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Vol. 59, Issue 1, 122-126, January 2001
Aventis Pharmaceuticals, Inc. Bridgewater, New Jersey (J.K., L.W., X.-L.C., D.R.); and State University of New York at Buffalo, Buffalo, New York (D.J.T.)
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Abstract |
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 Top
 Abstract
 Introduction
Materials and Methods
Results
Discussion
References
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Administration of certain fluoroquinolone antibacterials has been associated with prolongation of the QT interval on the electrocardiogram and, on rare occasions, ventricular arrhythmia. Blockade of the human cardiac K+ channel HERG often underlies such clinical findings. Therefore, we examined a series of seven fluoroquinolones for their ability to interact with this channel. Using patch-clamp electrophysiology, we found that all of the drugs tested inhibited HERG channel currents, but with widely differing potencies. Sparfloxacin was the most potent compound, displaying an IC50 value of 18 µM, whereas ofloxacin was the least potent compound, with an IC50 value of 1420 µM. Other IC50 values were as follows: grepafloxacin, 50 µM; moxifloxacin, 129 µM; gatifloxacin, 130 µM; levofloxacin, 915 µM; and ciprofloxacin, 966 µM. Block of HERG by sparfloxacin displayed a positive voltage dependence. In contrast to HERG, the KvLQT1/minK K+ channel was not a target for block by the fluoroquinolones. These results provide a mechanism for the QT prolongation observed clinically with administration of sparfloxacin and certain other fluoroquinolones because free plasma levels of these drugs after therapeutic doses approximate those concentrations that inhibit HERG channel current. In the cases of levofloxacin, ciprofloxacin, and ofloxacin, inhibition of HERG occurs at concentrations much greater than those observed clinically. The data indicate that clinically relevant HERG channel inhibition is not a class effect of the fluoroquinolone antibacterials but is highly dependent upon specific substitutions within this series of compounds. HERG channel affinity should be an important criterion for the development of newer fluoroquinolones.
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Introduction |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Acquired or drug-induced long QT
syndrome is a potentially dangerous side effect that is associated with
the administration of certain prescription medications. This syndrome
is characterized by a prolongation in the QT interval on the
electrocardiogram and is thought to contribute to the generation of the
ventricular arrhythmia torsades de pointes (Ben-David and Zipes, 1993
).
Block of voltage-dependent K+ channels in the
human heart is one means by which drugs can prolong cardiac
repolarization and precipitate ventricular arrhythmia. Advances in
cellular electrophysiology and molecular biology have lead to the
discovery and cloning of several human cardiac K+
channels. KvLQT1, for example, complexes with the minK subunit to form
the K+ channel that underlies the slow component
of the delayed rectifier current IKs (Barhanin et
al., 1996: Sanguinetti et al., 1996). The human
ether-a-go-go-related gene, HERG, expresses the
K+ channel that underlies the rapid component of
the delayed rectifier current (IKr) in the human
heart (Sanguinetti et al., 1995). Mutations in HERG lead to the type 2 form of congenital long QT syndrome, LQT2 (Curran et al., 1995).
Moreover, blockade of the HERG channel seems to be the main mechanism
through which a number of drugs act to produce acquired long QT
syndrome and associated ventricular arrhythmia. These drugs include the
antihistamines terfenadine and astemizole (Roy et al., 1996; Zhou et
al., 1999), the antipsychotic drugs sertindole and pimozide (Rampe et
al., 1997; Kang et al., 2000), and the gastric motility agent cisapride
(Rampe et al., 1997; Mohammad et al., 1997).
The fluoroquinolone class of antibacterials is widely prescribed for
the treatment of infections. Development of this class of drugs is
ongoing and seeks not only to improve antimicrobial activity but also
to reduce adverse events, including CNS toxicity and phototoxicity
(Domagala, 1994; Lipsky and Baker, 1999). Electrocardiographic changes,
manifested by a prolongation in the QT interval, represent another
adverse effect that is observed with some fluoroquinolones. For
instance, sparfloxacin produces a dose-dependent increase in QT
interval with significant prolongation apparent at normal clinical
doses (Morganroth et al., 1999a,b). Therapeutic doses of grepafloxacin
have also been shown to prolong QT interval (Ball et al., 1999; Lipsky
and Baker, 1999; Stahlmann and Lode, 1999). Concerns over the potential
for proarrhythmia have recently prompted the withdrawal of
grepafloxacin from the market (Medwatch, 1999). On the other hand, no
reports have linked ciprofloxacin and ofloxacin to prolongation in the
QT interval despite extensive therapeutic use of these drugs. In light
of these findings, the present study was undertaken to examine the
effects of a series of fluoroquinolones on the HERG cardiac
K+ channel and to determine their relative
potencies for inhibiting this channel.
