Changes in Monoamine Release in the Ventral Horn and Hypoglossal Nucleus Linked to Pontine Inhibition of Muscle Tone: An In Vivo Microdialysis Study

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (42)

Citing Articles via Google Scholar

Google Scholar

Articles by Lai, Y.-Y.

Articles by Siegel, J. M.

Search for Related Content

PubMed

PubMed Citation

Articles by Lai, Y.-Y.

Articles by Siegel, J. M.

Previous Article  |  Next Article

The Journal of Neuroscience, September 15, 2001, 21(18):7384-7391

Changes in Monoamine Release in the Ventral Horn and Hypoglossal Nucleus Linked to Pontine Inhibition of Muscle Tone: An In Vivo Microdialysis Study
Yuan-Yang Lai¹, Tohru Kodama¹^,², and Jerome M. Siegel¹
¹ Department of Psychiatry and Biobehavioral Neuroscience, School of Medicine, University of California Los Angeles, and Veterans Affairs, Greater Los Angeles Health Care System Medical Center, North Hills, California 91343, and ² Department of Psychology, Tokyo Metropolitan Institute of Neuroscience, Fuchu, Tokyo 183 8526, Japan

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

A complete suppression of muscle tone in the postural muscles and a reduction of muscle tone in the respiratory related musculatureoccur in rapid eye movement (REM) sleep. Previous studies haveemphasized the role of glycine in generating these changes. Becausethe activity of norepinephrine- and serotonin-containing neuronsis known to decrease in REM sleep, we hypothesized that a decreasein release in one or both of these transmitters might be detectedat the motoneuronal level during muscle tone suppression elicitedby brainstem stimulation in the decerebrate animal. We comparedrelease in the ventral horn with that in the hypoglossal nucleusto determine whether the mechanism of muscle tone suppressiondiffers in these nuclei as has been hypothesized. Electrical stimulationand cholinergic agonist injection into the mesopontine reticularformation produced a suppression of tone in the postural and respiratorymuscles and simultaneously caused a significant reduction of norepinephrineand serotonin release of similar magnitude in both hypoglossalnucleus and spinal cord. Norepinephrine and serotonin releasein the motoneuron pools was unchanged when the stimulation wasapplied to brainstem areas that did not generate bilateral suppression.No change in dopamine release in the motoneuron pools was seenduring mesopontine stimulation-induced atonia. We hypothesizethat the reduction of monoamine release that we observe exertsa disfacilitatory effect on both ventral horn and hypoglossalmotoneurons and that this disfacilitatory mechanism contributesto the muscle atonia elicited in the decerebrate animal and inthe intact animal during REMsleep.

Key words: decerebration; REM sleep; respiration; tongue; locus coeruleus; raphe nucleus; norepinephrine; serotonin; hypoglossal nucleus; spinal cord; sleep apnea

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Magoun and Rhines (1946) discovered that stimulation of the medial medulla in the decerebrate animal produces a short-latencyinhibition of reflex response in skeletal muscle systems. Morerecently we found that the regions that generate muscle tone suppressionby electrical stimulation extend from the medulla through thepons and into the caudal midbrain (Lai and Siegel, 1990, 1999).Electrical and chemical stimulation in the pontine inhibitoryarea (PIA; Lai et al., 1993), including the central portion ofthe nucleus pontis centralis oralis and caudalis, generates muscletone suppression in the decerebrate animal (Lai and Siegel, 1988,1991; Hajnik et al., 2000). In the chronic animal, the PIA canbe chemically activated to produce a long period of REM sleep-likeactivity (George et al., 1964; Van Dongen et al., 1978; Lai andSiegel, 1988). Damage to this region produces REM sleep withoutatonia (Jouvet and Delorme, 1965; Henley and Morrison, 1974).A population of neurons in this area is selectively active inREM sleep (Sakai et al., 1981; Siegel et al., 1981). Thus, thePIA is part of the mechanism for generating REMsleep.

Electrical stimulation of the brainstem monoaminergic cell groups facilitates motoneuronal activity (Fung and Barnes, 1981,1989; Lai et al., 1989; Nagase et al., 1997). Dopamine is alsoknown to facilitate motoneuronal activity in the anesthetizedcat (Baker and Anderson, 1972). Therefore, inactivation of monoaminergicsystem could elicit muscle tone suppression by disfacilitation.On the other hand, active inhibition by GABA and glycine has beenshown to decrease both spinal and hypoglossal (XII) motoneuronexcitability (Kawai and Sasaki, 1964; Bruggencate and Sonnhof,1972; Soja et al., 1987, 1991; Yamuy et al., 1999). Kubin et al.(1993) concluded that the hypoglossal and possibly other cranialmotoneurons had a different mechanism of motor inhibition thanspinal motoneurons. They suggested that hypoglossal motoneuronswere not subject to glycinergic inhibition but were inactivatedby a reduction in serotonin (5-HT) release during REM sleep (Kubinet al., 1993).

Therefore, we had two goals in the present study. The first was to determine whether stimulation of the inhibitory mesopontineregion in the decerebrate animal produced a reduction in monoaminerelease by measuring norepinephrine (NE), 5-HT, and dopamine (DA)release. The second was to determine whether any observed changesin monoamine release were confined to the XII nucleus or whetherthey were also present in lumbar motoneuron pools. Collectionof dialysates collected from multiple sites allowed us to simultaneouslyevaluate the role of monoamines in the control of cranial andspinal motoneuronactivity.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animal preparation. Two male and five female young adult cats weighing from 2.5-3.5 kg were used. Tracheotomy, laminectomy,and decerebration were performed while the animals were anesthetizedwith a halothane-oxygen mixture. Decerebration was done at thepostmammillary-precollicular level. The spinal cord was exposedfrom the L₆ to S₁ segments. The medial cerebellum was removedby aspiration to allow insertion of the microdialysis probes intothe hypoglossal nucleus. Blood pressure was recorded from thefemoral artery. Data collected from animals in which the meanarterial pressure remained >80 mmHg were analyzed. Rectal temperaturewas monitored through a thermoregulator connected to a heatingpad and set to maintain the body temperature at 38 ± 0.5°C.

Stimulation and electromyogram recording. A bipolar stainless steel microelectrode (SNEX-100; David Kopf Instruments, Tujunga,CA) was used for mesopontine electrical stimulation. A 300 or500 msec train of 0.2 msec, 100 Hz, and 10-40 µA cathodal rectangularpulses was administered to the brainstem. When we identified amesopontine site at which stimulation produced muscle tone suppression,stimulation with the same parameters was delivered once every10 sec for a period of 5 min. Each site received two parametricallyidentical stimulations 2 hr apart. Five of the electrical stimulationsites also received an injection of 0.5 µl of 1 M acetylcholine(Ach).

