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Section of Cardiology, Department of Medicine, University of Wisconsin, Madison, Wisconsin 53792
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ABSTRACT |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Cisapride, a gastrointestinal prokinetic
agent, is known to cause long Q-T syndrome and ventricular
arrhythmias. The cellular mechanism is not known. The human
ether-á-go-go-related gene (HERG), which encodes the rapidly
activating delayed rectifier K+
current and is important in cardiac repolarization, may serve as a
target for the action of cisapride. We tested the hypothesis that
cisapride blocks HERG. The whole cell patch-clamp
recording technique was used to study HERG channels stably
expressed heterologously in HEK293 cells. Under voltage-clamp
conditions, cisapride block of HERG is dose dependent
with a half-maximal inhibitory concentration of 6.5 nM at 22°C
(n = 25 cells). Currents rapidly
recovered with drug washout. The onset of block by cisapride required
channel activation indicative of open or inactivated state blockage.
Block of HERG with cisapride after channel activation
was voltage dependent. At 
20 mV, 10 nM cisapride reduced HERG
tail-current amplitude by 5%, whereas, at +20 mV, the tail-current
amplitude was reduced by 45% (n = 4 cells). At 20 and +20 mV, 100 nM cisapride reduced tail-current
amplitude by 66 and 90%, respectively. We conclude that cisapride is a
potent blocker of HERG channels expressed in HEK293 cells. This effect
may account for the clinical occurrence of Q-T prolongation and
ventricular arrhythmias observed with cisapride.
rapidly activating delayed-rectifier potassium current; potassium channels; Q-T interval; torsades de pointes; gastrointestinal motility
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INTRODUCTION |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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CISAPRIDE (Propulsid, Janssen Pharmaceutical) is a benzamide derivative that is widely used as a prokinetic agent in the treatment of a variety of gastrointestinal motility disorders, including gastroparesis and gastroesophageal reflux disease. There have been case reports of palpitations and prolonged Q-T intervals from cisapride use dating back to 1989 (13). Recently, the Food and Drug Administration reported 57 cases of cardiac arrhythmia associated with the use of cisapride that it had received through its MedWatch reporting program over a period of 3 years (27). These included 34 cases of torsades de pointes, 23 patients with long Q-T syndrome (LQT), and 4 reported deaths.
Warmke and Ganetzky (25) identified the human ether-á-go-go-related gene (HERG), which, when expressed in Xenopus oocytes and HEK293 cells, has properties similar to cardiac rapidly activating delayed-rectifier K+ current (IKr) (16, 18, 22, 28). HERG current exhibits nanomolar sensitivity to methanesulfonamides, dependence on external K+ concentration, and inward rectification. HERG mRNA is strongly expressed in the heart of several mammalian species, including humans (26). Mutations in HERG have been shown to cause chromosome 7-linked inherited LQT (5), and several drugs that block IKr cause acquired LQT and torsades de pointes and also have been shown to block HERG (15, 18, 19). Thus HERG is an important target in both acquired and inherited forms of LQT.
The cellular basis for the cardiac electrophysiological effect of cisapride is not known. Cisapride was recently reported to increase action potential duration and to induce early afterdepolarizations in isolated rabbit Purkinje fibers (14). This raises the possibility that cisapride may prolong action potential duration in vivo and cause LQT by inhibiting IKr or HERG. We used HERG stably transfected HEK293 cells to test the hypothesis that cisapride is a potent blocker of HERG channel current.
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METHODS |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Stable transfection. HERG cDNA (22, 23, 28) was subcloned into BamH I and EcoR I sites of the pCDNA3 vector (Invitrogen, San Diego, CA). This vector contains a CMV promoter and an SV40 promoter, which drive the expression of the inserted cDNA (HERG) and neomycin-resistant gene, respectively. The HEK293 cells were transfected with this construct using the lipofectamine method (GIBCO, Grand Island, NY). After selection in 800 µg/ml Geneticin (G-418, GIBCO) for 15-20 days, single colonies were picked with cloning cylinders and tested for HERG current. The stably transfected cells were cultured in minimal essential medium (MEM) supplemented with 10% fetal bovine serum and 400 µg/ml G-418. All cells were from a single cell line producing high current levels and were stable for >6 mo. For electrophysiological study, the cells were harvested from the culture dish by trypsinization, washed twice with standard MEM medium, and stored in this medium at room temperature for later use. Cells were studied within 8 h of harvest.
