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Vol. 293, Issue 3, 870-878, June 2000
Department of Pharmacology (P.S., J.Z., E.A.S., H.H.S.) and Brain Research Institute (A.K., C.P.), University of Vienna, Vienna, Austria
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Abstract |
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 Top
 Abstract
 Introduction
Materials and Methods
Results
Discussion
References
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HEK 293 cells stably expressing the human serotonin transporter (hSERT) were grown on coverslips, preincubated with [3H]5-hydroxytryptamine (5-HT), and superfused. Substrates of the hSERT [e.g., p-chloroamphetamine (PCA)], increased the basal efflux of [3H]5-HT in a concentration-dependent manner. 5-HT reuptake blockers (e.g., imipramine, paroxetine) also raised [3H]5-HT efflux, reaching approximately one-third of the maximal effect of the hSERT substrates. In uptake experiments, both groups of substances inhibited [3H]5-HT uptake. Using the low-affinity substrate [3H]N-methyl-4-phenylpyridinium (MPP+) to label the cells in superfusion experiments, reuptake inhibitors failed to enhance efflux. Similar results were obtained using human placental choriocarcinoma (JAR) cells that constitutively express the hSERT at a low level. By contrast, PCA raised [3H]MPP+ efflux in both types of cells, and its effect was inhibited by paroxetine. The addition of the Na+,K+-ATPase inhibitor ouabain (100 µM) to the superfusion buffer enhanced basal efflux of [3H]5-HT-loaded hSERT cells by approximately 2-fold; the effect of PCA (10 µM) was strongly augmented by ouabain, whereas the effect of imipramine was not. The Na+/H+ ionophore monensin (10 µM) also augmented the effect of PCA on efflux of [3H]5-HT as well as on efflux of [3H]MPP+. In [3H]5-HT-labeled cells, the combination of imipramine and monensin raised [3H]5-HT efflux to a greater extent than either of the two substances alone. In [3H]MPP+-labeled cells, imipramine had no effect on its own and fully reversed the effect of monensin. The results suggest that the [3H]5-HT efflux caused by uptake inhibitors is entirely due to interrupted high-affinity reuptake, which is ongoing even under superfusion conditions.
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Introduction |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The
action of serotonin [5-hydroxytryptamine (5-HT)] released at nerve
terminals is ended by high-affinity reuptake of the neurotransmitter
from the synaptic cleft. This process is mediated by a selective
Na+- and Cl
-dependent
serotonin transporter (SERT). Moreover, the SERT is responsible not
only for inward transport of released transmitter but also for outward
movement of transmitter under certain pharmacological, physiological,
and pathophysiological conditions (Levi and Raiteri, 1993
).
Many drugs of therapeutic interest as well as drugs of abuse exert
their action via this transmembrane protein. Antidepressants such as
the tricyclics (e.g, imipramine, clomipramine) or the selective
serotonin reuptake inhibitors (e.g., fluoxetine, citalopram) bind to
the transporter and prevent substrate translocation. The subsequent
rise of the 5-HT concentration in the vicinity of the postsynaptic
receptors is believed to be the initial step in the therapeutic action
of these drugs. On the other hand, the anorectic agent fenfluramine or
the amphetamine derivative p-chloroamphetamine (PCA)
competes with 5-HT for translocation and thereby promotes release of
5-HT both in vivo (Fuller et al., 1965) and in vitro (Rudnick and Wall,
1992; Gobbi et al., 1993) by a reversed transport mechanism.
Classic experimental models to study carrier-mediated serotonin
transport are synaptosomes or blood platelets (for a review, see
Rudnick, 1997). However, there are some disadvantages to these systems.
