2.1. Pharmacological Agents

Stock solutions of muscarinic receptor antagonist, scopolamine hydrobromide (Sigma, St Louis, MO, USA), a broad-spectrum opioid antagonist (naloxone hydrochloride (Tocris, Bristol, UK)), a $\mu$-receptor antagonist (naloxonazine dihydrochloride (Tocris)), a $\delta$-receptor antagonist (naltrindole hydrochloride (Tocris)) and a κ-receptor antagonist (nor-binaltorphimine dihydrochloride (Tocris)) were dissolved in pyrogen-free saline (PFS). The stock solutions were stored at 4°C until use. The dose of scopolamine used was 20 $\mu$g $\mu$L⁻¹, whereas naloxone, naloxonazine, naltrindole and nor-binaltorphimine were microinjected at three different doses, 0.1, 1.0 and 10 $\mu$g $\mu$L⁻¹. The total volume used for each microinjection was 1 $\mu$L.

2.2. Animals

Male Sprague-Dawley rats (250–300 g; National Laboratory Animal Breeding and Research Center, Taiwan) were used in this study. Rats were anesthetized by intraperitoneal injection with ketamine/xylazine (87/13 mg kg⁻¹) and were given an analgesic (1 mg/rat morphine) and an antibiotic (5000 IU/rat penicillin G benzathine) to reduce pain and avoid infection. Rats were surgically implanted with three electroencephalogram (EEG) screw electrodes as earlier described [19] and the microinjection guide cannulae directed into the NTS (AP, 13.30 mm from bregma; ML, 1.2 mm and DV, 8.2 mm relative to bregma). The coordinates were adopted from the Paxinos and Waton rat altas [20]. Two unilateral screw EEG electrodes were placed over the right hemisphere of the frontal and parietal cortices and a third EEG electrode was placed over the cerebellum and served to ground the animal to reduce signal artifacts. Insulated leads from EEG electrodes were routed to a Teflon pedestal (Plastics One, Roanoke, VA, USA). The Teflon pedestal was then cemented to the skull with dental acrylic (Tempron, GC Co., Tokyo, Japan). The incision was treated topically with polysporin (polymixin B sulfate—bacitracin zinc) and the animals were allowed to recover for 7 days prior to the initiation of experiments. The rats were housed separately in individual recording cages in the isolated room, in which the temperature was maintained at 23  $\pm$  1°C and the light:dark rhythm was controlled in a 12 : 12 h cycle (40 Watt $\times$ 4 tubes illumination). Food (5001 rodent diet, LabDiet) and water were available ad libitum. All procedures performed in this study were approved by the National Taiwan University Animal Care and Use Committee.

