Vol. 279, Issue 5, H2095-H2103, November 2000
Fast pacing facilitates discontinuous action potential
propagation between rabbit atrial cells
Yang-Gan
Wang,
Mary B.
Wagner,
Rajiv
Kumar,
William N.
Goolsby, and
Ronald W.
Joyner
Todd Franklin Cardiac Research Laboratory, Children's Heart
Center, Department of Pediatrics, Emory University School of
Medicine, Atlanta, Georgia 30322
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ABSTRACT |
We examined the critical coupling
conductance (GC) for propagation at different
pacing cycle lengths (CLs) (1,000 and 400 ms). As
GC was progressively reduced, propagation failed
at a CL of 1,000 ms, whereas propagation succeeded at a CL of 400 ms over a range of GC values before failing at a CL
of 400 ms at a lower GC, showing facilitation of
propagation at the shorter CL. Critical GC was
(means ± SE) 0.8 ± 0.1 nS for a CL of 400 ms and
1.3 ± 0.1 nS for a CL of 1,000 ms (a 63% increase,
P < 0.002, n = 9 cell pairs). In 14 uncoupled cells, action potential duration at 30% repolarization
(APD30) increased from 19.9 ± 2.5 to
41.8 ± 2.6 ms (P < 0.001) as CL decreased from
1,000 to 400 ms. In five cell pairs, critical GC
with 4-aminopyridine (4-AP) was reduced to 0.4 ± 0.1 nS at a CL
of 1,000 ms (P < 0.05 compared with control solution),
and critical GC in 4-AP was unchanged by
decreasing CL to 400 ms. It is possible that the "remodeling" of
atrial cells due to atrial fibrillation or tachycardia, which has been
shown to produce a decrease in the transient outward current, may
result in an enhanced ability to propagate, possibly facilitating
further development of fibrillation under conditions of decreased
cellular coupling.
electrophysiology; heart; arrhythmias
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INTRODUCTION |
ATRIAL
ARRHYTHMIAS FREQUENTLY OCCUR either with or without a preexisting
myopathy associated with atrial dilatation from ventricular disease or
valvular dysfunction (4, 22). In the National Institutes
of Health-sponsored Cardiovascular Health Study of 5,201 people over
the age of 60 yr, 4.8% of women and 6.2% of men had atrial
fibrillation (4). In studies of atrial arrhythmias (11, 12, 19, 26), there has been a considerable emphasis on the complex three-dimensional anatomic structure of the atrium in
which many regions of slowed conduction, which may be discontinuous, have been described. There is also a well-known frequency dependence of
the initiation of atrial fibrillation with atrial tachycardia, perhaps
associated with atrioventricular reentry, "degenerating" into atrial fibrillation (20). Lesh et al.
(17) discussed the importance of discontinuous conduction
in many clinical atrial arrhythmias, identifying the crista terminalis
(CT) as a major factor in both reentrant and focal arrhythmias,
primarily due to its marked electrical anisotropy (21).
Recent work (19) has shown that the CT and eustachian
ridge may form the posterior barrier in human atrial flutter. In normal
atria, the CT has poor transverse coupling, but in patients with
flutter, there is nearly complete uncoupling (either congenital or
acquired) along the length of the CT. Atypical flutter may only use a
portion of the CT to form the line of block, and these lines of block
may be partly functional and develop at faster rates. Focal atrial
arrhythmias are also likely to arise from the CT because the poor
coupling protects an ectopic focus from the surrounding electrotonic
influences of the quiescent atria, which would tend to suppress the
automaticity. Kalman et al. (15) found that 14 of 18 focal
right atrial tachycardias arose from the CT, with fractionated
electrograms indicating discontinuous conduction. Atrial fibrillation
may result from several different mechanisms, including rapid focal
activity that cannot propagate in a 1:1 fashion to the atria or rapid
reentry around multiple uncoupled regions. The CT may be a region of
uncoupling around which the reentrant wave may circulate. Spach et al.
(25) demonstrated that premature stimuli produced
unidirectional block and microreentry in isolated nonuniformly
anisotropic human atrial trabeculae from older patients but
smooth propagation in trabeculae from younger patients, and similar
results in vivo have been reported (17). There may be a
spectrum of the degree and extent of discontinuous conduction so that
typical atrial flutter occurs with uncoupling along the entire CT and
eustachian ridge, paroxysmal "flutter/fib" may occur with only a
small portion of the CT having discontinuous conduction, and very fine
atrial fibrillation may occur at the cellular level with cell-to-cell
uncoupling distributed through many regions of the atrium, allowing
multiple wavelets to exist (17).