Patch-clamp recording technique.
Cells used for electrophysiological study were transferred to a small
cell bath mounted on the stage of an inverted microscope (Diaphot,
Nikon) and were superfused with
N-2-hydroxyethylpiperazine-N'-2-ethanesulfonic acid (HEPES)-buffered Tyrode solution containing (in mM) 137 NaCl, 4 KCl, 1.8 CaCl2, 1 MgCl2, 10 glucose, and 10 HEPES
(pH 7.4 with NaOH). Solution exchanges were completed within 2 min.
Membrane currents were recorded in a whole cell configuration using
suction pipettes (7, 24). The pipettes had inner diameters of
1-1.5 µm and, when filled with the internal pipette solution,
had resistances of 2-4 M
. The internal pipette solution
contained (in mM) 130 KCl, 1 MgCl2, 5 ethylene
glycol-bis(
-aminoethyl
ether)-N,N,N',N'-tetraacetic acid, 5 MgATP, and 10 HEPES (pH 7.2 with KOH). An Axopatch 1D patch-clamp amplifier was used to record membrane currents. Computer software (pCLAMP; Axon Instruments, Foster City, CA) was used to
generate voltage-clamp protocols, acquire data, and analyze voltage and
current signals. All experiments were performed at room temperature
(22-23°C).
Drugs and chemicals. Cisapride was obtained from Research Diagnostics (Flanders, NJ; drug purity >99.8%). Cisapride was dissolved in 100% ethanol to give a stock concentration of 5 mM. Final drug concentrations were made within 48 h of experiments by diluting stock solution with the extracellular HEPES-buffered Tyrode solution. Ethanol control (n = 3 cells), at a concentration (0.01%) equivalent to the highest cisapride dilution studied, had no effect on HERG current. Other chemicals were purchased from Sigma Chemical (St. Louis, MO).
Statistical methods. Data are given as means ± SE. Curve fitting was done using a nonlinear least-squares regression analysis (Sigmaplot; Jandel Scientific, Corte Madera, CA). Statistical significance was analyzed using Student's t-test and permutation analysis.
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RESULTS |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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The effect of cisapride on HERG current was studied in
a stably transfected HEK293 cell line. Figure
1, A and
B, shows voltage-clamp data obtained
with 100 nM cisapride. Families of current traces from one cell are
shown for control conditions (Fig.
1A) and after exposure to
cisapride (Fig. 1B), with the
voltage-clamp protocol shown in Fig.
1A,
inset. Cells were clamped at a holding
potential of 80 mV. Depolarizing steps were applied for 4 s to
voltages between 60 and +50 mV in 10-mV increments. For control
conditions, depolarizing steps activated a time-dependent outward
current that increased in amplitude with more positive voltage steps to reach a maximum at +10 mV. Depolarizing steps to more positive voltages
resulted in inward rectification. After the repolarizing step to
50 mV, an outward tail current was recorded. Tail-current amplitude, measured as the difference between the peak current and
leak-corrected baseline current at 50 mV, increased with depolarizing steps from 60 to +20 mV and was then superimposed on further depolarizing steps to +50 mV. Cisapride (100 nM) suppressed both the outward and tail currents, as shown in Fig.
1B. In other experiments, Zhou et al.
(28) showed that HERG current in these cells is blocked
nearly completely by E-4031 (300 nM). Finally, there is minimal
contamination of HERG current in these cells by endogenous current, as
shown in Fig. 1C in the current
records obtained from a nontransfected HEK293 cell.
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Current-voltage plots of steady-state current present at the end of the
depolarizing step and peak tail current are depicted in Fig. 1,
D and
E, respectively, before and after
exposure to 100 nM cisapride (n = 4 cells). For control conditions, the threshold for activating
HERG current was close to 40 mV and full
activation was obtained at voltages near +20 mV. In the presence of 100 nM cisapride, steady-state current and peak tail-current amplitude were
reduced compared with control conditions.