2.3. Experimental Protocol

On the second postsurgical day, the rats were connected to the recording apparatus via a flexible tether. As such, the rats were allowed relatively unrestricted movement within their own cages. Three groups of rats were used in the study as follows: Group 1 (n = 8) was used to determine the effects of opioid receptor antagonist (naloxone) and $\mu$-receptor antagonist (naloxonazine) on EA-induced alterations in sleep; Group 2 (n = 8) was used to elucidate the effects of $\delta$-receptor antagonist (naltrindole) and κ-receptor antagonist (nor-binaltorphimine) on EA-induced alterations in sleep; Group 3 (n = 24) was used to depict the action of NTS muscarinic receptors on EA-induced $\beta$-endorphin expression (determined by enzyme-linked immunosorbent assay (ELISA)) after microinjection of scopolamine into the NTS. One week after rats had adapted to the 12 : 12 h light : dark cycle after surgery, a 23-h undisturbed baseline recordings were obtained beginning at dark onset on the first recording day in rats in Groups 1 and 2. When EA was given (see later), all rats were lightly anesthetized with one-third of the dose of ketamine/xylazine used in the surgery, after which rat wake-up time is 20–25 min. A 20-min period of EA stimulation was administered before the onset of the dark period. The anesthetization was given 25 min prior to the dark period onset and lasted for 20 min. The rationale for carrying out the experiment in the darkness is that rats are active with a lowest level of sleep during the dark period, and a manipulation, if it possesses ability to increase sleep, would significantly augment sleep during the dark period. In contrast, it may not be easy to enhance sleep during the light period when sleep activity is at its highest circadian level. Since we expected to find a sleep enhancement after the EA stimuli at the Anmian (EX17), we therefore manipulated the EA stimulation before the onset of the dark period and analyzed the sleep alteration during the subsequent dark period. The rats in group 1 were both administered PFS intraperitoneally (IP) and microinjected into the NTS (_ipPFS $+$ PFS) at 25 min prior to the dark onset on two consecutive days, and recordings obtained for 24-h beginning after the second injection. The effects of anesthesia with the NTS microinjection of PFS (_ipketamine $+$ PFS) on sleep were determined after IP injection of ketamine/xylazine and the NTS PFS microinjection on two consecutive days. A sham EA (_ipketamine $+$ PFS $+$ sham EA) was delivered to control for the non-specific effect of the electrical stimulation, although our previous study had confirmed that no non-specific effect was observed after the sham EA [17]. The EA stimuli under anesthesia (_ipketamine $+$ PFS $+$ EA) were also performed before the dark onset on two consecutive days and sleep-wake behavior after the second EA stimulation was then determined. Subsequently, three different doses (0.1, 1.0 and 10 $\mu$g) of naloxone (_ipketamine $+$ naloxone $+$ EA) and naloxonazine (_ipketamine $+$ naloxonazine $+$ EA) were administered 25 min prior to the dark onset on the second day of EA stimulation and the 24-h sleep pattern was determined. At least 1 day without injections was scheduled between each manipulation. The EA stimulus was delivered via the bilateral insertion of stainless needles (32 gauge $\times$ 1^″, Shanghai Yanglong Medical Articles Co.) on Anmian (EX17) points in the depth of 2 mm. The stimulus consisted of a train of biphasic pulses (150 $\mu$s duration each) of 10 Hz with intensity of 3 mA, and was delivered by Functions Electrical Stimulator (Trio 300, I.T.O., Japan). The acupoint “Anmian (EX17)” is located at midpoint between Yifeng (TH 17) and Fengchi (GB 20); Yifeng (TH 17) locates posterior to the lobule of the ear in the depression between the mandible and mastoid process and Fengchi (GB 20) locates in the depression between the upper portion of musculus sternocleidomastoideus and musculus trapezius in human. The location of Anmian (EX17) in rats is at the relative anatomical location between the strenocleidomastoideus muscle and the splenius capitis muscle, as in the human acupoint map. Sham EA was performed by stimulation of a non-acupoint located at the ventral conjunction between the forelimb and the trunk as described earlier [17]. Those rats in group 2 underwent a similar protocol to those in group 1, except that the substances administered were naltrindole (_ipketamine $+$ naltrindole $+$ EA) and nor-binaltorphimine (_ipketamine $+$ nor-binaltorphimine $+$ EA). Rats in group 3 were divided into four subgroups and received _ipketamine $+$ PFS, _ipketamine $+$ PFS $+$ sham EA, _ipketamine $+$ PFS $+$ EA and _ipketamine $+$ scopolamine $+$ EA, respectively. Microinjection of scopolamine into the NTS was administered prior to the second EA stimulation. Rats were then decapitated at the dark onset and five distinct brain regions, including the hypothalamus, cortex, brainstem, hippocampus and striatum, were dissected and frozen in $-$80°C until assay. These tissues were used for $\beta$-endorphin ELISA as described in the following.

2.4. Apparatus and Recording

Signals from the EEG electrodes were fed into an amplifier (Colbourn Instruments, Lehigh Valley, PA; model V75-01). The EEG was amplified (factor of 5000) and analog bandpass filtered between 0.1 and 40 Hz (frequency response: $\pm$3 dB; filter frequency roll off: 12 dB/octave). Gross body movements were detected by custom-made infrared-based motion detectors (Biobserve GmbH, Germany) and the movement activity was converted to a voltage output which was digitized and integrated into 1-s bins. These conditioned signals (EEGs and gross body movements) were subjected to analog-to-digital conversion with 16-bit precision at a sampling rate of 128 Hz (NI PCI-6033E; National Instruments, Austin, TX). The digitized EEG waveform and integrated values for body movement were stored as binary computer files pending subsequent analyses.