In synaptosomes, for instance, the characterization of the
neurochemical events associated with the uptake and release of a
specific neurotransmitter is complicated by their metastable structure
and great heterogeneity. Thrombocytes as well as synaptosomes not only
transport 5-HT across their plasmalemmal membrane via the SERT but also
concentrate 5-HT intracellularly in vesicles via the vesicular
monoamine transporter. Therefore, cellular systems containing only the
SERT have met with increased interest in studies on the function and
regulation of this protein. In particular, an analysis of
carrier-mediated processes on a molecular level has been allowed by the
cloning and heterologous expression of high numbers of the human SERT
(hSERT) in mammalian cells (Ramamoorthy et al., 1993; for a review, see
Blakely et al., 1997). Typically in these studies, the cells are grown
in wells and incubated with radiolabeled transmitter in the absence and
presence of drugs. For measurements of transporter-mediated efflux, the
cells are first loaded with radiolabel, and then the release of
radioactivity is monitored by pipetting medium from the well or by
measuring the amount of radiolabel in the cells. This approach,
however, has methodological limitations, because it detects only
changes in net movement of neurotransmitter molecules, which may result from influences on inward or outward transport across the membrane. It
also does not allow a satisfactory time resolution of the process under
study. To circumvent these disadvantages, we applied a method that
allows the superfusion of transfected cells after they have been loaded
with radiolabeled neurotransmitter (Pifl et al., 1995). Superfusion is
expected to quickly remove released radiolabel and thus to prevent
reuptake (Raiteri et al., 1974).
Here, we present uptake and superfusion experiments in HEK 293 cells
stably expressing the hSERT and in human placental choriocarcinoma (JAR) cells, which constitutively express the hSERT (Prasad et al.,
1996). By using [3H]5-HT and
[3H]N-methyl-4-phenylpyridinium
(MPP+), two substrates of different affinity for
the hSERT and of different transmembrane diffusion properties, as well
as by experimental alterations of the transmembrane ion gradients with
ouabain or monensin, we were able to distinguish drug effects on
carrier-mediated inward and outward transport and to discern active
reverse transport from diffusion of [3H]5-HT
out of the cell.
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Materials and Methods |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Cell Line Transfection.
The plasmalemmal hSERT was
originally cloned in pBluescript II KS
(Ramamoorthy et al., 1993). The hSERT cDNA was a generous gift of Dr.
R. D. Blakely (Department of Pharmacology and Center for Molecular
Neuroscience, School of Medicine, Vanderbilt University, Nashville,
TN). The cDNA was excised with XbaI and HindIII
and ligated into pEGFP-C1 (Clontech, Palo Alto, CA), which had been opened with NheI and HindIII and
dephosphorylated. The GFP-tag is excised using these two enzymes, and
therefore the cDNA is placed after the promoter without being modified.
For stable expression into HEK 293 cells, the same method was used as
described previously (Pifl et al., 1996). The stable transfectants
(hSERT cells) were grown in minimal essential medium with
Earle's salts and
L-alanyl-L-glutamine (L-GlutaMAX I; Gibco Life Technologies, Grand
Island, NY), 10% heat-inactivated fetal bovine serum, 50 mg/l
gentamicin, and 500 µg/ml geneticin (G418) on 100-mm-diameter cell
culture dishes at 37°C in an atmosphere of 5%
CO2, 95% air.
JAR Cells. JAR cells were a generous gift of Dr. H. Bönisch (Institute of Pharmacology and Toxicology, University of Bonn, Bonn, Germany). JAR cells were grown in RPMI-1640 medium, 10% fetal calf serum, 100 U/ml penicillin, and 100 µg/ml streptomycin at 37°C in an atmosphere of 5% CO2, 95% air.
Uptake Experiments. The experiments were performed in poly(D-lysine)-coated 24-well plates (1 day after plating; 5 × 104 or 105 cells/well for hSERT or JAR cells, respectively). Each well was washed with 0.5 ml of KRH buffer (Krebs-Ringer-HEPES buffer containing 10 mM HEPES, 120 mM NaCl, 3 mM KCl, 2 mM CaCl2, 2 mM MgCl2, final pH 7.3) and incubated with 0.05 ml of buffer containing 0.1 µCi of [3H]5-HT or [3H]MPP+ (27.5 Ci/mmol [3H]5-HT and 60 Ci/mmol [3H]MPP+, respectively) and various concentrations of unlabeled 5-HT, MPP+, or drugs in a total volume of 0.5 ml. After 2.5 min at room temperature, the uptake buffer was rapidly aspirated, and the cells were washed twice with 1 ml of ice-cold buffer. Cells were lysed with 0.5 ml of 1% SDS and transferred into scintillation vials for liquid scintillation counting. Nonspecific uptake was defined as uptake in the presence of 30 µM clomipramine and amounted to less than 2% of the total uptake in the presence of 120 mM NaCl. In experiments in which the effect of competing drugs was tested, the substances of interest were added 5 min before the addition of [3H]5-HT using at least six different concentrations.
