANCE of the n-3 and n-6 polyunsaturated fatty acids (PUFAs), so called because of the location of the first double bond (at carbon no. 3 or 6, respectively, from the methyl end of the carbon chain), is becoming widely recognized in human physiology. Many studies suggest that n-3 fatty acids have beneficial effects on human health. In contrast, a diet enriched in n-6 fatty acids provokes atherosclerosis, carcinogenesis, and heart disease (see Ref. 19 for review). Although the underlying mechanisms of these dramatic differences are presently unclear, a different sensitivity of ionic channels to n-3 and n-6 types of fatty acids might contribute to this phenomenon.
Voltage-gated K+ channels control many aspects of cardiac performance in health and disease. In particular, these channels determine ventricular repolarization and modulate antiarrhythmic drug effects. It is known that the properties of K+ channels are influenced by their lipid environment (23, 25), and recently a large body of evidence has evolved indicating that changes in cardiac K+-channel properties are induced by fatty acids (8, 13, 17, 18). However, these studies did not differentiate the effects of n-3 versus n-6 PUFAs on K+ currents.
The purpose of the present study was to compare the effects of the n-3 and n-6 PUFAs on the transient K+ outward current (Ito) and other K+ currents. It has been shown that with the notable exception of guinea pigs, the Ito plays an important role in the cardiac action potential repolarization of several mammalian tissues, including human atrium (26) and ventricular myocytes from humans (30), dogs (20), rabbits (11), ferrets (3), and rats (1). In the present study to characterize the effects of PUFAs, we used rat ventricular myocytes in which K+ currents were recorded by the whole cell patch-clamp technique.
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METHODS |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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All the experiments were conducted at room temperature
(21-23°C) on cardiac myocytes enzymatically isolated from
2- to 3-mo-old Sprague-Dawley rats as previously described
(4). A whole cell voltage clamp was employed using an Axopatch 1D (
,
or gain, = 0.1; Axon Instruments). The recording pipette
resistance ranged between 1.5 and 3 M
. To isolate
K+ currents,
Na+ and
Ca2+ currents were blocked by
means of replacing external Na+
with N-methyl-D-glucamine and by adding 0.2 mM
CdCl2. The bath solution contained
(in mM) 137 N-methyl-D-glucamine, 3.7 KCl, 1.2 KH2PO4, 1 CaCl2, 1.2 MgSO4, 15 glucose, and 20 N-2-hydroxyethylpiperazine-N'-2-ethanesulfonic acid (HEPES), with pH adjusted to 7.4 using KOH. The solution in the
recording pipette contained (in mM) 110 KCl, 10 ethylene glycol-bis(-aminoethyl
ether)-N,N,N',N'-tetraacetic
acid, 10 HEPES, 3 MgATP, 0.1 Na2GTP, 5 glucose, and 10 NaCl,
with pH adjusted to 7.2 using KOH. When the action potentials of
myocytes were recorded in current-clamp mode using 1.5× threshold
pulses with a duration of 5 ms, the bath solution contained 137 mM
NaCl (instead of N-methyl-D-glucamine) and
no Cd2+ was used.
The peak Ito transient amplitude was measured as the difference between peak current and the steady current at the end of a 200-ms voltage step. The inactivation time constant for Ito was quantified by fitting with a single exponential function. To demonstrate the currents affected by the drug, the difference currents were obtained by subtraction of currents before the drug application from those after the drug. Note that in traces of difference currents upward deflections represent an increase in net outward membrane current and downward deflections represent a decrease in outward current with application of the drug.
In some studies, 4-aminopyridine (4-AP), indomethacin, and eicosatetraynoic acid (ETYA) were also used. Fatty acids and ETYA were diluted with nitrogen-saturated ethanol, and the stock solution was added to the superfusion solution to achieve the final desired concentration immediately before each experiment. These solutions were used within 60 min of preparation to minimize oxidation of fatty acids and were protected from light. 4-AP was prepared as a 5 M stock solution with pH adjusted to 7.4 with HCl. Indomethacin was made fresh at 0.1 M in dimethyl sulfoxide.
