Midbrain Raphe Modulation of Nonphotic Circadian Clock Resetting and 5-HT Release in the Mammalian Suprachiasmatic Nucleus

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The Journal of Neuroscience, August 20, 2003, 23(20):7451-7460

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Midbrain Raphe Modulation of Nonphotic Circadian Clock Resetting and 5-HT Release in the Mammalian Suprachiasmatic Nucleus
J. David Glass, Gregory H. Grossman, Laure Farnbauch, and Lisa DiNardo
Department of Biological Sciences, Kent State University, Kent, Ohio 44242-0001

   Abstract

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Serotonin (5-HT) is an important regulator of the mammaliancircadian clock of the suprachiasmatic nucleus (SCN); however,critical questions remain concerning the control of serotonergicactivity in the SCN and how this relates to the putative clock-resettingactions of 5-HT. Previously, we reported that electrical stimulationof the dorsal raphe nucleus (DRN) or median raphe nucleus (MRN)in hamsters evoked 5-HT release in the SCN. This DRN-stimulated5-HT release was blocked by systemic injection of 5-HT antagonists,indicating a 5-HT receptor-mediated pathway from the DRN tothe SCN. In the present study, targeted injections of the 5-HT_1,2,7 antagonist metergoline or the selective 5-HT₇ antagonist DR4004 into the DRN or MRN attenuated DRN-electrically stimulated SCN5-HT release, supporting a multisynaptic DRN $->$ MRN $->$ SCN route. Intra-DRNand intra-MRN injections of the GABA_A antagonist bicuculline significantly stimulated SCN 5-HT release, whereas intra-DRNor intra-MRN injections of the GABA_A agonist muscimol suppressedthis release. The 5-HT release induced by intra-DRN bicucullinewas also blocked by co-injection of DR4004. In complementarybehavioral trials, SCN 5-HT release associated with a phase-advancingsleep deprivation stimulus at midday was prevented by intra-DRNinjection of metergoline. Also, phase-advance shifts inducedby novel wheel access at midday were suppressed, but not blocked,by intra-DRN injection of DR4004 or muscimol. These resultsindicate that 5-HT₇ and GABAergic receptors of the DRN andMRN regulate behaviorally induced 5-HT release in the SCN,and that DRN output modulates nonphotic phase-resetting responses.

Key words: serotonin; suprachiasmatic nucleus; circadian; raphe; GABA; hamster; behavior; phase resetting

   Introduction

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Circadian rhythms in mammals are generated and maintained bya neural clock located within the suprachiasmatic nucleus (SCN) (Rusak and Zucker, 1979; Moore, 1983; Klein et al., 1991).Clock time is synchronized to the light/dark cycle by photicinformation relayed from the retina to the SCN via the retinohypothalamictract (Hendrickson et al., 1972; Moore and Lenn, 1972; Pickard,1982; Youngstrom and Nunez, 1986; Johnson et al., 1988) andby an indirect projection from the intergeniculate leaflet(IGL) (Card and Moore, 1982; Johnson et al., 1989). Projectionsfrom the IGL and the midbrain raphe nuclei also convey nonphotic input to the SCN via neuropeptide Y-containing and serotonin(5-HT)-containing projections, respectively (Albers and Ferris,1984; Biello et al., 1994; Meyer-Bernstein and Morin, 1996;Marchant et al., 1997).
Despite the extensive literature on the action of 5-HT in theSCN, its physiological roles, particularly those related tobehavioral phase regulation, remain speculative. For example,there is evidence that 5-HT acts in the SCN to mediate theclock-resetting effects of behavioral stimulation. This includesfindings that 5-HT agonists applied to the SCN in vitro orin vivo reset circadian phase (Prosser et al., 1990, 1993; Medanic and Gillette, 1992; Challet et al., 1998; Ehlen etal., 2001) and that behavioral phase-resetting manipulationsevoke SCN 5-HT release (Dudley et al., 1998; Grossman et al.,2000). Conversely, reports that raphe lesions (Meyer-Bernsteinand Morin, 1998), treatment with 5-HT antagonists (Antle etal., 1998), or depletion of 5-HT in the SCN (Bobrzynska et al., 1996) do not block behavioral phase shifting argue againsta role of 5-HT in circadian clock resetting.
Critical questions also remain regarding the respective rolesof the dorsal raphe nucleus (DRN) and the median raphe nucleus(MRN) in regulating SCN serotonergic activity. Mapping studiesreveal that the MRN is the sole source of SCN serotonergicinnervation (Vertes and Kocsis, 1994; Meyer-Bernstein et al.,1997; Moga and Moore, 1997). Nevertheless, stimulation ofthe DRN produces 5-HT-related effects in the SCN, includinginhibition of light-induced Fos expression (Meyer-Bernsteinand Morin, 1997) and neuronal discharge (Yu et al., 1997),attenuation of light-induced phase shifts (Weber et al., 1998),and 5-HT release (Dudley et al., 1999). These findings, togetherwith the raphe-SCN mapping results, suggest that the DRN communicateswith the SCN via a multisynaptic interaction through the MRN. This hypothesis is supported by reports that the MRN and DRNare functionally connected (Mokler et al., 2001; Morin andPace, 2001) and that DRN-electrically stimulated, but not MRN-electrically stimulated, SCN 5-HT release is blocked by5-HT antagonists, indicative of a multisynaptic DRN $->$ MRN $->$ SCN pathway (Glass et al., 2000). The present experiments were undertakento characterize this pathway using targeted intra-raphe injectionsof 5-HT antagonists with electrical and behavioral stimulations.This approach was also used to test the hypothesis that thispathway modulates behavioral phase-resetting responses. Because intra-raphe GABAergic transmission is important for regulatingserotonergic activity (Gervasoni et al., 2000), its role incontrolling SCN 5-HT release and nonphotic phase resettingwas also a major focus of this study.

