Selective Activation of the Extended Ventrolateral Preoptic Nucleus during Rapid Eye Movement Sleep

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The Journal of Neuroscience, June 1, 2002, 22(11):4568-4576

Selective Activation of the Extended Ventrolateral Preoptic Nucleus during Rapid Eye Movement Sleep
Jun Lu¹, Alvhild A. Bjorkum¹^,², Man Xu¹, Stephanie E. Gaus¹, Priyattam J. Shiromani³, and Clifford B. Saper¹
¹ Department of Neurology, Beth Israel Deaconess Medical Center, Boston, Massachusetts 02215, ² Department of Physiology, University of Bergen, Bergen N-5009, Norway, and ³ Department of Neurology, Veterans Affairs Medical Center, West Roxbury Harvard Medical School, Boston, Massachusetts 02132

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We found previously that damage to a cluster of sleep-active neurons (Fos-positive during sleep) in the ventrolateral preopticnucleus (VLPO) decreases non-rapid eye movement (NREM) sleep inrats, whereas injury to the sleep-active cells extending dorsallyand medially from the VLPO cluster (the extended VLPO) diminishesREM sleep. These results led us to examine whether neurons inthe extended VLPO are activated during REM sleep and the connectivityof these neurons with pontine sites implicated in producing REMsleep: the laterodorsal tegmental nucleus (LDT), dorsal raphenucleus (DRN), and locus ceruleus (LC). After periods of darkexposure that triggered enrichment of REM sleep, the number ofFos-positive cells in the extended VLPO was highly correlatedwith REM but not NREM sleep. In contrast, the number of Fos-positivecells in the VLPO cluster was correlated with NREM but not REMsleep. Sixty percent of sleep-active cells in the extended VLPOand 90% of sleep-active cells in the VLPO cluster in dark-treatedanimals contained galanin mRNA. Retrograde tracing from the LDT,DRN, and LC demonstrated more labeled cells in the extended VLPOthan the VLPO cluster, and 50% of these in the extended VLPO weresleep-active. Anterograde tracing showed that projections fromthe extended VLPO and VLPO cluster targeted the cell bodies anddendrites of DRN serotoninergic neurons and LC noradrenergic neuronsbut were not apposed to cholinergic neurons in the LDT. The connectionsand physiological activity of the extended VLPO suggest a specializedrole in the regulation of REMsleep.

Key words: laterodorsal tegmental nucleus; dorsal raphe nucleus; locus ceruleus; galanin; GABA; c-Fos

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Recent studies show that the ventrolateral preoptic nucleus (VLPO) contains a cluster of sleep-active neurons (Sherin et al.,1996, 1998; Szymusiak et al., 1998). These sleep-active cellscontain galanin and GABA (Sherin et al., 1998; Gaus et al., 2002)and project to many components of the arousal system includingthe histaminergic tuberomammillary nucleus (TMN), the serotoninergicdorsal raphe nucleus (DRN), and the noradrenergic locus ceruleus(LC) (Sherin et al., 1998; Steininger et al., 2001), suggestingthat they may inhibit the ascending monoaminergic arousal systemduring sleep. After preoptic lesions, loss of neurons in the VLPOcluster correlates closely with the loss of non-rapid eye movement(NREM) sleep (Lu et al., 2000). Although REM sleep is also diminishedafter lesions of the VLPO region, this is not correlated withthe loss of cells in the VLPO cluster, suggesting that cells nearbybut outside the VLPO cluster regulate REM sleep. Numerous galaninergiccells are located dorsally and medially to the VLPO cluster (theextended VLPO), and many of them are sleep-active (Fos-positive)during sleep and are galaninergic (Gaus et al., 2002). We foundthat loss of sleep-active cells in the extended VLPO is correlatedwith a decrease in REM sleep but not NREM sleep (Lu et al., 2000).

This hypothetical role of the extended VLPO cells in REM sleep control is consistent with the observations that some cellsin the VLPO region fire faster during REM sleep compared withduring NREM sleep or wakefulness (Koyama and Hayaishi, 1994; Osakaand Matsumura, 1994; Szymusiak et al., 1998). However, these single-unitrecording studies could not determine whether the REM-active neuronswere galaninergic. In addition, very little is known about theprojections of the extended VLPO neurons compared with the VLPOcluster.

To address these questions, we developed a model for identifying anatomically the REM active neurons in the VLPO area. Previousstudies had found that exposing rats to darkness during the dailylight cycle when they are usually asleep triggers REM sleep (Alfoldiet al., 1991; Benca et al., 1991, 1998; Miller et al., 1998).We therefore correlated the number of sleep-active cells in theextended VLPO with REM sleep during dark exposure. We also determinedby the combination of anterograde and retrograde tracing withimmunocytochemistry and in situ hybridization whether the sleep-activecells in the extended VLPO during periods of enhanced REM sleepcontain galanin and project to pontine sites believed to controlproduction of REM sleep [i.e., the laterodorsal tegmental nucleus(LDT), DRN, and LC].

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals
Pathogen-free adult male Sprague Dawley rats (275-300 gm; n = 82) purchased from Harlan Sprague Dawley (Indianapolis, IN)were used. The rats were individually housed and had access tofood and water ad libitum. All animals were housed under controlledconditions (12 hr of light starting at 7:00 A.M.; 200 lux) inan isolated ventilated chamber maintained at 20-22°C. All protocolswere approved by the Institutional Animal Care and Use Committeesof Beth Israel Deaconess Medical Center and Harvard MedicalSchool.