Muscles in the neck (occipitoscapularis and splenius), hindlimb (gastrocnemius), tongue (genioglossus), and diaphragm wereimplanted with bipolar multistranded stainless steel electromyogram(EMG) electrodes (2 mm uninsulated portions exposed and 4-6 mminterelectrode separation). EMG activity was integrated througha Grass integrator (model 7P10F) and recorded polygraphically(Grass model 78E). The integrated muscle activity was measuredfor 5 min during the prestimulation period to determine baselinelevel and for 5 min during the stimulationperiod.

Microdialysis sampling. Microdialysis probes with a tip length of 1 mm (Type A-1-02; Eicom, Kyoto, Japan) were inserted intothe XII nucleus, and another pair of probes with a tip lengthof 2 mm (59-7005; Harvard Apparatus, South Natick, MA) were insertedinto the lumbar ventral horn bilaterally. Microdialysis probeswere perfused with artificial CSF (Harvard Apparatus) at a flowrate of 2 µl/min. Dialysates were collected for 5 min intervalsduring the prestimulation period, the stimulation period, andthe poststimulation period. Ten microliters of dialysate werecollected in each polypropylene sample tube under acidic conditions,pH 3.5, at 10°C. They were frozen at $-$ 80°C within 5 min of collection.Experiments were started at least 3 hr after the insertion ofmicrodialysis probes and lasted for 24hr.

Monoamine assay. The NE, DA, and 5-HT levels in the dialysates were determined by an HPLC and electrochemical detection (450mV) system (DTA-300; Eicom). The mobile phase for DA/5-HT was80% 100 mM phosphate buffer, pH 6.0, and 20% methanol, containing500 mg/l octansulphonic acid and 50 mg/l EDTA-2Na. Norepinephrinewas detected with a mobile phase consisting of 95% 100 mM phosphatebuffer, pH 6.0, and 5% methanol, containing 400 mg/l octansulphonicacid and 50 mg/l EDTA-2Na. The detection limit of our analysissystem was 0.5 fmol per 20 µlinjection.

Histology and data analysis. At the end of the study, a 50 µA anodal direct current was delivered into the stimulation sitethrough the stimulation electrode for 20 sec to deposit iron.Animals were anesthetized with Nembutal (35 mg/kg, i.v.) and perfusedintracardially with saline followed with buffered 10% formalin.Brain tissues were cut at 50 µm and stained with Neutral Red.Sections were counterstained with ferrocyanide to detect the irondeposit. The collecting sites from the XII nucleus and spinalventral horn were identified by the tracts of the microdialysisprobe. The stimulation and dialysate collecting sites in the brainstemwere reconstructed according to the atlas of Berman (1968).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Stimulation and dialysate collection sites

Electrical stimulation sites in the mesopontine area are presented in Figure 1. Ten of these sites were located in the PIA.The remaining stimulation sites were found in the caudal mesencephalicreticular formation (MRF; two sites), pedunculopontine tegmentalnucleus (PPN; two sites), medial longitudinal bundle (MLB; twosites), dorsolateral tegmental nucleus (LDT; one site), and brachiumconjunctium (BC; one site). The five sites that received Ach injectionwere located in the PIA (Fig. 1).

View larger version (32K):
[in this window]
[in a new window]
Figure 1. Histology showing the stimulation sites in the mesopontine reticular formation. Seven stimulation sites were on the left side of the brain. Dots (electrical stimulation) and triangles (both electrical and chemical stimulation) represent the sites in which stimulation elicited a bilateral reduction of muscle tone, whereas the sites from which stimulation failed to induce muscle tone suppression are marked by filled squares. AQ, Aqueduct; BC, brachium conjunctivum; CNF, cuneiform nucleus; IC, inferior colliculus; LDT, dorsolateral tegmental nucleus; P, pyramidal tract; PAG, periaqueductal gray; PG, pontine gray; PIA, pontine inhibitory area; PPN, pedunculopontine tegmental nucleus.

Figure 2 shows the location of the 15 microdialysis probes in the brainstem and 13 probes in the spinal cord. Eleven sitesin the brainstem and eight sites in the spinal cord were usedfor electrical stimulation, whereas the rest of four sites inthe brainstem and five sites in the spinal cord were used forthe chemical injection experiment. In the electrical stimulationexperiment, eight microdialysis probes were localized to the XIInucleus, with six located at the rostral and the other two locatedat the caudal part of the nucleus. The remaining three probeswere localized to the gigantocellularis nucleus (two cases), andone probe was located in the midline (one case). Seven microdialysisprobes were localized in the spinal ventral horn, whereas onesite was located in the lateroventral funiculus for the electricalstimulation study. In the Ach injection experiment, all four siteswere localized at the XII nucleus, with three located at the rostraland the remaining one site located at the caudal part of the nucleus.In the spinal cord, all five probes were localized to the ventralhorn.

View larger version (39K):
[in this window]
[in a new window]
Figure 2. Histology showing the dialysate collecting sites in the brainstem and spinal cord. Dialysates were collected from both sides of hypoglossal nucleus and spinal cord. Among 12 dialysis probes found in the spinal ventral horn, three were located at position a, two probes were located at b, and seven probes were found at c. One probe (d) was found in the lateroventral funiculus. DH, Dorsal horn; NPM, nucleus paramedianus; VH, ventral horn; 5ST, spinal trigeminal tract; 12, hypoglossal nucleus.

Muscle response to electrical stimulation in mesopontine reticular formation

Electrical stimulation applied in the PIA, PPN, and MRF produced muscle tone suppression in the diaphragm, genioglossus, hindlimbmuscles, and bilaterally in the neck muscles. Figure 3 shows thechange in EMG activity during brainstem electrical stimulation.In the postural (neck) (Fig. 3) muscle, three types of EMG activity,a brief suppression (A), a prolonged suppression (B), and sustainedatonia (C) were found during repetitive mesopontine stimulation.The responses of muscle tone to the mesopontine stimulation werenot site- and time-dependent. Stimulation of a single site couldproduce any type or any two and/or three combinations of muscleactivity during a single stimulation period. The percentage decreaseof integrated muscle activity in postural muscles during 5 mintrain stimulation ranged from 5 to 48% with an average of 18.7%from the baseline amplitude. In contrast to the postural muscles,mesopontine electrical stimulation never elicited sustained atoniain the respiratory-related muscles. In the genioglossus, mesopontinestimulation generated either a brief suppression (18 of 28 cases)or a prolonged suppression (10 of 28 cases) (Fig. 3) of muscleactivity. Both inspiratory activity and basal muscle tone of thegenioglossus were suppressed by brainstem electrical stimulation.The average reduction of integrated genioglossus muscle activityduring the 5 min repetitive brainstem stimulation was 22.4% fromthe baseline (Table 1). In the diaphragm, mesopontine electricalstimulation produced a brief suppression of muscle activity. Neithera prolonged suppression of inspiratory amplitude nor sustainedatonia was produced in the diaphragm by electrical stimulationof mesopontine inhibitory sites.

