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The Journal of Neuroscience, September 13, 2006, 26(37):9426-9433; doi:10.1523/JNEUROSCI.2012-06.2006
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Behavioral/Systems/Cognitive
Homeostatic Regulation of Sleep: A Role for Preoptic Area Neurons
Irma Gvilia,1,2,4 Feng Xu,1 Dennis McGinty,1,3 andRonald Szymusiak1,2 1Research Service, Veterans Affairs Greater Los Angeles Healthcare System, North Hills, California 91343, Departments of 2Medicine and 3Psychology, University of California, Los Angeles, California 90095, and 4I. Beritashvili Institute of Physiology, Tbilisi 0160, Georgia
Abstract
Top
Abstract
Introduction
The median preoptic nucleus (MnPN) and the ventrolateral preoptic area (vlPOA) contain putative sleep-regulatory neurons that exhibit elevated discharge rates during sleep compared with waking. Expression of c-Fos protein immunoreactivity (IR) in GABAergic neurons in the MnPN and the vlPOA is high in spontaneously sleeping rats and in rats undergoing recovery sleep after sleep deprivation. However, it is unclear whether c-Fos-IR in these neurons is evoked by increases in sleep pressure or by increases in sleep amount. We examined c-Fos-IR in MnPN and vlPOA neurons under experimental conditions that dissociated homeostatic sleep pressure, sleep amount, and time of day. Groups of rats with strong diurnal rhythms in sleep-wake organization were killed after (1) spontaneous sleep in the light, (2) spontaneous sleep in the dark, (3) sleep deprivation (SLD) in the light and (4) recovery sleep after SLD in the light. Numbers of GABAergic neurons expressing c-Fos-IR in the MnPN were significantly higher after SLD in the light compared with spontaneous sleep and recovery sleep in the light. In contrast, Fos-IR in vlPOA GABAergic neurons was most prevalent after spontaneous sleep and recovery sleep in the light. No light–dark differences in Fos-IR were observed in the MnPN after SLD in groups of rats with weak or absent diurnal sleep-waking rhythms. Our findings define potential roles for MnPN and vlPOA GABAergic neurons in homeostatic aspects of sleep regulation.
Key words: sleep deprivation; non-REM sleep; ventrolateral preoptic area; median preoptic nucleus; GABA; sleep diurnality
Introduction
The median preoptic nucleus (MnPN) and the ventral lateral preoptic area (vlPOA) of the hypothalamus contain sleep-active neurons. Both the MnPN and the vlPOA exhibit sleep-associated c-Fos protein immunoreactivity (Fos-IR) (Sherin et al., 1996, 1998
Original studies on functional mapping of Fos-IR reported low levels of Fos-positive neurons in the MnPN of rats that were sleep deprived compared with spontaneously sleeping rats (Gong et al., 2000
Little is known about specific neuronal systems that regulate homeostatic aspects of sleep control. The goal of the present study was to evaluate a hypothesis that activation of GABAergic neurons in the MnPN and vlPOA is associated with increasing homeostatic sleep drive/pressure and not with increasing sleep amount. Patterns of c-Fos-IR were compared among groups of rats exhibiting different levels of sleep pressure and different amounts of sleep. Experiment 1 used groups of rats with inherently strong diurnal rhythms in sleep-waking organization, with the assumption that such rats have comparatively high homeostatic sleep pressure during the light/rest period compared with the dark/active phase. Experiment 2 used rats with inherently weak diurnal rhythms in the distribution of sleep and waking, with the assumption that homeostatic sleep pressure in such rats is similar during the light and dark periods. Results indicate that MnPN GABAergic neurons are most strongly activated in response to increasing sleep pressure, whereas vlPOA GABAergic neurons are most strongly activated in response to increasing sleep amount.
Materials and Methods
All experiments were approved by the Animal Care and Use Committee at the Veterans Affairs Greater Los Angeles Health Care System and were conducted according to the guidelines of the National Research Council.Animals and experimental environment
Thirty-three male Sprague Dawley rats, weighing 280–320 g at the beginning of the experiments, were acclimated to a 12 h light/dark cycle (lights on at 8:00 A.M.). The rats were housed individually in environmental chambers. Food and water were available ad libitum and the ambient temperature was maintained at 23 ± 0.5°C.Surgical procedures and recording
Under ketamine/xylazine anesthesia (80/10 mg/kg, i.p.), rats were surgically implanted with chronic cortical electroencephalogram (EEG) and dorsal neck electromyogram (EMG) electrodes for assessment of sleep-wakefulness states. Briefly, stainless steel screw electrodes were implanted in the skull for EEG recordings and flexible insulated stainless steel wires were threaded into neck muscles for EMG recordings. Leads from the electrodes were soldered to a small Amphenol connector and the complete assembly was anchored to the skull with dental acrylic.On the 8th–13th days after surgery, animals were connected to a recording cable that was lightly suspended above them by a counter–weighted beam and were adapted to the recording procedure for 5–6 h (beginning at 8:00 A.M.) each day. During experiments, EEG and EMG signals were recorded continuously using a polysomnographic recording device (Embla; Medcare Flaga Medical Devices, Reykjavik, Iceland). The EEG and EMG signals were digitally displayed and stored on a computer using Somnologica software (Somnologica Studio; Medcare Flaga Medical Devices).
