Serotonin Clearance In Vivo Is Altered to a Greater Extent by Antidepressant-Induced Downregulation of the Serotonin Transporter than by Acute Blockade of this Transporter

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The Journal of Neuroscience, August 1, 2002, 22(15):6766-6772

Serotonin Clearance In Vivo Is Altered to a Greater Extent by Antidepressant-Induced Downregulation of the Serotonin Transporter than by Acute Blockade of this Transporter
Saloua Benmansour¹, William A. Owens¹, Marco Cecchi¹, David A. Morilak¹, and Alan Frazer¹^,²
¹ Department of Pharmacology, University of Texas Health Science Center at San Antonio, San Antonio, Texas 78229, and ² South Texas Veterans Health Care System, San Antonio, Texas 78284

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Serotonin uptake, mediated by the serotonin transporter (SERT), is blocked acutely by antidepressants such as the selectiveserotonin reuptake inhibitors (SSRIs), but such blockade doesnot correlate temporally with the onset of therapeutic improvement.Treatment with SSRIs for 21 d induced downregulation of the SERT(Benmansour et al., 1999). The time course of SERT downregulationas well as the time course for its recovery after cessation oftreatment with the SSRI sertraline were investigated using tritiatedcyanoimipramine to measure SERT binding sites. To determine ifthere was a temporal correlation between the time when sertralineinduced downregulation of the SERT and when marked alterationin SERT function occurred, clearance of locally applied 5-HT intothe CA3 region of hippocampus was achieved using in vivo electrochemistry.After 4 or 10 d treatment with sertraline, SERT binding sitesdecreased very little (15-30%), and the chronoamperometric signalsfor serotonin in sertraline-treated rats were comparable withones obtained in control animals. By contrast, after 15 d of treatment,when SERT binding sites were markedly reduced by 80%, there wasrobust decrease in the clearance of 5-HT. Moreover, the functionalconsequences of SERT downregulation as measured by chronoamperometrywere significantly greater than those seen after acute blockadeof the SERT by SSRIs. SERT binding sites decreases are not a consequenceof reduced SERT gene expression, as revealed by in situ hybridizationmeasurements. SSRI-induced downregulation of the SERT may be akey component for the clinical response toSSRIs.

Key words: serotonin transporter; antidepressant; sertraline; chronoamperometry; downregulation; mRNA

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

It is widely believed that the onset of beneficial drug effect in depression is delayed for 2-3 weeks (Gelenberg and Chesen,2000), although some behavioral dimensions of the illness mayrespond more quickly (Katz et al., 1996, 1997). Early researchon antidepressants (ADs) focused on their acute effects on noradrenergicand/or serotonergic systems. The idea that there is a delay intherapeutic effect led to studies of their longer-term pharmacologiceffects, with much of this work focused on receptor regulation(Mongeau et al., 1997; Piñeyro and Blier, 1999). More recently,this work has been extended to studies of protein kinases, transcriptionfactors, and gene regulation (Duman et al.,1997, 1999; Popoliet al., 2000). What seems clear is that the acute pharmacologicenhancement of serotonergic and/or noradrenergic transmissionis what initiates the cascade of events that eventually producesclinical improvement (Delgado et al., 1999), although acute enhancementseems insufficient. Initially, enhanced transmission was thoughtto occur acutely as a direct consequence of AD-induced blockadeof either the serotonin transporter (SERT) and/or the norepinephrinetransporter. However, a variety of rapid compensatory mechanismsalso occur that diminish the ability of transporter blockade aloneto significantly enhance synaptic transmission. Subsequent tosuch rapid compensatory changes, regulatory responses then occur,primarily thought to involve receptor desensitization, that permitsynaptic transmission to be enhanced (Artigas et al., 2001). Thetime required for such secondary compensatory effects to occurand to enhance synaptic transmission has been speculated to accountfor the delay in therapeutic benefit (Artigas et al., 2001).

It is now recognized, however, that biogenic amine transporters are the key cellular elements regulating the concentrationof these transmitters in the extracellular fluid (Giros et al.,1996) and, furthermore, that these transporters can be regulatedin vitro. It has been shown that activation of protein kinaseC (PKC) induces SERT phosphorylation and sequestration and thatthis is associated with a decrease in the SERT activity. Thiseffect was shown to be modulated in vitro by 5-HT and selectiveserotonin reuptake inhibitors (SSRIs) (Ramamoorthy and Blakely,1999). Also recently it has been shown that SERT forms a complexwith the catalytic subunit of protein phosphatase 2A. These heteromericassemblies are subject to regulation by PKC activation or proteinphosphatase inhibition, which leads to phosphorylation and downregulationof the SERT (Bauman et al., 2000).