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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.
The cDNA encoding the HERG
K+ channel was cloned from a human neuroblastoma
cell line. Chinese hamster ovary cells (CHO cells; American Type
Culture Collection, Manassas, VA) were transfected with the cDNA as
described previously (Rampe et al., 1997; Kang et al., 2000). Cells
were grown in Ham's F-12 media supplemented with 10% fetal bovine
serum and 500 µg/ml G418 (Life Technologies, Gaithersburg, MD)
in an atmosphere of 95% air/5% CO2. KvLQT1 and minK were cloned from human heart and stably expressed in CHO cells as
described previously (Kang et al., 2000). Cells used for
electrophysiological experiments were seeded onto glass or plastic
coverslips 24 h before use.
Electrophysiology.
HERG and KvLQT1/minK channel currents
were recorded using the whole-cell configuration of the patch-clamp
technique (Hamill et al., 1981). Electrodes (2-6 M
resistance) were
fashioned from TW150F glass capillary tubes (World Precision
Instruments, Sarasota, FL). Electrodes were filled with the following
solution: 120 mM potassium aspartate, 20 mM KCl, 4 mM
Na2ATP, 5 mM HEPES, 1 mM MgCl2, pH 7.2, with KOH. For KvLQT1/minK current
recordings, the internal solution was further supplemented with 14 mM
sodium phosphocreatine, 0.3 mM sodium GTP, and 50 U/ml creatine
phosphokinase. The external solution contained 130 mM NaCl, 5 mM KCl,
2.8 mM sodium acetate, 1.0 MgCl2, 10 mM HEPES, 10 mM glucose; 1.0 mM CaCl2, pH 7.4, with NaOH.
Currents were recorded at room temperature using an Axopatch 1-D or
Axopatch 200 B amplifier (Axon Instruments, Foster City, CA) and were
conditioned by a 4-pole, low-pass filter with a cutoff frequency of
between one quarter and one half the sampling frequency. Currents were
analyzed using the pCLAMP suite of software (Axon Instruments).
IC50 values were obtained by nonlinear
least-squares fit of the data (GraphPAD Software, San Diego, CA).
Chemicals. All antibiotics used in the study were obtained from Aventis Pharmaceuticals, Inc (Romanville, France) except ofloxacin, which was obtained from Sigma Chemical (St. Louis, MO), and gatifloxacin, which was a generous gift of R.W. Johnson Pharmaceuticals, Inc. (New Brunswick, NJ). All other chemicals were obtained from Sigma.
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Results |
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Figure 1 shows the chemical
structures for the fluoroquinolones used in this study and Fig.
2 illustrates the effects of these drugs
on HERG K+ channel currents. In these
experiments, a 2-s depolarizing pulse to +20 mV from a holding
potential of 
80 mV was followed by repolarization of the cell to 40
mV to produce large, slowly deactivating tail currents characteristic
of HERG (Sanguinetti et al., 1995). The effect of these antibiotics on
HERG is typified by moxifloxacin and shown in Fig. 2A. All of the drugs
tested reduced peak tail current amplitude measured at 40 mV in a
dose-dependent manner. Dose-response relationships (Fig. 2B) generated
from this protocol yielded IC50 values (95%
confidence limits) as follows: sparfloxacin, 18 µM (13-26 µM);
grepafloxacin, 50 µM (37-66 µM); moxifloxacin, 129 µM (99-167
µM); gatifloxacin, 130 µM (87-192 µM); levofloxacin, 915 µM
(724-1150 µM); ciprofloxacin, 966 µM (562-1670 µM) and ofloxacin, 1420 µM (794-2500 µM).
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Figure 3 shows the effects of
sparfloxacin on HERG channel currents measured over a wide range of
test potentials. In these experiments, cells were held at 80 mV and
currents were elicited by 2-s depolarizing pulses to potentials ranging
from 40 mV to +30 mV in 10 mV increments. The membrane potential was
then returned to 100 mV and peak inward tail currents were recorded.
