Coupling of Muscarinic Cholinergic Receptors and cGMP in Nocturnal Regulation of the Suprachiasmatic Circadian Clock

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Volume 17, Number 2, Issue of January 15, 1997 pp. 659-666
Copyright ©1997 Society for Neuroscience

Coupling of Muscarinic Cholinergic Receptors and cGMP in Nocturnal Regulation of the Suprachiasmatic Circadian Clock

Chen Liu¹, Jian M. Ding¹^,², Lia E. Faiman², and Martha U. Gillette¹^,²^,³
¹ Neuroscience Program and Departments of ² Cell and Structural Biology and ³ Molecular and Integrative Physiology, University of Illinois at Urbana-Champaign, Urbana, Illinois 61801

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Acetylcholine has long been implicated in nocturnal phase adjustment of circadian rhythms, yet the subject remains controversial.Although the suprachiasmatic nucleus (SCN), site of the circadianclock, contains no intrinsic cholinergic somata, it receives cholineacetyltransferase-immunopositive projections from basal forebrainand mesopontine tegmental nuclei that contribute to sleep andwakefulness. We have demonstrated that the SCN of inbred ratsin a hypothalamic brain slice is sensitive to cholinergic phaseadjustment via muscarinic receptors (mAChRs) only at night. Weused this paradigm to probe the muscarinic signal transductionmechanism and the site(s) gating nocturnal responsiveness. Thecholinergic agonist carbachol altered the circadian rhythm ofSCN neuronal activity in a pattern closely resembling that foranalogs of cGMP; nocturnal gating of clock sensitivity to eachis preserved in vitro. Specific inhibitors of guanylyl cyclase(GC) and cGMP-dependent protein kinase (PKG), key elements inthe cGMP signal transduction cascade, blocked phase shifts inducedby carbachol. Further, carbachol administration to the SCN atnight increased cGMP production and PKG activity. The carbachol-inducedincrease in cGMP was blocked both by atropine, an mAChR antagonist,and by LY83583, a GC inhibitor. We conclude that (1) mAChR regulationof the SCN is mediated via GC $right-arrow$ cGMP $right-arrow$ PKG, (2) nocturnal gating ofthis pathway is controlled by the circadian clock, and (3) a gatingsite is positioned downstream from cGMP. This study is among thefirst to identify a functional context for mAChR-cGMP couplingin the CNS.
Key words: suprachiasmatic nucleus; acetylcholine; carbachol; circadian rhythm; guanylyl cyclase; muscarinic receptor; cyclic GMP; cGMP-dependent protein kinase; KT5823; LY83583; enzyme activity assay; scintillation proximity assay; sleep

INTRODUCTION

The near 24 hr oscillations of physiological and behavioral functions in mammals are controlled by a central pacemaker, orclock, within the suprachiasmatic nucleus (SCN) of the hypothalamus.The SCN receives diverse neural and hormonal inputs by which signalscommunicating environmental and organismic states are transmittedto the SCN and can modify its phase (for review, see Inouye andShibata, 1994; Moore, 1996). Clock properties are endogenous tothe SCN; spontaneous neuronal activity continues to oscillatein a circadian rhythm under constant conditions in a hypothalamicslice of SCN from rat (Green and Gillette, 1982; Prosser and Gillette,1989), and the phasing of this rhythm can be reset by treatingthe SCN slice with the transmitters or peptides contained in afferentfibers (for review, see Gillette et al., 1995). Although the circadianclock is sensitive to resetting by diverse neurotransmitters,the sensitivity to each is restricted, or gated, to discrete phasesof the clock's 24 hr cycle (Gillette, 1996).

One class of afferent projections to the SCN contains acetylcholine (ACh), as revealed by choline acetyltransferase (ChAT,biosynthetic for ACh) immunostaining (van den Pol and Tsujimoto,1985; Ichikawa and Hirata, 1986; Rao et al., 1987; Tago et al.,1987). Bidirectional tract-tracing combined with immunocytochemistryfor ChAT localized cholinergic neurons that project to the ratSCN to the major cholinergic regions of the CNS: the basal forebrainas well as the peduncular pontine tegmental and the lateral dorsaltegmental nuclei of the brainstem (Bina et al., 1993). These cholinergicnuclei contribute to state changes in multiple brain sites, includingthose underlying sleep and wakefulness (Semba, 1991; Steriadeand McCarley, 1990).

The functional significance of the cholinergic projections to the SCN has been unclear. Attempts to address this issue invivo have involved administration of carbachol, a general cholinergicagonist. Although these studies present variability in both designand data, there is concordance that phasing of the circadian systemcan be modulated by cholinergic stimulation at night (Zatz andBrownstein, 1979; Zatz and Herkenham, 1981; Ernest and Turek,1983, 1985; Meijer et al., 1988; Wee et al., 1992). Within andnear the rat SCN, some neurons are cholinoceptive (Nishino andKoizumi, 1977; Shibata et al., 1983; Kow and Pfaff, 1984; Milleret al., 1987; Liu, 1995), and modest evidence exists for nicotinicor muscarinic ACh receptors (mAChRs) (Fuchs and Hoppens, 1978;van der Zee et al., 1991). Direct and specific cholinergic stimulationof the SCN in a brain slice preparation induces large phase advancesin the SCN neuronal activity rhythm; this response is mediatedby an mAChR, possibly an M1 subtype (Liu and Gillette, 1996).