All averaged and normalized results are presented as means ± SE. Statistical significance of differences in the calculated mean values was evaluated using Student's t-test, and P values are provided (in parentheses) in the text. The level of statistical significance was considered at P < 0.05.
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RESULTS |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Under control conditions in the presence of
Ca2+- and
Na+-channel blockade,
depolarization steps of 200 ms from a holding potential of 
70 mV
evoked an outward K+ current. This
outward current rose to a peak and then slowly decayed (Fig.
1,
left). The outward
K+ current is thought to consist
of two components that can be separated both kinetically and
pharmacologically (1, 14). The rapidly activating (and inactivating)
transient outward current,
Ito, is defined
by its sensitivity to 4-AP. The second current component remaining
after Ito
inactivation was named as the sustained depolarization-induced current
(Isus) because
the delayed, time-dependent current
(IK) is either
absent or insignificant in rat ventricular myocytes (5, 27).
Isus activates
more slowly than
Ito and is not
sensitive to 4-AP. Original tracings of
K+ currents before and after
addition of 4-AP (5 mM) are shown in Fig. 1,
right. 4-AP clearly abolishes
Ito, whereas no
significant changes in the steady current at the end of the test step
can be detected. These characteristics of the outward current indicate that the current being studied under these conditions is
Ito (1, 14). We
have thus taken the difference between a peak
Ito and the
current at the end of the 200-ms voltage step
(Isus) as the amplitude of Ito.
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Effects of n-3 PUFAs on Ito current. The time course of docosahexaenoic (C22:5n-3) acid (DHA) effect on outward current amplitude is shown in Fig. 2. Gradually increasing downward deflections of difference currents (decreased net outward current) with time after DHA addition appear to indicate a reduction only of Ito, because the difference currents have kinetic properties similar to those of Ito. These effects of DHA were not observed when 4-AP (5 mM) was present in the bath (not shown).
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) evoked by a voltage step from 70 to +60 mV was 41.0 ± 2.6 ms (n = 4). In the presence of DHA
(5 µM), decreased within 3 min to 27.5 ± 1.7 ms
(P < 0.02). This effect was reversed
by superfusion of the cell with a fatty acid-free solution containing 0.1% bovine serum albumin (BSA), which binds fatty acids, thus releasing them from their cell binding sites. Figure
3B illustrates the time course of the
effect of 5 µM DHA to reduce the of
Ito and the
reversibility in BSA-containing solution.
To determine whether the effects of DHA were related to the effects of
its cyclooxygenase products, we tested the effects of DHA in the
presence of a cyclooxygenase inhibitor, indomethacin (22). Indomethacin
(10 µM) did not modify the effects of DHA (not shown).
To permit comparison of the amplitude of
Ito before and
after PUFA across a wide range of test potentials,
Ito was expressed as a function of control current at a step to +30 mV. These normalized currents were then plotted as a function of clamp voltage (Fig. 4). The inhibition of
Ito amplitude by
50 µM DHA did not depend on the test potential and was close to 60%
of control value at each potential.
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70 to +60 mV was inhibited by 73 ± 6% relative
to control (data not shown).
Concentration-dependent effects of n-3 PUFAs on Isus. The effects of PUFAs on K+ currents were concentration dependent between 5 and 50 µM (Fig. 5). Bath application of 5 and 10 µM EPA caused a decrease in Ito without affecting other outward K+ currents. At the higher concentrations of EPA tested (20 and 50 µM, n = 4) the inhibition of Isus (measured at the end of the 300-ms voltage step) was significant and concentration dependent (16 ± 4 and 56 ± 11%, respectively). Application of 50 µM DHA suppressed Isus by 32 ± 9% (data not shown).
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Effects of n-3 PUFAs on
IK1.
Although the present study focused mainly on the effects of PUFA on the
outward K+ currents, we also
investigated PUFA effects on inward rectifier K+ current
(IK1).
