Inhibition of cAMP Response Element-Binding Protein or Dynorphin in the Nucleus Accumbens Produces an Antidepressant-Like Effect

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The Journal of Neuroscience, December 15, 2002, 22(24):10883-10890

Inhibition of cAMP Response Element-Binding Protein or Dynorphin in the Nucleus Accumbens Produces an Antidepressant-Like Effect
Samuel S. Newton¹, Johannes Thome¹, Tanya L. Wallace¹, Yukihikko Shirayama¹, Lee Schlesinger¹, Norio Sakai¹, Jingshan Chen¹, Rachael Neve², Eric J. Nestler³, and Ronald S. Duman¹
¹ Division of Molecular Psychiatry, Abraham Ribicoff Research Facilities, Connecticut Mental Health Center, Yale University School of Medicine, New Haven, Connecticut 06508, ² McLean Hospital, Harvard University, Belmont, Massachusetts 02478, and ³ Department of Psychiatry, The University of Texas Southwestern Medical Center, Dallas, Texas 75390

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The cAMP response element-binding protein (CREB) is a critical integrator of neural plasticity that is responsive in a brainregion-specific manner to a variety of environmental and pharmacologicalstimuli, including widely prescribed antidepressant medications.We developed inducible transgenic lines of mice that express eitherCREB or a dominant-negative mutant of CREB (mCREB) in forebrainregions and used these mice to determine the functional significanceof this transcription factor in the learned helplessness paradigm,a behavioral model of depression. We also use a complementaryviral-mediated gene transfer approach to directly test the effectof mCREB in the nucleus accumbens, a brain region important formotivation and reward. The results demonstrate that blockade ofCREB by overexpression of mCREB in transgenic mice or by viralexpression of mCREB in the nucleus accumbens produces an antidepressant-likeeffect, whereas overexpression of CREB in transgenic mice resultsin the opposite phenotype. In addition, mCREB expression was colocalizedwith and decreased the expression of prodynorphin in nucleus accumbensmedium spiny neurons, and antagonism of dynorphin in the nucleusaccumbens was sufficient to produce an antidepressant-like effectsimilar to that observed after blockade of CREB. Together, theresults demonstrate that nucleus accumbens CREB-dynorphin influencebehavior in the learned helplessness model and suggest that thissignaling cascade may contribute to symptoms ofdepression.

Key words: learned helplessness; dysphoria; depression; prodynorphin; $kappa$ -opiate receptors; behavior

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Despite more than 40 years of clinical use, the molecular and cellular mechanisms underlying the long-term, therapeutic actionsof antidepressants remain poorly understood. In recent years,the focus of research has been at a level beyond the serotoninand norepinephrine transporters, the acute targets for the antidepressantreuptake blockers, to the intracellular signal transduction cascadesthat underlie the regulation of neuronal function (Duman et al.,1997, 2000; Manji et al., 2001b; Nestler et al., 2002). A requirementfor adaptations of intracellular signaling pathways, includingregulation of transcription factors and gene expression, couldaccount for the time delay of weeks to months in the therapeuticresponse to antidepressants. Identification of these long-termadaptations has been a major focus of research and could leadto drug targets for the development of faster-acting and moreefficacioustreatments.

Adaptations of the cAMP signal transduction cascade in response to chronic (14-21 d) but not acute (1-7 d) antidepressanttreatment have been reported, suggesting that this second-messengersystem could account for the actions of antidepressants (Dumanet al., 2000). These adaptations include upregulation of the functionand expression of the cAMP response element-binding protein (CREB)in limbic brain regions implicated in mood disorders, includingthe hippocampus and amygdala (Nibuya et al., 1996; Thome et al.,2000; Blom et al., 2002). CREB is a critical mediator of neuralplasticity and has been implicated in learning, memory, and thelong-term actions of opiates and psychostimulants, as well asantidepressants (Nestler and Aghajanian, 1997; Milner et al.,1998; Silva et al., 1998). A role for CREB in depression and inmediating the action of antidepressant treatments is supportedby several recent studies. First, viral-mediated expression ofCREB in the hippocampus produces an antidepressant-like effectin behavioral models of depression (Chen et al., 2001). Second,postmortem studies have demonstrated that levels of CREB in cerebralcortex are decreased in patients with depression and significantlyincreased when patients were receiving antidepressant treatmentat the time of death (Dowlatshahi et al., 1998). Third, drugsthat block the metabolism of cAMP and hence increase cAMP function(e.g., rolipram, an inhibitor of cAMP-specific phosphodiesterasetype IV) produce antidepressant effects in both animal and clinicalstudies (Duman et al., 2000). However, there are also reportssuggesting that blockade of the cAMP-CREB cascade underlies theactions of antidepressant treatment. Repeated antidepressant administrationdecreased levels of phosphorylated CREB in frontal cortex (Rossbyet al., 1999; Manier et al., 2002), although hippocampus and amygdalawere not examined in these studies. In addition, viral-mediatedexpression of a dominant-negative mutant of CREB (mCREB) in thenucleus accumbens produces an antidepressant-like effect in theforced swim model of depression, whereas expression of CREB inthis brain region produces the opposite effect (Pliakas et al.,2001). Finally, null mutation of CREB also results in an antidepressant-likeeffect in the forced swim paradigm (Conti et al., 2002).