   Materials and Methods

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Animals
Adult male Syrian hamsters (Mesocricetus auratus), raised from breeder pairs obtained from Harlan Sprague Dawley (Indianapolis,IN), were used in these studies. These animals were group housed(two to three per cage) in a climate-controlled (20-22°C)vivarium under a 14 hr light/10 hr dark photo period (LD) (200-250lux). Preceding experimentation, animals were individuallyhoused in a circular polycarbonate cage to facilitate microdialysisand brain stimulation procedures. Rodent chow (Prolab 3000;PMI Feeds, St. Louis, MO) and water were provided ad libitum.
Electrical and pharmacological stimulations of the raphe
Animals received intracranial implants (DRN-stimulating or MRN-stimulating electrode, DRN or MRN microinjection cannula, and SCN microdialysisprobe) using stereotaxic surgical procedures (head level ina stereotaxic frame) with sodium pentobarbital (Nembutal; 50mg/kg) as anesthetic. A bipolar-stimulating electrode (PlasticsOne, Roanoke, VA) was aimed at the DRN [anteroposterior (AP)= -4.7 mm from bregma; lateral (L) = +1.7 mm from midline; horizontal(H) = -4.8 mm from dura at a 20 ^o angle] or MRN (AP = -4.4mm from bregma; L = -2.3 mm from midline; H = -6.8 mm fromdura at a 20 ^o angle), and a unilateral 24 gauge stainlesssteel guide cannula (Plastics One) was implanted contralaterallywith its tip situated 1 mm above the DRN (AP = -4.7 mm frombregma; L = -1.7 mm from midline; H = -3.8 mm from dura at a20 ^o angle) or MRN (AP = -4.4 mm from bregma; L = -2.3 mm from midline; H = -5.8 mm from dura at a 20° angle). A microdialysisprobe was targeted at the lateral margin of the SCN (AP = 0.3mm from bregma; L = +0.3 mm from midline; H = -8.0 mm fromdura). The implants were secured to the skull by three stainlesssteel screws and dental acrylic. Experiments were initiated24 hr after surgery.
For DRN stimulation, constant current (20 min duration at 150or 500 µA, 10 Hz stimulus frequency, and 2.0 msec pulseduration) was delivered to a bipolar electrode from a stimulusisolator (World Precision Instruments, Sarasota, FL) coupledto a Grass S11 stimulator (Grass Instruments, Quincy, MA).Drug injections into the DRN or MRN were undertaken by insertinga 31 gauge injection needle connected by polyethylene tubingto a 10 µl Hamilton syringe into the guide cannula withits tip extending 1.0 mm beyond the end of the cannula. A 31gauge stylet inserted into the guide cannula was used to maintainpatency between injections. Details of microdialysis probe methodology are provided below.
Microdialysis-HPLC
Procedures for microdialysis probe construction are similarto those of previous studies (Dudley et al., 1998). Concentricallydesigned probes were constructed from a 26 gauge stainlesssteel outer cannula (Small Parts, Miami, FL) into which was inserted a beveled 32 gauge fused silica tube (Polymicro Technologies, Phoenix, AZ). Hemicellulose dialysis tubing [molecular weightof 12 kDa cutoff; 230 µm outer diameter; Spectra-por(Fisher Scientific, Pittsburgh, PA)] was inserted $~$ 1.0 mm intothe outer cannula and secured with epoxy glue. The distal endof the membrane was cut to a length of 1.5 mm, and the tipwas sealed with epoxy, providing an active dialyzing lengthof 1.0 mm. Microdialysis was performed by continuously perfusingprobes with filtered artificial CSF (ACSF) composed of thefollowing (in mM): 147 NaCl, 4.0 KCl, 1.8 CaCl₂, pH 7.5, ata flow rate of 1.2 µl/min using a calibrated syringepump (CMA/100; Bioanalytical Systems, West Lafayette, IN) attachedto an overhead liquid swivel (Instech, Plymouth Meeting, PA).The assembly allowed the animals freedom of movement withinthe cage throughout the duration of the experiment. For allexperiments, measurement of extracellular 5-HT in the SCN wasaided by adding 4.0 µM citalopram to the perfusate. Thesampling interval was 20 min.
Microdialysate was analyzed for 5-HT using HPLC (BioanalyticalSystems) with amperometric electrochemical detection. Sampleswere injected onto a 100 x 1 mm 3µ C-18 reverse-phasemicrobore column. The mobile phase consisted of 9.45 gm ofmonochloroacetic acid (Fisher Scientific), 0.2 gm of octanesulfonicacid, and 0.25 gm of Na₂ EDTA (Eastman Kodak, Rochester, NY)dissolved in 1.0 l HPLC-grade distilled water, pH 3.1. Tetrahydrofuran(6.0 ml) was added after filtration. Flow rate of the mobile phase through the column was 90 µl/min. A 3.0 mm glassycarbon radial-flow electrochemical detector set at a potentialof 590 mV relative to an AgCl reference electrode was usedto measure 5-HT. The lower level of sensitivity (signal $>=$ 5x background) was $~$ 500 fg. Electrode output was interfaced with an IBM-compatible computer that recorded andanalyzed the data. Authenticity of the 5-HT peak in SCN microdialysatewas verified by predictable changes in its size after electricaland pharmacological stimulations of the raphe and localizedadministration of pharmacological agents to the SCN via thedialysis probe (Dudley et al., 1998).
Circadian wheel-running activity measurements
Daily wheel-running activity was recorded by a magnetic switchattached to a running wheel (14 inch diameter, 1.5 kg; zcomNalgeNunc International, Rochester, NY) with its output interfacedwith a computerized data acquisition system (Dataquest, Sunriver,OR). Circadian phase resetting was assessed using a modifiedAschoff type II procedure (Aschoff, 1965), in which animalsmaintained under LD up to the time of experimentation were released into total darkness (DD) at the beginning of the experimentaltreatments initiated at zeitgeber time (ZT) 6. Phase shiftsof the circadian wheel-running rhythm were calculated as thedifference between the averaged activity onset for 5 d precedingdrug treatment and onsets predicted by least squares regressionanalysis of activity onsets from days 3-10 after treatment. Activity onset was defined as the first 10 min period in whichthe total number of wheel revolutions (revs) exceeded 50% ofthe maximum number of revolutions per 10 min measured thatday and was followed by at least 1 hr of sustained activity.
Experimental protocols
Effects of 5-HT antagonists on DRN-electrically stimulated SCN5-HT release. A 20 min period of DRN electrical stimulationwas begun in the middle of the light phase at ZT 6 (ZT 12 wastime of lights off). Microinjections of drugs [the 5-HT_1,2,7antagonist metergoline (2 µg, 1 µl volume; Sigma,St. Louis MO); the selective 5-HT₇ antagonist DR4004 (Kikuchiet al., 1999) (2 µg, 1 µl volume; Meiji Seika Kaisha,Yokohama, Japan)] or vehicle (1:1 ACSF/DMSO, 1 µl volume)were administered via an injection cannula aimed at the DRNor MRN 20 min before the onset of the DRN stimulation. ForSCN measurements, the microdialysis probe was perfused for a 2 hr equilibration period beginning at ZT 3, followed by a 1hr sample collection period to establish baseline 5-HT releaselevels. Microdialysis sampling was continued for 2 hr afterthe antagonist injection. Trials were conducted over 3 consecutivedays on the same animal, with drugs or injection vehicle administeredrandomly. Control experiments assessing the effects of intra-rapheadministration of metergoline, DR4004, or vehicle alone (without electrical stimulation) on SCN 5-HT release were also undertaken.
