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The Journal of Neuroscience, December 1, 1999, 19(23):10494-10501
Effects of Chronic Antidepressant Treatments on Serotonin Transporter Function, Density, and mRNA Level
Saloua Benmansour1, Marco Cecchi1, David A. Morilak1, Greg A. Gerhardt4, Martin A. Javors1, 2, Georgianna G. Gould1, and Alan Frazer1, 3 Departments of 1 Pharmacology and 2 Psychiatry, University of Texas Health Science Center, San Antonio, Texas 78284, 3 South Texas Veterans Health Care System, San Antonio, Texas 78284, and 4 Departments of Anatomy and Neurobiology, University of Kentucky, Lexington, Kentucky 40536
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
To investigate functional changes in the brain serotonin transporter (SERT) after chronic antidepressant treatment, several techniques were used to assess SERT activity, density, or its mRNA content. Rats were treated by osmotic minipump for 21 d with the selective serotonin reuptake inhibitors (SSRIs) paroxetine or sertraline, the selective norepinephrine reuptake inhibitor desipramine (DMI), or the monoamine oxidase inhibitor phenelzine. High-speed in vivo electrochemical recordings were used to assess the ability of the SSRI fluvoxamine to modulate the clearance of locally applied serotonin in the CA3 region of hippocampus in drug- or vehicle-treated rats. Fluvoxamine decreased the clearance of serotonin in rats treated with vehicle, DMI, or phenelzine but had no effect on the clearance of serotonin in SSRI-treated rats. SERT density in the CA3 region of the hippocampus of the same rats, assessed by quantitative autoradiography with tritiated cyanoimipramine ([3H]CN-IMI), was decreased by 80-90% in SSRI-treated rats but not in those treated with phenelzine or DMI. The serotonin content of the hippocampus was unaffected by paroxetine or sertraline treatment, ruling out neurotoxicity as a possible explanation for the SSRI-induced decrease in SERT binding and alteration in 5-HT clearance. Levels of mRNA for the SERT in the raphe nucleus were also unaltered by chronic paroxetine treatment. Based on these results, it appears that the SERT is downregulated by chronic administration of SSRIs but not other types of antidepressants; furthermore, the downregulation is not caused by decreases in SERT gene expression.
Key words: serotonin transporter; antidepressants; in vivo electrochemistry; [3H]CN-IMI binding; mRNA for the SERT; dorsal hippocampus
INTRODUCTION
The serotonin transporter (SERT) is the primary initial target for many classes of antidepressants, including selective serotonin reuptake inhibitors (SSRIs) (Frazer, 1997
). SSRIs rapidly inhibit the uptake of serotonin (5-HT). However, maximal antidepressant effects are obtained only after weeks or even months of repeated treatment, suggesting that in addition to the inhibition of serotonin reuptake, other longer-term, adaptive changes occur that contribute to therapeutic efficacy. Most long-term studies of antidepressants have focused on their effects on autoreceptors or postsynaptic receptors and the responses they elicit (Blier and Bouchard, 1994
Although there is little research on antidepressant-induced regulation of SERT function in vivo, there have been numerous studies of the effects of such treatment on the binding of ligands to the SERT or its mRNA content. Such studies have yielded conflicting results, with some studies reporting increases (Hrdina and Vu, 1993
To control variability in drug exposure of the SERT to drug, we administered antidepressants in this study from osmotic minipumps and measured steady-state serum concentrations to select doses that produced drug concentrations either within or close to the "therapeutic range." Antidepressants were selected that block the uptake of 5-HT selectively (paroxetine and sertraline), the uptake of norepinephrine (NE) selectively (desipramine; DMI), or inhibit monoamine oxidase (MAO; phenelzine). In addition, in vivo chronoamperometry was used to measure serotonin clearance and its modulation by local application of the SSRI fluvoxamine in the CA3 region of rat hippocampus, because it had been established that active clearance of 5-HT in this region is attributable primarily to activity of the SERT (Daws et al., 1998
MATERIALS AND METHODS
Animals. Male Sprague Dawley rats (Harlan Sprague Dawley, Indianapolis, IN) weighing 175-200 gm at the time of initiation of drug treatment were housed individually on a 12 hr light/dark cycle with lights on at 7:00 A.M. and with food and water provided ad libitum. All animal procedures were in strict accordance with the National Institutes of Health Guide for the Care and Use of Laboratory Animals. All efforts were made to minimize both the number of animals used and stress or discomfort to the animal during the experimental procedure.