ACh has been linked to cGMP production in brain and cultured neurons through a muscarinic mechanism (Tonnaer, 1991; Castoldiet al., 1993; Hu and El-Fakahany, 1993; Mathes and Thompson, 1996).However, functional contexts for this coupling in the CNS havenot been reported. We hypothesized that cholinergic activationof a cGMP pathway within the SCN mediates nocturnal phase resetting.Following up on our preliminary report (Liu and Gillette, 1994),we tested this hypothesis by attempting to block the phase shiftsinduced by carbachol through inhibiting cGMP-dependent proteinkinase (PKG) and guanylyl cyclase (GC). We then measured directlythe activity of PKG and the production of cGMP in the SCN in responseto carbachol. We also tested the ability of the muscarinic antagonistatropine and of a GC inhibitor to block the effect of carbacholon cGMP production. Our results demonstrate that carbachol advancesthe phase of the SCN clock at night via mAChR-mediated activationof a GC/cGMP/PKG pathway.

MATERIALS AND METHODS
Animals and brain slice preparation. Eight-week-old Long-Evans rats from our inbred colony were used in this study. This colonyhas been inbred in our Illinois facility for more than 32 generationsand, thus, exceeds the level of inbreeding required for genetichomogeneity. Animals were maintained and tissue prepared in fullaccord with institutional and federal guidelines for the humanetreatment of animals. The rats were kept on a schedule of 12:12hr light/dark cycle, with access to food and water ad libitum.They were killed between circadian time 7-10 (CT 7-10, where CT0 is defined as the beginning of the light period of the animalcolony), and the brain was quickly dissected from the skull. Thebrain was then manually sectioned to form a block of tissue containingthe hypothalamic region. This block of tissue was transferredto a mechanical tissue chopper, where 500 µm coronal slices weremade. The hypothalamic slices containing the SCN were then transferredto the brain slice dish, where they were maintained for up to3 d. Under these conditions, the SCN generates near 24 hr oscillationsin neuronal activity (Green and Gillette, 1982) that are stableover 3 d (Prosser and Gillette, 1989). The unperturbed sinusoidalpattern of ensemble activity is stable, running very close to24 hr. It is predictably high in the day (peaking mid-day nearCT 7) and is low at night (Gillette and Prosser, 1988), so thatmeasure of the time-of-peak can be used as an accurate assessmentof the phase of the circadian oscillation (Gillette et al., 1995).

The brain slice dish, consisting of an inner and an outer chamber, was modeled after Hatton et al. (1980). The outer chamberof the dish was filled with dH₂O warmed to 37°C and continuouslybubbled with 95% O₂/5% CO₂. Brain slices were maintained at thegas/liquid interface within the inner chamber and perifused at35 ml/hr with warmed, oxygenated Earle's balanced salt solution(EBBS, Life Technologies, Gaithersburg, MD) supplemented to 24.6mM glucose, 26.3 mM NaHCO₃, and 0.005% gentamicin, pH 7.3-7.4.

In the experiments measuring cGMP levels and PKG activity, a reduced SCN slice was made using iridectomy scissors under adissecting microscope and then transferred into the brain slicechamber. At the appropriate CT (>2 hr later), the reduced slicewas either (1) frozen at $-$ 80°C until assay for PKG activity, or(2) transferred to equilibrated EBSS at 37°C in an Eppendorf tubegassed with 95% O₂/5% CO₂ and maintained stably for 60 min inIBMX (100 µM) for assay of cGMP accumulation. For the cGMP measurements,inhibitors, such as atropine and LY83583, were added after 45min and for a total of 15 min; carbachol was added to the tubeduring the last 3-4 min, after which cGMP was extracted by EtOH(100%). The reduced SCN slice contains the paired SCN, a thinrim of hypothalamic tissue around the SCN, and the underlyingoptic chiasm. The circadian oscillation in neuronal firing ismaintained in reduced SCN slices (Gillette and Reppert, 1987).

Extracellular electrical recording and data analysis. The method for recording the circadian rhythm of the ensemble of SCNneurons has been detailed and thoroughly validated (Prosser andGillette, 1989); it is only briefly summarized here. Extracellularsignals of single neurons were recorded using glass microelectrodesfilled with 5 M NaCl. An electrode was lowered into the SCN bya hydraulic microdrive until the signal from a single cell wasencountered. Electrical signals exceeding twice the level of thebackground noise were isolated using a window discriminator, observedfor stability over at least 2 min, and counted by computer. Thefiring rate of each cell was monitored over two consecutive 120sec periods, using 10 sec bins. The electrode was then repositionedwithin the SCN so as to sample throughout the nucleus and advanceduntil another cell was encountered.