Experimental paradigm
On the 14th day after surgery, all rats (n = 33) were recorded for 24 h to determine baseline diurnal organization of sleep and waking. Rats (n = 24) exhibiting60% sleep during the light period and
30% sleep in the dark were assigned for experiment 1, whereas rats (n = 9) with weaker diurnal rhythms in sleep and waking were assigned for experiment 2. All other experimental recordings described below were conducted on the 15th day after surgery.
Experiment 1. One group of rats (n = 6) was allowed 2 h spontaneous sleep and waking during the light period (ZT1–3). A second group of rats (n = 6) was allowed 2 h spontaneous sleep-waking behavior during the dark period (ZT13–15). A third group of rats (n = 12) was subjected to 2 h sleep deprivation during the light period (ZT1–3) and then divided into two subgroups: rats (n = 6) that were killed right after the termination of the deprivation procedure and rats (n = 6) that were allowed 1 h recovery sleep after the deprivation. To interrupt sleep episodes, rats were subjected to gentle arousing stimuli (tapping on the cage and/or slight movement of the cage) within 3–5 s of the first appearance of EEG signs of sleep. Animals were adapted to the sleep deprivation procedures on the 5th–13th postsurgical days, by exposing them to the stimuli used to interrupt sleep for several 5–10 min periods each day, between 8:00 A.M. and 3:00 P.M.
Experiment 2. A group of nine rats, exhibiting a weak diurnal rhythm in sleep-waking organization, was subjected to 2 h sleep deprivation during either the light period (ZT1–3; n = 5) or in the dark period (ZT13–15; n = 4). Immediately after the end of all recordings, rats were given a lethal dose of anesthetic followed by perfusion.
Immunohistochemistry
Under deep pentobarbital anesthesia (100 mg/kg), animals were transcardially perfused with 0.12 M Millonig’s phosphate buffer (MPB) for 5 min, followed by 500 ml of 4% paraformaldehyde (PFA) in 0.12 M MPB. After perfusion, the bodies of the perfused animals were kept at 4°C for 1 h. The brains were then removed, postfixed in the same PFA solution for 1 h, washed in 0.12 M MPB and transferred successively to 10, 20, and 30% sucrose at 4°C until they sank. Brain tissue was processed for double immunostaining for Fos, the protein product of the immediate-early gene c-fos (Morgan and Curran, 1986Data analysis
Sleep analysis. Sleep-wakefulness states of the rats were determined by an experienced scorer on the basis of the predominate state within each 10 s epoch. The scorer was blind to experimental condition and group identity of the animal. Wakefulness was defined by the presence of low-amplitude and high-frequency EEG activity combined with elevated neck muscle tone. Non-REM sleep consisted of a high-amplitude slow-wave EEG together with a low-EMG tone relative to wakefulness. REM sleep was identified by the presence of a moderate-amplitude EEG with dominant theta-frequency activity coupled with minimal neck EMG tonus except for occasional brief twitches.During sleep deprivation, sleep pressure was defined by counting the number of sleep entries within the experimental procedure. To track the accumulation of sleep pressure, the number of sleep entries in each animal was averaged per consecutive 10 min interval of the 2 h sleep deprivation period.
Cell counts. Cell counts were conducted by an individual who was blind to the experimental condition of the animals. The Neurolucida computer-aided plotting system (MicroBrightField, Williston, VT) was used to identify and quantify neurons that were single labeled for c-Fos-IR and double-labeled for Fos plus GAD-IR. Section outlines were drawn under 20x magnification. Fos IRNs and Fos plus GAD IRNs were mapped in the section outlines under 400x magnification. All cell counts were calculated for constant rectangular grids corresponding to four areas of interest. (1) The rostral MnPN (rMnPN) grid was a 600 x 600 µm square, centered on the apex of the third ventricle rostral to the decussation of the anterior commissure and to bregma (anterior, 0.1 mm) (Gong et al., 2000
For both the rMnPN and the cMnPN, cell counts were made in three sections and averaged to yield a single value for each rat. For vlPOA, cell counts were made bilaterally in three sections containing the largest part of the vlPOA. Those six counts were then averaged to yield a single value for both the vlPOA core and extended vlPOA (medial and dorsal sections combined) for each rat.
