Sleep and Sleep Regulation in Normal and Prion Protein-Deficient Mice

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Volume 17, Number 5, Issue of March 1, 1997 pp. 1869-1879
Copyright ©1997 Society for Neuroscience

Sleep and Sleep Regulation in Normal and Prion Protein-Deficient Mice

Irene Tobler¹, Tom Deboer¹, and Marek Fischer²
Institutes of ¹ Pharmacology and ² Molecular Biology, University of Zürich, CH-8057 Zürich, Switzerland

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Mice are the preferred mammalian species for genetic investigations of the role of proteins. The normal function of the prionprotein (PrP) is unknown, although it plays a major role in theprion diseases, including fatal familial insomnia. We investigatedits role in sleep and sleep regulation by comparing baseline recordingsand the effects of sleep deprivation in PrP knockout mice (129/SV)and wild-type controls (129/SV × C57BL/6), which are the miceused for most gene targeting experiments and whose behavior isnot well characterized. Although no difference was evident inthe amount of vigilance states, the null mice exhibited a largerdegree of sleep fragmentation than the wild-type with almost doublethe amount of short waking episodes. As in other rodents, corticaltemperature closely reflected the time course of waking. The increaseof slow-wave activity (SWA; mean EEG power density in the 0.25-4.0Hz range) at waking to nonrapid eye movement (NREM) sleep transitionswas faster and reached a lower level in the null mice than inthe wild-type. The contribution of the lower frequencies (0.25-5.0Hz) to the spectrum was smaller than in other rodents in all threevigilance states, and the distinction between NREM sleep and REMsleep was most marked in the theta band. After the sleep deprivation,SWA was increased, but the changes in EEG power density and SWAwere more prominent and lasted longer in the PrP-null mice. Ourresults suggest that PrP plays a role in promoting sleep continuity.
Key words: prion protein; mice; sleep; sleep regulation; EEG spectral analysis; sleep deprivation; brain temperature; knockout mice; transgenic mice

INTRODUCTION

The genetic factors determining sleep are still unresolved, although in mice several sleep variables appear to be inherited(Valatx et al., 1972, 1980; Friedman, 1974; Valatx and Bugat,1974; Cespuglio et al., 1975). Gene targeting allows a selectiveapproach to investigate inheritance (Capecci, 1994) and is usuallyperformed in the inbred mouse strain "129" backcrossed with C57BL(Gerlai, 1996). The behavior of the mouse strains and their hybrids,including sleep, needs to be characterized (Crawley, 1996) toprovide a basis for the investigation of sleep in mice subjectedto gene targeting.

Prion protein (PrP) gene mutations lead to prion diseases including fatal familial insomnia (FFI) (Lugaresi et al., 1986;Goldfarb et al., 1991; Galassi et al., 1992; Medori et al., 1992;Monari et al., 1994; Aguzzi and Weissmann, 1996). In FFI, thereis a severe reduction of sleep, a gradual disappearance of spindleactivity in the sleep EEG (Gambetti et al., 1995; Reder et al.,1995; Sforza et al., 1995), and a disruption of hormone rhythms(Portaluppi et al., 1994, 1995; Montagna et al., 1995). The mainneurological features include hypometabolism, loss of neurons,and astrogliosis, with the first and most severe neuropathologyappearing in the thalamus (Gambetti et al., 1995). Thus, PrP maybe important for sleep regulation, because the thalamus is implicatedin the regulation of sleep spindles and EEG slow waves (Steriadeet al., 1993). PrP is a glycoprotein localized on neuronal membranesand in astrocytes (Collinge et al., 1994; Moser et al., 1995)that may promote neuronal cell differentiation and maintain neuronalfunction (Clinton et al., 1993), but its function is not yet understood(Estibeiro, 1996). There are indications that the loss of thenatural PrP function may be responsible for the pathology in priondiseases (Collinge et al., 1995; Gambetti et al., 1995).

The investigation of the prion diseases and the normal function of PrP involved the generation of mice devoid of PrP (forreview, see Prusiner, 1991, 1996; Weissmann, 1996). They exhibitedno abnormal behavior or learning ability (Büeler et al., 1992;Manson et al., 1994), although ataxia and loss of Purkinje cellshave been observed in older mice with a larger deletion (Sakaguchiet al., 1996). Moreover, PrP may be necessary for synaptic functionand sleep and rhythm regulation, because long-term potentiationwas impaired (Collinge et al., 1994; Manson et al., 1995; Whittingtonet al., 1995), the period of circadian motor activity was morestabilized, and sleep fragmentation and the response to sleepdeprivation (SDEP) were more prominent in PrP-null mice (Tobleret al., 1996).

Our purpose was to compare in detail sleep in the hybrid mouse strain used for the deletion, with the PrP-deficient mice.Because SDEP has served to uncover differences in sleep regulationbetween species (Tobler, 1995), the effects of SDEP on the twogenotypes were compared.

