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Vol. 297, Issue 2, 753-761, May 2001
Department of Cardiology, Medical University Hospital Heidelberg, Heidelberg, Germany (D.T., G.W.-N., K.R., J.K.); and Rammelkamp Center for Education and Research, MetroHealth Medical Center, Case Western Reserve University, School of Medicine, Cleveland, Ohio (E.F., A.M.B.)
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Abstract |
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 Top
 Abstract
 Introduction
Materials and Methods
Results
Discussion
References
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Human ether-a-go-go-related gene (HERG) potassium channels are one primary target for the pharmacological treatment of cardiac arrhythmias by class III antiarrhythmic drugs. These drugs are characterized by high antiarrhythmic efficacy, but they can also initiate life-threatening "torsade de pointes" tachyarrhythmias. Recently, it has been suggested that combining potassium and calcium channel blocking mechanisms reduces the proarrhythmic potential of selective class III antiarrhythmic agents. BRL-32872 is a novel antiarrhythmic drug that inhibits potassium and calcium currents in isolated cardiomyocytes. In our study, we investigated the effects of BRL-32872 on cloned HERG channels heterologously expressed in Xenopus oocytes. Using the two-microelectrode voltage clamp technique, we found that BRL-32872 caused a high-affinity, state-dependent block of open HERG channels (IC50 = 241 nM) in a frequency-dependent manner with slow unbinding kinetics. Inactivated channels mainly had to open to be blocked by BRL-32872. The HERG S620T mutant channel, which has a strongly reduced degree of inactivation, was 51-fold less sensitive to BRL-32872 block, indicating that BRL-32872 binding was enhanced by the inactivation process. In an additional approach, we studied HERG channels expressed in a human cell line (HEK 293) using the whole-cell patch-clamp technique. BRL-32872 inhibited HERG currents in HEK 293 cells in a dose-dependent manner, with an IC50 value of 19.8 nM. We conclude that BRL-32872 is a potent blocker of HERG potassium channels, which accounts for the class III antiarrhythmic action of BRL-32872.
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Introduction |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Repolarization
of cardiac ventricular myocytes is due mainly to outward potassium
currents (Carmeliet, 1993
). One of the most important currents is the
delayed rectifier potassium current, IK, which
has both rapidly (IKr) and slowly activating
components (Sanguinetti and Jurkiewicz, 1990). Activation of the rapid
component of the delayed rectifier potassium current,
IKr, initiates repolarization and terminates the
plateau phase of the cardiac action potential. The human
ether-a-go-go-related gene (HERG) (Curran et al., 1995; Sanguinetti et
al., 1995; Trudeau et al., 1995) encodes the major protein underlying
IKr, and mutations in the HERG gene account for
chromosome 7-linked inherited long QT syndrome-2 (Keating, 1995;
Sanguinetti et al., 1996; Viskin, 1999; Ficker et al., 2000). Patients
diagnosed with long QT-2 syndrome present with prolonged QT intervals
in the surface electrocardiogram and have a high risk for ventricular
"torsade de pointes" arrhythmias, a cause of sudden cardiac death.
Recently, a patient with homozygous premature truncation of HERG and
therefore complete absence of IKr, has been
reported by Hoorntje et al. (1999). This patient had severe cardiac
arrhythmias, but there was no evidence of dysfunction in any other
organ. Thus, the role of HERG in other functional systems is either
limited or compensated during the development.
Class III antiarrhythmic drugs, such as dofetilide, amiodarone, or
clofilium, have been shown to be potent inhibitors of HERG potassium
channels (Kiehn et al., 1996, 1999b; Suessbrich et al., 1997). A block
of IKr causes lengthening of the cardiac action potential, which produces a class III antiarrhythmic effect.
Prolongation of cardiac refractoriness has been proposed as a mechanism
to prevent atrial and ventricular arrhythmias resulting from re-entrant pathways (Singh and Nademanee, 1985). However, the therapeutical use of
class III antiarrhythmic drugs is limited by their proarrhythmic potential: excessive prolongation of the cardiac action potential can
lead to acquired long QT syndrome and life-threatening "torsade de
pointes" arrhythmias (Napolitano et al., 1994; El-Sherif and Turitto,
1999).
