Excitatory Mechanisms in the Suprachiasmatic Nucleus: The Role of AMPA/KA Glutamate Receptors

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Excitatory Mechanisms in the Suprachiasmatic Nucleus: The Role of AMPA/KA Glutamate Receptors

Stephan Michel,^* Jason Itri,^* and Christopher S. Colwell

Mental Retardation Research Center, Department of Psychiatry and Biobehavioral Sciences, University of California, Los Angeles, California 90024-1759

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Michel, Stephan, Jason Itri, and Christopher S. Colwell. Excitatory Mechanisms in the Suprachiasmatic Nucleus: The Role of AMPA/KA Glutamate Receptors. J. Neurophysiol. 88: 817-828, 2002. A variety of evidence suggests that the effects of light on the mammalian circadian system are mediated by direct retinalganglion cell projection to the suprachiasmatic nucleus (SCN).This synaptic connection is glutamatergic and the release of glutamateis detected by both N-methyl-D-asparate (NMDA) and amino-methylproprionic acid/kainate (AMPA/KA) iontotropic glutamate receptors(GluRs). It is well established that NMDA GluRs play a criticalrole in mediating the effects of light on the circadian system;however, the role of AMPA/KA GluRs has received less attention.In the present study, we sought to better understand the contributionof AMPA/KA-mediated currents in the circadian system based inthe SCN. First, whole cell patch-clamp electrophysiological techniqueswere utilized to measure spontaneous excitatory postsynaptic currents(sEPSCs) from SCN neurons. These currents were widespread in theSCN and not just restricted to the retino-recipient region. ThesEPSC frequency and amplitude did not vary with the daily cycle.Similarly, currents evoked by the exogenous application of AMPAonto SCN neurons were widespread within the SCN and did not exhibita diurnal rhythm in their magnitude. Fluorometric techniques wereutilized to estimate AMPA-induced calcium (Ca²⁺) concentration changes in SCN neurons. The resulting data indicatethat AMPA-evoked Ca²⁺ transients were widespread in the SCN and that there was a dailyrhythm in the magnitude of AMPA-induced Ca²⁺ transients that peaked during the night. By itself, blockingAMPA/KA GluRs with a receptor blocker decreased the spontaneousfiring of some SCN neurons as well as reduced resting Ca²⁺ levels, suggesting tonic glutamatergic excitation. Finally, immunohistochemicaltechniques were used to describe expression of the AMPA-preferringGluR subunits GluR1 and GluR2/3s within the SCN. Overall, ourdata suggest that glutamatergic synaptic transmission mediatedby AMPA/KA GluRs play an important role throughout the SCN synapticcircuitry.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The circadian clock regulates many aspects of an organism's behavior and physiology. In mammals, the part of the nervous systemresponsible for most circadian behavior can be localized to apair of structures in the hypothalamus known as the suprachiasmaticnucleus (SCN). Importantly, when SCN cells are removed from theorganism and maintained in a brain slice preparation, they continueto generate circadian rhythms in electrical activity, secretion,and gene expression (reviewed by Gillette 1997). Previous studiessuggest that the basic mechanism responsible for the generationof these rhythms is intrinsic to individual cells in the SCN (Welshet al. 1995) and perhaps in other cell types (Balsalobre et al.1998). The core molecular mechanism driving these cellular oscillationsappears to be a negative feedback loop operating at the transcriptional/translationallevels (e.g., King and Takahashi 2000; Reppert and Weaver 2001).The circadian oscillator located in these cells generates a rhythmthat repeats with a frequency of close to but not equal to 24h. To function adaptively, these cells must be synchronized tothe exact 24 h cycle of the physical world. The daily cycle oflight and dark is the dominant cue used by organisms to synchronizetheir biological clocks to the environment. Thus a major goalof research in this area is to understand the mechanisms by whichlight acts to synchronize circadianoscillators.

The SCN receives photic information directly through a monosynaptic projection from the retina known as the retinal hypothalamictract (RHT) as well as through an indirect connection from theintergeniculate leaflet (Ibata et al. 1999; Moore 1996; Morin1994). The RHT appears to be necessary and sufficient for entrainmentby light, and thus a focal point of research in this area hasbeen to identify the transmitters released by the RHT and theresulting signal transduction cascades activated in the SCN. Thereis now very good evidence that glutamate mediates the effectsof light on the circadian system through its role as a transmitterat the RHT/SCN synaptic connection (Colwell and Menaker 1996;Ebling 1996; Mintz et al. 1999; Obrietan et al. 1998). In thesimplest case, light causes the release of glutamate that initiatesa signal-transduction cascade in SCN neurons that ultimately resultsin a phase shift of the circadian system. This release of glutamateis detected by both N-methyl-D-asparate (NMDA) and amino-methylproprionic acid/kainate (AMPA/KA) iontotropic glutamate receptors(GluRs). There is a variety of evidence to suggest that the NMDAreceptor plays a special role in the transduction of the lightinput to the SCN and that the function of these receptors is gatedby the circadian system (e.g., Colwell 2001; Pennartz et al. 2001;for review: Ebling 1996). The role of AMPA/KA-type GluRs in theSCN is less clear. The receptors are present in the SCN (e.g.,Gannon and Rea 1993, 1994; Mikkelsen et al. 1995; Stamp et al.1997; van den Pol et al. 1994) and a circadian rhythm of AMPAreceptor GluR2/3 subunit immunoreactivity has been reported (Chambille1999). The excitatory postsynaptic responses recorded in the SCNare largely mediated by AMPA/KA GluRs (e.g., Cahill and Menaker1989; Cui and Dyball 1996; de Vries et al. 1994; Jiang et al.1997; Kim and Dudek 1991). Finally, light-induced phase shiftsof the circadian rhythm in locomotor activity were prevented bythe administration of AMPA/KA GluR blockers (Colwell and Menaker1992; Rea et al. 1993). In many synapses, NMDA GluRs work in concertwith the AMPA/KA GluRs that are responsible for the initial depolarizationof the postsynaptic membrane. The depolarization is required beforethe membrane potential moves into the voltage range at which theNMDA GluR can become active. Postsynaptic responses of SCN neuronsseem to follow the same principal with an additional circadianmodulation of the NMDA GluR sensitivity (Colwell 2001; Pennartzet al. 2001). In other neurons, the active regulation of the AMPAGluR plays a major role in determining the contribution of theNMDA GluR to the postsynaptic response (e.g., Durand et al. 1996;Isaac et al. 1995; Luthi et al. 1999). Thus we became interestedin better understanding the physiology of AMPA/KA-mediated currentsin SCNneurons.

The present study utilized whole cell patch electrophysiological techniques to record AMPA-mediated currents in SCN cellsin a brain slice preparation. As a first step, spontaneous excitatorypostsynaptic currents (sEPSC) were recorded from SCN slices fromanimals maintained in a light-dark (LD) cycle. Comparisons weremade between ventrolateral (VL) and dorsomedial (DM) regions ofthe SCN as well as between day and night. Electrophysiologicalmethods were also used to directly measure AMPA-mediated currentsin SCN neurons and to determine if the magnitude of these currentsvaried between SCN regions or from day to night. Next, fluorometricmeasurements using the Ca²⁺ indicator dye fura2-AM were used to measure AMPA-induced Ca²⁺ transients. Finally, immunocytochemical techniques were usedto confirm the presence of AMPA GluR subunits in the SCN and toexamine the distribution of the protein throughout thestructure.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Animals and brain slice preparation

The UCLA Animal Research Committee approved the experimental protocols used in this study. Brain slices were prepared usingstandard techniques from rats (Sprague-Dawley) between 10 and14 days of age. For reasons that are not completely understood,infrared differential interference contrast (IR-DIC) videomicroscopyand dye-loading with acetoxymethyl (AM) esters work better inslices from young animals. The circadian oscillator based in theSCN is functional by this age (e.g., Reppert and Schwartz 1984;Shibata and Moore 1987). Rats were killed by decapitation, andbrains were dissected and placed in cold oxygenated artificialcerebral spinal fluid (ACSF) containing (in mM) 130 NaCl, 26 NaHCO₃,3 KCl, 5 MgCl₂, 1.25 NaH₂PO₄, 1 CaCl₂, and 10 glucose (pH 7.2-7.4;osmolality, 290-300 mosM). After cutting slices, transverse sections(350 µm) were placed in ACSF (25-27°C) for at least 1 h (in thissolution, CaCl₂ was increased to 2 mM, MgCl₂ was decreased to2 mM). Slices were constantly oxygenated with 95% O₂-5% CO₂. Sliceswere placed in a perfusion chamber (Warner Instruments, Hamden,CT) attached to the stage of the fixed-stage upright microscope.The slice was held down with thin nylon threads glued to a platinumwire and submerged in continuously flowing, oxygenated ACSF at2 ml/min. Solution exchanges within the slice were achieved bya rapid gravity feed delivery system. In our system, the effectsof bath applied drugs begin within 15 s and are typically completeby 1-2min.

