Dopaminergic Control of Sleep-Wake States

doi:10.1523/JNEUROSCI.1767-06.2006

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The Journal of Neuroscience, October 11, 2006, 26(41):10577-10589; doi:10.1523/JNEUROSCI.1767-06.2006

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Behavioral/Systems/Cognitive
Dopaminergic Control of Sleep–Wake States
Kafui Dzirasa,¹ Sidarta Ribeiro,¹ Rui Costa,¹^,6 Lucas M. Santos,¹ Shih-Chieh Lin,¹ Andres Grosmark,¹ Tatyana D. Sotnikova,⁴ Raul R. Gainetdinov,⁴ Marc G. Caron,⁴ and Miguel A. L. Nicolelis¹^,2^,3^,5
Departments of ¹Neurobiology, ²Biomedical Engineering, ³Psychological and Brain Sciences, and ⁴Cell Biology and ⁵Center for Neuroengineering, Duke University Medical Center, Durham, North Carolina 27710, and ⁶Laboratory for Integrative Neuroscience, National Institute on Alcohol Abuse and Alcoholism, National Institutes of Health, Bethesda, Maryland 20892-9411

   Abstract

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Conclusion
References

Dopamine depletion is involved in the pathophysiology of Parkinson'sdisease, whereas hyperdopaminergia may play a fundamental rolein generating endophenotypes associated with schizophrenia.Sleep disturbances are known to occur in both schizophreniaand Parkinson's disease, suggesting that dopamine plays a rolein regulating the sleep–wake cycle. Here, we show thatnovelty-exposed hyperdopaminergic mice enter a novel awake statecharacterized by spectral patterns of hippocampal local fieldpotentials that resemble electrophysiological activity observedduring rapid-eye-movement (REM) sleep. Treatment with haloperidol,a D₂ dopamine receptor antagonist, reduces this abnormal intrusionof REM-like activity during wakefulness. Conversely, mice acutelydepleted of dopamine enter a different novel awake state characterizedby spectral patterns of hippocampal local field potentials thatresemble electrophysiological activity observed during slow-wavesleep (SWS). This dopamine-depleted state is marked by an apparentsuppression of SWS and a complete suppression of REM sleep.Treatment with D₂ (but not D₁) dopamine receptor agonists recoversREM sleep in these mice. Altogether, these results indicatethat dopamine regulates the generation of sleep–wake states.We propose that psychosis and the sleep disturbances experiencedby Parkinsonian patients result from dopamine-mediated disturbancesof REM sleep.

Key words: dopamine; sleep; REM; psychosis; schizophrenia; Parkinson's

   Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Conclusion
References

Dopamine is critically involved in regulating processes responsiblefor the generation of complex movement and emotions (Carlsson,1987). Altered central dopaminergic synaptic transmission hasbeen implicated in several neurological and psychiatric disorders,such as Parkinson's disease, schizophrenia, and attention deficithyperactivity disorder (Carlsson, 1987; Mazei-Robison et al.,2005; Greenwood et al., 2006). Individuals with these diseasesdemonstrate dramatic sleep disturbances, such as excessive daytimesleepiness (Adler, 2005), rapid-eye-movement (REM) sleep behaviordisorder (Gagnon et al., 2002; Abbott, 2005), decreased REMsleep latency, and disturbed sleep architecture (Maggini etal., 1986; O'Brien et al., 2003). Overall, these observationssuggest that dopamine may play a role in regulating the sleep–wakecycle as well.
Dramatic changes in neurotransmitter levels are known to occuras the brain progresses through the sleep–wake cycle.These changes are coordinated by complex interactions that systematicallymodulate the firing rate of cholinergic (Hobson et al., 1993),orexinergic (Lin et al., 1999), noradrenergic (Aston-Jones andBloom, 1981), histaminergic (John et al., 2004), and serotonergic(Espana and Scammell, 2004) neurons. These neurons, in turn,send efferent projections to cortical and subcortical structures,generating patterns of brain and muscle activity characteristicof the three major brain states: waking, slow-wave sleep (SWS),and REM sleep. During waking, the cortex displays low-amplitudefast oscillations in the gamma (33–55 Hz) frequency range,and muscle activity is highest (Steriade et al., 1993). As thebrain transitions to SWS, fast cortical oscillations are replacedby high-amplitude, low-frequency oscillations, and muscle activitydecreases (Steriade et al., 1993; Hobson and Pace-Schott, 2002).During REM sleep, the cortex and subcortical structures displayfast gamma oscillations similar to those observed during waking,and the hippocampus displays characteristic local field potential(LFP) oscillations in the 4–9 Hz range called theta rhythm(Vanderwolf, 1969; Timo-Iaria et al., 1970; Cantero et al.,2003). Additionally, muscle activity is primarily inhibitedduring REM sleep, with the exception of eye movements in humansand whisker movements in rodents (Aserinsky and Kleitman, 1953;Dement and Kleitman, 1957a,b; Jouvet et al., 1959). Althoughthe mean firing rate of dopaminergic neurons does not changesignificantly throughout the sleep–wake cycle (Milleret al., 1983), REM sleep is also characterized by an increasein dopamine release (Maloney et al., 2002; Lena et al., 2005).Together with the sleep disturbances displayed by individualswith altered dopaminergic transmission, this evidence furthersupports the hypothesis that dopamine plays an important rolein regulating the sleep–wake cycle.
To test this hypothesis, we investigated patterns of neuraland electromyographic (EMG) activity throughout the sleep–wakecycle in mice with genetically and pharmacologically manipulatedlevels of dopamine. Dopamine transporter–knock-out (DAT-KO)mice lack the gene encoding the dopamine transporter (DAT),a transmembrane protein that is responsible for regulating thereuptake of synaptic dopamine and replenishing dopamine storesin the presynaptic terminal (Gainetdinov and Caron, 2003). Assuch, the DAT plays the key role in controlling dopamine homeostasis.Because of the loss of the DAT, DAT-KO mice exhibit profounddepletion of intraneural dopamine stores as well as a fivefoldincrease in extracellular dopamine levels (Gainetdinov and Caron,2003). Thus, when exposed to novelty, DAT-KO mice experiencea marked period of behavioral hyperactivity (Gainetdinov etal., 1999). A similar phenotype is displayed by normal micetreated with amphetamine, which causes effective reversal ofDAT-mediated dopamine transport and a subsequent 5- to 10-foldincrease in extracellular dopamine (Jones et al., 1998).
Because intracellular dopamine stores originate from both denovo synthesis and DAT-mediated recycling of released dopamine,normal mice treated with the tyrosine hydroxylase inhibitor ${alpha}$ -methyl-p-tyrosine ( ${alpha}$ MT) demonstrate only a partial (60%) reductionin striatal dopamine levels. Because DAT-KO mice are unableto recycle dopamine, dopamine concentrations are solely dependenton de novo synthesis. Thus, treatment with ${alpha}$ MT produces a statein DAT-KO mice in which the striatal dopamine concentrationis reduced to 0.2% of the level in control animals [dopamine-depletedDAT-KO (DDD) mice] (Sotnikova et al., 2005). By treating normaland DAT-KO mice with amphetamine and ${alpha}$ MT, respectively, one canacutely manipulate dopaminergic tone and subsequently assessthe role of dopamine in regulating the sleep–wake cycle.

   Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Conclusion
References

Animal care and use. All experiments were conducted in accordance with National Institutesof Health guidelines for the care and use of animals and withan approved animal protocol from the Duke University InstitutionalAnimal Care and Use Committee. Experiments were performed withDAT-KO mice and their wild-type (WT) littermates that had beenbackcrossed into a C57B/6J background. Mice were housed fouror five to a cage and maintained under standard laboratory conditions(12 h light/dark cycle) with food and water provided ad libitum.Adult mice were separated into individual cages and surgicallyimplanted with electrodes and EMG wires. Experiments were conductedfollowing a 1 week recovery.
Surgery. Mice were anesthetized and placed in a stereotaxic device, andground screws were secured to the cranium. Tungsten microwirearray electrodes (diameter, 30 µm; impedance, 2 M ${Omega}$ at 1kHz, 5 nA) were implanted through a small cranial window intothe dorsal hippocampus (stereotaxic coordinates: –2.3mm anteroposterior, 1.6 mm mediolateral, and 1.8 mm dorsoventralfrom bregma) and anchored to ground screws using dental acrylic.Tungsten EMG wires were placed in the trapezius muscle, andskin was closed using surgical sutures.
Experimental setup. All experiments were conducted in a novel environment and duringthe animals' normal light cycle to ensure a significant amountof sleep. The novel environment consisted of an empty cage bottom(11.5 x 7 x 4.5 inches) that was marked into six equal sections,and gross motor activity was determined from the number of sectioncrosses during the waking period (see Fig. 1). Two pieces ofrodent feed and a small piece of paper were placed in the cagebottom, and a water bottle was suspended from the side wall.

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Figure 1. Behavioral dynamics of DAT-KO and WT control mice. a, Locomotion of DAT-KO mice and WT control mice in a novel environment. b, DAT-KO mice display locomotor hyperactivity during the WK-N period compared with WT control mice (n = 7). There was no significant difference between DAT-KO and WT mice during the habituated period (Kruskal–Wallis test: df = 3, p < 0.0001; followed by Mann–Whitney test; *p < 0.01 for comparisons of DAT-KO and WT control mice during WK-N, p > 0.05 for comparisons during WK-H; n = 8 for DAT-KO; n = 7 for WT control mice). Error bars indicate SEM.

Data acquisition. LFPs were preamplified (500x), filtered (0.3–400 Hz),and digitized at 500 Hz using a Digital Acquisition card (NationalInstruments, Austin, TX) and a Multi-Neuron Acquisition Processor(Plexon, Dallas, TX). Behaviors were recorded with a CCD videocamera and a video cassette recorder. Video and neural recordingswere synchronized with a millisecond precision timer (modelVTG-55; For-A, Tokyo, Japan).
Construction of the two-dimensional state space map. The two-dimensional state space was defined by two spectralamplitude ratios calculated by dividing integrated spectralamplitudes at selected frequency bands from LFPs recorded fromthe dorsal hippocampus. First, all data segments with amplitudesaturation were discarded from the working data set (2.31 ±0.75%; mean ± SEM of the total data per mouse). WithMatlab (MathWorks, Natick, MA), a sliding window Fourier transformwas applied to the LFP signal using a 2 s window with a 1 sstep. The Fourier transform parameters were chosen to allowfor a frequency resolution of 0.5 Hz. Then two spectral amplituderatios were calculated by integrating the spectral amplitude(absolute value) over selected frequency bands for each datawindow. The ratios were heuristic, resulting from a thoroughsearch for parameters aimed at the best separation of states.A low-cut frequency of 0.5 Hz was used to eliminate the DC component.For each animal, spectral amplitude ratios were further smoothedwith a Hanning window of 20 s to reduce within-state variability.These two ratios were used to construct the two-dimensionalstate space in which each point represents 1 s of ongoing brainactivity. The overlap of behavioral clusters was determinedby applying the Matlab "inpolygon" function to the two-dimensionalstate map.
EMG activity. Fourier transform was applied to the LFP signal using a 2 swindow with a 1 s step. The Fourier transform parameters werechosen to allow for a frequency resolution of 0.5 Hz. EMG activitywas then calculated by taking the root mean square of the spectralamplitude over selected frequency bands: 30–56 and 64–250Hz. All EMG traces were high-pass filtered at 30 Hz.
Behavioral state identification using two-dimensional state map and EMG. Parameters of the state map were chosen to generate clusterseparation based on the high-amplitude theta (4–9 Hz)and gamma (33–55 Hz) oscillations characteristic of REMsleep, the absence of gamma oscillations and the high-amplitudedelta (1–4 Hz) characteristic of SWS, and the high-amplitudegamma and theta oscillations characteristic of waking. Similarparameters have been shown to produce 95% cluster separationin state maps generated from LFP oscillations recorded fromrat dorsal hippocampus. The minor scoring errors in these mapstypically occurred in differentiating REM sleep from waking.Thus, EMG analysis was used to identify periods of atonia consistentwith REM sleep and combined with the two-dimensional state mapcluster scoring method for all sleep experiments conducted inthis study. Behavioral state selections were confirmed usingbehavioral observations and direct LFP and EMG analysis in twoWT and two DAT-KO mice. Spectral trajectories with high speeds,which represented transitions between behavioral states, wereexcluded from behavioral state cluster selections.
Selecting a 2 h habituated period. To create representative REM and habituated waking (WK-H) spectrogrampatterns, we empirically selected a two-hour period during thelast 4 h of the recording in which the mouse experienced atleast 10 min of waking and 2 min of REM sleep.
Peak theta powers distribution. Behavioral state clusters were selected using Statemap, EMGanalysis, and Matlab, and mean power spectrums were calculatedfor waking after novelty exposure (WK-N), WK-H, and REM. Thef_max (frequency, in the 4.5–11 Hz range, at which themax power occurs) was determined for each mean power spectrum,and the maximum power in a 1 Hz window surrounding f_max wascalculated for each second during the behavioral period. Thesepeak power values were normalized to the maximum peak powerobserved during REM and placed into nine equally spaced bins.Importantly, the mean power spectrum observed during REM remainedunchanged when DAT-KO mice were pretreated with haloperidoland when 12 h experimental recordings were conducted on DAT-KOmice in their home cage. This suggests that the peak theta powerobserved during REM can be used effectively as the baselinevariable wherewith to normalize the peak theta power distribution.
Wake–REM similarity index. Values were calculated by taking the sum of the absolute valueof the difference between waking and REM peak theta power distributionsand bounded between 1, for identical waking and REM distributions,and 0, as follows:

Dopamine depletion and REM recovery. All dopamine depletion studies were started 30 min after treatmentwith 250 mg/kg ${alpha}$ MT. In REM recovery experiments, L-DOPA, Quinpirole,or SKF-81297 was administered after an additional 30 min baselinedopamine depletion recording period. To ensure that the recoveryof REM sleep was attributable to the administration of exogenousdopaminergic agonists, and not enhanced tyrosine hydroxylasesynthesis resulting from repeated dopamine depletion, the REMrecovery recording period was limited to 6.5 h from the initialtreatment with ${alpha}$ MT. REM sleep was scored by the presence of 10continuous seconds of LFP spectral ratios and EMG activity withinthe normal REM boundaries established during the initial baselinesleep recordings conducted in untreated mice. Periods of REMsleep were always preceded and followed by high-speed inter-clusterdata points representing interstate transitions.
Confirmation of REM suppression using the sleep scoring method based on standard LFP and EMG analysis. To confirm the absence of bouts of REM sleep in DDD mice, weused an additional sleep scoring method based on standard LFPand EMG analysis. First, we analyzed the baseline sleep recordingsconducted in untreated DAT-KO mice and determined the maximumEMG power observed in REM sleep for each mouse. Next, we identifiedall 10 s epochs in DDD animals where EMG activity remained belowthe maximum value observed during normal REM sleep. This wasdone to maintain high sensitivity for bouts of REM sleep. Thismethod was also highly selective for epochs of low muscle activityoccurring during SWS and quiet waking, and 10 s epochs identifiedby this method often overlapped with each other. Next, we excludedall epochs in which mean fast (gamma) activity was lower thanthe mean fast activity observed across SWS during the baselinesleep recordings. Finally, we used video data to perform behavioralobservations and determine state-specific postures of the miceduring each epoch (e.g., curling quietly, moving, standing,rearing, etc.). This process excluded all 10 s epochs in dopamine-depletedmice and identified bouts of REM sleep in dopamine-depletedmice treated with L-DOPA and Quinpirole. In several DDD mice,there were no 10 s epochs in which EMG activity was lower thanthat observed during REM sleep. In other animals, there wereno 10 s epochs of low EMG activity with high-frequency brainactivity.
Theta power control in hyperactive animals. Wake–REM Similarity Index (WRSI) values were determinedfor each 1 min period in which animals displayed 10–15section crosses/min. These values were normalized over the numberof observations for each animal (14 ± 2 1 min periodsper mouse). All animals with five or less 1 min time periodsof 10–15 sections crosses were excluded from the analysis.
Statistics. Statistical significance of data from this study was analyzedby the Mann–Whitney test for single comparisons and theKruskal–Wallis test, followed by the Mann–Whitneytest for multiple comparisons. A p value <0.05 was consideredsignificant.

   Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Conclusion
References

Mice with genetically induced hyperdopaminergia display REM-like neural oscillations after exposure to a novel environment
Twenty-one adult DAT-KO and 13 WT littermate control mice weresurgically implanted with tungsten multielectrode arrays inthe hippocampus and tungsten electrodes in the trapezius muscle.After a 1 week recovery period, animals were subjected to continuoushippocampal LFP and EMG recordings for 12 h, while their behaviorswere recorded with a video camera. Eight DAT-KO mice were recordedin a novel cage, to induce behavioral hyperactivity (Fig. 1).All of the WT mice were recorded in the novel cage as controls,and 11 DAT-KO mice were subjected to continuous recordings for8 h in their home cage, to determine their baseline sleep patterns.To quantitatively distinguish WK, SWS, and REM sleep, we useda method recently developed in our laboratory that separateswake and sleep states as distinct clusters in a two-dimensionalstate map derived from two LFP spectral ratios (Gervasoni etal., 2004). The first ratio (ratio 1) produces cluster separationbased on high-frequency gamma (33–55 Hz) spectral oscillations(Steriade et al., 1993), whereas the second (ratio 2) producescluster separation based primarily on theta (4–9 Hz) spectraloscillations (Vanderwolf, 1969; Timo-Iaria et al., 1970; Canteroet al., 2003) (Fig. 2). The real-time version of the two-dimensionalstate map predicted behavioral states consistent with standardmethods for scoring sleep in mice based on direct observationsof LFP activity, EMG activity, behavioral activity, and state-specificpostures (Fig. 3). WK periods were characterized by high brainactivity and high muscle activity, SWS was characterized bylow brain activity and low muscle activity, and REM was characterizedby high brain activity and negligible muscle activity (atonia).

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Figure 2. Determination of state map ratios from power spectrum analysis. Behavioral state maps were generated by plotting the following spectral ratios: x-axis, 2–4.5 Hz/2–9 Hz (Ratio 2); y-axis, 2–20 Hz/2–55 Hz (Ratio 1).

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Figure 3. LFP and EMG activity during state map predicted behavioral states. Mice were introduced into a novel cage and subjected to 12 h continuous LFP (hippocampus) and EMG (trapezius) recordings. Real-time two-dimensional behavioral state maps were generated by plotting the following spectral ratios: x-axis, 0.5–4.5 Hz/0.5–9 Hz; y-axis, 0.5–20 Hz/0.5–55 Hz. Raw LFP and EMG activity was analyzed during periods of WK, SWS, and REM sleep predicted by the two-dimensional state map. As demonstrated previously, WK was characterized by high brain activity and high muscle activity, SWS was characterized by low brain activity and low muscle activity, and REM was characterized by high brain activity and negligible muscle activity (atonia).

To ensure accurate identification of sleep–wake states,we combined analysis of EMG activity patterns with an off-lineversion of our two-dimensional state map for all experimentspresented in this report. As observed previously in rats (Gervasoniet al., 2004), three spectral clusters were clearly visiblein two-dimensional state maps obtained from WT control mice,corresponding to WK, SWS, and REM sleep (Fig. 4a). Surprisingly,in the hyperdopaminergic DAT-KO mice recorded in the novel cage,a substantial overlap between WK and REM sleep clusters wasobserved in two-dimensional state maps generated from 12 h electrophysiologicalrecordings. No alteration in the SWS cluster was observed inthese animals (Fig. 4a,b) (percentage of overlap values: DAT-KOvehicle, 48 ± 6%; WT vehicle, 10 ± 4%; mean ±SEM; n = 8 for both groups; Mann–Whitney test, p <0.01). The increased percentage of WK-REM overlap values inDAT-KO mice suggests that a greater percentage of the LFP spectralratios typically observed during REM sleep appear during periodswhen the animals are awake. Importantly, during REM sleep, therelative power spectrum of hippocampal LFP oscillations at differentfrequencies was equivalent between WT and DAT-KO animals (Fig. 4c,d;Table 1).

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Figure 4. DAT-KO mice display novel REM-like awake state. Mice were introduced into a novel cage and subjected to 12 h continuous LFP (hippocampus) and EMG (trapezius) recordings. Two-dimensional behavioral state maps were generated by plotting the following spectral ratios: x-axis, 2–4.5 Hz/2–9 Hz; y-axis, 2–20 Hz/2–55 Hz. EMG data were used to disambiguate WK and REM clusters. All unassigned time points, typically corresponding to interstate transitions, were coded gray. a, WT mice displayed clear separation of the WK (blue), SWS (red), and REM (green) clusters. b, DAT-KO mice displayed distinct SWS clusters (red) but showed fused WK (blue) and REM (green) clusters. c, WT mice displayed state-dependant power spectral patterns characteristic of REM (green), SWS, and WK (blue) in rodents. REM was characterized by high-amplitude theta (4–9 Hz) and gamma (33–55 Hz) oscillations, SWS was characterized by high-amplitude delta (1–4 Hz) and low-amplitude gamma oscillations, and WK was characterized by high-amplitude gamma oscillations. d, DAT-KO mice displayed state-dependant power spectral oscillations characteristic of REM and SWS. WK spectrogram patterns displayed an REM-like distribution after exposure to novelty (blue) and normalized once the animals habituated to the novel environment (black).

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Table 1. Relative spectral power of WT and DAT-KO mice during REM sleep

The increased overlap of WK and REM sleep clusters in DAT-KOmice was not present in state maps generated from LFP oscillationsrecorded during the last 4 h of the experimental period (Fig. 5),suggesting that the waking period in which the LFP spectralratios assumed an REM-like character typically occurred duringthe initial period of exposure to novelty (Fig. 4d), and subsequentlysubsided as the animals habituated to the new environment. Thus,we set out to compare spectrogram patterns of the hippocampalLFPs observed during the first 2 h of the recording (WK-N) withthose observed after habituation to the novel environment, duringboth waking (WK-H) and REM sleep (note that there was no REMsleep in DAT-KO mice during the 2 h immediately after WK-N).The habituated period corresponded to 8–12 h after thebeginning of the recording session. To further investigate thetemporal nature of the striking WK-REM overlap in DAT-KO mice,we also calculated the peak spectral power, in the theta frequencyrange, over time.