MATERIALS AND METHODS
Animals. Adult mice devoid of prion protein (Prn-p^0/0) (Büeler et al., 1992) and wild-type controls (Prn-p^+/+; inbred strains C57BL-6J/129SV), mean age 80.6 ± 4.3 d (SEM)and weighing 26.69 ± 0.93 gm at the onset of recordings, servedas experimental animals. Both genotypes had a genetic backgroundderived from two inbred mouse strains, 129/SV (ev) backcrossedwith C57BL/6J (Bühler et al., 1992). In addition, three micetransgenic for the PrP protein (TG) were recorded. For their generation,a PrP minigene comprising 5.5 kb of the PrP promotor, exon 1,intron 1, exon 2, exon 3, and 2.3 kb of a 3 $'$ -nontranscribed sequencewas constructed and introduced into the germline of a Prn-p^+/0 mouse. Breeding with Prn-p^0/0 mice gave rise to transgenic mice that were TG^+/0;Prn-p^0/0 (line20) (Fischer et al., 1996). The mice were individually keptin Macrolon cages (36 × 20 × 35 cm) and placed in sound-attenuatedchambers. Food and water were available ad libitum. The animalswere maintained under a 12 hr light/dark cycle (light from 10:00A.M. to 10:00 P.M.; daylight-type fluorescent tubes, 18 W, ~150lux 5 cm above the floor level). The animals were adapted to theseconditions for a minimum of 3 weeks before the experiment. Meanvalues of ambient temperature continuously recorded for 4 secepochs in two of the four boxes was in the range of 21.8-22.4°Cduring the three recording days.

Surgery. EEG and EMG electrodes and an epidural thermistor were implanted under deep anesthesia (50 mg/kg pentobarbital sodium,i.p.). Two gold-plated, round-tipped miniature screws ( $phi$ = 1.19mm) served as EEG electrodes and were screwed through the skullonto the dura over the right cortex (2.0 mm lateral to the midline,3.5 mm posterior to bregma) and the cerebellum (at the midline,1.5 mm posterior to lambda). Two entwined wires ( $phi$ = 0.2 mm) wereinserted into the neck muscle tissue to record the EMG. A thermistor(Thermometrics, P20, R_(25°C) = 1 k $Omega$ , I_CONST. = 1 mA, maximum $phi$ = 0.5 mm) inserted between the skull and dura through a holein the skull over the left frontal cortex (the tip lying overthe occipital cortex) was used to measure cortical temperature(T_CRT). The electrodes and the thermistor were anchored to theskull with dental cement.

Experimental protocol and data acquisition. The mice were connected to counterbalanced recording leads for habituation atleast 8 d before the experiment. Three consecutive 24 hr recordingsof the EEG, EMG, and T_CRT were obtained. The first 2 d servedas baseline (1 Prn-p^+/+ mouse was recorded for 1 baseline only), and on day 3 the micewere subjected to 6 hr SDEP and recorded for the remaining 18hr. Sleep deprivation began at light onset and was attained bydisturbing the animals acoustically and by introducing objectsinto the cage whenever the animals looked drowsy, attempted toengage in a sleeping posture, or the EEG showed signs of low-frequencyactivity. The EEG and EMG signals were amplified (amplificationfactor ~ 2000), conditioned by analog filters (high-pass filter: $-$ 3 dB at 0.016 Hz; low-pass filter: $-$ 3 dB at 40 Hz; less than $-$ 35 dB at 128 Hz), sampled with 256 Hz, digitally filtered (EEG:low-pass filter FIR filter 25 Hz; EMG: band-pass FIR filter 20-50Hz), stored with a resolution of 128 Hz, and displayed on a PCmonitor. Subsequently, EEG power spectra were computed for consecutive4 sec epochs by an FFT routine within the frequency range of 0.25-25.0Hz (between 0.25 and 5.0 Hz, the values were collapsed into 0.5Hz bins, between 5.25 and 25.0 Hz into 1 Hz bins). The amplifiedEMG signal was AD-converted, full-wave-rectified, and integratedover 4 sec epochs. T_CRT and the ambient temperature inside thechambers were recorded at 4 sec intervals. All data were recordedsimultaneously and stored on optical disks. Before the beginningof the recordings, a calibration signal (10 Hz sine wave, 300µV_PP) was recorded on the EEG channels.

Vigilance states and analysis. The vigilance states were determined as follows. For each epoch, the EEG power density in thedelta (0.75-4.0 Hz) and theta band (6.25-9.0 Hz), the integratedEMG value, and T_CRT were displayed on a PC monitor. Three vigilancestates $---$ (1) waking (high EMG and low EEG amplitude and high thetaactivity concomitant with highest EMG values), (2) NREM sleep(low EMG and high EEG amplitude, high delta activity), and (3)REM sleep (low EMG and low EEG amplitude, high theta activity) $---$ weredetermined for 4 sec and the scores were entered into the PC viathe keyboard. Epochs the vigilance state of which could not beidentified, and epochs containing two different vigilance stateswithin a 4 sec epoch, were given the score of the predominantstate but not used for spectral analysis (0.18 ± 0.05%). Epochscontaining EEG artifacts were marked and omitted from furtheranalysis of the power spectra (6.55 ± 0.91% of total recordingtime). The vigilance states were expressed as a percentage ofartifact-free recording time.