IR-DIC videomicroscopy

Slices were viewed with an upright compound microscope (Olympus BX50), using a water-immersion lens (×40) and DIC optics.They were illuminated with near IR light by placing an IR band-passfilter (750-1050 nm) in the light path. The image was detectedwith an IR-sensitive video camera (Hamamatsu C2400, Bridgewater,NJ) and displayed on a video monitor. A camera controller allowedanalog contrast enhancement and gain control. Cells were typicallyvisualized from 30 to 100 µm below the surface of the slice. Inthe present study, IR videomicroscopy was utilized to visualizecells within the brain slice and to limit some of the uncertaintyas to the cell type. This imaging technique allowed us to clearlysee the SCN and to exclude cells from the surrounding hypothalamicregions. In addition, morphological criteria were used to targetSCN neurons and to avoid taking measurements from cells that wereclearly glia. While size is hardly foolproof, in a few cases,electrophysiological recording and fluorescent imaging were combinedto demonstrate that the cells from which Ca²⁺ levels were being measured indeed show the electrical propertiesof neurons (n = 5). Accordingly, it is likely that most of thedata were collected from SCNneurons.

Whole cell patch-clamp electrophysiology

Methods were similar to those described previously (Colwell et al. 1998). Briefly, electrodes were pulled on a multistagepuller (Sutter P-97, Novato, CA). Electrode resistance in thebath was typically 4-6 M $Omega$ . The standard solution in the patchpipette contains (in mM) 125 Cs-methanesulfonate, 8 HEPES, 5 MgATP,4 NaCl, 3 KCl, 9 EGTA, MgCl₂, 1 GTP, 0.1 leupeptin, and 10 phosphocreatine.The pH was adjusted to 7.25-7.3 using CsOH and the osmolarityto 280-290 mosM using sucrose. For sEPSCs and cell-attached recordings,Cs⁺ was replaced by K⁺ in the pipette solution. Whole cell recordings were obtainedwith an Axon Instruments 200B amplifier and monitored on-linewith pCLAMP (Axon Instruments, Foster City, CA). To minimize changesin offset potentials with changing ionic conditions, the groundpath used an ACSF agar bridge. Cells were approached with slightpositive pressure (2-3 cm H₂O), and offset potentials were corrected.The liquid junction potential was measured to be $-$ 14 mV. The pipettewas lowered to the vicinity of the membrane keeping a positivepressure. After forming a high-resistance seal (2-10 G $Omega$ ) by applyingnegative pressure, a second pulse of negative pressure was usedto break the membrane. While entering the whole cell mode, a repetitivetest pulse of 10 mV was delivered in a passive potential range(approximately equal to $-$ 60 to $-$ 70 mV). Whole cell capacitanceand electrode resistance were neutralized and compensated (50-80%)using the test pulse. Data acquisition was then initiated. Seriesand input resistance was monitored repeatedly by checking theresponse to small pulses in a passive potential range. Seriesresistance was not compensated, and the maximal voltage errordue to this resistance was calculated to be 6 mV. The access resistanceof these cells ranged from 20 to 40 M $Omega$ while the cell capacitancewas typically between 6 and 18pF.

Under voltage-clamp (V_m = $-$ 70 mV), the holding current was monitored throughout the experiment. In addition, the neuron'scurrent-voltage relationship was measured every 2-3 min by movingthe cells membrane potential through a series of steps or a rampof voltages. In these experiments, after the initial control ramps(no drug), each cell was exposed to one concentration of AMPAfollowed by a wash until the response returned to baseline. TheAMPA-evoked currents were determined from neurons using a rampcommand voltage from $-$ 70 to +40 mV (over 5 s) and then back to $-$ 90 mV (1 s). All data were collected from the downward ramp.Current-voltage relationships were calculated as the responseto the agonist minus the baseline response in the absence of theagonist. Current measurements were normalized to cell size bydividing peak inward current divided by cellcapacitance.

Spontaneous postsynaptic currents were analyzed using the MiniAnalysis program (Synaptosoft, Decatur, GA). The software wasused to automatically record the number and peak amplitude ofsEPSCs recorded in gap-free mode of pCLAMP software. Each automaticallydetected event was then manually checked to ensure that the baselineand peak were accurately determined. The mean frequency, amplitude,rise time and decay time of the EPSCs was then calculated foreach neuron during 60- to 360-s samplingperiods.

Calcium imaging

A cooled CCD camera (Princeton Instruments, Microview model 1317 × 1035 pixel format) was added to the Olympus fixed-stagemicroscope to measure fluorescence after passing a dichroic filterwith a cutoff at 430 nm. To load the indicator-dye into cells,slices were incubated in membrane permeable fura2-AM (10 µM, MolecularProbes) at 37°C for 10 min. The fluorescence of fura2 was excitedalternatively at wavelengths of 357 nm and 380 nm by means ofa high-speed wavelength-switching device (Sutter, Lambda DG-4).Image analysis software (MetaFlour, Universal Imaging) allowedthe selection of several "regions of interest" within the fieldfrom which measurements are taken. To minimize bleaching, theintensity of excitation light and sampling frequency was keptas low as possible. In these experiments the intensity of excitationlight was measured as 18 µW out of the objective and measurementswere normally made once every 2s.

Calibration of Ca²⁺ signals

Free [Ca²⁺] was calculated from the ratio (R) of fluorescence at 357 and 380 nm, using the following equation: [Ca²⁺] = K_d × Sf × (R $-$ R_min)/(R_max $-$ R) (Grynkiewicz et al. 1985).The K_d was assumed to be 135 nM while values for R_min and R_maxwere all determined via calibration methods. Initially an in vitromethod was used to make estimate values. With this method, rectangularglass capillaries were filled with a high Ca²⁺ (fura2 + 10 mM Ca²⁺), a low Ca²⁺ (fura2 + 10 mM EGTA) and a control solution without fura2. Thefluorescence (F) at 380 nm excitation of the low Ca²⁺ solution was imaged and the exposure of the camera adjusted tomaximize the signal. These camera settings were then fixed andmeasurements were made with 380- and 357-nm excitation of thethree solutions. R_min = F357 in low Ca²⁺/F380 in low Ca²⁺; R_max = F357 in high Ca²⁺/F380 in high Ca²⁺; Sf = F380 in low Ca²⁺/F380 in high Ca²⁺. In addition, an in vivo calibration method was also used. Forthis, SCN cells were loaded via the patch pipette using solutionsinside the electrode similar to the normal internal solution butcontaining either no Ca²⁺ (20 mM EGTA) or 10 mM Ca²⁺ for R_min and R_max,respectively.

Immunocytochemistry

Animals were anesthetized then perfused transcardially with saline followed by 4% paraformaldehyde. Brains were immersed infixative overnight and then sectioned (30 µm thick) on a cryostat.Sections were blocked for endogenous peroxidase in 3% hydrogenperoxide plus 10% methanol in PBS. The tissue was then incubatedin a serum block solution of 3% normal goat serum and 0.3% TritonX in PBS for 1 h. Sections were incubated with the primary antibody(diluted with serum block solution) for 48 h at 4°C. The tissuewas then incubated for 1 h in biotinylated secondary antibody(1:200; diluted with 1% normal goat serum in PBS) at room temperature,followed by incubation in an avidin-biotin-peroxidase (1:50) complexat room temperature for 1 h at room temperature (Vector, Elitekit, Burlingame, CA). Sections were incubated in DAB (final dilution0.05%) plus hydrogen peroxide (final dilution 0.0015%) in PB for5-10 min. All previous steps (except serum block) were followedby rinses in PBS (3 × 5 min each). The tissue was mounted on slides,dehydrated, and cleared in alcohols and xylenes before cover-slipping.Polyclonal antibodies for GluR1 and GluR2/3 raised in rabbit werepurchased (Chemicon, Temecula, CA). A dilution series was performedfor both antibodies in tissue from 21-day-old animals with optimaldilution found to be 1:100.

Lighting conditions

To investigate possible diurnal variations in any of the measured values, animals were maintained on a daily light-dark cycleconsisting of 12 h of light followed by 12 h of dark. It is alreadywell established that cells in the SCN continue to show circadianoscillations when isolated from the animal in a brain slice preparation(e.g., Green and Gillette 1982). Accordingly, care must be takenas to the time in the daily cycle when the data are collected.Some of the animals were killed 30 min before the time that thelights would have turned off in the light-dark (LD) cycle. Thedata from these animals were collected between zeitgeber time(ZT) 14 and 18 and pooled to form a "night" group. For comparison,some of the animals were killed immediately after the lights cameon. The data from these animals were collected between ZT 2-6and pooled to form a "day"group.