Vmax, Km, EC50, and IC50 values were calculated using nonlinear regression fits performed with Prism (GraphPad, San Diego, CA). The equation used to estimate Km and Vmax values was Y = Vmax × X/(Km + X), where Y = V (picomoles per 106 cells per minute) and X = substrate concentration (moles per liter). Uptake experiments on parental HEK 293 cells were performed in poly(D-lysine)-coated 12-well plates (1 day after plating; 2 × 105 cells in 500 µl of medium/well). The final concentrations of 5-HT and MPP+ were 10 µM; 20 µl of unlabeled 5-HT (260 µM) was added for HPLC experiments; for radiochemical experiments 2 µCi [3H]5-HT was added additionally. To study MPP+ accumulation, 260 µM unlabeled MPP+ and 2 µCi of [3H]MPP+ were used. After several time points of incubation at 37°C, the medium was removed quickly, and each well was washed twice with 2 ml of ice-cold KRH buffer. To perform HPLC detection, cells were lysed with 500 µl of 0.1 M perchloric acid and transferred to a 1.5-ml tube. The wells were washed with an additional 500 µl of 0.1 M perchloric acid. The cells were sonicated and centrifugated at 15,000g for 10 min at 4°C. The supernatant was transferred onto the HPLC column. For radiochemical detection, cells were lysed with 1 ml of 1% SDS and transferred into scintillation vials for liquid scintillation counting.Superfusion Experiments.
The cells were grown overnight onto
round glass coverslips (diameter, 5 mm) coated with
poly(D-lysine) (25 µg/ml) at 2 × 104 cells/well for hSERT cells,
105 cells/well for JAR cells, and 4 × 104 cells/well for parental HEK 293 cells. For
preincubation with labeled substrates, the following conditions
applied: hSERT cells were incubated with
[3H]5-HT (5 µM, 0.38 µCi/well) or
[3H]MPP+ (10 µM, 1.54 µCi/well) for 20 min at 37°C in a final volume of 0.225 ml of
culture medium. JAR cells were incubated with
[3H]5-HT (1.7 µM, 2.3 µCi/well) or
[3H]MPP+ (17 µM, 1.88 µCi/well) for 30 min at 37°C in a final volume of 0.125 ml of
culture medium. Parental HEK 293 cells were incubated with
[3H]5-HT (3.8 µM, 10 µCi/well) for 60 min
at 37°C in a final volume of 0.11 ml of culture medium. Coverslips
were then transferred to small superfusion chambers (0.2 ml) and
superfused with KRH buffer (0.7 ml/min) as described recently (Pifl et
al., 1995). Because of the very rapid loss of
[3H]5-HT at 37°C, which seriously interfered
with the observation of drug effects, a superfusion temperature of
25°C was chosen. A similar observation was made by Johnson et al.
(1998) in hSERT transfected C6 glioma cells. After a washout period of
45 min to establish a stable efflux of radioactivity, the experiment was started with the collection of fractions (4-min duration). At the
end of the experiment, cells were lysed in 1% SDS. Tritium in the
superfusate fractions and in the SDS lysates was determined by liquid
scintillation counting. The release of 3H was
expressed as fractional rate (i.e., the radioactivity released during a
fraction was expressed as a percentage of the total radioactivity present in the cells at the beginning of that fraction). Drug-induced release was calculated by subtracting the estimated basal release from
total release during the first 8 min of drug exposure and is expressed
as a percentage of radioactivity in the cell at the beginning of drug exposure.
HPLC Experiments. The chromatography system consisted of a Jasco 980 HPLC pump (0.8 ml/min; Jasco International, Tokyo, Japan), a Rheodyne 7125 valve (100-µl loop; Rheodyne, Cotati, CA), a reversed phase column (250 × 4.6 mm; Hi-Pore RP Column; Bio-Rad Laboratories, Richmond, CA), and an LC-4C electrochemical detector (Bioanalytical Systems, West Lafayette, IN). The detector potential was set at 600 mV versus an Ag/AgCl reference electrode [mobile phase: 75 mM NaH2PO4, 0.11 mM EDTA, 0.2 mM sodium octane sulfonate, and 12% (v/v) methanol, with a final pH of 4.05].