To further address this issue, a combination of approaches, including inducible transgenic mice, viral-mediated gene transfer,and microinfusions of a receptor antagonist, were used to examinethe role of CREB in the learned helplessness model of depression.The results demonstrate that blockade of CREB or dynorphin (aputative target gene for CREB) in the nucleus accumbens producesan antidepressant effect and, together with previous studies,indicate that CREB can produce different effects in depressionmodels depending on the brain region in which it isexpressed.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Transgenic mice. To assess the effect of CREB and mCREB on behavior in models of depression, we generated transgenic miceexpressing CREB or mCREB under the tetracycline responsive promoter(Furth et al., 1994; Chen et al., 1998). We described recentlythe expression pattern and neurochemical phenotype of the CREBbitransgenic line of mice used in this study (Sakai et al., 2002);the current paper focuses on characterization of the expressionpattern of the mCREB bitransgenic mice and the behavioral phenotypeof both mouse lines. The CREB mutant contains a serine-to-alaninesubstitution at position 133, eliminating the protein kinase Aphosphorylation site but maintaining charge balance (Gonzalezand Montminy, 1989). Nonphosphorylated mCREB can still bind tocAMP response elements (CREs) but inhibits CREB action by occupyingthe CRE and preventing access by wild-type CREB and other CRE-bindingproteins (Shaywitz and Greenberg, 1999). A 1.1 kb fragment ofthe vector containing mCREB (a gift from Michael E. Greenberg,Harvard Medical School, Boston, MA) was engineered with a FLAGtag peptide (Asp-Tyr-Lys-Asp-Asp-Asp-Asp-Lys) and subcloned intoa modified TetOP (tetracycline regulated) promtor construct (Shockettet al., 1995). The new plasmid was designated as pTetOP-mCREB.A DNA fragment [containing the promoter, open reading frame, simianvirus 40 intron, and poly(A⁺) signal] from pTetOP-mCREB was purified by electroelution andmicroinjected into the pronuclei of oocytes from SJL × C57BL/6mice. The mice expressing the tetracycline transactivator (tTA)gene under the control of the neuron-specific enolase (NSE) promoterwere generated by our laboratory as described previously (Chenet al., 1998; Kelz et al., 1999; Sakai et al., 2002). Tail DNAfrom both mice was isolated using Tissue Amp DNA kit (Quiagen,Chatsworth, CA), and analyzed for the transgene by PCR, dot blotting,or Southern blotting (Sambrook et al., 1989). Of these techniques,PCR was used for routine genotyping of the transgenic mice. Thefounder mice were crossbred with ICR outbred mice to generateF1 mice. F2 homozygous transgenic mice were obtained by crossbreedingF1 siblings; the homozygous genotype was confirmed by crossbreedingthem with wild-type mice. We used only one of each single transgenicline for the present study. During the prenatal period to postnatalweek 3, the transgenic mice were given doxycycline (100 µg/ml;Sigma, St. Louis, MO), an analog of tetracycline, in drinkingwater to turn off the expression of CREB or mCREB in mice carryingthe NSE-tTA gene plus the TetOP-mCREB or TetOP-CREB gene as describedpreviously (Chen et al., 1998). From postnatal week 3 to 10, micewere fed without doxycycline to wash out doxycycline and expressthe target gene. At postnatal week 10, single (NSE-tTA⁺/TetOP-CREB or NSE-tTA⁺/TetOP-mCREB) or bitransgenic (NSE-tTA⁺/TetOP-CREB⁺ or NSE-tTA⁺/TetOP-mCREB⁺) mice were used for characterization of the expression patternor to determine the behavioral phenotype. Animal use procedureswere in accordance with the NIH Guide for the Care and Use ofLaboratory Animals and were approved by the Yale University AnimalCare and UseCommittee.

Immunohistochemistry. All mice were killed via intracardial perfusion with 4% paraformaldehyde under anesthetization withsodium pentobarbital (100 mg/kg, i.p.). Brains were removed andfixed in paraformaldehyde for an additional 4 hr and then immersedovernight in 20% glycerol. A freezing microtome was used to collectserial coronal 30 µm sections through the entire forebrain. Immunodetectionof FLAG-tagged mCREB was performed using free-floating 30 µm sections.Sections were incubated in 0.5% Triton X-100 in TBS for 45 minat 4°C, blocked in 5.0% normal horse serum-0.1% Triton X-100 inTBS for 45 min at 4°C, and incubated overnight at 4°C in mousemonoclonal antibody against FLAG (1:1000; Sigma). The avidin-biotinblocking kit (Vector Laboratories, Burlingame, CA) was used toreduce nonspecific labeling. Sections were then incubated in biotinylatedsecondary antibody for 1 hr at room temperature, followed by incubationin a preformed avidin and biotinylated horseradish peroxidasemacromolecular complex (ABC reagent; Vector Laboratories). mCREB-positivecells were visualized by DAB staining as per the instructionsof the manufacturer (VectorLaboratories).

