Chronic Treatment of C6 Glioma Cells with Antidepressant Drugs Results in a Redistribution of Gsalpha

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Vol. 59, Issue 6, 1426-1432, June 2001

Chronic Treatment of C6 Glioma Cells with Antidepressant Drugs Results in a Redistribution of Gs $alpha$

Robert J. Donati, Chandrashekhar Thukral, and Mark M. Rasenick

Departments of Physiology and Biophysics (R.J.D., C.T., M.M.R.) and Psychiatry (M.M.R.), University of Illinois at Chicago, College of Medicine, Chicago, Illinois

	Abstract

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Previous studies have demonstrated that chronic treatment of C6 glioma cells with the antidepressants desipramine and fluoxetineincreases the Triton X-100 solubility of the G protein Gs $alpha$ (Tokiet al., 1999). The antidepressants also caused a 50% decreasein the amount of Gs $alpha$ localized to caveolae-enriched membrane domains.In this study, laser scanning confocal microscopy reveals thatGs $alpha$ is localized to the plasma membrane as well as the cytosolin both treated and control cells. However, striking differencesare seen in the distribution of Gs $alpha$ in the long cellular processesafter chronic treatment with these antidepressant drugs. Controlcells display Gs $alpha$ along the entire process with an especiallyhigh concentration of that G protein at the distal ends. Desipramine-or fluoxetine-treated cells show a more centralized clusteringof Gs $alpha$ in the Golgi region of the cell and a drastic reductionof Gs $alpha$ in the cellular processes. There is no change in the distributionof Go $alpha$ after desipramine treatment and the antipsychotic drugchlorpromazine does not alter Gs $alpha$ . These results suggest thatantidepressant-induced changes in the association of Gs $alpha$ withthe plasma membrane may translate into altered cellular localizationof this signal transducing protein. Thus, modification of thecoupling between Gs-coupled receptors and adenylyl cyclase mayunderlie both antidepressant therapy and depressive illnesses.This report also suggests that modification of the membrane domainoccupied by Gs $alpha$ might represent a mechanism for chronic antidepressanteffects.

	Introduction

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Over the past 4 decades, electroconvulsive therapy and antidepressant drugs have been used for the treatment of clinical depressionand other psychiatric disorders. Several distinct pharmacologicalcompounds show therapeutic efficacy. These include monoamine oxidaseinhibitors, tricyclic compounds, selective serotonin and norepinephrinereuptake inhibitors, as well as some atypical drugs. The possibilitythat these diverse agents converge on a single postsynaptic targethas been an area of great research interest. Menkes et al. (1983)first reported that long-term administration of various antidepressantsenhanced guanylyl-5'-imidodiphosphate- and fluoride-stimulatedadenylyl cyclase activity in rat cortex and hypothalamus membranes.This suggested that the stimulatory $alpha$ -subunit of the Gs proteinwas a target of antidepressant action and that antidepressanttreatment facilitated the activation of adenylyl cyclase by Gs.These initial findings involving the stimulation of adenylyl cyclasevia Gs $alpha$ after antidepressant treatment have been substantiatedby later studies (Ozawa and Rasenick, 1989, 1991; De Montis etal., 1990; Kamada et al., 1999). Increased cAMP activity has beendemonstrated in rat cerebral cortex in response to antidepressanttreatment (Perez et al., 1989, 1991). Consistent with these findings,it has been reported that chronic antidepressant treatment increasesthe expression and activity of cAMP response element binding proteinin the rat brain (Nibuya et al., 1996; Duman et al., 1997; Takahashiet al., 1999; Thome et al., 2000). Furthermore, similar antidepressant-inducedincreases in guanylyl-5'-imidodiphosphate-stimulated adenylylcyclase activity have been observed in vitro using C6 glioma cells(Chen and Rasenick, 1995a).