The firing rates of individual SCN neurons recorded during each experiment were grouped into 2 hr running averages using 15min lags. The time-of-peak was determined by visual inspectionof a plot of these values for the symmetrically highest point.Phase shifts were determined by comparing the time-of-peak electricalactivity in treated slices with that of vehicle-treated slices.Differences among groups were evaluated by ANOVA, with Duncan'stest for post hoc comparisons.

Experimental treatments. The protocol for drug administration to the SCN used in this study has been described (Liu and Gillette,1996). Briefly, brain slices were equilibrated in the recordingchamber for $>=$ 2 hr before administration of the reagent (dissolvedin EBSS then prepared to match the physical characteristics ofnormal medium in the chamber). Agonists were administered in amicrodrop (1 µl) applied to the surface of each SCN; this coveredonly the SCN tissue of the slice. After 5 min, the surface ofthe slice was rinsed toward the optic chiasm with warmed, gassedEBSS, and perifusion with normal medium was resumed. Antagonistswere applied as a static bath 10 min before, 5 min during, and15 min after the treatment. Results were compared with controlstreated in the same way with microdrops of EBSS only.

Assay of PKG activity. Endogenous PKG activity was measured according to Glass and Krebs (1982) using the PKG-specific heptapeptidesubstrate for PKG RKRSRAE (Peninsula Labs). Reduced SCN sliceswere exposed to carbachol for from 0 to 10 min, then frozen ondry ice. Single reduced slices were sonicated cold for 10 secin 50 µl buffer containing glycerophosphate 10 mM and a cocktailof protease inhibitors [phenylmethylsulfonyl fluoride (100 µM),phenanthroline (10 mM), leupeptin (2 µM), pepstatin (0.2 µM),and aprotinin (1%) (Sigma, St. Louis, MO)], BSA (0.1 mg/ml), KT5720(protein kinase A inhibitor, 0.1 µM), Tris (20 mM), pH 7.4, Mg²⁺ acetate (20 mM), and isobutylmethylxanthine (IBMX, 100 µM), andthen centrifuged at 2000 × g for 3 min at 4°C. A 30 µl aliquotof supernatant was taken and mixed with 15 µl of buffer containingthe heptapeptide substrate RKRSRAE (400 µg/ml), [³²P]ATP (1 µCi/tube), and unlabeled ATP (14 µM), and then incubatedfor 2 min at 37°C. The reaction was stopped by cooling on iceand adding 10 µl of 1N HCl. A 35 µl aliquot of the reaction productwas placed on filter paper (Whatman P81 disks) and air-dried.The filter paper was washed with 0.5% orthophosphoric acid untilno more radioactivity appeared in the effluent. The dried filterpaper was placed in a scintillation vial with 5 ml scintillationfluid and counted for 2 min. Activity is expressed as a percentageof the average activity immediately before carbachol administration(100%).

Scintillation proximity assay (SPA) of cGMP levels. The SPA assay for cGMP was performed according to the manufacturer's directions(Amersham, Arlington Heights, IL). The acetylation procedure wasfollowed both for the standard curve and for the samples. Briefly,single frozen reduced slices, ~30 µg of protein (Bradford, 1976),in 100 µl of EBSS without phenol red, were treated with 150 µlof 100% ethanol and the supernatant pipetted off to a fresh tube.The slices were resuspended and washed 1 time with 65% ethanol,and the supernatants of each slice pooled. These pooled supernatantswere lyophilyzed to dryness and resuspended in 100 µl of 0.05M acetate buffer containing 0.01% sodium azide. Equal amountsof cGMP standard, radioactive tracer, primary antibody, and secondaryantibody conjugated to beads were added. The mixtures were shakenovernight and counted in a Beckman scintillation counter. Effectsof treatment conditions on cGMP levels were compared by ANOVA,with Fisher's post hoc test.