Current traces in the absence and presence of 30 µM sparfloxacin are
shown in Fig. 3, A and B, respectively. The resultant current-voltage relationship averaged from five cells is presented in Fig. 3C. Although
sparfloxacin reduced the current amplitude at all test potentials,
greater inhibition was observed at more depolarized levels. When
inhibition of HERG current is plotted as a function of test potential,
a statistically significant (p < 0.05, ANOVA) correlation between voltage and drug effect was observed with inhibition ranging from 24% at 30 mV to 58% at +30 mV (Fig. 3D).
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We also examined the effects of the fluoroquinolones on the KvLQT1/minK
K+ channel that underlies
IKs in the human heart. Even at high
concentrations, none of the drugs tested produced substantial block of
this channel. Sparfloxacin (100 µM) reduced KvLQT1/minK
current by 3 ± 5% (n = 3; Fig.
4). At 1 mM concentration, moxifloxacin,
gatifloxacin, levofloxacin, ciprofloxacin, and ofloxacin reduced
KvLQT1/minK channel current by 12 ± 6, 4 ± 7, 6 ± 2, 6 ± 9, and 14 ± 5%, respectively (n = 3-4). Grepafloxacin was not tested because of lack of compound supply.
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Table 1 compares the inhibition of HERG
channel current recorded in this study to the peak free (unbound)
plasma levels of these drugs measured in clinical settings. All of the
drugs listed in the table are clinically available with the exception
of grepafloxacin, which was recently withdrawn from the market. For all
drugs, we sought to report the highest free plasma levels after
therapeutic doses. The plasma concentrations and protein binding values
were obtained from the Physicians' Desk Reference (1999) or, in the case of gatifloxacin and moxifloxacin, from product information (package insert) supplied for the drugs by the manufacturers. For those
drugs where both oral and intravenous dosing is available, the plasma
levels for both routes of administration are reported.
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Discussion |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The present study is the first to examine the effects of the
fluoroquinolone antibacterials on human cardiac
K+ channels. KvLQT1/minK was not a target for
block by the fluoroquinolones because high concentrations of these
drugs produced only modest (~10%) reductions in KvLQT1/minK
currents. Conversely, we found that each of the compounds tested
inhibit HERG channel currents in a dose-dependent fashion, albeit with
widely differing potencies. IC50 values ranged
from 18 µM for sparfloxacin to 1420 µM for ofloxacin. The effects
of sparfloxacin were voltage-dependent with the greatest block observed
at more depolarized potentials. This suggests that sparfloxacin
interacts with an activated state of the HERG channel. In this respect,
sparfloxacin is similar to other drugs that are known to block HERG and
produce QT prolongation including cisapride (Mohammad et al., 1997;
Rampe et al., 1997) and sertindole (Rampe et al., 1998).
The series of fluoroquinolones reported here demonstrate a wide range
of potencies against HERG
approximately a 100-fold difference from
sparfloxacin to ofloxacin. Fairly extensive structure-activity relationships are already available for the antibiotic activity of
these agents (Domagala, 1994) and the data presented here offer the
first, albeit limited, opportunity to compare that SAR with the
anti-HERG SAR. For antibacterial potency, substitution at C6 by F and C3 by COOH is
known to be important, as is the quinolone carbonyl functionality, but
significant substituent variation is permissible at
C5, C7,
C8, and N1. It is thus of
interest that levofloxacin, ciprofloxacin, and ofloxacin all lack
C5 substituents, whereas those agents most potent
against HERGsparfloxacin and grepafloxacinhave substituents at this
position. Interestingly, at C8, the least potent
compounds against HERG are either unsubstituted (ciprofloxacin) or are
substituted in a conformationally restricting manner with a bridge to
N1 (levofloxacin and ofloxacin). Of note also are
the equipotent gatifloxacin and moxifloxacin
(IC50 values ~ 130 µM) which both have
---OMe substitutions at C8. The small series and
their nonhomologous relationship make it difficult to speculate more
about the different SARs for antibacterial and anti-HERG activities,
save that there are important apparent differences and that a more
comprehensive analysis may further delineate these.