Chronic drug treatments. Groups of 6-15 rats were treated for 21 d with various antidepressants. Paroxetine (5 or 10 mg · kg
1 · d
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Table 1. Serum concentrations of the antidepressants In vivo chronoamperometry. This was performed as described previously (Daws et al., 1998
1000:1 and a linear response (r2
Rats were anesthetized with chloralose (70 mg/kg)-urethane (700 mg/kg), and the electrode, attached to a multibarrel micropipette, was positioned in the CA3 region of the dorsal hippocampus. The distance between electrode and pipette tips was 275-325 µm. Multibarrel micropipettes were filled with either 5-HT (200 µM; Sigma), fluvoxamine (400 µM; Pharmacia and Upjohn, Kalamazoo, MI), or desipramine (400 µM). The pH of all solutions was 7.4. All drugs were delivered by pressure ejection in a volume of 20-100 nl. Twenty to thirty minutes after lowering of electrode, chronoamperometric recordings were started. Once reproducible electrochemical signals from 5-HT were obtained, drug was applied 60-90 sec before the next application of 5-HT.
High-speed chronoamperometric recordings were made using the Fast-12 system (Quanteon, Denver, CO). Oxidation potentials consisted of 100 msec pulses of +0.55 V versus Ag/AgCl that were delivered one per second; the electrode was held at a resting potential of 0.0 V between measurements. The reference electrode was positioned in the superficial cortex. Oxidation and reduction currents were digitally integrated during the last 80 msec of each 100 msec voltage pulse.
Several parameters are obtained from the electrochemical signal produced by exogenous applications of 5-HT. Signal amplitude was maintained between 0.6 and 0.8 µM by applying various amount of 5-HT (4-21 pmol) to facilitate comparison between different treatment groups. Other parameters analyzed were T80, the time it takes for the peak amplitude to be reduced by 80%; T40-80, the time for the signal to decrease from 80% of its peak value to 40%; and the total time course (t course), the total time for the signal to return to baseline from the time of application of 5-HT.
Autoradiographic procedures. After completing the in vivo chronoamperometry recordings, rats were decapitated, and their brains were frozen quickly on dry ice and stored at
80°C until sectioning. Brain sections (20 µm) were cut in a cryostat at
Serotonin uptake sites were measured using [3H]cyanoimipramine as previously described (Kovachich et al., 1988
HPLC analysis of 5-HT content. Hippocampi from the contralateral hemispheres were used to determine levels of 5-HT by HPLC coupled with electrochemical detection as described by Hall et al. (1989)
HPLC analysis of serum drug levels. Serum was collected after 7-10 d of treatment (to measure steady-state drug levels) or at the end of the electrochemical recording session. Serum concentrations of sertraline, paroxetine, and desipramine were determined by HPLC with a Waters spherisorb S5 CN column and UV detection at 214 nm. Samples were spiked with doxepin as an internal standard. Drugs were extracted from plasma with a hexane-isopropanol mixture (19:1, v/v), then back-extracted into a phosphate buffer, pH 2.5. Aliquots of the back-extractions were injected into the HPLC. Plasma drug concentrations are expressed in nanograms per milliliter.
In situ hybridization. Animals treated chronically with paroxetine (10 mg · kg
Methods for in situ hybridization were essentially as previously described (Domyancic and Morilak, 1997
-35S-UTP (New England Nuclear), to a specific activity of 2 × 109 cpm/µg. All prehybridization solutions were treated with diethylpyrocarbonate and sterilized. Brain sections were thawed, hydrated, acetylated, and rinsed in 2× SSC (1× SSC is 150 mM sodium chloride, 15 mM sodium citrate, pH 7.2). Sections were then dehydrated, delipidated, and air-dried. Hybridization buffer consisted of 50 mM sodium phosphate, 3× SSC, 5× Denhardt's solution, 0.1 mg/ml salmon sperm DNA, 0.1 mg/ml yeast tRNA, 10 mM dithiothreitol, 10% dextran sulfate, and 50% deionized formamide, to which radiolabeled riboprobe was added to a final concentration of 4 × 107 cpm/ml (~20 ng/ml). Sections were incubated overnight in a sealed humidified chamber at 60°C. Control sense-strand probe was applied to a small number of sections to verify specificity of the label.