We found recently (Benmansour et al., 1999) that 21 d of treatment of rats with SSRIs, at clinically relevant and stable serumconcentrations (achieved by the use of osmotic minipumps), causedrobust downregulation of the SERT. In this study, the time coursefor such downregulation and its recovery is measured as well aspotential mechanisms producing these effects. Importantly, theconsequences of SERT downregulation on the functioning of theSERT in vivo was measured directly using chronoamperometry. Theuse of this technique revealed for the first time that such downregulationproduces a much more marked inhibition of 5-hydroxytryptamine(5-HT; serotonin) clearance in vivo than that seen after acuteblockade of the SERT withSSRIs.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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Animals. Male Sprague Dawley rats (Harlan, Indianapolis, IN) weighing 175-200 gm at the time of initiation of drug treatmentwere housed individually on a 12 hr light/dark cycle with lightson at 7:00 A.M. and with food and water provided ad libitum. Allanimal procedures were in strict accordance with the NationalInstitutes of Health Guide for the Care and Use of LaboratoryAnimals. All efforts were made to minimize both the number ofanimals used and stress or discomfort to the animal during theexperimentalprocedure.

Chronic drug treatments. Schedule of treatment for onset effects: rats were treated with sertraline (Pfizer, Groton, CT),7.5 mg · kg¹ · d¹ for 4, 10, 15, or 21 d, subcutaneously by means of osmotic minipumps(2ML4; Alza, Palo Alto, CA) to produce stable serum concentrations,and experiments were performed after 2 d of drug washout to reduceserum concentration to <2 ng/ml (Benmansour et al., 1999). Controlgroups received vehicle (50% ethanol:water).

Schedule of treatment for the time course of recovery: rats were treated with sertraline for 21 d followed by either 2, 6,8, 10, or 16 d ofwashout.

Autoradiographic procedures. After completing the treatment regimen and, for some rats, in vivo chronoamperometry recordings,rats were decapitated, and their brains were frozen quickly ondry ice and stored at $-$ 80°C until sectioning. Serotonin uptakesites were measured using [³H]-cyanoimipramine (CN-IMI) as a ligand (Kovachich et al., 1988;Benmansour et al., 1999). Brain sections (20 µm) were incubatedwith 1 nM [³H]-CN-IMI (80-85 Ci/mmol; American Radiolabeled Chemicals, St.Louis, MO) in a buffer consisting of 50 mM Tris, pH 7.4, and 120mM NaCl at 4°C for 24 hr. Nonspecific binding was defined using5 µM sertraline and was ~5% of total binding. Dried slide-mountedsections were placed into spring-loaded cassettes and apposedto tritium-sensitive film ([³H] Ultrofilm; Amersham Pharmacia Biotech, CEA AB, Sweden) at roomtemperature for 12-14 d. Autoradiograms were analyzed using NIHImage (National Institutes of Health (NIH), Bethesda, MD) andusing the Scion software package. Quantitation was achieved usingplastic-embedded tritium standards (American Radiolabeled Chemical)calibrated using brain mash sections. Measurements were takenat the level of plate 33 of the atlas of Paxinos and Watson (1986).The concentration of [³H]-CN-IMI used is approximately eight time its K_D value (Kovachichet al., 1988), so the values obtained approximate B_maxvalues.