Statistical analysis. All results are reported as mean ± SEM. One-way nonrepeated-measures ANOVA was calculated for behavioral stage percentages across animals that were allowed spontaneous sleep-waking behavior during the light period and in the dark and the light sleep-deprived rats (Table 1). A similar ANOVA was calculated for the number of attempts to enter into sleep across all groups of sleep-deprived (light SLD, experiment 1; light SLD, experiment 2; and dark SLD, experiment 2) rats (Table 2).
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Table 1. Percentage of time spent in wakefulness, REM sleep, and non-REM sleep and mean numbers of non-REM sleep onsets
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Table 2. Mean numbers of attempts to enter into sleep during sleep deprivation periods and mean numbers of single Fos-IR and Fos plus GAD double IR neurons
For single Fos-IR cell counts in MnPN and vlPOA sites across all four groups of experiment 1, a one-way nonrepeated-measures ANOVA was calculated (Figs. 5A, 6A). A similar ANOVA was calculated for Fos plus GAD IRNs in MnPN and vlPOA sites across the same groups of rats (Figs. 5B, 6B) and for Fos-IR cell counts across all groups of sleep-deprived rats (See Table 2). After all ANOVAs, significance of the differences between individual group means was assessed by Newman–Keuls post hoc tests.
Results
Experimental rats (n = 33) showed different profiles of their sleep-waking diurnal organization estimated by percentage time spent in sleep during the light/rest period versus the dark/active period. A large group of rats (n = 24) exhibited strong diurnal rhythms in sleep amounts during 24 h baseline recordings; mean percentage of sleep time during the light period was 64.87 ± 1.6%, whereas the percentage of sleep time during the dark period was 26.99 ± 3.0%. These 24 rats were the subjects for experiment 1. Nine rats did not exhibit diurnality in sleep-waking behavior during 24 h baseline recordings; the mean percentage of sleep time during the light period (50.4 ± 2.6) was not significantly different from the percentage of sleep time during the dark period (47.35 ± 1.9%). These rats were the subjects for experiment 2. Figure 1 presents mean sleep-waking amounts during 24 h baseline recordings for six rats exhibiting strong diurnal rhythms in sleep-waking (A) and six rats exhibiting weak or absent diurnal rhythms in sleep and waking (B).
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Figure 1. Mean percentages of time spent in waking, non-REM sleep, and REM sleep during 24 h baseline recordings for six rats exhibiting strong diurnal organization of sleep and wakefulness that were assigned to experiment 1 (A) and six rats exhibiting weak diurnal organization of sleep and wakefulness that were assigned to experiment 2 (B).
Experiment 1
Rats (n = 6) that were allowed spontaneous sleep and waking during the dark period manifested low percentage of sleep (8.8 ± 3.4%) during 1 h before death whereas the light period recorded rats (n = 6) exhibited 73.7 ± 2.6% sleep (Table 1, Fig. 2A,B). Sleep-deprived rats accumulated 5.6 ± 1.4% of non-REM sleep and no REM sleep during the deprivation period (Table 1, Fig. 2C). Rats (n = 6) that were allowed a 1 h of recovery sleep after sleep deprivation during the light period exhibited 88.9 ± 1.3% sleep (Table 1, Fig. 2D).
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Figure 2. Examples of sleep-waking organization during the last 1 h period before killing and brain tissue harvest in representative animals from experiment 1. A, Spontaneous sleep-waking during the dark period. B, Spontaneous sleep-waking during the light period. C, Sleep deprivation in the light period. D, Recovery sleep after sleep deprivation during the light period. W, Waking; NREM, non-REM sleep.
All sleep-deprived rats (n = 12) manifested evidence of gradual elevation of sleep pressure; the number of sleep entries progressively increased within the deprivation period (Fig. 3). Both total sleep time and the number of sleep onsets were significantly elevated in 1 h recovery sleep animals compared with animals exhibiting spontaneous sleep in the light (Table 1). Rebound increases in these measures during recovery sleep provide further evidence that sleep pressure was elevated at the end of the 2 h sleep deprivation period.