Effects of intra-DRN 5-HT antagonists on sleep deprivation-inducedSCN 5-HT release. The procedures used for sleep deprivationwere similar to those used in a previous study (Grossman etal., 2000). Beginning at ZT 6, animals outfitted with a microdialysisprobe in the SCN and an injection reentry cannula aimed at the DRN were aroused and maintained in the waking state in theirhome cage for 3 hr by continuous gentle handling and lightpuffs of air. After the 3 hr experimental period, the animalswere left undisturbed. These procedures were performed underdim red light (<1.0 lux) because bright light inhibits nonphoticphase resetting (Antle and Mistlberger, 2000). Microdialysissampling was undertaken continuously from ZT 5 to 10 with a20 min sampling interval. An initial intra-DRN metergoline[(experimental) 2 µg, 1 µl volume)] or vehicle [(control) 1:1 DMSO/ACSF, 1 µl volume] microinjectionwas administered 20 min before the onset of the sleep deprivation,and a second microinjection of the same respective solutionwas delivered 2 hr later. The experiment was undertaken usinga paired design in which the animals received both experimentaland control treatments in random order over 2 consecutive days.
Intra-DRN and intra-MRN GABAergic effects on SCN 5-HT release. Microinjections of the GABA_A antagonist bicuculline (125 ng,500 nl volume) or the GABA_A agonist muscimol (25 ng, 500 nlvolume; Sigma) were administered to the DRN and the MRN toexplore the role of raphe GABAergic mechanisms in regulatingSCN 5-HT release. All drugs were administered by microinjectionaimed at the DRN or MRN at ZT 6. Microdialysis measurementsof SCN 5-HT release were undertaken as described above. Sampling was undertaken continuously for 3 hr (1 hr before and 2 hr afterdrug injection).
Intra-DRN 5-HT₇ and GABA_A antagonist effects on SCN 5-HT release.Coapplications of bicuculline and DR4004 in the DRN were undertakento determine whether stimulation of SCN 5-HT release elicitedby GABA_A receptor antagonism is prevented by 5-HT₇ receptor blockade in the same manner as DRN-electrically stimulated SCN5-HT release is blocked with 5-HT antagonists. Animals receivedmicroinjection of DR4004 (2 µg, 1 µl volume) 20min before microinjection of bicuculline (125 ng, 500 nl volume)delivered from the same cannula at ZT 6. Microdialysis measurementsof SCN 5-HT release were undertaken continuously for 3 hr (1hr before and 2 hr after bicuculline injection).
Intra-DRN 5-HT₇ antagonist and GABA_A agonist effects on novelwheel-induced phase resetting. Intra-DRN injections of DR4004and muscimol were undertaken to determine whether the pharmacologicalinterventions that suppressed SCN 5-HT release could also inhibitbehavioral phase resetting. Novel wheel access was used ratherthan sleep deprivation in these trials because the former stimulus,due to the inter-animal variation in wheel-running performance,offers the advantage of testing drug effects over a broaderrange of phase-resetting response. A possible potentiating effectof bicuculline on phase resetting was not evaluated becauseof the acute arousal reaction induced by intra-DRN injectionof this drug. The circadian wheel-running activity rhythm ofhamsters outfitted with a unilateral reentry injection cannulaaimed at the DRN was measured for a minimum of 10 d under LD preceding experimentation. On the day of treatment, the animalsreceived an injection of DR4004, muscimol (same doses as thoseused in the 5-HT release experiments), or vehicle and wereremoved from their home cage and confined in a novel wheelfora3hr period beginning at ZT 6. A second injection of respectivedrug or vehicle was administered at ZT 7.5, and the animalswere returned to their home cage at ZT 9. The animals werereleased into DD at the beginning of the novel wheel confinement,and their phase-resetting response was determined using themodified Aschoff II procedure described above. The number ofrevolutions induced by the novel wheel exposure was recordedover the 3 hr experimental period and after return to the homecage and wheel.
Histological evaluations of intracranial implant sites
After completion of the experiments, the locations of the implantswere verified histologically. Hamsters were deeply anesthetizedwith Nembutal and perfused intracardially with 100 ml of buffered4% paraformaldehyde. The brains were removed and postfixedin 4% paraformaldehyde overnight. Cryostat sections of theSCN region (20 µm) were stained with cresyl violet for light microscopic verification of microdialysis probe placement.A separate tissue block containing the midbrain was seriallysectioned (60 µm) on a vibratome and processed immunocytochemicallyfor 5-HT to verify electrode or cannula tip location among5-HT neurons of the MRN or DRN. Staining for 5-HT was undertakenusing a rabbit polyclonal anti-5-HT (Eugenetech, Farmendale, NJ).
Brain implant specificity considerations.
Electrical stimulations Nonspecific excitation by passive current spread from the DRN to the MRN was evaluated previously usingelectrodes aimed $~$ 0.8 mm dorsolateral to the MRN (Dudley etal., 1999). Stimulation from these electrodes did not affectSCN 5-HT release; therefore, it is unlikely that passive currentflow from electrodes in the DRN would affect MRN neurons locatedfarther away ( $~$ 2.0 mm ventral) from the stimulation site.
Drug stimulations. Diffusion of drugs between the DRN and MRNwas evaluated by comparing responses of the different nucleiwith the same doses of drugs. The differential effects obtained[i.e., threefold greater response to 8-OH-DPAT or WAY 100635injections into the MRN versus the DRN (Dudley et al., 1999)] indicate that the effects of the drugs were registered primarilyat the site of injection. Also, the lack of effect of DRN injectionsthat were off target by $~$ 1 mm supports this contention.
5-HT microdialysis measurements. Site specificity of the SCN microdialysis measurements has been empirically evaluated (Dudleyet al., 1999). Probes with a small window of active dialysismembrane were aimed medially at the SCN to limit sample contaminationfrom 5-HT of extra-SCN origin. This method provided equivalentestimations of peak DRN-stimulated 5-HT release as obtainedusing the conventional concentric probes, confirming that mostof the of 5-HT measured by these probes is from SCN origin.
Statistics
The SCN 5-HT release data were normalized as a percentage ofthe pretreatment baseline level. Pretreatment versus post-treatmentcomparisons were undertaken using one-way repeated measuresANOVA followed by the Student-Newman-Keuls test. Treatmentversus control comparisons for a given time point were analyzedusing a paired t test. A two-way ANOVA was also undertakento compare treatment and site effects over time. Drug effects on wheel-running-induced phase resetting were analyzed usinga one-way ANOVA followed by the Student-Newman-Keuls test.For all procedures, the level of significance was set at p< 0.05.