Combined immunohistochemistry and in situ hybridization. Double immunohistochemistry and in situ hybridization analysis wasconducted according to a recently developed protocol (Newton etal., 2002). Briefly, immunohistochemistry was performed as mentionedabove with modifications to achieve RNase-free conditions. Theavidin-biotin blocking step was replaced by blocking solutionof 2.5% BSA, RNase inhibitor (40 U/ml) and heparin (3000 U/ml)in PBS. Overnight primary antibody incubation was in solutioncontaining 1% Triton X-100, 1% BSA, heparin, and Superase-in RNaseinhibitor (Ambion, Austin, TX) in PBS. After incubation in secondaryantibody at room temperature for 1 hr, sections were treated withABC complex, DAB stained, rinsed in PBS, mounted on "probe-on"slides (Fisher Scientific, Houston, TX), and airdried.

In situ hybridization was performed as per standard protocols. Slide pretreatment steps included incubation in ProteinaseK (0.5 µg/ml in Tris-EDTA buffer for 10 min) and chloroform tofacilitate riboprobe penetration. After successful in situ hybridizationwith ³⁵S-labeled riboprobes, determined by film autoradiography, slideswere dipped in nuclear track emulsion (Kodak NTB; Eastman Kodak,Rochester, NY) and stored at 4°C. Slides were developed basedon the observation that 1 d film exposure corresponds to 1 weekin emulsion. Sections were counterstained in cresyl violet andcoverslipped with DPX mountant (Fluka, Neu-Ulm,Germany).

Learned helplessness paradigm in mice. In this paradigm, an animal is initially exposed to uncontrollable shock stress. Whenthe animal is later placed in a situation in which shock is controllable(escapable), the animal not only fails to acquire the escape responsesbut also often makes no efforts to escape the shock at all. Thisescape deficit is reversed by chronic antidepressant treatment(Willner, 1984; Thiébot et al., 1992; Chen et al., 2001). Learnedhelplessness behavioral tests were performed with the Gemini AvoidanceSystem (San Diego Instruments, San Diego, CA). This apparatusis divided into two equal compartments by a retractabledoor.

Mice were subjected to 120 inescapable electric footshocks (IES) (0.45 mA, 15 sec duration, average interval of 45 sec) inone of the two closed compartments. One day later, a two-way conditionedavoidance test was performed. This test session consisted of 30trials in which electric footshock [0.45 mA, 24 sec duration,at random intervals (mean of 30 sec, averaging 22-38 sec)] waspreceded by a 3 sec conditioned stimulus tone that remained onuntil the shock was terminated. The Gemini Avoidance System recordedthe numbers of escape failures andlatencies.

Surgical microinfusions of viral vectors or dynorphin antagonists and learned helplessness in rats. Male Sprague Dawley rats(225-300 gm, Charles River Laboratories, Wilmington, MA) wereused. The animals were housed under 12 hr light/dark cycle withaccess to food and water ad libitum. Surgery was performed ina stereotaxic apparatus (David Kopf Instruments, Tujunga, CA)under anesthesia with pentobarbital sodium solution (50 mg/kg,i.p.; Abbott Laboratories, North Chicago, IL). For viral-mediatedexpression studies, infusions of herpes simplex virus (HSV)-LacZ(control) and HSV-mCREB were made into the nucleus accumbens usinga standard protocol (Carlezon et al., 1998; Chen et al., 2001).Infusions of 0.5 µl of HSV-LacZ or HSV-mCREB were made bilaterallyinto the nucleus accumbens. The coordinates for the nucleus accumbens(relative to bregma according to the atlas of Paxinos and Watson,1997) were as follows: 2.0 mm anteroposterior (AP), ±1.6 mediolateral(ML), and $-$ 7.2 dorsoventral (DV) from the skull. The infusionswere made over a total of 15 min, and, after an additional 5 minwait period, the injection syringe was removed. Three days later,when HSV-mediated viral expression is maximal (Carlezon et al.,1998; Chen et al., 2001), rats were placed in the learned helplessnesschamber and received 90 inescapable shocks (0.8 mA, 15 sec duration)preceded by a 1 sec conditioned stimulus tone over a 90 min period.The animals were then returned to their home cages and testedin the active avoidance chambers the next day. This test sessionconsisted of 30 trials in which electric footshock [0.8 mA, 30sec duration, at random intervals (mean of 30 sec, averaging 26-34sec)] was preceded by a 3 sec conditioned stimulus tone that remainedon until the shock was terminated. The numbers of escape failuresand escape latencies in each of the 30 trials were recorded bythe Gemini Avoidance System. After the behavioral tests, the ratswere killed bydecapitation.