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Figure 3. Average numbers of attempts to enter sleep during consecutive 10 min intervals across 2 h periods of total sleep deprivation for rats with different patterns of baseline sleep-waking diurnal organization. A, Sleep deprivation during the light period in the condition of a strong diurnal rhythm in baseline sleep and waking (light SLD, experiment 1; n = 6). B, Sleep deprivation during the light period in the condition of a weak diurnal rhythm in baseline sleep and waking (light SLD, experiment 2; n = 5). C, Sleep deprivation during the dark period in the condition of a weak diurnal rhythm in baseline sleep-waking (dark SLD, experiment 2; n = 4)
Examples of the distribution of Fos- and Fos plus GAD-IR neurons in the MnPN and vlPOA for representative animals are shown in Figure 4. Mean numbers of single Fos-IR and Fos plus GAD double IR neurons in MnPN and vlPOA sites across all four groups of animals are shown in Figures 5 and 6. The numbers of Fos plus GAD double-IR neurons in rostral and caudal MnPN were highest in sleep-deprived rats that were not allowed a recovery sleep and lowest in rats permitted sleep during the dark cycle (Fig. 5B). In vlPOA sites, Fos plus GAD double-IR cell counts were highest in rats permitted sleep during the light period and sleep-deprived rats that were allowed recovery sleep after the deprivation (Fig. 6B). See Figures 5 and 6 and the accompanying legends for a summary of other between group differences.
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Figure 4. A–C', Line drawings showing distribution of Fos single-labeled and Fos plus GAD double-labeled neurons located in counting grids for the rostral MnPN and vlPOA sites, including the vlPOA cluster and extended vlPOA, from dark-sleeping (A, A’), light-sleeping (B, B’), and light sleep-deprived (C, C’) rats. D, Examples of Fos single-labeled (filled arrowhead), GAD single-labeled (open arrow), and Fos plus GAD double-labeled (filled arrow) neurons in the MnPN of a light-sleeping rat. The Fos protein is stained black and confined to the nucleus. The GAD IRNs are stained brown, and the staining is evident throughout the soma and the proximal dendrites.
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Figure 5. Mean numbers of Fos IRNs (A) and Fos plus GAD IRNs (B) in rMnPN and cMnPN, respectively, across all four groups of rats from experiment 1. For single Fos-IR cell counts in the MnPN, ANOVA indicated significant effects of experimental conditions in both the rostral (F(3,20) = 59.57; p < 0.001) and caudal (F(3,20) = 50.28; p < 0.001) portions of the MnPN. There were significant effects of experimental conditions for double Fos plus GAD-IR cell counts in both rostral (F(3,20) = 56.15; p < 0.001) and caudal MnPN (F(3,20) = 41.37; p < 0.001). Individual group mean differences as determined by post hoc tests (Newman–Keuls) are indicated by asterisks (*p < 0.01; **p < 0.001).
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Figure 6. Mean numbers of Fos IRNs (A) and Fos plus GAD IRNs (B) in vlPOA cluster and extended vlPOA, respectively, across all four groups of experiment 1. For single Fos-IR cell counts in the vlPOA, ANOVA indicated significant effects of experimental conditions in both the vlPOA cluster (F(3,20) = 11.37; p < 0.001) and extended vlPOA (F(3,20) = 22.35; p < 0.001). There were significant effects of experimental conditions for double Fos plus GAD-IR cell counts in both the vlPOA cluster (F(3,20) = 11.51; p < 0.001) and extended vlPOA (F(3,20) = 26.99; p < 0.001). Individual group mean differences as determined by post hoc tests (Newman–Keuls) are indicated by asterisks (*p < 0.01; **p < 0.001).
Experiment 2
Light-sleep deprived (n = 5) and dark-sleep deprived (n = 4) rats exhibited similar degrees of sleep homeostatic pressure estimated by total numbers of sleep entries within the experimental period (Table 2). As shown, the number of attempts to initiate sleep in these two groups of rats was significantly lower compared with the number of sleep attempts in rats that were sleep-deprived during the light/rest period in experiment 1. However, sleep-deprived rats in experiment 2 manifested evidence of gradual accumulation of sleep pressure; the number of required awakenings progressively increased within the deprivation period (Fig. 3).The numbers of single Fos-IR and Fos plus GAD double-IR neurons in the MnPN of light-sleep and dark-sleep deprived rats in experiment 2 were not significantly different, but values were lower than those for rats that were subjected to deprivation during the light period under the condition of a strong diurnal rhythm in baseline sleep and waking (Table 2).
