Differential cAMP Gating of Glutamatergic Signaling Regulates Long-Term State Changes in the Suprachiasmatic Circadian Clock

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The Journal of Neuroscience, October 15, 2000, 20(20):7830-7837

Differential cAMP Gating of Glutamatergic Signaling Regulates Long-Term State Changes in the Suprachiasmatic Circadian Clock
Shelley A. Tischkau¹^,³, Eve A. Gallman¹, Gordon F. Buchanan², and Martha U. Gillette¹^,²^,³
Departments of ¹ Cell and Structural Biology, ² Molecular and Integrative Physiology, and ³ the Neuroscience Program, University of Illinois at Urbana-Champaign, Urbana, Illinois 61801

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We investigated a role for cAMP/protein kinase A (PKA) in light/glutamate (GLU)-stimulated state changes of the mammaliancircadian clock in the suprachiasmatic nucleus (SCN). NocturnalGLU treatment elevated [cAMP]; however, agonists of cAMP/PKA didnot mimic the effects of light/GLU. Coincident activation of cAMP/PKAenhanced GLU-stimulated state changes in early night but blockedlight/GLU-induced state changes in the late night, whereas inhibitionof cAMP/PKA reversed these effects. These responses are distinctfrom those mediated by mitogen-activated protein kinase (MAPK).MAPK inhibitors attenuated both GLU-induced state changes. AlthoughGLU induced mPer1 mRNA in both early and late night, inhibitionof PKA blocked this event only in early night, suggesting thatcellular mechanisms regulating mPer1 are gated by the suprachiasmaticcircadian clock. These data support a diametric gating role forcAMP/PKA in light/GLU-induced SCN state changes: cAMP/PKA promotesthe effects of light/GLU in early night, but opposes them in latenight.

Key words: suprachiasmatic nucleus; glutamate; signal transduction; mPer1; protein kinase A; MAP kinase; rat

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The circadian clock is a complex biological structure in which a dynamic set of cellular state progressions generates near24 hr rhythms at behavioral, physiological, cellular, and molecularlevels. The oscillatory mechanism is a self-sustained transcriptional-translationalfeedback loop (for review, see King and Takahashi, 2000). In mammals,rhythmicity is modulated by the impingement of numerous neurochemicalinputs, which provide information regarding the external and internalenvironments, on a central clock in the suprachiasmatic nucleus(SCN) (Moore and Lenn, 1972; Pickard, 1982; Johnson et al., 1988).These afferent signals use specific signal transduction pathwaysto interface with core clock elements to induce long-term statechanges, or phase shifts, in the clock. Clock sensitivity to state-alteringsignals and activation of signaling pathways are gated by theSCN (Gillette, 2000). For example, cAMP activation alters circadiantiming only during subjective day, whereas sensitivity to cGMP-dependentstate changes are restricted to subjective night (for review,see Gillette and Tischkau, 1999). Thus, the accessibility of specificsignaling pathways is key to regulation oftiming.

Light signaling pathways intersect with the molecular clockworks via the mammalian period1 (mPer1) gene. Translation of mPer1mRNA is required for light-induced phase resetting in the earlynight (Akiyama et al., 1999). Light elevates mPer1 mRNA in bothearly and late night (Albrecht et al., 1997; Shearman et al.,1997; Shigeyoshi et al., 1997; Takumi et al., 1998; Zylka et al.,1998). Light responsiveness of other clock genes differs. Levelsof mPer2 increase robustly after light in the early night, butthe response in the late night is not as clear (Albrecht et al.,1997; Takumi et al., 1998; Zylka et al., 1998). mTim mRNA levelsare also augmented in response to light in the early night [Tischkauet al. (1999), but see King and Takahashi (2000)].

Dissection of elements required for SCN processing of light information points to commonalities and disparities between earlyand late night. Glutamate (GLU) is the primary neurotransmittertransmitting light signals to the SCN (Pickard, 1982; Johnsonet al., 1988; Castel et al., 1993; De Vries et al., 1993; Dinget al., 1994; Shirakawa and Moore, 1994; Hannibal et al., 2000).Throughout the night, a phase-resetting light stimulus evokesrelease of GLU from the retinohypothalamic tract (RHT) and activationof multiple GLU receptor types, of which NMDA receptors are critical(Colwell and Menaker, 1992; Ding et al., 1994; Shibata et al.,1994; Shirakawa and Moore, 1994, Mintz et al., 1999). The consequentinflux of Ca²⁺ activates nitric oxide synthase (NOS) to produce nitric oxide(NO) (Ding et al., 1994; Amir et al., 1995). After liberationof NO, the light signaling pathways diverge (Gillette, 2000).In early night, light/GLU-induced state change, which delays theclock's rhythm, requires activation of neuronal ryanodine receptors(RYRs) to release intracellular stores of Ca²⁺ (Ding et al., 1998). In late night, the light/GLU signal activatesan RYR-independent, cGMP/protein kinase G (PKG)-dependent signaltransduction cascade to initiate a phase advance (Weber et al.,1995; Mathur et al., 1996; Ding et al., 1998). Finally, light/GLUsignaling in both early and late night induces phosphorylationof Ca²⁺/cAMP response element binding protein (CREB) and CRE-mediatedtranscriptional activation (Ginty et al., 1993; Ding et al., 1997;Obrietan et al., 1998, 1999).

Although activation of PKA can be downstream from NMDA receptor-triggered Ca²⁺ transients in other brain regions (Greengard et al., 1991; Bitoet al., 1997), a role for cAMP in nocturnal light/GLU signalingSCN state changes has yet to be determined. Recently, pituitaryadenylyl cyclase-activating polypeptide (PACAP) was demonstratedto modulate circadian state changes stimulated by light/GLU (Chenet al., 1999). These data suggest that activation of cAMP/PKAcould contribute to light/GLU signal transduction. We hypothesizedthat a GLU-primed cAMP/PKA response system modulates light/GLU-inducedstate changes. We examined the effects of cAMP/PKA modulationof early and late night glutamatergic input to the SCN in termsof rodent behavioral and SCN electrical activity rhythms and onmPer1mRNA.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals and circadian time. Long-Evans rats (6-12 weeks old) were used for all in vitro experiments. This line has been inbredfor >35 generations, surpassing the requirements for genetic homogeneity,which leads to low variation in physiological experiments. Ratswere provided food and water ad libitum and entrained to a dailycycle of 12 hr light and 12 hr dark. Over the 2-3 d of experimentationin vitro, the SCN generates stable, near 24 hr oscillations inneuronal activity that do not deviate from the entrained 24 hrcycle (Prosser and Gillette, 1989). Therefore, in vitro clocktime was determined from the lighting cycle in the donor colony.The time of lights-on was designated as circadian time (CT) 0;subjective day was CT 0-12. Subjective night (CT 12-24) correspondedto the dark portion of the donor'scycle.