To allow the comparison of the duration and frequency of episodes with other rodents, the same minimal interruption criteriawere applied as used previously for the rat and Djungarian hamster(Franken et al., 1991; Deboer et al., 1994). The algorithm isbased on the frequency and the duration of episode interruptions.

Differences between the baselines and between baseline 2 and recovery from SDEP were compared by t tests. Overall effectson the 2 hr mean values within a genotype were analyzed by two-wayANOVA with the factors Time (2 hr intervals) and Condition (baseline2 vs recovery). Whenever significant effects were present, contrastswere assessed by t tests. The 2 hr spectral values of the recoveryday were expressed for each individual relative to the corresponding2 hr reference value of baseline 2, and statistics were performedafter log transformation. Comparisons between Prn-p^+/+ and Prn-p^0/0 were performed by post hoc t tests and Bonferroni correctionsfor multiple tests if significance was reached in an ANOVA forthe factor Genotype or interaction Genotype × Interval. To avoidmultiple tests, the 2 hr intervals and the 30 frequency bins werecomprised to 6 or 12 hr values and three frequency bands, respectively.

RESULTS

Baseline vigilance states, T_CRT, and slow-wave activity
All mice exhibited a marked diurnal preference for sleep (Figs. 1, 2; Table 1), and no significant difference was found betweenbaseline 1 and 2 within either genotype. The mice spent ~70% ofthe light period in sleep, and a considerable amount occurredalso in the dark period (30%). The Prn-p^0/0 mice did not differ from the wild-type in the 24 hr values ofthe baseline vigilance states (Table 1, Fig. 2), with the exceptionof a higher value for REM sleep per total sleep time (TST) inthe Prn-p^0/0 mice (Table 1). A difference in the distribution of waking andNREM sleep was apparent only in the second half of the dark period,in which waking was more prominent and NREM sleep lower in thePrn-p^0/0 mice in both baselines (Fig. 2, Table 2). REM sleep was moreabundant in the first half of the dark period in the null mice.In all mice, REMS/TST exhibited a minor, significant increasein the course of the light period (data not shown).
Fig. 1. Individual 24 hr sleep and brain temperature records of the two genotypes. Individual 3 d records (baseline 1, baseline 2,and day 3 consisting of sleep deprivation and recovery) of a wild-type(Prn-p^+/+) and a prion protein-deficient mouse (Prn-p^0/0). Cortical temperature (T_CRT), slow-wave activity (SWA; EEG powerdensity 0.75-4.0 Hz) in NREM sleep (N), and the vigilance stateswaking (W), N, and REM sleep (R). The bars at the top mark the12 hr light/dark cycle. The calibration mark on the left correspondsto 50 µV².
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Fig. 2. Distribution of the vigilance states and brain temperature across the two baselines. Vigilance states (W, waking; N, NREMsleep; R, REM sleep), slow-wave activity (SWA; power density 0.75-4.0Hz in N), and cortical temperature (T_CRT) for the 48 hr baselinerecording in Prn-p^+/+ and Prn-p^0/0 mice. Mean 2 hr values ± 2 SEM, n = 8 for each strain (1 Prn-p^+/+ mouse contributed with 1 baseline). ANOVA factor "genotype" (Prn-p^+/+ vs Prn-p^0/0) was not significant for all 12 and 24 hr variables.
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Table 1. Vigilance states in the two baselines

WAKING
NREMS
REMS
TST
REMS/TST

Light Dark Light Dark Light Dark Light Dark Light Dark

Prn-p^+/+

BL1 33.6 64.3 54.5 30.8 11.8 4.9 66.4 35.7 17.8 13.8

(2.1) (2.7) (1.9) (2.5) (0.9) (0.5) (2.1) (2.8) (1.2) (1.2)

BL2 31.3 64.4 57.3 30.8 11.4 4.8 68.7 35.6 16.5 13.9

(1.4) (3.8) (1.6) (3.5) (0.9) (0.5) (1.4) (3.8) (1.3) (1.3)

Prn-p^0/0

BL1 32.3 66.6 54.4 27.5 13.3 5.9 67.7 33.4 19.6 17.8^*

(2.2) (1.7) (1.8) (1.5) (0.7) (0.4) (2.2) (1.7) (0.8) (1.3)

BL2 32.1 65.0 55.0 29.3 13.0 5.7 67.9 35.0 19.1 16.6

(2.6) (2.4) (2.1) (2.3) (0.7) (0.4) (2.6) (2.4) (0.7) (1.5)

Values are means ± SEM for the 12 hr intervals of the light and dark period; n = 8 for each strain (except for BL1 wild-type,where n = 7). BL1, BL2, Baselines 1 and 2; REMS, rapid eye movementsleep; NREMS, non-rapid eye movement sleep. REMS is also expressedas a percentage of total sleep time (REMS/TST). Comparisons BL1vs BL2 within each genotype, and Prn-p^+/+ vs Prn-p^0/0, were not significant for all variables, except for REMS/TSTin BL1, dark ( ^* p < 0.04 Prn-p^+/+ vs Prn-p^0/0; two-tailed t test). ANOVA factor "LD" within each genotype, p < 0.02 for each vigilance state.