Statistical analyses

Between group differences were evaluated using t-tests or Mann-Whitney rank sum tests when appropriate. Values were consideredsignificantly different if P < 0.05. All tests were performedusing SigmaStat (SPSS, Chicago, IL). In the text, values are shownas means ±SE.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Data were collected from a total of 1,272 cells from 104 animals. Every experimental and control group in this study containsdata from at least four animals. Each of these cells were determinedto be within the SCN by directly visualizing the cell's locationwith IR-DIC videomicroscopy before any data were collected. Inmost cases, the IR-DIC video images were sufficient to label acell as being in VL or DM regions of the SCN. In addition, someneurons were filled with biocytin through the patch electrodeand histologically processed. Slices containing these labeledcells were counter-stained with a Nissl stain to confirm the neuron'slocation within the SCN. All of the cells, which had been visuallydetermined to be in the dorsal (6/6) or ventral (6/6) regionsof the SCN, also demonstrated this localization with biocytinfills and Nisslstain.

sEPSCs recorded in VL and DM SCN

The mean frequency and the mean amplitude of sEPSCs recorded at a holding potential of $-$ 70 mV were 0.26 ± 0.04 (SE) events/s(n = 51; range: 1.29-0.01 events/s) and $-$ 17.5 ± 0.8 pA (range:37-7 pA), respectively. The time to rise and the time to decay(latency of the inward current peak from the baseline) were 1.5± 0.04 ms (range: 3.6-1.4 ms) and 2.2 ± 0.1 ms (range: 4.6-1 ms),respectively. These sEPSCs did not appear to be driven by actionpotentials as neither the amplitude nor the frequency of the currentswas significantly altered by the application of the sodium (Na⁺) channel blocker tetrodotoxin (TTX, n = 6). The sEPSCs were completelyabolished with AMPA/KA GluR antagonist 6-cyano-7-nitroquinoxaline-2,3-dione(CNQX, 25 µM, 5 of 5 neurons tested), indicating that they aremediated by AMPA/KA GluRs (Fig. 1, top). Interestingly, thesesEPSCs could be recorded from both VL and DM SCN, and there wereno significant differences between the currents recorded in eachregion. In the DM SCN, the mean frequency and amplitude of sEPSCswere 0.30 ± 0.07 events/s and $-$ 18.9 ± 1.4 pA (n = 23), respectively.Whereas in VL SCN, the mean frequency and amplitude of sEPSCswere 0.23 ± 0.03 events/s and $-$ 16.3 ± 1.0 pA (n = 28), respectively.Thus sEPSCs are not restricted to the retinal recipient VL regionbut instead are a general feature of cells within the SCN.

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Fig. 1. Example of spontaneous excitatory postsynaptic currents (sEPSCs) recorded in the day (top) in the suprachiasmatic nucleus (SCN). The sEPSCs were blocked by the bath application of CNQX (25 µM; middle). The sEPSCs were completely abolished with 6-cyano-7-nitroquinoxalene-2,3-dione (CNQX, 25 µM, 5 of 5 neurons tested), indicating that they are mediated by AMPA/kainate (KA) glutamate receptors (GluRs). Averaged sEPSCs are shown at an expanded time scale as indicated. Experiments were carried out in presence of bicuculline to prevent GABA_A-mediated inhibitory postsynaptic currents (IPSCs). Middle: histograms indicate the average sEPSC amplitude and frequency recorded in slices from the animal's day (n = 29) or night (n = 22). The amplitude and frequency did not vary between day and night. Bottom: sEPSC frequency as a function of time-of-day (ZT) the recordings were obtained. Although there was a trend for the frequency to be lower at night, this trend was not significant.

Spontaneous EPSCs frequency and amplitude did not vary between day and night in the SCN

The next experiment was designed to determine whether sEPSCs recorded in SCN neurons varied between day and night. These experimentswere performed with brain slices taken from animals during theirday and compared with data obtained from brain slices from animalsduring their night. Rats were killed 2-3 h after lights-on forthe "day" group or immediately before lights-off for the "night"group. Other than the time that the animals are killed, all conditionsbetween the day and night groups remained constant. The data werecollected between zeitgeber time (ZT) 4-8 and ZT 14-16 and werepooled to form "day" and "night" groups, respectively. There wereno significant differences in the amplitude, frequency, rise,or fall times of the sEPSCs (Fig. 1). During the day, sEPSCs hada mean amplitude of 16.5 ± 1.0 pA with a mean frequency of 0.27± 0.05 Hz (range: 1.2-0.05 Hz; n = 29). Similarly, during thenight, the mean amplitude of the sEPSCs was found to be 18.8 ±1.3 pA with a frequency of 0.25 ± 0.06 Hz (range: 0.65-0.01 Hz;n = 22). These data indicate that the presynaptic release as wellas postsynaptic sensitivity to glutamate is fairly constant throughoutthe dailycycle.

AMPA-evoked currents recorded in SCN neurons

Whole cell patch-clamp recording techniques were used to directly measure currents evoked by a submaximal dose of AMPA (25µM) in SCN neurons. In these experiments, the current requiredto hold the cell's membrane potential at $-$ 70 mV was monitored.In addition, the voltage dependence of the AMPA-evoked currentswas measured by moving the cell through either a ramp of voltages(from $-$ 70 to 40 then back to $-$ 90 mV) or a series of voltage-steps(from $-$ 120 to 40 mV) before, during, and after treatment withAMPA in the bath. Because activation of voltage-dependent Na⁺, Ca²⁺, and K⁺ currents could distort measurement of AMPA-evoked currents, cesium(Cs⁺, 125 mM) was used in the patch pipette while tetraethyl-ammoniumchloride (TEA, 10 mM), cadmium (Cd²⁺, 25 µM), and TTX (1 µM) were in the bath. Figure 2, top, showsthe current-voltage relationship of an AMPA current recorded usingthis protocol. Most SCN neurons (91%; 78 of 86 neurons tested)exhibited AMPA-evoked currents. These inward currents exhibiteda linear voltage dependency with reversal potentials around 0mV. AMPA-evoked currents were eliminated by the addition of theAMPA/KA GluR antagonist CNQX (25 µM; n = 16).

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Fig. 2. AMPA currents in SCN neurons. Whole cell patch-clamp recording techniques were used to directly measure currents evoked by AMPA in SCN neurons. The voltage dependence of the AMPA-evoked currents was measured by moving the membrane potential of the cell through a series of voltage steps before, during, and after treatment with AMPA (25 µM) in the bath. These experiments were performed in the presence of cadmium (Cd²⁺, 25 µM), and TTX (1 µM) in the bath. Top: an AMPA response recorded using this protocol. AMPA currents blocked by the application of CNQX. Bottom: histograms summarizing AMPA evoked currents in the SCN. These currents did not vary between day (n = 88) and night (n = 34) and were blocked by CNQX (n = 16). There was no difference in the magnitude of the AMPA evoked currents recorded in the dorsomedial (DM, n = 66) and ventrolateral (VL, n = 16) SCN regions.

AMPA-evoked currents could be recorded from both VL and DM SCN, and there were no significant differences between the currentsrecorded in each region. In the DM SCN, the bath application ofAMPA (25 µM) produced a normalized peak current of $-$ 4.1 ± 0.5pA/pF (range: 0.5 to $-$ 21.6 pA/pF; n = 66) while in the VL SCNthe same treatment produced a peak current of $-$ 3.2 ± 0.7 pA/pF(range: 1.2 to $-$ 9.9 pA/pF; n = 16). The next experiment was designedto determine whether these inward currents evoked by bath applicationof AMPA varied between day and night in SCN neurons. As describedin the preceding text, these experiments were performed with brainslices taken from animals during their day and compared with dataobtained from brain slices from animals during their night. Underthese conditions, there was no day/night difference in AMPA-evokedinward currents. During the day, AMPA (25 µM, 120-300 s) producedan average peak inward current of $-$ 3.7 ± 0.5 pA/pF (range: 0.8to $-$ 16.2 pA/pF; n = 52), whereas during the night, this same treatmentproduced an average peak current of $-$ 3.6 ± 0.6 pA/pF (0.3 to $-$ 14.8pA/pF; n = 33). These data provide additional support for theconclusions that AMPA-sensitive neurons are found throughout theSCN and that the sensitivity of these cells to AMPA stimulationdoes not vary with time ofday.

AMPA regulation of Ca²⁺ transients in SCN neurons

A bulk loading procedure was used to load cells with a membrane-permeable form of the Ca²⁺ indicator dye fura2. This procedure loads many cells in SCN slicesfrom young animals (10- to 15-day-old rats were used in the currentstudy). Cells that exhibited uneven loading due to dye sequestrationwere not included in the data set. Small cell types includingglia were easily identified and were not included in the dataset. Bath application of AMPA (1-100 µM, 60 s, day) caused Ca²⁺ transients in SCN cells in the brain slice (Fig. 3). For example,AMPA (25 µM, 60 s) produced an average increase in Ca²⁺ of 45 ± 1% or increased estimated free [Ca²⁺ ]_i 20.6 ± 2 nM (range 144 to $-$ 12 nM; n = 1027). This responsewas widespread within the SCN with 93% of cells (960/1027) examinedshowing a Ca²⁺ increase of 5% or greater. AMPA-evoked Ca²⁺ transients could be recorded from both VL and DM SCN, and therewere no significant differences between the responses recordedin each region. In the DM SCN, the bath application of AMPA (25µM) produced a peak Ca²⁺ increase of 43 ± 3% (mean: 20 ± 1 nM; range: 161 to $-$ 3 nM; n= 300). In the VL SCN, the same treatment produced a peak Ca²⁺ increase of 47 ± 5% (mean: 21 ± 2 nM; range: 125 to $-$ 0.5 nM;n = 139). These AMPA-induced Ca²⁺ transients were blocked by treatment with the AMPA/KA GluR antagonistCNQX (AMPA + CNQX: 1.3 ± 0.2%, n = 50).