Preparation and treatment of brain slices. Brain slices were prepared $>=$ 2 hr before the onset of the dark phase of the light/darkcycle. A block of hypothalamic tissue was cut with a mechanicalchopper into 500 µm coronal slices containing the SCN. Sliceswere studied for up to 3 d in vitro with continuous perifusionof Earle's Essential Balanced Salt Solution (EBSS, Sigma, St.Louis, MO), supplemented with 24.6 mM glucose, 26.2 mM NaHCO₃,and 2.5 mg/l gentamicin, and saturated with 95% O₂/5% CO₂ at 37°C,pH 7.4. Neuronal activity, measured by single-unit recording,is low at night and peaks around midday (CT 7) (Gillette and Prosser,1988). Therefore, measurement of time-of-peak provides an accurateassessment of circadian phase (Gillette et al., 1995).

For all experiments except scintillation proximity assay (SPA), SCN slices were treated in the brain slice chamber. Perifusionwas stopped during treatment. GLU (10 mM, 10 min) was appliedby microdrop (1 µl) to the SCN at the surface of the slice. Allother treatments were applied 30 min before the time of GLU treatmentby replacing the bath with EBSS containing the reagent to be tested.At the conclusion of treatment, slices were washed, the bath wasreplaced with fresh EBSS, and perifusion was resumed. For SPAexperiments, SCN slices were trimmed to contain only the SCN andunderlying optic chiasm. This reduced slice preparation retainsSCN clock properties (Gillette and Reppert, 1987).

cAMP measurements. At either CT 14 or CT 20, reduced slices were transferred to microfuge tubes containing 100 µl of 10 mMGLU or vehicle control. Tubes containing reduced slices and treatmentmedia were snap frozen in a dry ice/methanol bath at the conclusionof treatment. After ethanol extraction from samples, cAMP wasassayed using the SPA (Amersham, Arlington Heights, IL) accordingto the protocol provided. Sample size was based on rigorous statisticaltesting of thehypothesis.

Single-unit recordings of SCN neuronal activity. The technique used to record single units extracellularly from the ensembleof SCN neurons has been described in detail previously and validatedthoroughly (Prosser and Gillette, 1989). Briefly, under visualguidance, a glass microelectrode filled with 5 M NaCl was loweredinto the SCN using a hydraulic microdrive until the signal froma single cell was encountered. Electrical signals from singleunits exceeding twice the background level were isolated, observedfor stability, and counted for 4 min using LabView software. Theelectrode was advanced until a different cell was encounteredand its activity was counted. After a complete pass through thebrain slice, the electrode was repositioned within the SCN tosample throughout the entire nucleus over the course of the experiment.Firing rates of individual neurons recorded during a single experimentwere grouped into 2 hr running averages using 15 min lags. Thetime-of-peak for each experiment was determined by visual inspectionof a plot of 2 hr running averages for the symmetrically highestpoint. Certain experiments were performed with the experimenterblind to treatment conditions. Results of such experiments wereidentical to "non-blind"recordings.

The average peak electrical activity of the ensemble of SCN neurons, which reliably occurs near CT 7 in untreated brain slicesmaintained in vitro, provides an accurate measure of clock time.A phase advance was defined as a peak that appeared before CT7 on the days after treatment; the time-of-peak appeared laterthan CT 7 for phase delays. Thus, phase shifts were determinedby comparing the mean time-of-peak from treatment groups withvehicle-treatedcontrols.

In situ hybridization. After early- or late-night treatment, brain slices containing the SCN were fixed overnight in 4% paraformaldehyde.Slices were transferred to 0.1 M PBS with 20% sucrose and maintainedat 4°C until sectioning. Ten micrometer sections were cut at $-$ 17°Con a cryostat. Hybridization was performed as previously described(Tischkau et al., 1999). The template for the mPer1 probe waskindly provided by Dr. U. Schibler (Université de Genève, Switzerland)(Balsalobre et al., 1998) and corresponded to nucleotides 660-780of the published sequence (Sun et al., 1997). The probe was labeledwith digoxygenin by in vitro transcription. A digoxygenin-labeledsense or antisense riboprobe for mPer1 (5 ng/µl) was applied inhybridization buffer (4× SSC, 40% formamide, 10% dextran sulfate,1× Denhardt's solution, 10 mM DTT, 1 mg/ml yeast tRNA, 1 mg/mlsalmon sperm DNA) overnight at 42°C. Probe hybridization was visualizedusing an alkaline phosphatase-labeled anti-digoxygenin antibody(1:100, Roche). Analysis of mPer1-positive cells was made in amidcaudal section of the SCN by an individual blind to the experimentaldesign and identity of thesamples.

In vivo wheel-running experiments. Male Syrian hamsters (Mesocricetus auratus) were housed individually in cages equippedwith running wheels (5.5 inch diameter). Animals were entrainedto a 14 hr light/10 hr dark schedule for at least 21 d beforerelease into constant darkness (DD). Wheel revolutions were countedby activation of reed switches (by a magnet attached to the wheel)and tallied using DATACOL 3 data acquisition software (Minimitter,Sun River, OR). Actograms were plotted using Ratman (Klemfussand Clopton, 1993). Treatment times were calculated from the timeof activity onset, designated CT 12. The magnitude of phase resettingwas measured as the distance between regression lines drawn throughdata from at least 5 d immediately before treatment and 5 d afterreestablishment of a stable circadian rhythm after treatment (Dinget al., 1998).

At least 7 d before release into DD, animals (70-110 gm at time of surgery) were stereotaxically implanted with guide cannulaedirected into the third ventricle (Ding et al., 1994). Under ananesthesia mixture of ketamine (125 mg/kg), xylazine (20 mg/kg),and acepromazine maleate (2 mg/kg), guide cannulae (26 gauge;Plastics One, Roanoke, VA) were implanted 1.0 mm anterior to bregmaat the midline (upper incisor bar at 0) to a depth of 2.8 mm inferiorto the dural surface. Guide cannulae were secured with a jeweler'sscrew and cranioplastic cement (Plastics One). Stainless steelstylets (33 gauge; Small Parts, Miami, FL) were inserted intocannulae to maintainpatency.

