Eight male Sprague-Dawley rats (Samtaco, Osan, Korea) weighing from 280 to 310 g (295.60±3.65) at surgery were used. All animals were housed individually in Plexiglas cages (28×42×18 cm high), were kept in a controlled environment with 23±2℃ ambient temperature, 12:12 h light-dark cycle (lights on from 07:00 to 19:00), and were fed with a commercial food (Hyochang Science, Daegu, Korea) and tap water available ad libitum, except on the days of the behavioral recordings. All procedures were conducted in accordance with the National Institutes of Health Guidelines for Care and Use of Laboratory Animal (1996).

The animal was anesthetized with an intraperitoneal injection of a 2 ml/kg cocktail of 10 ml of ketamine hydrochloride (50 mg/ml, Ketamine, Yuhan Co., Seoul, Korea), 1.1 ml of xylazine hydrochloride (23.32 mg/ml, Rumpun, Bayer Co., Seoul, Korea), and 2.67 ml of saline. After fixed to a stereotaxic apparatus (David-Kopf Instrument Co., CA, USA), the scalp was locally anesthetized with a subcutaneous injection of 2% lidocaine with 1:100,000 epinephrine (Lidocaine hydrochloride Epinephrine, Huons Co., Seoul, Korea) and then, the midline of the scalp was incised and the skull surface was cleaned. For electroencephalogram (EEG), four stainless steel screws (1.1 mm in diameter), served as recording electrodes, were inserted into the bilateral frontal (+2.5 mm anterior and ±2.5 mm lateral to the bregma) and parietal bones (5.0 mm posterior and ±2.5 mm lateral to the bregma), without perforation the dura mater, and two stainless steel screws, served as reference and ground electrodes, were inserted into the inter-parietal bone (10.0 mm posterior and ±2.5 mm lateral to the bregma). The electrodes were soldered to connecting pins which were arranged in a 3×2 matrix, and the whole assembly was fixed over the skull with dental cement (Ortho-jet, Lang Dental Manufacturing Co., PA, USA).

At least 7 days were allowed to recover from the surgery. The animal was acclimated to the recording setup from 09:30 to 17:30 (8 h) on the day before the recording. Recording chamber was a sound-attenuated and electrically shielded box (80 cm wide×60 cm deep×80 cm high). The vibration measurement plate, constructed in our lab [13] was placed on the floor of the chamber to measure animal activity. On the day of the recording, a Plexiglas cage was put on the vibration measurement plate and the rat was placed into the cage at 09:30. Its head pins were connected to the amplifier via a flexible cable and swivel system. EEG signals from the frontal and parietal cortices and vibration signal were fed to amplifiers (Model 3500, A-M systems, Inc., WA, USA and CyberAmp 380, Axon instruments Inc., CA, USA) from 09:30 to 17:30 (8 h). The EEG signals and the vibration signal were amplified with 10,000× and 10× gain, respectively, and were filtered with 1~100 Hz. The signals were digitized at a rate of 1 KHz (DAQ PAD6015, National Instrument Inc., CA, USA), averaged with 5 consecutive samples, and stored at a rate of 200 Hz with custom-made LabView program (National Instrument INC., CA, USA).

Sleep-wake states were scored by an experienced experimenter with EEG and vibration signals. Each 10-second epoch was assigned to one of the following sleep-wake states: active wake (aW), quiet wake (qW), transition to slow wave sleep (tSWS), slow wave sleep (SWS), transition to paradoxical sleep (tPS) and paradoxical sleep (PS). As described previously [14], aW was scored according to the presence of high and phasic vibration together with high-frequency and theta activity on the parietal EEG; qW by the presence of moderate vibration with low-voltage fast EEG activity; tSWS by the presence of low vibration with delta activity less than 50% of the epoch and/or a sleep spindle; SWS by the presence of minimal vibration with delta activity more than 50% of the epoch; tPS by absent vibration with almost continuous spindle activity and interlaced theta activity; and PS by absent vibration with prominent theta activity on the parietal cortex.