All post-hybridization solutions contained 1 mM dithiothreitol. After hybridization, excess probe was removed by rinsing in four washes of 2× SSC and digesting with RNase A (20 µg/ml, 30 min at 37°C). Sections were then taken through a series of increasingly stringent washes: 10 min each in 1×, 0.5×, and 0.2× SSC at 24°C, followed by 3 × 1 hr in 0.1× SSC at 60°C. They were then rinsed in 1× SSC, dehydrated, and apposed, along with 14C-radioactive standards, to Kodak Biomax MR x-ray film for 24 hr before developing.
Digitized autoradiographic film images were captured with a Sony XC-77 CCD camera coupled to a Scion LG-3 capture board in a PowerMac 7100 computer. Integrated signal density overlying the dorsal and median raphe, calibrated from the standards on each film and expressed in standard units of nanocuries per milligram, was measured in three to six sections per brain, corresponding approximately to plate 49 in the atlas of Paxinos and Watson (1986)
Statistical analysis. Data were analyzed by t test or by one-way ANOVA followed by Newman-Keuls post hoc multiple comparisons, with significance determined at p < 0.05.
RESULTS
Drug levels in serum
Steady-state levels of antidepressants were measured after 7-10 d of continuous infusion by osmotic minipump. The mean steady-state serum concentration obtained after administration of 10 mg/kg of paroxetine, 411 ± 78 ng/ml (Table 1) was much higher than that measured (80 ± 20 ng) after giving half the dose. Doses used for paroxetine (5 mg/kg) and desipramine (15 mg/kg) produced serum concentrations found within the therapeutic range (Table 1). The higher dose of paroxetine (10 mg/kg) produced serum concentrations larger than those recommended therapeutically (Table 1); however, because this dose was used by others examining the effect of paroxetine on SERT function (Piñeyro et al., 1994
Serum levels of the drugs at the end of each experiment were also measured to rule out effects caused by the presence of residual drug. At 48 hr after cessation of paroxetine (10 mg/kg) treatment (which is the common washout time used in many studies, e.g., Piñeyro et al., 1994
Effects on serotonin clearance parameters
Figure 1 shows the electrochemical signal produced by pressure ejection of the same amount of 5-HT (24 pmol) into the CA3 region of a control rat and a paroxetine-treated rat. In the paroxetine-treated rat, peak signal amplitude was markedly greater, and the time course of the signal was much longer than that measured in the control rat. To equalize the amplitude of the signal produced by 5-HT in control and SSRI-treated rats, the amount of 5-HT ejected was reduced so that similar baseline amplitude (0.6- 0.8 µM) was achieved in all treatment groups. In the SSRI-treated rats, the amount of 5-HT (7 ± 1 pmol) required to generate an electrochemical signal of equivalent amplitude to that seen in the control animals was significantly lower (21 ± 5 pmol; p < 0.01).
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Figure 1. Representative electrochemical signals generated by the local application of the same amount of 5-HT (24 pmol) into the CA3 region of a control (solid line) or a paroxetine-treated rat (dashed line). For clarity, only the oxidation current curves are shown.
A representative 5-HT signal generated by local application of exogenous serotonin in the CA3 region is shown in Figure 2. Consistent with an earlier report (Daws et al., 1998
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Figure 2. Representative 5-HT electrochemical signals from the CA3 region of dorsal hippocampus in a control (A) and a paroxetine-treated rat (B) before administration of fluvoxamine (solid line). The signal was generated by local application of 5-HT. The amount of 5-HT applied was 26 pmol for the control rat and 8 pmol for the paroxetine rat. The effect of local application of fluvoxamine on 5-HT clearance is illustrated by the dashed line. Fluvoxamine was pressure-ejected 60-90 sec before the next application of 5-HT. For clarity, only the oxidation current curves are shown.