There has been much recent interest in the organization of G protein signaling complexes at the plasma membrane (Huang etal., 1997). G proteins interact with several other membrane-associatedproteins and are unlikely to diffuse freely through the plasmamembrane (Neubig, 1994). The localization of G proteins to specificmembrane domains such as caveolae (Li et al., 1995) and raftshas generated interest in these cholesterol- and sphingolipid-rich,detergent-resistant membrane domains and how they effect G proteintargeting and function (Brown and London, 2000; Moffett et al.,2000). Bayewitch et al. (2000) have shown that chronic exposureto agonists of Gi $alpha$ - coupled receptors leads to a decrease in thecholate solubility of these G protein subunits and a "superactivation"of adenylyl cyclase. These studies indicate that the lipid environmentof the G protein may play an important role in itsfunction.

Previous studies demonstrated that Gs $alpha$ from C6 rat glioma cells migrates from a Triton X-100 (TTX-100) insoluble membranedomain to a TTX-100 soluble membrane domain in response to chronicantidepressant treatment (Toki et al., 1999). In this same study,it was also reported that there was a comigration of adenylylcylase with Gs $alpha$ into the more TTX-100 soluble membrane fractions.Interestingly, there was no comparable shift in the localizationof Gi $alpha$ to a more TTX-100 soluble membrane domain after antidepressanttreatment, suggesting that the antidepressant effect on G proteinmembrane localization is Gs $alpha$ specific.

Immunofluorescence laser scanning confocal microscopy was used to investigate the effect of chronic antidepressant treatmenton the distribution of Gs $alpha$ in C6-2B cells. This study reportsthat chronic antidepressant treatment results in the redistributionof Gs $alpha$ from the cell processes and process tips to the cell body.This may be caused in part by an alteration of the lipid environmentin which Gs $alpha$ normally resides, allowing the protein to be moremobile and thus able to interact with downstream effectors. Onthe other hand, antidepressant-induced increased mobility of Gs $alpha$ may be caused by a disruption of the interactions between Gs $alpha$ and other membrane-bound proteins or cytoskeletalelements.

	Materials and Methods

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Cell Culture. C6-2B cells (between passages 30 and 50) were plated onto coverslips and allowed to attach overnight in Dulbecco's modifiedEagle's medium, 4.5 g/l glucose, 10% bovine serum, and 100 µg/mlpenicillin and streptomycin at 37°C in a humidified 10% CO₂ atmosphere.As reported previously, desipramine treatment regimens of 3 µMfor 5 days and 10 µM for 3 days yielded similar biochemical results(Chen and Rasenick, 1995b). Therefore, the latter treatment paradigmwas used in these experiments because it was easier to maintainthe cell cultures for 3 days. In some instances, 10 µM fluoxetinewas used. The culture media and drug were changed daily. Neitherdesipramine nor fluoxetine treatment altered cell growth (as determinedby the confluence of the cell monolayer and total protein estimation)or cell viability (as determined by 4,6-diamidino-2-phenylindolestaining and visualization under a fluorescence microscope withUV light). During the treatment duration, no morphological changeswere observed in the cells. After the treatment duration, thecells were incubated in drug-free media for 45 to 60 min beforefixation.

Indirect Immunofluorescence Laser Scanning Confocal Microscopy. After treatment, cells were washed once with phosphate-buffered saline (PBS; 136 mM NaCl, 2.6 mM KCl, 5.4 mM Na₂PO₄·7H₂O,pH 7.4) and fixed with ice-cold methanol for 10 min. Cells werethen washed three times with PBS followed by 2 h of blocking in5% normal goat serum/0.2% fish skin gelatin in PBS. Primary antibodywas added for 1.5 h, Gs $alpha$ /RM1 (PerkinElmer Life Sciences, Boston,MA) 1:50 and Go $alpha$ (Santa Cruz Biotechnology, Santa Cruz, CA) 2µg/ml, followed by three washes with PBS. Oregon Green-labeledsecondary antibody (Molecular Probes, Eugene, OR) was added ata concentration of 8 µg/ml for 1 h followed by three PBS washes.The coverslips were mounted onto slides with Vectashield (VectorLaboratories, Burlingame, CA) containing diamidino-2-phenylindoleas a mounting medium. Images were acquired using a Zeiss LSM510laser-scanning confocal microscope (Carl Zeiss Inc., Thornwood,NY). A single 488-nm beam from an argon/krypton laser was usedfor excitation of the Oregon Green. Differential interferencecontrast images were also acquired. Five experiments were performedand coverslips were examined. Approximately 2100 cells from controland desipramine-treated coverslips were counted by two investigatorsblind to the experimental conditions over the course of the fiveexperiments.