RESULTS

Comparison of the phase-response relationships of carbachol and 8-Br-cGMP
Cholinergic effects on phasing of SCN circadian rhythms have been studied after a 5 min exposure to carbachol and other cholinergicagonists in a 1 µl microdrop (Liu and Gillette, 1996), whereasthe effects of 8-Br-cGMP have been assessed after 1 hr bath administration(Prosser et al., 1989). Therefore, we evaluated the phase shiftsinduced by microdrop versus bath treatments. We applied carbachol(100 µM) or 8-Br-cGMP (500 µM) as a 1 µl microdrop to the surfaceof the SCN in vitro for 5 min at CT 18 and compared the effectson the subsequent time-of-peak activity in the circadian rhythmSCN neuronal firing. The pattern of this endogenous circadianrhythm is normally a near 24 hr oscillation that peaks midsubjectiveday near CT 7 (7 hr into the light portion of the entrained light/darkcycle of the rat) (Fig. 1A). Mean time-of-peak for media-treatedcontrols in this study was CT 6.8 ± 0.1 (n = 5). The 5 min exposureto carbachol at CT 18 (midnight) induced a 6.0 hr phase advance(Fig. 1B) in the SCN neuronal activity rhythm (which is in agreementwith +6.3 ± 0.2 hr, n = 3, Liu and Gillette, 1996). 8-Br-cGMPadministered in this way induced a 6.0 ± 0.3 hr phase advance(n = 3) (Fig. 1C). These advances caused by brief, localized applicationof cGMP analog are not significantly different (p > 0.05) fromphase resetting induced by bathing the SCN for 1 hr in 500 µM8-Br-cGMP (+6.5 ± 0.2 hr, n = 3, Prosser et al., 1989). Thus,a 5 min exposure of the SCN to either carbachol or 8-Br-cGMP ina microdrop is sufficient to initiate the same phase shift asthat observed after bathing the whole hypothalamic slice in thecGMP analog for 1 hr at CT 18. Together, these data suggest thatSCN sensitivity to carbachol may be functionally related to itssensitivity to cGMP analogs.
Fig. 1. Carbachol and 8-Br-cGMP applied by microdrop at CT 18 induce similar phase advances of SCN circadian rhythms in brain slicesfrom inbred rats. A, In control brain slices, the SCN spontaneouslygenerates a circadian rhythm of neuronal activity that peaks nearCT 7 on days 2 and 3 in vitro (replotted from Ding et al., 1994).B, When a microdrop of carbachol (Carb, 100 µM in 1 µl) was appliedto the SCN at CT 18 for 5 min, peak activity was advanced by 6.0hr on subsequent days. C, When 8-Br-cGMP (500 µM in 1 µl) wasapplied to the SCN using this microdrop protocol, peak activitywas advanced by 6.5 hr. The 2 hr running averages ± SEMs of ensembleSCN neuronal firing rates are plotted against the CT of recording.Horizontal bars represent subjective night (the time of lights-offin the donor colony). Thin dashed line indicates the mean timeof peak activity in media-treated slices (CT 6.8 ± 0.1; n = 5).
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When we compared the phase-response relationships between the CT of treatment and responses of the SCN clock to carbachol(100 µM for 5 min in a 1 µl microdrop, Liu and Gillette, 1996)with those to 8-Br-cGMP (500 µM for 60 min in the bath, Prosseret al., 1989), the patterns were strikingly similar (Fig. 2).This similarity included the circadian timing of SCN sensitivityto both stimuli as well as the amplitude and direction of thephase shifts in the SCN rhythm. The SCN was generally unresponsiveto carbachol and 8-Br-cGMP treatments when either was administeredduring subjective day but responded with phase advances to treatmentsadministered throughout subjective night. The largest phase advancesto either carbachol or 8-Br-cGMP (+6.3 and +6.5 hr, respectively)were induced when the treatment was administered at CT 18. Wehave demonstrated that this nocturnal effect of carbachol on SCNphasing is mediated via an mAChR (Liu and Gillette, 1996); thus,it follows that the signal may activate a cGMP-dependent pathwayto initiate phase resetting.
Fig. 2. Comparison of the phase-response relationships for carbachol and 8-Br-cGMP in resetting the SCN circadian clock. The phaseshifts induced by carbachol (100 µM in 1 µl microdrops, solidcircles, Liu and Gillette, 1996) and by 8-Br-cGMP (500 µM in thebathing medium, open circles, Prosser et al., 1989) are plottedagainst the CT at which the treatment was administered. Each pointis the result of a single experiment in which the time-of-peakneuronal activity on the day after treatment (as in Fig. 1C) wasderived from recording 4-9 neurons/hr over 8-14 hr to define thepeak in neuronal activity. Symbols as in Figure 1.