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Figure 5. Habituated DAT-KO display normal behavioral state maps. Mice were introduced into a novel cage and subjected to 12 h continuous LFP (hippocampus) and EMG (trapezius) recordings. State maps were generated from LFPs, recorded 8–12 h after the animal was introduced into the novel cage, by plotting the following spectral ratios: x-axis, 2–4.5 Hz/2–9 Hz; y-axis, 2–20 Hz/2–55 Hz. EMG data were used to disambiguate WK and REM clusters. DAT-KO mice displayed clear separation of the WK (blue), SWS (red), and REM (green) clusters during the behaviorally habituated period.

WT mice displayed peak theta power distributions that were similarduring WK-N and WK-H. Furthermore, peak theta power was distributedover a wider range during REM sleep than any of the waking periodsin WT mice (Fig. 6a). In contrast, DAT-KO mice displayed peaktheta power distributions during the first 2 h in the novelenvironment that were virtually identical to those observedduring REM sleep (Fig. 6b). To quantify these differences, wedefined a WRSI that measures the correlation between the peaktheta power distribution of a given waking period and REM sleep.DAT-KO mice displayed significant WK/REM similarity during theWK-N period (i.e., animal awake after initial exposure to novelty).During the WK-H period (i.e., after habituation), however, theWK/REM similarity was much lower and statistically indistinguishablefrom that observed in WT mice (Fig. 6c). These results demonstratethat after exposure to novelty, hyperdopaminergic DAT-KO miceenter a novel awake state characterized by patterns of hippocampalneural activation similar to those observed during REM sleep.Interestingly, this state is also characterized by significantlyincreased hippocampal oscillations in the gamma frequency range(Fig. 7).

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Figure 6. Hyperdopaminergia and WK-N are necessary for generation of the REM-like awake state. a, b, Peak theta power distributions were determined for WT (a) and DAT-KO (b) mice during awake periods in a novel (WK-N) environment (x), habituated (WK-H) environment ( ${square}$ ), and REM sleep (solid line) behavioral periods and normalized to the maximum peak power observed during REM. c, The WRSI shows that the peak theta power distribution during WK-N in DAT-KO mice (n = 8) is significantly more similar to that of REM than the WK-H/DAT-KO, WK-H/WT, and WK-N/WT (n = 8) distributions (Kruskal–Wallis test: df = 3, p < 0.0001; followed by Mann–Whitney test; *p < 0.001). There was no statistical difference between WT and DAT-KO animals during the habituated period (p > 0.1).

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Figure 7. Novelty-induced hippocampal gamma oscillations in hyperdopaminergic mice. WT and DAT-KO mice were introduced into a novel cage and subjected to 12 h continuous LFP (hippocampus) and EMG (trapezius) recordings. Mean hippocampal gamma power was determined during the waking period immediately after WK-N and after habituation (WK-H). These values were then normalized to the mean gamma power observed during REM sleep for each animal. Novelty exposure significantly increased hippocampal gamma oscillations in DAT-KO mice (Kruskal–Wallis test: df = 3, p < = 0.01; followed by Mann–Whitney test; *p < 0.01) but not in WT mice (Mann–Whitney test, p > 0.05; n = 8 for DAT-KO and WT control mice). There was no statistical difference in hippocampal gamma power observed in DAT-KO and WT mice after habituation (Mann–Whitney test, p > 0.05). Treatment with 3.0 mg/kg amphetamine (Amp) significantly increased hippocampal gamma oscillations in WT control mice (Mann–Whitney test; ^#p < 0.05 compared with WT control mice/WK-N). Treatment with 0.3 mg/kg haloperidol (Hal) significantly reduced gamma oscillations in novelty-exposed DAT-KO mice (Mann–Whitney test; ^##p < 0.05 compared with DAT-KO mice/WK-N).

Although WT and DAT-KO mice display similar abundances of WK,SWS, and REM during the dark cycle (Wisor et al., 2001), theargument could be raised that the REM-like neural oscillationsobserved in awake DAT-KO mice during the WK-N period may beattributable to subtle differences in the preceding dark-cyclesleep–wake patterns, and not exposure to novelty. To determinewhether the REM-like neural oscillations observed in awake DAT-KOmice were indeed as a result of novelty exposure, we conducted12 h electrophysiological recordings and behavioral observationsacross the light cycle of five DAT-KO mice in their home cage.The DAT-KO mice recorded in their home cage displayed WRSI valuesduring the initial recording period that were statisticallysimilar to those observed in novelty-exposed DAT-KO mice duringthe habituated period [WRSI values: DAT-KO home cage, 0.55 ±0.08 (n = 5); DAT-KO habituated, 0.56 ± 0.02 (n = 8);mean ± SEM; p > 0.1, Mann–Whitney test]. Theseresults demonstrate that the REM-like neural oscillations observedin DAT-KO mice during awake states are indeed attributable toexposure to the novel environment. Importantly, exposure tonovelty does not further increase dopaminergic tone in DAT-KOmice (Gainetdinov et al., 1999). Therefore, because the "REM-like"patterns of neural activation cease as the animal habituatesto the environment, whereas dopaminergic tone remains constant(Gainetdinov et al., 1999), our results suggest that hyperdopaminergiais not sufficient to generate the REM-like oscillations in awakeDAT-KO mice.
Haloperidol reduces REM-like neural activity during wakefulness in DAT-KO mice
Next, we set out to determine whether hyperdopaminergia is necessaryto generate the REM-like oscillations in awake novelty-exposedDAT-KO mice. Four DAT-KO mice were treated with 0.3 mg/kg haloperidol,which has been shown to attenuate novelty-induced behavioralhyperactivity (Spielewoy et al., 2000), and 12 h electrophysiologicalrecordings and behavioral observations were repeated. Treatmentwith the D₂ dopamine receptor antagonist haloperidol causedsignificant suppression of the REM-like neural alterations observedin novelty-exposed DAT-KO mice, resulting in reduced overlapof WK and REM clusters (Fig. 8). Furthermore, this was concomitantto a significant decrease in WK/REM similarity observed duringthe WK-N period of treated animals [WRSI values: DAT-KO vehicle,0.84 ± 0.02 (n = 8); DAT-KO treated with haloperidol,0.67 ± 0.02 (n = 4); mean ± SEM; p < 0.05,Mann–Whitney test]. These results demonstrate that theWK/REM similarity observed in novelty-exposed DAT-KO mice canbe attenuated by blockade of the D₂ dopamine receptor, suggestingthat hyperdopamergia is indeed necessary to generate the REM-likeneural oscillations in novelty-exposed mice. Moreover, theseresults demonstrate that the WK-REM similarity is mediated viathe interaction of novelty exposure and activation of the D₂dopamine receptor pathway. Importantly, treatment with haloperidolalso reduced hippocampal oscillations in the gamma frequencyrange [normalized gamma power: DAT-KO vehicle, 1.18 ±0.05 (n = 8); DAT-KO treated with haloperidol, 1.02 ±0.06 (n = 4); Mann–Whitney test, p < 0.05] (Fig. 7).

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Figure 8. D₂ antagonist attenuates REM-like awake state in novelty-exposed DAT-KO mice. After initial recordings (left column), DAT-KO animals were given intraperitoneal injections of a single dose of 0.3 mg/kg haloperidol (right column), placed in a novel environment, and subjected to additional 12 h recordings. The haloperidol-treated group displayed significantly less overlap of WK (blue) and REM (green) clusters compared with the untreated group (p < 0.05, Mann–Whitney test). All unassigned time points, typically corresponding to interstate transitions, are coded gray.