Table 2 summarizes the effects of each antidepressant treatment on various 5-HT signal parameters obtained by in vivo chronoamperometry. In control rats, local application of the SSRI fluvoxamine significantly decreased the clearance of 5-HT from 33 to 56%, depending on the parameter measured. This inhibitory effect of fluvoxamine on 5-HT clearance parameters was also observed to be statistically significant in the groups of rats pretreated with either phenelzine or DMI. By contrast, in rats treated with either dose of paroxetine or with sertraline, the inhibitory effect of local application of fluvoxamine on these signal parameters was essentially abolished. For comparative purposes, the fluvoxamine-induced changes in the T80 value for each treatment group are shown in Figure 3. Only in rats treated with SSRIs was the fluvoxamine-induced change in the T80 value significantly less from that measured in the control rats. Similar results were obtained with the other clearance parameters (data not shown).
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Table 2. Effects of chronic antidepressant treatments on serotonin signal parameters
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Figure 3. Effects of antidepressants on fluvoxamine-induced changes in the T80 parameter of 5-HT clearance. Electrochemical recordings were performed in the CA3 region of dorsal hippocampus of rats treated for 21 d with paroxetine (PRX; 5 or 10 mg), sertraline (SRTL), desipramine (DMI), phenelzine (PHEN), or vehicle (CTR). Fluvoxamine was pressure-ejected 60-90 sec before the second application of 5-HT. Bars and brackets represent mean ± SEM. The number of animals in each group is indicated at the bottom of each bar. *p < 0.01 comparison of each treatment group with control group, ANOVA, Newman-Keuls post hoc comparison.
Effects on SERT density
Autoradiograms showing the effect of each drug treatment on the binding of [3H]CN-IMI in multiple brain areas are shown in Figure 4. It is apparent that treatment with the SSRIs markedly reduced binding, whereas treatment with either DMI or phenelzine did not. These values were quantified for the CA3 region of the hippocampus, the same area in which the electrochemical experiments were performed. These results are shown in Figure 5. Chronic treatment of rats with either dose of paroxetine or with sertraline resulted in a very marked reduction of [3H]CN-IMI binding, ~80-90%. Unexpectedly, DMI treatment caused a 50% increase in the binding of [3H]CN-IMI, whereas phenelzine treatment had no significant effect.
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Figure 4. Representative autoradiograms of [3H]CN-IMI (1 nM) binding in coronal rat brain sections taken at the level of plate 33 of the atlas of Paxinos and Watson (1986)
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Figure 5. Effects of antidepressants on [3H]CN-IMI binding (1 nM) in the CA3 region. Values are expressed as the percentage of the control value (100%), which is 351 ± 42 fmol/mg protein (n = 15). Bars and brackets represent mean ± SEM. The number of animals per drug-treated group is indicated at the bottom of each bar. *p < 0.01 comparison of each treatment group with control group, ANOVA, Newman-Keuls post hoc comparison.
Effects on serotonin content
Chronic treatment of rats with SSRIs had similar effects as lesioning rats with the serotonergic neurotoxin, 5,7-DHT, on 5-HT clearance parameters (Daws et al., 1998
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Table 3. Hippocampal content of 5-HT and 5-HIAA (ng/gm wet weight of tissue) Effects on mRNA levels for the SERT
In situ hybridization histochemistry was used to quantify mRNA levels of the SERT in the raphe nuclei to study if the effects of SSRI treatments were caused by a decrease in SERT gene expression. In Figure 6, representative coronal sections through dorsal and median raphe nuclei show a high level of mRNA labeling of the SERT in the dorsomedial, ventromedial, and lateral portions of the dorsal raphe as well as in the median raphe nucleus, both in a control and paroxetine-treated rat. Treatment with paroxetine (10 mg/kg) had no significant effect on the mRNA level for the SERT in the median raphe nucleus (Fig. 7); however the 33% increase in mRNA observed in the dorsal raphe nucleus in the paroxetine-treated rats almost reached significance (p < 0.058; t test).