For the dynorphin antagonist studies, rats received bilateral injections of nor-binaltorphimine dihydrochloride (norBNI) orsaline (0.9%) into one of three different sites: the lateral ventricle,the nucleus accumbens, or the hippocampus. For the lateral ventricleinfusions, norBNI (2.5 µg/side) was infused in a total volumeof 1.0 µl into each side over 15 min, and the injection syringewas left in place for an additional 5 min to allow for diffusionand to prevent flow up the syringe track. The coordinates forthe lateral ventricle (relative to bregma according to the atlasof Paxinos and Watson, 1997) were as follows: $-$ 0.3 mm AP, ±1.2ML, and $-$ 3.1 DV from the skull. For the nucleus accumbens andthe hippocampus, norBNI (1.0 µg/side) was infused in a total volumeof 0.5 µl into each side over 15 min, and the injection syringewas left in place for an additional 5 min. The injection syringewas angled at 10° from the midline for the nucleus accumbens andthe coordinates were as follows: 1.7 mm AP, ±3.9 ML, and $-$ 6.5DV from the skull. The coordinates for the hippocampus were $-$ 3.8mm AP, ±2.0 ML, and $-$ 6.5 DV. Learned helplessness was conductedas described above for the viral infusionstudies.

Statistical analysis. Statistical differences among more than three groups were estimated by a one-way ANOVA, followed bythe Scheffe's test. For comparison of the mean values betweenthe two groups, statistical evaluation was done using the two-tailedStudent's ttest.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Pattern of transgene expression in mCREB bitransgenic mice

To investigate the role of CREB in behavioral models of depression, we developed inducible and brain region-specific transgenicmice using the tetracycline-regulated system (Furth et al., 1994)as described previously by our group (Chen et al., 1998; Kelzet al., 1999; Sakai et al., 2002). An NSE promoter was used todrive expression of the tTA, and the TetOp promoter was used todrive expression of either FLAG-tagged mCREB or wild-type CREB.Single transgenic mice expressing one of the transgenes (e.g.,tTA⁺/mCREB) or bitransgenic mice expressing both genes (tTA⁺/mCREB⁺) were raised on doxycycline to repress tTA expression until weaning.Doxycycline was then removed from the water for 6-8 weeks to allowfor washout and transgene expression beforeanalysis.

Transgene expression in the mCREB and CREB bitransgenic mice was observed in several forebrain regions in a pattern similarto that observed in other NSE-tTA-regulated mice characterizedby our group (Fig. 1) (Chen et al., 1998; Kelz et al., 1999).We characterized recently the expression pattern of the CREB bitransgenicmice (Sakai et al., 2002). Relatively high levels of FLAG-mCREBexpression were observed in the striatum, including both the dorsalstriatum and the nucleus accumbens, and in certain aspects ofcerebral cortex and subfields of hippocampus (Fig. 1). FLAG-mCREBwas observed predominantly in the medial portion of dorsal striatumand primarily the core subdivision of the nucleus accumbens, althoughexpression of FLAG-mCREB was observed in other aspects of theseregions. High-power magnification demonstrates that FLAG-mCREBexpression is restricted to the cell nucleus as would be expectedfor a transcription factor (Fig. 1; see Fig. 4). FLAG-mCREB wassparsely expressed in the deep and superficial layers of parietalcortex (Fig. 1). Moderate levels of FLAG-mCREB expression werealso observed in subregions of the hippocampus, including theCA1 pyramidal cell layer (Fig. 1) and the dentate gyrus granulecell layer (data not shown). In contrast, there was no expressionof FLAG-mCREB observed in the single transgenic mice expressingeither NSE-tTA only (tTA⁺/mCREB) or TetOp-mCREB alone (tTA/mCREB⁺) (data not shown), the latter demonstrating that there was no"leak" expression of the TetOp-mCREB gene. In addition, when animalsare maintained on doxycycline, there is no expression of FLAG-mCREBin the bitransgenic mice (data not shown). A similar pattern oftransgene expression and regulation by doxycycline has been demonstratedin the CREB bitransgenic mice (Sakai et al., 2002).

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Figure 1. Pattern of FLAG-mCREB overexpression in the forebrain of bitransgenic mice. FLAG-mCREB expression was determined by immunohistochemistry in bitransgenic (tTA⁺/mCREB⁺) mice. Doxycycline was administered to bitransgenic mice until weaning, and brains were harvested at 10 weeks of age for immunohistochemical analysis of FLAG-mCREB. In bitransgenic mice, intense staining of FLAG-mCREB is observed in many cells throughout the striatum, particularly the dorsal and medial aspects, and in the nucleus accumbens. A cross section at the level of the dorsal hippocampus also demonstrates FLAG-mCREB staining in deep layers of cerebral cortex and in the CA1 pyramidal cell layers. Higher magnification demonstrates that FLAG-mCREB is localized in the nucleus. Results are representative of the analysis of at least three animals in each group. No FLAG-mCREB was observed in wild-type or single transgenic (tTA⁺/mCREB) mice (data not shown).