View larger version (26K):
[in this window]
[in a new window]
Figure 3. Electrical stimulation of the mesopontine reticular formation elicited muscle tone suppression in postural as well as respiratory muscles. Three hundred millisecond trains with 100 Hz, 0.2 msec, and 20 µA cathodal pulses were applied into the pontine inhibitory area. Three types of muscle tone suppression, a short (A), a prolonged (B) suppression, and atonia (C), in the neck muscle could be induced by mesopontine stimulation. However, a prolonged suppression in the genioglossus and a short period of suppression in the diaphragm were seen in all cases. DIP, diaphragm; GG, genioglossus muscle.


View this table:
[in this window]
[in a new window]
Table 1. Percentage of decrease in norepinephrine and serotonin release in the motoneuron pools and muscle activity during mesopontine inhibitory area stimulation

Electrical stimulation in the MLB produced ipsilateral facilitation and contralateral inhibition of the postural muscles,with no effect on the respiratory-related muscles. Neither respiratory-relatednor postural muscle activity was significantly changed when thestimulation was administered to the LDT andBC.

Muscle response to chemical stimulation in mesopontine reticular formation

Consistent with our previous study (Lai and Siegel, 1988), Ach microinjected into the PIA suppressed postural muscle tone.Respiratory muscle activity was also suppressed by PIA Ach injection(Fig. 4). Acetylcholine injection into the PIA suppressed bothinspiratory activity and basal muscle tone in the diaphragm (Fig.4) and genioglossus. Both the amplitude and duration of the inspiratoryphase of diaphragmatic activity were suppressed by pontine Achinjection. Pontine Ach injection-induced tone suppression hada latency of 47.8 ± 10.7 sec and duration of 4.8 ± 0.7 min inboth postural and respiratory-related muscles. The average decreaseof muscle tone was 31.7% in the genioglossus muscle and 42.5%in postural muscles from the baseline level (Table 1).

View larger version (28K):
[in this window]
[in a new window]
Figure 4. Acetylcholine injection into the PIA induced muscle tone suppression in the postural muscles and diaphragm (DIP). Both tonic and phasic inspiratory activity in the diaphragm were suppressed by the injection. A shows muscle activity before and during acetylcholine injection, B shows recovery of muscle tone, and C shows electrical stimulation into the same site of injection producing muscle tone suppression in both neck muscles and diaphragm. LOS, Left occipitoscapularis muscle; RS, right splenius muscle.

Effect of probe insertion

As with our previous study (Kodama et al., 1998), dialysates were collected 2-3 hr after probe insertion. Dialysates werecollected immediately before, during, and after stimulation thatinduced muscle tone suppression. The effects that were seen couldtherefore not be attributable to the insertion of the probes themselves.We continued collecting from dialysis sites for a mean of 24 hr.Differences between temporally adjacent baseline and stimulationresults obtained at the end of this period did not differ fromthose seen at the beginning. The studies lasted for 18-30hr.

Norepinephrine release in the hypoglossal nucleus and spinal cord

We found a reduction of NE release in both sides of the XII nucleus and spinal ventral horn during unilateral electrical stimulationof the PIA, MRF, and PPN that induced muscle tone suppression.Norepinephrine release during electrical stimulation induced muscletone suppression was significantly reduced from the baseline controllevels in the XII nucleus (p < 0.001; t = 3.2; df = 48) and spinalventral horn (p < 0.01; t = 2.6; df = 46) (Fig. 5). There wasno significant difference in the magnitude of the reduction inNE release between the sides ipsilateral and contralateral tothe stimulation. Reduction of NE release was of equal magnitudein samples collected from the rostral and caudal XII nucleus.The average percentage reduction of NE release was 25.4% in theXII nucleus and 18.9% in the spinal cord (Table 1).

View larger version (39K):
[in this window]
[in a new window]
Figure 5. Changes in norepinephrine release in both hypoglossal (black columns) nucleus and spinal ventral horn (white columns). Norepinephrine release was significantly decreased in the hypoglossal nucleus and spinal ventral during electrical stimulation applied into the pontine inhibitory area. Release of norepinephrine recovered to baseline levels by 10 min after stimulation. C, Baseline control; Stm, stimulation. $star$ p < 0.05.

Norepinephrine release in both sides of the XII nucleus (p > 0.9; t = 0.11; df = 13) and spinal cord (p > 0.7; t = 0.335;df = 15) was not changed when electrical stimulation was appliedto MLB, LDT, and BC sites, at which stimulation produced eitherunilateral or no effect on muscleactivity.

Serotonin release in the hypoglossal nucleus and spinal ventral horn

Significant decreases in 5-HT release in the XII nucleus (p < 0.05; t = 3.0; df = 50) and spinal ventral horn (p < 0.05; t= 2.3; df = 52) (Fig. 5) were found during electrical stimulationin the mesopontine inhibitory area. As with NE, 5-HT release inboth ipsilateral and contralateral as well as the rostral andcaudal XII nucleus showed a similar reduction. The percentagedecrease in 5-HT release in the XII nucleus and spinal cord was25.5 and 19.1%, respectively (Table 1).

Serotonin release in both sides of XII nucleus (p > 0.7; t = 0.322; df = 9) and spinal ventral horn (p > 0.5; t = 0.693; df= 11) was not changed when electrical stimulation was appliedto the MLB, LDT, and BC, areas that did not induce muscle tonesuppressionbilaterally.

Norepinephrine and 5-HT release in the motoneuron pools during PIA Ach-induced muscle tone suppression

As with electrical stimulation, Ach microinjected into the PIA also produced a significant decrease in NE (spinal cord: p< 0.05, t = 2.3, df = 9; XII nucleus: p < 0.05, t = 2.45, df =11) and 5-HT (spinal cord: p < 0.05, t = 3.07, df = 9; XII nucleus:p < 0.05, t = 2.28, df = 11) release in the motoneuron pools.The percentage decrease in NE release in the spinal cord was 22.4%and in the XII nucleus was 21.4% (Table 1). Reduction of 5-HTrelease in the spinal cord was 26.4% and in the XII nucleus was28.8% (Table 1).