Physiology
Implantation for EEG/EMG. After animals were anesthetized with chloral hydrate, the skull was exposed. Four screw electrodeswere implanted into the skull, in the frontal (two electrodes)and parietal (two electrodes) bones of each side, and two flexiblewire electrodes were placed in the nuchal muscles. The incisionswere closed by wound clips. The electrodes were soldered to socketsthat were connected via flexible recording cables and a commutatorto a Grass polygraph (Grass Instruments, West Warwick, RI) andacomputer.
Dark treatment and EEG recording. After 1 week on a 12 hr light/dark schedule (lights on at 7:00 A.M.), including 2 d of adaptationto the EEG/EMG cables, animals were exposed to extended darknessor normal light from 7:00 A.M. to 10:00 A.M. EEG/EMG was continuouslyrecorded during this period. After the dark or light exposure,animals were killed by vascular perfusion (seebelow).
Sleep analyses. The EEG/EMG signals were amplified by a polygraph (Grass Instruments) and digitized by an Apple Macintosh(Cupertino, CA) power computer running Icelus (G Systems Inc.,Plano, TX). Wake-sleep states were manually scored in 12 sec epochson the digitized EEG/EMG. Wakefulness was identified by the presenceof a desynchronized EEG and phasic EMG activity. NREM sleep consistedof a high-amplitude slow-wave EEG together with a low-EMG tonerelative to waking. REM sleep was identified by the presence ofregular theta activity coupled with low-EMG tone relative to NREMsleep. The amount of time spent in a wake state, NREM sleep, andREM sleep was determined for eachhour.

Histology and tracing
Tracer injections. Under chloral hydrate anesthesia (7% in saline; 350 mg/kg), a fine glass pipette containing a 2.5% solutionof the anterograde tracer Phaseolus vulgaris leucoagglutinin (PHA-L)in saline was lowered into the extended VLPO and VLPO clusterstereotaxically [anteroposterior (AP), $-$ 0.6 mm; dorsoventral (DV), $-$ 8.5 mm; mediolateral (ML), $-$ 1.0 mm; with the bitebar at $-$ 3.3mm (Paxinos and Watson, 1986)]. PHA-L was injected by iontophoresiswith a current of 5 µA for 15 min (7 sec on and 7 sec off) togive a discrete injection site (~200-300 µm in diameter). After2 additional min, the pipette was slowly withdrawn. Cholera toxinsubunit B (CTB; List Biological, Campbell, CA) was injected beforeimplantation for EEG/EMG using an air-pressure delivery systemto inject 6 nl of CTB solution (1% in saline). CTB targets includedthe central DRN (AP, $-$ 7.80 mm; ML, 0 mm; DV, $-$ 5.6 mm), the lateralwing of the DRN (AP, $-$ 7.80 mm; ML, 0.4 mm; DV, 5.6 mm), the LDT(AP, $-$ 8.0 mm; ML, 0.8 mm; DV, 5.8 mm), and the LC (AP, $-$ 9.30 mm;ML, 1.0 mm; DV, 6.0 mm). Incisions were closed with wound clipsand animals survived for 7d.
Perfusion and histology. Animals were deeply anesthetized by chloral hydrate (350 mg/kg) and then perfused through the heartwith 50 ml of saline followed by 500 ml of 10% formalin. The brainswere removed and postfixed in 10% formalin for 4 hr and then equilibratedin 20% sucrose in PBS at 4°C.
Immunohistochemistry. The brains were sectioned on a freezing microtome into four series (40 µm thickness) for immunostainingonly or five (30 µm thickness) series of sections for immunostainingplus in situ hybridization. Sections were washed in PBS (threechanges) and incubated in PBS containing 0.3% Triton X-100 (PBT)and 0.2% sodium azide for 1 hr at room temperature, followed bythe primary antiserum: Fos, Ab-5, 1:150,000, rabbit (OncogeneSciences, Uniondale, NY); CTB, 1:100,000, goat (List Biological);PHA-L, 1:10,000, goat (Vector Laboratories, Burlingame, CA); cholineacetyltransferase (ChAT), 1:20,000, rabbit UO93 (gift from Dr.Louis Hersh, University of Kentucky); tyrosine hydroxylase (TH),1:200, TE-101, rabbit (Eugene Tech, Eugene, OR); 5-HT, 1:10,000,goat (Chemicon, Temecula, CA) for 1 d at room temperature. Sectionswere then washed in PBS and incubated in biotinylated secondaryantiserum (against appropriate species IgG; 1:1000 in PBT) for1 hr, washed again in PBS, and incubated in avidin-biotin complexreagents for 1 hr. Sections were then washed again and incubatedin a 0.06% solution of 3,3-diaminobenzidine tetrahydrochloride(DAB; Sigma, St. Louis, MO) plus 0.02% H₂O_2. The sections werestained brown with DAB only or black by adding 0.05% cobalt chlorideand 0.01% nickel ammonium sulfate to the DAB solutions. Fos andPHA-L staining was done using the black reaction, and CTB, ChAT,5-HT, and TH staining was done using the brown reaction, as describedpreviously (Chou et al., 2002). For double labeling of Fos andgalanin mRNA, sections were stained for Fos with the brown reactionand then used for in situhybridization.
In situ hybridization. The sections (30 µm thickness) with Fos staining were acetylated and hybridized overnight (55°C) witha ³⁵S-labeled cRNA probe synthesized from a plasmid containing thecomplete coding sequence of rat galanin (Vrontakis et al., 1987).After washing, the tissue was treated with RNase-A (BoehringerMannheim, Indianapolis, IN) followed by a succession of washesof increasing stringency (1 hr each in 2× SSC/1 mM DTT, 50°C;0.2× SSC/1 mM DTT, 55°C; 0.2× SSC/1 mM DTT, 60°C), and then dehydratedin alcohols and air-dried. The sections were exposed to x-rayfilm (Eastman-Kodak, Rochester, NY) for 2-3 d, and then the slideswere dipped in Kodak NTB-2 emulsion and exposed for 1 month. Slideswere developed in Kodak D-19, fixed, and then dehydrated andcoverslipped.
Cell counting. Fos-positive cells were counted in brightfield by an observer who was blinded to physiological treatment, inthree consecutive sections (AP level: from $-$ 0.3 mm to $-$ 0.7 mm)through the midpart of the VLPO and extended VLPO. The spacingbetween the sections was 160 µm. For experiments in which therewas no galanin-staining present to define the borders of the VLPO,we constructed a set of counting boxes based on the distributionof galaninergic neurons: the VLPO cluster box was 300 µm wideby 300 µm high, placed along the base of the brain just medialto the diagonal band of Broca, as shown in Figure 1B. The medialextended VLPO box was medial to the VLPO cluster and 400 µm wideby 300 µm high (Fig. 1A); the dorsal extended VLPO box was 200µm wide by 300 µm high, positioned above the VLPO cluster andmedial extended VLPO boxes, and centered over their border. Becausethe mean diameter of Fos-labeled nuclei was not different betweenexperimental groups and controls, and we were interested onlyin relative cell numbers; we did not apply a correction factorfor double counting (Guillery and Herrup, 1997).