Chemicals. Tissue culture reagents were from Gibco Life Technologies. RPMI-1640 medium was obtained from Sigma-Aldrich Handels GmbH (Vienna, Austria). [3H]MPP+ and [3H]5-HT were purchased from New England Nuclear Life Sciences Products (Boston, MA). Paroxetine was kindly donated by SmithKline Beecham (Worthing, UK). MPP+ and fluoxetine were obtained from Research Biochemicals International (Natick, MA). Monensin, d-fenfluramine, PCA, imipramine, and serotonin were obtained from Sigma-Aldrich Handels GmbH. All other chemicals were obtained from commercial sources.
Statistical Analysis. All results were expressed as mean ± S.E. values. Statistical analysis consisted of Spearman's correlation and repeated measures ANOVA followed by t test for paired or independent observations, as appropriate. A value of P < .05 was considered to be the level of statistical significance.
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Results |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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HEK 293 cells permanently expressing the hSERT exhibited a clomipramine-sensitive and time-, temperature-, and concentration-dependent accumulation of [3H]5-HT. Saturation analysis of initial uptake rates revealed a Vmax value of 141 ± 17 pmol/min/106 cells and a Km value of 0.396 ± 0.034 µM (mean ± S.E. of eight independent determinations). When [3H]MPP+ was used as substrate, a Vmax value of 196 ± 4 pmol/min/106 cells and a Km value of 13.68 ± 3.6 µM (mean ± S.E. of three independent determinations) were obtained.
Effects of hSERT Substrates and 5-HT Reuptake Inhibitors on Release
and Uptake of [3H]5-HT.
Basal efflux of
radioactivity from hSERT cells preincubated with
[3H]5-HT amounted to 1.32 ± 0.07% during
min 8 to 12, corresponding to 65.95 ± 5.43 pCi (n = 25; mean ± S.E.). HPLC analysis revealed that more than 95% of
the radioactivity in superfusates and cells coeluted with authentic
[3H]5-HT (data not shown). The addition of
substrates of hSERT such as PCA or d-fenfluramine or
inhibitors of 5-HT reuptake such as imipramine, paroxetine, or
fluoxetine to the superfusion buffer caused a concentration- and
time-dependent increase in [3H]5-HT efflux.
Representative, the effects of PCA and imipramine are shown in Fig.
1. Both drugs caused a
concentration-dependent increase in efflux that reached a plateau after
8 min of drug exposure, with imipramine being approximately one-fourth
as effective as PCA. Figure 2A shows
concentration-response curves for various hSERT substrates and 5-HT
reuptake inhibitors, and the resulting EC50
values are given in Table 1. The maximum
effects on release expressed as a percentage of radioactivity released
during the first 8 min of drug exposure were 13 to 16% for the hSERT
substrates and approximately 4% for the reuptake inhibitors. All drugs
were also tested for inhibition of [3H]5-HT
uptake. The concentration-response relationships are shown in Fig. 2B,
and the corresponding IC50 values are given in
Table 1. There was a good correlation between the log
IC50 values obtained from uptake experiments with
the log EC50 values obtained from superfusion
experiments (r = 0.933, P < .01).
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Interaction between hSERT Substrates and hSERT Blockers.
The
effect of the potent uptake inhibitor paroxetine on PCA-induced
[3H]5-HT release was analyzed. After a 16-min
exposure to different concentrations of paroxetine (0.1 nM to 1 µM),
PCA (10 µM) was added to the superfusion buffer for an additional 20 min. As shown in Fig. 3A, paroxetine
alone increased [3H]5-HT efflux in a
concentration-dependent manner but likewise inhibited further efflux
induced by PCA. At paroxetine concentrations of more than 10 nM, the
release-enhancing action of PCA was abolished. The same experiment was
carried out using
[3H]MPP+ as substrate
instead of [3H]5-HT. Under these conditions,
paroxetine did not increase
[3H]MPP+ efflux but
inhibited the effect of PCA, causing complete suppression at 100 nM
(Fig. 3B).
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Parental HEK 293 Cells.