Comparison of NE and 5-HT release in the XII nucleus and spinal cord

We compared the change of NE and 5-HT release in the XII nucleus and spinal cord during mesopontine electrical stimulationover consecutive 5 min epochs. In the XII nucleus, the magnitudeof the decrease in NE release was not different (F = 2.97; p =0.12; df = 1,10) from that of 5-HT release during mesopontinestimulation-induced muscle tone suppression. Similarly, no differencein the reduction of NE and 5-HT release (F = 1.85; p = 0.20; df= 1,10) in the spinal cord was found during mesopontine electricalstimulation induced decrease in muscle tone. We also comparedthe XII nucleus and spinal cord NE and 5-HT release during stimulation-inducedtone suppression. The magnitude of the decrease in NE releaseduring stimulation was not significantly different between theXII nucleus and spinal cord (F = 0.03; p = 0.87; df = 1,10). Similarly,the percentage change of 5-HT release in the XII nucleus and spinalcord was not significantly different (F = 0.19; p = 0.65; df =1,10) with pontinestimulation.

The time course of the reduction of NE and 5-HT release in both spinal cord and XII nucleus was compared. We found that bothNE and 5-HT release in the spinal cord returned to a level thatwas not significantly different from the baseline level afterthe stimulation, whereas hypoglossal levels remained below baselinefor 5 min (Figs. 5, 6).

View larger version (22K):
[in this window]
[in a new window]
Figure 6. Changes in serotonin release in both hypoglossal (black columns) nucleus and spinal ventral horn (white columns). Serotonin release was significantly decreased in the hypoglossal nucleus and spinal ventral horn during electrical stimulation applied into the pontine inhibitory area. Serotonin release recovered to baseline control levels by 10 min after stimulation. $star$ p < 0.05.

Dopamine release in the hypoglossal nucleus and spinal cord

Unlike NE and 5-HT, DA release in the motoneuron pools was unchanged during either electrical stimulation or Ach injectioninto the mesopontine inhibitory area. Dopamine release in theXII nucleus (electrical stimulation: p > 0.2, df = 15; Ach injection:p > 0.9, df = 11) and spinal cord (electrical stimulation: p >0.2, df = 15; Ach injection: p > 0.7, df = 9) (Fig. 7) duringmesopontine-induced muscle tone suppression was not significantlydifferent from the baseline control level.

View larger version (19K):
[in this window]
[in a new window]
Figure 7. Unchanged dopamine release in the hypoglossal nucleus (black columns) and spinal ventral horn (white columns) during brainstem electrical stimulation induced atonia.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the present study, we found that electrical stimulation of the PIA, PPN, and MRF, and Ach injection into the PIA produceda suppression of postural muscle tone, as reported in our previousstudies (Lai and Siegel, 1988, 1991, 1999). The same stimulationalso decreased muscle activity in the genioglossus and diaphragm.We found that mesopontine electrical and chemical stimulation-inducedmuscle tone suppression was accompanied by a reduction in NE and5-HT release in both spinal cord and XII nucleus. Although motoneuronsinnervating the hypoglossus, a tongue retractor, and genioglossus,a tongue protruder, are segregated within the anteroposteriorregions of the XII nucleus (Aldes, 1995; Dobbins and Feldman,1995), the same pattern of NE and 5-HT release suppression wasfound in the rostral and caudal portions of the XII nucleus duringatonia induced by mesopontine stimulation. This result indicatesthat monoaminergic mechanisms may be equally important in thecontrol of tongue muscles that have opposite physiological function.Previous studies showed that coactivation of the protruder andretractor tongue muscles is required to increase inspiratory flow(Eisele et al., 1997).

Although electrical stimulation in the mesopontine area produced muscle tone suppression in all recorded muscles, the patternof tone suppression was different in postural and respiratory-relatedmuscles. A brief and a prolonged suppression as well as a sustainedatonia seen in the present study in postural muscles was consistentwith our previous findings in the rat (Hajnik et al., 2000). Incontrast to the postural muscles, a sustained atonia was neverseen in the genioglossus or diaphragm during repetitive electricalstimulation of the mesopontine region. However, the postural andrespiratory muscles had the same latency and the same durationof tone suppression after Ach injection into thePIA.

Kubin et al. (1993) hypothesized that different mechanisms were responsible for the regulation of cranial and spinal motorsystems. They suggested that inactivation of the serotonergicsystem in the XII nucleus and activation of glycinergic mechanismin the spinal cord cause muscle tone suppression in the respiratoryand postural muscles during REM sleep, respectively. However,our present finding of decrease in NE and 5-HT release in bothXII nucleus and spinal ventral horn during mesopontine stimulation-inducedmuscle tone suppression indicates that both noradrenergic andserotoninergic systems may play an equal role in the regulationof cranial and spinal motoneuronactivity.

We hypothesize that the reduction of NE and 5-HT release in motor nuclei was related to muscle tone change, based on the followingconsiderations. First, the magnitude of reduction of NE and 5-HTrelease in the motoneuron pools was similar to the percentagedecrease in muscle tone. Second, electrical stimulation in a widespreadarea of the nervous system, cerebellum, periaqueductal gray, medullaryreticular formation, and cortex facilitates noradrenergic andserotoninergic neuron activity (Nakamura et al., 1980; Maciewiczet al., 1984; Morris, 1987). In contrast, we see a reduction ofNE and 5-HT release in the motoneuron pools only during pontinestimulation that produced a suppression of muscle tone. Third,carbachol injection into the PIA produces REM sleep-like activityand simultaneously decreases raphe neuronal activity in the chronicanimal and muscle atonia in the decerebrate animal (Steinfelset al., 1983). On the other hand, 5-HT microinfused into the XIInucleus increases genioglossus activity in the rat (Jelev et al.,2001). Fourth, NE and 5-HT have been shown to increase motoneuronexcitability in the rat and cat (White and Fung, 1989; Takahashiand Berger, 1990; Berger et al., 1992; Parkis et al., 1995). Microinfusionof NE generates an increase in masseteric reflex in behaving cats(Stafford and Jacobs, 1990). Finally, we did not see a reductionof NE and 5-HT release in the motoneuron pools when electricalstimulation was applied to brainstem areas that failed to producemuscle tone suppressionbilaterally.