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Figure 6. Serotonin transporter messenger RNA in the raphe nuclei of rats detected by in situ hybridization in a control and paroxetine-treated rat (10 mg/kg). Coronal brain sections were taken at the level of plate 49 of the atlas of Paxinos and Watson (1986)
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Figure 7. Effect of chronic paroxetine treatment (10 mg · kg
DISCUSSION
A key goal of the present study was to investigate possible functional changes produced by chronic antidepressant treatments on the functioning of the SERT in vivo and to determine if such changes correlate with alterations in the density of the SERT and/or its mRNA levels. To directly assess SERT function, chronoamperometry was used, a technique that examines SERT function in vivo by measuring the clearance of exogenously administered 5-HT. The present study demonstrated that only chronic treatment of rats with the SSRIs paroxetine and sertraline produced changes in SERT function, as evidenced by altered 5-HT clearance characteristics in response to fluvoxamine and by decreased SERT density.
Results from previous studies that examined the effect of chronic antidepressant treatment on SERT density and mRNA levels have been inconsistent (for review, see Blakely et al., 1997
Treatment with either paroxetine or sertraline induced a dramatic decrease in [3H]CN-IMI binding throughout brain (Fig. 4); quantitation of this effect in the CA3 region of hippocampus revealed an 80-90% decrease in binding (Fig. 5). A decrease of similar magnitude in SERT density has previously been observed after chronic treatment with paroxetine (Piñeyro et al., 1994
No changes in SERT density were found in rats chronically treated with the MAO inhibitor phenelzine, a result consistent with a previous study that examined the effect of chronic treatment with other MAOIs, clorgyline or selegiline (Yeghiayan et al., 1997
To assess SERT function in vivo, 5-HT signal recordings were measured within a discrete part of the CA3 region of the hippocampus where the norepinephrine transporter does not play a significant role in removal of exogenously applied 5-HT (Daws et al., 1998
The reductions of SERT function and density seen with paroxetine treatment (Figs. 3, 5) were similar to those observed after lesioning serotonin neurons with the neurotoxin 5,7-DHT (Hensler et al., 1994
In addition to protein synthesis, another important aspect of neuronal regulation is control of gene expression. In the present study, chronic administration of paroxetine failed to significantly alter mRNA level of SERT in the raphe nucleus (Figs. 6, 7). Similar findings have previously been reported based on either Northern blot analysis (Spurlock et al., 1994
Although the mRNA hybridization signal for the SERT in the raphe nucleus was not altered by chronic paroxetine treatment, we cannot exclude the possibility of a transient alteration in mRNA expression during the earlier stages of antidepressant treatment. Indeed, Neumaier et al. (1996)
The mechanism by which SSRIs such as paroxetine and sertraline downregulate the SERT is not currently known. Long-term SSRI administration could induce regulation at the posttranslational level. Using heterologous expression systems, Qian et al. (1997)
There is at least one interesting potential clinical implication of these data. There seems to be some proportion of depressed patients who respond beneficially to SSRI treatment but in whom the benefit wanes over time (Byrne and Rothschild, 1998
In conclusion, the therapeutic efficacy of SSRI and non-SSRI antidepressants probably derives from different adaptive changes. The SSRIs (paroxetine and sertraline) decrease SERT density and reduce SERT function, as indicated by failure of fluvoxamine to prolong 5-HT clearance. Whether this is produced by all SSRIs remains to be established. Nevertheless, non-SSRI antidepressants gave no evidence of altering SERT function and did not decrease SERT density.
FOOTNOTES Received June 24, 1999; revised Sept 13, 1999; accepted Sept. 16, 1999.
This work was supported by United States Public Health Service Grants, MH57001 (A.F.), MH53851 (D.A.M.), and MH01245 (G.A.G.). We thank Dr. Aurelio Galli for critical reading of this manuscript and helpful discussions.
Correspondence should be addressed to Dr. Saloua Benmansour, Department of Pharmacology, University of Texas Health Science Center at San Antonio, 7703 Floyd Curl Drive, San Antonio, TX 78284-7764. E-mail: benmansour{at}uthscsa.edu.
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