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PKG and GC inhibitors block the response to carbachol
To explore the possibility that carbachol acts via a cGMP-dependent pathway, we tested selective inhibitors of steps in cGMPsignaling. First, the SCN slice was preincubated with an inhibitorspecific for cGMP-dependent PKG, KT5823, to determine whetherthis could block the phase advance induced by carbachol. In additionto activating PKG, 8-Br-cGMP can act directly on cGMP-dependentphosphodiesterases or ion channels to exert its effect (for review,see Corbin et al., 1990). To evaluate the potential contributionof these non-PKG-mediated mechanisms, we also tested whether KT5823could block the phase advance induced by 8-Br-cGMP. Microdropapplication of carbachol or 8-Br-cGMP for 5 min at CT 18 inducedrobust phase advances of >6 hr (Fig. 3A,B). KT5823 (0.1 µM), whenapplied in the bath during the period surrounding agonist treatment,blocked the phase-advancing effects of both carbachol (100 µM)and 8-Br-cGMP (500 µM) (+1.1 ± 0.3 hr, n = 3 and +1.2 ± 0.3 hr,n = 3, respectively) (Fig. 3C,D); the timing of the peak of theneuronal rhythm was not significantly different from the effectof KT5823 alone (+1.1 ± 0.2 hr, n = 3; p > 0.05) (Fig. 3E). Theseresults suggest that both carbachol and 8-Br-cGMP reset the SCNclock through activation of PKG and, further, that carbachol mayincrease endogenous cGMP by stimulating GC.
Fig. 3. The PKG-specific inhibitor KT5823 blocks the phase-advancing effects of both carbachol and 8-Br-cGMP. A microdrop of carbachol(heavy vertical dashed line) or 8-BR-cGMP (vertical dotted line)applied for 5 min at CT 18 caused 6.4 and 6.0 hr phase advances,respectively (A, B), in the time of the next peak. A 30 min bathapplication of KT5823 (0.1 µM) (vertical solid bar) induced asmall phase advance of ~1 hr (C). The effects of carbachol and8-Br-cGMP were blocked by the KT5823 pulse (D, E). Symbols areas in Figure 1.
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To determine whether the phase shift induced by carbachol requires activation of GC, the biosynthetic enzyme for cGMP, weevaluated the effect of LY83583, a specific inhibitor of GC. A30 min exposure of the SCN slice to LY83583 (3 µM) at CT 18 hadno effect on the time-of-peak in neuronal activity in the followingcircadian cycle (Fig. 4A). The same LY83583 treatment fully blockedthe phase-advancing effect of carbachol (Fig. 4B) (mean phaseadvance = 0.3 ± 0.2 hr, n = 3) (Fig. 5). However, it did not blockthe effect of 8-Br-cGMP (Fig. 4C) (+6.3 ± 0.3 hr, n = 3) (Fig.5). The fact that the same phase-advancing effect was inducedby the cGMP analog in the presence of the GC inhibitor is consistentwith cGMP acting downstream from GC in the signaling pathway.These experiments, together with the similarity of phase-responserelationships between carbachol and 8-Br-cGMP, support the hypothesisthat the cholinergic agonist carbachol regulates the SCN througha GC/cGMP/PKG-dependent mechanism.
Fig. 4. The GC inhibitor LY83583 blocks the effect of carbachol but not that of 8-Br-cGMP. A 30 min bath exposure to LY83583 (3 µM,vertical solid bar) did not affect the time-of-peak of the SCNfiring rate (A). LY83583 blocked the phase-advancing effects ofcarbachol but not of 8-Br-cGMP (B, C; compare with Fig. 3A, B).Symbols are as in Figure 1.
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Fig. 5. Effects of KT5823 (KT, 0.1 µM) and LY83583 (LY, 3 µM) on the phase advances induced by a microdrop of carbachol (CARB, 100µM) or 8-Br-cGMP (500 µM). The phase advances induced by CARB,8-Br-cGMP, and 8-Br-cGMP + LY were highly significantly differentfrom controls (**p < 0.01), whereas the other treatments werenot (p > 0.05). Average phase advances induced by each treatmentare represented by bars, with treatments labeled on top of eachbar. Plotted are the mean ± SEM (n = 3 for each).
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Carbachol rapidly stimulates cGMP production and PKG activity in the SCN