Figure 2 shows drug block of
HERG current by cisapride in a different transfected
cell. In this experiment, HERG current was rapidly
activated by a 100-ms-long depolarizing step to +60 mV (see
Ref. 18) from a holding potential of 80 mV, and the cell was
then clamped at +10 mV for 10 s. Tail currents were recorded after
repolarization to 50 mV. The control current, the current activated by the first depolarizing step after a 10-min-long exposure to 100 nM cisapride, and the current obtained after 10 min of drug
washout are shown. The cell was held at 80 mV during the washin
and washout periods. After drug washin, the initial outward current
amplitude with the first depolarizing step was only slightly decreased
compared with control current, indicating little closed-state block.
The outward current amplitude subsequently decreased during the
depolarizing step to reach maximal block. Current was recovered nearly
completely after 10 min of drug washout.
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Cisapride block of HERG current was concentration
dependent. Steady-state block was obtained by applying depolarizing
steps from 80 to +10 mV for a 20-s period every 30 s, and peak
tail current was measured after repolarizing steps to 50 mV for
5 s at different drug concentrations. Analysis of the data obtained from a total of 25 cells with the Hill equation gave a half-maximal inhibitory concentration (IC50)
value of 6.5 nM. The decrease in peak tail current as a function of
drug concentration is shown in Fig. 3.
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Block of HERG current by cisapride varied with voltage,
exhibiting a higher degree of block at more positive voltages, as shown
in Fig. 4. In four transfected cells, 10 nM
cisapride at 20 mV reduced peak tail-current amplitude by 5%
from 282 ± 91 to 268 ± 77 pA
(P > 0.05), whereas at +20 mV it
reduced peak tail-current amplitude by 45% from 944 ± 89 to 511 ± 97 pA (P < 0.05). At 100 nM
cisapride, the voltage dependence of drug block was again evident, with
HERG current reduced from 232 ± 95 to 80 ± 17 pA (66% reduction) and from 1,010 ± 48 to 96 ± 55 pA (90%
reduction), at 20 and +20 mV, respectively (see Fig. 1;
P < 0.05 compared with control). The
amount of block at each drug concentration was greater at +20 mV than
at 20 mV (P < 0.05). Thus
cisapride block of HERG current exhibits voltage
dependence.
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DISCUSSION |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Several reports of cardiac arrhythmias with the use of cisapride have appeared in the literature over the last decade (1, 2, 13). Recently, the Food and Drug Administration reported 57 cases of torsades de pointes and/or Q-T prolongation in patients that were administered cisapride (27). The development of Q-T prolongation and torsades de pointes in cisapride users frequently appeared to be associated with the concomitant use of medications that compete for drug metabolism by the cytochrome P-450 3A4 isozyme, the presence of renal insufficiency, and with administration of high doses of cisapride.
After oral administration, total cisapride peak serum values of 60-80 µg/l (120-170 nM) are achieved, of which >95% is plasma protein bound (11, 25a). The drug is extensively metabolized by the cytochrome P-450 enzyme system in the liver with an elimination half-life of ~10 h. The half-life of cisapride may be prolonged in patients with hepatic disease and in the elderly (11). Coadministration of drugs metabolized through the cytochrome P-450 enzyme system can also result in higher drug levels.
The results of our study demonstrate that cisapride is a potent blocker of HERG channels expressed heterologously in HEK293 cells. The drug concentrations we studied were similar to the therapeutic levels achieved in the clinical use of this drug. We conclude that blockage of HERG current may underlie the proarrhythmic effect of cisapride. Thus this report shows HERG to be a molecular target for the action of cisapride and may help to explain the mechanism of Q-T prolongation and occurrence of torsades de pointes with this drug.
Block of HERG by cisapride was voltage dependent. Drug block does not occur via closed-state block, because nearly normal peak outward current was recorded on the first depolarizing step after drug washin, as shown in Fig. 2. Rather, the onset of HERG-current block by cisapride required channel activation, suggestive of open- or inactivated-state drug block. Our protocols, however, do not easily distinguish between open- and inactivated-state block. In the study of cisapride block of HERG, it is important to recognize that the IC50 of drug block is voltage dependent.