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Fig. 3. Examples of Ca²⁺ transients measured from SCN cells in a brain slice loaded with the Ca²⁺ indicator dye fura2. Top: SCN cells show an increase in Ca²⁺ concentration in response to bath application of AMPA (25 µM, 60 s). Each line represents data collected from an individual cell. These data were collected in the presence of TTX that was included to block voltage-sensitive Na⁺ currents. Middle: AMPA-induced Ca²⁺ transients were inhibited by the presence of the AMPA/KA GluR antagonist CNQX (25 µM). Data collected from single SCN slice from a 14-day-old rat. Bottom: histograms summarizing AMPA regulation of Ca²⁺ levels in the SCN. Bath application of AMPA (25 µM, 60 s) produced Ca²⁺ transients in most cells (93%) within the SCN (P < 0.001, n = 1027). These AMPA-induced Ca²⁺ transients were blocked by treatment with the AMPA/KA GluR antagonist CNQX (25 µM, P < 0.001, n = 50) and by treatment with a blocker of high-voltage activating calcium channels (Cd²⁺, P < 0.001, n = 119). Finally, there was no difference in the magnitude of the AMPA responses recorded in the DM and VL SCN regions.

Neuronal Ca²⁺ influx can be mediated directly by Ca²⁺-permeable AMPA receptors and indirectly by depolarization-induced activationof voltage-gated Ca²⁺ channels. In addition, in some preparations, reverse Na⁺/Ca²⁺ exchange contributes to glutamate-induced Ca²⁺ influx (e.g., Hoyt et al. 1997; Schroeder et al. 1999). To investigatethe extracellular source of Ca²⁺ influx, we examined the effect of blocking voltage-gated Ca²⁺ channels with Cd²⁺ and the reverse mode of the Na⁺/Ca²⁺ exchange with the selective inhibitor 2-[2-[4-(4-nitrobenzyloxy)phenyl]ethyl]isothiourea(KB-R7943) on the AMPA-induced Ca²⁺ transients. By itself, KB-R7943 (10-25 µM) did not have any effecton resting Ca²⁺ (0.9 ± 0.4%). When AMPA was applied in the presence of KB-R7943,there was no significant effect on the magnitude of the AMPA-inducedCa²⁺ transients. For example, AMPA (25 µM) in the presence of KB-R7943increased estimated free [Ca²⁺ ]_i by 29.9 nM (range: 168 to $-$ 7 nM, n = 88), whereas the samecells treated with AMPA alone increased Ca²⁺ by 28.9 nM (range: 155 to $-$ 10 nM, n = 88). In contrast, the applicationof the Ca²⁺ channel blocker Cd²⁺ (25 µM) produced a major reduction in the magnitude of the AMPA-evokedresponse (AMPA alone: 45 ± 1%, n = 1027; Cd²⁺ + AMPA: 4 ± 1%, n = 119; Fig. 3). In the presence of Cd²⁺, bath application of AMPA (25 µM) still produced significantCa²⁺ transients (P < 0.05). However, these responses were restrictedto only a few cells (10 of 119 SCN cells exhibited a more than5% increase in Ca²⁺) with most SCN neurons not exhibiting a detectable Ca²⁺ transient in the presence of Cd²⁺. Overall, the majority of the AMPA-induced Ca²⁺ influx is sensitive to Cd²⁺, and it can be assumed to result from the activation of voltage-sensitiveCa²⁺ channels byAMPA.

Circadian rhythm in the magnitude of AMPA-induced Ca²⁺ transients

The next experiment was designed to determine whether Ca²⁺ transients evoked by bath application of AMPA in SCN neurons variedbetween day and night. As described in the preceding text, theseexperiments were performed with brain slices taken from animalsduring their day and compared with data obtained from brain slicesfrom animals during their night. There was a daily rhythm in Ca²⁺ transients with peak AMPA responses significantly higher duringthe night than during the day (P < 0.001; Fig. 4). During theday, bath application of AMPA (25 µM) produced Ca²⁺ transients with an average peak value 31 ± 26% above baselinehaving increased estimated [Ca²⁺ ]_i 14 ± 0.7 nM (range: 78 to $-$ 12 nM; n = 418). The same treatmentduring the night, caused an average increase of 55 ± 2% havingincreased estimated [Ca²⁺ ]_i 25 ± 0.8 nM (range: 144 to $-$ 1 nM; n = 609). An examinationof the distribution of the Ca²⁺ transients (Fig. 4, bottom) indicates that the larger mean responsesat night was due to a combination of more cells responding toAMPA as well as a larger average response per cell. For example,if analysis is limited to those cells that showed at least a 10%increase in Ca²⁺, only about half of the cells tested (212/419) reached this thresholdcompared with 80% at night (473/609). In these responding cells,a diurnal rhythm is still present with AMPA causing an averageof 40% change during the day and a 61% change at night. In contrast,treatment with a solution high in potassium (K⁺, 50 mM, 15 s) produced Ca²⁺ transients that were not different from day to night (day: 101± 7 nM increase, n = 83; night: 102 ± 6 nM increase, n = 83).

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Fig. 4. Diurnal rhythm in AMPA-evoked Ca²⁺ transients in SCN cells. In these experiments, AMPA-evoked Ca²⁺ transients were measured in SCN neurons in brain slices from animals during their day and compared with data obtained from brain slices from animals during their night. Slices were prepared at either ZT 0 for the day group or ZT 11.5 for the night group. Each cell was sampled only once. Top: histogram showing average magnitude of AMPA-evoked Ca²⁺ transients measured in SCN neurons in day or night. AMPA-evoked Ca²⁺ transients peaked during night (P < 0.001). Bottom: distribution of responses in day and night. The larger average Ca²⁺ transients at night was due to a combination of more cells responding to AMPA as well as a larger average response per cell.

Tonic activation of AMPA/KA GluRs may contribute to resting Ca²⁺ concentration and tonic firing rate of some SCN neurons

The next experiment was designed to determine if AMPA-mediated currents tonically influence the firing rate of SCN neurons(Fig. 5, top). To address this question, the firing rate of SCNneurons was monitored using the cell-attached recording technique.With this configuration, the patch electrode forms a giga-ohmseal but the membrane is not ruptured. The frequency of spontaneousaction potential generation was monitored before and after applicationof the AMPA/KA GluR antagonist CNQX. Again, CNQX did not havea significant effect (P > 0.05) on frequency of firing of theSCN neurons sampled (n = 16). However, a subset of SCN neurons(6/16 or 37% of cells examined) did show a marked decrease infiring rate after application of CNQX. These six cells exhibitan average decrease of 49%. To examine the possibility of tonicglutamatergic contribution to the resting Ca²⁺ concentration, SCN cells were treated with CNQX (25 µM) aloneduring the day (Fig. 5, bottom). Overall, there was no significanteffect (P > 0.05) of CNQX on resting Ca²⁺ concentration; however, many cells (28/73 or 38% of cells examined)did show a reduction of $>=$ 5%. On these cells, application of CNQXproduced a modest reduction of 8 ± 0.4%. Together, these resultsraise the possibility that tonic excitatory drive may influencethe activity of at least some cells within the SCN.

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Fig. 5. Application of AMPA/KA GluR antagonist CNQX decreases the firing rate and resting calcium levels of a subset of SCN neurons. Top: example of SCN neuron before and after treatment with CNQX (25 µM). The firing rate of this SCN neuron was monitored using the cell-attached recording technique. This treatment with CNQX did not have a significant effect (P > 0.05) on frequency of firing of the SCN neurons sampled (n = 16). However, as illustrated in this example, a subset of SCN neurons (6/16 or 37% of cells examined) did show a marked decrease in firing rate after application of CNQX. Bottom: SCN cell showed a decrease in estimated Ca²⁺ concentration in response to bath application of CNQX (25 µM, 60 s). Overall, there was no significant effect (P > 0.05) of CNQX on resting Ca²⁺; however, many cells (28/73 or 38% of cells examined) did show a reduction of $>=$ 5%.

AMPA receptors are expressed in SCN in both VL and DM subdivisions

To examine the pattern of expression of receptors likely involved in mediating the AMPA-evoked currents, an antibody raisedagainst an AMPA preferring GluR subunit, GluR1, was utilized (Fig.6). Rats (age 18-21 days) were perfused at ZT 2-4, and sectionscontaining the SCN were examined immunohistochemically. The GluR1immunoreactivity was clear in the SCN but more diffuse comparedwith staining in cortex or hippocampus. Most cell bodies werenot clearly stained and those that were stained showed "halo"of immunoreactivity around the soma that may represent stainingof cell membrane but not cytoplasm. Staining was most robust intwo regions of the SCN including the ventral lateral portionsas well as a dorsal region of SCN near the 3rd ventricle. Thisdorsal region contained the most labeled cell bodies, whereasthe staining in the ventral region was mostly limited to the neuropil.There was a core region in the center of the SCN that did notexhibit any clear staining. This general pattern was seen throughoutthe rostral to caudal extent of the SCN. To look for possibleday-night differences in immunoreactivity, staining in tissuecollected from ZT 2-4 was compared with those collected betweenZT 13-15. Qualitatively, there were no obvious differences betweenthese two time points.