Hyperpolarization from 70 to 120 mV produced a
time-independent inward current,
IK1. Figure
6, left,
shows IK1
tracings in control and 10 min after the addition of 50 µM EPA.
IK1 amplitude was
measured at the end of the 200-ms voltage step. Superfusion of cells
(n = 5) for up to 12 min did not have any significant effect on
IK1. EPA failed
to induce any significant changes in
IK1 at all
voltage steps studied (120 to 80 mV). Figure 6,
right, demonstrates the recordings of
outward K+ currents in control and
10 min after application of 50 µM EPA in the same cell. An absence of
effects on IK1
was also observed for DHA (data not shown).
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Effects of n-3 PUFAs on action potential duration. Figure 7 illustrates a concentration-dependent effect of EPA on the action potential in rat ventricular myocytes. At low concentrations of EPA (5 and 10 µM), the action potential duration was gradually increased without change in amplitude. At a higher concentration (20 µM), a lengthening in the action potential duration was accompanied by a significant reduction in amplitude and decrease of the maximal rate of depolarization. In some experiments, the high concentration of EPA elicited a block of excitation. The decrease in the maximal rate of depolarization is in accordance with blocking effects of PUFAs on Na+ channels observed earlier (15, 31).
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Effects of n-6 PUFA on K+ currents and
action potential.
The effects of arachidonic (C20:4n-6) acid (AA), which belongs to the
n-6 class of PUFA, are shown in Fig. 8.
Like n-3 PUFA, AA had no effect on
IK1 (Fig.
8A,
left). In contrast to n-3 PUFA, AA
markedly increased the steady-state current,
Isus (Fig.
8A, right). Values of the current at the
end of the 200-ms step were normalized to the value of the current in
control in response to a voltage step to +30 mV for each cell
(n = 5) and are plotted as a function
of clamp voltage in Fig. 8B. AA (50 µM) increased Isus by ~80%
within 10 min. There was an 80% increase in
Isus regardless
of the test potential (30 to +60 mV).
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control)
after 5 µM AA addition. In contrast with longer-term effects (>3
min), earlier traces of the difference currents have a component with
kinetics similar to
Ito. Note that 5 µM AA decreases
Ito within 2 min
without an effect on
Isus. Application
of 5 µM AA for >3 min induced an increase in
Isus. Similarly,
the inhibitory effect of 50 µM AA on
Ito was visible only during the first 90 s after AA application (arrows in Fig. 9B); it was subsequently hidden by
the marked increase in
Isus.
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DISCUSSION |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Apkon and Nerbonne (1) reported that there are two K+ current components that contribute to the total depolarization-activated outward currents in adult rat ventricular myocytes: 1) a 4-AP-sensitive current that activates and inactivates rapidly on depolarization (Ito) and 2) a TEA-sensitive component that, after a delay, activates slowly to a steady level (Isus). The results presented here in adult rat ventricular myocytes reveal that at low concentrations (5 and 10 µM), Ito is suppressed by both n-3 and n-6 PUFAs and that this depression is mediated by both a decrease in Ito amplitude and an apparent acceleration of Ito decay. This suppression cannot be attributed to the action of cyclooxygenase metabolites, because a cyclooxygenase inhibitor, indomethacin, did not prevent this effect. We also observed similar results in experiments with cardiomyocytes isolated from dog ventricle, where 10 µM DHA completely abolished the Ito current (Bogdanov, unpublished observation). The application of PUFAs (5-50 µM) to cells pretreated with 4-AP (Ito blocker) had no effect on K+ currents. This further supports the interpretation that PUFAs at micromolar concentrations affect Ito current in rat ventricular myocytes.