Several monoaminergic cell groups within the brainstem could be responsible for the changes in monoamine release that we see.Electrical or chemical stimulation of the medullary raphe nucleusincreases XII nerve activity (Rose et al., 1995). Electrical stimulationin the LC complex produces an increase in hypoglossal nerve activity(Kuna and Remmers, 1999) and monosynaptic reflex amplitude inthe spinal cord (Lai et al., 1989) in decerebrate animals. EPSPscan be seen in spinal motoneurons after stimulation of the LC(Fung and Barnes, 1981, 1987). On the other hand, LC activityis reduced during the natural REM sleep state (Aston-Jones andBloom, 1981; Hobson et al., 1983) and systemic application ofeserine induced REM sleep-like state with atonia in decerebratecats (Pompeiano and Hoshino, 1976). Locus coeruleus neurons ceasedischarge during cataplexy, an abrupt loss of muscle tone duringwaking, seen in the narcoleptic dog (Wu et al., 1999). Lesionsin the LC or injection of clonidine, an $alpha$ ₂ receptor agonist thatinhibits noradrenergic neuron activity, into the LC reduces muscletone in decerebrate animals (Pompeiano et al., 1987; D'Ascanioet al., 1989). Intracerebroventricular administration of 5,7-dihydroxytryptamine,a 5-HT neurotoxin, decreases muscle tone in the decerebrate rat(Sakai et al., 2000).

Electrical stimulation of a number of nuclei within the mesopontine area, including MRF, PPN, and PIA, has been shown to suppressNE and 5-HT release in the present study. Anatomically, neuronsin the MRF, PPN, and PIA project to the medullary raphe nuclei(Gallager and Pert, 1978; Carlton et al., 1983) and LC complex(Sugaya et al., 1988; Kohama, 1992). Alternatively, neurons inthe MRF and PPN project to the PIA (Lai et al., 1993), which inturn projects to the monoaminergic nuclei in the brainstem (Gallagerand Pert, 1978; Carlton et al., 1983; Sugaya et al., 1988; Kohama,1992). Monoaminergic projections from the LC complex to the motoneuronpools have been identified (Lai and Barnes, 1985; Aldes et al.,1992). Projections from A5 and A7 (Fritschy and Grzanna, 1990;Aldes et al., 1992) and medullary raphe nuclei (Basbaum and Fields,1979; Manaker and Tischler, 1993) have also been seen. We hypothesizethat activation of the PIA inhibits the activity of noradrenergicand serotonergic neurons that project to the motoneuron pools.Our previous work demonstrated that electrical stimulation inthe PIA induces an increase in GABA release in the rodent LC anddecreases discharge in LC neurons (Mileykovskiy et al., 2000).We also found that GABA is released onto LC and raphe neuronsduring their period of discharge cessation in REM sleep (Nitzand Siegel, 1997a,b). Lesions of the PIA that produce REM sleepwithout atonia cause dorsal raphe cells, normally silent in REMsleep, to become tonically active during REM sleep (Trulson etal., 1981). Thus, elicitation of atonia in the decerebrate animalis linked to cessation of monoamine release. The reduction inmonoamine release along with a simultaneous release of glycine(Kawai and Sasaki, 1964; Chase et al., 1989) and GABA (Bruggencateand Sonnhof, 1972) onto motoneurons would cause hyperpolarizationand muscleatonia.

Dopaminergic terminals are present in the spinal ventral horn (Holstege et al., 1996). However, we saw no change of DA releasein either XII nucleus or spinal ventral horn during mesopontinestimulation in our present study. Unit recording studies haveshown little change in the activity of mesencephalic DA cell acrossthe sleep cycle (Steinfels et al., 1981; Miller et al., 1983)despite the suppression of muscle tone in REM sleep. However,changes in DA release in the motoneuron pools during sleep cannotbe ruled out. Terminal release from DA neurons may be independentof somatic action potentials (Verma and Moghaddam, 1998). Thehypothalamic A11 group has been identified as a major source ofdescending dopaminergic input to the motoneuron pools (Hokfeltet al., 1979; Skagerberg and Lindvall, 1985). Unchanged DA releasein the motor nuclei during mesopontine stimulation could be attributableto the absence of the hypothalamic A11 group in our decerebratepreparation. Studies in the intact animal would be necessary totest thishypothesis.

In conclusion, we found that the reduction of muscle tone seen in the postural muscles during electrical stimulation of thepons also affects the accessory respiratory musculature. We finddecreased release of NE and 5-HT in both XII nucleus and spinalcord during muscle tone suppression. These findings lead us tosuggest that mesopontine-induced postural and respiratory-relatedmuscle tone suppression is mediated partially through a disfacilitatoryeffect caused by a reduction in 5-HT and NE release onto motoneuronsand that the mechanisms responsible for this link are containedin the brainstem. The tone in the upper airway muscles is minimalin REM sleep (Orem and Lydic, 1978; Remmers et al., 1978). Thisreduction in tone increases airway resistance in sleep comparedwith waking (Orem et al., 1977). In individuals with relativelysmall airways, this leads to sleep apnea (McGinty et al., 1982;Horner, 1996). Pharmacological activation of NE and 5-HT receptorsmight be a useful approach to increasing airway muscle tone duringsleep.

  FOOTNOTES

Received March 26, 2001; revised June 26, 2001; accepted July 5, 2001.