In vivo chronoamperometry. This procedure was performed as described previously (Daws et al., 1998; Benmansour et al., 1999).Carbon fiber electrodes (30 µm tip diameter; 95-175 µm lengthin the active region) were coated with Nafion (a perfluorinatedion exchange resin), tested for sensitivity to 5-hydroxyindoleacetic acid (250 µM; Sigma, St. Louis, MO), and calibrated invitro to 5-HT. After completing the appropriate treatment andwashout time, rats were anesthetized with chloralose (70 mg/kg)/urethane(700 mg/kg) and the electrode, attached to a multibarrel pipette,was positioned in the CA3 region of the dorsal hippocampus. Theinternal diameter of each micropipette tip was 8-12 µm, and thedistance between electrode and pipette tips was 275-325 µm. Multibarrelmicropipettes were filled with either 5-HT (200 µM; Sigma), orfluvoxamine (400 µM; Pharmacia-Upjohn, Kalamazoo, MI). The pHof all solutions was 7.4. 5-HT was delivered by pressure ejectionin a volume of 26, 52, or 78 nl. High-speed chronoamperometricrecordings were made using the Fast-12 system (Censet, Lexington,KY). Oxidation potentials consisted of 100 msec pulses of +0.55V versus Ag-AgCl that were delivered one per second; the electrodewas held at a resting potential of 0.0 V between measurement.The reference electrode was positioned in the superficial cortex.Oxidation and reduction currents were digitally integrated duringthe last 80 msec of each 100 msec voltagepulse.

Several parameters are obtained from the electrochemical signal produced by exogenous applications of 5.2, 10.4, or 15.6 pmolof 5-HT. Parameters analyzed were signal amplitude; T80, the timeit takes for the peak amplitude to be reduced by 80%; and thetotal time course (t-course), the total time for the signal toreturn to baseline from the time of application of 5-HT.

In situ hybridization. Animals treated chronically with sertraline (7.5 mg · kg¹ · d¹) or vehicle (used for the in vivo chronoamperometry experiments)were killed by rapid decapitation. Brains were frozen in isopentaneon dry ice and stored at $-$ 70°C. Alternate series of 20 µm sectionswere cut through the dorsal raphe, thaw mounted onto silane-coatedglass microscope slides, fixed for 15 min in 4% paraformaldehyde,dehydrated, and stored at $-$ 70°C.

Methods for in situ hybridization were as described previously (Domyancic and Morilak, 1997; Benmansour et al., 1999). The660 nucleotide SERT riboprobe (obtained from Dr. Stanley WatsonUniversity of Michigan) was transcribed with the addition of $alpha$ -³⁵S-UTP (New England Nuclear, Boston, MA), to a specific activityof 2 × 10⁹ cpm/µg. Brain sections were hydrated, acetylated, and rinsedin 2× SSC (1× SSC is 150 mM sodium chloride, 15 mM sodium citrate,pH 7.2), then dehydrated, delipidated, and air-dried. Sectionswere incubated in hybridization buffer containing 4 × 10⁷ cpm/ml radiolabeled riboprobe (~20 ng/ml), overnight in a sealedhumidified chamber at 60°C.

All posthybridization solutions contained 1 mM dithiothreitol. After rinsing in four washes of 2× SSC and digesting with RNaseA (20 µg/ml, 30 min at 37°C), sections were taken through a seriesof increasingly stringent washes: 10 min each in 1×, 0.5×, and0.2× SSC at 24°C, followed by 3 × 1 hr in 0.1× SSC at 60°C. Theywere then rinsed, dehydrated, and apposed, along with 14C-radioactivestandards, to Kodak Biomax MR x-ray film for 24 hr before developing.Integrated signal density overlying the dorsal raphe, calibratedfrom the standards on each film, and expressed in standard unitsof nanocuries per milligram, was measured in three to six sectionsper brain corresponding approximately to plate 49 in the atlasof Paxinos and Watson (1986), using the NIH Image software package(version 1.55; Wayne Rasband,NIH).

Serum levels of sertraline. Serum was collected after 10 or 15 d treatment with sertraline to measure steady-state levels.Serum concentrations of sertraline were determined by HPLC asdescribed previously (Benmansour et al., 1999).

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 or by Mann-Whitney UTest for percentagecomparison.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Downregulation of the SERT

Chronic treatment with sertraline induced a time-dependent downregulation of SERT binding sites. Figure 1 shows data obtainedfrom the CA3 region of hippocampus, parietal cortex, and basolateralamygdala nucleus; similar data were observed throughout the restof brain. Sertraline caused only a modest reduction in SERT bindingsite density during the first 10 d of treatment (not more thana 25% decrease in [³H]-CN-IMI binding). This reduction became statistically significantat 10 d of treatment. After 15 d, a marked loss (>70%) of SERTbinding sites occurred, and this persisted with further treatmentup to 21 d. Shown also in Figure 1 is the recovery of bindingsites for the SERT after cessation of sertraline treatment. Recoverywas slow, taking at least 10 d after cessation of treatment toapproach values obtained in vehicle-treated rats (Fig. 1).