   Results

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Abstract
Introduction
Materials and Methods
Results
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References

Intra-raphe 5-HT antagonist injection inhibits 5-HT release in the SCN
DRN 5-HT antagonist treatments
Pretreatment with an intra-DRN injection of metergoline abolishedthe DRN-electrically stimulated release of 5-HT in the SCN[peak levels within 40 min after stimulation were 176 ±17 vs 96 ± 10% of baseline for vehicle and metergolinetreatments, respectively (n = 6 per group; p < 0.01) (Fig. 1A)]. A two-way ANOVA revealed that drug treatment, time, andtheir interaction were all significant (p < 0.01). In a similar manner, pretreatment of DRN-electrically stimulatedanimals with intra-DRN injection of the highly selective 5-HT₇antagonist DR4004 blocked the stimulation of 5-HT release inthe SCN [peak levels within 40 min after stimulation were 196± 26 vs 100 ± 9% of baseline for vehicle andDR4004 treatments, respectively (n = 5 per group; p < 0.01)(Fig. 1B)]. Drug treatment, time, and their interaction were all significant (p < 0.01). Intra-DRN injections of metergolineor DR4004 alone (without electrical stimulation) reduced basalrelease of 5-HT in the SCN during an equivalent sampling periodby $~$ 25% versus vehicle (n = 4 per group; p < 0.05 for bothdrugs) (Fig. 1C).

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Figure 1. Suppressive effects of intra-DRN microinjection of 5-HT antagonists on SCN 5-HT release evoked by electrical DRN stimulation. A, Metergoline (MET; n = 6). B, DR4004 (n = 5). Both drug treatments abolished the stimulated 5-HT release seen in vehicle (VEH) controls (n = 6, n = 5, respectively). These antagonists also suppressed basal SCN 5-HT output by $~$ 25% when injected into the DRN alone without electrical stimulation (C; n = 4 per group). ^ap < 0.05 versus pretreatment baseline levels; ^*p < 0.05 versus vehicle controls for a given time point. The 20 min period of electrical stimulation is represented by the horizontal bars designated STIM; INJ, drug or vehicle injection. Data are mean ± SEM.

MRN 5-HT antagonist treatments
Pretreatment of DRN-electrically stimulated animals with intra-MRN injection of metergoline or DR4004 had similar effects as thosedescribed for intra-DRN antagonist applications. DRN-electricallystimulated release of 5-HT in the SCN was prevented by metergoline[peak levels within 40 min after stimulation were 187 ±17 vs 104 ± 15% of baseline for vehicle and metergolinetreatments, respectively (n = 6 per group; p < 0.01) (Fig.2A)]. Drug treatment, time, and their interaction were allsignificant (p < 0.01). Similar to metergoline, DRN-stimulatedSCN 5-HT release was blocked by DR4004 [peak levels within40 min after stimulation were 168 ± 20 vs 95.5 ±6% of baseline for vehicle and DR4004 treatments, respectively(n = 4 per group; p < 0.05) (Fig. 2B)]. Drug treatment,time, and their interaction were all significant (p < 0.01).