In the search for novel antiarrhythmic drugs with reduced proarrhythmic
risk, compounds with diverse electrophysiological effects have been
tested. In particular, it has been suggested that combining potent
inhibition of IKr and moderate calcium channel blockade might lead to a reduced risk of proarrhythmic side effects (Bril et al., 1996, 1998; Chouabe et al., 1998; Zhang et al., 1999; Noble and Colatsky, 2000). BRL-32872, a novel compound derived from the calcium and potassium channel antagonist verapamil (Zhang et
al., 1999), was found to inhibit the delayed rectifier potassium current and the L-type calcium current in guinea pig ventricular cardiomyocytes (Bril et al., 1995). Furthermore, it has been
demonstrated that BRL-32872 has a potent antiarrhythmic effect and
induces fewer proarrhythmic events than the typical class III
antiarrhythmic agent E-4031 in a dog model of programmed electrical
stimulation-induced arrhythmias (Bril et al., 1996). In addition,
Faivre et al. (1999) found that BRL-32872 does not cause early after
depolarizations (EADs) in canine Purkinje fibers and suppresses EADs
induced by clofilium, a selective inhibitor of the delayed rectifier
potassium current (Suessbrich et al., 1997) in the same model.
The aim of the present study was to investigate the potential interaction of BRL-32872 with cloned HERG potassium channels heterologously expressed in Xenopus laevis oocytes and in the human cell line HEK 293. This approach revealed detailed insights into the biophysical mechanism of high-affinity HERG channel block by BRL-32872.
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Materials and Methods |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Molecular Biology.
Procedures for in vitro transcription and
oocyte injection have been published previously (Kiehn et al., 1999b).
Briefly, HERG wild-type (Warmke and Ganetzky, 1994; GenBank accession
no. hs04270) (a kind gift from M. T. Keating) and HERG S620T
(Ficker et al., 1998) cRNAs were prepared with the mMESSAGE mMACHINE
kit (Ambion, Austin, TX) using SP6 RNA polymerase after linearization with EcoRI (Roche Diagnostics, Mannheim, Germany). Stage
V-VI defolliculated Xenopus oocytes were injected with 46 nl
of cRNA per oocyte.
Electrophysiology and Statistics.
Two-microelectrode
voltage-clamp recordings from Xenopus laevis oocytes were
carried out as published previously (Thomas et al., 1999). In brief,
recordings were performed using a Warner OC-725A amplifier (Warner
Instruments, Hamden, CT) and Pclamp software (Axon Instruments, Foster
City, CA) for data acquisition and analysis. Microelectrodes had tip
resistances ranging from 1 to 5 megaohms. The recording chamber was
continually perfused.
). HEK 293 cells used for electrophysiological study were seeded on glass
coverslips 24 to 72 h before use. On the day of experiments,
coverslips were transferred into a small cell bath mounted on the stage
of an inverted microscope (IM 35, Zeiss, Jena, Germany). Data were
filtered at 2 kHz before digitalization to 10 kHz. Electrodes (1-4
megaohms resistance when filled with the internal solution) were pulled
from TW150F glass capillary tubes (World Precision Instruments, New
Haven, CT). All experiments were carried out at room temperature
(20-22°C), and no leak subtraction was done during the experiments.
Concentration-response relationships for BRL-32872 block were fit to a
Hill equation of the following form:
IBRL-32872/Icontrol = 1/[1 + (B/IC50)n],
where I indicates current, B is the BRL-32872
concentration, n is the Hill coefficient, and
IC50 is the concentration necessary for 50%
block. Activation curves were fit with a Boltzmann distribution: G(V) = Gmax/(1 
exp[(V1/2 V)/k]), where V is the test pulse potential, V1/2 is the half-maximal
activation potential, and k is the slope of the activation
curve. All data are expressed as the mean ± S.D. We used the
unpaired Student's t test to compare the statistical
significance of the results: p < 0.05 was considered statistically significant.