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Figure 1. Time course of the reduction (A) and recovery (B) of the binding of [³H]-CN-IMI (1 nM) after sertraline treatment. To study the onset of effects (A), rats were treated by osmotic minipump with sertraline (7.5 mg · kg¹ · d¹, s.c.) or vehicle (for control rats) for 4, 10, 15, or 21 d, always followed by a 2 d washout. To study the time course of recovery (B), rats were treated for 21 d with sertraline or vehicle followed by 2, 6, 8, 10, or 16 d of washout. Serotonin uptake sites were measured using quantitative autoradiography for [³H]-cyanoimipramine binding, as described in Materials and Methods. Results obtained were similar throughout the brain. Shown for illustration are results obtained in the CA3 region of the hippocampus, the parietal cortex (Par. CTX), and the basolateral amygdaloid nucleus posterior (BLP). The number of animals in each drug-treated group was four; the control group included eight animals. *p < 0.05 comparison of each time point for the treatment group with the corresponding time point of the control group. ANOVA, followed by Newman-Keuls post hoc comparison.

Clearance of 5-HT

Given that the time course for marked loss of SERT binding sites (10-15 d) corresponds to the time when drug-induced behavioralimprovement becomes evident in patients, it may be that the lossof SERT binding sites is important for achieving long-lastingand marked enhancement of serotonergic transmission with subsequentbehavioral improvement. Consequently, the functional consequencesof SSRI-induced loss of SERT binding sites was studied in detail.Measurement of SERT function was performed by in vivo chronoamperometryin rats treated with vehicle or sertraline for 4, 10, or 15 d.The primary measure in this study was the clearance of 5-HT afterpressure-ejection of exogenous 5-HT (5.2, 10.4, 15.6 pmol) intothe CA3 region of the hippocampus of vehicle- or sertraline-treatedrats. The CA3 region was selected for the study because previouswork has shown that the active clearance of 5-HT from the extracellularfluid of this brain area is caused primarily by activity of theSERT (Daws et al., 1998). Shown in Figure 2 is the chronoamperometricsignal caused by 5-HT in a control rat or in a rat treated withsertraline for 15 d, when robust downregulation of the SERT hasoccurred. After 15 d of sertraline treatment and the 2 d washoutperiod, the 5-HT signal was augmented markedly for each amountof serotonin applied into the CA3 region (Fig. 2). In the sertraline-treatedrat, each amount of 5-HT produced much larger peak signal amplitudeand a slower decline of the chronoamperometric signal than thatmeasured in the control rat.

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Figure 2. Representative 5-HT electrochemical signals from the CA3 region of the dorsal hippocampus in a control rat (dashed lines) and in one treated with sertraline for 15 d (solid lines). In vivo chronoamperomeric measurements were performed, as described in Materials and Methods, in rats treated with sertraline by osmotic minipump (7.5 mg · kg¹ · d¹, s.c.) for 15 d followed by a 2 d washout. Once reproducible electrochemical signals from 5-HT were obtained, the response to three different amounts of 5-HT (5.2, 10.4, 15.6 pmol) was tested in each drug-treated or control rat. For clarity, only oxidation current curves are shown. Each amount of serotonin produced a greater response in the sertraline-treated rat than in the control one.

In contrast, these effects were not seen in rats treated for 4 or 10 d with sertraline. Analysis of three representative serotoninsignal parameters (amplitude, T80, and time course) showed nostatistically significant increases either in the peak amplitudesof the signals produced by 5-HT or in the time course of clearanceof 5-HT in rats treated with sertraline for 4 or 10 d (Fig. 3).However, marked, significant increases in all these parameterswere measured in rats treated with sertraline for 15 d. The greatereffect on 5-HT clearance in rats treated with sertraline for 15d as compared with those treated for 10 d is not caused by differencesin the serum concentration of sertraline obtained in these animals.In the 10 d-treated rats, the serum concentration of sertralinewas 37.6 ± 5.5 ng/ml (n = 6), whereas it was 26 ± 3.4 ng/ml (n= 6) in those treated for 15 d (p > 0.05).