Table 2. Vigilance states and cortical temperature for 6 h intervals

WAKING
NREMS
REMS
REMS/TST
T_CRT

Light Dark Light Dark Light Dark Light Dark Light Dark

Prn-p^+/+

Hours

BL2 0 -6 28.7 77.2 60.3 20.9 11.0 2.5 15.4 11.8 35.3 36.9

(2.1) (7.0) (2.0) (6.3) (1.9) (0.0) (1.2) (1.3) (0.2) (0.3)

7 -12 33.9 52.0 54.4 41.0 11.7 7.0 17.7 14.3 35.5 35.9

(1.0) (2.9) (1.5) (2.3) (1.0) (0.9) (1.5) (1.4) (0.2) (0.3)

SD+REC 0 -6 97.0 64.0 3.0 30.6 0.0 5.5 0.0 13.1 37.2^a 36.6

(0.9) (8.4) (0.9) (7.2) (0.0) (1.4) (0.0) (2.4) (0.2) (0.3)

7 -12 25.0 45.0 62.2 46.6 12.7 8.4 17.0 15.2 35.5 35.8

(1.7) (1.9) (1.6) (1.3) (1.1) (0.7) (1.4) (0.9) (0.2) (0.2)

Prn-p^0/0

Hours

BL2 0 -6 25.9 66.1 60.6 28.7 13.5 5.3^b 18.2 15.6 35.4 36.8

(3.2) (4.1) (2.6) (3.6) (0.8) (1.0) (0.6) (2.3) (0.1) (0.1)

7 -12 38.4 63.9^b 49.3 30.0^b 12.4 6.1 19.9 16.7 35.8 36.7^b

(4.1) (4.3) (3.2) (3.5) (1.1) (1.0) (1.2) (1.5) (0.1) (0.1)

SD+REC 0 -6 97.6 58.1 2.4 34.2 0.0 7.7 0.0 18.8 37.4^a 36.6

(0.5) (4.1) (0.5) (3.4) (0.0) (0.9) (0.0) (1.3) (0.1) (0.1)

7 -12 23.1 54.7 61.4 37.6 15.5^a 7.7 20.3^a 17.0 35.8 36.5

(1.9) (3.9) (1.8) (3.1) (0.4) (0.9) (0.6) (0.8) (0.1) (0.1)

Values are means ± SEM expressed as percentage of recording time; n = 8. Baseline 2 (BL2), sleep deprivation (SDEP), recovery(REC), REMS, rapid eye movement sleep; NREMS, non-rapid eye movementsleep. REMS, REM sleep is also expressed as a percentage of totalsleep time (REMS/TST). ^a p < 0.04 BL2 vs recovery within a genotype. ^bp < 0.04, Prn-p^+/+ vs Prn-p^0/0 (two-tailed t test).

Slow-wave activity (SWA) encompasses the frequency band between 0.75 and 4.0 Hz and is computed within NREM sleep, becausein this vigilance state slow waves are most prominent in mammals(Tobler, 1995). SWA in NREM sleep decreased progressively in thecourse of the 12 hr light period and increased in the dark, wheremost values were higher than in the light (Fig. 2). In the wild-typemice, a decrease of SWA began already in the second half of thedark period, reflecting the differences in waking and NREM sleepbetween the genotypes in this interval. The larger amount of NREMsleep in the wild-type mice allowed an earlier dissipation ofSWA, compared to the null mice, which were awake more.

T_CRT largely reflected the time course of waking, reaching its peak value at dark onset (Figs. 1, 2; Table 2). The only differencein T_CRT between the genotypes was a significantly higher T_CRTin the second half of the dark period in the null mice, whichcorresponds to their larger amount of waking in that interval(Table 2). The difference in T_CRT between the genotypes remainedwhen T_CRT was determined for waking alone (p < 0.05, two-tailedt test), indicating that the null mice may also have been moreactive during this interval.

Because we had found previously a marked difference between the genotypes in the amount of brief awakenings (Tobler et al.,1996), we analyzed this aspect of sleep in more detail (Fig. 3,Table 3). The 12 hr values revealed that within both the lightand the dark periods of the baselines waking episodes shorterthan 4, 8, and 16 sec invariably were significantly more prominentin the null mice. The episode histogram of the frequency of thethree vigilance states illustrates that the Prn-p^+/+ mice exhibited less brief waking episodes lasting 4 sec and lessbrief NREM sleep episodes of 32-124 sec, concomitant with a higheramount of longer NREM sleep episodes. The analysis of the 24 hrtime course of brief waking episodes < 16 sec showed that thebrief awakenings were consistently more abundant in the Prn-p^0/0 than in the Prn-p^+/+ mice throughout the entire recording (data not shown). Althoughthere were no LD differences in episode duration, the frequencyof NREM sleep and REM sleep episodes was significantly lower inthe dark period compared with the light period in both genotypes.However, there were differences between the genotypes. Thus, REMsleep episodes were more abundant (episodes per hr: Prn-p^0/0, 4.3 ± 0.6; Prn-p^+/+, 2.6 ± 0.5; p < 0.05, two-tailed t test) and REM sleep and NREMsleep episode duration was shorter in the dark period in the Prn-p^0/0 mice (REM sleep: Prn-p^0/0, 0.9 ± 0.1 min; Prn-p^+/+, 1.2 ± 0.1 min; NREM sleep: 5.8 ± 0.5 min, 7.6 ± 0.6 min, respectively;p < 0.05, two-tailed t test).
Fig. 3. Episode frequency histogram of the three vigilance states. Waking, NREM sleep, and REM sleep episodes during the light (openbars) and dark period (black bars) of baseline 2 for the Prn-p^+/+ and Prn-p^0/0 mice. Time bins are shown with logarithmically increasing size.The inclusive range of eight consecutive bins was: 4, 8-12, 16-28,32-60, 64-124, 128-252, 512-1020, and 1024-2048 sec. Bars representmeans ± SEM of 8 animals. The abscissae denote lower bin limits.Triangles indicate significant differences between the two genotypes(p < 0.005, two-tailed t test after Bonferroni correction). Orientationof triangles indicates the direction of deviation.
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Table 3. Brief awakenings as a measure of sleep fragmentation