Influence of mCREB and CREB on behavior in the learned helplessness model of depression

The influence of mCREB and CREB in the bitransgenic mice on depression-like behavior was assessed using the learned helplessnessmodel of depression. In this paradigm, exposure to an inescapable,aversive stimulus disrupts the ability of an animal to learn toescape a subsequent noxious stimulus. This deficit is observedin a large number of animal species, including mice, rats, andhumans (Seligman and Beagley, 1975). Although it is difficultto access the clinical relevance of animal models of complex behavioraldisorders, inescapable stress leads to many physiological andbehavioral abnormalities that are observed in depression, andmany of these effects are reversed by antidepressant treatment(Shanks and Anisman, 1989; Thiébot et al., 1992; Caldarone etal., 2000).

Single or bitransgenic mCREB or CREB transgenic mice were exposed to IES and then analyzed for escape deficits in an activeavoidance test. In both the single transgenic and bitransgenicmCREB or CREB mice, exposure to IES resulted in a significantincrease in the number of escape failures and latency to escaperelative to sham-treated control animals that were exposed tothe shuttle box chambers but did not receive IES (Fig. 2). Moreover,IES resulted in a significant difference between the single andbitransgenic animals, and the effect was opposite in the mCREBversus the CREB bitransgenic animals. In the mCREB bitransgenicmice (tTA⁺/mCREB⁺), there was a significant decrease in the number of escape failuresand the latency to escape, or an antidepressant-like effect, relativeto single transgenic controls (tTA⁺/mCREB). In contrast, in CREB bitransgenic mice (tTA⁺/CREB⁺), there was a significant increase in the number of failuresand latency to escape, a depression-like effect, relative to singletransgenic controls (tTA⁺/CREB) (Fig. 2).

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Figure 2. Transgenic expression of mCREB or CREB produces opposite effects in the learned helplessness model of depression. Single (tTA⁺/mCREB or tTA⁺/CREB) or bitransgenic (tTA⁺/mCREB⁺ or tTA⁺/CREB⁺) mice were exposed to sham treatment or IES and subsequently tested in an active avoidance paradigm (30 trials of 30 sec duration). The results demonstrate that there is a significant reduction in the number of escape failures and the latency to escape in the mCREB bitransgenic mice and that the opposite phenotype is observed in the CREB bitransgenic mice. There was no difference in escape failures or latency between the sham-treated single or bitransgenic animals, indicating that the alteration in active avoidance behavior is a specific response to IES exposure. The results are presented as the mean ± SEM for each group (n = 8-15 per group). *p < 0.05 compared with single transgenic mice (ANOVA and Fisher's post hoc test).

Although exposure to IES resulted in significant effects in the active avoidance test, there was no difference between singleand bitransgenic animals exposed to sham treatment (Fig. 2). Inall cases, the number of escape failures and escape latenciesin sham-treated animals were comparable in the single and bitransgenicmCREB and CREB mice. This indicates that there was no generalizedeffect on escape behavior that could underlie the differencesthat are induced by exposure to IES between the single and bitransgenicCREB and mCREBmice.

To determine whether transgene expression in the nucleus accumbens, a region known to regulate motivation and reward, couldaccount for the behavioral phenotype of the transgenic mice, weused a viral expression approach. Stereotaxic microinfusions ofHSV-mCREB or HSV-LacZ (control) were made into the nucleus accumbensaccording to standard procedures as described previously (Carlezonet al., 1998; Chen et al., 2001). Rats were used for these studiesto increase the accuracy of the microinfusions. These viral microinfusionsresult in mCREB or LacZ expression in a circumscribed region ofthe nucleus accumbens (Fig. 3) (Carlezon et al., 1998). Infusionof HSV-mCREB significantly decreased the number of escape failuresand the latency to escape relative to infusions of HSV-LacZ (Fig.3).

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Figure 3. Viral-mediated expression of mCREB in the nucleus accumbens produces an antidepressant-like effect in the learned helplessness paradigm. HSV-LacZ (control) or HSV-mCREB was infused into the nucleus accumbens of rats as described in Materials and Methods. Three days later, when levels of viral expression are maximal, rats were exposed to IES and subsequently tested in an active avoidance paradigm (30 trials, 30 sec duration). Rats receiving intra-accumbens infusions of HSV-mCREB displayed a significant decrease in the number of escape failures and latency to escape. The results are expressed as the mean ± SEM (n = 10 animals per group). *p < 0.05 compared with HSV-LacZ controls (Student's t test). NAc, Nucleus accumbens; ac, anterior commissure; $beta$ -gal; $beta$ -galactosidase.