These experiments with inhibitors indicate that increased GC synthesis of cGMP and subsequent PKG activation are necessaryfor carbachol to induce resetting of the circadian clock. Therefore,we directly evaluated the effect of carbachol on each of theseeffectors. First, to assess the rate of the activation process,we examined the time course of PKG phosphotransferase activitytoward a PKG-selective substrate in response to carbachol treatment.To ensure that we measured responses localized within the SCN,the brain slice was surgically reduced to include only the 500µm slice of SCN centered along the rostrocaudal axis, a thin rimof surrounding hypothalamus, and the adherent optic chiasm. Thephosphodiesterase inhibitor IBMX (200 µM, 1 hr preincubation)was included to preserve cyclic nucleotides generated by the treatment;this increased basal PKG activity by ~30%, to 6500 cpm, on average.This value was then used as the normalized basal level beforecarbachol treatment. Carbachol application rapidly and significantlyincreased PKG activity; ³²P incorporation rose by up to 40% between 2 and 5 min of exposureto carbachol, with statistical significance at 5 min comparedwith 0 (p < 0.005), 1 and 10 min (both p < 0.05) (Fig. 6). Thecontrol procedure, which involved the same manipulation as withcarbachol but using only medium, did not increase the PKG activityafter 3 min (100 ± 15%, n = 4; p > 0.05). Therefore, carbacholadministration induces a rapid and transient activation of PKGin the SCN at CT 18, the time when it induces phase resetting.
Fig. 6. Carbachol administration activates PKG within the SCN. PKG activity in extracts of reduced SCN slices was measured by monitoring³²P incorporation into the preferred artificial PKG substrate peptideRKRSRAE. The general phosphodiesterase inhibitor IBMX (200 µM)and the specific PKA inhibitor KT 5720 (0.1 µM) were includedin the reaction. The average activity of PKG in each reduced sliceimmediately before carbachol treatment (0 min) was taken as 100%.The PKG activity in the SCN slice exposed to carbachol (100 µM)for 1, 2, 3, 5, and 10 min was measured and normalized to a percentageof the basal activity. Transient increase in the PKG activitywas observed, with 5 min showing significant elevation (asterisk)over 0 (p < 0.005), 1 and 10 min (both p < 0.05). The number ofsamples in each group is noted.
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To confirm that carbachol treatment increased cGMP levels, we measured total cGMP in the tissue and assay medium. Based onthe time course of the increase in PKG activity (Fig. 6), we examinedthe cGMP level at 3 min after carbachol or control treatments.After treatment at CT 18, cGMP levels increased dramatically (fivefold,on average) in SCN treated with carbachol (Fig. 7). The cGMP levelin vehicle-treated controls was 63.6 ± 4.6 fmol/reduced slice,whereas that in carbachol-treated samples was 291.8 ± 78.0 fmol/reducedslice (n = 7 and 8, respectively; p < 0.02).
Fig. 7. Carbachol increases cGMP production in the reduced SCN slice via an mAChR. Levels of cGMP in the SCN slices and assay mediumwere measured in the presence of IBMX by SPA (Amersham). Whenreduced SCN slices were treated with carbachol (100 µM) for 3min at CT 18, the level of cGMP increased significantly, from63.6 ± 4.6 fmol/reduced slice in vehicle-treated samples to 291.8± 78.0 fmol/reduced slice (n = 7 and 8; p < 0.002). This carbachol-inducedincrease in the cGMP was completely blocked by the muscarinicantagonist atropine (1 µM) as well as by the GC inhibitor LY83583(3 µM), which themselves had no effect on the cGMP level in theSCN (n = 4 and 3, respectively; p > 0.05). Results of individualexperiments (open circles) overlay the bars representing the mean± SEM.
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Our previous results demonstrated that phase shifts of SCN rhythms by cholinergic agonists are mediated by an M1-like mAChRmechanism (Liu and Gillette, 1996). To evaluate the pathway bywhich carbachol increases cGMP production in the SCN slice, weexamined the effects of the muscarinic antagonist atropine andof the GC inhibitor LY83583 at CT 18. Atropine (1 µM) itself hadno effect on the phase of the SCN circadian rhythm but blockedthe ability of carbachol to induce phase advances (Liu and Gillette,1996). Pretreatment of the reduced SCN slice with atropine inthe presence of IBMX completely inhibited the carbachol-stimulatedincrease in cGMP; thus, cGMP levels were equivalent to when atropinealone was added (65.9 ± 6.3 fmol/reduced slice and 58.5 ± 5.0fmol/reduced slice, n = 4 and 3, respectively; p < 0.05). Likewise,a 15 min exposure to LY83583 was without effect and also fullyblocked the carbachol-induced stimulation of cGMP (65.2 ± 1.2fmol/reduced slice and 58.2 ± 7.1 fmol/reduced slice, respectively;n = 3 for each; p < 0.05). These results demonstrate that administrationof carbachol to the SCN at CT 18 initiates an mAChR-mediated signalingcascade that increases cGMP production and, in turn, activatesPKG.