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Figure 2. The suppressive effects of intra-MRN microinjection of 5-HT antagonists on SCN 5-HT release evoked by electrical DRN stimulation. A, Metergoline (MET; n = 6). B, DR4004 (n = 4). Similar to DRN injections, both drugs injected into the MRN abolished DRN-stimulated 5-HT release. ^ap < 0.05 versus pretreatment baseline levels; ^*p < 0.05 versus vehicle (VEH) controls for a given time point. The 20 min period of electrical stimulation is represented by the horizontal bars designated STIM; INJ, drug or vehicle injection. Data are mean ± SEM.

Intra-DRN metergoline blocks behaviorally induced 5-HT release in the SCN
Like previous reports from this laboratory (Grossman et al.,2000), 3 hr of sleep deprivation under dim red light duringthe subjective midday induced a prolonged increase in 5-HTrelease in the SCN with maximal levels [151 ± 10% ofpretreatment baseline (n = 5); p < 0.05] occurring within2 hr from the onset of treatment (Fig. 3). The average increase in 5-HT release throughout the entire 3 hr treatment periodwas 134 ± 3% (p < 0.05 vs baseline). In marked contrast,the stimulatory effect of sleep deprivation on SCN 5-HT releasewas abolished in animals treated with an intra-DRN injectionof the 5-HT_1,2,7 antagonist metergoline (Fig. 3). The averagechange in 5-HT release throughout this treatment period was-17 ± 9% [p > 0.37 vs pretreatment baseline (n =5); p < 0.05 vs vehicle controls]. Two-way ANOVA revealeda significant difference between metergoline and vehicle treatment(p < 0.01).

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Figure 3. Blocking effect of intra-DRN microinjection of metergoline (MET) on sleep deprivation-induced 5-HT release in the SCN. Consistent with our previous published results, sleep deprivation caused $~$ 150% increase in SCN 5-HT release. This was completely blocked by the metergoline treatment. Inset, Integrated values for 5-HT release as a percentage of pretreatment baseline over the 3 hr sleep deprivation period designated by the horizontal bar. For both graphs, ^ap < 0.05 versus pretreatment baseline levels; ^*p < 0.05 versus vehicle (VEH) controls for a given time point. Data are mean ± SEM (n = 5 per group).

Raphe GABA receptors modulate 5-HT release in the SCN
Bicuculline stimulates SCN 5-HT release
Microinjection of the GABA_A receptor antagonist bicucullineinto the DRN dramatically stimulated 5-HT release in the SCN,with maximal levels (264 ± 64% of baseline; p < 0.05;n = 5) sustained over a 40 min period after injection (Fig. 4A). The stimulated increase of 5-HT release was approximatelytwice that observed in response to electrical stimulation or sleep deprivation (Fig. 4A). Injection of bicuculline intothe MRN also had a stimulatory effect on SCN 5-HT release,but this was less than induced by the DRN treatment, with maximallevels (174 ± 16% of baseline; p < 0.05; n = 5) occurringwithin 40 min after injection (Fig. 4A). Two-way ANOVA revealedsignificance between DRN and MRN groups, time, and the interactionbetween time and groups (p < 0.01).

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Figure 4. Effects of intra-raphe microinjection of GABA_A receptor ligands on SCN 5-HT release. A, Injection of the GABA_A agonist bicuculline (BICUC) into the DRN (n = 5) and MRN (n = 5) significantly stimulated 5-HT release. B, Injection of the GABA_A antagonist muscimol (MUSC) into the DRN (n = 6) and MRN (n = 5) suppressed 5-HT release, with the duration of this effect being greater in the DRN. C, The stimulatory effect of intra-DRN injection of bicuculline is abolished by intra-DRN pretreatment with DR4004 (n = 5 per group). For all graphs, ^ap < 0.05 versus pretreatment baseline levels; ^*p < 0.05 versus complementary site-drug treatment for a given time point. Data are mean ± SEM. Differences in bicuculline potency between the two experiments were caused primarily by the greater variability in response in A and possibly differences in drug potency between different lots that were used.

Muscimol inhibits SCN 5-HT release
Microinjection of the GABA_A receptor agonist, muscimol, intothe DRN reduced 5-HT release in the SCN to 72 ± 8% ofbaseline levels within 20 min after injection (p < 0.05;n = 6) (Fig. 4B). Microinjection of muscimol to the MRN alsoreduced SCN 5-HT release (73 ± 7% of baseline; n = 5;p < 0.05) (Fig. 4B). A two-way ANOVA revealed differencesbetween DRN and MRN groups (p < 0.01), time (p < 0.01),and the interaction between time and groups (p < 0.05).However, as evident in the bicuculline response, the latencyof muscimol action in the MRN was greater than that observedfor the DRN, with maximal suppression occurring 60 min afterinjection.
Intra-DRN DR4004 inhibits bicuculline-stimulated SCN 5-HT release
Pretreatment with intra-DRN microinjection of DR4004 blockedthe stimulatory effect of intra-DRN microinjection of bicucullineon SCN 5-HT release (Fig. 4C). Two-way ANOVA revealed differencesbetween bicuculline and DR4004 plus bicuculline treatmentsand time (p < 0.01). The similarity in action between theblocking effects of intra-DRN 5-HT antagonists on GABA antagonistand electrical and behavioral stimulations of SCN 5-HT output indicates the involvement of GABA in the same pathway(s) mediatingboth the exogenous and endogenous DRN-mediated activation of5-HT release in the SCN.
Electrical DRN stimulation induces 5-HT release in the MRN
A direct functional serotonergic communication between the DRNand MRN is indicated by our finding that stimulation of theDRN elicits 5-HT release in the MRN. The 20 min pulse of DRNelectrical stimulation increased extracellular 5-HT releasein the MRN by 142 ± 21% of nonstimulated control levels(p < 0.05; n = 6) (Fig. 5).