This work supported by United States Public Health Service Grants HL 41370 and HL 60296 and the Department of VeteransAffairs.
Correspondence should be addressed to Y. Y. Lai, Neurobiology Research (151A3), Veterans Affairs, Greater Los Angeles HealthCare System Sepulveda, 16111 Plummer Street, North Hills, CA 91343.E-mail: yylai{at}ucla.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aldes LD (1995) Subcompartmental organization of the ventral (protrusor) compartment in the hypoglossal nucleus of the rat. J Comp Neurol 353:89-108[Web of Science][Medline].
Aldes LD, Chapman ME, Chronister RB, Haycock JW (1992) Sources of noradrenergic afferents to the hypoglossal nucleus in the rat. Brain Res Bull 29:931-942[Web of Science][Medline].
Aston-Jones G, Bloom FE (1981) Activity of norepinephrine-containing locus coeruleus neurons in behaving rats anticipates fluctuations in the sleep-waking cycle. J Neurosci 1:876-886[Abstract].
Baker RG, Anderson EG (1972) The effect of L-3,4-dihydroxy-phenylalanine on spinal reflex activity. J Pharmacol Exp Ther 173:212-223[Abstract/Free Full Text].
Basbaum AI, Fields HL (1979) The origin of descending pathways in the dorsolateral funiculus of the spinal cord of the cat and rat: further studies on the anatomy of pain modulation. J Comp Neurol 187:513-532[Web of Science][Medline].
Berger AJ, Bayliss DA, Viana F (1992) Modulation of neonatal rat hypoglossal motoneuron excitability by serotonin. Neurosci Lett 143:164-168[Web of Science][Medline].
Berman AL (1968) In: The brainstem of the cat. Madison, WI: University of Wisconsin.
Bowker RM, Westlund KN, Sullivan MC, Coulter JD (1982) Organization of descending serotonergic projections to the spinal cord. Prog Brain Res 57:239-265[Web of Science][Medline].
Bruggencate G ten, Sonnhof U (1972) Effect of glycine and GABA, and blocking actions of strychnine and picrotoxin in the hypoglossus nucleus. Pflügers Arch 334:240-252[Medline].
Carlton SM, Leichnetz GR, Young EG, Mayer DJ (1983) Supramedullary afferents of the nucleus raphe magnus in the rat: a study using the transcannula HRP gel and autoradiographic techniques. J Comp Neurol 214:43-58[Web of Science][Medline].
Chase MH, Soja PJ, Morales FR (1989) Evidence that glycine mediates the postsynaptic potentials that inhibit lumbar motoneurons during the atonia of active sleep. J Neurosci 9:743-751[Abstract].
D'Ascanio P, Pompeiano M, Tononi G (1989) Inhibition of vestibulospinal reflexes during the episodes of postural atonia induced by unilateral lesion of the locus coeruleus in the decerebrate cat. Arch Ital Biol 127:81-97[Medline].
Dobbins EG, Feldman JL (1995) Differential innervation of protruder and retractor muscles of the tongue in rat. J Comp Neurol 357:376-394[Web of Science][Medline].
Eisele DW, Smith PL, Alam DS, Schwartz AR (1997) Direct hypoglossal nerve stimulation in obstructive sleep apnoea. Arch Otolaryngol Head Neck Surg 123:57-61.
Fritschy J-M, Grzanna R (1990) Demonstration of two separate descending noradrenergic pathways to the rat spinal cord: evidence for an intragriseal trajectory of locus coeruleus axons in the superficial layers of the dorsal horn. J Comp Neurol 291:553-582[Web of Science][Medline].
Fung SJ, Barnes CD (1981) Evidence of facilitatory coerulospinal action in lumbar motoneurons of cats. Brain Res 216:299-311[Web of Science][Medline].
Fung SJ, Barnes CD (1987) Membrane excitability changes in hindlimb motoneurons induced by stimulation of the locus coeruleus in cats. Brain Res 402:230-242[Web of Science][Medline].
Fung SJ, Barnes CD (1989) Raphe-produced excitation of spinal cord motoneurons in the cat. Neurosci Lett 103:185-190[Web of Science][Medline].
Gallager DW, Pert A (1978) Afferents to brain stem nuclei (brain stem raphe, nucleus reticularis pontis caudalis and nucleus gigantocellularis) in the rat as demonstrated by microiontophoretically applied horseradish peroxidase. Brain Res 144:257-275[Web of Science][Medline].
George R, Haslett WL, Jenden DJ (1964) A cholinergic mechanism in the brainstem reticular formation: induction of paradoxical sleep. Int J Neuropharmacol 3:541-552.
Hajnik T, Lai YY, Siegel JM (2000) Atonia related regions in the rodent pons and medulla. J Neurophysiol 84:1942-1948[Abstract/Free Full Text].
Henley K, Morrison AR (1974) A re-evaluation of the effects of lesions of the pontine tegmentum and locus coeruleus on phenomena of paradoxical sleep in the cat. Acta Neurobiol Exp 34:215-232[Medline].
Hobson JA, McCarley RW, Nelson JP (1983) Location and spike-train characteristics of cells in anterodorsal pons having selective decreases in firing rate during desynchronized sleep. J Neurophysiol 50:770-783[Abstract/Free Full Text].
Hokfelt T, Phillipson O, Goldstein (1979) Evidence for a dopaminergic pathway in the rat descending from the A11 cell group to the spinal cord. Acta Physiol Scand 107:393-395[Web of Science][Medline].
Holstege JC, van Dljken H, Buijs RM, Goedknegt H, Gosens T, Bongers CMH (1996) Distribution of dopamine immunoreactivity in the rat, cat, and monkey spinal cord. J Comp Neurol 376:631-652[Web of Science][Medline].
Horner RL (1996) Motor control of the pharyngeal musculature and implications for the pathogenesis of obstructive sleep apnea. Sleep 19:827-853[Web of Science][Medline].
Jelev A, Sood S, Liu H, Nolan P, Horner RL (2001) Microdialysis perfusion of 5-HT into hypoglossal motor nucleus differentially modulates genioglossus activity across natural sleep-wake states in rats. J Physiol (Lond) 532:467-481[Abstract/Free Full Text].
Jouvet M, Delorme F (1965) locus coeruleus et sommeil paradoxal. C R Soc Biol 159:895-899.
Kawai I, Sasaki K (1964) Effects of strychnine upon supraspinal inhibition. Jpn J Physiol 14:309-317.
Kodama T, Lai YY, Siegel JM (1998) Enhanced glutamate release during REM sleep in the rostromedial medulla as measured by in vivo microdialysis. Brain Res 780:178-181[Web of Science][Medline].
Kohama T (1992) Neuroanatomical studies on the urine storage facilitatory areas in the cat brain, part I: input neuronal structures to the nucleus locus subcoeruleus and the nucleus reticularis pontis oralis. Jpn J Urol 83:1469-1477.
Kubin L, Kimura H, Tojima H, Davies RO, Pack AI (1993) Suppression of hypoglossal motoneurons during the carbachol-induced atonia of REM sleep is not caused by fast synaptic inhibition. Brain Res 611:300-312[Web of Science][Medline].
Kuna ST, Remmers JE (1999) Premotor input to hypoglossal motoneurons from Kolliker-Fuse neurons in decerebrate cats. Respir Physiol 117:85-95[Web of Science][Medline].
Lai YY, Barnes CD (1985) A spinal projection of serotonergic neurons of the locus coeruleus in the cat. Neurosci Lett 58:159-164[Medline].
Lai YY, Siegel JM (1988) Medullary regions mediating atonia. J Neurosci 8:4790-4796[Abstract].
Lai YY, Siegel JM (1990) Muscle tone suppression and stepping produced by stimulation of midbrain and rostral pontine reticular formation. J Neurosci 10:2727-2734[Abstract].
Lai YY, Siegel JM (1991) Pontomedullary glutamate receptors mediating locomotion and muscle tone suppression. J Neurosci 11:2931-2937[Abstract].