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Fig. 6. Photomicrographs showing immunoreactivity for GluR1 and GluR2/3 in the suprachiasmatic nucleus. 3rdV, third ventricle; OC, optic chiasm. Left panel: The GluR1 immunoreactivity was most robust in 2 regions of the SCN including the ventral lateral portions as well as a dorsal region of SCN near the 3rd ventricle. This dorsal region contained the most labeled cell bodies, whereas the staining in the ventral region was mostly limited to the neuropil. There was a core region in the center of the SCN that did not exhibit any clear staining. This general pattern was seen throughout the rostral to caudal extent of the SCN. Middle panel: GluR2/3 immunoreactivity was seen on cell bodies and in the neuropil throughout the SCN. The staining was most robust in the ventral region of the SCN near the optic chiasm. This was particularly true in the more rostral regions of the SCN as the staining became more diffuse in the caudal regions. Right panel: Higher power view of GluR1-IR. Most cell bodies were not clearly stained and those that were stained showed "halo" of immunoreactivity around the soma that may represent staining of cell membrane but not cytoplasm. Tissue collected from rats (age 18-21 days) that were perfused between ZT 4-6.

An antibody raised against other AMPA preferring GluR subunits, GluR2/3, was also used (Fig. 6). The GluR2/3 immunolabelingin the SCN was quite different that the GluR1. In general GluR2/3immunoreactivity was seen on cell bodies and in the neuropil throughoutthe SCN. The staining was most robust in the ventral region ofthe SCN near the optic chiasm. This was particularly true in themore rostral regions of the SCN as the staining became more diffusein the caudal regions. Similar to the GluR1 immunoreactivity,most cell bodies stained showed "halo" of immunoreactivity aroundthe soma. Qualitatively, the staining in tissue collected fromZT 2-4 was similar to that observed from tissue collected betweenZT 13-15. Overall, the immunocytochemistry analysis clearly indicatesthe presence of AMPA preferring GluR subunits within the SCN.These receptors are rather broadly expressed and certainly notrestricted to the retino-recipient ventral SCNregions.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Summary

In the present study, whole cell patch-clamp techniques were used to measure sEPSCs from SCN neurons. These currents werewidespread in the SCN and not just restricted to the retino-recipientregion. The sEPSC frequency and amplitude did not vary with thedaily cycle. Similarly, currents evoked by the exogenous applicationof AMPA onto SCN neurons were widespread within the SCN and didnot exhibit a diurnal rhythm in their magnitude. Imaging techniquesand the indicator dye fura2 were utilized to estimate AMPA-inducedCa²⁺ changes in SCN cells. The resulting data indicate that AMPA-evokedCa²⁺ transients were widespread in the SCN and that there was a dailyrhythm in the magnitude of AMPA-induced Ca²⁺ transients that peaked during the night. By itself, blockingAMPA/KA GluRs with CNQX decreased the spontaneous firing rateand resting Ca²⁺ of some SCN neurons, suggesting that tonic glutamatergic excitationmay influence electrical activity of at least a subset of SCNneurons. Finally, immunohistochemical techniques were used todemonstrate the expression of the AMPA-preferring GluR subunitsGluR1 and GluR2/3 within the SCN. Overall, our data demonstratethat glutamatergic synaptic transmission mediated by AMPA/KA GluRsis a general feature of SCN neurons. AMPA-evoked Ca²⁺ responses recorded in SCN neurons expressed a diurnal rhythm,presumably regulated by the circadian timing loop. These observations,coupled with those of previous studies, suggest that glutamatergicsynaptic transmission plays an important role in synaptic circuitrythroughout theSCN.

Spontaneous EPSCs and AMPA-evoked responses are widespread within the SCN

Anatomical studies support the subdivision of the rat SCN into at least two subdivisions (Moore and Silver 1998; van den Pol1980). There is a dorsomedial division, or shell, with small cells(10-12 µm in diameter) that typically express vasopressin (VP).These cells are tightly packed with cell bodies in close contactwith their neighbors (somato-somatic appositions). This regionreceives inputs mainly from the cortex, basal forebrain, and otherhypothalamic regions while sending projections that largely targetthe dorsomedial hypothalamus (DMH) and medial subparaventricularzone (sPVZ) (Leak et al. 1999; Moga and Moore 1997). The shellsits atop a ventrolateral division, or core, which contains cellsexpressing vasoactive intestinal peptide (VIP) or gastrin releasingpeptide (GRP). These neurons (12-15 µm in diameter) are foundat a lower density, and their cell bodies are in close contactwith glia. Both retinal and thalamic input as well as serotonergicinputs from the raphe mainly project to cells in the core. Neuronsfrom this region project predominantly to the lateral sPVZ. Giventhat the RHT input to the SCN is known to be glutamatergic andthese retinal afferents project to the VIP-containing ventrolateralregions (Card et al. 1981; Tanaka et al. 1993; van den Pol andTsujimoto 1985), we expected to see a more robust AMPA currentsin the retino-recipient, ventrolateral region of the SCN. However,contrary to our expectations, most cells in the SCN show an excitatoryresponse to AMPA in the presence of TTX. For example, in the presentedelectrophysiological measurements, 91% of cells sampled exhibitedan AMPA-induced inward current and 51% expressed sEPSCs. Similarly, $<=$ 93% of fura2-loaded cells showed a Ca²⁺ increase in response to bath application of AMPA. Although peptideexpression was not characterized in these cells, video microscopywas used to visually place neurons within general regions of theSCN. Of 86 cells from which AMPA currents were recorded, 66 cellswere visually judged to be in the DM SCN and 16 in the VL SCNregions (a few could not be categorized). There were no significantdifferences between the currents recorded from one region or theother, and certainly SCN neurons in both the VL and DM subdivisionsrespond to AMPA. Similar observations were made with regard tosEPSPs and AMPA-evoked Ca²⁺ transients (see RESULTS). This physiological data indicatingthat most cells within the SCN are capable of being excited byAMPA is consistent with our immunocytochemical data suggestingthat AMPA preferring GluRs are widely distributed within thisnucleus (also see Gannon and Rea 1993, 1994; Mikkelsen et al.1995; Stamp et al. 1997; van den Pol et al. 1994).

As described previously, the best-known glutamatergic afferents to the SCN are the terminals of the retinal ganglion cellsthat make up the RHT. These excitatory inputs are restricted tothe VL-SCN. The presented data indicate that sEPSCs and AMPA-evokedresponses were a general feature of SCN neurons including thosein the DM-SCN. This raises an obvious question as to what is thesource of these glutamatergic terminals. Retrograde axonal transportof the select neuronal tracer [³H]-aspartate was used to demonstrate possible sources of excitatoryinput to the SCN in the albino rat (Moga and Moore 1997). Followinginjection of [³H]-aspartate into the SCN, neurons were retrogradely labeled inthe infralimbic cortex, the lateral septal nucleus, the paraventricularthalamic nucleus, and a variety of hypothalamic nuclei. So besidesthe retina, it appears that there may be a number of regions thatsend excitatory projections to the SCN. In addition, though anatomicalnot well characterized, there is a growing body of evidence thatsuggests that there are glutamatergic cells within the SCN. Thebest evidence comes from studies of the pathways by which SCNneurons regulate other hypothalamic nuclei. Stimulation of theSCN evokes short-latency inhibition and excitation of neuronsin the ventromedial preoptic area (Sun et al. 2000), the paraventricularnucleus (Cui et al. 2001; also see Csáki et al. 2000), and thearcuate nucleus (Saeb-Parsy et al. 2000). Many of these evokedresponses to SCN stimulation had short latencies (<20 ms) andwere sensitive to GluR blockers, suggesting that they were mediatedby monosynaptic, excitatory connections. As with any of this typeof study, it is difficult to rule out that the electrical stimulationactivated fibers traveling through the SCN region and not originatingin this nucleus. Nevertheless, this body of work certainly suggeststhat glutamatergic projection neurons may be present within theSCN. Such neurons could easily be involved in communication betweenSCN regions and be the source of some of the glutamatergic inputthat we observed throughout theSCN.