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Figure 3. Effect of increasing the amount of 5-HT on the serotonin signal of control and sertraline-treated rats. Rats were treated with vehicle or sertraline for 4, 10, or 15 d followed by 2 d of washout, as described in Materials and Methods. Several parameters are obtained from the electrochemical signal in response to local application of equal amounts of 5-HT (5.2, 10.4, or 15.6 pmol) into the CA3 region of the hippocampus of these rats. Parameters analyzed here were signal amplitude, T80, the time it takes for the peak amplitude to be reduced by 80%; total time course (t-course), the total time for the signal to return to baseline from the time of application of 5-HT. Each point represents the means ± SEM of an n of five to eight rats. *p < 0.05 comparison of each time point in the treatment groups with the corresponding time in the control group; ANOVA, followed by Newman-Keuls post hoc comparison.

The effect that sertraline-induced downregulation of the SERT has on the chronoamperometric signal caused by 5-HT was comparedwith that caused by acute SSRI-induced pharmacologic blockadeof the SERT. To do this, rats treated with vehicle at the sametime others rats were treated for 15 d with sertraline, were givenlocal application of both 5-HT and fluvoxamine into the CA3 regionof the hippocampus. As shown previously (Benmansour et al., 1999;Daws et al., 2000), local administration of an SSRI such as fluvoxamineinto the CA3 region caused a modest, statistically significanteffect on the clearance of 5-HT, as reflected by the increasein the T80 value, but had no significant effect on peak amplitude(Table 1). Similarly, acute systemic administration of the SSRIparoxetine (10 mg/kg, i.p.) caused an increase in the 5-HT clearanceparameter, T80, comparable with that seen with local applicationof fluvoxamine directly into the CA3 region, while having no significanteffect on signal amplitude (Table 1). However, chronic treatmentof rats with sertraline caused a significantly greater effecton the T80 value than that seen with either local or acute systemicadministration of an SSRI, and furthermore, such chronic treatmentcaused a significant increase in signal amplitude as well (Table1).


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Table 1. Effects of SSRIs on serotonin signal parameters

mRNA for the SERT

Previously, we have shown that 21 d of treatment with the SSRI paroxetine had no effect on SERT gene expression (Benmansouret al., 1999). To determine if changes occurred at earlier stagesduring treatment, mRNA for the SERT was measured in the dorsalraphe nucleus (DRN) by in situ hybridization in the same ratsused for the [³H]-CN-IMI binding experiments. Message levels for the SERT increasedslowly, reaching a statistically significant increase, by a maximumof 29% after 10 d of treatment, then decreased back to baselineafter 21 d of treatment (Fig. 4). Message levels again rose significantly6 d after 21 d of treatment was terminated, and then returnedback to control levels rapidly (Fig. 4). Shown also for comparativepurposes in Figure 4 are SERT binding sites in the DRN. Transientincreases in mRNA early in the course of treatment may have opposedthe SSRI-induced downregulation of SERT binding sites. Only whenmessage levels had declined after the initial increase did SERTbinding sites show a marked reduction. However, the short-livedincrease in message after the cessation of treatment is accompaniedby a more sustained increase in binding sites.

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Figure 4. Time course of the effect of sertraline treatment and cessation of treatment on the density and mRNA levels of the SERT in the dorsal raphe nucleus. SERT density (solid line) was measured by quantitative autoradiography of [³H]-CN-IMI (1 nM) binding, and mRNA levels for the SERT (dashed line) were measured by in situ hybridization in the same group of animals treated with sertraline, as described in Materials and Methods. Each point is expressed as a percentage of respective control values ± SEM of an N of 4-11 rats. SEM for percentage of control binding is shown by the dashed horizontal lines, and the one for percentage of control mRNA is shown by the solid horizontal lines. Control values for [³H]-CN-IMI in the DRN were 3097 ± 70 fmol/mg of protein, and the mean integrated density for mRNA levels in control rats was 2.27 ± 0.3 nCi/mg. The x-axis of the graph represents the number of days of treatment plus the washout time. Up to 23 d, this represents a variable number of treatment days plus a fixed 2 d washout time. After day 23, the numbers represent a fixed 21 d treatment plus a variable number of washout days. *p < 0.05 comparison of each time point of treatment with the appropriate time point of the control group; ANOVA followed by Newman-Keuls post hoc comparisons.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

These results demonstrate that sertraline-induced decreases in SERT binding site density are not caused by decreased SERTgene expression, but recovery of binding sites after cessationof treatment may be attributable to increased synthesis of theSERT after an increase in gene expression. The time course ofrecovery of binding sites is consistent with the turnover rateof the SERT (Vicentic et al., 1999). Most importantly, these datashow that the time-dependent loss of SERT binding sites has amuch greater effect on the 5-HT electrochemical signal than thatseen after acute blockade of the transporter with SSRIs, eithergiven locally orsystemically.