Prodynorphin is colocalized with and regulated by mCREB

To examine the neurobiological mechanisms underlying the actions of mCREB in the nucleus accumbens, the localization of thistransgene in subsets of dynorphin- and enkephalin-positive neuronsin this brain region was determined. Colocalization studies wereconducted by immunoperoxidase staining for FLAG-mCREB combinedwith in situ hybridization using ³⁵S-labeled riboprobes for prodynorphin or proenkephalin mRNA asdescribed previously (Kelz et al., 1999; Nakagawa et al., 2002).For quantitative analysis, FLAG-mCREB-immunopositive cells frombitransgenic animals were identified, and the number of cellsthat express prodynorphin or proenkephalin in the striatum andnucleus accumbens were counted. A total of 331 and 502 FLAG-mCREBcells were counted for colocalization with prodynorphin or proenkephalin,respectively (n = 3 or 4 animals, respectively). FLAG-mCREB-positivecells in both subfields of the striatum were found to expressprodynorphin mRNA, with ~40% of the cells in the nucleus accumbensand 55% in the dorsal striatum being double labeled (Fig. 4).FLAG-mCREB-positive cells were also found to express proenkephalinmRNA, although the percentage of cells was lower than for prodynorphin-labeledcells. Approximately 25% of the cells in the nucleus accumbensand 40% in the striatum were double labeled for FLAG-mCREB andproenkephalin mRNA.

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Figure 4. FLAG-mCREB in bitransgenic mice is colocalized with prodynorphin- and proenkephalin-positive neurons in the striatum. FLAG-mCREB immunohistochemistry was combined with ³⁵S-prodynorphin or ³⁵S-proenkephalin in situ hybridization to characterize the subpopulations of neurons that express mCREB. Emulsion grains for both prodynorphin and proenkephalin were localized in the FLAG-mCREB immunoperoxidase-stained cells in the nucleus accumbens (A, B) and dorsal striatum (data not shown). The total number of FLAG-mCREB cells that were positive for either prodynorphin or proenkephalin were counted (331 and 502 for prodynorphin or proenkephalin, in 3 or 4 animals, respectively). The percentage ± SEM of FLAG-mCREB and double-labeled prodynorphin or proenkephalin cells is shown in C. The level of prodynorphin expression in the FLAG-mCREB-immunopositive cells was also determined. The number of ³⁵S-prodynorphin emulsion grains over FLAG-mCREB-positive cells or adjacent FLAG-mCREB-negative cells in the same sections (50 of each, from 3 different animals) was determined. The results (D) are presented as percentage of control and are the mean ± SEM. *p < 0.05 compared with mCREB-negative controls (Student's t test). NAc, Nucleus accumbens.

Studies in cultured cells and in brain demonstrate that the expression of prodynorphin is increased by activation of the cAMP-CREBcascade and three cAMP response elements in the dynorphin genepromoter (Collins-Hicok et al., 1994; Cole et al., 1995; Carlezonet al., 1998; Sakai et al., 2002). In the present study, the influenceof mCREB expression on prodynorphin mRNA was analyzed to determinewhether mCREB produces an effect opposite to that of CREB. Thenumbers of prodynorphin emulsion grains over either FLAG-mCREB-positivecells or adjacent cresyl violet stained/FLAG-mCREB-negative cells(control) in the same sections were determined (Fig. 4). A totalof 50 FLAG-mCREB and 50 control cells were counted in each ofthree animals (total of 150 cells for each). The results demonstratethat levels of prodynorphin expression are significantly decreasedby >30% in the FLAG-mCREB-positive cells relative to adjacentcontrol cells not expressingmCREB.

Inhibition of dynorphin in nucleus accumbens produces an antidepressant effect

Decreased expression of prodynorphin mRNA in the mCREB bitransgenic mice raises the possibility that downregulation of thisneuropeptide underlies the behavioral phenotype observed in themCREB mice. To directly test this hypothesis, the influence ofa direct-acting dynorphin receptor antagonist on behavior in thelearned helplessness paradigm was determined. The antagonist usedfor these studies was norBNI, an irreversible, long-lasting, andselective antagonist of the dynorphin- $kappa$ -opioid receptor relativeto the µ- and $delta$ -opiate receptor subtypes (Spanagel and Shippenberg,1993). Once again, rats were used to increase the accuracy ofthe surgical microinfusions of norBNI into specific brain regions.Bilateral infusions of norBNI into the lateral ventricles produceda significant decrease in the number of escape failures and thelatency to escape (Fig. 5), an effect similar to that observedin the bitransgenic mCREB mice and similar to the effect of HSV-mCREBinfusions. Moreover, bilateral microinfusions of norBNI directlyinto the nucleus accumbens resulted in a similar decrease in thenumber of escape failures and latency to escape, indicating thatblockade of dynorphin in this brain region is sufficient to producean antidepressant effect. In contrast, bilateral microinfusionsof norBNI into the dentate gyrus of the hippocampus did not significantlyinfluence failure number or escape latency, further demonstratingthe regional specificity of the effect of norBNI (Fig. 5).