A coupling clamp technique (see Refs. 27 and 28) allows the electrical
coupling of real isolated heart cells with a controlled value of
coupling conductance (GC). When two cells are
coupled with a relatively low GC, the conduction
delay between the two cells becomes prolonged and is described as
discontinuous conduction. The action potential shape of atrial
cells is fundamentally different from that of ventricular cells,
particularly due to the presence of a rapid early repolarization in
atrial cells, which is largely produced by the activation of a
transient outward current (Ito) (5). We (14, 27) showed previously that the
amplitude of the early plateau was important in ventricular cells in
allowing discontinuous conduction because the membrane potential during this early plateau supplies the current for charging the distal cell(s). Because the Ito of atrial cells has
been shown to be frequency dependent, with less
Ito at higher frequencies of pacing, we
hypothesized that at increased pacing frequencies, a pair of atrial
cells would have successful propagation at values of
GC that did not allow successful propagation at
lower pacing frequencies.
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METHODS |
Cell isolation and electrodes.
Single atrial myocytes were prepared from adult New Zealand White
rabbits weighing 2.5-3.5 kg. The rabbits were anesthetized using
50 mg/kg iv pentobarbital sodium and 500 U iv heparin, the heart was rapidly extracted via thoracotomy with artificial
respiration, and the aorta was cannulated for Langendorff perfusion.
Single cells were isolated according to the methods described
previously by Hancox et al. (8). Briefly, the cannulated
heart was perfused sequentially at 37°C with base solution + 750 µM CaCl2 for 5 min, base solution + 100 µM EGTA
for 5 min, and base solution + 240 µM CaCl2 + enzyme for 5 min (see Solutions). The interatrial septum was
then excised, cut into thin strips, and further digested in the
recirculated enzyme solution used above for 6 min. Cells were isolated
by triturating the tissue strips and were then placed in a potassium
glutamate solution for 1 h at room temperature.
The cells were placed in a chamber that was continuously perfused with
Tyrode solution at 2 ml/min and that always maintained the temperature
at 35 ± 0.5°C. The pipettes were pulled from borosilicate glass
and, after fire polishing, had resistances of 3-4 M
when filled
with the internal solution. High-resistance seals were formed
with the cell membrane by applying light suction, and the membrane was
disrupted by applying transient suction. The junctional potential was
corrected by zeroing the potential before the pipette tip touched the
cell membrane.
Solutions.
The base solution contained (in mM) 130 NaCl, 4.5 KCl, 3.5 MgCl2, 0.4 NaH2PO4, 5 HEPES, and 10 dextrose at pH 7.25. The enzyme solution contained 1 mg/ml collagenase
(type IIA, Worthington), 0.07 mg/ml protease (type XIV, Sigma), and
base solution + 240 µM CaCl2. The potassium
glutamate solution had (in mM) 100 potassium glutamate, 25 KCl, 10 KH2PO4, 0.5 EGTA, 1 MgSO4, 20 taurine, 5 HEPES, and 10 dextrose at pH 7.2. The normal Tyrode solution
contained (in mM) 148.8 NaCl, 4 KCl, 1.8 CaCl2, 0.53 MgCl2, 0.33 NaH2PO4, 5 HEPES, and 5 dextrose at pH 7.4. The internal solution was composed of (in mM) 135 KCl, 5 disodium creatine phosphate, 5 MgATP, and 10 HEPES at pH 7.2.
Electrical coupling of atrial cell pairs.
Suguira and Joyner (27) developed an electrical circuit
that can provide a variable GC between two
isolated myocytes that are not actually in contact with each other. We
define V1 as a time-varying membrane potential
of cell 1 and V2 as a time-varying membrane potential of cell 2. If the two cells were coupled
together by an intercellular conductance GC,
there would be a time-varying current (IC)
flowing from cell 1 to cell 2 given by
IC = (V1 
V2) × GC. We used a
500-MHz Pentium III PC computer (Gateway) with a fast analog-to-digital
and digital-to-analog (Digidata 1200, Axon Instruments, Foster City,
CA) system to compute the value of IC from the
sampled values of V1 and
V2 and a selected value of
GC at time intervals of less than 80 µs. This value of IC is then added to
cell 2 and subtracted from cell 1 (added with a
negative sign) to produce the effect of the desired value of GC. Stimulation current pulses of a 2-ms
duration are also added to cell 1 and/or cell 2 at defined cycle lengths. Membrane potentials were recorded with an
Axoclamp 2A dual amplifier (Axon Instruments) in the current clamp mode
as previously described (27), using the internal
voltage-to-current converters to feed back the desired currents to each
headstage. Series resistance was carefully compensated by internal
bridge balance adjustments after recording of the membrane potential
was established.
Statistical analysis.