Cisapride is a widely used gastrointestinal prokinetic agent in humans and animals. Cisapride augments motility throughout the gastrointestinal tract and is used in the treatment of gastroesophageal reflux disease and gastroparesis (3, 25a). The mechanism of action is not fully elucidated but is thought to be through the release of acetylcholine mediated by postganglionic nerve endings in the myenteric plexus of the gut (9). Cisapride is an agonist of serotonin [5-hydroxytryptamine (5-HT)] at the 5-HT4 receptor as well as an antagonist at the 5-HT3 receptor (4). Cisapride seems to enhance gastroduodenal motility in humans by enhancing cholinergic transmission through stimulation of 5-HT4 receptors on the enteric nerve endings (17, 21, see also Ref. 20). Cisapride also has a direct stimulating effect on gastrointestinal smooth muscle tissue without the involvement of 5-HT receptors. In experiments with guinea pig stomach circular smooth muscle, cisapride was found to cause depolarization of the muscle membrane (6), and, in taenia coli preparations from guinea pig colon, cisapride was shown to cause depolarization, enhancement of spike activity, increases in muscle tone, and potentiation of contraction (12).
Our findings raise the possibility that the prokinetic effect of cisapride may be explained, in part, by its blockage of gastrointestinal K+ channels located either on the smooth muscle cells of the gut or on the presynaptic nerve terminals of the myenteric plexus. Recent reports showed widespread distribution of HERG mRNA in different tissues, including small intestine (26). It is possible that cisapride causes membrane depolarization of smooth muscle cells or causes release of excitatory neurotransmitters from nerve endings by blocking HERG channels present in the gastrointestinal tract. Further studies are needed to define the cellular distribution of HERG in the gastrointestinal tract and the possible interaction of HERG and cisapride in the gut.
The findings of this study have several important implications. Our study shows that cisapride in low concentrations blocks HERG; therefore, this may be the mechanism responsible for the Q-T prolongation and torsades de pointes associated with cisapride use in humans. Moreover, the concentration of drug associated with 50% block in vitro (IC50 = 6.5 nM) is within the therapeutic range achieved with oral dosing in humans. The reason that arrhythmic effects are not observed more frequently may be due to the fact that >95% of the drug is bound to plasma proteins. Only when high free-drug levels are achieved, such as from liver disease, drugs competing for metabolism, or overdosage, do Q-T prolongation and torsades de pointes occur. In addition, these findings may prove helpful in developing newer and safer gastrointestinal prokinetic drugs devoid of the undesirable side effects of Q-T prolongation.
Because we only studied HERG-transfected cells, possible effects of cisapride on other membrane currents cannot be excluded. In addition, we did not study the effects of metabolites, such as norcisapride, on HERG current. Therefore, in vivo contributions by the metabolites to the drug effects cannot be excluded. Finally, cisapride has been demonstrated to be a partial agonist of 5-HT4 receptors in human right atrium. This mechanism is unlikely to be important in the genesis of ventricular arrhythmias because of the absence of functional 5-HT4 receptors in the human ventricle (8).
In conclusion, cisapride blocks HERG-encoded channels expressed in HEK293 cells. This effect may account for the clinical occurrence of Q-T prolongation and ventricular arrhythmias observed with the use of cisapride. This is a new class of drugs shown to block HERG, further supporting the evidence that HERG is an important target for many cardiovascular and noncardiovascular drugs.
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ACKNOWLEDGEMENTS |
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The authors thank Drs. Jonathan Makielski and Chandar Singaram for reviewing the manuscript.
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FOOTNOTES |
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Address for reprint requests: C. T. January, Section of Cardiology, Rm. H6/352 CSC, Univ. of Wisconsin Hospitals and Clinics, 600 Highland Ave., Madison, WI 53792.
Received 21 May 1997; accepted in final form 12 July 1997.
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Abstract
Introduction
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Discussion
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