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Figure 1. A pair of photomicrographs showing the distributions of Fos-ir cells in the extended VLPO and VLPO cluster in an animal exposed to light (12% REM sleep, A) and in an animal exposed to dark treatment (30% REM sleep, B) during the early part of the sleep cycle. The counting boxes used for the VLPO cluster and the dorsal and medial extended VLPO are shown in B. These sections are approximately at the level of AP $-$ 0.5 in Paxinos and Watson (1986). OC, Optic chiasm.

Statistical analysis
We used Student's two-tailed t test to compare the differences in the amounts of NREM and REM sleep time and in the numbersof Fos-positive and double-labeled cells in the extended VLPOand VLPO cluster, under control conditions and after darktreatment.
For correlational analysis, the mean number of Fos-immunoreactive (Fos-ir) cells (per section per side) in the extended VLPOor the VLPO cluster was plotted against amounts of NREM sleepor REM sleep during the hour before perfusion. Pearson correlationcoefficients and p values werecalculated.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The relationship of Fos-positive neurons in the extended VLPO and sleep

To determine the relationship of the Fos-ir cells in the extended VLPO and REM sleep, on the day of the experiment we exposedanimals (n = 19) to dark from 7:00 A.M. to 10:00 A.M. (dark treatment)after 1 week on a 12 hr light/dark cycle. Control animals (n =10) were exposed to light from 7:00 A.M. to 10:00 A.M. as usual.Dark treatment increased REM sleep consistently across the 3 hrperiod. NREM sleep occupied 65.2 ± 4.2% (mean ± SEM) and REM sleepoccupied 13.1 ± 4.9% of the first hour; NREM was 60.2 ± 4.5% andREM was 16.1 ± 2.1% in the second hour; and NREM was 56.1 ± 4.5%and REM was 17.1 ± 3.4% of the third hour. Over the third hour,dark treatment increased REM sleep by twofold over controls (dark,17.1 ± 3.4%; light, 8.5 ± 3.1%; p < 0.001),but had no significanteffect on NREM sleep (dark, 56.1 ± 4.5%; light, 62.2 ± 8.4%; p> 0.05).

Dark-treated animals had a significant increase in the number of Fos-ir cells compared with controls in the medial extendedVLPO (22.9 ± 1.3 vs 12.8 ± 1.0 cells · section¹ · side¹; p < 0.01) and dorsal extended VLPO (13 ± 1.3 vs 6.6 ± 1.7 cells· section¹ · side¹; p < 0.01). However, the number of Fos-ir cells in the VLPO clusterdid not differ (dark treatment, 20.4 ± 5.3 cells · section¹ · side¹ vs controls, 18.0 ± 5.5 cells · section¹ · side¹; p > 0.05).

Putting together the light- and dark-treated animals, the number of Fos-ir cells in the medial extended VLPO (r = 0.76; p< 0.01) or dorsal extended VLPO (r = 0.71; p < 0.01) was significantlycorrelated with REM sleep during the previous hour but was notsignificantly correlated with NREM sleep (r = 0.12, 0.34; p >0.05) (Fig. 2). In contrast, the number of VLPO cluster cellswas not significantly correlated with REM sleep (r = 0.07; p >0.05) (Fig. 2); however, it was significantly correlated withNREM sleep (r = 0.76; p < 0.01) (Fig. 2).

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Figure 2. Correlation (illustrated by solid line) of the number of Fos-ir cells in the extended VLPO and VLPO cluster in light- and dark-treated animals with the amounts of REM sleep or NREM sleep that the animals experienced during the hour before perfusion.

Sleep-active cells in the extended VLPO and VLPO cluster of dark-treated animals contain galanin

The relationship of Fos-ir cells and neurons containing galanin mRNA in the extended VLPO was determined in rats that receiveddark treatment (n = 10) versus controls (n = 7) (Fig. 3). In thedark-treated animals, 90.2 ± 8.2% of the Fos-positive cells inthe VLPO cluster and 60.5 ± 6.1% of Fos cells in the extendedVLPO contained galanin mRNA. In control rats, a high percentageof Fos-ir cells also contained galaninergic mRNA in the VLPO cluster(93.2 ± 9.5%) and the extended VLPO (80.7 ± 10.2%).

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Figure 3. Photomicrographs showing dual labeling of Fos (brown immunostaining) and galanin mRNA (black silver grains representing in situ hybridization) in the extended VLPO and VLPO cluster. Arrowheads indicate double-labeled cells. Many Fos-ir cells in the extended VLPO and particularly in the VLPO cluster contain galanin mRNA. A shows the VLPO complex with boxes that are shown at higher magnification in B-D. Note that these fields are not equivalent to the counting boxes shown in Figure 1. OC, Optic chiasm.

Relationship of Fos-positive and retrogradely labeled cells after injections of CTB into the LDT, LC, and DRN after dark treatment

To determine whether the cells in the extended VLPO and VLPO cluster that project to the LDT, DRN, and LC expressed Fos duringREM sleep, we injected the retrograde tracer CTB into the regioncontaining the LDT (n = 10), LC (n = 12), or DRN (central area,n = 10; lateral wing, n = 9). The animals were then perfused asdescribed above after dark treatment, and the brains were stainedfor CTB (brown) and Fos (black). All cell counts were done onthe ipsilateral side of the brain, which contained the heaviestretrograde labeling. Animals in this series were analyzed if theyspent >50% of the hour before death in NREM sleep and >10% inREMsleep.