Fluorescence Quantification. The cellular distribution of Gs $alpha$ was quantified in confocal imaged C6-2B cells using NIH-Image software (http://rsbinfonihgov/nih-image)as described previously (Southwell et al., 1998a,b; Jenkinsonet al., 1999). Images of 9 × 1 µm optical, planar sections takenfrom four randomly selected control and four randomly selecteddesipramine-treated cells were captured and the middle five sectionsfrom each cell were quantified. Total cellular Gs $alpha$ fluorescencewas measured by counting the number of pixels with intensity abovethreshold (determined by minimum intensity above background, inthis case 50 pixels). The areas of intensity were numbered anddivided visually into those localized to the cell body and thoselocalized to the processes and process tips. The total from eachregion was divided by the total cell pixel intensity and expressedas a percentage of total. This was done for each section of eachcell and the sections were averaged per cell to give an averagepercentage total percell.

In a separate investigation, seven sets of 300 cells each from control group and desipramine-treated cells from five experimentswere counted to determine the primary localization (processesand process tips or cell body) of Gs $alpha$ within these cells. Themajority of the cells stained positively for Gs $alpha$ throughout theentire cell, but there was usually an enhancement in one of theseregions. Overly flattened and fragmented cells were omitted fromcounting, as were cells that did not display processes. The countsare displayed as the ratio of process and process tip localization/cellbodylocalization.

Data Analysis. Images were evaluated by two investigators blinded to the treatment condition. Student's t test was performed for statisticalanalysis. Values of p < 0.05 were taken to indicatesignificance.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Chronic Antidepressant Treatment Leads to a Shift in the Cellular Localization of Gs $alpha$ . Studies have shown that chronic antidepressant treatment of C6-2B glioma cells alters the detergent solubility of Gs $alpha$ (Tokiet al., 1999). C6-2B cells were treated with the tricyclic antidepressantdesipramine (10 µM) for 3 days and were then examined by laserscanning confocal microscopy to visualize these changes in membranelocalization. Examination of 300 to 500 control and desipramine-treatedcells by three independent researchers revealed that desipraminetreatment did not alter the overall structure of C6-2B cells (Fig.1), but drastically reduced the presence of Gs $alpha$ in the processtips (Fig. 2, arrowheads and Fig. 3). In addition, there was anincrease in the presence of Gs $alpha$ within the cell body of many ofthe desipramine-treated cells (Fig. 2, arrows), as well as a decreasewithin the cell processes themselves (Fig. 2, asterisks). In someinstances, there was an intense clustering of Gs $alpha$ staining inthe cell body (Fig. 2C, arrows), but the majority of the cellsdid not exhibit such a focused increase in Gs $alpha$ staining.

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Fig. 1. Chronic desipramine treatment of C6-2B glioma cells does not alter the overall shape of the cell. Differential interference microscopy images of control and desipramine treated C6-2B cells are shown to demonstrate similarities in overall cell shape between the two groups. Cells were treated and processed for microscopy as described under Materials and Methods. A representative image of five independent experiments is shown. Bar, 10 µm.

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Fig. 2. Chronic desipramine treatment results in an enhancement of Gs $alpha$ immunofluorescence in the cell body and a decrease in the cell processes and process tips. Untreated C6-2B glioma cells (A and B) display ubiquitous staining of Gs $alpha$ with an enhancement at the process tips (arrowheads) and cell processes (asterisks). Desipramine treated cells (C and D) show a decrease in Gs $alpha$ staining at the process tips (arrowheads) and cell processes (asterisks) and simultaneously display an increase in cell body staining (arrows). Cells were treated and prepared for microscopy as described previously. Bar = 10 µm.