Animals were allowed to free-run under constant conditions for 10-14 d before the first intracerebroventricular injection.Injections were performed as described previously (Chen et al.,1999). Briefly, saline and KT5720 (5 µM) injections were performedin dim red light (~1 lux). Injections (2 µl) were administeredover a 1 min interval. When injections were accompanied by a lightpulse, the light stimulus (15 min, 20 lux) (Weber et al., 1995)was initiated 15 min after the injection. Subsequent injectionswere set at 10-14 d intervals to allow recovery of a stable, free-runningrhythm. Each animal received up to three treatments (saline +light, KT5720, KT5720 +light).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

GLU stimulates cAMP accumulation in the SCN

To evaluate cAMP-mediated signal transduction in state changes, or phase shifts, that arise as a consequence of light/GLUstimulation, we first determined whether SCN cAMP levels changein response to GLU in early (CT 14) and late (CT 20) subjectivenight. CT 14 and CT 20 correspond to the circadian times mostsensitive to phase resetting in response to GLU in the rat. Atime course for the cAMP response at CT 14 established that SCNcAMP levels increased significantly 2 min after GLU treatment(p < 0.05), peaked at 3 min (p < 0.01), and returned to basallevels 10 min after treatment (Fig. 1A,B). At CT 20, cAMP wasalso elevated significantly 3 min (p < 0.01) after GLU treatment.Data shown are the results of six independent experiments foreach treatment.

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Figure 1. cAMP measurements after GLU stimulation at CT 14 or CT 20. A, At CT 14, GLU elevated cAMP levels in a time-dependent manner. cAMP was elevated significantly 2 min (p < 0.01), 3 min (p < 0.01), and 5 min (p < 0.01) after GLU treatment, but returned to basal levels by 10 min after GLU treatment. Peak levels were observed 3 min after GLU stimulation. B, cAMP levels were elevated after GLU treatment at both CT 14 and CT 20. ** indicates statistical significance (p < 0.01) compared with controls (ANOVA with Student-Newman-Keuls).

cAMP potentiates GLU-induced phase delays but inhibits GLU-induced phase advances in vitro

To test the hypothesis that cAMP modulates GLU-induced state changes that are expressed as phase shifts of circadian rhythms,we examined the effects of GLU on SCN clock phase in the presenceof the membrane-permeable cAMP analog, 8-Br-cAMP. Control slicesexhibit a persistent, near 24 hr oscillation with a mean time-of-peakoccurring at CT 6.80 ± 0.15 (Fig. 2A,H) (n = 6). Application of8-Br-cAMP at CT 14 (time-of-peak, CT 6.75 ± 0.25, n = 3) or CT20 (time-of peak, CT 6.62 ± 0.15, n = 4) had no effect on thesubsequent phase of the SCN neuronal activity rhythm (Fig. 2,B and E, respectively), confirming earlier observations (Prosserand Gillette, 1989). GLU application at CT 14 stimulated a characteristic(Ding et al., 1994) phase delay (time-of-peak, CT 9.9 ± 0.35,n = 5) of ~3 hr (Fig. 2C,H). Interestingly, coapplication of 8-Br-cAMPpotentiated the phase delay stimulated by GLU. The 4.29 ± 0.15hr phase delay that ensued after treatment with 8-Br-cAMP + GLUat CT 14 (time-of-peak, CT 11.09 ± 0.13; n = 4) (Fig. 2D,H) wassignificantly greater (p < 0.05) than the phase delay producedby GLU alone.

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Figure 2. Exogenous cAMP modulates GLU-induced phase resetting of the SCN electrical activity rhythm in vitro. A, A control recording demonstrated that the electrical activity rhythm persists for 2 d in vitro, with a peak near CT 7 on both days. B, The membrane-permeable cAMP analog 8-Br-cAMP (200 µM) had no effect on the time-of-peak electrical activity at CT 14. C, At CT 14, GLU (10 mM) induced a 3 hr phase delay in the SCN electrical activity rhythm. D, 8-Br-cAMP significantly increased (p < 0.05, Student's t test) the magnitude of the GLU-induced phase delay from ~3 to ~4.5 hr. E, 8-Br-cAMP (200 µM) had no effect on the electrical activity rhythm when applied alone at CT 20. F, At CT 20, GLU (10 mM) advanced the electrical activity rhythm by ~3 hr. G, 8-Br-cAMP (200 µM) blocked the GLU-stimulated phase advance. H, Summary of the phase shifting effects of GLU ± 8-Br-cAMP at CT 14 and CT 20. Bars indicate the mean ± SEM of three to six experiments. a, b, and c indicate values significantly different from each other and from controls (p < 0.05; Student's t test).

At CT 20, GLU induced a phase advance of ~3.5 hr (Fig. 2F,H) (time-of-peak CT 3.29 ± 0.32, n = 4), corroborating previousstudies (Ding et al., 1994). When 8-Br-cAMP was applied in combinationwith GLU at CT 20 (Fig. 2G,H), the time-of-peak neuronal activityoccurred, as in controls, at CT 6.55 ± 0.17 (n = 4). Thus, 8-Br-cAMPblocked the GLU-induced phase advance at CT20.

PKA inhibition blocks GLU-induced phase delays but potentiates GLU-induced phase advances in vitro

A ubiquitous consequence of cAMP elevation is activation of PKA. To determine whether PKA mediates the effects of GLU thatgenerate phase-shifting state changes in the SCN throughout subjectivenight, we used KT5720, an isoquinoline inhibitor of PKA. Applicationof KT5720 alone at either CT 14 (time-of-peak, CT 6.75 ± 0.18,n = 4) or CT 20 (time-of-peak 6.66 ± 0.25, n = 4) had no effecton the time-of-peak electrical activity from the ensemble of SCNneurons (Figs. 3, C, H and F, H, respectively). Coapplicationof KT5720 completely blocked the GLU-induced phase delay of theSCN electrical activity rhythm at CT 14 (time-of-peak CT 6.98± 0.30, n = 3) (Fig. 3D,H). Conversely, at CT 20, KT5720 potentiatedthe phase-advancing effects of GLU. KT5720 + GLU caused a 6.25± 0.42 hr (n = 4) (Fig. 3G,H) phase advance, which is significantlylarger (p < 0.01) than the phase advance induced by applicationof GLU alone at this time. Thus, although GLU stimulation increasescAMP levels throughout the night, the resultant PKA activationproduces opposite consequences on phase resetting in responseto glutamatergic stimuli in early versus late night.

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Figure 3. Inhibition of PKA, using KT5720, modulates GLU-induced phase resetting of the SCN electrical activity rhythm in vitro. A, The same control recording described in Figure 2. B, KT5720 (100 nM) had no effect on the time-of-peak electrical activity at CT 14. C, At CT 14, GLU (10 mM) induced a 3 hr phase delay in the SCN electrical activity rhythm. D, KT5720 fully blocked the GLU-induced phase delay. E, KT5720 (100 nM) had no effect on the electrical activity rhythm when applied alone at CT 20. F, At CT 20, GLU (10 mM) advanced the electrical activity rhythm by ~3 hr. G, KT5720 enhanced the GLU-stimulated phase advance by 1.5 hr to a total of 4.5 hr. H, Summary of the phase shifting effects of GLU ± KT5720 at CT 14 and CT 20. Bars indicate the mean ± SEM of three to six experiments. a, b, and c indicate values significantly different from each other and from controls (p < 0.05; Student's t test).