In seven rats that had injections into the LDT (Fig. 4), many more CTB-labeled cells were found in the extended VLPO (5.8± 2.5 cells/ipsilateral section; p < 0.05) than in the VLPO cluster(2.8 ± 0.9 cells/ipsilateral section). Of CTB-labeled cells, 62.2± 19.5% in the extended VLPO and 95.0 ± 5.0% in the VLPO clusterwere Fos-positive (Fig. 5). Three control rats in which the CTBinjections were dorsal to the LDT showed no retrogradely labeledcells in either the extended VLPO or the VLPO cluster.

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Figure 4. Camera lucida drawings showing selected injection sites (black solid and dashed lines) of CTB in the region of the DRN (A), LDT (B), and LC (C) as well as four injection sites of PHA-L in the VLPO region (D). Gray shading shows borders of key nuclei; gray lines show other brain structures. Br, Barrington's nucleus; HDB, horizontal limb of the nucleus of the diagonal band of Broca; mlf, medial longitudinal fasciculus; MnRn, median raphe nucleus; OC, optic chiasm; scp, superior cerebellar peduncle; VTg, ventral tegmental nucleus.

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Figure 5. Dual labeling of CTB retrograde transport (brown) and Fos expression (black) in cells within the extended VLPO and VLPO cluster (B, E, H) after the injections of CTB into the central DRN (A, experiment R2049), LDT (D, experiment R1969), and LC (G, experiment R2219), respectively, in the rats exposed to 3 hr of darkness. In B, E, and H, the VLPO cluster is identified by a large arrow and the extended VLPO by a large double-headed arrow. The rectangular boxes identify the fields that are magnified in C, F, and I, respectively. Double-labeled cells in the extended VLPO and VLPO cluster are indicated by small arrows and single CTB labeled cells are indicated by small arrowheads.

Five of 12 injections aimed at the LC largely filled the nucleus; in the rest of the animals, the injections were medial,lateral, or ventral to the LC, and these rats were used as anatomicalcontrols. In the five sleeping rats with injections filling theLC, more CTB-labeled cells were found in the extended VLPO thanin the VLPO cluster (6.5 ± 1.5 vs 3.0 ± 1.4 cells/ipsilateralsection; p < 0.05). In these dark-treated animals, 46.6 ± 7.4%of the CTB-labeled cells in the extended VLPO and 56.0 ± 3.1%of CTB-labeled cells in the VLPO cluster were Fos-positive (Fig.5). We also noticed CTB-labeled cells scattered in the medialpreoptic area and dorsolateral preoptic area, but these cellswere not Fos-positive during sleep (Fig. 5). The injections inthe areas immediately medial (R2103), lateral (R2091 and R2099),or ventral (R2090 and R2098) to the LC did not retrogradely labelcells in the extended VLPO or the VLPO cluster (Fig. 4).

In 10 rats with injections of CTB into the central part of the DRN, more retrogradely labeled cells were found in the extendedVLPO than in the VLPO cluster (5.5 ± 2.1 vs 2.4 ± 1.1 cells/ipsilateralsection; p < 0.05). Only 15.0 ± 8.2% of CTB-labeled cells in theextended VLPO and 12.5 ± 4.5% of CTB-labeled cells in the VLPOcluster were Fos-positive (Fig. 5). We found numerous CTB-labeledcells in the diagonal band nucleus, the median preoptic nucleus,and the dorsolateral preoptic area, but very few cells in theseregions were Fos-positive duringsleep.

Four rats that had CTB injections into the lateral wing of the dorsal raphe nucleus (also called the paradorsal raphe nucleus;see injection 2203 in Fig. 4A) and were asleep for most of thehour before perfusion (NREM, 53.5 ± 5.6%; REM, 18.2 ± 4.3%) showedretrogradely labeled cells in the extended VLPO (3.0 ± 0.8 cells/ipsilateralsection) and VLPO cluster (3.0 ± 0.81 cells/ipsilateral section).In these animals, a large percentage of retrogradely labeled neuronswas also Fos-positive in the VLPO cluster (64.2 ± 27.4%) and extendedVLPO (56.5 ± 7.0%). Two rats that had injections ventral to thelateral wing of the DRN (experiments R2222 and R2223) (Fig. 4A)showed no double-labeled cells in the VLPO cluster and very fewin the extended VLPO. Two other rats that had injections intothe lateral wing of the DRN and >70% wakefulness during the hourbefore perfusion also showed no double-labeled cells in the extendedVLPO and VLPOcluster.

Anterograde tracing of inputs from the extended VLPO and VLPO cluster to the LDT, DRN, and LC

To determine the relationship of efferents from the extended VLPO and VLPO cluster to chemically identified neurons in theLDT, DRN, and LC, PHA-L was injected into the extended VLPO andthe VLPO cluster in five rats, and sections through the brainstemwere immunostained for PHA-L (black) axons and with antisera against5-HT, ChAT, or TH(brown).

The VLPO complex was successfully labeled in four cases: two involving the cluster plus part of the extended VLPO and twoinvolving primarily the extended VLPO (Fig. 4D). All of them gaverise to a similar pattern of efferent projection. In case R2133,the PHA-L injection filled the VLPO cluster and dorsal extendedVLPO and partially filled the medial extended VLPO. Labeled efferentsterminated extensively in the LDT, LC, and DRN, as well as inthe median raphenucleus.

In the LDT, labeled axons primarily terminated in the dorsal LDT region. The efferent terminal field only partially overlappedwith the region occupied by cholinergic cells. Double stainingshowed that labeled terminals did not form appositions with theChAT-ir cell bodies or proximal dendrites in the LDT, but ratherappeared to terminate in the region between the cholinergic cellbodies (Fig. 6). Using Nissl staining, we found that some terminalsapposed small-sized cells in the LDT region. Compared with theLDT, relatively few labeled axons terminated in the cholinergicpedunculopontine tegmental nucleus (PPT) and the efferent terminalsdid not appose cholinergic cells.