Statistical analysis was performed with SigmaStat for Windows (Jandel
Scientific). Statistical significance was determined by Student's
t-test. P values <0.05 were regarded as
significant. Data are presented as means ± SE in the text.
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RESULTS |
To examine the propagation of action potentials between two atrial
cells at two different cycle lengths (CLs) for stimulation, we followed
a protocol in which we established a certain value of
GC between two cells, paced one of the cells of
the cell pair repetitively for 15 stimulations at a CL of 1,000 ms,
followed by 25 stimulations at a CL of 400 ms, and then another 10 stimulations at a CL of 1,000 ms. We subsequently changed the value of
GC and repeated the stimulation protocol. At
high levels of GC, we found that propagation was
successful for all cell pairs at both CLs. This phenomenon is
illustrated in Fig. 1, in which we show
membrane potential recordings from the stimulated cell (top)
and the follower cell (middle) and the coupling current
(lower) with GC = 1.0 nS. The
recordings show the last three stimulations at a CL of 1,000 ms, 25 stimulations at a CL of 400 ms, and the first four stimulations after
the return to a CL of 1,000 ms. All of the action potentials are
propagated successfully, but a closer examination of the action potential properties shows some significant differences at the two
values of CL. Figure 2
(top) shows, at a faster time scale, the action
potentials of the leader cell (V1) and the
follower cell (V2) for the action potentials at
the last stimulation at a CL of 1,000 ms and the 13th stimulation at a
CL of 400 ms of Fig. 1. For the leader cell, the action
potential amplitude is nearly the same for the two values of CL, but
the early repolarization occurs much more quickly at a CL of 1,000 ms
than at a CL of 400 ms. The slowed early repolarization at a CL of 400 ms produces a greater voltage difference between the leader cell and
the follower cell during the propagation process. As shown in Fig. 2
(bottom), which plots the coupling current (positive in the
direction from the leader cell to the follower cell), the peak value of
coupling current is the same at the two values of CL, but the decline
in coupling current is much slower for a CL of 400 ms. Thus the charge transferred from the leader cell to the follower cell (the time integral of the coupling current), which produces the depolarization of
the follower cell, occurs more quickly at a CL of 400 ms than at a CL
of 1,000 ms. Therefore, the conduction delay between the leader cell
and the follower cell is decreased.
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Fig. 1.
Recordings of membrane potential of the leader cell
(top) and the follower cell (middle) of an atrial
cell pair coupled with a coupling conductance
(GC) = 1.0 nS as the cycle length (CL) for
stimulation is changed from 1,000 to 400 ms and then back to 1,000 ms.
The data shown are the last three stimulations at a CL of 1,000 ms, 25 stimulations at a CL of 400 ms, and the first four stimulations after
the return to a CL of 1,000 ms. Bottom: coupling current
plotted as positive in the direction from the leader cell to the
follower cell. Each stimulation is a current pulse of 2 ms duration
applied to the leader cell. a and b, last
stimulation at CL of 1,000 ms and the 13th stimulation at a CL of 400 ms, respectively. Experiment 090199at, cell pair
a.
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Fig. 2.
Comparison of the action potentials of a and
b of Fig. 1 at a faster time base. The action potentials of
the leader cell (V1, solid lines) and the
follower cell (V2, dotted lines) are shown
superimposed (top). Horizontal dashed line, zero reference
line. Bottom: coupling current
[IC = GC × (V1 V2), where
GC = 1.0 nS and IC
is the coupling current] that was applied during the experiment as a
current added to the follower cell and subtracted from the leader cell
through the pipettes attached to the respective real cells.
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This effect occurs as soon as the CL is changed from 1,000 to 400 ms
and rapidly reverses when the CL is changed back to 1,000 ms, as shown
in Fig. 3. Figure 3 (top)
shows the action potential duration at 30% repolarization
(APD30) values for the leader cell for the last
three action potentials at a CL of 1,000 ms, 25 stimulations at a CL of
400 ms, and the first three stimulations after the return to a CL of
1,000 ms. Note that the APD30 is increased for all of the
stimulations at the shorter CL. Figure 3 (bottom) shows the
conduction delay (the difference in activation times for the follower
cell and the leader cell) for the same stimulations, with a decreased
conduction delay for all of the stimulations at a CL of 400 ms compared
with a CL of 1,000 ms.
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Fig. 3.
Analysis of the data plotted in Fig. 1. Top: time from
the upstroke of the action potential to the occurrence of 30%
repolarization back to the resting potential (APD30) of the
leader cell for the last three action potentials at a CL of 1,000 ms,
25 action potentials at a CL of 400 ms, and the first three action
potentials after the switch back to a CL of 1,000 ms.
Bottom: conduction delay (the elapsed time from the upstroke
of the leader cell to the upstroke of the follower cell) for the same
action potentials.