BASELINE 1
BASELINE 2
RECOVERY

Light Dark Light Dark Light Dark

Shorter than 16 sec

Prn-p^+/+ 21.0 19.0 17.5 18.1 16.7 17.4

(0.8) (1.9) (1.5) (2.6) (2.7) (1.6)

Prn-p^0/0 35.2^* 35.1^* 33.1^* 33.8^* 30.4 32.5

(4.9) (4.9) (4.0) (4.2) (3.1) (3.5)

Shorter than 8 sec

Prn-p^+/+ 17.0 15.0 14.4 14.5 13.9 13.8

(1.1) (1.7) (1.4) (2.4) (2.4) (1.6)

Prn-p^0/0 31.5^* 30.8^* 29.0^* 29.6^* 26.3 28.7

(4.7) (4.5) (3.8) (4.0) (2.9) (3.3)

Shorter than 4 sec

Prn-p^+/+ 11.9 10.5 10.0 10.0 9.7 9.3

(1.1) (1.5) (1.3) (2.0) (1.9) (1.5)

Prn-p^0/0 24.7^* 24.1^* 22.2^* 23.1^* 20.1 22.7

(3.8) (3.5) (2.6) (2.9) (2.2) (2.6)

Brief awakenings are expressed per hour of total sleep time. Values are 12 hr means ± SEM (n = 8, except baseline, 1 Prn-p^+/+, n = 7). No significant differences between the light and thedark period (baseline 1 and 2) and between baseline 2 and recoveryafter 6 hr sleep deprivation were present. Comparison of baselinesbetween Prn-p^+/+ and Prn-p^0/0, ^* p < 0.02, two-tailed t test.

Time course of SWA within NREM sleep episodes
The time course of SWA within NREM sleep episodes may reflect the dynamics underlying the generation of SWA. If the normalprion protein were involved in the thalamocortical generationof SWA, the null mice would be expected to attain less SWA thanthe wild-type mice or to reach the maximum more slowly. For theanalysis of SWA within NREM sleep, all NREM sleep episodes > 4min within baseline 2 were pooled for each mouse. Statisticalcomparisons were performed on the mean values of the last minutebefore the waking-to-NREM sleep transition and for 4 min afterthe transition. The null mice reached the highest SWA value significantlyfaster than the wild-type mice (Fig. 4). Thus, the time courseof the SWA increase differed significantly between the genotypesfor the first minute after the transition, whereas they did notdiffer in the minute before the transition. Moreover, when SWAwas expressed as percentage of the first 4 sec NREM sleep epochafter the transition within each genotype, the SWA values attainedafter 4 min were as follows: 151.0 ± 5.5% for Prn-p^+/+ and 101.3 ± 3.7% for Prn-p^0/0 (p < 0.05, two-tailed t test).
Fig. 4. Time course of slow-wave activity within NREM sleep episodes. SWA, Mean EEG power density in the 0.75-4.0 Hz band. All NREMsleep episodes of the light period of baseline 2 lasting at least4 min were pooled for each mouse. The curves connect mean 4 secbins for 1 min before and 4 min after the transition from wakingto NREM sleep separately for each genotype (n = 8 mice per genotype).The curves are expressed as a percentage of the 24 hr baselinevalue for each genotype. The genotypes differed significantlyin the first 1 min interval after the transition (p = 0.004, two-tailedt test), whereas the 1 min interval before the transition wasnot significant (p = 0.083).
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Baseline EEG power spectra
The absolute EEG power density values (0.25-25.0 Hz) computed for each of the three vigilance states (pooled values of thetwo baselines) did not differ significantly between the two genotypes(data not shown). Clear differences were seen in the EEG powerspectra between the three vigilance states within each genotype(Fig. 5). Thus, NREM sleep exhibited higher values than both REMsleep and waking in the 0.5-4.0 Hz band, whereas REM sleep valuesin the theta band (6.25-9.0 Hz) were above those in NREM sleepand waking in both phenotypes. Moreover, NREM sleep power densitywas above the values of both waking and REM sleep in a broad frequencyband (11.25-25 Hz) in the null mice, whereas this difference wasnot significant in the wild-type.
Fig. 5. Spectral distribution of EEG power density in the three vigilance states. Waking (W), NREM sleep (N), and REM sleep (R) forPrn-p^+/+ and Prn-p^0/0 mice computed for pooled 24 hr values of Baseline 1 and 2. Thecurves represent logarithmic mean values of absolute power densities(log µV²/0.25 Hz, n = 8 for each genotype, except n = 7 for Baseline 1,Prn-p^+/+). Lines below the abscissa indicate frequency bands that differsignificantly between two vigilance states (p < 0.05, two-tailedt test).
[View Larger Version of this Image (26K GIF file)]