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Figure 6. Photomicrographs showing the relationships of anterogradely labeled efferent axons (black) from the extended VLPO and VLPO cluster with neurons in the DRN, LDT, and LC that are stained (brown) for serotonin, choline acetyltransferase, or tyrosine hydroxylase, respectively. In A, the efferent terminals concentrate dorsal to the cluster of the cholinergic cells in the LDT. Occasionally we found that terminal boutons were near choline acetyltransferase-immunoreactive neurons such as in B; however careful observation indicated that such boutons were not on the same plane as the cholinergic cell body. In C and D, efferent terminal boutons clearly appose serotonin-immunoreactive neurons in the DRN. E and F show labeled efferent axons apposing tyrosine hydroxylase-immunoreactive neurons in the LC.

In the LC, terminal boutons were located predominantly in the ventral LC, especially in the region containing a dense bundleof noradrenergic dendrites, where many boutons apposed TH-ir dendrites.In addition, labeled terminals also were apposed to the noradrenergiccell bodies in the core of the LC (Fig. 6).

In the DRN, efferent terminals were heavily distributed throughout the nucleus and especially in its lateral wing. Doublestaining demonstrated that many labeled terminals apposed serotoninergiccell bodies and dendrites in the DRN (Fig. 6), although many terminatedon unlabeled (presumably nonserotoninergic) cells. Labeled axonsalso terminated heavily in the ventrolateral periaqueductal graymatter (PAG), dorsolateral to the lateral wing of theDRN.

Cases in which the injections involved the extended VLPO but avoided the VLPO cluster (e.g., experiments R2132 and R2134)(Fig. 4D) showed very similar distributions of efferent terminalswith respect to appositions onto the monoaminergic and cholinergicneurons in the midbrain and pons. The only major exception wasa relatively smaller number of terminals onto serotoninergic neuronsin the central DRN in thesecases.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Our principal findings were that in dark-treated rats with increased amounts of REM sleep, the number of Fos-positive cellsin the extended VLPO was positively correlated with REM sleeptime but was not correlated with NREM sleep time. In contrast,the number of Fos-positive cells in the VLPO cluster was positivelycorrelated with NREM sleep time but was not correlated with REMsleep time. A high percentage of Fos-positive cells in the VLPOcluster (>90%) and the extended VLPO (>60%) contained galaninmRNA. By injecting retrograde tracer into the LDT and LC, we foundthat the extended VLPO of dark-treated rats contained more retrogradelylabeled cells than the VLPO cluster, and that ~50% of the labeledcells were Fos-positive in dark-treated sleeping animals. Althoughwe found that numerous retrogradely labeled cells in the extendedVLPO project to the central part of the DRN, a relatively smallnumber of them (12-15%) were Fos-positive during sleep in dark-treatedanimals. However, injections of CTB into the lateral wing of theDRN yielded more retrogradely labeled and double-labeled cells(CTB plus Fos) in the VLPO cluster (64%). Anterograde tracingshowed that the efferents of the extended VLPO and VLPO clusterapposed the serotoninergic cell bodies and proximal dendritesin the DRN especially in the lateral wing region and the noradrenergiccell bodies in the LC, but there were few appositions with thecholinergic cells in the LDT or PPT. We hypothesize that the extendedVLPO may enhance REM sleep by its influence on the LDT, DRN, andLC.

Technical considerations

Four methods have been used previously to study brain activity during enhanced REM sleep in rats and cats: auditory stimulation,recovery from REM sleep deprivation (platform method), injectionof carbachol into the brainstem, and dark treatment. Using thefirst two methods, Merchant-Nancy et al. (1995) found significantFos induction in the brainstem (nucleus of the solitary tract,LDT, PPT, and parabrachial nucleus) and diencephalon (suprachiasmaticnucleus, lateral hypothalamus), and amygdaloid nucleus. Injectionof carbachol into a region of the pontine reticular formationthat receives the LDT/PPT cholinergic efferents (Semba et al.,1990) causes prolonged and persistent REM sleep in cats and rats(Shiromani et al., 1992, 1995; Marks and Birabil, 1998; Hornerand Kubin, 1999) and produces Fos in both cholinergic and noncholinergiccells such as GABAergic ones in the LDT and PPT (Shiromani etal., 1992, 1995; Yamuy et al., 1998; Xi et al., 1999; Torteroloet al., 2001). Similar Fos expression patterns in the LDT/PPThave also been observed during recovery from REM sleep deprivation(Maloney et al., 1999). In contrast, Fos immunoreactivity wasnot expressed in the serotoninergic DRN cells and noradrenergicLC cells during REM sleep (Maloney et al., 1999). These resultsare consistent with the hypothesis that REM sleep is triggeredby activity of cholinergic LDT/PPT neurons, occurring in associationwith inactivity of the monoaminergic cells in the DRN and LC (Maloneyet al., 1999, 2000; see below). However, these previous studiesdid not examine the hypothalamus indetail.

We chose to use dark treatment to induce REM sleep because it does not involve inherently stressful or invasive procedures.The mechanism by which dark treatment triggers REM sleep is notclear, although this phenomenon appears to occur in albino butnot pigmented rats (Benca et al., 1991, 1998). Direct retinalprojections have been found to the sleep-active, galaninergiccells in the extended VLPO and VLPO cluster (Lu et al., 1999)and to the DRN (Shen and Semba, 1994; Fite et al., 1999). Thispathway could potentially mediate the effect of dark treatmenton REM sleep. However, Miller et al. (1998) reported that lesionsof the pretectum and superior colliculus could diminish the dark-mediatedincrease in REMsleep.

We realize that demonstration of synaptic contacts from the extended VLPO and VLPO cluster with neurons in the brainstem willrequire electron microscopy. However, the spatial relationshipof the terminal boutons with cell bodies in our materials suggeststhe likelihood of synapticcontacts.

Brainstem regulation of REM sleep

It is well established that the cholinergic cells in the LDT/PPT, which show increased firing rates during REM sleep and arealmost inactive during NREM sleep, play a central role in generatingREM sleep (Kayama et al., 1992; Sakai and Koyama, 1996). Lesionsof the LDT abolish REM sleep in cats (Webster and Jones, 1988),and electrical stimulation of the LDT or glutamate injection intothe PPT increases REM sleep (Thakkar et al., 1996; Datta and Siwek,1997). Injection of the cholinergic agonist carbachol into themedial pontine reticular formation, a target of the PPT (Rye etal., 1987), induces prolonged and persistent REM sleep in catsand rats (Shiromani et al., 1992, 1995; Marks and Birabil, 1998).