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Fig. 3. Enlarged view of the process tips in control versus desipramine treated C62B cells shown in Fig. 2. The process tips from the control cell in Fig. 2A were enlarged to show the intense Gs $alpha$ staining (A and B) and the corresponding process tips of the desipramine treated cell in Fig. 2C are shown to demonstrate the reduction of Gs $alpha$ staining after antidepressant treatment (C and D).

Twenty-one hundred cells from each group (control versus desipramine-treated) over a series of five experiments were examinedto quantify the extent of the antidepressant effect. The cellswere grouped into two categories: those that displayed intensestaining at the process tips as well as overall staining in theprocesses and cell body (category A) versus those that displayedintense staining in the cell body region and decreased processand process tip staining (category B). Abnormal cells or thosenot displaying processes were not included in the cell count.Cells (300-450) were counted per experiment and the ratio of categoryA cells to category B cells for each group is shown in Fig. 4.Twice as many control cells (64%) displayed Gs $alpha$ staining at theprocess tips and throughout the entire cell than those treatedwith desipramine (32%). This demonstrates that Gs $alpha$ relocalizationis not an all-or-none response to antidepressant treatment andthat some cells may be more responsive to treatment than others.

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Fig. 4. Qualitative differences between control and desipramine-treated cells demonstrate a loss of Gs $alpha$ staining in the cell processes and process tips. Over 2000 cells from each group were counted as described under Materials and Methods and the ratio of cells displaying an intense process and process tip staining to those displaying intense cell body staining is displayed in the graph. There is a 2-fold difference in the ratio of process tip staining to cell body staining in desipramine-treated cells. These results were determined to be significant by a paired Student's t test; **p < 0.05.

To determine quantitative differences between the groups, five 1 µm optical, planar sections through each of four cells ineach group were examined by confocal microscopy and the digitalimages were captured. These images were then analyzed using theprogram NIH Image according to methods published previously (Southwellet al., 1998a

; Jenkinson et al., 1999

). This was done to accountfor changes in Gs $alpha$ localization at different focal planes of thecell. The percentages of Gs $alpha$ localized to the cellular processesand process tips of control versus treated cells were comparedby dividing the pixel density above threshold in these regionsby the total cellular pixel density (Table 1). There was a 3-folddecrease in Gs $alpha$ localization in the processes and process tipsbetween control cells and desipramine-treated cells as 12% ofthe total cellular Gs $alpha$ was located in the process tips of controlcells versus 4% present in the tips after desipramine treatment.

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TABLE 1
Percentage of Gs $alpha$ Immunofluorescence Distribution in the Cell

Antidepressant Induced G Protein $alpha$ Subunit Cellular Relocalization Is Specific to Gs. To determine whether antidepressant-induced mobility is specific to Gs $alpha$ , Go $alpha$ distribution was examined in approximately 500cells under the same treatment conditions. Figure 5 demonstratesthat there was little if any change in the distribution of Go $alpha$ after desipramine treatment. Go $alpha$ appears throughout the cell withoutspecific regions displaying an increased staining intensity incontrol or treated cells. Some of the control cells (Fig. 5, Aand B) have a slight increase in staining intensity at the processtips, but this is also seen in the treated cells (Fig. 5, C andD), indicating that antidepressant treatment does not effect Go $alpha$ localization within the cell.

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Fig. 5. Go $alpha$ does not undergo antidepressant induced relocalization. Untreated (A and B) and desipramine-treated (C and D) cells show similar Go $alpha$ immunofluorescence profiles. There is staining throughout the cell body and processes of both sets of cells. The figure is typical of approximately 500 cells that were examined. Bar, 10 µm.