At high concentrations (20 and 50 µM) all PUFAs except AA inhibited the slowly activating K+ current, Isus, in whole cell recordings of rat ventricular cells. This result is in accordance with a report by Honore et al. (13) that DHA (30 µM) blocks the cardiac delayed rectifier K+ channel (Kv1.5) and whole cell K+ currents in neonatal mouse and rat cardiomyocytes. To determine whether fatty acid blockade of the Kv1.5 channel occurred from the intracellular or the extracellular side of the membrane, Honore et al. (13) filled pipettes with the PUFAs and found no effect of fatty acids applied from inside. However, this null effect in their experiments might be the result of limited diffusion from the pipette to the cell interior because of sticking of the PUFA to the glass and high light sensitivity of the PUFAs. In contrast to our results, Honore et al. (13) also observed an inhibition of Isus by 30 µM AA. The reason for this discrepancy is not clear. Molecular studies (9) reveal at least five subunit messages in adult rat heart (Kv1.2, Kv1.4, Kv1.5, Kv2.1, and Kv4.2). However, the relationship between the expression of these subunits and the functional properties of K+ channels in vivo is unknown, although it has been suggested (9) that the Kv4.2 subunit contributes to the Ito in adult rat ventricular myocytes.
However, the significance of our data obtained after direct exposure of free PUFAs to cells, as in the present study, is unclear because PUFAs incorporated into phospholipids of the membrane bilayer may have different effects on ionic channels (10, 12) than do free fatty acids. Also, concentrations of free fatty acids >20 µM can contain micelles and can cause various nonspecific effects, such as detergent effects, on ion channels (32). Therefore, the inhibition of Isus observed after application of 20 and 50 µM PUFA (see Figs. 5 and 6), in principle, could be caused by the detergent effects of the PUFAs.
The present study demonstrates similarities and also significant differences in the effects of AA and other PUFAs tested on outward K+ currents. Like all PUFAs, AA initially depressed Ito. However, after 3 min, micromolar concentrations of AA began to increase the steady-state outward K+ current, Isus. The results suggest that the AA-induced noninactivating K+ current seems to be Ito with no or very slow inactivation kinetics. In adult rat ventricular cells, the AA-activated K+ current, IK,AA, was found by Kim and Duff (18). They proposed that AA in micromolar concentrations can cause activation of IK,AA in heart cells, altering the gating properties of an existing K+ channel. Our data suggest that the K+ channel affected by AA could be the Ito channel. Pronounced voltage dependence of the AA-induced noninactivating K+ current (see Fig. 8B) can be considered as evidence that the current is not the voltage-independent K+ current found by Kim and Clapham (17) in neonatal atrial cells.
Damron et al. (8) also observed an inhibition of Ito in rat cardiomyocytes after application of 50 µM AA. However, they did not report a delayed increase in Isus as described in the present study. This apparent discrepancy could be explained by differences in voltage clamp technique (perforated patch vs. classic whole cell method in our experiments). The effect of AA to increase Isus is likely caused by an action of AA metabolites, because the nonmetabolizable analog of AA, ETYA (see Fig. 11), inhibited both Ito and Isus. A faster rate of biosynthesis of eicosanoids from the AA and their stronger activity than those formed from other PUFAs (19) could be possible causes of the AA effect found in present study. It is also possible that the conditions of Damron et al. (8) did not permit the metabolism of AA or that in our whole cell experiments soluble factors, such as protein kinases A and C, that regulate the cardiac K+ channel (29) were washed out.
Although the function of Ito is not fully understood, in most mammalian tissues including human, dog, rabbit, ferret, and rat ventricle (1, 3, 11, 20, 30) it is one of the currents that underlie repolarization of the action potential. In addition, Ito, because of its nonuniform distribution across the myocardium, can play an important role contributing to the heterogeneity of myocardial repolarization. Previous data had shown that Ito is significantly greater in myocytes from epicardial regions than in endocardial myocytes (20, 30). This electrical heterogeneity is intensified during ischemia and may facilitate the development of reentrant arrhythmias in epicardium (20). The accumulation of AA occurs early during myocardial ischemia and has been estimated to be between 20 and 40 µM in the dog after 1 h of ischemia (6). Thus the concentrations of AA used in this study (5-50 µM) may be similar to those observed in ischemic myocardial tissue. It has been suggested that selective blockade of Ito (e.g., by 4-AP or all PUFAs except AA) may be a useful antiarrhythmic intervention. Experimental results obtained by Tsuchihashi and Curtis (28) also support this hypothesis.