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Figure 5. Antagonism of dynorphin- $kappa$ -opioid receptors produces an antidepressant-like effect in the learned helplessness paradigm. Rats were exposed to IES as described in Materials and Methods. One day later, the $kappa$ -opioid receptor antagonist norBNI was microinfused into the lateral ventricles, the nucleus accumbens, or the dentate gyrus of the dorsal hippocampus, and, 3 d later, the animals were tested in an active avoidance paradigm (30 trials, 30 sec duration). The results demonstrate that intracerebroventricular or intra-accumbens, but not intrahippocampal, microinfusions of norBNI significantly decrease the number of escape failures and the latency to escape. The results are expressed as means ± SEM (n = 8-10 animals per group for intracerebroventricular and intra-accumbens infusions; n = 4 for intrahippocampus infusions). *p < 0.05 compared with saline controls (Student's t test).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study uses a combination of approaches to investigate the role of CREB in the learned helplessness model of depression.Results from the inducible CREB and mCREB bitransgenic mice demonstratethat inhibition of CREB produces an antidepressant-like effect.Although the expression pattern is limited in the bitransgenicmice, complementary viral-mediated gene expression studies wereused to demonstrate that inhibition of CREB in the nucleus accumbensis sufficient to replicate the effect observed in the mCREB bitransgenicmice. Finally, direct infusions of a $kappa$ -opioid receptor antagonistproduced an antidepressant-like effect, indicating that downregulationof prodynorphin expression in the mCREB bitransgenic mice couldaccount for the behavioral phenotype in theseanimals.

In this study, we characterized the expression pattern of mCREB in a new inducible bitransgenic mouse in which transgene expressionis under the control of the NSE promoter. Immunohistochemicalanalysis demonstrates the expression of FLAG-mCREB in severalforebrain regions, including the dorsal striatum and nucleus accumbens,as well as in deep layers of cerebral cortex and subfields ofhippocampus. This pattern of expression is similar to the expressionin other lines of conditional bitransgenic mice under the controlof the NSE promoter, including those expressing CREB (Sakai etal., 2002) or $Delta$ FosB (Kelz et al., 1999). This limited and discretepattern of expression provides a useful approach for studyingthe function of a transgene in specific brain regions that cannotbe achieved with constitutive transgenic mice. In addition, theability to turn gene expression on after weaning reduces the chancefor adaptive responses to transgene expression also encounteredin constitutive transgenic lines ofmice.

Previous studies have implicated CREB in the actions of antidepressant treatments (see introductory remarks). Such a rolefor CREB was tested in the present study by analyzing the phenotypeof the CREB and mCREB bitransgenic mice in the learned helplessnessmodel of depression. In these studies, overexpression of CREBincreased the number of escape failures and latency to escape,effects that are interpreted as a more depressive phenotype. Incontrast, overexpression of mCREB produced the opposite effecton failure number and escape latency or an antidepressant-likeeffect. In sham-treated mice (i.e., not exposed to inescapableshock), there was no difference in active avoidance behavior,indicating that the differences observed in both CREB and mCREBbitransgenic lines develop in response to exposure to inescapablestress and not altered training in the active avoidance test perse.

These results in the learned helplessness studies are surprising based on our previous reports that antidepressant treatmentupregulates the cAMP-CREB cascade in the hippocampus, amygdala,and cerebral cortex (Nibuya et al., 1996; Thome et al., 2000).In addition, we reported that viral-mediated expression of CREBin the hippocampus produces an antidepressant-like effect in thelearned helplessness and the forced swim paradigms (Chen et al.,2001). Postmortem studies demonstrating that levels of CREB aredecreased in cerebral cortex of depressed patients and upregulatedin patients receiving antidepressant medication also support thehypothesis that activation of the cAMP-CREB cascade is associatedwith an antidepressant response (Dowlatshahi et al., 1998). Basedon these findings and the expression patterns in the transgenicmice, we hypothesized that the behavioral effects observed couldbe attributable to expression in striatum, particularly the nucleusaccumbens. To test this hypothesis, we used a viral-mediated genetransfer approach to express mCREB in the nucleus accumbens. Microinfusionsof HSV-mCREB into the nucleus accumbens decreased the number ofescape failures and latency to escape, effects similar to thoseobserved in the mCREB bitransgenic mice. Because viral-mediatedgene transfer results in the expression of mCREB in a specificand circumscribed region of the nucleus accumbens, the resultsindicate that the behavioral effects of HSV-mCREB, as well asthe effects in the mCREB bitransgenic mice, are mediated by actionsin the nucleus accumbens. This finding is in agreement with arecent report demonstrating that HSV-mediated mCREB expressionin the nucleus accumbens produces a similar antidepressant-likeeffect in the forced swim model of depression (Pliakas et al.,2001). Similar results were observed using the forced swim testin constitutive CREB partial null mutant mice, although the brainregions underlying this effect were not examined (Conti et al.,2002). Together, the results demonstrate that the influence ofCREB in behavioral models of depression is brain region specific,which is not unexpected given the widespread distribution of thistranscription factor in different brain regions and celltypes.