Mice with pharmacologically induced hyperdopaminergia display REM-like neural oscillations while awake
To investigate whether hyperdopaminergia would generate REM-likeneural oscillations in the hippocampus of awake normal mice,and thus increase the WK/REM similarity, we treated five novelty-exposedWT control mice with amphetamine (Guix et al., 1992; Jones etal., 1998) and repeated our recording protocol. As predicted,WT mice treated with 3.0 mg/kg D-amphetamine displayed peaktheta power distributions that were wider during WK-N than thoseobserved during the WK-N period of untreated control mice andpower spectral distributions that were similar to those observedduring their periods of REM sleep (Fig. 9a,b). These electrophysiologicalalterations were parallel to a significant increase in WK-NWRSI values in the amphetamine-treated group [WRSI values: WTvehicle, 0.59 ± 0.03 (n = 8); WT D-amphetamine, 0.81± 0.02 (n = 5); mean ± SEM; p < 0.01, Mann–Whitneytest]. Moreover, the WK/REM similarity observed in the amphetamine-treatedcontrol mice was statistically indistinguishable from that observedin the hyperdopaminergic DAT-KO mice after exposure to novelty(p > 0.1, Mann–Whitney test). Interestingly, WT micetreated with amphetamine also displayed a significant increasein hippocampal oscillations in the gamma frequency range [normalizedgamma power: WT vehicle, 1.02 ± 0.04 (n = 8); WT D-amphetamine,1.19 ± 0.03 (n = 5); p < 0.01] (Fig. 7) that was statisticallyindistinguishable from that observed in novelty-exposed DAT-KOmice (p > 0.1, Mann–Whitney test) (Fig. 7).

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Figure 9. The role of hyperdopaminergia and locomotor hyperactivity in generating WK/REM similarity. After initial recordings (left column), WT animals were given intraperitoneal injections of a single dose of 3.0 mg/kg amphetamine (right column), placed in a novel environment, and subjected to 12 h recordings. a, b, WT mice treated with amphetamine displayed WK-N peak theta power distributions (a) and LFP power spectrum oscillations (b) that were similar to those observed during REM. c, Hippocampal LFP oscillations displayed REM-like distribution in amphetamine-treated WT mice even after the cessation of behavioral hyperactivity. d, WT mice treated with amphetamine (n = 5) displayed significantly elevated WRSI values after cessation of behavioral hyperactivity compared with untreated WT control mice (n = 5) during WK-N. DAT-KO mice treated with 0.3 mg/kg haloperidol (n = 4) displayed significantly elevated WRSI values during WK-N compared with WT control mice during WK-H (p < 0.05, Mann–Whitney test).

REM-like oscillations can be caused by hyperdopaminergia and novelty even in the absence of hyperlocomotive behavior
Although these results strongly suggest that the WK/REM similarityis mediated via the interaction of novelty and dopamine, andthat hyperdopaminergia alone is sufficient to generate REM-likeoscillations in awake WT control mice exposed to novelty, theyalso raise the possibility that the increased WRSI values observedduring the WK-N period of the hyperdopaminergic mice could emergebecause of changes in hippocampal theta oscillations resultingfrom enhanced exploratory behavior observed in these animals(Vanderwolf, 1969; Winson, 1974). To test whether the increasedWK/REM similarity was simply the result of enhanced exploratorybehavior rather than hyperdopaminergia, we determined WRSI valuesfor hyperdopaminergic mice in three behaviorally controlledparadigms. First, we calculated WRSI values for all 1 min timeperiods during the WK-N period in which WT mice, DAT-KO mice,and WT mice treated with amphetamine displayed 10–15 sectioncrosses. This level of behavioral locomotion was consideredelevated for WT mice (5.2 ± 1.1 section crosses per WKminute), low for DAT-KO mice (22.4 ± 4.6 section crossesper WK minute), and average for WT mice treated with amphetamine(18.8 ± 2.3 section crosses per WK minute). Althoughthe DAT-KO mice and amphetamine-treated WT mice displayed similardegrees of behavioral hyperactivity as the untreated WT mice[section crosses: WT, 12.1 ± 0.3 (n = 7); DAT-KO, 12.4± 0.3 (n = 7); WT-amphetamine, 12.5 ± 0.2 (n =5); mean ± SEM; p > 0.1 for both comparisons, Mann–Whitneytest], WK/REM similarity values were significantly elevatedin the DAT-KO mice and amphetamine-treated WT mice when comparedwith the untreated WT mice [WRSI values: WT vehicle, 0.65 ±0.03 (n = 7); DAT-KO vehicle, 0.77 ± 0.02 (n = 7); WT-amphetamine,0.77 ± 0.00 (n = 5); mean ± SEM; Mann–Whitneytest, p < 0.05 for both comparisons].
Next, we determined WRSI values for the five amphetamine-treatedWT mice during the 2 h control period immediately after thecessation of behavioral hyperactivity. This period typicallyoccurred 2 h after administration of amphetamine. Although theamphetamine-treated WT mice no longer displayed behavioral hyperactivityduring the control period, they continued to display REM-likeneural oscillations during wakefulness (Fig. 9c). Importantly,WRSI values remained significantly elevated in the amphetamine-treatedmice during the control period compared with WK-N WRSI valuesobserved in untreated animals (Fig. 9d, right side of the graph)[WRSI values: WT amphetamine/control period, 0.74 ± 0.03(n = 5); WT vehicle/WK-N, 0.60 ± 0.03 (n = 8); mean ±SEM; p < 0.01, Mann–Whitney test; square crossings/WKminute values: WT amphetamine/control period, 4.7 ± 0.7;WT vehicle/WK-N, 5.2 ± 1.1; mean ± SEM; p >0.1, Mann–Whitney test]. These results suggest that theWK/REM similarity observed in normal mice treated with amphetaminedoes not result from enhanced exploratory behavior, becauseit was observed even after the cessation of behavioral hyperactivity.
Next, we set out to compare WK/REM similarity values observedin DAT-KO mice with reduced behavioral hyperactivity profilesto those observed in normal mice. Thus, we compared WK-N WRSIvalues observed in haloperidol-treated DAT-KO mice with thoseobserved in WT mice during the habituated period. Importantly,the WK/REM similarity observed in the haloperidol-treated DAT-KOmice was significantly greater than that observed in WT micewith similar behavioral profiles (Fig. 9d, left side of thegraph) [WRSI values: DAT-KO haloperidol, 0.67 ± 0.02(n = 4); WT vehicle, 0.48 ± 0.03 (n = 8); mean ±SEM; p < 0.05, Mann–Whitney test; square crossings/WKminute values: DAT-KO haloperidol, 0.6 ± 0.4; WT vehicle,0.9 ± 0.2; mean ± SEM; p > 0.1, Mann–Whitneytest]. This result strongly suggests that both the hyperdopaminergicstate and exposure to novelty, but not hyperlocomotion, arenecessary and sufficient for the appearance of REM-like neuraloscillations in awake WT and DAT-KO mice, because it was observedduring periods of elevated, normal, and decreased locomotoractivity compared with control mice with equivalent behavioralprofiles.
Hippocampal theta oscillations are highly correlated with behaviorssuch as changes in posture or limb position, walking, head movements,and rearing and have been shown to vary on the order of hundredsof milliseconds (Vanderwolf and Baker, 1986). Thus, the argumentcan be raised that behavioral experiments that control locomotionacross 1 min or 2 h time periods are not sufficient to accountfor behavior-associated increases in theta oscillations. Toaddress this issue, we analyzed LFP and EMG recordings in DAT-KOand WT mice and found that DAT-KO mice appeared to display elevatedtheta oscillations during the WK-N period even at low levelsof muscle activity (Fig. 10). Thus, we used video recordingsto identify all 1 s intervals during the WK-N period in whichanimals were completely immobile (resting all four paws on thefloor) and calculated the mean theta power relative to thatobserved during subsequent episodes of REM sleep. Even duringperiods of immobility, hyperdopaminergic DAT-KO mice displayedsignificantly elevated power in the theta frequency range comparedwith WT control mice [percentage of REM theta power: DAT-KOimmobile, 87 ± 4% (n = 4); WT immobile, 66 ± 3%(n = 4); mean ± SEM; p < 0.05, Mann–Whitneytest]. Importantly, the WT and DAT-KO animals displayed similarlevels of theta power during REM sleep [REM theta power: DAT-KO,9 ± 3 µV² (n = 4); WT, 12 ± 4 µV²(n = 4); mean ± SEM; p > 0.1, Mann–Whitney test].These results demonstrate that DAT-KO mice display a significantincrease in hippocampal theta oscillations, providing strongevidence that the WK/REM similarity is mediated via the interactionbetween enhanced dopaminergic transmission and novelty, ratherthan simply resulting from enhanced locomotor behavior.