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The shorter conduction delay at a CL of 400 ms compared with a CL of
1,000 ms suggests that conduction is facilitated at the shorter value
of CL. As we decreased GC from 1.0 to 0.9 nS and repeated the same protocol on the same cell pair, we got the results shown in Fig. 4. The last three
stimulations at a CL of 1,000 ms all show conduction failure, as
indicated by the full amplitude action potential in the leader cell
(top) and the much smaller passive response in the follower
cell (middle). However, all of the stimulations at a CL of
400 ms show successful propagation from the leader cell to the follower
cell. The effects of the changes in CL are not instantaneously
manifested. Note that the first two action potentials after the return
to a CL of 1,000 ms show propagation, although the third and fourth
action potentials after this transition fail to propagate, as did the
subsequent action potentials at this CL (data not shown). There is also
a gradual transition in the propagation characteristics when CL is
changed from 1,000 to 400 ms, as illustrated in Fig.
5. In Fig. 5, the membrane potential of
the leader cell and the follower cell are plotted along with the
corresponding coupling current. The first stimulation shown is the last
of the stimulations at a CL of 1,000 ms, followed by the first three
stimulations at a CL of 400 ms. Note that the first stimulation shown
results in propagation failure, and thus the coupling current is
entirely positive (flowing from the leader cell to the follower cell). For the subsequent three stimulations, there is propagation success, and the coupling current has a reversal of direction resulting in both
a positive and negative phase. Interestingly, the APD30 of
the action potential of the follower cell progressively increases for
each successful activation. Because the follower cell was not activated
during the period of a CL of 1,000 ms, it has a large
Ito (and thus a very rapid early repolarization)
for the first successful propagation. Ito
decreases over several successful activations, resulting in a gradual
increase in APD30 until a steady state is reached. Figure
6 shows the transition from a CL of 400 ms to a CL of 1,000 ms at GC = 0.9 nS. For
this figure, the first stimulation shown is the last stimulation at a
CL of 400 ms, followed by the first three stimulations after the return to a CL of 1,000 ms. The three stimulations at a CL of 1,000 ms show a
progressive prolongation of conduction time to conduction failure for
the third stimulation at a CL of 1,000 ms as the APD30 of
the follower cell progressively decreases.
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Fig. 4.
Recordings of membrane potential of the leader cell
(top) and the follower cell (middle) of the same
atrial cell pair as for Fig. 1 but now coupled with
GC = 0.9 nS as the CL for stimulation is
changed from 1,000 to 400 ms and then back to 1,000 ms. The data shown
are the last three stimulations at a CL of 1,000 ms, 25 stimulations at
a CL of 400 ms, and the first four stimulations after the return to a
CL of 1,000 ms. Bottom: coupling current plotted as positive
in the direction from the leader cell to the follower cell. *Successful
propagation of the first 2 action potentials after the switch back to a
CL of 1,000 ms.
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Fig. 5.
Replotting of the data of Fig. 4 at a faster time base for the
transition from a CL of 1,000 ms to a CL of 400 ms. Top:
superimposed membrane potentials of the leader cell (solid line) and
the follower cell (dotted line). Bottom: coupling current
for the last stimulation at a CL of 1,000 ms followed by the first
three stimulations at a CL of 400 ms.
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Fig. 6.
Replotting of the data of Fig. 4 at a faster time base for the
transition from a CL of 400 ms to a CL of 1,000 ms. Top:
superimposed membrane potentials of the leader cell (solid line) and
the follower cell (dotted line). Bottom: coupling current
for the last stimulation at a CL of 400 ms followed by the first three
stimulations at a CL of 1,000 ms. *Successful propagation of the first
two action potentials after the switch back to CL of 1,000 ms (as in
Fig. 4).
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As we further reduced GC for this cell pair,
repeating the protocol, we found that propagation was successful at a
CL of 400 ms at a GC value as low as 0.65 nS but
failed at GC = 0.6 nS, as illustrated in
Fig. 7. Figure 7 (top) shows
the membrane potential for the leader cell and the follower cell during
steady-state propagation at a CL of 400 ms, with each stimulation
producing successful propagation. Figure 7 (bottom) shows a
recording from the same time period at a CL of 400 ms stimulation for
GC = 0.6 nS, showing that each stimulation
now results in failure of propagation. In nine cell pairs, the mean
value of critical GC for successful propagation
decreased from 1.3 ± 0.1 nS at a CL of 1,000 ms to 0.8 ± 0.1 nS at a CL of 400 ms (P < 0.002). Compared with
the critical GC at a CL of 400 ms, the increase
in CL to 1,000 ms required a 63% increase in the critical value of
GC required for propagation, demonstrating that
conduction was facilitated at a CL of 400 ms compared with that at a CL
of 1,000 ms.