Solutions and Chemicals. Voltage-clamp measurements of Xenopus oocytes were performed in a physiological potassium solution containing (in mM): 5 KCl, 100 NaCl, 1.5 CaCl2, 2 MgCl2, and 10 HEPES (pH 7.4 with NaOH). Current and voltage electrodes were filled with 3 M KCl solution. For whole-cell patch-clamp recordings from HEK 293 cells, electrodes were filled with the following solution (in mM): 100 K-aspartate, 20 KCl, 2.0 MgCl2, 1.0 CaCl2, 10 EGTA, 10 HEPES, and 40 glucose (pH 7.2 with KOH). The external solution for these experiments contained (in mM): 140 NaCl, 5.0 KCl, 1.0 MgCl2, 1.8 CaCl2, 10 HEPES, and 10 glucose (pH 7.4 with NaOH).
BRL-32872 (hydrochloride salt; kindly supplied by SmithKline Beecham, Munich, Germany) (Bril et al., 1995) was prepared as a 10 mM stock
solution in water and stored at 20°C. On the day of experiments,
aliquots of the stock solution were diluted to the desired
concentration with the bath solution.
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Results |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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BRL-32872 Blocks HERG Potassium Currents.
Figure
1 shows the effects of BRL-32872 on HERG
potassium channels expressed in Xenopus laevis oocytes. HERG
currents were elicited by a 2-s depolarizing step to +20 mV, followed
by a repolarizing step to 40 mV for 1.6 s to produce large,
slowly decaying outward tail currents that are a characteristic of HERG
potassium currents (Sanguinetti et al., 1995). The holding potential
was 80 mV in all experiments performed in this study. This voltage
protocol was repeated every 10 s during superfusion with the drug
solution, and the amplitude of the current was monitored until no
changes in current amplitude could be recorded for 3 min. After this
monitoring period, test pulses were applied to determine the amount of
block. HERG tail currents were blocked potently by BRL-32872 at
nanomolar concentrations as shown in Fig. 1A. To study the
concentration dependence of HERG current block by BRL-32872, inhibition
of HERG peak tail currents was normalized to the respective control
values and plotted as relative current amplitude in Fig. 1B
(n = 5-6 oocytes at each concentration). The
IC50 for the block of tail currents was 241.4 nM.
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BRL-32872 Blocks HERG Potassium Channels in the Open State and with
Lower Affinity in the Inactivated State.
To determine whether the
channel is blocked in the closed or open and inactivated states, we
activated currents by use of a protocol with a single depolarizing step
to 0 mV for 30 s (Kiehn et al., 1999b). After having obtained the
control measurement (Fig. 2A), we allowed
10 µM of the drug to wash in for 10 min while holding all channels in
the closed state at 80 mV membrane potential. The first pulse after
this equilibrium period showed no effect on the initial time course of
current activation, but revealed a time-dependent block of HERG current
that developed during the depolarizing step (Fig. 2A). Apparently,
there is mainly a block of open or inactivated channels with no marked
inhibition of closed channels. Subsequent depolarizing pulses at 10-s
intervals showed no time-dependent component of block, thus indicating
that BRL-32872 had not dissociated appreciably from the channel due to
slow unbinding kinetics within this time frame.
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80 mV. Strong inward rectification could be
observed in the control trace without BRL-32872 during the step to 80 mV (Fig. 2B; protocol 1), before the current continued its normal time
course during the step back to 0 mV. The recording of control
measurements was followed by application of 10 µM BRL-32872 to the
oocyte for a period of 10 min, during which the cell was held at 80
mV without pulsing. The first recording from a typical oocyte after
this wash-in period is shown in Fig. 2C. In the first step to 0 mV, the
normal kinetics of open channel block were seen. During the second step
at 0 mV, normal kinetics of BRL-32872 block were resumed, but the
current amplitude at the beginning of this step was larger than it
would have been during a continuous 0 mV step. This can be demonstrated
by exponential fits to the currents before and after the intervening
step to 80 mV, displaying a discontinuity of block (see arrow in Fig.
2C). We conclude from this qualitative comparison that blockade by
BRL-32872 is weaker when HERG channels are mostly inactivated at 80 mV,
compared with 0 mV, when larger fractions are open and therefore
available for high-affinity block. Thus, HERG channels are likely to be
blocked with the highest affinity in the open state. A block occurs to
channels during inward rectification as well, since the current
amplitude at the beginning of the second 0 mV step was reduced,
compared with the end of the first 0 mV step.