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Figure 10. Activity independent theta oscillations during WK-N in DAT-KO mice. WT and DAT-KO mice were introduced into a novel cage and subjected to 12 h continuous LFP (hippocampus) and EMG (trapezius) recordings. Peak theta power and EMG activity was determined for each second period. WT mice displayed similar levels of theta power immediately after exposure to novelty (blue) and after habituation (red) at low levels of EMG activity (arrows). DAT-KO mice displayed higher theta power after exposure to novelty (blue) than after habituation (red) at low levels of EMG activity as seen by the increase in visible blue area.

Dopamine depletion alters sleep–wake states in WT and DAT-KO mice
After verifying that excess dopamine generates a different awakestate in novelty-exposed mice, we set out to examine whetherdopamine depletion would also alter sleep–wake states.After the initial baseline recording period, five WT and fiveDAT-KO mice were treated with ${alpha}$ MT, and the recording protocolwas repeated. WT mice treated with ${alpha}$ MT demonstrated a partial(60%) reduction in striatal dopamine levels (Sotnikova et al.,2005). Although the WT animals treated with ${alpha}$ MT neither experiencechanges in their motor behavioral profile (Sotnikova et al.,2005) nor significant shifts in their LFP spectral ratios duringthe 6 h recording period, they all demonstrate a reduction inthe total REM sleep time [62 ± 18% reduction in totalREM time (n = 5); mean ± SEM; p < 0.05, Mann–Whitneytest] (Fig. 11a). Although these results suggest that dopaminergictransmission mediates REM sleep in normal mice, they also raisethe possibility that the reduction in total REM time observedin the ${alpha}$ MT-treated WT mice may be attributable to secondary depletionof norepinephrine or epinephrine (Sotnikova et al., 2005). However,this is highly unlikely because manipulations that decreasenorepinephrine have been shown to increase the abundance ofREM sleep (Kaur et al., 2004) and because the main source ofnorepinephrine in the brain, the locus ceruleus, ceases firingduring REM sleep (Aston-Jones and Bloom, 1981).

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Figure 11. Dopamine depletion suppresses REM sleep and generates novel awake state in DAT-KO mice. a, After baseline behavioral state recordings (left), WT mice were treated with a single dose of 250 mg/kg ${alpha}$ MT intraperitoneally, placed in a novel environment, and subjected to 6 h LFP (hippocampus) and EMG (trapezius) recordings. Two-dimensional behavioral state maps were generated by plotting the following spectral ratios: x-axis, 0.5–4.5 Hz/0.5–9 Hz; y-axis, 0.5–20 Hz/0.5–55 Hz. EMG data were used to disambiguate WK and REM clusters. All unassigned time points, typically corresponding to interstate transitions, are coded gray. WT mice treated with ${alpha}$ MT (right) continued to display REM sleep clusters during the 6 h recording period, although total REM time was dramatically reduced. b, c, After baseline behavioral state recordings in their home cage (left), DAT-KO mice were treated with a single dose of 250 mg/kg ${alpha}$ MT intraperitoneally, placed in a novel environment, and subjected to 8 h LFP (hippocampus) and EMG (trapezius) recordings. b, DAT-KO mice treated with ${alpha}$ MT displayed LFP spectral ratios that were indistinguishable from those observed during SWS sleep in untreated animals. Because our state map method did not produce cluster separation between WK and SWS in DDD mice, we termed this state " ${alpha}$ MT." This phenomenon lasted the entire 8 h period, and no REM clusters were observed. c, Dopamine-depleted DAT-KO mice also displayed significant increases in EMG activity during this period, corresponding to increased muscle rigidity. d, DAT-KO mice treated with ${alpha}$ MT displayed high-amplitude, low-frequency LFP oscillations by during awake periods marked by high muscle tone. e, State-dependent hippocampal LFP power spectral data observed in DAT-KO mice before and after being treated with ${alpha}$ MT. The ${alpha}$ MT (black) state was characterized by a reduction in mean hippocampal theta spectral power compared with WK (blue) and REM (green) in untreated animals and a reduction in mean hippocampal gamma spectral power compared with WK, SWS (red), and REM.

DAT-KO mice lack the key controller of dopamine homeostasis(Gainetdinov and Caron, 2003). These mice display remarkabledysregulation of intracellular and extracellular dopamine compartmentalization,and dopamine concentrations are solely dependent on ongoingdopamine synthesis. Treatment with 250 mg/kg ${alpha}$ MT in DAT-KO micereduces striatal dopamine concentration to <0.2% of the levelobserved in control animals (Sotnikova et al., 2005). As a consequence,DAT-KO mice treated with ${alpha}$ MT (DDD mice) display severe akinesiaand rigidity, which resembles late stages of Parkinson's diseasein humans (Sotnikova et al., 2005). Importantly, DDD mice demonstratea similar reduction in norepinephrine levels as WT mice treatedwith ${alpha}$ MT (Sotnikova et al., 2005). Thus, we predicted that ifthe reduction in REM time observed in WT mice treated with ${alpha}$ MTwas indeed attributable to dopamine depletion, DDD mice woulddemonstrate a much more profound suppression of REM sleep. Interestingly,treatment with ${alpha}$ MT generated a novel awake state in DAT-KO micecharacterized by LFP spectral ratios that were similar to thoseobserved during periods of SWS in untreated animals (Figs. 3,11b) and increased EMG activity corresponding to muscle rigidity(Fig. 11c). After analysis of hippocampal LFP activity, we foundthat awake DDD mice (high EMG activity, eyes open, and standingon all four paws) displayed high-amplitude, low-frequency LFPoscillations similar to those observed during SWS (Fig. 11d).These high-amplitude, low-frequency LFP oscillations were observedin striatum and cortex as well (Costa et al., 2006). Moreover,this state was marked by a dramatic reduction in LFP oscillationsin the gamma and theta frequency range (Fig. 11e). From directvisual observations, these animals appeared not to enter intosleep of any kind. However, given that our LFP recordings couldnot be used to distinguish brain activity in the dopamine-depletedstate from that observed during SWS, we focused our studieson investigating the absence of REM sleep in the dopamine-depletedDAT-KO mice.
Treatment with ${alpha}$ MT led to complete REM suppression in DAT-KOmice, which lasted for the entire 8 h of our original recordingsessions. To confirm that the DDD mice truly experience a completesuppression of REM sleep, we used a second method of scoringsleep–wake states based on standard analysis of 10 s epochsof LFP and EMG activity and behavioral observations. Using thismethod, we never observed epochs of muscular atonia accompaniedby desynchronized brain activity. Thus, we were unable to identifyany periods of REM sleep in DDD mice using this standard method.Later we discovered that complete REM suppression could be producedfor up to 16 h by treating these mice with an additional doseof 250 mg/kg ${alpha}$ MT immediately after the initial 8 h period ofdopamine depletion (n = 2; data not shown). These results stronglysuggest that dopamine is also involved in the induction of normalphysiological REM sleep, because complete depletion of thisneurotransmitter causes complete abolishment of REM sleep periods.
Activation of the D₂ pathway recovers REM sleep in dopamine-depleted mice
Next, we set out to test whether administration of exogenousdopaminergic agonists would induce recovery of REM sleep inDDD mice. It has been shown that high doses of the dopamineprecursor L-DOPA and combined D₁/D₂ receptor stimulation restorelocomotion in DDD mice (Sotnikova et al., 2005). Here, fiveDDD mice were treated with a dose (50 mg/kg) of L-DOPA thatis considered insufficient for restoring mobility (Sotnikovaet al., 2005). Strikingly, DDD mice treated with these lowerdoses of L-DOPA displayed recovery of REM sleep during the ensuing6 h recording period, although they did not recover mobility(Sotnikova et al., 2005) (Fig. 12a) [REM onset time: 1.4 ±0.3 h in DAT-KO mice treated with L-DOPA (n = 5) compared with1.7 ± 0.3 h in DAT-KO mice treated with vehicle (n =6); mean ± SEM; p > 0.1, Mann–Whitney test].We were able to identify periods of REM sleep using both ourstate-space method and the standard method of scoring sleep–wakestates. Moreover, LFP activity traces during these time periodsdisplayed trains of theta oscillations characteristic of REMsleep and EMG traces showed atonia (Fig. 13). Interestingly,DDD mice treated with L-DOPA displayed significantly less boutsof REM sleep compared with untreated DAT-KO mice [REM boutsper mouse: 8 ± 2 in DDD mice treated with L-DOPA (n =5) compared with 21 ± 3 in DAT-KO mice treated with vehicle(n = 6); mean ± SEM; p < 0.05, Mann–Whitneytest], although mean time spent in each bout of REM sleep wasthe same [REM time per bout: 59 ± 7 s in DDD mice treatedwith L-DOPA (n = 39 total bouts) compared with 42 ± 3in DAT-KO mice treated with vehicle (n = 123 total bouts); mean± SEM; p > 0.1, Mann–Whitney test]. These resultsdemonstrate that REM sleep can be recovered in DDD mice by administeringan endogenous dopamine precursor, even at doses insufficientto restore motor behaviors. Importantly, treatment with L-DOPArecovers both norepinephrine and epinephrine to some extentin DDD mice. Thus, although these results strongly suggest thatREM sleep is mediated via dopaminergic transmission, they donot eliminate the possibility that the suppression and recoveryof REM sleep in DDD mice is attributable to depletion and recoveryof other catecholamines.