The ability of CREB to exert opposite effects in the learned helplessness paradigm depending on the brain region in whichit is expressed could result from regulation of different targetgenes in these regions. One potential target gene in the hippocampusis brain-derived neurotrophic factor, which is induced by activationof the cAMP-CREB cascade and is sufficient to produce an antidepressanteffect when infused into the hippocampus (Shaywitz and Greenberg,1999; Shirayama et al., 2002). In the nucleus accumbens, as wellas dorsal striatum, the prodynorphin and proenkephalin genes havebeen identified as targets of CREB (Borsok et al., 1994; Coleet al., 1995; Carlezon et al., 1998), and these neuropeptidesdefine different subpopulations of projection neurons (Gerfenand Young, 1988; Curran and Watson, 1995). Prodynorphin is expressedin the direct projection, and proenkephalin is expressed in theindirect projection, medium spiny neurons. Colocalization studiesof the mCREB bitransgenic mice demonstrate that mCREB is expressedin both dynorphin- and enkephalin-positive neurons in the nucleusaccumbens, as well as dorsal striatum, with a higher percentageof mCREB-positive cells expressing dynorphin relative to enkephalin.In addition, the levels of prodynorphin mRNA expression are significantlydecreased in cells expressing mCREB, demonstrating a functionalinhibition of endogenous CREB by the dominant-negative mutant.In the CREB bitransgenic mice, we reported that induction of prodynorphinand CREB-mediated gene transcription is increased (Sakai et al.,2002).

These findings suggest that downregulation of prodynorphin gene expression could contribute to the behavioral phenotype observedin mCREB bitransgenic mice and in response to viral expressionof mCREB in the nucleus accumbens. This possibility is supportedby studies demonstrating that infusion of a $kappa$ -opioid receptorantagonist, norBNI, produced an antidepressant-like effect similarto that observed in the mCREB bitransgenic mice and in responseto infusion of HSV-mCREB (i.e., decreased number of escape failuresand latency to escape). The antidepressant effect of norBNI isobserved after infusions into the nucleus accumbens or lateralventricle but not into the dentate gyrus of the hippocampus, indicatingthat the effect of the antagonist is mediated by the nucleus accumbens.This finding is consistent with, and extends, the results of arecent study demonstrating that infusion of norBNI into the lateralventricle produces an antidepressant-like effect in the forcedswim test (Pliakas et al., 2001). As discussed by Pliakas et al.(2001), the neurobiological mechanisms underlying the actionsof CREB and dynorphin could be related to the regulation of dysphoriaby dynorphin in the mesolimbic dopamine system. Dynorphin agonistsinduce a state of dysphoria in humans, and upregulation of dynorphinis proposed to mediate some of the negative emotional symptoms(which in some patients resemble depression) that occur duringcocaine withdrawal. Dynorphin-mediated dysphoria is thought tooccur via $kappa$ -opioid receptor regulation of dopamine release inthe nucleus accumbens (Spanagel et al., 1990; Pliakas et al.,2001).

Upregulation of the enkephalin neuropeptide system is also reported to produce antidepressant effects in the learned helplessnessparadigm (Baamonde et al., 1992; Tejedor-Real et al., 1998). Thissuggests that inhibition of proenkephalin gene expression by mCREBwould produce a depression-like phenotype and that CREB wouldproduce an antidepressant-like effect, actions that are oppositeto those observed in the current study. Why the predominant effectin the bitransgenic mice or in response to viral expression ofmCREB is consistent with regulation of prodynorphin, and not proenkephalin,expression is not clear. One possibility is that, when both systemsare regulated by CREB, the actions of prodynorphin override theactions of proenkephalin. Another likely possibility is that thereare additional genes that are regulated by CREB and mCREB thatalso contribute to the behavioralphenotype.

The results of this study support the notion the mesolimbic dopamine system is involved in the etiology and treatment of depressionand suggest that depression in general, or subtypes of this disorder,may be more responsive to antidepressant drugs that include efficacyfor inhibition of the dopamine transporter. Moreover, the resultsindicate that another potential target for development of antidepressantmedication is blockade of dynorphin- $kappa$ -opioid receptors. In addition,although the region-specific effects of CREB make it an unlikelycandidate, it is possible that upstream elements in the cAMP-CREBcascade, such as isoforms of cAMP phosphodiesterases that aredifferentially expressed in the mesolimbic dopamine system versusother limbic brain structures, could be targeted for potentialantidepressant drugdevelopment.

  FOOTNOTES

Received Aug. 15, 2002; revised Sept. 27, 2002; accepted Oct. 3, 2002.

This work is supported by United States Public Health Service Grants MH45481 and 2 PO1 MH25642, a Veterans AdministrationNational Center grant for posttraumatic stress disorder, and bythe Connecticut Mental HealthCenter.

Correspondence should be addressed to Ronald S. Duman, Division of Molecular Psychiatry, Abraham Ribicoff Research Facilities,Connecticut Mental Health Center, Yale University School of Medicine,New Haven, CT 06508. E-mail: ronald.duman{at}yale.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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