Postsynaptic Muscarinic M1 Receptors Activate Prefrontal Cortical EEG of C57BL/6J Mouse

doi:10.1152/jn.00318.2002

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Postsynaptic Muscarinic M1 Receptors Activate Prefrontal Cortical EEG of C57BL/6J Mouse

Christopher L. Douglas,¹^,² Helen A. Baghdoyan,¹ and Ralph Lydic¹

¹Department of Anesthesiology, University of Michigan, Ann Arbor, Michigan 48109; and ²Department of Neuroscience and Anatomy, The Pennsylvania State University, College of Medicine, Hershey, Pennsylvania 17033

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Douglas, Christopher L., Helen A. Baghdoyan, and Ralph Lydic. Postsynaptic Muscarinic M1 Receptors Activate Prefrontal Cortical EEG of C57BL/6J Mouse. J. Neurophysiol. 88: 3003-3009, 2002. Recent pharmacological studies exploring the functional roles of muscarinic cholinergic receptor (mAChR) subtypes in prefrontalcortex of C57BL/6J (B6) mouse have provided evidence for a presynapticM2 autoreceptor. The B6 mouse was chosen for these studies becauseit is a genetically well-characterized model that also providesthe genomic background for many genetically modified mice. Inaddition to increasing ACh release, one functional consequenceof pharmacologically blocking the cortical M2 autoreceptor isactivation of the contralateral prefrontal cortical EEG. To date,the mechanisms through which M2 autoreceptor antagonism causescortical EEG activation have not been investigated. The presentstudy tested the hypothesis that, in the B6 mouse, prefrontalcortical ACh activates the contralateral prefrontal EEG via postsynapticM1 receptors. This hypothesis was tested in 15 mice using in vivomicrodialysis delivery of muscarinic antagonists with simultaneousquantification of ACh release, number of 7- to 14-Hz EEG spindles,and fast Fourier transformation analysis of prefrontal EEG. Dialysisdelivery of the nonsubtype selective muscarinic antagonist scopolamine(10 nM) significantly (P = 0.01) increased ACh release. QuantitativeEEG analysis showed that scopolamine did not alter contralateralprefrontal cortical EEG. To differentiate mAChR subtypes mediatingpre- versus postsynaptic responses, additional experiments usedmuscarinic antagonists with different affinities for the fivemAChR subtypes. Microdialysis delivery of 3 nM AF-DX 116, a muscarinicantagonist with relatively high affinity for the M2 and M4 subtypes,significantly (P < 0.01) increased prefrontal cortical ACh releaseand activated EEG in the contralateral prefrontal cortex. EEGactivation was characterized by a significant decrease in numberof 7- to 14-Hz EEG spindles (P < 0.0001) and power (Vrms) of EEGslow waves (P < 0.05). Microdialysis delivery of 3 nM AF-DX 116plus 3 nM pirenzepine, a relatively selective M1 and M4 muscarinicantagonist, also significantly (P < 0.01) increased ACh releasebut did not decrease the number of EEG spindles and did not changeEEG slow waves. The differential EEG and ACh responses to dialysisdelivery of the muscarinic antagonists support the conclusionthat, in B6 mouse, postsynaptic muscarinic receptors of the M1subtype are a primary site by which ACh activates theEEG.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Following discovery of the ascending reticular activating system (Moruzzi and Magoun 1949), ACh was postulated as a principalneurotransmitter regulating sleep-wake and anesthetically inducedalterations in arousal (Domino et al. 1968; Krnjevic 1967). Thispostulate emerged from the findings that ACh excites corticalneurons (Krnjevic 1967) and that cortical levels of ACh are positivelycorrelated with an activated EEG (Jasper and Tessier 1971; Marrosuet al. 1995). Volatile anesthetics that diminish behavioral arousaland deactivate the cortical EEG (Mitchell 1963) also decreaselevels of ACh in the cortex (Griffiths et al. 1995).

Many effects of ACh in the neocortex are mediated by muscarinic cholinergic receptors (mAChRs). There are five subtypes ofmAChRs identified pharmacologically and molecularly as M1-M5 (reviewedin Caulfield and Birdsall 1998). The M1 and M2 receptors are themost abundant subtypes in mammalian cortex (Levey et al. 1991),but the cellular distribution of these receptors has not beenfully elucidated. Electron and light microscopic studies in nonhumanprimates and in rat have localized some M2 receptors to the presynapticterminals of cortical neurons (reviewed in Levey 1996). In mouse,in vivo (Douglas et al. 2001) and in vitro (Zhang et al. 2002)studies have provided evidence that the M2 subtype acts as a cholinergicautoreceptor in cortex. Further studies have demonstrated thatone functional consequence of increasing ACh release by deliveringan M2 antagonist into one prefrontal cortex is activation of thecontralateral cortical EEG (Douglas et al. 2002). These data raisean important question. In prefrontal cortex ipsilateral to autoreceptorenhanced ACh release, what postsynaptic receptors mediate EEGactivation in the contralateral prefrontal cortex? Therefore thepresent study tested the hypothesis that prefrontal cortical AChactivates the contralateral prefrontal EEG via postsynaptic M1receptors.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Animal preparation for simultaneous EEG recordings and microdialysis