The Biophysical Mechanism of HERG Channel Blockade by
BRL-32872.
We further elucidated the blockade of HERG channels
during depolarization and questioned how HERG channels are blocked at the end of the cardiac action potential while recovering from inactivation. To answer this question, we applied a two-step protocol. During the first step from the holding potential of 80 mV to 80 mV (5 s) channels are mainly inactivated (Kiehn et al., 1999a). The fraction
of open channels was increased during a second voltage step to 0 mV (5 s), before returning to 80 mV (Smith et al., 1996). The graphical
overlay of a typical control measurement and the first pulse after
incubation with 10 µM BRL-32872 for 10 min at 80 mV (without
pulsing) is displayed in Fig. 3A. The inlet shows the beginning of the test pulse (Fig. 3A). After
application of the drug, the current trace shows a time-dependent
increase and reaches a peak amplitude larger than the control trace.
Then, the current after drug application became smaller than the
control current (n = 4).
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). Transitions occur
between the different states as indicated by arrows (Fig. 3B). After
application of BRL-32872, HERG channels are blocked with high affinity
during the inactivating 80 mV pulse, since the current amplitude is
already markedly decreased at the beginning of the 0 mV step. The
increased initial peak current during the 80 mV step indicates that
more channels are transformed from the dominant inactivated state into
the open state, compared with the control. This could be explained by a
high-affinity block of open HERG channels by BRL-32872. The enhanced
transition rate from open to blocked states causes a lack of channels
in the open state. To regain equilibrium between open and inactivated
states, the transition rate from inactivated to open states (directly or via the closed state) is consecutively increased (Fig. 3C), which
becomes visible in the initial peak current at 80 mV (indicated by the
arrow in Fig. 3A). These results further support that mainly open HERG
channels are blocked with high affinity, and that the inactivated
channels have to open before they can be blocked by BRL-32872. In
addition, the fraction of open channels might be further increased by
drug molecules inside the channel pore preventing open channels from
closing and from inactivating. Taking into account the results
displayed in Fig. 2C, direct block of inactivated channels cannot be
excluded. However, the mechanism described here seems to be the major pathway.
HERG S620T Mutant Channels Show Reduced Sensitivity to BRL-32872
Blockade.
Previous studies have shown that the S620T mutation in
HERG almost abolishes C-type inactivation and modifies block of HERG channels by antiarrhythmic drugs (Suessbrich et al., 1997; Ficker et
al., 1998). Because we observed that BRL-32872 block is reduced by HERG
channel inactivation, drug effects were tested on the HERG S620T
channel under the same conditions as previously described for the HERG
wild-type (WT) channel (see Fig. 1A). Figure
4A displays typical current traces
recorded from HERG S620T channels during the test pulse at +20 mV
(compare with Fig. 1A). HERG S620T peak tail currents were only blocked
by 50.2 ± 9.5% at a BRL-32872 concentration that caused an
almost complete block of HERG WT channels (10 µM), and the
concentration dependence analysis resulted in an
IC50 value of 12.4 µM (Fig. 4B;
n = 6 cells studied at each concentration), which is 51 times higher compared with the IC50 obtained from
HERG WT channels in Xenopus oocytes (241.4 nM).
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BRL-32872 Does Not Markedly Affect Inactivation of HERG
Channels.
We investigated the effects of BRL-32872 on HERG current
inactivation by testing whether the rate of inactivation was affected by the drug. Pulses were applied to 40 mV for 900 ms where channels are
partially open but mostly inactivated. A brief repolarization to 100
mV for 16 ms caused rapid recovery from inactivation without marked
deactivation. During a second depolarizing pulse (150 ms) to different
voltages ranging from 60 mV to 40 mV (increment 20 mV), large,
rapidly inactivating currents were produced. The holding potential was
80 mV. Inactivating currents were recorded before (Fig.
5A) and after equilibration of the block
with 300 nM BRL-32872 (Fig. 5B) by current monitoring. Single
exponential fits to the large inactivating currents yielded the time
constants of inactivation at different voltages. In a set of four
cells, no significant changes in the time constant for HERG channel
inactivation were observed (Fig. 5C).