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Figure 12. Selective recovery of REM sleep in DDD mice. DDD mice were treated intraperitoneally with a single dose of 50 mg/kg L-DOPA, 5 mg/kg Quinpirole, or 10 mg/kg SKF 81297, placed in a novel environment, and subjected to 6 h LFP (hippocampus) and EMG (trapezius) recordings. Two-dimensional behavioral state maps were generated by plotting the following spectral ratios: x-axis, 0.5–4.5 Hz/0.5–9 Hz; y-axis, 0.5–20 Hz/0.5–55 Hz. EMG data were used to disambiguate WK and REM clusters. All unassigned time points, typically corresponding to interstate transitions, are coded gray. a, Treatment with 50 mg/kg L-DOPA recovered a clear state map REM sleep cluster (left) that was marked by low EMG activity (right), although it did not completely reverse the ${alpha}$ MT state observed in DDD mice. State maps and EMG plots observed in untreated DDD mice are displayed at the top left of each plot. b, DDD mice treated with the D₂ dopamine receptor agonist Quinpirole (5 mg/kg) displayed a clear REM sleep cluster (left) that was marked by low EMG activity (right). Treatment with Quinpirole did not reverse the ${alpha}$ MT observed in DDD mice. c, DDD mice treated with the D₁ dopamine receptor agonist SKF 81297 (10 mg/kg) displayed neither recovery of an REM sleep cluster nor reversal of the ${alpha}$ MT state.

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Figure 13. Raw LFP and EMG activity during selective recovery of REM sleep in DDD mice. DDD mice were treated intraperitoneally with a single dose of 50 mg/kg L-DOPA or 5 mg/kg Quinpirole, placed in a novel environment, and subjected to 6 h LFP (hippocampus) and EMG (trapezius) recordings. DDD mice displayed trains of theta oscillations and atonia during periods of REM sleep recovered by treatment with L-DOPA or Quinpirole, similar to that observed during REM sleep in untreated DAT-KO mice.

To determine whether REM suppression in DDD mice was directlyattributable to depletion of dopamine, we treated DDD mice withdirect D₁ and D₂ dopamine receptor agonists. When administeredtogether (but not separately), D₁ and D₂ dopamine receptor agonistshave been shown to recover movement in DDD mice (Sotnikova etal., 2005). Five DDD mice were treated with 5 mg/kg of the selectiveD₂ dopamine receptor agonist Quinpirole, and the recording protocolwas repeated. This dose was chosen because it has been shownto cause activation of D₂ dopamine receptors sufficient to recoveryof forward locomotion in DDD mice treated with a D₁ dopaminereceptor agonist. Again, although this treatment alone was notsufficient to induce recovery of mobility in DDD mice, Quinpirolerecovered REM sleep during the ensuing 6 h recording period(Fig. 12b) [REM onset time: 1.8 ± 0.5 h in DDD mice treatedwith Quinpirole (n = 5) compared with 1.7 ± 0.3 h inDAT-KO mice treated with vehicle (n = 6); mean ± SEM;p > 0.1, Mann–Whitney test]. Periods of REM sleep wereidentified by both our state-space method and the standard methodof scoring sleep–wake states. Again, LFP activity tracesduring these time periods display trains of theta oscillationscharacteristic of REM sleep, and EMG traces demonstrate atonia(Fig. 13). Thus, activation of the D₂ receptor was sufficientto recover REM sleep in DDD mice. Interestingly, DDD mice treatedwith Quinpirole demonstrate a similar number of bouts of REMsleep compared with DDD mice treated with L-DOPA [REM bouts:10 ± 3 in DDD mice treated with Quinpirole (n = 5); mean± SEM; p > 0.1, Mann–Whitney test], though themean time spent in each of these bouts of REM is significantlyreduced (REM time/bout: 37 ± 7 s in DDD mice treatedwith Quinpirole (n = 48 total bouts), mean ± SEM; p <0.01, Mann–Whitney test]. Importantly, Quinpirole activatesD₂ dopamine receptors in DDD mice without recovering norepinephrineand epinephrine. Thus, these results demonstrate that dopaminedoes indeed mediate the generation of REM sleep. Interestingly,because DDD mice treated with Quinpirole demonstrate shorterbouts of REM sleep than DDD mice treated with L-DOPA, our findingsalso suggest that other catecholamines may play a role in regulatingthe maintenance of REM sleep (Ouyang et al., 2004). Curiously,selective activation of the D₁ dopamine receptor pathway, viainjection of the selective D₁ dopamine receptor agonist SKF-81297(10 mg/kg), did not induce any recovery of REM sleep (Fig. 12c)(n = 5). This dose of SKF-81297 was chosen because it was sufficientto recover forward locomotion in DDD mice treated with a D₂dopamine receptor agonist (Sotnikova et al., 2005). Importantly,we never observed epochs of atonia that were accompanied bydesynchronized brain activity. Thus, we were unable to identifyany episodes of REM sleep using our state-space method or standardsleep-scoring method.
Altogether, these results indicate that selective activationof the D₂, but not the D₁, dopamine receptor pathway is sufficientto recover REM sleep in DDD mice. This is of particular importancegiven that the novelty-induced, REM-like neural oscillationsobserved in awake hyperdopaminergic mice could be attenuatedby blocking the D₂ pathway. Thus, our results demonstrate thatboth physiological REM sleep and the novelty-induced, REM-likeneural oscillations are mediated by the D₂ receptor pathwayin DAT-KO mice, suggesting that the REM-like neural oscillationsobserved in awake hyperdopaminergic mice may result from aberrantactivation of a physiological REM sleep pathway during awakebehaving periods.