Fluoxetine Treatment Also Promotes Gs $alpha$ Migration. If the redistribution of Gs $alpha$ is truly an antidepressant effect, then other classes of antidepressant drug should have a similareffect. Desipramine and fluoxetine have both been shown to evokea similar biochemical redistribution of Gs $alpha$ (Toki et al., 1999).Confocal microscopic images of C6-2B cells treated with 10 µMfluoxetine for three days show a similar Gs $alpha$ staining patterncompared with desipramine-treated cells (Fig. 6 A). The most strikingsimilarity of desipramine and fluoxetine effects on Gs $alpha$ localizationis the loss of staining in the processes and process tips (compareFig. 2, C and D, and Fig. 6A with Fig. 2, A and B). Approximately100 cells were examined for qualitative differences as describedabove for Fig. 4. Of the fluoxetine-treated cells, 45% displayedintense staining in the process tips compared with the 64% ofcontrol and 32% of desipramine-treated cells mentioned previously.

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Fig. 6. Fluoxetine (10 µM) treatment for 3 days has effects similar to those of desipramine on Gs $alpha$ cellular localization. Cells were treated with fluoxetine (A) or chlorpromazine (B) and processed for confocal microscopy as described under Materials and Methods. Like desipramine, fluoxetine treatment results in a drastic reduction of Gs $alpha$ immunofluorescence in the cell process (arrow) and process tips (arrowhead), whereas chlorpromazine treatment results in a uniform distribution of Gs $alpha$ similar to control (compare to Fig. 2, A and B). The differential interference contrast image to the right of the fluorescence image shows that these drugs have no effect on global cell shape. Bar, 10 µm.

Chlorpromazine Treatment Does Not Alter the Distribution of Gs $alpha$ . The antipsychotic drug chlorpromazine was used as a control for antidepressant effects. When cells were treated with 10 µMchlorpromazine for 3 days, Gs $alpha$ staining was evident throughoutthe cell body (Fig. 6 B). There is Gs $alpha$ immunostaining throughoutthe cell body, cell process, and process tip. This pattern ofGs $alpha$ distribution was similar to other control cells; 68% of approximately100 cells demonstrated distinct staining in the cell processesand processtips.

Other Treatment Paradigms Have a Similar Effect on Gs $alpha$ . A lower dosage and longer exposure time for desipramine treatment (3 µM for 5 days) was also tested. Control cells have intensestaining at the process tips, whereas the desipramine treatedcells do not (data not shown). The main difference between thehigh-dose/3-day and the low-dose/5-day treatment regimens is thecell body localization of Gs $alpha$ . A majority of C6-2B cells treatedwith 10 µM desipramine display intense clustering of Gs $alpha$ in theperinuclear region whereas cells treated with 3 µM desipramineshow a more even distribution between intense cell body stainingand a more nondescript staining. One-day/10 µM desipramine treatmentof C6-2B cells resulted in a Gs $alpha$ distribution similar to thatof cells treated with 3 µM for 5 days (data not shown). Underthe acute treatment condition (1 day, 10 µM) the number of cellslacking Gs $alpha$ in the process tips was not significantly differentfrom the control cell population seen in Table 1 and Fig. 4.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Over the past several decades, there has been a great deal of research attempting to determine a common mechanism of antidepressantaction. Such a mechanism, if a single one exists, has yet to beclearly established. One of the classic hallmarks of chronic antidepressanttreatment is the down-regulation of several types of neurotransmitterreceptor in the brain (Sulser, 1984) and $beta$ -adrenergic receptorsin rat C6 glioma cells (Fishman and Finberg, 1987). However, thetime course between the change in the receptor number and theclinical efficacy of antidepressant treatment cannot be fullyexplained by these biochemical data (Rasenick et al., 1996).