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Figure 5. Electrical stimulation of the DRN induces 5-HT release in the MRN. Solid circles, Electrical stimulation; solid squares, nonstimulated controls. a is significantly different from controls for a given time point; p < 0.05.

The DRN modulates behavioral circadian phase resetting
Similar to other studies in the Syrian hamster (Bobrzynskaand Mrosovsky, 1998; Meyer-Bernstein and Morin, 1998), therewas a wide range of response to novel wheel access, with themajority of animals of the vehicle control and drug treatment groups running <400 revolutions over the 3 hr treatment period (Fig. 6). Control animals exceeding the 400-500 revolutionlevel exhibited peak phase-advancing responses averaging 136± 23 min (n = 4), whereas most individuals running belowthis level responded with considerably smaller responses averaging44 ± 10 min (n = 11; p < 0.05). Thus, under controlconditions, the 400-500 revolution range was considered tobe an index for attaining maximal phase-advancing response. Animals receiving intra-DRN muscimol that ran at or above thisrange had phase advances that were significantly smaller thancontrols running in this range (46 ± 22 min; n = 4;p < 0.05 vs controls) (Fig. 7). Muscimol-treated animalsrunning below this range (n = 6) also had phase advances that were less than those of controls running in a similar range(11 ± 6 min; n = 6; p < 0.05 vs controls). Animalsreceiving intra-DRN DR4004 that ran above this range had phaseadvances that were smaller than controls (31 ± 15 min;n = 3; p < 0.05 vs controls) (Fig. 7). DR4004-treated animalsrunning less than this range had phase advances similar toboth the control and muscimol groups (26 ± 5 min; n =12; both p > 0.05). Actograms representing the three treatmentgroups are presented in Figure 8.

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Figure 6. Relationship between the number of wheel revolutions during the 3 hr novel wheel exposure and induced phase-advance shifts in animals that received intra-DRN injection of vehicle (VEH), muscimol (MUSC), or DR4004. For reference, a line was plotted for the control data only, using a sigmoidal 3 parameter equation (Sigma Plot, Jandel Scientific, Corte Madera, CA).

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Figure 7. Effects of intra-DRN muscimol and DR4004 injection on novel wheel-induced phase resetting. Top, Phase-advance shifts for animals that ran at or exceeded the 400-500 revolution index range for maximal shifting response. Bottom, Number of wheel revolutions for groups of animals represented in the top. Vehicle, n = 4; muscimol, n = 4; DR4004, n = 3. For each graph, bars with different letters are significantly different. Data are mean ± SEM.

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Figure 8. Double-plotted wheel-running activity records showing representative profiles from the three treatment groups. Days are indicated vertically from top to bottom, and time is indicated horizontally. Asterisks represent the onset of the novel wheel exposure at ZT 6 and release into constant darkness for the Aschoff type II protocol. Activity on the novel wheel was recorded by switching the output signal of the wheel into the home cage monitor channel. After 3 hr, the animal was returned to the home cage (with wheel unlocked). See Materials and Methods for details of the behavioral phase-shifting measurements. A, B, Intra-DRN vehicle control. C, D, Intra-DRN muscimol. E, F, Intra-DRN DR4004. The bottom axis represents external time.

Despite the individual variability in wheel-running response,the overall average revolutions for every animal in each treatmentgroup during the 3 hr treatment period did not differ significantly(control, 337 ± 55 revs; muscimol, 386 ± 71 revs;DR4004, 214 ± 62 revs; both drug groups p > 0.15vs control). However, overall analysis of phase shifting forevery animal in each group revealed significant drug-relateddifferences in response (control, 68 ± 14 min; muscimol,25 ± 10 min; DR4004, 27 ± 5 min; both drug groups,p < 0.05 vs control). Also, for animals running at or abovethe 400-500 revolution range, the mean level of running forcontrols also was not statistically significant from the druggroups (control, 630 ± 93; muscimol, 628 ± 51;DR4004, 612 ± 106; p < 0.98) (Fig. 7). Therefore,the reduced phase-resetting response of animals treated withmuscimol or DR4004 that performed at or above this range isnot attributable to a drug-related suppression of wheel running.