To investigate a possible role of
diffusion in the efflux of [3H]5-HT or
[3H]MPP+ from cells
expressing the hSERT, parental HEK 293 cells were studied. The cells
were incubated with the radiolabeled substrates (10 µM), and the
amount of radioactivity entering the cells was measured.
[3H]5-HT easily entered the cells during the
60-min incubation, reaching approximately 0.2 nmol/106 cells. By contrast,
[3H]MPP+ displayed
considerably lower intracellular accumulation (Fig. 4A).
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JAR Cells. JAR cells, which constitutively express the hSERT at a low density, were studied in uptake and superfusion experiments. The cells concentration and time dependently accumulated [3H]5-HT. Saturation analysis of initial rates of [3H]5-HT uptake yielded a Vmax value of 2.44 ± 0.3 pmol/min/106 cells and a Km value of 0.58 ± 0.1 µM (n = 4, with the latter value being similar to that found in hSERT cells).
On superfusion, a high fractional rate of efflux of approximately 4% was observed (Fig. 5A). This was 2 to 4 times higher than the rate in hSERT cells superfused in parallel (not shown). The addition of PCA (10 µM) or imipramine (10 µM) had no significant effect on efflux (Fig. 5A). By contrast, the use of [3H]MPP+ as loading substrate resulted in a basal efflux of approximately 1%, comparable to hSERT cells. On the addition of PCA (10 µM), a significant increase in [3H]MPP+ release was observed, whereas the addition of imipramine (10 µM) did not alter [3H]MPP+ release (Fig. 5B).
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Effects of Ouabain and Monensin on Efflux of [3H]5-HT and [3H]MPP+. To investigate in more detail the unexpected finding that reuptake inhibitors caused an increase in release of [3H]5-HT, a series of experiments were performed under the conditions of an increased intracellular sodium concentration, which is expected to facilitate outward transport of substrate. For this purpose, the Na+,K+-ATPase inhibitor ouabain and the Na+/H+-selective ionophore monensin were used.
Ouabain (100 µM) led to a slow increase of [3H]5-HT efflux. When it was included in the superfusion buffer during the 45-min washout period, the efflux rate at the beginning of superfusate collection was more than twice as high as that under ouabain-free conditions (3.43 ± 0.37%, n = 9, versus 1.19 ± 0.11%, n = 9; P < .001: pooled values from Fig. 6B). On the addition of PCA (10 µM) to the ouabain-containing buffer (cells were superfused for 57 min with ouabain at this point), efflux of [3H]5-HT was massively enhanced to a rate of more than 37% (Fig. 6A). Likewise, the subsequent addition of ouabain to PCA caused a pronounced enhancement of [3H]5-HT efflux (Fig. 6A).
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Discussion |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The aim of the present study was to characterize 5-HT transport in
cells stably expressing hSERT. For this purpose, the effects of uptake
inhibitors as well as hSERT substrates were studied in uptake and
superfusion experiments. All drugs inhibited uptake with
IC50 values between 4 nM and 1 µM, displaying a
comparable rank order of potency as described recently (Barker et al.,
1994) using the same clone expressed in a different cell line.
Superfusion experiments involved preincubation of the cells with
[3H]5-HT and monitoring the subsequent efflux
of radioactivity. A particular advantage of this technique is believed
to be the avoidance of concomitant high-affinity reuptake of released
transmitter (Raiteri et al., 1974). Superfusion rests on the premise
that the transmitter leaving the cell is immediately diluted by the superfusion medium and therefore is not available for reuptake. By
contrast, performing the experiment using a stationary incubation in
culture dishes or wells will allow reuptake of released 5-HT, which
constitutes a recognized confounding factor in this type of studies.
Superfusion conditions should thus enable different mechanisms of
substances acting on hSERT to be clearly distinguished. If releasing
drugs such as the hSERT substrates PCA or d-fenfluramine are
added to superfused cells, the rate of [3H]5-HT
efflux should increase, but if uptake blockers such as imipramine or
paroxetine are added, which bind to the transporter and block transport
in both directions, the rate of [3H]5-HT
release into the superfusate should not change or even decrease.