DISCUSSION
In the present study, we compared the effect of carbachol on the circadian rhythm of SCN neuronal activity with the effectof a cGMP analog, 8-Br-cGMP, studied previously by Prosser etal. (1989). We found that the phase advance initiated by a 5 minapplication of carbachol was of the same amplitude as that inducedby a 5- or 60 min exposure to 8-Br-cGMP. The phase-response relationshipsbetween timing of SCN sensitivity to carbachol and 8-Br-cGMP andtheir phase-resetting effects are fully overlapping; sensitivityto each is restricted to the subjective night. The specific PKGinhibitor KT5823 blocked the phase advances induced at midsubjectivenight (CT 18) by microdrop application of carbachol or 8-Br-cGMPto the SCN, whereas the GC inhibitor LY83583 blocked the phaseadvances induced by carbachol but not 8-Br-cGMP. PKG activityin the reduced SCN slice was transiently increased by 5 min aftercarbachol administration. Exposure of the SCN to carbachol rapidlyincreased cGMP levels; this increase was blocked by inhibitingeither mAChRs or GC. We conclude that muscarinic cholinergic regulationof the SCN circadian clock at night is mediated via activationof a GC/cGMP/PKG signaling pathway.

Evidence that ACh activates a nocturnally gated GC/cGMP/PKG pathway
Our conclusions are supported by three lines of evidence. First, both the coincidence in the circadian timing of SCN sensitivitiesand the similarity of responses to carbachol and 8-Br-cGMP suggestthat they may use a common pathway to induce phase shifts. Thecircadian clock in the SCN can be reset by a number of intercellularmessengers, including serotonin (Prosser et al., 1990; Medanicand Gillette, 1992), neuropeptide Y (Medanic and Gillette, 1993),glutamate (Ding et al., 1994), and melatonin (McArthur et al.,1997). Yet, the ability of the SCN to respond to each of thesestimuli is restricted, or gated, to discrete domains of the circadiancycle. Further, these changes in gating occur in SCN under constantconditions in vitro; therefore, differential gating must be aclock-controlled process (Gillette, 1996). Responses of the SCNto several candidate intracellular messengers are also differentiallygated (Prosser and Gillette, 1989; Prosser et al., 1989; Dinget al., 1994, 1997). This implies that a critical level of clock-controlledgating lies downstream from the second messenger(s) activatedby various neurotransmitter systems (Gillette, 1996). It followsthat the apparent similarity in the responses of the SCN clockto carbachol and 8-Br-cGMP suggests that they act via a commonsignaling pathway that can access the clock mechanism only atnight and that gating of this response can be controlled at asite downstream from cGMP.

Second, both the PKG inhibitor KT5823 and the GC inhibitor LY83583 blocked the effect of carbachol on clock phasing. KT5823is a highly selective inhibitor of PKG (K_i = 0.2 µM for PKG, K_i> 10 µM for PKA, and K_i = 4 µM for PKC) (Glass and Krebs, 1982).Thus, it is unlikely that KT5823, used at 0.1 µM in these experiments,acted through nonspecific inhibition of other kinases. LY83583,a widely used GC inhibitor that also inhibited cGMP productionin the SCN (Fig. 7), did not block the effect of 8-Br-cGMP. Thisis consistent with cGMP lying downstream from GC in the signalingpathway by which the clock mechanism is accessed. The observationthat two inhibitors acting at different levels of the same cGMPsignal transduction pathway each inhibited the effects of carbacholin the SCN indicates that the carbachol-induced nocturnal phaseshift is caused by specific activation of GC and PKG.

Third, carbachol significantly increased both PKG activity and cGMP production in the SCN. We monitored ³²P incorporation into the preferred substrate of PKG (Glass andKrebs, 1982; Weber, 1995) in the presence of a selective PKA inhibitor,KT 5720, conditions unlikely to measure phosphorylation causedby a kinase other than PKG. Furthermore, KT5823 is an effectiveinhibitor of this kinase in this tissue; it blocks ³²P incorporation into natural substrate proteins of SCN tissueby endogenous PKG (L. Faiman, unpublished observations). The timecourse of the increase in PKG activity in the SCN by carbacholis similar to the time course of the cGMP increase in rat superiorcervical ganglia (Ando et al., 1994). To further test our hypothesis,a highly specific cGMP immunoassay was used to measure cGMP productionin response to carbachol; a significant increase in cGMP was observedwithin 3 min. The relatively smaller amplitude of increase inthe PKG activity stimulated by carbachol compared with enhancementof actual cGMP levels could reflect a limited amount of PKG availablefor activation by cGMP. Nevertheless, the increases in both thecGMP level and PKG activity in SCN stimulated by carbachol stronglysupport the conclusion that carbachol acts through a cGMP/PKGpathway to induce phase shifts.
Coupling of mAChR-activation to a cGMP pathway The increase in cGMP induced by carbachol was blocked by 1 µM atropine, indicating involvement of an mAChR. Our study of thepharmacology of cholinergic regulation of the SCN circadian rhythmconcluded that the nocturnal response to cholinergics is mediatedby an M1-like mAChR subtype (Liu and Gillette, 1996). The relativepotencies of muscarinics inducing phase advance at CT 18 are ACh> McN-A-343 > carbachol ~ muscarine, and relative efficacies ofantagonists in blocking carbachol are atropine > pirenzepine >4-DAMP. Molecular cloning has revealed five subtypes of mAChRs,m1-m5 (Bonner et al., 1987, 1988), the first four of which correspondto the M1-M4 receptors identified pharmacologically (Waelbroecket al., 1986, 1990; Ehlert and Tran, 1990; Watson and Abbot, 1992).These muscarinic subtypes can impinge on a range of signal transductionpathways, including activating phospholipase C through m1, m3,and m5 receptors, inhibiting adenylyl cyclase through m2 and m4receptors, as well as activating G-protein-mediated ion channels(Hulme et al., 1990).