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120 to 30 mV (increment 10 mV) for 20 ms. Finally, the resulting peak
outward currents at constant 20 mV as a measure for steady-state
inactivation were recorded (Smith et al., 1996). After having obtained
the control measurements (Fig. 5D), we equilibrated the block with 300 nM BRL-32872 by pulsing as described. The holding potential was 80 mV
to avoid destruction of the cell, as it would occur when holding the
cell at 20 mV for approximately 15 to 20 min. One typical recording in
the presence of the drug is displayed in Fig. 5E. The inactivating
outward current amplitude measured at 20 mV was normalized and plotted
against the test pulse potential, giving the steady-state inactivation
curve (Fig. 5F). Values for the half-maximal inactivation voltage were
fit with a Boltzmann distribution and yielded 72.3 ± 1.5 mV for
control and 76.2 ± 2.3 mV for BRL-32872 measurements
(n = 4). There was only a small mean shift of
3.9 ± 1.5 mV in the inactivation curves.
BRL-32872 Has No Effect on HERG Channel Activation.
The effect
of BRL-32872 on HERG current-voltage (I-V) relationship was
investigated under isochronal recording conditions. Oocytes were
clamped at a holding potential of 80 mV. Depolarizing pulses were
applied for 2 s to voltages between 80 and +80 mV in 10 mV
increments, and tail currents were recorded during a constant
repolarizing step to 60 mV for 1.6 s. Families of current traces
from one cell are shown for control conditions and after exposure to
300 nM BRL-32872 in Fig. 6. The currents
activated at potentials greater than 50 mV, reached a peak at 10 mV,
and then decreased at more positive potentials due to inactivation (Sanguinetti et al., 1995; Smith et al., 1996; Spector et al., 1996),
giving the I-V relationship its typical bell-shaped appearance (Fig.
6C). The peak tail current, measured during the repolarizing second
step of the voltage protocol, increased with voltage steps from 40 mV
to +20 mV and then plateaued for test pulse potentials positive to +20
mV (Fig. 6D). HERG currents at the end of the test pulse to 0 mV were
reduced by 45.2 ± 17.8% (n = 4), and peak tail
currents were blocked by 45.1 ± 7.7% (n = 4).
Figure 6D displays peak tail currents normalized to their respective
peak values as a function of the test pulse potential, resulting in
isochronal activation curves. BRL-32872 caused no significant change in
the half-maximal activation voltage
V1/2 of 2.3 ± 2.6 mV from
21.2 ± 2.9 mV to 23.5 ± 3.4 mV (n = 4).
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Block of HERG Channels by BRL-32872 Is Not Voltage-Dependent.
To address the question whether HERG current block by BRL-32872 varies
with voltage, we applied the following methodical approach. Since
mainly open channels were blocked and because unblocking was extremely
slow, only one experiment at each potential could be carried out with
one individual oocyte. Activating currents were elicited by 35-s
depolarizing pulses ranging from 50 mV to +80 mV from a holding
potential of 80 mV, and peak inward tail currents were recorded
during a second step to 120 mV (400 ms). First, control currents were
recorded. Then, oocytes were superfused with the drug solution (1 µM
BRL-32872) while holding the cell at constant 80 mV for 10 min, where
HERG channels are in the closed state. After this, the measurement at
the test pulse potential was obtained. Typical recordings for 40 mV
and 80 mV are shown in Fig. 7, A and B. Percent inhibition of the peak tail currents was plotted as a function
of the preceding test pulse potential (Fig. 7C; n = 6-7 cells studied at each potential). BRL-32872 application reduced
the currents throughout all voltages, but the degree of blockade was
not significantly different at the potentials tested, indicating that
block by the drug was not voltage-dependent.
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Frequency Dependence of Block.
HERG block by BRL-32872 was
frequency-dependent, as shown in Fig. 8.