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Fig. 7.
Recordings from the same cell pair as in Fig. 1 at a CL of 400 ms
at GC = 0.65 nS (top, successful
propagation) and GC = 0.6 nS
(bottom, failure of propagation). For each part, the leader
cell is plotted as the solid line and the follower cell is plotted as a
dotted line.
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The increase in APD30 by shortening the CL is not produced
by the propagation process. This is illustrated in Fig.
8 (top), which shows the
membrane potential for a single isolated atrial cell in which the
stimulus CL is changed from 1,000 to 400 ms. The data plotted show the
last stimulation at a CL of 1,000 ms and the first three stimulations
at a CL of 400 ms. The APD30 of the action potentials is
closely approximated by the time that each action potential is above
the 0 mV line and this is clearly increased at the short CL value. When
we exposed this cell to 2 mM 4-AP to block Ito
and repeated the stimulation protocol, we obtained the data shown in
Fig. 8 (bottom). The APD30 is clearly increased
at a CL of 1,000 ms [compared to the control solution, Fig. 8
(top)] and is now not further increased by switching the CL
to 400 ms. When we analyzed APD30 for isolated atrial cells (no coupling) at a CL of 1,000 and 400 ms, we found an increase in
APD30 in the control solution from 19.9 ± 2.5 to
41.8 ± 2.5 ms (an increase of 110%, n = 14, P < 0.001). In the 2 mM 4-AP solution, the mean
APD30 values were 60.9 ± 5.2 ms (CL of 1,000 ms,
n = 12, P < 0.001 compared with a CL
of 1,000 ms in control solution) and 62.8 ± 5.7 ms
(n = 12, CL of 400 ms, not significantly different from
the APD30 values at a CL of 1,000 ms in 4-AP).
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Fig. 8.
Effects of 4-aminopyridine (4-AP) on the action potential shape as
CL is changed from 1,000 to 400 ms for an uncoupled isolated atrial
cell. Top: transition in the control solution.
Bottom: transition after addition of 2 mM 4-AP to the
external solution. Experiment 050400at, cell pair
a.
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These results with 4-AP suggested that propagation for cell pairs in
the 4-AP solution would have a lower critical GC
and show less frequency dependence of propagation success than those in
the control solution. This is illustrated in Fig.
9, which shows data from a coupled atrial
cell pair exposed to 2 mM 4-AP and stimulated at a CL of 1,000 ms.
Figure 9 (top) shows a transition from a CL of 1,000 ms to a
CL of 400 ms with GC = 0.4 nS, with all of
the stimulations of the leader cell followed by activation of the
follower cell at both values of CL. For the same cell pair, with
GC = 0.3 nS [Fig. 9 (bottom)],
failure of propagation occurs at a CL of 1,000 ms and at a CL of 400 ms. Thus the presence of 4-AP lowers the critical
GC for action potential conduction (in this case
to between 0.3 and 0.4 nS) compared with the control solution and
removes the frequency dependence of conduction. For five cell pairs
exposed to 2 mM 4-AP, the critical value of GC required to sustain conduction at a CL of 1,000 ms was 0.4 ± 0.1 nS (P < 0.05 compared with control solution, CL of
1,000 ms), and the critical GC in the 4-AP
solution was unchanged by decreasing CL to 400 ms.
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Fig. 9.
Action potential propagation (top,
GC = 0.4 nS) and failure of propagation
(bottom, GC = 0.3 nS) for a pair
of atrial cells in a solution with 2 mM 4-AP. In each panel, the leader
cell is plotted as a solid line and the follower cell is plotted as a
dotted line. Experiment 050200at, cell pair a.
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DISCUSSION |
Sugiura and Joyner (27) previously showed that for
discontinuous conduction in guinea pig ventricular cell pairs,
decreases of the stimulation CL from 500 ms to 400, 300, 200, 190, 180, and 160 ms could maintain consistent 1:1 discontinuous conduction from
cell 1 to cell 2, but the conduction delay
progressively increased as the CL was decreased and block occurred at
CL 130 ms as 2:1 conduction. Sugiura and Joyner (27) also
showed that 1 µM nifedipine significantly increased and isoproterenol
significantly decreased the delay between the activation of two coupled
cells at a given GC, suggesting that the primary
determination of the increased conduction delay at a shorter CL was the
residual inactivation of the L-type calcium current. In contrast to
these results with guinea pig ventricular cells, the present results
with rabbit atrial cells show a very different phenomenon with a change
in CL from 1,000 to 400 ms actually producing a shorter conduction delay and a greater safety factor (requiring less
GC) for conduction. One major difference in
these two cell types is the dominant effects of
Ito in atrial cells on the early repolarization
after the spike of the action potential. When the cycle length
decreases, Ito during the early repolarization
phase will decrease due to the incomplete recovery from inactivation.