Diurnal rhythm in AMPA-evoked calcium transients

The Ca²⁺ influx associated with ligand-gated receptor activation is thought to produce a brief, high-concentration (>100 µM),localized gradients of Ca²⁺ near open channels (e.g., Neher 1998; Yuste et al. 2000). Thesegradients are rapidly dissipated by diffusion and binding to buffersand would not be seen by slow, volume-averaged measurements usedin the present study. However, these rapid influxes would contributeto the Ca²⁺ load in a slower and diffuse Ca²⁺ pool that is referred to as residual Ca²⁺ (e.g., Tank et al. 1995). It is this pool that we measured withthe high-affinity Ca²⁺ indicator fura2. These responses are both slower and of loweramplitude than those directly associated with the direct openingof a Ca²⁺ permeable ion channel. It may well be that this Ca²⁺ pool in the soma is more directly related to the role of Ca²⁺ as a regulator of gene expression than the faster transientsrecorded from the dendrites. The free [Ca²⁺ ]_i in the cytoplasm results from the highly regulated balancebetween the rates of Ca²⁺ influx and removal/buffering. Although the present study didnot explore the possibility of circadian regulation of Ca²⁺ removal/buffering mechanisms, there is good reason to suspectthat the rhythm in AMPA-induced increases in Ca²⁺ concentration can be accounted for by a daily rhythm in evokedCa²⁺ influx. Our experimental data indicate that voltage-gated currentsare the main contributors to the Ca²⁺ transients (see Fig. 3). AMPA application during the night increasedCa²⁺ levels by 55%, whereas in the presence of Ca²⁺ channel blocker Cd²⁺, the same treatment increased Ca²⁺ by 4%. This suggests that the Cd²⁺-sensitive currents are responsible for the vast majority of theAMPA-evoked Ca²⁺ transients. Nevertheless, when these currents were blocked withCd²⁺, there were still some cells in which an AMPA-evoked Ca²⁺ transient was present. AMPA GluRs that lack the GluR2 subunitare capable of directly fluxing Ca²⁺ (e.g., Geiger et al. 1995; Hollmann et al. 1991). Two observationsfrom our data suggest that these Ca²⁺ permeable AMPA receptor types may be present in the SCN. First,immunocytochemical analysis indicated that there was a clear mismatchbetween expression patterns of GluR1 and GluR2/3. This suggeststhat some AMPA GluRs may be constructed without the GluR2 subunitespecially in the dorsal SCN region. We did not observe any significantregional variation in current density. However, the loss of theGluR2 subunit could have opposing effects on the AMPA-evoked currentdensity. The absence of GluR2 should decrease the AMPA-evokedcurrent at resting membrane potentials (Washburn et al. 1997),whereas single-channel conductance can be dramatically increasedby the absence of GluR2 (Swanson et al. 1997). The balance ofthese opposing effects determines the overall effect changes inGluR2 abundance on GluR properties. Second, though most SCN neuronsdid not exhibit an AMPA response in the presence of Cd²⁺, those that did respond (8% of cells tested) exhibited Ca²⁺ transients that were indistinguishable from those measured undernormal conditions (28 ± 2 vs. 25 ± 0.8 nM). These cells were locatedin the DM-SCN and suggest that there may well be a subpopulationof SCN neurons that express Ca²⁺ fluxing AMPAchannels.

The simplest mechanistic explanation for the rhythm in Ca²⁺ transients in the SCN is that the rhythm is a direct result of adaily variation in the magnitude of the AMPA-evoked current. However,in this case, data from the present study indicate that AMPA currentsdo not vary from day to night. There are at least three possiblemechanisms that could explain the rhythm. First, the AMPA GluRsubunit composition may change from day to night such that thereceptor is more permeable to Ca²⁺ during the night. In hippocampal neurons, synaptic activity canlead to the rapid rearrangement of AMPA GluR subunit compositionat synapses (Liu and Cull-Candy 2000). Furthermore, in the SCN,a circadian rhythm of AMPA preferring GluR2/3 immunoreactivityhas been reported with peak expression during the day (Chambille1999). This observation is of particular interest because thepresence of GluR2 in an AMPA receptor greatly reduces its Ca²⁺ permeability (Geiger et al. 1995: Hollmann et al. 1991). Thereforethe higher GluR2/3 immunoreactivity during the day could be reflectedin less Ca²⁺-permeable AMPA GluRs and lower amplitude AMPA-induced Ca²⁺ transients. Second, there is substantial evidence for multipletypes of voltage-dependent Ca²⁺ channels in other regions of the CNS. These include low-voltageactivating Ca²⁺ channels (LVA) and high-voltage activating Ca²⁺ channels (HVA) that are generally subdivided into L, N, P, R,and Q-types. Although not extensively studied, there is evidencefor both HVA and LVA Ca²⁺ currents in SCN neurons (Akasu et al. 1993; Huang 1993). We havefound that Cd²⁺ (25 µM) blocks the HVA but not the LVA Ca²⁺ currents in SCN neurons (Colwell unpublished data). Thereforea second possible mechanism that could explain the rhythm in AMPA-evokedresponse would be a rhythm in HVA Ca²⁺ currents. Other studies have reported evidence for diurnal rhythmsin membrane properties of SCN neurons (de Jeu et al. 1998; Jianget al. 1997; Schaap et al. 1999). Third, it may well be that therhythm in AMPA evoked responses is due to a regulation of Ca²⁺-induced release of Ca²⁺ from internal stores. Previous studies have implicated ryanodinereceptors and intracellular calcium stores in mediating lightand glutamate induced phase delays of the mammalian circadianclock (Ding et al. 1998; Hamada et al. 1999). These three possibilitiesare not mutually exclusive and can be experimentallyresolved.

Functional importance

One of the fundamental features of circadian oscillators is that their response to environmental stimulation varies dependingon the phase of the daily cycle when the stimuli are applied.For example, the same light treatment, which can produce phaseshifts of the oscillator when applied during the subjective night,has no effect when applied during the subjective day. This periodicsensitivity to photic stimulation is a central feature of entrainment,i.e., the process by which circadian oscillators are synchronizedto the environment. Despite its importance, the cellular and molecularmechanisms behind this differential sensitivity are just beginningto be explored in mammals. There is some evidence that this regulationmay occur at the level of the SCN neurons. Two previous studieshave demonstrated a daily rhythm in the response of SCN cellsto photic and electrical stimulation of the RHT (Cui and Dyball1996; Meijer et al. 1998). In addition, electrical stimulationof the RHT causes the same daily pattern of light-like phase shiftsof the circadian system both in vivo (de Vries et al. 1994) andin vitro (Shibata and Moore 1993), i.e., phase shifts during thenight but not during the day. Glutamate is the transmitter atthe retinal input to the SCN and exogenous application of GluRagonists cause light-like phase shifts of the circadian rhythmin neuronal activity in the SCN in vitro (Ding et al. 1994; Shibataet al. 1994; Shirakawa and Moore 1994). In addition, two recentstudies demonstrate that there are daily rhythms in both synapticevoked, NMDA-induced Ca²⁺ transients and NMDA currents recorded from SCN neurons in a brainslice preparation (Colwell 2001; Pennartz et al. 2001).

In many synapses, AMPA and NMDA GluRs work in concert with the AMPA GluRs that are responsible for the initial depolarizationof the postsynaptic membrane. This depolarization is requiredbefore the neuron's membrane potential moves into the voltagerange at which the NMDA GluR can become activated. A recent studyindicates that in the SCN the relative contribution of the NMDAGluR to the postsynaptic response is larger during the night thanduring the day (Pennartz et al. 2001). The active regulation ofAMPA GluR can play a major role in determining the contributionof NMDA GluR to the postsynaptic response. For example, in somesynapses, it appears that NMDA GluRs, but not AMPA GluRs are expressed.This makes this connection electrophysiologically "silent" asthe postsynaptic cell would not normally be in a voltage rangein which the NMDA receptors would be active. However, in responseto appropriate patterns of stimulation, the AMPA GluRs can berapidly inserted into the postsynaptic membrane (e.g., Durandet al. 1996; Isaac et al. 1995; Luthi et al. 1999). We thoughtthat the rapid regulation of AMPA receptors could be a logicalmechanism to gate the light input to the circadian system. However,our data do not support such a hypothesis (also see Pennartz etal. 2001).

Even if the current evoked by AMPA GluRs is not gated by the circadian system, these receptors are still likely to play criticalrole in transduction of environmental information to the SCN.First, we have found that AMPA/KA GluR mediate most excitatorysynaptic transmission in the SCN (also see Cahill and Menaker1989; Cui and Dyball 1996; de Vries et al. 1994; Jiang et al.1997; Kim and Dudek 1991) and are a general feature of SCN neurons.Both spontaneous and evoked AMPA/KA-mediated currents were justas prevalent in the DM-SCN as in the VL-SCN. These GluRs are likelyto function as permissive partners to the NMDA-evoked responseas they are required to depolarize the cell and remove the magnesiumblockade of the NMDA GluR. Support for this model of coordinationbetween NMDA and AMPA/KA GluRs comes from studies of light andglutamate regulation of gene expression in the SCN (e.g., Abeet al. 1992; Guido et al. 1999; Schurov et al. 1999). For example,in cultured SCN cells, neither AMPA nor NMDA alone causes muchchange in CREB phosphorylation while application of the two agoniststogether caused a robust induction of pCREB immunoreactivity (Schurovet al. 1999). By itself, application of AMPA causes phase shiftsof neural activity rhythms recorded from SCN brain slices duringthe night and prevent 5HT-evoked phase shifts during the day (e.g.,Prosser 2001; Shibata et al. 1994). Finally, administration ofAMPA/KA GluR blockers (CNQX, DNQX) prevents the effects of lighton the circadian rhythm of wheel-running activity (Colwell andMenaker 1992; Rea et al. 1993). These observations lead us toconclude that AMPA/KA receptors are likely to play a broad rolein transduction of signals onto theSCN.