Excellent clinical data are available correlating plasma levels of
sparfloxacin with concomitant changes in the corrected QT interval
(QTc). After an oral dose of 400 mg, peak plasma levels average about
1.3 µg/ml or about 2 µM free drug (Morganroth et al., 1999a,b). At
this plasma concentration, QTc is increased by an average of 16 ms
(approximately 4%). After a dose of 1600 mg, free plasma levels of
sparfloxacin are approximately 7 µM and result in a mean increase in
QTc of 55 ms (14%) (Morganroth et al., 1999b). We found that
sparfloxacin inhibited HERG channel current at concentrations of 1 µM
and above (15 ± 2% inhibition at 1 µM; p < 0.05, paired t test). Thus, plasma levels of sparfloxacin that are associated with QT prolongation correspond to those that block
HERG in the present set of experiments by about 15 to 30%. This makes
HERG/IKr blockade the most likely mechanism to
account for the QT interval prolongation observed with sparfloxacin
treatment and for torsades de pointes arrhythmia that has been reported with its use (Dupont et al., 1996).
Grepafloxacin, moxifloxacin, and gatifloxacin displayed intermediate
potencies for inhibiting HERG channel current. The ratio of the HERG
IC50 values to peak free plasma concentrations
ranged from 13- to 22-fold (Table 1). Unlike sparfloxacin, detailed clinical studies relating plasma levels to QT interval changes are not
available for these drugs. However, grepafloxacin is well known to
prolong cardiac repolarization and has been reported to increase the QT
interval by an average of 10 ms in clinical trials (Ball et al., 1999;
Lipsky and Baker, 1999; Stahlmann and Lode, 1999). Recently,
grepafloxacin was withdrawn from the market because of concerns over QT
interval prolongation and rare cases of ventricular arrhythmia,
including torsades de pointes, in patients receiving the drug
(Medwatch, 1999). Less clinical information is available for
moxifloxacin and gatifloxacin, two newer fluoroquinolones that have
only recently been approved by the Food and Drug Administration. Clinical trials have shown both drugs can prolong QT interval by
several milliseconds (Ball et al., 1999; gatifloxacin product information, Bristol-Myers Squibb Company, Princeton NJ). The clinical
significance of these findings relative to their affinity for HERG
awaits further clinical study and postmarketing surveillance.
Levofloxacin, ciprofloxacin, and ofloxacin were significantly less
potent inhibitors of HERG compared with the other fluoroquinolones tested. One case study has associated levofloxacin with QTc
prolongation and ventricular arrhythmia in an elderly patient with
structural heart disease and atrial fibrillation (Samaha, 1999).
However, no changes in QTc have been detected with levofloxacin in
numerous clinical trials (Ball et al., 1999; Lipsky and Baker, 1999;
Stahlmann and Lode, 1999) and, to our knowledge, there are no other
published reports associating levofloxacin with QT prolongation.
Similarly, we know of no published reports that causally link QT
prolongation or ventricular arrhythmia with the use of ciprofloxacin or
ofloxacin despite the fact that these drugs have been clinically
available for more than 10 years. This probably reflects the lower
potency of these drugs for HERG both in absolute terms
(IC50 valuess ~ 1000 µM) and relative to
their peak free plasma levels (9-14 µM). Indeed, statistically
significant inhibition of HERG channel current was detected for these
drugs only at concentrations > 100 µM.
In conclusion, the present report is the first to detail the effects of the fluoroquinolone antibacterials on human cardiac K+ channels. We found that these drugs were ineffective at blocking KvLQT1/minK but inhibited HERG with widely differing potencies. Clinically relevant blockade of HERG and the attending proarrhythmic potential do not seem to be a class effect but instead indicate the existence of specific structural features in these molecules that contribute separately to their antimicrobial activity and to HERG blockade. Separation of these structural features will be very important to the development of new fluoroquinolones.
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Acknowledgments |
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We thank Dr. Patrick Shum for his help in the preparation of this manuscript.
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Footnotes |
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Received July 14, 2000; Accepted September 19, 2000
Send reprint requests to: David Rampe, Ph.D., Aventis, Inc., Route 202-206, P.O. Box 6800, Bridgewater, NJ 08807-0800. E-mail: david.rampe{at}aventis.com
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Abbreviations |
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HERG, human ether-a-go-go-related gene; SAR, structure-activity relationship.
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References |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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), grepafloxacin (
), moxifloxacin
(
), gatifloxacin (
), levofloxacin (
), ciprofloxacin (
), and
ofloxacin (
) are shown. Inhibition of peak outward tail currents at