The dynamics of the EEG power spectrum in NREM sleep in the course of the light period is illustrated in a broad frequencyrange (0.5-25 Hz) for consecutive 2 hr intervals. EEG power densityshowed a decreasing trend in the low frequencies (0.25-4.5 Hz)in the null mice, whereas only one bin in this range reached significancein the wild-type (Fig. 7, top; ANOVA factor "2 hr interval").In contrast, most frequencies above ~7 Hz increased progressivelyin the course of the light period in both genotypes, reachinga maximum in the last 2 hr interval of the light period.
Fig. 7. Time course of EEG power density in NREM sleep. Top, Light period of baseline 2 (six 2 hr intervals; 1-6). Bottom, Light periodafter sleep deprivation (three 2 hr intervals; 1-3) for the Prn-p^+/+ and Prn-p^0/0 mice. The curves connect geometric means of relative EEG powerdensity for consecutive 2 hr intervals (n = 8 for each genotype).Values are plotted at the upper limit of each bin. The baselinedata are expressed relative to the first 2 hr interval of thelight period (=100%). Consecutive 2 hr intervals of recovery areexpressed relative to the first three consecutive 2 hr intervalsof the light period of Baseline 2 (=100%). Lines below the abscissaindicate frequency bands that differed significantly from 100%(p < 0.05, top, one-way ANOVA "2 hr intervals"; bottom, frequencybands: 0.5-4.0, 6.25-9.0, 11.25-25 Hz; two-tailed t test).
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Effects of sleep deprivation
No difference was found in the effect of SDEP on the vigilance states between the wild-type and null mice. After SDEP, NREMsleep showed a minor, significant increase in the first 2 hr inthe wild-type, but the 6 hr interval did not differ between thegenotypes (Fig. 6, Table 2). Also, SWA was significantly enhancedabove baseline and decreased progressively, but the magnitudeof the increase differed significantly between Prn-p^+/+ and Prn-p^0/0 (ANOVA "genotype" for the three 6 hr recovery intervals vs baseline2; p < 0.02). The increase of SWA in all three 6 hr recovery intervalswas significantly larger in the null mice (p < 0.04, two-tailedt test). These differences were not attributable to differencesbetween the genotypes during the deprivation because the amountof NREM sleep the mice obtained during the deprivation was similar(Prn-p^+/+: 3.0 ± 0.9%; Prn-p^0/0: 2.4 ± 0.5%). Furthermore, the minimum criterion of 6 min NREMsleep per 2 hr interval of SDEP to compute SWA reliably was notattained by either genotype.
Fig. 6. Effects of sleep deprivation on sleep and brain temperature. Vigilance states, slow-wave activity (SWA; mean EEG power densityin the 0.75-4.0 Hz band), and cortical temperature (T_CRT) forthe Prn-p^+/+ and Prn-p^0/0 mice. The curves represent 2 hr mean values ± 2 SEM (n = 8 foreach genotype) for Baseline 2 (dashed lines), 6 hr sleep deprivation,and recovery (solid lines). SWA is expressed as 95% of mean 24hr value (=100%). Triangles indicate significant differences withina genotype between recovery and baseline (p < 0.05; two-tailedt test, after Bonferroni correction). For the vigilance statesand SWA, the 2 hr recovery intervals of the light period werecompared with consecutive intervals of baseline beginning withlights on. For T_CRT, all intervals were compared with baselineintervals corresponding to the time of day.
[View Larger Version of this Image (39K GIF file)]

T_CRT was above baseline during the SDEP in both genotypes, and in the Prn-p^0/0 it remained above baseline in the first 2 hr recovery interval(Table 2, Fig. 6).

In the first 2 hr after SDEP, a significant increase of EEG power density was observed in the three frequency bands $---$ delta,beta, and sigma $---$ in both genotypes (Fig. 7). In the wild-type,a gradual decrease and a narrowing of the frequencies in the low-frequencyrange were observed in the course of the recovery, whereas inthe null mice the highest values in the low frequencies were presentin interval 1, followed by a decrease from interval 1 to 2. Ininterval 3, the values were still above baseline in the low- andhigh-frequency band in both genotypes.