This expectation was fully borne out by the results regarding
substrates of the hSERT (i.e., 5-HT, PCA, and
d-fenfluramine), all of which increased the efflux of
[3H]5-HT. However, uptake inhibitors did not
display the expected effect but instead caused a distinct enhancement
of release. Substrate efflux induced by uptake inhibitors from cell
lines expressing the SERT was also described by Wall et al. (1995) and
Johnson et al. (1998). The apparent releasing effect would best be
explained by a block of ongoing reuptake of
[3H]5-HT diffusing out of the cells. However,
such an effect is typical for slice or isolated organ preparations but
is not expected in superfused cells or synaptosomes. For example, the
uptake-blocking drug cocaine did not enhance transmitter efflux from
superfused COS-7 cells transfected with either the plasmalemmal
dopamine or noradrenaline transporter (Pifl et al., 1995, 1999).
Moreover, releasing effects of various reuptake inhibitors in
superfused rat brain synaptosomes preloaded with
[3H]5-HT were not observed (Collard et al.,
1981; Raiteri et al., 1984). By contrast, the effects of the
uptake-inhibiting drugs in the present experiments had
EC50 values in the nanomolar range and exhibited
clearly defined maxima. If their action was indeed a consequence of
interrupted high-affinity reuptake, several conditions should apply: 1)
the uptake of an hSERT substrate that is added to the superfusion
buffer should be inhibited, 2) diffusion must play a quantitatively
significant role in the efflux of [3H]5-HT, and
3) the affinity of the substrate that is used for loading the
cells and 4) the density of transporters expressed at the surface of
the cell should determine reuptake. All four premises were tested
experimentally. First, the interaction of the reuptake inhibitor
paroxetine and the hSERT substrate PCA was studied. Paroxetine by
itself enhanced efflux concentration dependently but clearly inhibited
in the same manner the effect of subsequently added PCA (Fig. 3A).
Inhibition by uptake blockade of substrate-induced release of 5-HT has
also been observed recently using d-fenfluramine as
releasing agent (Gobbi et al., 1992; Cinquanta et al., 1997).
Information pertinent to the question of diffusion and substrate
Km was obtained when the experiment
was repeated using the substrate
[3H]MPP+ instead of
[3H]5-HT. Under this condition, paroxetine
still inhibited the effect of PCA but did not increase the efflux of
[3H]MPP+ by itself (Fig.
3B). The positively charged substrate
[3H]MPP+ showed
considerably less diffusion through the plasma membrane of parental HEK
293 cells compared with 5-HT (Fig. 4A) and has a more than 30-fold
higher Km value for the hSERT (14 µM
for [3H]MPP+ and 0.4 µM
for [3H]5-HT). These properties can both be
expected to reduce reuptake by the hSERT: there is less substrate
leaving the cell, and it is more easily diluted to a concentration at
which reuptake is negligible. Finally, as to the premise of an
influence of transporter density on the effect of uptake inhibitors,
experiments were performed on JAR cells. These cells express the hSERT
constitutively but display an initial uptake rate of
[3H]5-HT that is <1% of the value obtained in
hSERT cells. Consequently, one would expect less reuptake during
superfusion, resulting in a high basal efflux rate and small or no
effects of uptake blockers on efflux. This was in fact the case. The
hSERT substrate PCA was also without apparent effect, probably due to
the high basal rate masking any small drug-induced effect. With use of
the less diffusible
[3H]MPP+ as substrate,
basal efflux was lower, and PCA displayed a distinct release-enhancing
effect, whereas imipramine again did not change efflux (Fig. 5B).
To further characterize the effects of uptake-inhibiting drugs and
hSERT substrates, we conducted a series of experiments in which the
intracellular sodium concentration was modified by the addition of
ouabain or monensin. Although ouabain inhibits Na+,K+-ATPase, monensin
acts as ion-selective ionophore, facilitating the transmembrane
exchange of sodium ions for protons (Mollenhauer et al., 1990). It is
known that a rise in the sodium concentration at the inside of the
plasma membrane results in a decrease in Km value for outward transport
(Raiteri et al., 1978; Liang and Rutledge, 1982; Bönisch, 1986).