   Discussion

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Serotonergic input to the SCN from the midbrain raphe nucleiis important for maintaining normal circadian rhythmicity;however, the respective roles of the DRN and MRN in regulatingthis input remain uncertain. The MRN is the only direct sourceof serotonergic innervation to the SCN in the Syrian hamster (Meyer-Bernstein et al., 1997), but stimulation of either raphenucleus in this species elicits multiple 5-HT-related effectsin the SCN (Meyer-Bernstein and Morin, 1996, 1997; Yu etal., 1997; Weber et al., 1998), including 5-HT release (Dudleyet al., 1999). We therefore proposed a multisynaptic DRN $->$ MRN $->$ SCN pathway to match these findings with the raphe-SCN mapping data.This pathway is supported by observations that DRN-electricallystimulated 5-HT release in the SCN is blocked by systemic treatmentwith the 5-HT_1,2,7 antagonist metergoline, indicative of amultisynaptic, 5-HT-sensitive route from the DRN to the SCN(Dudley et al., 1999; Glass et al., 2000). The present resultsreveal also that the 5-HT-sensitive components of this pathwayare associated with the raphe nuclei themselves because DRN-electricallystimulated SCN 5-HT release is blocked by intra-DRN and intra-MRNinjections of 5-HT antagonists and DRN stimulation induces 5-HT release in the MRN. The physiological significance of theseobservations is underscored by the demonstration that the acuteincrease in SCN 5-HT release induced by sleep deprivation issimilarly blocked by intra-DRN treatment with metergoline.Importantly, a modulatory role of the DRN in nonphotic phase resetting is indicated by the finding that intra-DRN injectionsof DR4004 or the GABA_A agonist muscimol (both of which suppressSCN 5-HT release) attenuate, but do not block, circadian phase-advanceshifts induced by novel wheel access.
It is notable that intra-DRN 5-HT antagonist application blocksthe effects of electrical stimulation of DRN cells, suggestingthat the 5-HT antagonists block postsynaptic targets of thestimulated DRN cells. The marked similarities between the inhibitoryeffects of intra-DRN 5-HT antagonists on behavioral, bicuculline,and electrically stimulated SCN 5-HT release indicate thatthe electrical stimulation activates the same population ofDRN neurons as do these other modes of stimulation.
Raphe 5-HT₇ receptors regulate behavioral 5-HT release in the SCN
The present observations that DRN-electrically stimulated SCN5-HT release and novel wheel-induced phase shifts are attenuatedby intra-DRN application of metergoline and/or DR4004, bothof which antagonize the 5-HT₇ receptor, implicate DRN 5-HT₇receptors in the regulation of circadian timekeeping. The 5-HT₇receptor has been localized immunocytochemically in fibersand cell bodies in various circadian-related brain sites, includingthe DRN and SCN (Pickard and Belenky, 2000; Duncan et al.,2001), and is thought to mediate the circadian phase-resettingeffect of 5-HT in the SCN (Lovenberg et al., 1993; Ehlen etal., 2001). 5-HT₇ receptor binding has been identified autoradiographicallyin the DRN, MRN, IGL, and SCN of hamsters, and significantly,only 5-HT₇ receptor binding in the DRN changes with aging andin accordance with age-related 8-OH-DPAT phase-resetting effects (Duncan et al., 1999). This points to a unique role of DRN5-HT₇ receptors in regulating serotonergic circadian clock-resettingresponses, which has direct relevance to the present data linkingthese DRN receptors to circadian phase-regulating mechanisms.
Serotonergic regulation of circadian phase
An important issue related to the present assessment of raphefunction is that of a direct phase-regulating action of 5-HTin the SCN (for review, see Morin, 1999; Mistlberger et al.,2000). The intrinsic pattern of activity of 5-HT neurons variesin accordance with behavioral state (Trulson and Jacobs, 1983;Jacobs and Fornal, 1997), and 5-HT release induced in the SCNby behavioral phase-resetting stimuli (Dudley et al., 1998;Grossman et al., 2000) could serve as an intrinsic clock-resettingfeedback signal. Although a role for 5-HT is not certain (Bobrzynskaet al., 1996; Mintz et al., 1997; Meyer-Bernstein and Morin, 1998), evidence supporting a phase-resetting action of 5-HTin the SCN includes reports that in vitro application of 5-HTreceptor agonists to the SCN brain slice preparation duringsubjective midday advances the circadian rhythm of neuronalactivity (Prosser et al., 1990, 1993; Medanic and Gillette,1992; Shibata et al., 1992). Also, in vivo administrationof 8-OH-DPAT into the third ventricle upstream from the SCNin rats (Edgar et al., 1993) or bilateral microinjections of8-OH-DPAT into the SCN region of hamsters (Challet et al., 1998) phase advances the circadian clock, and depletion of 5-HTin the SCN by neurotoxic lesioning prevents entrainment todaily schedules of activity in mice (Edgar et al., 1997; Marchantet al., 1997). More recently, perfusions of the SCN with 8-OH-DPATor 5-HT using reverse microdialysis in hamsters were shownto phase advance the clock at midday in a tetrodotoxin-insensitivemanner, suggesting a direct in vivo phase-resetting actionof 5-HT on clock cells (Ehlen et al., 2001).
Intra-raphe GABAergic mechanisms regulate SCN 5-HT release
The respective stimulatory and inhibitory effects of intra-rapheinjection of the GABA_A antagonist bicuculline and the GABA_A agonist muscimol on SCN 5-HT release support a role of GABAin the regulation of midbrain raphe activity. These resultsare consistent with reports that GABA inhibits DRN neuronalactivity (Gallager and Aghajanian, 1976; Levine and Jacobs, 1992) and mediates IPSPs in DRN serotonergic cells (Pan andWilliams, 1989). Also, reduced DRN neuronal discharge duringsleep is associated with increased GABA release, and this reductionis reversed by bicuculline (Levine and Jacobs, 1992; Nitzand Siegel, 1997; Gervasoni et al., 2000). The suspected regulatoryactions of raphe GABAergic transmission in SCN 5-HT releaseand the timing of the sleep-wake cycle have important implicationsfor circadian phase regulation. Notably, behavior-related changesin raphe GABAergic activity could underlie the circadian phase-resettingeffects of sleep deprivation (Antle and Mistlberger, 2000).During the day, when SCN 5-HT release is low (Dudley et al.,1998), there is strong GABAergic inhibition of raphe activityassociated with the sleep state (discussed above). In the proposedmodel in Figure 9, sleep deprivation-induced SCN 5-HT release (Grossman et al., 2000) is attributed to a behavior-arousal-mediatedsuppression of DRN GABAergic tone. The potentiated 5-HT outputmay in turn mediate behaviorally induced phase resetting. Thismodel is supported by the present findings that (1) 5-HT releaseat midday is stimulated by bicuculline, and (2) this releaseis blocked by intra-DRN injection of metergoline, as is sleepdeprivation-induced SCN 5-HT release. It is possible that thecircadian phase-related actions of intra-DRN GABA involve thesame GABA_A-benzodiazepine receptor population responsible formediating the phase-resetting effects of triazolam (Turek andLosee-Olson, 1986; Turek and Van Reeth, 1988; Van Reeth andTurek, 1989; Marchant and Morin, 1999). However, it is unlikelythat the DRN is a target for the phase-shifting action of triazolam(Meyer-Bernstein and Morin, 1998; Marchant and Morin, 1999),and triazolam and behavioral stimuli do not act via the samephase-resetting mechanism (Meyer-Bernstein and Morin, 1998;Janik and Mrosovsky, 1992; Marchant and Morin, 1999).