A beneficial effect of long-chain n-3 PUFAs from fish oil on cardiac
performance has been well recognized (see Ref. 19 for review). Recent
studies by McLennan et al. (21) demonstrate an important role for fish
oil PUFAs in the prevention of fatal ventricular arrhythmias. Billman
et al. (2) also observed that infusion of 
-3 PUFA in dogs could
prevent ventricular fibrillations occurring in response to acute
occlusion of a coronary artery. The present results in rat and those in
dog (Bogdanov, unpublished observation) ventricular cells support the
hypothesis that the antiarrhythmic effects of the fish oil PUFAs in
situ may be related in part to the inhibition of
Ito and
Isus.
Kang et al. (15) found that the n-3 PUFAs (DHA and EPA) decrease the action potential duration of neonatal rat cardiac myocytes. This result conflicts with data obtained by us in experiments on adult rat cardiomyocytes (see Fig. 7). However, Kilborn and Fedida (16) reported that the contribution of the transient versus sustained currents to the total outward K+ current in rat ventricle was age dependent. They observed a fourfold increase in Ito from neonatal to adult age in rat cells, indicating that Ito appears to play a major role in repolarization of adult but not neonatal ventricular action potentials. No differences were observed in the kinetic properties of Ito (16). Thus the shortening of the action potential in neonatal rat cardiomyocytes caused by 10 µM EPA (15) could be explained by the very small amplitude of the Ito in these cells and by an inhibitory effect of the PUFAs on ICa (Bogdanov, unpublished observation).
Large-conductance channels predominantly permeable to Cl ions are
present in cardiac plasma membranes of the newborn rat heart cells (7).
Therefore, in principle, a part of the effect of PUFAs on outward
currents observed could be caused by an action on
Cl
current. However, a
reversal potential
(Erev) for a
putative Cl current in our
experiments in adult rat cells should be positive (as a result of 110 mM Cl inside vs. 6 mM outside), about +75 mV. In contrast, as indicated
by Figs. 4 and 8B, the current-voltage relationships show a negative
Erev for the
currents affected by PUFAs, suggesting that PUFAs affected
K+ currents rather than
Cl currents.
As shown in Fig. 7, 20 µM EPA blocked excitation of the cell and this result is in agreement with data by Xiao et al. (31), in which the blocking effect of PUFAs on Na+ channels was demonstrated in neonatal rat ventricular cells. A prior study (24) failed to observe a significant effect of 5 µM AA or DHA on Ca2+ current (ICa) amplitude in adult rat ventricular cells. However, other recent studies (Y.-F. Xiao, J. X. Kang, J. P. Morgan, and A. Leaf, personal communication) have shown effects of low concentrations of PUFAs on both ICa and Isus. Further study is required to determine why the potency of the PUFA effect on specific ion channels differs among these studies.
In summary, we conclude that at low concentrations (5 and 10 µM) both n-3 and n-6 PUFAs inhibit Ito current in adult rat cardiac myocytes and this lengthens the action potential. Higher concentrations of PUFAs (20 and 50 µM) further inhibited Ito and also inhibited Isus and ICa. However, our results indicate that noninactivating outward K+ current, Isus, is also augmented by AA metabolites. Thus the overall effect of AA on action potential repolarization is determined by the overall net effect, which likely varies with the cellular metabolic state. It is presently unknown whether results obtained in experiments with direct application of free fatty acids can be used to study the beneficial effects of diet enriched with PUFAs.
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FOOTNOTES |
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Address for reprint requests: E. G. Lakatta, Laboratory of Cardiovascular Science, Gerontology Res. Ctr., NIA, 4940 Eastern Ave., Baltimore, MD 21224.
Received 26 November 1996; accepted in final form 29 October 1997.
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REFERENCES |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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1.
Apkon, M.,
and
J. M. Nerbonne.
Characterization of two distinct depolarization-activated K+ currents in isolated adult rat ventricular myocytes.