Serotoninergic cells in the DRN and noradrenergic cells in the LC are active during wakefulness, less active during NREM sleep,and inactive during REM sleep (Heym et al., 1982; Fornal et al.,1985; Sakai, 1986; Reiner and McGeer, 1987; Yamuy et al., 1995,1998; Thakkar et al., 1998; Gervasoni et al., 2000). Both cellgroups project to the LDT/PPT (Semba and Fibiger, 1992; Hondaand Semba, 1994; Leonard et al., 1995; Steininger et al., 1997)where they are thought to inhibit the cholinergic neurons. Theinhibition of serotoninergic and noradrenergic neurons by theextended VLPO would thereby promote REM sleep (Jones, 1991; Hobsonet al., 1998; Crochet and Sakai, 1999).

The quiescence of sertoninergic cells during REM sleep is caused by GABAergic inputs (Levine and Jacobs, 1992; Wang et al.,1992; Nitz and Siegel, 1997a; Gervasoni et al., 2000). Becausevirtually all VLPO and extended VLPO neurons that contain galaninalso contain GABA, the extended VLPO may be a critical sourceof inhibition of monoaminergic regions during REM sleep (Sherinet al., 1998; Gervasoni et al., 2000; J. E. Sherin and C. B. Saper,unpublished observations). Stimulation of the preoptic area bywarming, which increases the firing of many sleep-active neurons,inhibits firing activity in the serotoninergic cells in the DRN(Guzman-Marin et al., 2000). Similarly GABAergic control of theLC is also thought to derive from the preoptic area (Luppi etal., 1995; Nitz and Siegel, 1997b; Sherin et al., 1998; Luppiet al., 1999). Sherin et al. (1998) attributed this projectionprimarily to the VLPO, but their injections of anterograde tracerincluded the medial and dorsal extended VLPO as well as the VLPOcluster. Our results indicate that much of the input to the DRNand LC attributed to the VLPO actually originates from the extendedVLPO.

We also identified an intense projection from the extended VLPO and VLPO cluster to the ventrolateral PAG. The ventrolateralPAG contains GABAergic cells (Gervasoni et al., 2000), and injectionof a GABAergic agonist into the ventrolateral periaqueductal graymatter increases REM sleep (Sastre et al., 1996). The mechanismby which GABAergic cells in the periaqueductal gray matter maycontribute to REM sleep remains to be determined, but our findingsuggests another potential pathway by which the extended VLPOand VLPO cluster may influence REMsleep.

Preoptic regulation of REM and NREM sleep

The sleep-active cells in the VLPO cluster were originally defined by their expression of Fos protein during sleep, theirexpression of the neurotransmitters galanin and GABA, and theirprojection to the histaminergic cells in the TMN (Sherin et al.,1996, 1998). Our previous studies (Sherin et al., 1998; Lu etal., 2000; Gaus et al., 2002) also found that many cells extendingbeyond the VLPO cluster in a dorsal and medial direction possessthe same qualities, and we speculated that they might projecttopographically to different targets. We found that lesions ofthe VLPO cluster primarily were correlated with loss of NREM sleep,whereas lesions of the extended VLPO correlated with loss of REMsleep (Lu et al., 2000). Here we show in dark-treated rats thatthe sleep-active cells in the extended VLPO are galaninergic cells,that their activity is highly correlated with REM sleep, and thatthey do indeed have slightly different projections from neuronsin the VLPO cluster, which are consistent with a role in regulatingREMsleep.

During NREM sleep, the sleep-active neurons in the VLPO cluster would inhibit the activity of the cells in the TMN, DRN, andLC by releasing galanin and GABA, thus maintaining slow-wave sleep.During the transitions from NREM to REM sleep, the firing of DRNand LC is further decreased (Heym et al., 1982; Fornal et al.,1985; Sakai, 1986; Reiner and McGeer, 1987). We propose that thistransition may be attributable at least in part to the recruitmentof inhibitory neurons in the extended VLPO that further decreaseLC and DRN firing, thus disinhibiting the LDT and PPT cholinergiccells. In addition, if extended VLPO efferents end on inhibitoryinterneurons in the LDT/PPT, they could further promote theirfiring during the transition to REM sleep. The connections ofthe extended VLPO neurons and their REM-active pattern would makethem prime candidates to fulfill thisrole.

  FOOTNOTES

Received Aug. 20, 2001; revised March 12, 2002; accepted March 13, 2002.

This work was supported by United States Public Health Service Grants NS3397, HL60292, AG47755, and MH12058. We thank QuanHa, Alex Adler, and Minh Ha for technicalassistance.