Postacquisition determination of the vigilance state was done by visual scoring of 12-s epochs using custom software (ICELUS, M. R. Opp) written in LabView for Windows (National Instruments). The animal's behavior was classified as SWS, rapid eye movement sleep (REMS) or waking based on previously defined criteria [19]. Briefly, SWS is characterized by large-amplitude EEG slow waves, high power density values in the delta frequency band (0.5–4 Hz) and lack of gross body movements. During REMS, the amplitude of the EEG is reduced, the predominant EEG power density occurs within the theta frequency (6–90 Hz) and there are phasic body twitches. During waking, the rats are generally active. There are protracted body movements. The amplitude of the EEG is similar to that observed during REMS, but power density values in the delta frequency band are generally greater than those in theta frequency band. In addition to the amount of time spent in each vigilance state, the number and duration of individual bouts of behaviors were determined using criteria modified from those of Tobler and colleagues [21, 22], as described earlier [19].

2.5. ELISA for $\beta$-Endorphin

Rat $\beta$-endorphin ELISA kits were obtained from Phoenix Pharmaceuticals Inc. (Burlingame, CA, USA) and the procedures followed the standard instructions provided by the manufacturers. Absorbance was measured by an ELISA plate reader (Multiskan EX, Thermo Electron Corp., Waltham, MA, USA) with the wavelength set at 450 and 550 nm. The sensitivity is 0.21 ng mL⁻¹, the assay range is between 0.21 and 3.15 ng mL⁻¹, the intra-assay coefficient of variation is $<$5% and the inter-assay coefficient of variation is $<$14%. There is no cross-reactivity for met-enkephalin and leu-enkephalin.

2.6. Statistical Analyses for Experiment Protocol

All values acquired from sleep-wake recording were presented as the mean  $\pm$  SEM for the indicated sample sizes. One-way analyses of variance (ANOVA) for the duration of each vigilance state (SWS, REMS, WAKE) and for sleep architecture parameters were performed, comparing before and after manipulation within subjects, across a certain of time block. An $\alpha$ level of $P\le .05$ was taken as indicating a statistically significant difference. If statistically significant differences were detected, a Scheffe post hoc comparison was made to determine which hourly intervals during experimental conditions deviated from values obtained from the same animals during control conditions. The statistical evaluation for the $\beta$-endorphin ELISA used an unpaired Student's t-test comparing the averages between the groups analyzed.

3.1. Naloxone and Naloxonazine Blocked the EA-Induced Alterations in Sleep

Anesthetization of rats for 25 min with ketamine/xylazine prior to the dark period suppressed both NREM and REM sleep for the first 4 h of the dark period. The time spent in NREM sleep during the first 4-h period after _ipketamine $+$ PFS decreased to 10.8  $\pm$  2.5% from 22.4  $\pm$  2.5% acquired after _ipPFS $+$ PFS (F_(1,62) = 10.711, $P=.002$, Figures 1(a) and 1(b)). REM sleep was suppressed from 6.5  $\pm$  1.8% obtained after _ipPFS $+$ PFS to 0.8  $\pm$  0.3% acquired after _ipketamine $+$ PFS (F_(1,62) = 8.697, $P=.005$, Figures 1(c) and 1(d)). A concomitant enhancement of wakefulness was observed during the first 4 h after receiving ketamine anesthetization (Figures 1(e) and 1(f)). Application of sham EA did not alter any aspect of sleep parameters (data not shown), which is similar to our previous observation [17]. Twenty-minute EA stimuli delivered before the dark period on two consecutive days significantly augmented NREM sleep during post-manipulation 5–8 h. The percentage of time spent in NREM sleep during 5–8 h increased from 18.3  $\pm$  2.7% obtained after _ipketamine $+$ PFS to 34.0  $\pm$  3.8% after vketamine $+$ PFS $+$ EA (F_(1,62) = 9.180, $P=.004$, Figures 1(a) and 1(b)). Analysis of 12-h dark period revealed that NREM sleep was enhanced from 14.8  $\pm$  1.5% after _ipketamine $+$ PFS to 21.7  $\pm$  2.1% after _ipketamine $+$ PFS $+$ EA (F_{(1, 190)} = 6.923, $P=.010$). REM sleep was not significantly altered by EA. A decrease of waking at the expense of SWS was observed during 5–8 h (Figures 1(e) and 1(f)).