In the present experiments, both ouabain and monensin massively
augmented PCA-induced release of [3H]5-HT. This
result was reproduced when monensin and PCA were studied in
[3H]MPP+-loaded cells
(Fig. 8A). The interactions with the uptake inhibitor imipramine,
however, revealed more complexity. The combination of ouabain and
imipramine raised the efflux rate of [3H]5-HT
to the same level as imipramine alone. The combination of monensin and
imipramine, on the other hand, increased the efflux rate to a
distinctly higher level than imipramine on its own. Adding the drugs in
sequence showed quite clearly the effect of monensin on top of the
imipramine-induced rise of efflux (Fig. 7B, filled circles). This
action of monensin was most likely not related to active transport.
Three observations strongly support this notion: 1) when the
less-diffusible [3H]MPP+
was used instead of [3H]5-HT to label the
cells, monensin did not display any effect after imipramine (Fig. 8B,
filled circles). 2) Imipramine was able to completely reverse a
monensin-induced rise in efflux of [3H]MPP+ when the uptake
inhibitor was added after the ionophore (Fig. 8B, filled triangles). 3)
When parental HEK 293 cells passively loaded with
[3H]5-HT were superfused, monensin increased
efflux of radioactivity (Fig. 9). This demonstrates an
hSERT-independent mechanism by which [3H]5-HT
leaves the cell in the presence of monensin. A possible explanation
could be monensin-induced alkalinization of the cell interior due to
outward movement of protons (Mollenhauer et al., 1990); an increase in
the intracellular pH value toward the
pKa value of 5-HT would favor outward
diffusion by enhancing the mole fraction of the more lipophilic neutral
form of 5-HT (Rudnick et al., 1989). The effect of imipramine on top of
monensin in [3H]5-HT-labeled cells (Fig. 7B,
filled triangles) indicates ongoing reuptake in the presence of the
ionophore. Taken together, the data point to a combined effect of
monensin (i.e., imipramine-sensitive outward transport of
[3H]5-HT together with an increase in outward
diffusion of [3H]5-HT, with the latter effect
being partially offset by concomitant reuptake).
The finding that raising the intracellular sodium concentration
drastically increases the releasing effect of PCA but not that of
uptake blockers strongly argues against the possibility that efflux
induced by uptake inhibitors is a consequence of reversed transport. A
similar conclusion was reached in a study of the effects of cocaine and
ouabain on dopamine efflux from LLC cells expressing the human
noradrenaline transporter (Chen et al., 1998). A point that has not
been experimentally addressed in the present study is whether the
observed differences between PCA and imipramine may be related to
changes in membrane potential brought about by the changes in ion
distribution. Many sodium-coupled transport systems are responsive to
changes in membrane potential (Wilson et al., 1998).
The present results may directly relate to a well known clinical
caveat: the concomitant use of a monoamine oxidase inhibitor and a
tricyclic antidepressant or a selective serotonin reuptake inhibitor is
contraindicated because of a severe adverse reaction known as
serotonergic syndrome (for a review, see Hilton et al., 1997). Symptoms
include alterations in cognition, behavior, autonomic system function,
and neuromuscular activity. Because treatment with monoamine oxidase
inhibitors raises cytoplasmic levels of 5-HT, a situation may be
created in vivo that is comparable to our experimental conditions in
vitro. According to our results, introducing an uptake inhibitor in the
presence of a relevant cytoplasmic pool of 5-HT should in fact lead to
a markedly enhanced availability of 5-HT in the extracellular space.
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Footnotes |
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Accepted for publication February 4, 2000.
Received for publication October 18, 1999.
1 This work was supported by the Austrian Science Foundation, Project P13183. Part of the work was presented at the Summer Meeting of the British and German Pharmacological Societies at the University of Nottingham, UK, July 1999.
Send reprint requests to: Dr. Harald H. Sitte, Department of Pharmacology, University of Vienna, Waehringerstr. 13a, A-1090 Vienna, Austria. E-mail: harald.sitte{at}univie.ac.at
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Abbreviations |
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5-HT, 5-hydroxytryptamine; hSERT, human serotonin transporter; SERT, serotonin transporter; PCA, p-chloroamphetamine; MPP+, N-methyl-4-phenylpyridinium.
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References |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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, PCA; 
, d-fenfluramine (d-FEN); 
,
5-HT; 
, paroxetine; 
, fluoxetine; 
, imipramine.
; 1 nM, 
,
effect of 100 µM ouabain added after 10 µM imipramine. 
, 
)
or 10 µM PCA (