   Discussion

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Abstract
Introduction
Materials and Methods
Results
Discussion
Conclusion
References

Our findings demonstrate that novelty-exposed mice with genetically(DAT-KO mice) or pharmacologically (WT animals treated withamphetamine) induced hyperdopaminergia display a novel awakestate characterized by hippocampal neural oscillations similarto those observed during REM sleep. Generally stated, REM-likeelectrophysiological activity appears during wakefulness inhyperdopaminergic mice. This activity is marked by a significantincrease in hippocampal theta and gamma oscillations that isnot trivially explained by enhanced exploratory behavior displayedby these mice. Additionally, treatment with the D₂ dopaminereceptor antagonist and antipsychotic agent haloperidol attenuatesthese REM-like hippocampal theta and gamma oscillations. Conversely,our findings also demonstrate that dopamine depletion diminishesREM sleep in normal mice and causes DAT-KO mice to enter a differentnovel awake state characterized by neural oscillations similarto those observed during SWS (increased cortical oscillationsin the delta frequency range and a virtual absence of gammaoscillations), an apparent suppression of normal SWS, and acomplete suppression of REM sleep. Finally, we showed that REMsleep can be recovered in these DDD mice by selective activationof the D₂, but not the D₁, dopamine receptor pathway. Altogether,these results demonstrate for the first time that dopamine playsa central role in regulating sleep–wake states and thatthis action is mediated via the D₂ dopamine receptor pathway.
REM sleep is a brain state during unconsciousness in which thebrain displays increased activation of cortical networks similarto that observed during waking and the body displays atonia(Steriade et al., 1993). The high-frequency brain activity observedduring waking and REM sleep is modulated via the ascending reticularactivating system (RAS), which arises from the brain stem andprojects to the cortex. The RAS has two main branches. The firstbranch consists of cholinergic projections from the pedunculopontineand laterodorsal tegmental nuclei to the thalamus. The secondbranch projects to the basal forebrain and cortex and consistsof serotonergic efferents from the dorsal and medial raphe nuclei,noradrenergic efferents from the locus ceruleus, histaminergicefferents from the tuberomammillary nucleus, and dopamine efferentsfrom the ventral periaqeuductal gray matter. These efferentsactivate neurons in the basal forebrain, which in turn modulatethe projections to the cortex (Saper et al., 2005). Both branchesof the RAS converge on a population of cells in the sublateraldorsal nucleus [SLD; anatomically corresponding to the peri-locusceruleus- ${alpha}$ (peri-LC ${alpha}$ ) in cats] thought to be responsible for thegeneration of REM sleep. Indeed, activation of the SLD/peri-LC ${alpha}$ via microinjection of glutamatergic agonists has been shownto generate a transient REM-like brain state accompanied byatonia (Boissard et al., 2002). The SLD/peri-LC ${alpha}$ nuclei receivemonoaminergic afferents, including dopamine afferents from theposterior hypothalamus. Interestingly, direct application ofdopaminergic agonists to the caudal SLD/peri-LC ${alpha}$ has been shownto generate an REM-like brain state that is not accompaniedby atonia (Crochet and Sakai, 1999). Here, we show that micewith genetically and pharmacologically induced hyperdopaminergiademonstrate REM-like neural oscillations during awake behavingperiods accompanied by an increase in hippocampal gamma oscillations.Moreover, we demonstrate that mice profoundly depleted of dopaminedisplay an awake state characterized by the virtual suppressionof hippocampal gamma oscillations and the absence of REM sleep.Together, this suggests that dopamine may modulate efferentsfrom the SLD/peri-LC ${alpha}$ responsible for coordinating the activationof thalamocortical networks during REM sleep. Thus, in the absenceof dopamine, the cortex displays widely synchronized oscillationscharacteristic of thalamocortical network inhibition, whereasin the presence of excess dopamine, the cortex displays increasedhigh-frequency oscillations. Indeed, the REM-like brain stateobserved in animals with dopamine agonists administered to theSLD/peri-LC ${alpha}$ may result from activation of REM sleep relay trackswithout the accompanying activation of upstream neurons responsiblefor the generation of muscle atonia.
Dopamine is critically involved in regulating neural processesresponsible for complex movements and emotions (Carlsson, 1987).Consequently, altered central dopaminergic transmission hasbeen implicated in several neurological and psychiatric disorderssuch as schizophrenia and Parkinson's disease. Dopaminergicdysfunction was first implicated in mediating psychosis whenthe therapeutic efficacy of classical antipsychotic agents (e.g.,haloperidol) was found to be directly correlated with theiraffinity for the dopamine D₂ receptor (Creese et al., 1976;Seeman et al., 1976). Furthermore, drugs that increase endogenousdopamine release (e.g., amphetamines) were found to induce psychosisin healthy individuals and exacerbate psychotic symptoms inschizophrenic patients (Snyder, 1972). Recent evidence alsosuggests that other pharmacological agents that induce psychosisin healthy individuals (e.g., PCP) demonstrate significant potencyfor the D₂ dopamine receptor (Kapur and Seeman, 2002; Seemanet al., 2005).
Freud and Kraepelin, the founding fathers of modern psychiatry,proposed that psychosis resulted from the intrusion of the sleepingmind on the conscious mind (Freud, 1900; Heynick, 1993). Here,we demonstrate that mice with genetically or pharmacologicallyinduced hyperdopaminergia display spectral changes in hippocampaltheta oscillations after exposure to novel environments. Notably,these spectral changes result in increased neural similaritybetween waking and REM sleep. We also demonstrate that normalREM sleep can be suppressed in both normal and DAT-KO mice bydiminishing dopaminergic tone. These results establish an importantand previously unreported role of dopamine in regulating physiologicalREM sleep. Finally, we showed that REM sleep requires activationof the D₂ dopamine receptor pathway, the very pathway implicatedin mediating psychosis, and that the D₂ dopamine receptor antagonistand antipsychotic agent haloperidol suppresses the novelty-induced,REM-like hippocampal neural oscillations observed in DAT-KOmice.
Hippocampal theta oscillations are driven by cholinergic inputfrom the medial septum, which receives afferent projectionsfrom A10 dopaminergic neurons in the ventral tegmental area(Bjorklund and Lindvall, 1984). When injected in the medialseptum or administered systemically, dopamine agonists increasetheta oscillations (Miura et al., 1987; Kichigina, 2004). Moreover,systemic administration of dopamine antagonists decreases thetaoscillations (Miura et al., 1987; Kichigina, 2004). Our resultsdemonstrate that normal mice treated with amphetamine demonstratea significant increase in hippocampal theta oscillations. Amphetamineinduces a dopamine-dependent release of acetylcholine in thehippocampus (Nilsson et al., 1992). Thus, although amphetaminedemonstrates efficacy for several monoamine transporters otherthan the DAT (Gainetdinov and Caron, 2003), the increased thetaoscillations observed in the hippocampus of normal mice treatedwith amphetamine are likely attributable to the action of amphetamineat the DAT. This suggests that hippocampal theta oscillationsmay be directly correlated with dopaminergic tone under normalphysiological conditions as well. REM is characterized by prominenthippocampal theta oscillations (Vanderwolf, 1969; Timo-Iariaet al., 1970