This shifts the balance of membrane current during this phase toward
less outward current and thus slows this early repolarization phase,
increasing APD30 and allowing more current to flow from the
leader cell to the follower cell, which allows the follower cell to
more quickly reach its voltage threshold for action potential
initiation. This action decreases the conduction delay and facilitates
the propagation at short cycle lengths.
Numerous studies have demonstrated the variable magnitude of
Ito (5) in different species and in
different regions of the heart. Ito has been
recorded in a wide range of cardiac tissues, including ventricular
cells from the rat (31), ferret (2), dog
(18), and rabbit (9), atrial cells from the
rabbit (3) and dog (33), and atrial and
ventricular cells from humans (24, 34) and rabbits
(7), with variable densities and kinetics. Ito can also be altered in physiological and
pathophysiological conditions. For example, it has been shown that
Ito has differences in both density and kinetics
in human subendocardial versus subepicardial ventricular cells
(34). There are also age-related changes
(32), and alterations in pathological conditions such as
myocardial infarction or ischemia (13), cardiac
hypertrophy (29), terminal heart failure, and atrial
dilatation (1, 16). Interactions between coupled myocytes
during the early plateau phase were studied by Huelsing et al.
(10), showing that the greater Ito
magnitude of rabbit Purkinje cells compared with rabbit ventricular
cells produced an intrinsically more rapid repolarization of the
Purkinje cell and thus caused complex interactions during the early
repolarization period, but in these experiments the cells were
simultaneously stimulated such that propagation of the action potential
was not studied. Although many of these studies have focused on either the magnitude of the current or the duration of the action potentials, few previous studies have focused on the effects of
Ito on action potential propagation. Because
action potential propagation between two adjacent cardiac cells with
high levels of GC occurs with very short delays,
the activation of Ito does not play a role in
propagation under these conditions, because conduction occurs before
activation of Ito. However, the long delays
associated with discontinuous conduction (with lower levels of
GC) make early plateau currents, such as the
L-type calcium current and Ito, important
components of the propagation process.
Our findings may have implications for clinical arrhythmias under
pathophysiological conditions. In regions of the atrium with low
GC, some premature beats may be conducted with
decreased delay and require less GC. This could
facilitate the initiation of atrial arrhythmias because the premature
beat may be able to propagate along a pathway that was blocked for the
regular excitations, thus changing the spatial pattern of the
activation wavefront. Ito was found to be
substantially decreased in atrial cells from patients with atrial
fibrillation (30) and in ventricular cells from patients
with heart failure (1). The decreased
Ito in the atrial cells after atrial tachycardia
or fibrillation may actually facilitate action potential conduction at
regions of low GC and may encourage the
reinitiation of atrial tachycardia or fibrillation. In addition, the
lower Ito in human subendocardial compared with
subepicardial ventricular cells (34) and the decreased Ito after myocardial infarction or ischemia
(13) may be important in the initiation of the ventricular
action potential at Purkinje-ventricular junctions and may facilitate
ventricular discontinuous conduction.
The limitations of the study are the following. Our experiments were
performed with rabbit atrial cells. Although the ionic properties in
rabbit atrial cells are similar to human atrial cells, the
Ito recovery time course was found to be faster
in human atrial cells than in rabbit atrial cells (6).
Further experiments need to be done to understand whether this
frequency-dependent facilitation of propagation happens in human atrial
cells. Action potential propagation within any electrical syncytium,
even if well coupled, can be described at a microscopic level as
discontinuous because propagation across the gap junctions takes more
time than propagation across an equivalent length of cytoplasm within
the cell. However, the type of discontinuous conduction we are studying with our coupling clamp technique is specifically that found at regions
such as the Purkinje-ventricular junction or in postischemic tissue, in
which there is a clearly measurable delay (on the order of 4-30
ms) between the activations of closely adjacent groups of cells with
electrotonic prepotentials in the distal cells. At large values of
GC, in which the conduction delay between
adjacent cells becomes on the order of 1 ms or less, any process (such as the L-type calcium current or Ito) that
develops with a delay of several milliseconds after the upstroke of the
action potential cannot directly alter propagation, which we showed
experimentally with modulation of L-type calcium current by nifedipine
(27) and which has been shown theoretically with strand
simulations (23).
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ACKNOWLEDGEMENTS |
This work was partially supported by the National Heart, Lung, and
Blood Institute Grant HL-22562 (to R. W. Joyner), an American Heart Association Fellowship (to M. B. Wagner), and the Emory Egleston Children's Research Center.