	ACKNOWLEDGMENTS

This work was supported by Whitehall Foundation Grant F98P15 and National Institutes of Health Grants HL-64582 and MH-59186.

	FOOTNOTES

^* The first two authors contributed equally to thisstudy.

Address for reprint requests: C. S. Colwell, Mental Retardation Res. Ctr., University of California, 760 Westwood Plaza, LosAngeles, CA 90024-1759 ( E-mail: ccolwell{at}mednet.ucla.edu).

Received 14 January 2002; accepted in final form 27 March 2002.

	REFERENCES

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Abe H, Rusak B, and Robertson HA. NMDA and non-NMDA antagonists inhibit photic induction of Fos protein in the hamster suprachiasmatic nucleus. Brain Res Bull 28: 831-833, 1992[Web of Science][Medline].
Akasu T, Shoji S, and Hasuo H. Inward rectifier and low-threshold calcium currents contribute to the spontaneous firing mechanism in neurons of the rat suprachiasmatic nucleus. Pflügers Arch 425: 109-116, 1993[Web of Science][Medline].
Balsalobre A, Damiola F, and Schibler U. A serum shock induces circadian gene expression in mammalian tissue culture cells. Cell 93: 929-937, 1998[Web of Science][Medline].
Cahill GM, and Menaker M. Effects of excitatory amino acid receptor antagonists and agonists on suprachiasmatic nucleus responses to retinohypothalamic tract volleys. Brain Res 479: 76-82, 1989[Web of Science][Medline].
Card JP, Brecha N, Karten HJ, and Moore RY. Immunocytochemical localization of vasoactive intestinal peptide-containing cells and processes in the suprachiasmatic nucleus of the rat. J Neurosci 1: 1289-1303, 1981[Abstract].
Chambille I. Circadian rhythm of AMPA receptor GluR2/3 subunit-immunoreactivity in the suprachiasmatic nuclei of Syrian hamster and effect of a light-dark cycle. Brain Res 833: 27-38, 1999[Web of Science][Medline].
Colwell CS. NMDA-evoked calcium transients and currents in the suprachiasmatic nucleus: gating by the circadian system. Eur J Neurosci 13: 1420-1428, 2001[Web of Science][Medline].
Colwell CS, Cepeda C, Crawford C, and Levine MS. Postnatal development of NMDA evoked responses in the neostriatum. J Dev Neurobiol 20: 154-163, 1998.
Colwell CS, and Menaker M. 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, 1992[Abstract/Free Full Text].
Colwell CS, and Menaker M. Excitatory Amino Acids: Their Role in Neuroendocrine Function., New York: CRC, 1996, p. 223-252.
Csáki A, Kocsis K, Halász B, and Kiss J. Localization of glutamatergic/aspartatergic neurons projecting to the hypothalamic paraventricular nucleus studied by retrograde transport of [³H]-aspartate autoradiography. Neuroscience 101: 637-655, 2000[Web of Science][Medline].
Cui LN, Coderre E, and Renaud L P. Glutamate and GABA mediate suprachiasmatic nucleus inputs to spinal-projecting paraventricular neurons. Am J Physiol Regulatory Integrative Comp Physiol 281: R1283-1289, 2001[Abstract/Free Full Text].
Cui LN, and Dyball REJ. Synaptic input from the retina to the suprachiasmatic nucleus changes with the light-dark cycle in the Syrian hamster. J Physiol (Lond) 497: 483-493, 1996[Abstract/Free Full Text].
de Jeu M, Hermes M, and Pennartz C. Circadian modulation of membrane properties in slices of rat suprachiasmatic nucleus. Neuroreport 9: 3725-3729, 1998[Web of Science][Medline].
de Vries MJ, Treep JA, de Pauw ESD, and Meijer JH. The effects of electrical stimulation of the optic nerves and anterior optic chiasm on the circadian activity rhythm of the Syrian hamster: involvement of excitatory amino acids. Brain Res 642: 206-212, 1994[Web of Science][Medline].
Ding JM, Buchanan GF, Tischkau SA, Chen D, Kuriashkina L, Faiman LE, Alster JM, McPherson PS, Campbell KP, and Gillette MU. A neuronal ryanodine receptor mediates light-induced phase delays of the circadian clock. Nature 394: 381-384, 1998[Medline].
Ding JM, Chen D, Iber ET, Faiman LE, Rea MA, and Gillette MU. Resetting the biological clock: mediation of nocturnal circadian shifts by glutamate and NO. Science 266: 1713-1717, 1994[Abstract/Free Full Text].
Durand GM, Kovalchuk Y, and Konnerth A. Long-term potentiation and functional synapse induction in developing hippocampus. Nature 381: 71-75, 1996[Medline].
Ebling FJP. The role of glutamate in the photic regulation of the suprachiasmatic nucleus. Prog Neurobiol 50: 109-132, 1996[Web of Science][Medline].
Gannon RL, and Rea MA. Glutamate receptor immunoreactivity in the rat suprachiasmatic nucleus. Brain Res 622: 337-342, 1993[Web of Science][Medline].
Gannon RL, and Rea MA. In situ hybridization of antisence mRNA oligonucleotides for AMPA, NMDA and metabotropic glutamate receptor subtypes in the rat suprachiasmatic nucleus at different phases of the circadian cycle. Mol Brain Res 23: 338-344, 1994[Medline].
Geiger JR, Melcher T, Koh DS, Sakmann B, Seeburg PH, Jonas P, and Monyer H. Relative abundance of subunit mRNAs determines gating and Ca²⁺ permeability of AMPA receptors in principal neurons and interneurons in rat CNS. Neuron 15: 193-204, 1995[Web of Science][Medline].
Gillette MU. Cellular and biochemical mechanisms underlying circadian rhythms in vertebrates. Curr Opin Neurobiol 7: 797-804, 1997[Web of Science][Medline].
Green DJ, and Gillette R. Circadian rhythm of firing rate recorded from single cells in the rat suprachiasmatic brain slice. Brain Res 245: 198-200, 1982[Web of Science][Medline].
Grynkiewicz G, Poenie M, and Tsien RY. A new generation of Ca²⁺ indicators with greatly improved fluorescence properties. J Biol Chem 260: 3440-3450, 1985[Abstract/Free Full Text].
Guido ME, de Guido L, Goguen D, Robertson HA, and Rusak B. Differential effects of glutamatergic blockade on circadian and photic regulation of gene expression in the hamster suprachiasmatic nucleus. Mol Brain Res 67: 247-257, 1999[Medline].
Hamada T, Liou SY, Fukushima T, Maruyama T, Watanabe S, Mikoshiba K, and Ishida N. The role of inositol trisphosphate-induced Ca²⁺ release from IP₃-receptor in the rat suprachiasmatic nucleus on circadian entrainment mechanism. Neurosci Lett 263: 125-128, 1999[Web of Science][Medline].
Hollmann M, Hartley M, and Heinemann S. Ca²⁺ permeability of KA-AMPA-gated glutamate receptor channels depends on subunit composition. Science 252: 851-853, 1991[Abstract/Free Full Text].
Hoyt KR, Arden SR, Aizenman E, and Reynolds IJ. Reverse Na⁺/Ca²⁺ exchange contributes to glutamate-induced intracellular Ca²⁺ concentration increases in cultured rat forebrain neurons. Mol Pharmacol 53: 742-749, 1997[Abstract/Free Full Text].
Huang R-C. Sodium and calcium currents in acutely dissociated neurons from rat suprachiasmatic nucleus. J Neurophysiol 70: 1692-1703, 1993[Abstract/Free Full Text].
Ibata Y, Okamura H, Tanaka M, Tamada Y, Hayashi S, Iijima N, Matsuda T, Munekawa K, Takamatsu T, Hisa Y, Shigeyoshi Y, and Amaya F. Functional morphology of the suprachiasmatic nucleus. Front Neuroendocrinol 20: 241-268, 1999[Web of Science][Medline].
Isaac JT, Nicoll RA, and Malenka RC. Evidence for silent synapses: implications for the expression of LTP. Neuron. 15: 427-434, 1995[Web of Science][Medline].
Jiang ZG, Yang YQ, Liu ZP, and Allen CN. Membrane properties and synaptic inputs of suprachiasmatic nucleus neurons in rat brain slices. J Physiol (Lond) 499 (1): 141-159, 1997[Abstract/Free Full Text].
Kim YI, and Dudek FE. Intracellular electrophysiological study of suprachiasmatic nucleus neurons in rodents: excitatory synaptic mechanisms. J Physiol (Lond) 444: 269-287, 1991[Abstract/Free Full Text].
King DP, and Takahashi JS. Molecular genetics of circadian rhythms in mammals. Annu Rev Neurosci 23: 713-742, 2000[Web of Science][Medline].