Correspondence should be addressed to Dr. Clifford B. Saper, Department of Neurology, Beth Israel Deaconess Medical Center,330 Brookline Avenue, Boston, MA 02215. E-mail: csaper{at}caregroup.harvard.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Alfoldi P, Franken P, Tobler I, Borbely AA (1991) Short light-dark cycles influence sleep stages and EEG power spectra in the rat. Behav Brain Res 43:125-131[ISI][Medline].
Benca RM, Bergmann BM, Leung C, Nummy D, Rechtschaffen A (1991) Rat strain differences in response to dark pulse triggering of paradoxical sleep. Physiol Behav 49:83-87[Medline].
Benca RM, Gilliland MA, Obermeyer WH (1998) Effects of lighting conditions on sleep and wakefulness in albino Lewis and pigmented Brown Norway rats. Sleep 21:451-460[ISI][Medline].
Chou TC, Bjorkum AA, Gaus SE, Lu J, Scammell TE, Saper CB (2002) Afferents to the ventrolateral preoptic nucleus. J Neurosci 22:977-990[Abstract/Free Full Text].
Crochet S, Sakai K (1999) Effects of microdialysis application of monoamines on the EEG and behavioural states in the cat mesopontine tegmentum. Eur J Neurosci 11:3738-3752[ISI][Medline].
Datta S, Siwek DF (1997) Excitation of the brain stem pedunculopontine tegmentum cholinergic cells induces wakefulness and REM sleep. J Neurophysiol 77:2975-2988[Abstract/Free Full Text].
Fite KV, Janusonis S, Foote W, Bengston L (1999) Retinal afferents to the dorsal raphe nucleus in rats and Mongolian gerbils. J Comp Neurol 414:469-484[Medline].
Fornal C, Auerbach S, Jacobs BL (1985) Activity of serotonin-containing neurons in nucleus raphe magnus in freely moving cats. Exp Neurol 88:590-608[ISI][Medline].
Gaus SE, Strecker RE, Tate BA, Parker RA, Saper CB (2002) Ventrolateral preoptic nucleus contains sleep-active, galaninergic neurons across the mammalian spectrum. Neuroscience, in press.
Gervasoni D, Peyron C, Rampon C, Barbagli B, Chouvet G, Urbain N, Fort P, Luppi PH (2000) Role and origin of the GABAergic innervation of dorsal raphe serotonergic neurons. J Neurosci 20:4217-4225[Abstract/Free Full Text].
Guillery RW, Herrup K (1997) Quantification without pontification: choosing a method for counting objects in sectioned tissues. J Comp Neurol 386:2-7[ISI][Medline].
Guzman-Marin R, Alam MN, Szymusiak R, Drucker-Colin R, Gong H, McGinty D (2000) Discharge modulation of rat dorsal raphe neurons during sleep and waking: effects of preoptic/basal forebrain warming. Brain Res 875:23-34[ISI][Medline].
Heym J, Steinfels GF, Jacobs BL (1982) Activity of serotonin-containing neurons in the nucleus raphe pallidus of freely moving cats. Brain Res 251:259-276[ISI][Medline].
Hobson JA, Stickgold R, Pace-Schott EF (1998) The neuropsychology of REM sleep dreaming. NeuroReport 9:R1-R14[ISI][Medline].
Honda T, Semba K (1994) Serotonergic synaptic input to cholinergic neurons in the rat mesopontine tegmentum. Brain Res 647:299-306[ISI][Medline].
Horner RL, Kubin L (1999) Pontine carbachol elicits multiple rapid eye movement sleep-like neural events in urethane-anaesthetized rats. Neuroscience 93:215-226[ISI][Medline].
Jones BE (1991) The role of noradrenergic locus coeruleus neurons and neighboring cholinergic neurons of the pontomesencephalic tegmentum in sleep-wake states. Prog Brain Res 88:533-543[Medline].
Kayama Y, Ohta M, Jodo E (1992) Firing of "possibly" cholinergic neurons in the rat laterodorsal tegmental nucleus during sleep and wakefulness. Brain Res 569:210-220[ISI][Medline].
Koyama Y, Hayaishi O (1994) Firing of neurons in the preoptic/anterior hypothalamic areas in rat: its possible involvement in slow wave sleep and paradoxical sleep. Neurosci Res 19:31-38[ISI][Medline].
Leonard CS, Kerman I, Blaha G, Taveras E, Taylor B (1995) Interdigitation of nitric oxide synthase-, tyrosine hydroxylase-, and serotonin-containing neurons in and around the laterodorsal and pedunculopontine tegmental nuclei of the guinea pig. J Comp Neurol 362:411-432[ISI][Medline].
Levine ES, Jacobs BL (1992) Neurochemical afferents controlling the activity of serotonergic neurons in the dorsal raphe nucleus: microiontophoretic studies in the awake cat. J Neurosci 12:4037-4044[Abstract].
Lu J, Shiromani P, Saper CB (1999) Retinal input to the sleep-active ventrolateral preoptic nucleus in the rat. Neuroscience 93:209-214[ISI][Medline].
Lu J, Greco M, Shiromani P, Saper CB (2000) Effects of the lesions of the ventrolateral preoptic nucleus on NREM and REM sleep. J Neurosci 20:3830-3842[Abstract/Free Full Text].
Luppi PH, Aston-Jones G, Akaoka H, Chouvet G, Jouvet M (1995) Afferent projections to the rat locus coeruleus demonstrated by retrograde and anterograde tracing with cholera-toxin B subunit and Phaseolus vulgaris leucoagglutinin. Neuroscience 65:119-160[ISI][Medline].
Luppi PH, Gervasoni D, Peyron C, Rampon C, Barbagli B, Boissard R, Fort P (1999) Norepinephrine and REM sleep. In: Rapid eye movement sleep (Mallick BN, Inoue S, eds), pp 107-122. New Delhi, India: Narosa.
Maloney KJ, Mainville L, Jones BE (1999) Differential c-Fos expression in cholinergic, monoaminergic, and GABAergic cell groups of the pontomesencephalic tegmentum after paradoxical sleep deprivation and recovery. J Neurosci 19:3057-3072[Abstract/Free Full Text].
Maloney KJ, Mainville L, Jones BE (2000) c-Fos expression in GABAergic, serotonergic, and other neurons of the pontomedullary reticular formation and raphe after paradoxical sleep deprivation and recovery. J Neurosci 20:4669-4679[Abstract/Free Full Text].
Marks GA, Birabil CG (1998) Enhancement of rapid eye movement sleep in the rat by cholinergic and adenosinergic agonists infused into the pontine reticular formation. Neuroscience 86:29-37[ISI][Medline].
Merchant-Nancy H, Vazquez J, Garcia F, Drucker-Colin R (1995) Brain distribution of c-fos expression as a result of prolonged rapid eye movement (REM) sleep period duration. Brain Res 681:15-22[ISI][Medline].