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FOOTNOTES |
Address for reprint requests and other correspondence: R. W. Joyner, Dept. of Pediatrics, Emory Univ. School of Medicine, 2040 Ridgewood Dr. NE, Atlanta, GA 30322 (E-mail:
rjoyner{at}cellbio.emory.edu).
The costs of publication of this
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Received 7 January 2000; accepted in final form 18 May 2000.
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REFERENCES |
1.
Beuckelmann, DJ,
Nabauer M,
and
Erdmann E.
Alterations of K+ currents in isolated human ventricular myocytes from patients with terminal heart failure.
Circ Res
73:
379-385,
1993[Abstract/Free Full Text].
2.
Campbell, DL,
Rasmusson RL,
Qu Y,
and
Strauss HC.
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[Abstract/Free Full Text].
3.
Clark, RB,
Giles WR,
and
Imaizumi Y.
Properties of the transient outward current in rabbit atrial cells.
J Physiol (Lond)
405:
147-168,
1988[Abstract/Free Full Text].
4.
DiMarco, JP,
and
Prystowsky EN.
Atrial Arrhythmias: State of the Art. Armonk, NY: Futura, 1995.
5.
Escande, D,
Coulombe A,
Faivre J,
Deroubaix E,
and
Coraboeuf E.
Two types of transient outward currents in adult human atrial cells.
Am J Physiol Heart Circ Physiol
252:
H142-H148,
1987[Abstract/Free Full Text].
6.
Fermini, B,
Wang Z,
Duan D,
and
Nattel S.
Differences in rate dependence of transient outward current in rabbit and human atrium.
Am J Physiol Heart Circ Physiol
263:
H1747-H1754,
1992[Abstract/Free Full Text].
7.
Giles, WR,
and
Imaizumi Y.
Comparison of potassium currents in rabbit atrial and ventricular cells.
J Physiol (Lond)
405:
123-145,
1988[Abstract/Free Full Text].
8.
Hancox, JC,
Levi AJ,
Lee CO,
and
Heap P.
A method for isolating rabbit atrioventricular node myocytes which retain normal morphology and function.
Am J Physiol Heart Circ Physiol
265:
H755-H766,
1993[Abstract/Free Full Text].
9.
Hiraoka, M,
and
Kawano S.
Calcium-sensitive and insensitive transient outward current in rabbit ventricular myocytes.
J Physiol (Lond)
410:
187-212,
1989[Abstract/Free Full Text].
10.
Huelsing, DJ,
Spitzer KW,
Cordeiro JM,
and
Pollard AE.
Modulation of repolarization in rabbit Purkinje and ventricular myocytes coupled by a variable resistance.
Am J Physiol Heart Circ Physiol
276:
H572-H581,
1999[Abstract/Free Full Text].
11.
Jalife, J,
and
Gray RA.
Importance of the complex three-dimensional anatomic structure in propagation during atrial fibrillation.
In: Atrial Flutter and Fibrillation: From Basic to Clinical Applications, edited by Saoudi N,
Schoels W,
and El-Sherif N.. Armonk, NY: Futura, 1998, p. 17-33.
12.
Janse, MJ.
Why does atrial fibrillation occur (Review)?
Eur Heart J
18, Suppl C:
C12-C18,
1997.
13.
Jeck, CD,
Pinto JM,
and
Boyden PA.
Transient outward currents in subendocardial Purkinje myocytes surviving in the infarcted heart.
Circulation
92:
465-473,
1995[Abstract/Free Full Text].
14.
Joyner, RW,
Kumar R,
Wilders R,
Jongsma HJ,
Verheijck EE,
Golod DA,
van Ginneken AC,
Wagner MB,
and
Goolsby WN.
Modulating L-type calcium current affects discontinuous cardiac action potential conduction.
Biophys J
71:
237-245,
1996[Abstract/Free Full Text].
15.
Kalman, JM,
Olgin JE,
Fitzpatrick AP,
Lee R,
Epstein LM,
and
Lesh MD.
"Cristal tachycardia": Relationship of right atrial tachycardias to the crista terminalis identified using intracardiac echocardiography.
Pacing Clin Electrophysiol
18:
861-872,
1995.
16.
Le Grand, B,
Hatem S,
Deroubaix E,
Couetil JP,
and
Coraboeuf E.
Depressed transient outward and calcium currents in dilated human atria.
Cardiovasc Res
28:
548-556,
1994[ISI][Medline].
17.
Lesh, MD,
Kalman JM,
Olgin JE,
and
Ellis WS.
Role of discontinuous electrical propagation in clinical atrial arrhythmias: current evidence and future directions.