Mitogen-activated protein kinase inhibition partially blocks both GLU-induced phase delays and advances

GLU-induced signal transduction can also activate the mitogen-activated protein kinase (MAPK) cascade to initiate neuronalstate changes (Bading and Greenberg, 1991; Rosen et al., 1994).cAMP-dependent activation of the MAPK pathway has been implicatedin the phase-resetting effects of light/GLU in the SCN (Gintyet al., 1993; Obrietan et al., 1998). To determine whether thecAMP-dependent effects that we observed were caused by activationof MAPK, we inhibited the MAPK signal transduction cascade attwo different sites in conjunction with GLU treatment at CT 14and CT 20. Olomoucine (Abraham et al., 1995) and apigenin (Kuoand Yang, 1995) inhibit p44 MAPK. PD98059 inhibits MEK (MAP kinasekinase) (Kultz et al., 1998). Each inhibitor partially blockedthe GLU-induced phase delay at CT 14 (Fig. 4) (n = 3 for eachinhibitor). Likewise, but in contrast to the effects of KT5720in tandem with GLU at CT 20, each MAPK inhibitor partially blockedthe GLU-induced phase advance. Thus, our data support a role forMAPK as one of several elements essential to signal transductionevents stimulated by GLU that initiate phase resetting at night.However, permissive effects of PKA on the MAPK pathway do notaccount for the effects we observe with KT5720. Importantly, inhibitionof MAPK alone cannot explain the potentiation of the GLU-inducedphase advance observed in the presence of KT5720.

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Figure 4. Inhibition of the MAPK kinase cascade attenuates GLU-induced phase shifts at both CT 14 and CT 20. Bars indicate the mean ± SEM of three to six experiments. Inhibitors of p44 MAPK, apigenin (50 µM), and olomoucine (100 µM) diminish the amplitudes of the GLU-induced phase delay at CT 14 from ~3 to ~1.5 hr (n = 3, p < 0.05, Student's t test) and phase advance at CT 20 from ~3.5 to ~1.75 hr (n = 3, p < 0.05, Student's t test). PD98059 (50 µM), an inhibitor of MEK, also decreased the GLU-induced phase delay to ~2 hr (n = 3, *p < 0.05, Student's t test) and phase advance to ~1.5 hr (n = 3, *p < 0.05, Student's t test).

PKA inhibition potentiates light-induced phase shifts in vivo

The importance of activation of cAMP/PKA signal transduction in response to light/GLU in the SCN was further evaluated invivo. A 20 lux light pulse at the time of maximal sensitivityto phase resetting by light caused a 1.24 ± 0.37 hr (n = 8) phaseadvance in the onset of the wheel-running rhythm in the hamster(Fig. 5). Injection of KT5720 at 30 min before a light pulse significantlypotentiated light-induced phase advances (1.92 ± 0.25 hr, n =10; p < 0.05) (Fig. 5B,D). Injection of KT5720 alone had no effecton the phase of wheel-running activity (Fig. 5C) (n = 8).

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Figure 5. The PKA inhibitor, KT5720, potentiated light-induced phase advances of hamster wheel-running activity rhythm in vivo. A-C, Sequential daily activity records from three hamsters representing the effects of the various treatments. Each line represents 24 hr. Light exposure (20 lux, 15 min) at CT 18 (6 hr after activity onset, indicated by star) after vehicle (2 µl) administration by intracerebroventricular injection induced a 1.24 ± 0.37 hr (n = 8) phase advance. KT5720 injection (2 µl) before light exposure significantly augmented the light-induced phase advance (1.92 ± 0.25 hr, n = 10; a, b indicate statistically significant differences, *p < 0.05, ANOVA with Student-Newman-Keuls). KT5720 alone did not induce significant phase shifts (0.08 ± 0.15 hr; n = 8).

PKA inhibition differentially alters GLU-induced mPer1 mRNA accumulation in a state-dependent manner

To determine whether cAMP/PKA mediates the rapid, transient elevation of mPer1 mRNA required for both phase delays (Akiyamaet al., 1999) and phase advances (S. A. Tischkau and M. U. Gillette,unpublished observations) in response to nocturnal light/GLU,in situ hybridizations were performed after treatment of SCN sliceswith GLU ± KT5720. Endogenous mPer1 mRNA was low at CT 14 andCT 20 (Fig. 6A,D). Consistent with the effects of light in vivo(Albrecht et al., 1997; Shearman et al., 1997; Shigeyoshi et al.,1997; Zylka et al., 1998), mPer1 mRNA was significantly elevated60 min after GLU treatment at either CT 14 or CT 20 (Fig. 6B,E)(n = 6). There was no significant difference in total contentof GLU-stimulated mPer1 at either time (Student's t test), butat CT 14, GLU-stimulated mPer1 was observed throughout the SCN,whereas GLU-stimulated mPer1 was restricted to the retinorecipientSCN at CT 20. KT5720 blocked the GLU-stimulated rise in mPer1at CT 14 (Fig. 6C) (n = 6) but did not diminish the accumulationof mPer1 after GLU treatment at CT 20. In contrast to samplestreated with GLU alone at CT 20, mPer1 was observed throughoutthe SCN in these samples (Fig. 6F) (n = 6). KT5720 had no effecton mPer1 levels when applied alone at either time (data not shown).

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Figure 6. Effects of PKA inhibition on GLU-induced mPer1 mRNA levels in the SCN at CT 14 and CT 20. A digoxygenin-labeled cRNA probe detected low levels of mPer1 mRNA in control sections at CT 14 (A) and CT 20 (D). GLU significantly elevated mPer1 mRNA 60 min after GLU treatment at either CT 14 (B) or CT 20 (E). Inhibition of PKA blocked GLU-induced mPer1 at CT 14 (C), but had no effect on GLU-induced mPer1 at CT 20 (F). G, For quantitation, positive cells were counted from one SCN in a single, midcaudal section by an experimenter blind to the treatment. Bars represent mean ± SEM for six independent experiments. ** represents statistically significant differences compared with control values at the same circadian time as determined by AVOVA (p < 0.01) with Student-Newman-Keuls post hoc analysis.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Overt SCN clock sensitivity to reagents that activate cAMP pathways (the neuromodulatory ligands PACAP and serotonin), stimulatecAMP accumulation (forskolin, cAMP phosphodiesterase inhibitors),or activate PKA (cAMP analogs) is restricted to subjective day;cAMP/PKA at night has no effect on clock phase (Prosser and Gillette,1989; Medanic and Gillette, 1992; Shibata et al., 1992; Hannibalet al., 1997). Thus, daytime activation of cAMP signal transductionis typical of a primary signaling pathway. Direct activation ofa downstream component, cAMP, evokes the same response as an extracellularsignal, PACAP or serotonin, whereas inhibition of a downstreamcomponent, PKA, blocks the response to the extracellularsignal.