All experiments were conducted in accordance with the Guide for the Care and Use of Laboratory Animals (National Academy ofSciences Press 1996). Fifteen adult male C57BL/6J (B6) mice (JacksonLabs, Bar Harbor, ME) were anesthetized with 2.5% halothane in100% O₂ and held in a David Kopf (Tujunga, CA) stereotaxic frame.Autonomic signs (core body temperature and respiratory rate) weremonitored during anesthesia. Delivered halothane was maintainedat 1.8% during all experiments as measured by a Raman spectrometer(Ohmeda Rascal II, Louisville, CO). A small craniotomy was createdto provide access to the prefrontal cortex, identified as FrAin the stereotaxic atlas (Paxinos and Franklin 2001). A CMA/11microdialysis probe (membrane: 1 mm long by 240-µm diam, 6 kDacutoff; CMA Microdialysis, North Chelmsford, MA) was aimed fora site 3.0 mm anterior to bregma and 1.6 mm lateral to the midline.The vertical descent of the probe was guided visually such thatthe dialysis probe membrane rested fully within the cortex. Twoadditional craniotomies directly opposite the microdialysis probe(3.0 mm anterior to bregma and 0.5 and 1.5 mm lateral to the midline)allowed placement of two 0.13-mm-diam stainless steel wire (CaliforniaFine Wire Company, Grover City, CA) electrodes for recording prefrontalcorticalEEG.

Microdialysis and HPLC with electrochemical detection (EC)

Ringer solution (147 mM NaCl, 2.4 mM CaCl₂, 4.0 mM KCl, and 10 µM neostigmine) constantly perfused the microdialysis probeat a rate of 2.0 µl/min. At intervals of 12.5 min, 25 µl dialysissamples from prefrontal cortex were injected into an HPLC/EC system[Bioanalytical Systems (BAS), West Lafayette, IN] for quantificationof ACh. Following injection, a 50 mM Na₂HPO₄ mobile phase carriedthe microdialysis sample to a reversed-phase column that separatedACh and choline based on size and hydrophobicity. The separatedACh and choline then passed through an immobilized enzyme reactioncolumn that converted them to equimolar amounts of hydrogen peroxide.An applied potential of 0.5 V (in reference to a Ag⁺/AgCl electrode) ionized the hydrogen peroxide and the resultingsignal created a chromatographic peak that was digitized usingChromGraph (BAS) software. Integration of the chromatogram yieldeda measurement of the area under the chromatographic peaks andACh was quantified as pmol/12.5 min using a standard curve producedbefore each experiment. The percentage of a known ACh solutionrecovered by each probe was measured before and after every experiment.If pre- and postexperimental probe recoveries were significantlydifferent according to t-test, the data were discarded. CorticalACh release was quantified initially in each mouse during dialysiswith Ringer solution alone (control). A CMA/110 liquid switchthen was activated to deliver Ringer containing muscarinic antagonists.In this way, each mouse served as its own control for quantifyingdependentmeasures.

Identifying functional roles of mAChR subtypes

The goal of the present study was to use an in vivo pharmacological approach to identify the mAChR subtype or subtypes mediatingthe ACh-induced activation of prefrontal cortical EEG. One limitationfor all studies aiming to identify functional roles of mAChRsis the lack of subtype-specific ligands. The selectivity of availablemuscarinic antagonists for the five mAChR subtypes is concentrationdependent (Caulfield and Birdsall 1998). Thus inferences regardingmAChR subtypes require determining the relative potencies of arange of concentrations of different mAChR antagonists for elicitingthe response of interest (Baghdoyan and Lydic 1999; Billard etal. 1995; Douglas et al. 2001).

A previous study used the approach described above to conclude that the M2 subtype functions as an autoreceptor in prefrontalcortex of B6 mouse (Douglas et al. 2001). In that study, the relativepotencies of scopolamine, AF-DX 116, and pirenzepine for increasingACh release were determined. Scopolamine is a muscarinic antagonistwith equal and high affinity for the five mAChR subtypes (Billardet al. 1995; Jones et al. 1992) and therefore was expected toantagonize all five subtypes. Scopolamine (3 nM) increased AChrelease in prefrontal cortex (Douglas et al. 2001). AF-DX 116has relatively high affinity for the M2 or M4 subtype mAChRs andmuch lower affinity for M1, M3, and M5 receptors (Billard et al.1995; Jones et al. 1992). Pirenzepine has relatively high affinityfor the M1 and M4 mAChRs and much lower affinity for the othermAChR subtypes (Billard et al. 1995; Jones et al. 1992). The lowestconcentration of AF-DX 116 that increased ACh release was 3 nM,which is closest to its affinity for the M2 subtype (Billard etal. 1995). The lowest effective concentration of pirenzepine forincreasing ACh release was 300 nM (Douglas et al. 2001), whichalso is closest to its affinity for the M2 subtype (Billard etal. 1995). Therefore increased ACh release was likely due to antagonismof the M2 receptorsubtype.