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Figure 9. The proposed mechanism by which behavioral information is encoded into serotonergic signaling relayed to the SCN (and possibly the IGL). This model is based on the present findings that (1) DRN-mediated SCN 5-HT release induced by electrical stimulation, GABA antagonist microinjection, or behavioral activation is blocked by intra-DRN or intra-MRN administration of 5-HT₇ receptor antagonists, indicating that the DRN communicates to the SCN via a 5-HT₇-sensitive multisynaptic DRN $->$ MRN $->$ SCN pathway. DRN-stimulated SCN 5-HT release is blocked by intra-MRN injected 5-HT₇ antagonists, indicating that the MRN is a critical component of this pathway. (2) Intra-DRN or MRN injection of GABA_A antagonist bicuculline stimulate SCN 5-HT release, indicating that raphe activity is tonically suppressed by GABA_A receptor activation. (3) Intra-MRN injection of bicuculline and the GABA_B antagonist 2-hydroxysaclofen (data not shown) equally stimulate SCN 5-HT release, indicating that MRN GABA_B and GABA_A receptors regulate SCN 5-HT release. (4) Electrical DRN stimulation induces 5-HT release in the MRN. This model proposes that behavioral activation suppresses the activity of GABA (1) neurons that tonically inhibit DRN 5-HT (1) neurons (and may also directly activate these 5-HT neurons). The 5-HT (1) neurons, when activated, inhibit DRN and MRN GABA (2 and 3) neurons that tonically suppress MRN 5-HT (2) neurons expressing both GABA_A and GABA_B receptors. Output from the stimulated 5-HT (1) neurons may also induce release of 5-HT in the IGL. The ensuing activation of the MRN 5-HT (2) neurons causes release of 5-HT from SCN terminals, according to the strength of the behavioral stimulus. This scheme does not rule out the possibility that behavior could also directly stimulate MRN activity. 5-HT₇ R, 5-HT₇ receptor; GABA_A R, GABA_A receptor; GABA_B R, GABA_B receptor; -, inhibition; +, activation.

DRN modulation of behavioral phase resetting
Intra-DRN treatments with DR4004 or muscimol at dosages thatsuppress DRN signaling to the SCN significantly attenuatedthe phase-advancing effect of novel wheel access. Notably,the mean shifting response of the drug-treated animals runningat or more than the 400-500 revolution range was only $~$ 30% ofmaximally shifting vehicle controls running with similar exertion.It is therefore apparent that inhibiting DRN output can attenuatebehavioral phase shifting, which is not caused by drug-relatedsuppression of running activity. As discussed above, we proposethat DR4004 and muscimol inhibit different components of theDRN pathway(s) that participate in phase resetting. Namely, DR4004 treatment inhibits the 5-HT₇ receptor-sensitive componentof the DRN system for conveying behaviorally coded serotonergicinput to the SCN. The muscimol treatment overrides an inhibitoryinfluence of behavior over the GABA_A receptor-mediated suppressionof DRN serotonergic activity. The actions of both drugs inhibitDRN output to a similar extent, resulting in a suppressed behavioralphase-shifting response. It is notable that the intra-DRN drugtreatments attenuated, but did not abolish, phase shifting, indicating that either DRN output was incompletely blocked bythe drugs or that behavioral shifting can occur without DRNoutput. The latter possibility is supported by the findingthat hamsters with 5-HT-specific neurotoxic lesioning of theDRN also can undergo novel wheel-induced phase advances (Meyer-Bernsteinand Morin, 1998). Interestingly, previous studies showing thatelectrical stimulation of the DRN at midday induces phase-advanceshifts indicate that DRN output can evoke circadian phase resetting (Meyer-Bernstein and Morin, 1997; Glass et al., 2000). Thus,serotonergic output from the DRN may be sufficient but notnecessary for behavioral phase resetting, and its physiologicalrole may be to augment the effects of other neuronal systemsmediating clock resetting. The IGL is a good candidate in thisregard because it receives serotonergic innervation from theDRN (Meyer-Bernstein and Morin, 1996), and bilateral injectionof 8-OH-DPAT in the IGL has a phase-advancing effect (Challetet al., 1998) [although unilateral IGL injection of 8-OH-DPATis ineffective (Mintz et al., 1997)]. Also, bilateral lesioningof the IGL blocks the phase-shifting effect of peripheral 8-OH-DPATinjection (Schuler et al., 1999), and there is recent evidencethat wheel-running at midday induces 5-HT release in the IGLregion (J. D. Glass and G. H. Grossman, unpublished observations).

   Footnotes

Received Dec. 13, 2002; revised Apr. 15, 2003; accepted Apr. 28, 2003.
This work was supported by National Institutes of Health GrantNS35229 to J.D.G. We thank Meiji Seika Kaisha Ltd. (Yokohama,Japan) for supplying DR4004.
Correspondence should be addressed to J. David Glass, Departmentof Biological Sciences, Kent State University, Kent, OH 44242-0001.E-mail: Jglass{at}kent.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/237451-10$15.00/0

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Materials and Methods
Results
Discussion
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