This study reveals a different role for cAMP/PKA-dependent processes in modulation of nocturnal glutamatergic input to theSCN. PKA acts to gate long-term state changes invoked by GLU,because inhibition of cAMP/PKA alters the GLU effects, but cAMP/PKAhas no effect independent of GLU. cAMP/PKA gating provides regulationby either blocking or enhancing signal flow through a primarypathway (Iyengar, 1996), as observed in other systems. Developmentally,PKA elevation blocks differentiation by the morphogenic Hedgehogsignal in Drosophila (Blair, 1995; Jiang and Struhle, 1995, Liet al., 1995; Perrimon, 1995) and mice (Fan et al., 1995). cAMPblocks H-Ras-induced transformation of NIH-3T3 cells (Chen andIyengar, 1994) and EGF-induced Raf-1 phosphorylation in rat1 fibroblasts(Wu et al., 1993), whereas cAMP alone is ineffective. In contrast,cAMP/PKA activation promotes synaptic potentiation by BDNF inXenopus neuromuscular synapses (Boulanger and Poo, 1999) and theearly phase of postsynaptic long-term potentiation (LTP) (Blitzeret al., 1995, 1998), whereas exogenous cAMP has noeffect.

Interestingly, both the positive and negative functions of the cAMP/PKA gate occur in the SCN (Fig. 7A,B). Light/GLU activationof the cAMP/PKA gate in early night permits signal transductionthrough the primary pathway but blocks signal transmission throughthe same primary signaling pathway in late night. Thus, the clockitself determines the effects of cAMP/PKA activation, and as such,cAMP/PKA contributes contextual information regarding clock stateat the time of light exposure.

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Figure 7. A, A schematic summary of the effects of the cAMP/PKA gate on long-term changes in the SCN neuronal activity rhythm induced by light/GLU. 8-Br-cAMP is ineffective in altering circadian state when applied alone at night. However, raising cAMP enhances GLU-in-duced phase delays in early night but blocks GLU-induced phase advances in late night. In contrast, blocking PKA in the presence of GLU abolishes GLU-induced phase delays in early night but potentiates GLU-induced phase advances in late night. In contrast, inhibition of the MAPK kinase cascade attenuates both GLU-induced phase delays and phase advances by 50%. B, A model depicts interaction of the cAMP/PKA gating pathway with the primary GLU signaling pathway that confers state change in the SCN when activated at night. Nocturnal light activates an NMDA receptor-mediated pathway that leads to liberation of NO in both early and late night. After NO, the pathway leading to circadian phase delay in early night diverges from the pathway that evokes phase advance in late night. However, each pathway eventually leads to activation of mPer1 mRNA and ultimately alters circadian time. The cAMP/PKA gating pathway modulates activity of the main pathway in both early and late night. Activation of cAMP/PKA in the early night opens the gate, thereby permitting signal flow through the main pathway. In contrast, activation of cAMP/PKA in the late night hinders signal transfer through the primary pathway; the cAMP/PKA gate is closed. Thus, the phase of the circadian clock itself is the gatekeeper that determines the downstream consequences of cAMP/PKA activation. The mechanism for activation of cAMP/PKA remains speculative at this time as indicated by the question marks. NMDA receptor-mediated Ca²⁺ influx may both activate the primary pathway and the cAMP/PKA gate, as occurs during hippocampal LTP (Blitzer et al., 1995). Alternatively, NMDA receptor-mediated Ca²⁺ influx may prime the system for other extracellular signals, such as PACAP (Chen et al., 1999) or serotonin (Moriya et al., 1998), to activate adenylyl cyclase.

State changes initiated by GLU in both early and late night are mediated by NMDA receptor-mediated Ca²⁺ influx that activates NOS (Ding et al., 1994). Subsequent signalingactivates multiple pathways specific to clock state but encompassesparallel, divergent, and convergent elements that induce phase-delayingstate change in early night, or phase-advancing state change inlate night. Convergent elements may include the MEK/MAPK pathwayand CREB. MAPK (Obrietan et al., 1998), CREB phosphorylation (Gintyet al., 1993; Ding et al., 1997; Obrietan et al., 1998), and CRE-mediatedgene transcription (Obrietan et al., 1999) have been implicatedin light/GLU-induced state changes in the SCN. Activation of MAPK,but not PKA, can substitute for light/GLU to induce CRE-mediatedgene transcription in the SCN (Obrietan et al., 1999).

This study provides functional evidence that MAPK signaling contributes to the effects of light/GLU on clock phase in bothearly and late night. Inhibition of MAPK attenuates both GLU-inducedphase shifts by ~50% (Fig. 4). Although higher concentrationsof the MAPK inhibitors were not tested, we predict that 50% isthe maximal response. Like KT5720, each of the MAPK inhibitorswas used at a concentration two times the IC₅₀. More importantly,these same concentrations of olomoucine and PD98059 block depolarization-inducedCREB and Erk phosphorylation in hippocampal slices (Impey et al.,1998). Moreover, MAPK inhibition reduces light-induced phosphorylationof CREB on serine-133 in the SCN by 50% (Obrietan et al., 1998).PKA-dependent nuclear translocation of Erk/MAPK can lead to CREBphosphorylation (Impey et al., 1998).

These data predict that CREB functions as a convergence point, or coincidence detector, within the primary light/GLU-signalingpathway. An unidentified pathway(s) must contribute the other50% of the light/GLU effect. Although PKA-dependent activationof MAPK can partially account for the signals that cause phasedelay, the fact that PKA inhibition increases the magnitude ofthe phase advance suggests activation of an additional, alternativepathway. Although further studies are necessary to determine whetherdirect activation of MAPK can substitute for GLU to induce phaseresetting at night, the aggregate data place MAPK on the primarypathway leading to long-term state changes in response to light/GLU.

Recent reports support a link between light signaling through GLU, NO, MAPK, and CREB phosphorylation to CRE elements in themPer1 promoter (Obrietan, 2000; Tei et al., 2000). CREB is notlikely a direct substrate for cAMP/PKA because nocturnal activationof cAMP/PKA alone in the SCN does not activate CRE-mediated genetranscription (Obrietan et al., 1999). This argues for placingCREB on the primary pathway, independent from the cAMP/PKA gatingpathway. CRE elements in the promoter allow tentative placementof mPer1 on the primary pathway because the light/GLU stimulusthat induces mPer1 (Albrecht et al., 1997; Shearman et al., 1997;Shigeyoshi et al., 1997; Zylka et al., 1998; present study) alsogenerates phosphorylated CREB (Ginty et al., 1993; Ding et al.,1997; Obrietan et al., 1998) and stimulates CRE-mediated transcription.Furthermore, antisense oligonucleotides against mPer1 completelyblock both GLU-induced phase delays (Akiyama et al., 1999) andphase advances (Tischkau and Gillette, unpublished observations).Although we cannot exclude placement of mPer1 on the gating pathwayin early night, the fact that inhibition of PKA does not inhibitmPer1 in late night eliminates it from a position on the cAMP/PKAgating pathway at that time. Thus, we favor placement of mPer1on the primary pathway, downstream of CREB, with intersectionof the cAMP/PKA gate upstream of these convergent elements (Fig.7).