Transgenic mice
The differences between the PrP-null mice and wild-type mice could indicate a specific role for the prion protein in sleep,or the differences may stem from the different genetic backgroundof the mice (Gerlai, 1996). The recording of transgenic mice,in which the prion gene has been reintroduced into the genomeof null mice and thereby expression of prion protein is reestablished,allowed us to investigate whether the reintroduction of PrP wouldalso restore the sleep characteristics of the wild-type mice.The results show that the transgenic mice were more similar tothe wild-type than to the null mice both in sleep fragmentationand in the response to SDEP. Thus, the number of brief awakenings(<16 sec) per hr total sleep time in the transgenic mice was asfollows: 12 hr baseline, 17.6 ± 6.1; 6 hr recovery, 19.5 ± 8.3(PrP^+/+: 17.5 ± 1.5 and 16.7 ± 2.7; PrP^0/0: 33.1 ± 4.0 and 30.4 ± 3.1). SWA was increased by 9.9 ± 10.2%in the first 2 hr interval after SDEP compared to the first 2hr interval of baseline. The corresponding values were as follows:Prn-p^+/+, 23.9 ± 4.3%; Prn-p^0/0, 41.1 ± 5.7%. The mean values ± SEM of NREM sleep and REM sleepfor the 12 hr light period in the transgenic mice were 42.0 ±2.2% and 12.6 ± 1.0% of recording time, respectively (n = 3).The amount of NREM sleep during the 6 hr recovery interval wasincreased (50.9 ± 1.5%) compared to the corresponding 6 hr baselinevalue (37.0 ± 2.3%).

DISCUSSION
The comparison of knockout mice lacking the prion protein with the corresponding wild-type controls showed a remarkably similardaily amount of NREM sleep and REM sleep that was comparable toprevious studies (Mitler et al., 1973, 1977; Oliverio and Malorni,1979; Faradji et al., 1980; Ibuka et al., 1980; Dazuta et al.,1983; Richardson et al., 1985; Edgar et al., 1991; Fang et al.,1995, 1996). The genotypes did differ in the distribution of NREMsleep in the dark period, which was reflected also in the timecourse of waking and in T_CRT. The use of a running wheel increasedtotal sleep time and enhanced the amplitude of the circadian sleep-wakerhythm (Welsh et al., 1988), but our mice were not provided withrunning wheels; thus, the nocturnal sleep patterns were not aconsequence of different running wheel activity.

Mice are similar to other rodents in that they exhibit little quiet wakefulness, and the activity during waking results inhigh T_CRT. Thus, the curves for waking and T_CRT were similar,as has been observed in the rat and the Djungarian hamster (Frankenet al., 1992; Deboer et al., 1994).

A remarkable difference between the two genotypes was the larger sleep fragmentation encountered in the PrP^0/0 mice. The 4 sec episodes included events that were equal to orshorter than 4 sec. Such events were not necessarily accompaniedby a behavioral change, and their significance is unknown. Theiroccurrence was almost double in the null mice irrespective oftheir duration (4-16 sec), reflecting a diminished capacity tosustain NREM sleep but not REM sleep. The build-up of SWA withina NREM sleep episode was not affected by an interruption of NREMsleep by a waking episode < 8 sec in the rat (Trachsel et al.,1988). Moreover, the number of brief awakenings correlated negativelywith the amount of SWA, reflecting a behavioral measure of sleepintensity (rat: Franken et al., 1991; Tobler et al., 1994; guineapig: Tobler and Franken, 1993). The build-up of SWA within NREMsleep was unhindered by the larger amount of brief awakeningsin the null mice, because it was faster than in the wild-type.

The analysis of the EEG power spectrum revealed a remarkable difference between the mice and other mammals in the lower frequencies.The relative contribution of slow waves to the spectrum, and especiallyto NREM sleep, is much smaller compared to other species (rat:Borbély et al., 1984; Djungarian hamster: Deboer et al., 1994;Syrian hamster: Tobler and Jaggi, 1987; rabbit: Tobler et al.,1990), which makes it more difficult to distinguish the vigilancestates. Slow waves and sleep spindles are closely related to cellularchanges in the thalamic and cortical neurons (Steriade et al.,1993, 1994), but it is not known which cellular characteristicsare responsible for the changes in the amount or amplitude ofslow waves. It is possible that the cortical layer of the micelacks the capacity to produce a substantial amount of slow waves.This notion is confirmed by the relatively similar, low valuesof absolute EEG power in mice and the Djungarian hamster, anothersmall rodent (Deboer and Tobler, 1996), compared to the rat. However,despite this similarity, SWA in the Djungarian hamster (Deboeret al., 1994) and the Syrian hamster (Tobler and Jaggi, 1987)is more prominent than in the mice in all vigilance states andis in this respect more similar to the rat (Borbély et al., 1984).The most distinctive feature discriminating NREM sleep from REMsleep was the prominent theta band peak in REM sleep, which wasabsent in NREM sleep.

Overall, the differences in the EEG power spectra between the vigilance states were similar in the null mice and the wild-type.Because mice strains differ in the occurrence of spindles in NREMsleep (Valatx et al., 1972; Valatx and Bugat, 1974), and spindlesare more prominent in a frontal or sensorimotor derivation thanin the parietal or occipital region (rat: Terrier and Gottesmann,1978; cat: Ursin and Sterman, 1981), comparisons of the EEG spectraderived from different electrode localizations are necessary toresolve the problem whether spindle activity is affected by theabsence of PrP.