J. Gen. Physiol.
97:
973-1011,
1991
2.
Billman, G. E.,
H. Hallaq,
and
A. Leaf.
Prevention of ischemia-induced ventricular fibrillation by n-3 fatty acids.
Proc. Natl. Acad. Sci. USA
91:
4427-4430,
1994
3.
Campbell, D. L.,
R. L. Rasmusson,
Y. Qu,
and
H. C. Strauss.
The calcium-independent transient outward potassium current in isolated ferret right ventricular myocytes. I. Basic characterization and kinetic analysis.
J. Gen. Physiol.
101:
571-601,
1993
4.
Capogrossi, M.,
A. Kort,
H. Spurgeon,
and
E. Lakatta.
Single adult rabbit and rat cardiac myocytes retain the Ca- and species-dependent systolic and diastolic contractile properties of intact muscle.
J. Gen. Physiol.
88:
589-613,
1986
5.
Chadwick, C. C.,
A. M. Ezrin,
B. O'Connor,
W. A. Volberg,
D. I. Smith,
K. J. Wedge,
R. J. Hill,
G. M. Briggs,
E. D. Pagani,
P. J. Silver,
and
D. S. Krafte.
Identification of a specific radioligand for the cardiac rapidly activating delayed rectifier K+ channel.
Circ. Res.
72:
707-714,
1993
6.
Chien, K. R.,
A. Han,
A. Sen,
L. M. Buja,
and
J. T. Willerson.
Accumulation of unesterified arachidonic acid in ischemic canine myocardium.
Circ. Res.
54:
313-322,
1984
7.
Coulombe, A.,
H. Duclohier,
E. Coraboeuf,
and
N. Touzet.
Single chloride-permeable channels of large conductance in cultured cardiac cells of new-born rats.
Eur. Biophys. J.
14:
155-162,
1987[Medline].
8.
Damron, D.,
D. Van Wagoner,
C. Moravec,
and
M. Bond.
Arachidonic acid and endothelin potentiate Ca transients in rat cardiac myocytes via inhibition of distinct K+ channels.
J. Biol. Chem.
268:
27335-27344,
1993
9.
Dixon, J. E.,
and
D. McKinnon.
Quantitative analysis of potassium channel mRNA expression in atrial and ventricular muscle of rats.
Circ. Res.
75:
252-260,
1994
10.
Durot, I.,
A. Fournier,
P. Athias,
and
A. Grynberg.
Effect of phospholipid content in long chain polyunsaturated fatty acids on rat cardiomyocyte function (Abstract).
J. Mol. Cell. Cardiol.
27:
A450,
1995.
11.
Giles, W. R.,
and
Y. Imaizumi.
Comparison of potassium currents in rabbit atrial and ventricular cells.
J. Physiol. (Lond.)
405:
123-145,
1988
12.
Gulch, R. W., C. Ross, A. Weible, and R. Jacob.
Influence of oil diets on mechanical and electrophysiological
properties of the heart (Abstract). Pflügers
Arch. 350, Suppl.:
R97, 1994.
13.
Honore, E.,
J. Barhanin,
B. Attali,
F. Lesage,
and
M. Lazdunski.
External blockade of the major cardiac delayed-rectifier K+ channel (Kv1.5) by polyunsaturated fatty acids.
Proc. Natl. Acad. Sci. USA
91:
1937-1944,
1994
14.
Josephson, I. R.,
J. Sanches-Chapula,
and
A. M. Brown.
Early outward current in rat ventricular cells.
Circ. Res.
54:
157-162,
1984
15.
Kang, J. X.,
Y.-F. Xiao,
and
A. Leaf.
Free, long-chain, polyunsaturated fatty acids reduce membrane electrical excitability in neonatal rat cardiac myocytes.
Proc. Natl. Acad. Sci. USA
92:
3997-4001,
1995
16.
Kilborn, M. J.,
and
D. Fedida.
A study of the developmental changes in outward current of rat ventricular myocytes.
J. Physiol. (Lond.)
430:
37-60,
1990
17.