Our results demonstrate that activation of the cAMP/PKA gate, a signaling consequence of adding GLU to the slice, attenuatesactivity of the primary GLU pathway in the late night. PKA inhibitionreleases this brake, potentiating GLU-induced phase resetting.However, PKA inhibition did not potentiate the induction of mPer1in the presence of GLU. These differences may reflect interpretivelimitations imposed by experimental design. mPer1 induction wasevaluated 60 min after GLU-stimulation of rat SCN slices. In themouse, light-stimulated mPer1 in vivo is a rapid, transient eventthat is initiated by 15-30 min in the retinorecipient SCN, peaksat 60 min, and spreads throughout the nucleus by 120 min (Albrechtet al., 1997; Shearman et al., 1997; Shigeyoshi et al., 1997;Takumi et al., 1998; Zylka et al., 1998). Our data suggest thatthe kinetics of mPer1 induction may differ between species and/ormay depend on the experimental paradigm. Sixty minutes after lightin early night, expression of mPer1 in the rat is not limitedto the retinorecipient SCN but has spread throughout the nucleus(Fig. 6B). In contrast, 60 min after light in late night, mPer1is found only in the retinorecipient SCN (Fig. 6, compare B andE). However, consistent with the concept that PKA inhibition removesa brake on the GLU-signaling pathway, mPer1 was expressed throughoutthe entire SCN (Fig. 6, compare F and E) when slices were co-treatedwith a PKA inhibitor and GLU in late night. PKA inhibition mayenhance flow through the signaling pathway, altering the kineticsof mPer1 induction in response to GLU. A thorough time coursemay reveal differences in total mPer1 that ultimately reflectthe magnitude of the GLU-induce phaseresponse.

Mechanisms for intersection of cAMP/PKA gating pathway with the primary light/GLU pathway are unknown. Because cAMP has oppositeeffects on the light/GLU-induced signal transduction in earlyversus late night, the intersection between the cAMP/PKA gatingpathway and the primary pathway likely occurs at elements uniqueto each pathway. For example, it seems unlikely that cAMP/PKAwould activate the NMDA receptor in early night and then inhibitthis same molecule in late night. Therefore, it is not unreasonableto speculate that the intersection points between the cAMP/PKAgating pathway and the primary signaling pathways lie somewheredownstream of NO, the divergence point (Fig. 7B). In the earlynight, cAMP/PKA must regulate the primary pathway upstream ofmPer1, because inhibition of PKA blocks mPer1 induction, i.e.,the signal is blocked before it reaches mPer1.

The mechanism for raising cAMP in response to GLU remains unresolved. Gating pathways (Jordan and Iyengar, 1998) can be constitutivelyactive, as in cAMP gating of the Hedgehog signal during development(Blair, 1995; Fan et al., 1995; Jiang and Struhle, 1995, Li etal., 1995; Perrimon, 1995), activated by intracellular signals,as in cAMP gating of early hippocampal LTP (Blitzer et al., 1995),or activated by a second extracellular signal, as in cAMP gatingof neuropeptide-induced survival of retinal ganglion cells (Meyer-Frankeet al., 1995). In the SCN, cAMP is not constitutively elevated.Peak levels occur near the end of subjective day and near theend of subjective night; low levels of cAMP are observed throughoutthe period of sensitivity to light/GLU (Prosser and Gillette,1991). GLU could activate both the primary pathway and the cAMP/PKAgate.

More likely, GLU activates the primary pathway and then permits activation of the cAMP pathway via a second extracellularsignal. Both PACAP (Chen et al., 1999), an extracellular messengerthat colocalizes with GLU in the RHT (Hannibal et al., 2000),and the 5-HT1A-specific agonist MKC-242 (Moriya et al., 1998)have the same modulatory effects as cAMP/PKA on light/GLU-inducedstate changes. Thus, any afferent signal capable of accessingthe cAMP/PKA gate in the presence of light/GLU may play a modulatoryrole. The cAMP/PKA gating pathway may provide contextual informationto allow integration of multiple signals that occur coincidentallywith light/GLU. Moreover, cAMP/PKA gating may explain discrepanciesbetween the magnitudes of light-induced phase shifts in vivo (asin Fig. 5), where the response reflects integration of informationfrom the RHT, as well as other afferents, and GLU-induced phaseshifts in vitro (as in Figs. 2-4), where the response is isolatedto the SCN. Elucidating the sites of intersection between thecAMP/PKA gating pathway and the primary signaling pathways stimulatedby GLU will provide insights into mechanisms for integrating multiplesignals to generate adaptive behavioral statechanges.

  FOOTNOTES

Received June 14, 2000; revised Aug. 4, 2000; accepted Aug. 9, 2000.