Although a small increase of serotonin peak signal amplitude (~30%) after local application of fluvoxamine has been observedearlier in our laboratory (Daws et al., 1998), this small effecton amplitude is no longer observed consistently as we have refinedthe technique (Benmansour et al., 1999; Daws et al., 2000) andwas not observed in the present study. This lack of effect offluvoxamine on serotonin signal amplitude is not caused by theuse of low dose of fluvoxamine (Daws et al., 1998, 2000). Furthermore,differences in 5-HT clearance observed in rats treated for 10versus 15 d with sertraline is not caused by these rats achievingdifferent serum concentrations of this SSRI and therefore, isunlikely to be caused by differences in occupancy of the SERTat thistimes.

Consistent with the inability of acute local application of an SSRI to raise the peak amplitude of the 5-HT electrochemicalsignal (Benmansour et al., 1999; Daws et al., 2000), there wasalso little to no change in maximal amplitude of the 5-HT electrochemicalsignal evoked in a brain slice preparation by either a singleelectrochemical pulse or a train of pulses (Bunin and Wightman,1998; Bunin et al., 1998). Thus, the inability of acute blockadeof the SERT to increase peak signal amplitude is seen both withexogenously administered 5-HT and with the evoked release of endogenous5-HT.

The loss of SERT binding sites has a much greater effect on the 5-HT electrochemical signal than that seen with acute blockade.Peak signal amplitude was markedly increased (approximately twofold),and clearance of 5-HT was delayed even more after SERT downregulationthan that seen with acute blockade (Table 1). These effects aresimilar to those seen after lesions of serotonin neurons withthe neurotoxin 5,7-dihydroxytryptamine (Daws et al., 1998). Itseems likely that this marked effect on 5-HT clearance is causedby the "absence" ofSERT.

The parameters used to analyze quantitatively the serotonin electrochemical signal (e.g., T80 values, total time course) wereselected because they clearly and reproducibly detect effectsof uptake inhibitors and are also known to reflect primarily theuptake process rather than metabolism or diffusion (Cass et al.,1993). However, the detection of neurotransmitter injected intobrain by a sensor located some distance from the site of injectionis a complex phenomenon. Factors that influence the shape of thesignals detected include not only uptake of the transmitter butalso its diffusion in obstructed extracellular space (Nicholsonand Phillips, 1981), as well, perhaps, as metabolism. In addition,experimental factors such as administration of material by, forexample, microiontophoresis versus pressure ejection (Gerhardtand Palmer, 1987), the internal diameter of the ejection pipette,and the distance between the ejection site and the detector (Nicholson,1995) can strongly influence the results obtained. Finally, withrespect to the uptake process itself, which is characterized withMichaelis-Menten kinetics, the V_max or K_m of the transporter inthe detection areas can also influence the data obtained (Wightmanand Zimmerman, 1990; Nicholson, 1995). Perhaps the best attemptto model such data is the elegant paper of Nicholson (1995), whoderived numerical solutions to this three-dimensional diffusionproblem with nonlinear uptake using the integral equation approachof Tosaka and Miyake (1982). Of the theoretical curves generatedfor dopamine using this approach, none are exactly like the electrochemicalsignals measured in vivo for serotonin (Fig. 2), but this maybe attributable to their analysis being based on microiontophoreticapplication versus the pressure-ejection technique used in thisstudy. Nevertheless, comparison of our signals with the theoreticalcurves obtained by Nicholson (1995) shows quite clearly that weare working at a distance between the micropipette ejection tipand the carbon fiber electrode where uptake does contribute tothe clearance and where measurable signals are detected. Underour experimental conditions of pressure-ejection of 5-HT, uptakeis strongly related to the magnitude of V_max. Consequently, reductionof V_max to 0, i.e., the "no uptake" condition in Nicholson's model(which could approximate in our case situations of SERT loss aftereither chronic SSRI treatment or 5,7-DHT lesions), increases signalamplitude and slows clearance very substantially, much more sothan increases in K_m as a result of local application of a competitiveinhibitor. Our results then, are in good agreement with Nicholson'smodel.