It was adapted from Lee et al. [15]. The raw EEG signals were visually inspected prior to analysis and 10-sec EEG epochs with artifacts were excluded from analysis. The one-day recording was divided into sixteen 30-min segments from 09:30 and was analyzed. Ten power spectra were calculated by using a fast Fourier transform from 10 Hanning-windowed 2-sec FFT epochs (1-sec overlap) of one 10-sec EEG epoch and then averaged to a power spectrum. The spectrum was divided to 5 frequency bands (delta, 0.5~4.0; theta, 4.5~8.0; alpha 8.5~12.0; beta, 12.5~24.5; and gamma, 25~49.5 Hz). All the calculations were performed by custom-made programs using MatLab (MathWorks Inc., Natick, MA, USA).

Sleep-wake states were estimated as W, S and P: W consists of aW and qW. S consists of tSWS and SWS. P consists of tPS and PS. Seven sleep-related parameters were evaluated as follows: (1) total duration, total time spent in each sleep-wake stage; (2) number of episode, total number of occurrence of each sleep-wake stage; and (3) mean episode duration, mean duration of each sleep-wake stage when it was once occurred for 2-h period (from 30 to 150 min after drug injection); (4) latency to 5-min S and (5) latency to 1-min P, the latency time in min from drug injection to the accumulation of total 5-min S and of total 1-min P, respectively.

The power parameters were calculated as follows: (1) delta activities, as power density of delta band (0.5~4.5 Hz) in the average spectrum of 2- and 8-h recording; (2) band power density during S and P, calculation respective delta (0.5~4.5 Hz), theta (4.5~6.5 Hz), alpha (8.5~12.5 Hz), beta (12.5~25 Hz) and gamma (25~50 Hz) of average spectrum in S and P during 2-h sleep after injection.

Galantamine hydrobromide (Reminyl, Janssen Korea Co., Seoul, Korea), donepezil hydrochloride (Aricept, Eisai Korea Co., Seoul, Korea), and memantine hydrochloride (Ebixa, Lundbeck Korea Co., Seoul, Korea) were gifted from each company. Animals were received all of the following drugs once: vehicle (1 ml/kg, Con), donepezil (0.15 mg/kg, Don), galantamine (0.25 mg/kg, Gal) and memantine (0.25 mg/kg, Mem). Each rat had 7-day washout period between drugs. The dosage of each drug was chosen from clinical dosing recommendations in a previous report [16]. All drugs were dissolved in distilled water before the administration. Animals received an intraperitoneal injection at a volume of 1 ml/kg at 09:00.

All data were represented as mean±S.E.M. One-way analysis of variance (ANOVA) with Tukey HSD test was used for statistical analysis to estimate the effects of the drugs (SPSS v. 17.0 for Window, Data solution, Seoul, Korea). A p-value below 0.05 was considered significantly different.

Three anti-dementia drugs, galantamine, donepezil and memantine, had differential effect on the sleep-wake architecture in rats. Donepezil and memantine increased active wake and decreased slow-wave sleep significantly. Memantine had stronger and longer effect. Its effect on active wake was continued to 150 min and its effect on slow-wave sleep was continued to 120 min after the injection. Donepezil has effect on active wake and on slow-wave sleep to 90 min after the injection. On the other hand, galantamine did not produce significant changes on duration of any sleep-wake stages, but rather increased slow-wave sleep during 120~150 min after the injection (Table 1).

Only memantine significantly increased W (aW+qW) and decreased S (tSWS+SWS) and P (tPS+PS) as compared to control group (Fig. 1A), in which the total durations were pooled for 2-h period. Three anti-dementia drugs caused no significant changes in number of episode. (Fig. 1B). Mean episode duration of S was significantly decreased by memantine while that of P was significantly decreased by all three anti-dementia drugs (Fig. 1C).

Memantine caused significant increases both in latency to S and latency to P, while donepezil and galantamine did not (Fig. 2A). Activity was estimated by power of vibration in this study. Memantine and donepezil significantly increased movement while galantamine did not (Fig. 2C).

Donepezil and memantine decreased delta activity of the frontal and parietal cortex during 2-h period (Fig. 2B). Memantine and donepezil cause significantly decrease of delta activity in frontal and parietal cortex. There were no significant differences of delta activity in frontal and parietal cortex by galantamine.