This research was supported by Public Health Service Grants NS22155, HL67007 (M.U.G), and NS10170 (S.A.T).
Correspondence should be addressed to Dr. Martha U. Gillette, Department of Cell and Structural Biology, University of Illinois,B107 CLSL, 601 S. Goodwin Avenue, Urbana, IL 61801. E-mail: mgillett{at}uiuc.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Abraham RT, Acquarone M, Andersen A, Asensi A, Belle R, Berger F, Bergouniuox C, Brunn G, Buquet-Fagot C, Fagot D (1995) Cellular effects of olomoucine, an inhibitor of cyclin-dependent kinases. Biol Cell 83:105-120[ISI][Medline].
Akiyama M, Kouzu Y, Takahashi S, Wakamatsu H, Moriya T, Maetani M, Watanabe S, Tei H, Sakaki Y, Shibata S (1999) Inhibition of light- or glutamate-induced mPer1 expression represses the phase shifts into the mouse circadian locomotor and suprachiasmatic firing rhythms. J Neurosci 19:1115-1121[Abstract/Free Full Text].
Albrecht U, Sun ZS, Eichele EE, Lee CC (1997) A differential response of two putative mammalian circadian regulators, mPer1 and mPer2, to light. Cell 91:1055-1064[ISI][Medline].
Amir S, Robinson B, Edelstein K (1995) Distribution of NADPH-diaphorase staining and light-induced Fos expression in the rat suprachiasmatic nucleus region supports a role for nitric oxide in the circadian system. Neuroscience 69:545-555[ISI][Medline].
Bading H, Greenberg ME (1991) Stimulation of protein tyrosine kinase phosphorylation by NMDA receptor activation. Science 253:912-914[Abstract/Free Full Text].
Balsalobre A, Damiola F, Schibler U (1998) A serum shock induces circadian gene expression in mammalian tissue culture cells. Cell 93:929-937[ISI][Medline].
Bito H, Deisseroth K, Tsien RW (1997) Ca²⁺-dependent regulation in neuronal gene expression. Curr Opin Neurobiol 7:419-429[ISI][Medline].
Blair SS (1995) Hedgehog digs up an old friend. Nature 373:656-657[Medline].
Blitzer RD, Wong T, Nouranifar R, Iyengar R, Landau EM (1995) Postsynaptic cAMP pathway gates early LTP in hippocampal CA1 region. Neuron 15:1403-1414[ISI][Medline].
Blitzer RD, Conner JH, Brown GP, Wong T, Shenoliker S, Iyengar R, Landau EM (1998) Gating of CAMKII by cAMP-regulated protein phosphatase activity during LTP. Science 280:1940-1942[Abstract/Free Full Text].
Boulanger L, Poo M (1999) Gating of BDNF-induced synaptic potentiation by cAMP. Science 284:1982-1984[Abstract/Free Full Text].
Castel M, Belenky M, Cohen S, Ottersen OP, Storm-Matheson J (1993) Glutamate-like immunoreactivity in retinal terminals of the mouse suprachiasmatic nucleus. Eur J Neurosci 5:368-381[ISI][Medline].
Chen D, Buchanan GF, Ding JM, Hannibal J, Gillette MU (1999) Pituitary adenylyl cyclase-activating peptide: a pivotal modulator of glutamatergic regulation of the suprachiasmatic circadian clock. Proc Natl Acad Sci USA 96:13468-13473[Abstract/Free Full Text].
Chen J, Iyengar R (1994) Suppression of Ras-induced transformation of NIH 3T3 cells by activated G $alpha$ _S. Science 263:1278-1281[Abstract/Free Full Text].
Colwell CS, Menaker M (1992) NMDA as well as non-NMDA receptor antagonists can prevent the phase-shifting effects of light on the circadian system of the golden hamster. J Biol Rhythms 7:125-136[Abstract/Free Full Text].
De Vries MJ, Nunes Cardozo B, van der Want J, de Wolf A, Meijer JH (1993) Glutamate immunoreactivity in terminals of the retinohypothalamic tract of the brown Norwegian rat. Brain Res 612:231-237[ISI][Medline].
Ding JM, Chen D, Weber ET, Faiman LE, Rea MA, Gillette MU (1994) Resetting the biological clock: mediation of nocturnal phase shifts by glutamate and NO. Science 266:1713-1717[Abstract/Free Full Text].
Ding JM, Hurst WJ, Faiman LE, Kuriashkina LR, Gillette MU (1997) Resetting the biological clock: mediation of nocturnal CREB phosphorylation through light, glutamate and nitric oxide. J Neurosci 17:667-675[Abstract/Free Full Text].
Ding JM, Buchanan GF, Tischkau SA, Chen D, Kuriashkina L, Faiman LE, Alster JM, McPherson PS, Campbell KP, Gillette MU (1998) A neuronal ryanodine receptor mediates light-induced phase delays of the circadian clock. Nature 394:381-384[Medline].
Fan C-M, Porter JA, Chiang DT, Beachy PA, Tessier-Lavigne M (1995) Long range sclerotome induction by Sonic Hedgehog: direct role of the amino-terminal cleavage product and modulation by the cAMP signaling pathway. Cell 81:457-465[ISI][Medline].
Gillette MU (2000) Cellular regulators of circadian timing. In: The regulation of sleep (Borbely AA, Hayaishi O, Sejnowski T, Altman J, eds).. Human Frontier Science Program 10th Anniversary Workshop, Strasbourg, FR, June, 1999.
Gillette MU, Prosser RA (1988) Circadian rhythm of the rat suprachiasmatic brain slice is rapidly reset by daytime application of cAMP analogs. Brain Res 474:348-352[ISI][Medline].
Gillette MU, Reppert SM (1987) The hypothalamic suprachiasmatic nuclei: circadian patterns of vasopressin secretion and neuronal activity in vitro. Brain Res Bull 19:135-139[ISI][Medline].
Gillette MU, Tischkau SA (1999) Suprachiasmatic nucleus: the brain's circadian clock. Rec Prog Hormone Res 54:33-59.
Gillette MU, Medanic M, McArthur AJ, Liu C, Ding JM, Faiman LE, Weber ET, Tcheng TK, Gallman EA (1995) Intrinsic neuronal rhythms in the suprachiasmatic nuclei and their adjustment. In: Circadian clocks and their adjustment (Ciba Foundation Symposium 183), pp 134-153 Chichester, UK: Wiley.
Ginty DD, Kornhauser JM, Thompson MA, Bading H, Mayo KE, Takahashi JS, Greenberg ME (1993) Regulation of CREB phosphorylation in the suprachiasmatic nucleus by light and a circadian clock. Science 260:238-241[Abstract/Free Full Text].
Greengard P, Jen J, Nairn AC, Stevens CF (1991) Enhancement of the glutamate response by cAMP-dependent protein kinase in hippocampal neurons. Science 253:1135-1138[Abstract/Free Full Text].
Hannibal J, Ding JM, Chen D, Fahrenkrug J, Larsen PJ, Gillette MU, Mikkelsen JD (1997) Pituitary adenylate cyclase-activating peptide (PACAP) in the retinohypothalamic tract: a potential daytime regulator of the biological clock. J Neurosci 17:2637-2644[Abstract/Free Full Text].
Hannibal J, Moller M, Ottersen OP, Fahrenkrug J (2000) PACAP and glutamate are co-stored in the retinohypothalamic tract. J Comp Neurol 418:147-155[ISI][Medline].
Impey S, Obrietan K, Wang ST, Poser S, Yano S, Wayman G, Deloulme JC, Chan G, Storm DR (1998) Cross talk between ERK and PKA is required for Ca²⁺ stimulation of CREB-dependent transcription and ERK nuclear translocation. Neuron 21:869-883[ISI][Medline].