Our data are consistent with that obtained using in vivo microdialysis in which chronic treatment of rats with SSRIs causedmuch greater increases in extracellular 5-HT than seen with singleacute systemic administration of an SSRI (Bel and Artigas, 1993;Rutter et al., 1994; Kreiss and Lucki, 1995; Tanda et al., 1996;Hervás et al., 2001). The interpretation of these microdialysisresults has, to date, focused on the hypothesis that chronic SSRItreatment produces desensitization of somatodendritic 5-HT1A autoreceptorsthat normally mediate feed-back inhibition of 5-HT release (Rutteret al., 1994; Invernizzi et al., 1994; Kreiss and Lucki, 1995).Thus, somatodendritic autoreceptor desensitization has been speculatedto play a key role in the ability of SSRIs to enhance serotonergictransmission over time to initiate behavioral improvement. Thedata in this report, though, describe for the first time an alternativeor, at least, an additional mechanism for the elevated levelsof extracellular 5-HT seen with chronic drug administration, i.e.,SERT downregulation facilitating the entry of 5-HT into the extracellularfluid to a greater extent than can be achieved by acute uptakeinhibition.

Studies of the effect of chronic antidepressants on the SERT have resulted in inconsistent reports (Owens and Nemeroff, 1998).Among the factors that may contribute to such inconsistency isthe route of drug administration. In most studies of chronic administrationof ADs to rats, the drugs are given either intraperitoneally orsubcutaneously, either once or twice daily. As rats metabolizethese drugs more rapidly than humans, such dosage schedules canresult in appreciable fluctuations in the serum concentrationof drug throughout the day. For certain pharmacologic effects,sustained drug action may be needed. A good example of this isa recent study (Cremers et al., 2000) of citalopram, which hasa half-life in the rat of 3-5 hr (Fredricson Overo, 1982; Melzackaet al., 1984). It was shown that chronic treatment with citalopraminduced a marked subsensitivity of somatodendritic 5-HT1A receptorsonly when given by osmotic minipump as opposed to daily injection.It seems likely also that sustained high occupancy of the SERTby SSRIs is needed to demonstrate regulatory effects (Piñeyroet al., 1994; Blier and Bouchard, 1994; El Mansari et al., 1995;Benmansour et al., 1999). Importantly, because the half-livesof many SSRIs in humans are >20 hr (Hiemke and Hartter, 2000),it is likely that these drugs are producing sustained pharmacologiceffects throughout the day inpatients.

To the extent that effects measured using chronoamperometry and exogenous administration of transmitter reflect changes insynaptic serotonergic transmission, it would seem that SSRIs causeonly a modest increase of transmission early in treatment. Onlyafter sustained treatment, when these drugs induce a loss of SERTbinding sites, would there be a marked enhancement of transmission.Importantly, the time required for this to occur approximatesthe time required for clinical improvement in behavior to becomemanifest (Quitkin et al., 1987). Thus, the loss of SERT bindingsites may be an important mechanism to further increase the initialmodest elevation in serotonergic transmission that occurs afteracute pharmacologic blockade of the transporter. Such mechanismscould involve phosphorylation and sequestration of transporter,as shown in vitro (Ramamoorthy and Blakely, 1999; Bauman et al.,2000), but this has yet to be demonstrated in vivo. Understandingthe mechanisms leading to SERT downregulation may permit the developmentof drugs that can induce this effect more rapidly, allowing perhapsa more rapid course of clinicalimprovement.

  FOOTNOTES

Received Jan. 11, 2002; revised May 3, 2002; accepted May 7, 2002.

This work was supported by Research Funds from Department of Veterans Affairs and United State Public Health Service GrantsMH57001 (A.F.) and MH53851 (D.A.M.). We thank Drs. GeorgiannaG. Gould and Martin A. Javors for providing help in measuringserum concentrations ofsertraline.

Correspondence should be addressed to Dr. Saloua Benmansour, Department of Pharmacology, University of Texas Health ScienceCenter at San Antonio, 7703 Floyd Curl Drive, San Antonio, TX78229-3900. E-mail: benmansour{at}uthscsa.edu.

  REFERENCES

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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