More recently, much work has focused on postreceptor neuronal cell signaling processes as mechanisms of antidepressant action(Ozawa and Rasenick, 1989; Duman et al., 1997; Takahashi et al.,1999; Toki et al., 1999; Thome et al., 2000). The downstream effectsinvolving cAMP have been the focus of much of this previous work(Perez et al., 1989, 1991; Nibuya et al., 1996; Duman et al.,1997; Takahashi et al., 1999; Thome et al., 2000). Toki et al.(1999) demonstrated that antidepressant treatment results in analteration in the detergent extractability of Gs $alpha$ from the plasmamembrane of C6 glioma cells and rat cerebral cortex. Altered detergentsolubility of Gi $alpha$ and G $beta$ $gamma$ has also been demonstrated after chronicactivation of Gi/o-coupled opiate receptors (Bayewitch et al.,2000). This change in detergent solubility corresponds to adenylylcyclase "superactivation". The current study centers on the visualizationof these changes in the detergent solubility of Gs $alpha$ after antidepressanttreatment using laser scanning confocal microscopy. The resultsof this study suggest that the cellular localization of Gs $alpha$ isaltered after chronic antidepressanttreatment.

In this study, it was demonstrated that chronic antidepressant treatment of C6 glioma cells results in a change in the cellularlocalization of Gs $alpha$ (Figs. 2-4 and 6). This redistribution of Gs $alpha$ was observed with two types of antidepressants: desipramine, atricyclic compound (Figs. 2-4), and fluoxetine, a selective serotoninreuptake inhibitor (Fig. 6A). Chlorpromazine, an antipsychoticagent with chemical similarities to tricyclic antidepressants,did not alter the distribution of Gs $alpha$ (Fig. 6B). Previous studieshave suggested that activated Gs $alpha$ can be released from the plasmamembrane into the cytosol; these results are certainly consistentwith those observations (Rasenick et al., 1984; Ransas et al.,1989; Levis and Bourne, 1992). Furthermore, the distribution ofGo $alpha$ was not modified by antidepressant treatment (Fig. 5). Theunique antidepressant response of Gs $alpha$ was also seen previously,as Gi $alpha$ solubility in TTX-100/TTX-114 was unchanged by desipraminetreatment (Toki et al., 1999). The data reflect a genuine redistributionof Gs $alpha$ , because the amount of this G protein is not altered byantidepressant treatment (Chen and Rasenick, 1995a; Emamghoreishiet al., 1996; Toki et al., 1999). Thus, these data suggest a reorganizationof the extant pool of Gs $alpha$ rather than an increase in proteinsynthesis.

The notion that G protein-coupled receptors, G proteins, and effectors are freely mobile in the plasma membrane is becomingless fact and more fiction. Significant limitations on the lateralmobility of plasma membrane proteins (both integral and peripheral)restrict movement much like a "corral" around the protein (Kuoand Sheetz, 1993). It has been suggested that an association withthe cytoskeleton (Carlson et al., 1986; Rasenick et al., 1990;Wang et al., 1990) may aid in significantly restricting the lateralmobility of G proteins in the plasma membrane (Neubig, 1994).Furthermore, some G proteins, including Gs, form specific complexeswith tubulin, the major microtubule protein (Wang et al, 1990),and this is a bidirectional process, with G proteins participatingin the regulation of the cytoskeleton (Roychowdhury and Rasenick,1997; Roychowdhury et al., 1999). G protein-coupled receptorsand the kinases that regulate those receptors have been shownto be associated with microtubules as well (Carman et al., 1998;Pitcher et al., 1998; Saunders and Limbird, 2000). Actin and themicrofilament cytoskeleton may also interface with G protein signaling(Carlson et al., 1986; Vaiskunaite et al., 2000)

Recently, the lipid environment in which G proteins and its effectors are localized has been under investigation. G proteinsseem to be present in caveolin-enriched plasma membrane domains,and caveolin may play a role in G protein-mediated signaling (Liet al., 1995). Ostrom et al. (2000) have recently shown a colocalizationof $beta$ -adrenergic receptor and adenylyl cyclase type 6 in caveolaeof cardiac myocytes. The direct association of G proteins withcaveolin has been disputed (Huang et al., 1997); however, theseauthors conclude that the proteins involved in the hormone-sensitiveadenylyl cyclase system are indeed localized to a specializedsubdomain of the plasma membrane. In fact, Moffett et al. (2000)have shown that it is the acylation of G protein subunits thattargets these signaling molecules to specific cholesterol- andsphingolipid-rich membrane domains calledrafts.