Lai YY, Siegel JM (1999) Muscle atonia and REM sleep. In: Rapid eye movement sleep (Mallick BN, Inoue S, eds), pp 69-90. New Delhi, India: Narosa.
Lai YY, Strahlendorf HK, Fung SJ, Barnes CD (1989) The actions of two monoamines on spinal motoneurons from stimulation of the locus coeruleus. Brain Res 484:268-272[Web of Science][Medline].
Lai YY, Clements JR, Siegel JM (1993) Glutamatergic and cholinergic projections to the pontine inhibitory area identified with horseradish peroxidase retrograde transport and immunohistochemistry. J Comp Neurol 336:321-330[Web of Science][Medline].
Maciewicz R, Sandrew BB, Phipps BS, Poletti CE, Foote WE (1984) Pontomedullary raphe neurons: intracellular responses to central and peripheral electrical stimulation. Brain Res 293:17-33[Web of Science][Medline].
Magoun HW, Rhines R (1946) An inhibitory mechanism in the bulbar reticular formation. J Neurophysiol 9:165-171[Free Full Text].
Manaker S, Tischler LJ (1993) Origin of serotoninergic afferents to the hypoglossal nucleus in the rat. J Comp Neurol 334:466-476[Web of Science][Medline].
McGinty D, Littner M, Beahm E, Ruiz-Primo E, Young E, Sowers J (1982) Sleep related breathing disorders in older men. Neurobiol Aging 3:337-350[Web of Science][Medline].
Mileykovskiy BY, Kiyashchenko LI, Kodama T, Lai YY, Siegel JM (2000) Activation of pontine and medullary motor inhibitory regions reduces discharge in neurons located in the locus coeruleus and the anatomical equivalent of the midbrain locomotor region. J Neurosci 20:8551-8558[Abstract/Free Full Text].
Miller JD, Farber J, Gatz P, Roffwarg H, German DC (1983) Activity of mesencephalic dopamine and non-dopamine neurons across stages of sleep and waking in the rat. Brain Res 273:133-141[Web of Science][Medline].
Morris R (1987) Responses of neurones in the brainstem raphe nuclei to stimulation of the cerebellar fastigial nuclei in the cat. Neurosci Lett 74:19-24[Medline].
Nagase Y, Moritani M, Nakagawa S, Yoshida A, Takemura M, Zhang L-F, Kida H, Shigenaga Y (1997) Serotonergic axonal contacts on identified cat trigeminal motoneurons and their correlation with medullary raphe nucleus stimulation. J Comp Neurol 384:443-455[Web of Science][Medline].
Nakamura S, Tsai C, Iwama K (1980) Recurrent facilitation of locus coeruleus neurons of the rat. In: The reticular formation revisited (Hobson JA, Brazier MAB, eds), pp 303-315. New York: Raven.
Nitz D, Siegel JM (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[Web of Science][Medline].
Orem J, Lydic R (1978) Upper airway function during sleep and wakefulness: experimental studies on normal and anesthetized cats. Sleep 1:49-68[Web of Science][Medline].
Orem J, Netick A, Dement WC (1977) Breathing during sleep and wakefulness in the cat. Respir Physiol 30:265-289[Web of Science][Medline].
Parkis MA, Bayliss DA, Berger AJ (1995) Actions of norepinephrine on rat hypoglossal motoneurons. J Neurophysiol 74:1911-1919[Abstract/Free Full Text].
Pompeiano O, Hoshino K (1976) Central control of posture: reciprocal discharge by two pontine neuronal groups leading to suppression of decerebrate rigidity. Brain Res 116:131-138[Medline].
Pompeiano O, D'Ascanio P, Horn E, Stampacchia G (1987) Effects of local injection of the $alpha$ ₂-adrenergic agonist clonidine into the locus coeruleus complex on the gain of vestibulospinal and cervicospinal reflexes in decerebrate cats. Arch Ital Biol 125:225-289[Medline].
Remmers JE, DeGroot WJ, Sauerland EK, Anch AM (1978) Pathogenesis of upper airway occlusion during sleep. J Appl Physiol 44:931-938[Free Full Text].
Rose D, Khater-Boidin J, Toussaint P, Duron B (1995) Central effect of 5-HT on respiratory and hypoglossal activities in the adult cat. Respir Physiol 101:59-69[Web of Science][Medline].
Sakai K, Sastre J-P, Kanamori N, Jouvet M (1981) State-specific neurons in the ponto-medullary reticular formation with special reference to the postural atonia during paradoxical sleep in the cat. In: Brain mechanisms and perceptual awareness (Pompeiano O, Marsan CA, eds), pp 405-429. New York: Raven.
Sakai M, Matsunaga M, Kubota A, Yamanishi Y, Nishsizama Y (2000) Reduction in excessive muscle tone by selective depletion of serotonin in intercollicularly decerebrated rats. Brain Res 860:104-111[Web of Science][Medline].
Siegel JM, Nienhuis R, Wheeler RL, McGinty DJ, Harper RM (1981) Discharge pattern of reticular formation unit pairs in waking and REM sleep. Exp Neurol 74:875-891[Web of Science][Medline].
Skagerberg G, Lindvall O (1985) Organization of diencephalic dopamine neurons projecting to the spinal cord in the rat. Brain Res 342:340-351[Web of Science][Medline].
Soja PJ, Morales FR, Baranyi A, Chase MH (1987) Effect of inhibitory amino acid antagonists on IPSPs induced in lumbar motoneurons upon stimulation of the nucleus reticularis gigantocellularis during active sleep. Brain Res 423:353-358[Web of Science][Medline].
Soja PJ, Lopez-Rodriguez F, Morales FR, Chase MH (1991) The postsynaptic inhibitory control of lumbar motoneurons during the atonia of active sleep: effect of strychnine on motoneuron properties. J Neurosci 11:2804-2811[Abstract].
Stafford IL, Jacobs BL (1990) Noradrenergic modulation of the masseteric reflex in behaving cat. J Neurosci 10:91-98[Abstract].
Steinfels GF, Heym J, Jacobs BL (1981) Single unit activity of dopaminergic neurons in freely moving cats. Life Sci 29:1435-1442[Web of Science][Medline].
Steinfels GF, Heym J, Strecker RE, Jacobs BL (1983) Raphe unit activity in freely moving cats is altered by manipulations of central but not peripheral motor systems. Brain Res 279:77-84[Web of Science][Medline].
Sugaya K, Mori S, Tsuchida S (1988) Input and output neuronal structures of the pontine micturition center. Part I. Mainly input neuronal structures. Jpn J Urol 79:1210-1218.
Takahashi T, Berger AJ (1990) Direct excitation of rat spinal motoneurones by serotonin. J Physiol (Lond) 423:63-76[Abstract/Free Full Text].
Trulson ME, Jacobs BL, Morrison AR (1981) Raphe unit activity during REM sleep in normal cats and in pontine lesioned cats displaying REM sleep without atonia. Brain Res 226:75-91[Web of Science][Medline].
Van Dongen PAM, Broekkamp CLE, Cools AR (1978) Atonia after carbachol microinjections near the locus coeruleus in cats. Pharmacol Biochem Behav 8:527-532[Medline].
Verma A, Moghaddam B (1998) Regulation of striatal dopamine release by metabotropic glutamate receptors. Synapse 28:220-226[Medline].
White SR, Fung SJ (1989) Serotonin depolarizes cat spinal motoneurons in situ and decreases motoneuron afterhyperpolarizing potentials. Brain Res 502:205-213[Web of Science][Medline].
Wu M-F, Gulyani SA, Yau E, Mignot E, Phan B, Siegel JM (1999) Locus coeruleus neurons: cessation of activity during cataplexy. Neuroscience 91:1389-1399[Web of Science][Medline].
Yamuy J, Fung SJ, Xi M, Morales FR, Chase MH (1999) Hypoglossal motoneurons are postsynaptically inhibited during carbachol-induced rapid eye movement sleep. Neuroscience 94:11-15[Web of Science][Medline].