Leak RK, Card JP, and Moore RY. Suprachiasmatic pacemaker organization analyzed by viral transynaptic transport. Brain Res 819: 23-32, 1999[Web of Science][Medline].
Liu SQ, and Cull-Candy SG. Synaptic activity at calcium-permeable AMPA receptors induces a switch in receptor subtype. Nature 405: 454-458, 2000[Medline].
Luthi A, Chittajallu R, Duprat F, Palmer MJ, Benke TA, Kidd FL, Henley JM, Isaac JT, and Collingridge GL. Hippocampal LTD expression involves a pool of AMPARs regulated by the NSF-GluR2 interaction. Neuron 24: 389-399, 1999[Web of Science][Medline].
Meijer JH, Watanabe K, Schaap J, Albus H, and Detari L. Light responsiveness of the suprachiasmatic nucleus: long-term multiunit and single-unit recordings in freely moving rats. J Neurosci 18: 9078-9087, 1998[Abstract/Free Full Text]
Mikkelsen JD, Larsen PJ, Mick G, Vrang N, Ebling FJ, Maywood ES, Hastings MH, and Moller M. Gating of retinal inputs through the suprachiasmatic nucleus: role of excitatory neurotransmission. Neurochem Int 27: 263-272, 1995[Web of Science][Medline].
Mintz EM, Marvel CL, Gillespie CF, Price KM, and Albers HE. Activation of NMDA receptors in the suprachiasmatic nucleus produces light-like phase shifts of the circadian clock in vivo. J Neurosci 19: 5124-5130, 1999[Abstract/Free Full Text].
Moga MM, and Moore RY. Organization of neural inputs to the suprachiasmatic nucleus in the rat. J Comp Neurol 389: 508-534, 1997[Web of Science][Medline].
Moore RY. Entrainment pathways and the functional organization of circadian. Prog Brain Res 111: 103-119, 1996[Web of Science][Medline].
Moore RY, and Silver R. Suprachiasmatic nucleus organization. Chronobiol Int 15: 475-487, 1998[Web of Science][Medline].
Morin LP. The circadian visual system. Brain Res Rev 19: 102-127, 1994[Medline].
Neher E. Vesicle pools and Ca²⁺ microdomains: new tools for understanding their roles in neurotransmitter release. Neuron 20: 389-399, 1998[Web of Science][Medline].
Obrietan K, Impey S, and Storm DR. Light and circadian rhythmicity regulate MAP kinase activation in the suprachiasmatic nuclei. Nat Neurosci 1: 693-700, 1998[Web of Science][Medline].
Pennartz CM, Hamstra R, and Geurtsen AM. Enhanced NMDA receptor activity in retinal inputs to the rat suprachiasmatic nucleus during the subjective night. J Physiol (Lond) 532: 181-194, 2001[Abstract/Free Full Text].
Prosser RA. Glutamate blocks serotonergic phase advances of the mammalian circadian pacemaker through AMPA and NMDA receptors. J Neurosci 21: 7815-7822, 2001[Abstract/Free Full Text].
Rea MA, Buckley B, and Lutton LM. Local administration of EAA antagonists blocks light-induced phase shifts and c-fos expression in the hamster SCN. Am J Physiol Regulatory Integrative Comp Physiol 265: R1191-1198, 1993[Abstract/Free Full Text].
Reppert SM, and Schwartz WJ. The suprachiasmatic nuclei of the fetal rat: characterization of a functional circadian clock using 2-deoxyglucose. J Neurosci 4: 1677-1682, 1984[Abstract].
Reppert SM, and Weaver DR. Molecular analysis of mammalian circadian rhythms. Annu Rev Physiol 63: 647-676, 2001[Web of Science][Medline].
Saeb-Parsy K, Lombardelli S, Khan FZ, McDowall K, Au-Yong IT, and Dyball RE. Neural connections of hypothalamic neuroendocrine nuclei in the rat. J Neuroendocrinol 12: 635-648, 2000[Web of Science][Medline].
Schaap J, Bos NP, de Jeu MT, Geurtsen AM, Meijer JH, and Pennartz CM. Neurons of the rat suprachiasmatic nucleus show a circadian rhythm in membrane properties that is lost during prolonged whole-cell recording. Brain Res 815: 154-166, 1999[Web of Science][Medline].
Schroeder UH, Breder J, Sabelhaus CF, and Reymann KG. The novel Na⁺/Ca²⁺ exchange inhibitor KB-R7943 protects CA1 neurons in rat hippocampal slices against hypoxic/hypoglycemic injury. Neuropharmacology 38: 319-321, 1999[Web of Science][Medline].
.
Morin LP. The circadian visual system. Brain Res Rev 19: 102-127, 1994.
Shibata S, and Moore RY. Development of neural activity in the rat suprachiasmatic nucleus. Brain Res 431: 311-315, 1987[Medline].
Shibata S, and Moore RY. Neuropeptide Y and optic chiasm stimulation affect suprachiasmatic nucleus circadian function in vitro. Brain Res 615: 95-100, 1993[Web of Science][Medline].
Shibata S, Watanabe A, Hamada T, and Ono Mand Watanabe S. N-methyl-D-aspartate induces phase shifts in circadian rhythm of neuronal activity of rat SCN in vitro. Am J Physiol Regulatory Integrative Comp Phyiol. 267: R360-364, 1994.
Shirakawa T, and Moore RY. Glutamate shifts the phase of the circadian neuronal firing rhythm in the rat suprachiasmatic nucleus in vitro. Neurosci Lett 178: 47-50, 1994[Web of Science][Medline].
Stamp JA, Piggins HD, Rusak B, and Semba K. Distribution of ionotropic glutamate receptor subunit immunoreactivity in the suprachiasmatic nucleus and intergeniculate leaflet of the hamster. Brain Res 756: 215-224, 1997[Web of Science][Medline].
Sun X, Rusak B, and Semba K. Electrophysiology and pharmacology of projections from the suprachiasmatic nucleus to the ventromedial preoptic area in rat. Neuroscience 98: 715-728, 2000[Web of Science][Medline].
Morin LP. The circadian visual system. Brain Res Rev 19: 102-127, 1994.
Swanson GT, Kamboj SK, and Cull-Candy SG. Single-channel properties of recombinant AMPA receptors depend on RNA editing, splice variation, and subunit composition. J Neurosci 17: 58-69, 1997[Abstract/Free Full Text].
Tanaka M, Ichitani Y, Okamura H, Tanaka Y, and Ibata Y. The direct retinal projection to VIP neuronal elements in the rat SCN. Brain Res Bull 31: 637-640, 1993[Web of Science][Medline].
Tank DW, Regehr WG, and Delaney KR. A quantitative analysis of presynaptic calcium dynamics that contribute to short-term enhancement. J Neurosci 15: 7940-7952, 1995[Abstract].
van den Pol AN. The hypothalamic suprachiasmatic nucleus of the rat: intrinsic anatomy. J Comp Neurol 191: 661-702, 1980[Web of Science][Medline].
van den Pol AN, Hermans-Borgmeyer I, Hofer M, Ghosh P, and Heinemann S. Ionotropic glutamate-receptor gene expression in hypothalamus: localization of AMPA, kainate, and NMDA receptor mRNA with in situ hybridization. J Comp Neurol 343: 428-444, 1994[Web of Science][Medline].
van den Pol AN, and Tsujimoto KL. Neurotransmitters of the hypothalamic suprachiasmatic nucleus: immunocytochemical analysis of 25 neuronal antigens. Neuroscience 15: 1049-1086, 1985[Web of Science][Medline].
Washburn MS, Numberger M, Zhang S, and Dingledine R. Differential dependence on GluR2 expression of three characteristic features of AMPA receptors. J Neurosci 17: 9393-9406, 1997[Abstract/Free Full Text].
Welsh DK, Logothetis DE, Weister M, and Reppert SM. Individual neurons dissociated from rat suprachiasmatic nucleus express independently phase circadian firing patterns. Neuron 14: 697-706, 1995[Web of Science][Medline].
Yuste R, Majewska A, and Holthoff K. From form to function: calcium compartmentalization in dendritic spines. Nat Neurosci 3: 653-659, 2000[Web of Science][Medline].

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				J. Itri, S. Michel, J. A. Waschek, and C. S. Colwell Circadian Rhythm in Inhibitory Synaptic Transmission in the Mouse Suprachiasmatic Nucleus J Neurophysiol, July 1, 2004; 92(1): 311 - 319. [Abstract] [Full Text] [PDF]

				C. S. Colwell, S. Michel, J. Itri, W. Rodriguez, J. Tam, V. Lelievre, Z. Hu, X. Liu, and J. A. Waschek Disrupted circadian rhythms in VIP- and PHI-deficient mice Am J Physiol Regulatory Integrative Comp Physiol, November 1, 2003; 285(5): R939 - R949. [Abstract] [Full Text] [PDF]

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Excitatory Mechanisms in the Suprachiasmatic Nucleus: The Role of AMPA/KA Glutamate Receptors

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