BRL-32872 (1 µM) was washed into the bath, and HERG channels were
rapidly activated by a depolarizing step to 20 mV for 300 ms followed
by a repolarizing step to 40 mV (300 ms) to elicit outward tail
currents, before returning to the holding potential of 80 mV. Pulses
were applied at intervals of 1, 2, 4, or 10 s to n = 5 to 6 oocytes, with each cell studied only at one frequency. The
development of current reduction was plotted versus time (Fig. 8), and
the resulting level of steady-state block is a measure for the
frequency dependence of block. Block was use-dependent with a stronger
steady-state level of block at higher frequencies. The time course of
the development of block did also depend on the frequency of channel
activation (Fig. 8).
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BRL-32872 Blocks HERG Channels in a Human Cell Line.
To
demonstrate BRL-32872 block of HERG in human cells, we expressed HERG
potassium channels heterologously in HEK 293 cells. Channels were
activated by a 2-s depolarization to +20 mV, and outward tail currents
were recorded during a step back to 40 mV for 1.6 s (Fig.
9). During the wash-in of the drug, we
applied the protocol as described (frequency 0.1 Hz) until the block
reached a maximum. The tail currents were blocked by BRL-32872 in a
concentration-dependent manner. The IC50 value
for the BRL-32872 block of peak HERG tail currents under these
conditions was 19.8 nM (n = 3-6 cells). In six control
experiments, a period of 20 min had no significant effect on the HERG
current amplitude (data not shown).
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Discussion |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The results of our study demonstrate that BRL-32872 is a potent
inhibitor of HERG potassium channels heterologously expressed in
Xenopus laevis oocytes and HEK 293 cells. Blockade of HERG expressed in HEK cells by BRL-32872 displayed an
IC50 value of 19.8 nM, which is almost identical
to the IC50 for IKr block
in guinea pig cardiomyocytes (28 nM) reported by Bril et al. (1995). In
contrast, our experiments with HERG channels expressed in
Xenopus oocytes revealed an IC50 of
241.4 nM for the BRL-32872 block. This discrepancy is due to specific
properties of the different expression systems. In particular, higher
concentrations of drugs are necessary in Xenopus oocyte
experiments when applied to the extracellular surface of whole oocytes.
For example, the block of HERG by dofetilide gave an
IC50 that was 20-fold higher when the drug was
applied to the bath, compared with the application of the drug to the
internal surface of the membrane in inside-out membrane patches (Kiehn
et al., 1996). One explanation for this observation is that the
viteline membrane and the yolk reduce the actual concentration of drugs
at the cell membrane. Nevertheless, the Xenopus oocyte
expression system is a suitable preparation for investigations of the
mechanism of block.
The present study was designed to analyze the biophysical mechanism of
HERG channel block by BRL-32872 to understand better the class III
antiarrhythmic properties of this novel compound. One important finding
of this study was that BRL-32872 blocks HERG channels with high
affinity in the open state, although weaker blockade of inactivated
channels cannot be excluded. A pronounced shift in the half-maximal
inactivation voltage, as reported for other HERG current inhibitors
(Wang et al., 1999; Tie et al., 2000) could not be observed. The
half-maximal inactivation voltage was only slightly shifted by 3.9
mV. Unblocking upon repolarization, which allows HERG channels to
become available for opening, occurred very slowly. As a consequence,
the block was use-dependent, with the block being stronger at higher
stimulation frequencies.
Our results revealed an interesting phenomenon that illustrates the strong state dependence of the HERG channel block by BRL-32872. At very positive inactivating potentials (80 mV; Fig. 3C) in the presence of the drug, channels appear to have to open before the drug binds to the channel. Block occurs mainly to the small fraction of open HERG channels, forcing more channels to change their conformation from inactivated to open. This results in an additional outward current due to a markedly increased amount of open channels upon strong depolarization at 80 mV in the presence of BRL-32872 (see Fig. 3C). In addition to this, the drug molecule inside the channel pore on its way to the putative binding site might prevent the open channel from closing and from inactivating, which could result in an increased fraction of open channels, consecutively causing a larger initial current amplitude compared with control conditions.
The slow rate of unblocking may be due to a trapping mechanism of the
drug at its binding site (Mitcheson et al., 2000). The finding of
reduced block in the inactivation-deficient HERG S620T mutant
demonstrates that channel inactivation has an enhancing effect on the
open channel block by BRL-32872 (Numaguchi et al., 2000). Inactivation
might be required for trapping of the drug molecule and for
high-affinity drug binding, as reported previously for other class III
antiarrhythmic drugs (Suessbrich et al., 1997; Ficker et al., 1998).