Kim, D.,
and
D. Clapham.
Potassium channels in cardiac cells activated by arachidonic acid and phospholipids.
Science
244:
1174-1179,
1989
18.
Kim, D.,
and
R. A. Duff.
Regulation of K+ channels in cardiac myocytes by free fatty acids.
Circ. Res.
67:
1040-1046,
1990
19.
Lands, W. E. M.
Biochemistry and physiology of n-3 fatty acids.
FASEB J.
6:
2530-2536,
1992[Abstract].
20.
Liu, D.-W,
G. A. Gintant,
and
C. Antzelevitch.
Ionic bases for electrophysiological distinctions among epicardial, midmyocardial, and endocardial myocytes from the free wall of the canine left ventricle.
Circ. Res.
72:
671-687,
1993
21.
McLennan, P. L.,
T. M. Bridle,
M. Y. Abeywardena,
and
J. S. Charnock.
Dietary lipid modulation of ventricular fibrillation threshold in the marmoset monkey.
Am. Heart J.
123:
1555-1561,
1992[Medline].
22.
Needleman, P.,
J. Turk,
B. A. Jakschik,
A. R. Morrison,
and
J. B. Lefkowith.
Arachidonic acid metabolism.
Annu. Rev. Biochem.
55:
69-102,
1986[Medline].
23.
Oxford, G. S.,
and
P. K. Wagoner.
The inactivating K+ current in GH3 pituitary cells and its modification by chemical reagents.
J. Physiol. (Lond.)
410:
587-612,
1989
24.
Pepe, S.,
K. Bogdanov,
H. Hallaq,
H. Spurgeon,
A. Leaf,
and
E. Lakatta.
Omega-3 polyunsaturated fatty acid modulates dihydropyridine effects on L-type Ca channels, cytosolic Ca, and contraction in adult rat cardiac myocytes.
Proc. Natl. Acad. Sci. USA
91:
8832-8836,
1994
25.
Rouzaire-Dubois, B.,
and
J. M. Dubois.
Modification of electrophysiological and pharmacological properties of K channels in neuroblastoma cells induced by the oxidant chloramine-T.
Pflügers Arch.
416:
393-397,
1990[Medline].
26.
Shibata, E. F.,
T. Drury,
H. Refsum,
V. Aldrete,
and
W. Giles.
Contributions of a transient outward current to repolarization in human atrium.
Am. J. Physiol.
257 (Heart Circ. Physiol. 26):
H1773-H1781,
1989
27.
Tande, P. M.,
H. Bjornstadt,
T. Yang,
and
H. Refsum.
Rate-dependent class III antiarrhythmic action, negative chronotropy, and positive inotropy of a novel IK blocking drug, UK-68, 798: potent in guinea pig but no effect in rat myocardium.
J. Cardiovasc. Pharmacol.
16:
401-410,
1990[Medline].
28.
Tsuchihashi, K.,
and
M. Curtis.
Influence of tedisamil on initiation and maintenance of ventricular fibrillation: chemical defibrillation by Ito blockade?
J. Cardiovasc. Pharmacol.
18:
445-456,
1991[Medline].
29.
Walsh, K. B.,
and
R. S. Kass.
Regulation of a heart potassium channel by protein kinase A and C.
Science
242:
67-69,
1988
30.
Wettwer, E.,
G. J. Amos,
H. Posival,
and
U. Ravens.
Transient outward current in human ventricular myocytes of subepicardial and subendocardial origin.
Circ. Res.
75:
473-482,
1994
31.
Xiao, Y.-F,
J. X. Kang,
J. P. Morgan,
and
A. Leaf.
Blocking effects of polyunsaturated fatty acids on Na+ channels of neonatal rat ventricular myocytes.
Proc. Natl. Acad. Sci. USA
92:
11000-11004,
1995
32.
Yamada, M.,
A. Terzic,
and
Y. Kurachi.
Regulation of potassium channels by G-protein subunits and arachidonic acid metabolites.
Methods Enzymol.
238:
394-422,
1994[Medline].
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