There is a large body of literature demonstrating that sleep is regulated as a function of prior wakefulness (human: Borbélyet al., 1981; Achermann et al., 1993; Borbély 1994; rat: Toblerand Borbély, 1986, 1990). In particular, SWA is used as an indexfor sleep intensity (Borbély et al., 1981; Franken et al., 1991).This is supported by the higher arousal threshold when SWA ishigh in the rat (Nekelmann and Ursin, 1993). SWA closely reflectedthe previous sleep-waking history in both mouse genotypes. Becausethe mice differed in the distribution of sleep and waking in thedark period, it was not surprising that SWA also differed in itstime course: the earlier SWA decrease in the dark period in thewild-type mice was attributable to the earlier occurrence of sleepin the later part of the dark period, which allowed the dissipationof SWA. This difference was seen also in the more prominent decreaseof EEG power density in the lower frequencies in the null mice.Furthermore, the effects of 6 hr SDEP were evident in the increaseof SWA at the beginning of recovery sleep in both genotypes. Thus,also in mice sleep appears to be regulated as a function of priorwakefulness.

A remarkable difference was the larger increase of SWA after SDEP in the Prn-p^0/0 mice than in the wild-type mice. It is consistent with the moreprominent sleep fragmentation encountered in the Prn-p^0/0 mice. We suggest the following explanation: the null mice havea low sleep pressure, which leads to (1) more frequent interruptionsof sleep, and (2) low amounts of SWA. This interpretation is supportedby the lower amount of SWA reached within NREM sleep episodesin the null mice. As a consequence, the propensity for SWA canincrease more during SDEP in these mice. This notion is consistentwith the findings in humans, in which habitual long sleepers displayeda larger increase in SWA after SDEP than habitual short sleepers(Aeschbach et al., 1996). It was concluded that the short sleeperslive at a higher SWA pressure and, therefore, that SDEP cannotenhance SWA to the same extent as in the long sleepers. BecauseTST in the mice was not different, it is possible that cellularmechanisms responsible for the increase of SWA are affected bythe lack of PrP. The absence of PrP, therefore, seems to affectsleep via two mechanisms that may be interrelated: (1) a decreasein sleep pressure, and (2) a diminished capacity to sustain NREMsleep. In addition, the faster increase of SWA at the transitionsfrom waking to NREM sleep in the null mice may reflect a differencein the underlying cellular mechanisms leading to this transitionbecause of the lack of PrP.

The SWA increase after SDEP was relatively small in both genotypes (20 and 40%). To investigate whether the larger responseto SDEP was merely a consequence of the larger amount of wakingpreceding the SDEP in the Prn-p^0/0 mice, correlations of the initial SWA increase after SDEP withthe amount of wakefulness in the second half of the dark periodpreceding SDEP were computed. No difference in the correlationcoefficients was found between the genotypes (data not shown).Furthermore, the initial SWA values before the SDEP did not differ.This raises the question why 6 hr of wakefulness did not elicita similar degree of compensation as in other rodents. The NREMsleep and REM sleep increase does indicate that sleep pressurewas enhanced by the deprivation. Moreover, the progressive decreaseand the narrowing of the lower-frequency band are indicationsfor a recovery process. It should be noted that the mice, in contrastto all other rodents previously recorded, can exhibit spontaneousbouts of waking (even in the absence of running wheels) that maylast up to 6 hr. It is intriguing that such a small species hasthe capacity to remain spontaneously awake for so long. Thus,it appears that the relatively small increase of SWA after SDEPis a reflection of limitations at the cellular level. Studiesprolonging SDEP are needed to clarify further the SWA dynamicsin mice.

Thus, several differences were found between the genotypes that may be related to the absence of PrP. It is important to notethat only a fine analysis of the vigilance states and the impositionof an SDEP revealed differences between the genotypes that otherwisemay have gone unnoticed. The transgenic mice were more similarto the wild-type than to the null mice in sleep fragmentationand in the response to SDEP, indicating that the phenotype wasrescued by the insertion of PrP in null mice. More extensive studiesin transgenic mice and in other genotypes are needed to investigatewhether genes adjacent to the PrP gene exerted a modulating effect.

The prion protein is a well conserved protein present in many mammalian species (Westaway and Prusiner, 1986), with a largedegree of homology between species (Krakauer et al., 1996); therefore,it may have a very basic biological function. Sleep and circadianrhythms are extremely basic functions of all mammals. The detailedanalysis of sleep in the two mice genotypes supports our previousnotion that the prion protein may be involved not only in theregulation of circadian motor activity but also in the maintenanceof sleep continuity and its regulation after sleep deprivation(Tobler et al., 1996).

FOOTNOTES

Received Aug. 28, 1996; revised Dec. 13, 1996; accepted Dec. 18, 1996.

This study was supported by Swiss National Science Foundation Grants 31.32574.91 and 3100-042500.94. The mice were obtainedfrom Prof. Ch. Weissmann. We thank S. Gaus, F. Morgenthaler, andB. Schwierin for technical assistance and scoring, and Dr. P.Achermann and Prof. A. A. Borbély for critical comments on thismanuscript.

Correspondence should be addressed to Prof. Irene Tobler, Institute of Pharmacology, University of Zürich, Winterthurerstrasse190, CH-8057 Zürich, Switzerland.

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