Miller AM, Obermeyer WH, Behan M, Benca RM (1998) The superior colliculus-pretectum mediates the direct effects of light on sleep. Proc Natl Acad Sci USA 95:8957-8962[Abstract/Free Full Text].
Nitz D, Siegel J (1997a) GABA release in the dorsal raphe nucleus: role in the control of REM sleep. Am J Physiol 273:R451-R455[Abstract/Free Full Text].
Nitz D, Siegel JM (1997b) GABA release in the locus coeruleus as a function of sleep/wake state. Neuroscience 78:795-801[ISI][Medline].
Osaka T, Matsumura H (1994) Noradrenergic inputs to sleep-related neurons in the preoptic area from the locus coeruleus and the ventrolateral medulla in the rat. Neurosci Res 19:39-50[ISI][Medline].
Paxinos G, Watson C (1986) In: The rat brain in stereotaxic coordinates. San Diego: Academic.
Reiner PB, McGeer EG (1987) Electrophysiological properties of cortically projecting histamine neurons of the rat hypothalamus. Neurosci Lett 73:43-47[ISI][Medline].
Rye DB, Saper CB, Lee HJ, Wainer BH (1987) Pedunculopontine tegmental nucleus of the rat: cytoarchitecture, cytochemistry, and some extrapyramidal connections of the mesopontine tegmentum. J Comp Neurol 259:483-528[ISI][Medline].
Sakai K (1986) Central mechanisms of paradoxical sleep. Brain Dev 8:402-407[Medline].
Sakai K, Koyama Y (1996) Are there cholinergic and non-cholinergic paradoxical sleep-on neurones in the pons? NeuroReport 7:2449-2453[ISI][Medline].
Sastre JP, Buda C, Kitahama K, Jouvet M (1996) Importance of the ventrolateral region of the periaqueductal gray and adjacent tegmentum in the control of paradoxical sleep as studied by muscimol microinjections in the cat. Neuroscience 74:415-426[ISI][Medline].
Semba K, Fibiger HC (1992) Afferent connections of the laterodorsal and the pedunculopontine tegmental nuclei in the rat: a retro- and antero-grade transport and immunohistochemical study. J Comp Neurol 323:387-410[ISI][Medline].
Semba K, Reiner PB, Fibiger HC (1990) Single cholinergic mesopontine tegmental neurons project to both the pontine reticular formation and the thalamus in the rat. Neuroscience 38:643-654[ISI][Medline].
Shen H, Semba K (1994) A direct retinal projection to the dorsal raphe nucleus in the rat. Brain Res 635:159-168[ISI][Medline].
Sherin JE, Shiromani PJ, McCarley RW, Saper CB (1996) Activation of ventrolateral preoptic neurons during sleep. Science 271:216-219[Abstract].
Sherin JE, Elmquist JK, Torrealba F, Saper CB (1998) Innervation of histaminergic tuberomammillary neurons by GABAergic and galaninergic neurons in the ventrolateral preoptic nucleus of the rat. J Neurosci 18:4705-4721[Abstract/Free Full Text].
Shiromani PJ, Kilduff TS, Bloom FE, McCarley RW (1992) Cholinergically induced REM sleep triggers Fos-like immunoreactivity in dorsolateral pontine regions associated with REM sleep. Brain Res 580:351-357[ISI][Medline].
Shiromani PJ, Malik M, Winston S, McCarley RW (1995) Time course of Fos-like immunoreactivity associated with cholinergically induced REM sleep. J Neurosci 15:3500-3508[Abstract].
Steininger TL, Wainer BH, Blakely RD, Rye DB (1997) Serotonergic dorsal raphe nucleus projections to the cholinergic and noncholinergic neurons of the pedunculopontine tegmental region: a light and electron microscopic anterograde tracing and immunohistochemical study. J Comp Neurol 382:302-322[Medline].
Steininger TL, Gong H, McGinty D, Szymusiak R (2001) Subregional organization of preoptic area /anterior hypothalamic projections to arousal-related monoaminergic cell groups. J Comp Neurol 429:638-653[ISI][Medline].
Szymusiak R, Alam N, Steininger TL, McGinty D (1998) Sleep-waking discharge patterns of ventrolateral preoptic/anterior hypothalamic neurons in rats. Brain Res 803:178-188[ISI][Medline].
Thakkar MM, Portas C, McCarley RW (1996) Chronic low-amplitude electrical stimulation of the laterodorsal tegmental nucleus of freely moving cats increases REM sleep. Brain Res 723:223-227[ISI][Medline].
Thakkar MM, Strecker RE, McCarley RW (1998) Behavioral state control through differential serotonergic inhibition in the mesopontine cholinergic nuclei: a simultaneous unit recording and microdialysis study. J Neurosci 18:5490-5497[Abstract/Free Full Text].
Torterolo P, Yamuy J, Sampogna S, Morales FR, Chase MH (2001) GABAergic neurons of the laterodorsal and pedunculopontine tegmental nuclei of the cat express c-fos during carbachol-induced active sleep. Brain Res 892:309-319[Medline].
Vrontakis ME, Peden LM, Duckworth ML, Friesen HG (1987) Isolation and characterization of a complementary DNA (galanin) clone from estrogen-induced pituitary tumor messenger RNA. J Biol Chem 262:16755-16758[Abstract/Free Full Text].
Wang QP, Ochiai H, Nakai Y (1992) GABAergic innervation of serotonergic neurons in the dorsal raphe nucleus of the rat studied by electron microscopy double immunostaining. Brain Res Bull 29:943-948[ISI][Medline].
Webster HH, Jones B (1988) Neurotoxic lesions of the dorsolateral pontomesencephalic tegmentum-cholinergic cell area in the cat. II. Effects upon sleep-waking states. Brain Res 458:285-302[ISI][Medline].
Xi M-C, Morales FR, Chase MH (1999) A GABAergic pontine reticular system is involved in the control of wakefulness and sleep. Sleep Res Online 2:43-48[Medline].
Yamuy J, Sampogna S, Lopez-Rodriguez F, Luppi PH, Morales FR, Chase MH (1995) Fos and serotonin immunoreactivity in the raphe nuclei of the cat during carbachol-induced active sleep: a double-labeling study. Neuroscience 67:211-223[ISI][Medline].
Yamuy J, Sampogna S, Morales FR, Chase MH (1998) c-fos expression in mesopontine noradrenergic and cholinergic neurons of the cat during carbachol-induced active sleep: double-labeling study. Sleep Res Online 1:28-40[Medline].

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