Iyengar R (1996) Gating by cyclic AMP: expanded role for an old signaling pathway. Science 271:461-463[ISI][Medline].
Jiang J, Struhle G (1995) Protein kinase and hedgehog signaling in Dros-ophila limb development. Cell 80:563-572[ISI][Medline].
Johnson RF, Moore RY, Morin LP (1988) Loss of entrainment and anatomical plasticity after lesions of the hamster retinohypothalamic tract. Brain Res 460:297-313[ISI][Medline].
Jordan JD, Iyengar R (1998) Modes of interactions between signaling pathways. Biochem Pharmacol 55:1347-1352[ISI][Medline].
King DP, Takahashi JS (2000) Molecular genetics of circadian rhythms in mammals. Annu Rev Neurosci 23:713-742[ISI][Medline].
Klemfuss H, Clopton PL (1993) Seeking tau: a comparison of six methods. J Interdiscip Cycle Res 24:1-16.
Kultz D, Madhany S, Burg MB (1998) Induction of GADD45 and GADD153 by osmosensing stress-activated protein kinase. J Biol Chem 273:13645-13651[Abstract/Free Full Text].
Kuo ML, Yang NC (1995) Reversion of v-H-ras-transformed NIH 3T3 cells by apigenin through inhibiting mitogen activated protein kinase and its downstream oncogenes. Biochem Biophys Res Commun 212:767-775[ISI][Medline].
Li W, Ohlymeyer JT, Lane ME, Kalderon D (1995) Function of protein kinase A in hedgehog signal transduction and Drosophila imaginal disc development. Cell 80:553-562[ISI][Medline].
Mathur A, Golombek DA, Ralph MR (1996) cGMP-dependent kinase inhibitors block light-induced phase advances of hamster circadian rhythms in vivo. Am J Physiol 270:R1031-R1036[Abstract/Free Full Text].
Medanic M, Gillette MU (1992) Serotonin regulates the phase of the rat suprachiasmatic circadian pacemaker in vitro only during the subjective day. J Physiol (Lond) 450:629-642[Abstract/Free Full Text].
Meyer-Franke A, Kaplan MR, Pfrieger FW, Barres BA (1995) Characterization of the signaling interactions that promote the survival and growth of developing retinal ganglion cells in culture. Neuron 15:805-819[ISI][Medline].
Mintz EM, Marvel CL, Gillespie CF, Price KM, Albers HE (1999) Activation of NMDA receptors in the suprachiasmatic nucleus produces light-like phase shifts of the circadian clock in vivo. J Neurosci 19:5124-5130[Abstract/Free Full Text].
Moore RY, Lenn NJ (1972) A retinohypothalamic projection in the rat. J Comp Neurol 146:1-14[ISI][Medline].
Moriya T, Yoshinobu Y, Yokota S, Akiyama M, Shibata S (1998) Potentiating action of MKC-242, a selective 5-HT1A receptor agonist, on the photic entrainment of the circadian activity rhythm in hamsters. Br J Pharmacol 125:1281-1287[ISI][Medline].
Obrietan K (2000) Circadian regulation of cAMP response element-mediated expression in the SCN. Meeting of the Society for Research on Biological Rhythms, Amelia Island, FL, May.
Obrietan K, Impey S, Storm DR (1998) Light and circadian rhythmicity regulate MAP kinase activation in the suprachiasmatic nuclei. Nat Neurosci 1:693-700[ISI][Medline].
Obrietan K, Impey S, Smith D, Athos J, Storm DR (1999) Circadian regulation of cAMP response element-mediated gene expression in the suprachiasmatic nuclei. J Biol Chem 274:17748-17756[Abstract/Free Full Text].
Perrimon N (1995) Hedgehog and beyond. Cell 80:517-520[ISI][Medline].
Pickard GE (1982) The afferent connections of the suprachiasmatic nucleus of the golden hamster with emphasis on the retinohypothalamic connection. J Comp Neurol 211:65-83[ISI][Medline].
Prosser RA, Gillette MU (1989) The mammalian circadian clock in the suprachiasmatic nuclei is reset in vitro by cAMP. J Neurosci 9:1073-1081[Abstract].
Prosser RA, Gillette MU (1991) Cyclic changes in cAMP concentration and phosphodiesterase activity in a mammalian circadian clock studied in vitro. Brain Res 568:234-238.
Rosen LB, Ginty DD, Weber MJ, Greenberg ME (1994) Membrane depolarization and calcium influx stimulate MEK and MAP kinase via activation of ras. Neuron 12:1207-1221[ISI][Medline].
Shearman LP, Zylka MJ, Weaver DR, Kolakowski LF, Reppert Jr SM (1997) Two period homologs: circadian expression and photic regulation in the suprachiasmatic nuclei. Neuron 19:1261-1269[ISI][Medline].
Shibata S, Tsuneyoshi A, Hamada T, Tominaga K, Watanabe S (1992) Phase-resetting effect of 8-OH-DPAT, a serotonin 1A receptor agonist, on the circadian rhythm of firing rate in the rat suprachiasmatic nuclei in vitro. Brain Res 582:353-356[ISI][Medline].
Shibata S, Watanabe A, Hamada T, Tominaga K, Watanabe S (1994) N-methyl-D-aspartate induces phase shifts in circadian rhythm of neuronal activity of rat SCN in vitro. Am J Physiol 267:R360-R364[Abstract/Free Full Text].
Shigeyoshi Y, Taguchi K, Yamamoto S, Takekida S, Yan L, Tei H, Moriya T, Shibata S, Loros JJ, Dunlap JC, Okamura H (1997) Light-induced resetting of a mammalian circadian clock is associated with rapid induction of the mPer1 transcript. Cell 91:1043-1053[ISI][Medline].
Shirakawa T, Moore RY (1994) Glutamate shifts the phase of the circadian neuronal firing rhythm in the rat suprachiasmatic nucleus in vitro. Neurosci Lett 178:47-50[ISI][Medline].
Sun ZS, Albrecht U, Zhuchenko O, Bailey J, Eichele G, Lee CC (1997) RIGUI, a putative mammalian ortholog of the Drosophila period gene. Cell 19:1003-1011.
Takumi T, Matsubara C, Shigeyoshi Y, Taguchi K, Yagita K, Maebayashi Y, Sakikida Y, Okumura K, Takashima N, Okamura H (1998) A new mammalian period gene predominantly expressed in the suprachiasmatic nucleus. Genes Cells 3:167-176[Abstract].
Tei H, Numano R, Sakaki Y, Yamazaki S, Menaker M (2000) Transgenic analysis of a mammalian clock gene, Per1. Meeting of Society for Research on Biological Rhythms Abstr 132.
Tischkau SA, Barnes JA, Lin F-J, Myers EM, Barnes JW, Meyer-Bernstein EL, Hurst WJ, Burgoon PW, Chen D, Sehgal A, Gillette MU (1999) Oscillation and light induction of timeless mRNA in the mammalian circadian clock. J Neurosci 19:RC15 (1-6).
Weber ET, Gannon RL, Rea MA (1995) cGMP-dependent protein kinase inhibitor blocks light-induced phase advances of hamster circadian rhythms in vivo. Neurosci Lett 197:227-230[ISI][Medline].
Wu J, Dent P, Jelinek T, Wolfman A, Weber MJ, Sturgill TW (1993) Inhibition of the EGF-activated MAP kinase signaling pathway by adenosine 3',5'-monophosphate. Science 262:1065-1069[Abstract/Free Full Text].
Zylka MJ, Shearman LP, Weaver DR, Reppert SM (1998) Three period homologs in mammals: differential light responses in the suprachiasmatic circadian clock and oscillating transcripts outside of the brain. Neuron 20:1103-1110[ISI][Medline].

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