Although these data do not show a direct effect on the cytoskeleton or the lipid environment in which Gs $alpha$ is localized, theydemonstrate that Gs $alpha$ relocates to the cell body of antidepressant-treatedcells. This relocalization may reduce the distance between G proteininduced cAMP production and the cascade of molecules involvedin the up-regulation of cAMP response element (CRE)-mediated genetranscription. In fact, previous data demonstrate an increasein immunoprecipitable Gs $alpha$ -adenylyl cyclase complexes after treatmentof rats with a variety of antidepressants and electroconvulsiveshock (Chen and Rasenick, 1995a). The high density of Gs $alpha$ in theprocesses and process tips of nontreated cells suggests a "housekeeping"role in which Gs $alpha$ is involved in maintaining structure and homeostasisin the cell. After chronic antidepressant treatment, Gs $alpha$ may playa role in stimulating the production of genes involved in cellgrowth and rearrangement. Levels of brain-derived neurotrophicfactor and tyrosine receptor kinase B have been shown to be elevatedin the brains of rats chronically treated with antidepressants(Nibuya et al., 1996). The fact that Gs $alpha$ migrates to the cellbody in response to antidepressant treatment suggests that thecAMP signaling machinery leading to increased expression of CREmay be located in close proximity to the nucleus. This relocalizationof G proteins followed by increases in CRE-mediated gene expressionseem to follow a time frame more consistent with the clinicalefficacy of antidepressant drugs than a direct receptoreffect.

Although C6 cells have glutamate uptake sites, there is no evidence that they have specific uptake sites for either norepinephrineor serotonin. Nonetheless, these cells have been shown to respondto antidepressants in a manner similar to rat brain (Fishman andFinberg, 1987; Chen and Rasenick, 1995a,b). This is not necessarilyproblematic; in fact, this may provide an ideal system to detectthe existence of a novel target of antidepressantaction.

There are probably multiple targets of antidepressant action. Although the data in this study are not sufficient to assigna specific mechanism of action for Gs $alpha$ in mediating the effectsof antidepressants, they do suggest a convergence of differentclasses of antidepressants that act through a postsynaptic signalingmechanism toward a common end. Further study on Gs $alpha$ signalingand antidepressant action may illuminate both the biology of depressionand the unique heterogeneity of G proteins during the processof cellsignaling.

	Acknowledgments

We would like to thank Drs. Juliana Popova, Tulika Sarma, Jiang-Zhou Yu, as well as Kimberly Chaney and Bindu Shah, for theirhelpful discussion and technical assistance. We are also gratefulto Dr. M. L. Chen for her expert assistance with the confocalmicroscopy.

	Footnotes

Received December 20, 2000; Accepted February 12, 2000

This work was supported in part by National Institute of Mental Health Grants MH57391 and MH39595. R.J.D. was supported byNational Institutes of Health Training Grant HL07692-09.

Send reprint requests to: Mark M. Rasenick, Ph.D., Department of Physiology & Biophysics, University of Illinois at Chicago, College of Medicine, 835 S. Wolcott Ave., M/C 901, Rm. E202, Chicago, IL 60612-7342. E-mail raz{at}uic.edu

	Abbreviations

PBS, phosphate-buffered saline; CRE, cAMP response element.

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				R. J. Donati, Y. Dwivedi, R. C. Roberts, R. R. Conley, G. N. Pandey, and M. M. Rasenick Postmortem Brain Tissue of Depressed Suicides Reveals Increased Gs{alpha} Localization in Lipid Raft Domains Where It Is Less Likely to Activate Adenylyl Cyclase J. Neurosci., March 19, 2008; 28(12): 3042 - 3050. [Abstract] [Full Text] [PDF]

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				B. Razani, S. E. Woodman, and M. P. Lisanti Caveolae: From Cell Biology to Animal Physiology Pharmacol. Rev., September 1, 2002; 54(3): 431 - 467. [Abstract] [Full Text] [PDF]