In: Discontinuous Conduction in the Heart, edited by Spooner PM,
Joyner RW,
and Jalife J.. Armonk, NY: Futura, 1997, p. 107-133.
18.
Litovsky, SH,
and
Antzelevitch C.
Transient outward current prominent in canine ventricular epicardium but not endocardium.
Circ Res
62:
116-126,
1988[Abstract/Free Full Text].
19.
Olgin, JE,
Kalman JM,
and
Fitzpatrick AP.
Role of right atrial endocardial structures as barriers to conduction during human type I atrial flutter. Activation and entrainment mapping guided by intracardiac echocardiography.
Circulation
92:
1839-1848,
1995[Abstract/Free Full Text].
20.
Prystowsky, EN.
Tachycardia-induced tachycardia: a mechanism of initiation of atrial fibrillation.
In: Atrial Arrhythmias: State of the Art, edited by DiMarco JP,
and Prystowsky EN.. Armonk, NY: Futura, 1995, p. 81-95.
21.
Saffitz, JE,
Kanter HL,
Green KG,
Tolley TK,
and
Beyer EC.
Tissue-specific determinants of anisotropic conduction velocity in canine atrial and ventricular myocardium.
Circ Res
74:
1065-1070,
1994[Abstract/Free Full Text].
22.
Saoudi, N,
Schoels W,
and
El-Sherif N.
Atrial Flutter and Fibrillation: From Basic to Clinical Applications. Armonk, NY: Futura, 1998.
23.
Shaw, RM,
and
Rudy Y.
Ionic mechanisms of propagation in cardiac tissue. Roles of the sodium and L-type calcium currents during reduced excitability and decreased gap junction coupling.
Circ Res
81:
727-741,
1997[Abstract/Free Full Text].
24.
Shibata, EF,
Drury T,
Refsum H,
Aldrete V,
and
Giles W.
Contributions of a transient outward current to repolarization in human atrium.
Am J Physiol Heart Circ Physiol
257:
H1773-H1781,
1989[Abstract/Free Full Text].
25.
Spach, MS,
Dolber PC,
and
Heidlage JF.
Influence of the passive anisotropic properties on directional differences in propagation following modification of the sodium conductance in human atrial muscle. A model of reentry based on anisotropic discontinuous propagation.
Circ Res
62:
811-832,
1988[Abstract/Free Full Text].
26.
Spach, MS,
Miler WT,
Dolber PC,
Kootsey JM,
Sommer JR,
and
Mosher CE.
The functional role of structural complexities in the propagation of depolarization in the atrium of the dog. Cardiac conduction disturbances due to discontinuities of effective axial resistivity.
Circ Res
50:
175-191,
1982[Free Full Text].
27.
Sugiura, H,
and
Joyner RW.
Action potential conduction between guinea pig ventricular cells can be modulated by calcium current.
Am J Physiol Heart Circ Physiol
263:
H1591-H1604,
1992[Abstract/Free Full Text].
28.
Tan, RC,
and
Joyner RW.
Electrotonic influences on action potentials from isolated ventricular cells.
Circ Res
67:
1071-1081,
1990[Abstract/Free Full Text].
29.
Tomita, F,
Bassett AL,
Myerburg RJ,
and
Kimura S.
Diminished transient outward currents in rat hypertrophied ventricular myocytes.
Circ Res
75:
296-303,
1994[Abstract/Free Full Text].
30.
Van Wagoner, DR,
Pond AL,
McCarthy PM,
Trimmer JS,
and
Nerbonne JM.
Outward K+ current densities and Kv1.5 expression are reduced in chronic human atrial fibrillation.
Circ Res
80:
772-781,
1997[Abstract/Free Full Text].
31.
Wahler, GM,
and
Dollinger SJ.
Time course of postnatal changes in rat heart action potential and in transient outward current is different.
Am J Physiol Heart Circ Physiol
267:
H1157-H1166,
1994[Abstract/Free Full Text].
32.
Wang, L,
and
Duff HJ.
Developmental changes in transient outward current in mouse ventricle.
Circ Res
81:
120-127,
1997[Abstract/Free Full Text].
33.
Wang, Z,
Fermini B,
and
Nattel S.
Mechanism of flecainide's rate-dependent actions on action potential duration in canine atrial tissue.
J Pharmacol Exp Ther
267:
575-581,
1993[Abstract/Free Full Text].
34.
Wettwer, E,
Amos GJ,
Posival H,
and
Ravens U.
Transient outward current in human ventricular myocytes of subepicardial and subendocardial origin.
Circ Res
75:
473-482,
1994[Abstract/Free Full Text].
Am J Physiol Heart Circ Physiol 279(5):H2095-H2103
0363-6135/00 $5.00
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