Coupling of mAChR activation and cGMP production has been demonstrated in both peripheral and central nervous tissue and incell culture. For example, stimulation of mAChRs causes cGMP accumulationin ganglionic tissues of various species (Wamsley et al., 1979;Frey and McIssac, 1981). More recently, ACh agonists have beenreported to increase cGMP synthesis via an mAChR in brain tissueand in neuroblastoma cells (Tonnaer, 1991; Castoldi et al., 1993;Hu and El-Fakahany, 1993; Mathes and Thompson, 1996). The linkbetween the mAChR and cGMP synthesis is indirect, because no G-protein-activatedGCs have been found. Instead, signaling through mAChRs appearsto involve an intermediary, such as Ca²⁺/nitric oxide (NO) (Schultz et al., 1973; Castoldi et al., 1993;Hu and El-Fakahany, 1993; Ando et al., 1994; Mathes and Thompson,1996), CO (Ingi et al., 1996), and/or a metabolite of arachidonicacid (Snider et al., 1984; McKinney and Richelson, 1986). It remainsto be tested whether NO, CO, arachidonic acid, or multiple pathwaysare involved in the muscarinic regulation of the SCN circadianrhythm.

cGMP and circadian clock regulation by cholinergic signals
ACh is among the longest-studied regulators of circadian timing. Cholinergics have been administered at a range of sites inthe periphery and CNS, and their effects on circadian rhythmshave been measured at various endpoints (behavior, hormone secretion,neuronal activity). Because the results have not produced a congruentprofile of timing of sensitivity, site of efficacy, or receptor-effectorcoupling, a question still remains as to the role of cholinergicsignaling in the regulation of the circadian system. Various cholinergicsensitivities at multiple brain and peripheral levels subservingcircadian rhythmic processes are likely to underlie the lack ofcoherence in these observations.

Yet despite the diversity in these experimental designs, the resulting windows of circadian sensitivity to cholinergics havestrong correlations with the window of circadian sensitivity tolight. Light is the most powerful nocturnal regulator of circadianrhythms. Retinal fibers project directly both to the SCN, siteof the circadian clock, and to the basal forebrain cholinergicneurons, which function in sleep and arousal (Semba, 1991; Steriadeand McCarley, 1990). Thus, light could activate neurons in thebasal forebrain complex to release ACh onto SCN neurons duringglutamatergic neurotransmission from projections of the retinohypothalamictract. Cholinergic-glutamatergic interactions are well documentedin brain sites modified by learning (Aigner, 1995). It followsthat the phase-resetting signal at the SCN may represent the integrationof ongoing activities in brain regions subserving sleep and wakefulnesswith those from other brain sites regulating the biological clock.Indeed, the GC/cGMP/PKG pathway, which we here demonstrate mediatescoupling of SCN mAChRs and circadian clock processes, contributesto light-stimulated nocturnal phase resetting in the phylogeneticallydistant clocks of both hamsters (Weber et al., 1995; Mathur etal., 1996) and sea hares (Eskin et al., 1984).

We have approached the contentious issue of whether and in what way cholinergic stimulation affects the circadian clock bystudying a brain slice preparation and selectively manipulatingthe neurochemical environment of this isolated SCN. Although wedo not exclude a nicotinic response at other times of day (seeTraschel et al., 1995), our evaluation of cholinergic mechanismsgenerates remarkably coherent support for our initial hypothesis:nocturnal cholinergic stimulation of mAChRs within the SCN canreset the circadian clock by stimulating GC, generating cGMP,and activating PKG. Important support for this pathway would becontributed by demonstration that M1 mAChRs are localized in proximityto cholinergic terminals within the SCN.

Although mechanisms that restrict the cholinergic response to the clock's nocturnal domain are unknown, access is likely regulatedalong signaling pathways. Because cGMP analogs reset the SCN atnight, but not daytime, at least one gating site lies downstreamfrom cGMP. Precisely which steps downstream from cGMP are gatedby the clock, what molecular mechanisms regulate their open state,and how they facilitate clock access during state-dependent changesin other brain regions, such as those contributing to sleep andwakefulness, will be important to establish. Nevertheless, thisdemonstration of mediation of nocturnal clock resetting is amongthe first studies to identify a specific functional consequenceof the coupling of mAChRs and the cGMP signaling pathway in theCNS.

FOOTNOTES

Received June 24, 1996; revised Oct. 17, 1996; accepted Nov. 12, 1996.

This work was supported by Public Health Service Grants NS22155 and NS33240 from the National Institute of Neurological Disordersand Stroke. We thank Liana Kuriashkina for excellent technicalassistance, E. Todd Weber and Shelley Tischkau for technical advice,and Dong Chen and Tom Tcheng for thoughtful comments.

Correspondence should be addressed to Prof. Martha U. Gillette, Department of Cell and Structural Biology, University of Illinois,B107 Chemical and Life Sciences Laboratory, MC-123, 601 SouthGoodwin Avenue, Urbana, IL 61801.

Dr. Liu's present address: Laboratory of Developmental Chronobiology, Children's Service, GRJ 1226, Massachusetts GeneralHospital, Boston, MA 02114.

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Volume 17, Number 2, Issue of January 15, 1997 pp. 659-666 Copyright ©1997 Society for Neuroscience

Coupling of Muscarinic Cholinergic Receptors and cGMP in Nocturnal Regulation of the Suprachiasmatic Circadian Clock

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Volume 17, Number 2, Issue of January 15, 1997 pp. 659-666
Copyright ©1997 Society for Neuroscience