Copyright © 2001 Society for Neuroscience 0270-6474/01/21187384-08$05.00/0

This article has been cited by other articles:

N. Taepavarapruk, P. Taepavarapruk, J. John, Y. Y. Lai, J. M. Siegel, A. G. Phillips, S. A. McErlane, and P. J. Soja
State-Dependent Changes in Glutamate, Glycine, GABA, and Dopamine Levels in Cat Lumbar Spinal Cord
J Neurophysiol, August 1, 2008; 100(2): 598 - 608.
[Abstract] [Full Text] [PDF]

C. Burgess, D. Lai, J. Siegel, and J. Peever
An Endogenous Glutamatergic Drive onto Somatic Motoneurons Contributes to the Stereotypical Pattern of Muscle Tone across the Sleep-Wake Cycle
J. Neurosci., April 30, 2008; 28(18): 4649 - 4660.
[Abstract] [Full Text] [PDF]

P. L. Brooks and J. H. Peever
Glycinergic and GABAA-Mediated Inhibition of Somatic Motoneurons Does Not Mediate Rapid Eye Movement Sleep Motor Atonia
J. Neurosci., April 2, 2008; 28(14): 3535 - 3545.
[Abstract] [Full Text] [PDF]

Y. Zhu, P. Fenik, G. Zhan, E. Mazza, M. Kelz, G. Aston-Jones, and S. C. Veasey
Selective Loss of Catecholaminergic Wake Active Neurons in a Murine Sleep Apnea Model
J. Neurosci., September 12, 2007; 27(37): 10060 - 10071.
[Abstract] [Full Text] [PDF]

E. Chan, H. W. Steenland, H. Liu, and R. L. Horner
Endogenous Excitatory Drive Modulating Respiratory Muscle Activity across Sleep-Wake States
Am. J. Respir. Crit. Care Med., December 1, 2006; 174(11): 1264 - 1273.
[Abstract] [Full Text] [PDF]

A. J. Fuglevand, A. P. Dutoit, R. K. Johns, and D. A. Keen
Evaluation of plateau-potential-mediated 'warm up' in human motor units
J. Physiol., March 15, 2006; 571(3): 683 - 693.
[Abstract] [Full Text] [PDF]

S. Sood, J. L. Morrison, H. Liu, and R. L. Horner
Role of Endogenous Serotonin in Modulating Genioglossus Muscle Activity in Awake and Sleeping Rats
Am. J. Respir. Crit. Care Med., November 15, 2005; 172(10): 1338 - 1347.
[Abstract] [Full Text] [PDF]

V. B. Fenik, R. O. Davies, and L. Kubin
REM Sleep-like Atonia of Hypoglossal (XII) Motoneurons Is Caused by Loss of Noradrenergic and Serotonergic Inputs
Am. J. Respir. Crit. Care Med., November 15, 2005; 172(10): 1322 - 1330.
[Abstract] [Full Text] [PDF]

K. Takakusaki, K. Takahashi, K. Saitoh, H. Harada, T. Okumura, Y. Kayama, and Y. Koyama
Orexinergic projections to the cat midbrain mediate alternation of emotional behavioural states from locomotion to cataplexy
J. Physiol., November 1, 2005; 568(3): 1003 - 1020.
[Abstract] [Full Text] [PDF]

M.-F. Wu, J. John, L. N. Boehmer, D. Yau, G. B. Nguyen, and J. M. Siegel
Activity of dorsal raphe cells across the sleep-waking cycle and during cataplexy in narcoleptic dogs
J. Physiol., January 1, 2004; 554(1): 202 - 215.
[Abstract] [Full Text] [PDF]

V. A Bouryi and D. I Lewis
The modulation by 5-HT of glutamatergic inputs from the raphe pallidus to rat hypoglossal motoneurones, in vitro
J. Physiol., December 15, 2003; 553(3): 1019 - 1031.
[Abstract] [Full Text] [PDF]

J. L Morrison, S. Sood, H. Liu, E. Park, X. Liu, P. Nolan, and R. L Horner
Role of inhibitory amino acids in control of hypoglossal motor outflow to genioglossus muscle in naturally sleeping rats
J. Physiol., November 1, 2003; 552(3): 975 - 991.
[Abstract] [Full Text] [PDF]

I. D. Hentall, R. Mesigil, A. Pinzon, and B. R. Noga
Temporal and Spatial Profiles of Pontine-Evoked Monoamine Release in the Rat's Spinal Cord
J Neurophysiol, June 1, 2003; 89(6): 2943 - 2951.
[Abstract] [Full Text] [PDF]

T. Kodama, Y.-Y. Lai, and J. M. Siegel
Changes in Inhibitory Amino Acid Release Linked to Pontine-Induced Atonia: An In Vivo Microdialysis Study
J. Neurosci., February 15, 2003; 23(4): 1548 - 1554.
[Abstract] [Full Text] [PDF]

B. Y Mileykovskiy, L. I Kiyashchenko, and J. M Siegel
Cessation of activity in red nucleus neurons during stimulation of the medial medulla in decerebrate rats
J. Physiol., December 15, 2002; 545(3): 997 - 1006.
[Abstract] [Full Text] [PDF]

V. Fenik, V. Marchenko, P. Janssen, R. O. Davies, and L. Kubin
A5 cells are silenced when REM sleep-like signs are elicited by pontine carbachol
J Appl Physiol, October 1, 2002; 93(4): 1448 - 1456.
[Abstract] [Full Text] [PDF]

J. Kong, P. N. Shepel, C. P. Holden, M. Mackiewicz, A. I. Pack, and J. D. Geiger
Brain Glycogen Decreases with Increased Periods of Wakefulness: Implications for Homeostatic Drive to Sleep
J. Neurosci., July 1, 2002; 22(13): 5581 - 5587.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (42)

Citing Articles via Google Scholar

Google Scholar

Articles by Lai, Y.-Y.

Articles by Siegel, J. M.

Search for Related Content

PubMed

PubMed Citation

Articles by Lai, Y.-Y.

Articles by Siegel, J. M.