Discussion
Neuronal substrates underlying homeostatic aspects of sleep regulation are poorly defined. We report for the first time that GABAergic neurons in the MnPN exhibit maximal expression of Fos-IR in situations of high homeostatic sleep need accompanied by minimal sleep (i.e., in response to sleep deprivation during the light/rest period) (Fig. 5B). In contrast, vlPOA GABAergic neurons exhibit maximal Fos-IR during recovery sleep and spontaneous sleep in the light (Fig. 6B). These results identify a potential mechanistic role for MnPN GABAergic neurons in homeostatic sleep regulation.Across the several conditions studied in experiments 1 and 2, dissociation of sleep pressure, sleep amount, and time of day were achieved. In experiment 1, Fos-IR in MnPN GABAergic neurons was lowest during spontaneous sleep in the dark, a condition of low sleep pressure and low sleep amount. However, in a condition of high sleep pressure and minimal sleep (sleep deprivation in the light period), Fos-IR in MnPN GABAergic neurons was maximal. In two conditions of high sleep amount, spontaneous sleep and recovery sleep in the light, Fos-IR in MnPN GABAergic neurons was higher in the condition with higher sleep pressure (i.e., recovery sleep). Collectively, these results demonstrate that activation of MnPN GABAergic neurons varies along the dimension of increasing sleep pressure.
Fos-IR in vlPOA GABAergic neurons was significantly higher during both spontaneous sleep and recovery sleep, compared with sleep deprivation (Fig. 6). This agrees with previous reports that Fos-IR in vlPOA neurons does not increase after sleep deprivation unless animals are permitted recovery sleep (Sherin et al.1996), and that sleep-related discharge of vlPOA neurons is elevated after 16 h of sleep deprivation, whereas waking-related discharge rates are unchanged (Szymusiak et al., 1998
Reduced Fos-IR in MnPN neurons during spontaneous sleep in the dark versus the light period is interpreted by us to reflect low sleep pressure during the dark period. Alternatively, low Fos-IR cell counts in the dark could be a consequence of light–dark modulation of c-fos expression in this nucleus. However, results of experiment 2 do not support such an explanation. Rats with weak diurnal rhythms exhibited similar levels of sleep pressure, defined by the number of attempts to initiate sleep, during SLD in the light period and SLD in the dark period (Table 2). That Fos plus GAD-IR cell counts did not differ in these two conditions (Table 2) is evidence that in the absence of diurnal variation in sleep pressure, no strong light–dark rhythm of c-fos expression is evident in MnPN neurons.
We previously reported low levels of Fos-IR in the MnPN after 2 h of sleep deprivation in the light period (Gong et al., 2000
It has been reported that more MnPN GABAergic neurons express Fos-IR after 3 h of recovery sleep compared with 3 h of sleep deprivation (Modirrousta et al., 2004
We reported previously that neurons in the MnPN and vlPOA express c-Fos-IR under conditions of increasing REM sleep homeostatic pressure (Gvilia et al., 2006
Studies of sleep-related neuronal discharge suggest different functional roles for vlPOA and MnPN neurons in sleep regulation, consistent with the results of Fos-IR studies reported here. Most sleep-active vlPOA neurons display increased activity during the immediate transition from waking to sleep and become progressively activated from light to deep non-REM sleep (Szymusiak et al., 1998
Anatomical and physiological evidence suggests that MnPN and vlPOA neurons function to promote sleep via descending inhibitory modulation of arousal systems located in the posterior hypothalamus and brainstem. The vlPOA heavily innervates wake-promoting histaminergic neurons in the tuberomammillary nucleus (TMN) (Sherin et al., 1996
The factor(s) responsible for activation of MnPN neurons during sleep deprivation and of vlPOA neurons during recovery sleep are unknown. The endogenous somnogen adenosine has been implicated in homeostatic sleep regulation and may play a role in regulating changes in vlPOA and MnPN neuronal activity in response to sustained wakefulness. Adenosine disinhibits vlPOA neurons in vitro via A1 adenosine receptors (Chamberlin et al., 2003
(IL-1
Footnotes
Received May 10, 2006; revised July 20, 2006; accepted Aug. 7, 2006.This work was supported by the Medical Research Service of the Department of Veterans Affairs and National Institutes of Health Grants MH63323 and HL60296. We thank Keng-Tee Chew and Bryan Angara for technical assistance.
Correspondence should be addressed to either Ronald Szymusiak or Irma Gvilia, Research Service (151A3), Veterans Affairs Greater Los Angeles Healthcare System, 16111 Plummer Street, North Hills, CA 19343. Email: rszym{at}ucla.edu or Email: irmagvilia{at}hotmail.com
Copyright © 2006 Society for Neuroscience 0270-6474/06/269426-08$15.00/0
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