[figures omitted; refer to PDF]

Administration of three different doses (0.1, 1.0 and 10.0 $\mu$g) of naloxone, a broad-spectrum opioid antagonist, into the NTS dose-dependently blocked EA-induced increases of NREM sleep, especially during post-manipulation 5–8 h (Figures 2(a) and 2(b)). Across the entire 12-h dark period recording, NREM sleep was suppressed from 21.7  $\pm$  2.1% after _ipketamine $+$ PFS $+$ EA to 13.4  $\pm$  2.1% after _ipketamine $+$ naloxone (10.0 $\mu$g) $+$ EA (F_(1,190) = 7.631, $P=.007$, Figures 2(a) and 2(b)). Administration of $\mu$-opioid receptor antagonist, naloxonazine, also exhibited a dose-dependent blockade of EA-induced NREM sleep enhancement (Figures 2(a) and 2(b)). Administration of 10 $\mu$g naloxonazine reduced NREM sleep from 21.7  $\pm$  2.1% after _ipketamine $+$ PFS $+$ EA to 14.9  $\pm$  2.1% (F_(1,190) = 5.100, $P=.026$, Figures 2(a) and 2(b)) during the 12-h dark period. Neither naloxone nor naloxonazine altered REM sleep (Figures 2(c) and 2(d)). A mirror effect on the EA-induced decrease of waking was also been observed for both naloxone and naloxonazine (Figures 2(e) and 2(f)).

[figures omitted; refer to PDF]

Analysis of sleep architecture parameters across 1–12 h during the dark period revealed that the effect of ketamine on the suppression of NREM and REM sleep was primarily due to an increase in episode duration of waking, although there was a tendency for decreases in both REM sleep episode number and in NREM sleep episode duration (Table 1). The increase of NREM sleep after EA stimuli was primarily because of the increase in the duration of a single episode (Table 1), which is similar to our previous result [17]. Effects of naloxone and naloxonazine on blocking EA-induced enhancement of NREM sleep were mediated by reversing the EA-induced augmentation of NREM sleep episode duration (Table 1).

Table 1

Effects of naloxone and naloxonazine on the alterations of sleep-wake architecture parameters induced by EAc of Anmain (EX17) acupoints in rats.

Values are means  $\pm$  SEM.

^a Number of bouts per hour (mean  $\pm$  SEM) for each vigilance state; ^bMean ($\pm$SEM) bout duration (min) for each vigilance state; ^cNumber of transitions from one behavioral state to another (mean  $\pm$  SEM) per hour; ^dExperimental manipulation; ^ePeriod of the light : dark cycle immediately prior to which injections were given: D = dark period; ^fVigilance states: WAKE, wakefulness; NREMS, non-rapid eye movement sleep; REMS, rapid eye movements sleep; *Denotes a statistically significant difference ($P<.05$) between values obtained after administration of _ipPFS $+$ PFS and those obtained after receiving _ipketamine $+$ PFS; ^#Depicts a statistically significant difference ($P<.05$) between values obtained after _ipketamine $+$ PFS $+$ EAc and those obtained after _ipketamine $+$ PFS; ^$Depicts a statistically significant difference ($P<.05$) after either receiving naloxone or naloxonazine.

3.2. Naltrindole and Nor-Binaltorphimine Did Not Affect EA-Induced Alterations in Sleep

Administration of either the $\delta$-opioid receptor antagonist naltrindole or the κ-receptor antagonist nor-binaltorphimine prior to EA stimulation did not affect EA-induced alterations in sleep (Figure 3). Similarly, these antagonists did not alter any aspect of sleep architecture (data not shown).

[figures omitted; refer to PDF]

3.3. Scopolamine Suppressed EA-Induced Expression of Endogenous $\beta$-Endorphin

Our result demonstrated that delivery of sham EA stimuli did not alter the concentrations of $\beta$-endorphin within five distinct brain structures, including the brainstem, hypothalamus, cortex, hippocampus and striatum (Figure 4). However, application of EA stimuli at Anmian (EX17) acupoints for 20 min significantly enhanced the levels of $\beta$-endorphin in the brainstem and hippocampus, but not in the cortex, hypothalamus and striatum (Figure 4). Administration of the muscarinic receptor antagonist scopolamine directly into the NTS before the EA stimuli blocked EA-induced increases of $\beta$-endorphin in the brainstem and hippocampus (Figure 4).

[figure omitted; refer to PDF]