As a result of the outcome of the survival with oral
d-sotalol SWORD trial (Waldo et al., 1996), where
treatment with the pure class III antiarrhythmic drug
d-sotalol caused an increase in mortality, recent research
has focused on drugs controlling re-entrant ventricular
tachyarrhythmias by having ancillary properties. BRL-32872 has been
shown to produce pronounced antiarrhythmic efficacy in several
arrhythmia models with fewer adverse effects than pure class III
antiarrhythmic substances (Bril et al., 1995, 1998; Gout et al., 1995;
Faivre et al., 1999). This is probably due to its electrophysiological
profile with a combination of potent block of potassium channels (HERG)
and moderate inhibition of L-type calcium channels (Bril et al., 1995;
Noble and Colatsky, 2000). In guinea pig cardiomyocytes, the L-type
calcium channel was 100-fold less sensitive to BRL-32872 than
IKr (Bril et al., 1995). This is consistent with
the observation that the increase in action potential duration in
papillary muscle preparations due to high-affinity BRL-32872 block of
IKr has been limited with increasing
concentrations of the drug, when calcium current inhibition counterbalances the action potential prolongation. This dual activity produces a bell-shaped dose-response relationship (Bril et al., 1995).
Similar mechanisms could also account for the relatively low incidence
of "torsade de pointes" arrhythmias in the clinical use of the
antiarrhythmic drug amiodarone (Hohnloser et al., 1994), since
amiodarone is known to exhibit not only HERG potassium current blocking
properties (Kiehn et al., 1999b), but also class I (Mason et al.,
1984), class II (Polster and Broeckhuysen, 1976), and class IV
antiarrhythmic action (Yabek et al., 1986).
In conclusion, the present results show that BRL-32872 is a high-affinity antagonist of cloned HERG potassium channels. The fact that the drug has the ability to block both potassium and calcium currents renders it a potentially useful action potential modulator. The pharmacological action with moderate calcium channel block counterbalancing excessive QT prolongation by strong potassium channel block possibly prevents the occurrence of "torsade de pointes" arrhythmias. Thus, BRL-32872 could serve as a promising starting point for more effective modern antiarrhythmic therapy with low proarrhythmic potential.
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Acknowledgments |
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The excellent technical assistance of K. Güth and S. Lück is gratefully acknowledged.
We also thank Dr. S. Kropff from SmithKline Beecham for the gift of BRL-32872, Dr. M. T. Keating for generously donating the HERG clone, and Dr. A. Bril for comments on the manuscript. The HEK 293 cell line stably transfected with HERG cDNA used in this study was kindly provided by Dr. B. A. Wible.
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Footnotes |
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Accepted for publication January 25, 2001.
Received for publication October 23, 2000.
This work was supported by grants from the Deutsche Forschungsgemeinschaft (Project A/11 to J.K. within the Sonderforschungsbereich 320 "Herzfunktion und ihre Regulation"), and by grants from the National Institutes of Health to A.M.B. (HL-36930, HL-55404, and HL-61642).
K.R. and D.T. were supported by the German National Merit Scholarship Foundation. Data presented here are part of the thesis of G.W.-N.
Send reprint requests to: Dr. Johann Kiehn, Medical University Hospital Heidelberg, Bergheimerstrasse 58, D-69115 Heidelberg, Germany. E-mail: johannkiehn{at}ukl.uni-heidelberg.de
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Abbreviations |
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IK, delayed rectifier potassium current; IKr, rapidly activating component of IK; HERG, human ether-a-go-go-related gene; BRL-32872, N-(3,4-dimethoxyphenyl)-N-[3[[2-(3,4-dimethoxyphenyl)ethyl]propyl]-4-nitrobenzamide hydrochloride; E-4031, N-(4-(1-[2-(6-methyl-2-pyridyl)ethyl]-4-piperidyl)-carbonyl]phenyl) methanesulfonamide dihydrochloride dihydrate; WT, wild type; I-V, current-voltage.
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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V1/2 = 