In the present study, the muscarinic antagonists scopolamine methyl bromide (10 nM, Sigma-Aldrich Corp., St Louis, MO), pirenzepinedihydrochloride (3 nM, Sigma), and AF-DX 116 (3 nM, Boehringer-Ingelheim,Ridgefield, CT) were diluted in Ringer solution before beginningeach experiment, as previously described (Douglas et al. 2001).Scopolamine was delivered at a concentration of 10 nM to ensureantagonism of all five mAChR subtypes. AF-DX 116 was used at aconcentration of 3 nM to block M2 and M4 subtypes. Pirenzepineat 3 nM would be expected to block M1 and M4 subtypes. Muscarinicantagonists were delivered by reverse dialysis via the same probesused to collect ACh. This made it possible to determine the relativeeffects of each antagonist on ipsilateral ACh release and on activationof the contralateral corticalEEG.

EEG spindle quantification and power spectral analysis

The presence of 7- to 14-Hz spindles in the cortical EEG represents recurrent activity within a thalamocortical projection(Steriade et al. 1993a). Halothane-induced EEG spindles were detectedin B6 mouse prefrontal cortex by the amplification and recordingof signals from the two electrodes above the right prefrontalcortex using a Grass (West Warwick, RI) Model 15RXi digital polygraphand Polyview software. Spindle frequency was confirmed in the7- to 14-Hz range by fast Fourier transformation (FFT) analysis.The number of EEG spindles/min and cortical ACh release were measuredsimultaneously. Signals from the same electrodes used to recordEEG spindles were amplified and digitized with a sampling rateof 128 Hz. The EEG was filtered electronically with the Model15RXi hardware at 0.3 and 30 Hz. The EEG was analyzed by FFT in2-s bins. Analyses were conducted in 0.5-Hz increments for frequenciesranging from 0.5 to 25 Hz. The bins were averaged over 1-min intervalsof EEG recordings. During microdialysis the total power (Vrms)for each frequency interval of prefrontal cortical EEG was quantifiedas power spectraldensity.

Histological and statistical analyses

Following each experiment, brains were removed and sectioned coronally at 40 µm on a Bright model OTF cryostat (Huntingdon,Cambridgeshire, England). Sections were mounted on gelatin-coatedslides, fixed with paraformaldehyde vapors at 80°C, and stainedwith cresyl violet. Digitized images of the stained sections wereused to localize microdialysis probe placements by comparisonof probe center to a stereotaxic atlas (Paxinos and Franklin 2001).The alpha level for all analyses was P < 0.05. Descriptive statisticsand repeated measures ANOVA with posthoc Tukey-Kramer statisticwere used to analyze the dependent measures of ACh release andnumber of EEG spindles/min during the control and the three drugconditions. Drug effects on EEG frequency were analyzed by repeated-measuresANOVA and posthoc comparisons with Bonferroni correction usingSAS (release 8.8, SAS Institute, Cary, NC). The numerator degreesof freedom (df) equals the number of conditions minus one andthe denominator df equals the product of the numerator df andthe number of frequency bins minusone.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Microdialysis and EEG data were included in the present study only if dialysis sites were histologically localized to be fullywithin prefrontal cortex. Figure 1A schematizes the relative locationsof cortical EEG electrodes and a microdialysis probe in the prefrontalcortex of B6 mouse. Figure 1B illustrates how histological localizationof microdialysis probe-induced lesions confirmed that ACh measureswere obtained from prefrontal cortex. The representative polygraphicrecord in Fig. 1C was taken during microdialysis with Ringer solutionand illustrates halothane-induced EEG spindles. A reduced numberof EEG spindles caused by dialysis delivery of the mAChR antagonistAF-DX 116 during the same experiment is illustrated in Fig. 1D.

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Fig. 1. Dialysis probe placement and EEG recordings. A: schematic illustrates simultaneous recordings and microdialysis of prefrontal cortex (FrA) (modified from Douglas et al. 2002

). B: digitized cresyl violet-stained section demonstrates dialysis site localization at the point of maximum probe-induced lesion (arrow). EEG tracings from prefrontal cortex show halothane-induced 7- to 14-Hz EEG spindling (C) and reduced EEG spindling (D) during microdialysis delivery of AF-DX 116. Coronal schematic (A) reprinted with permission (Paxinos and Franklin 2001

Mean prefrontal cortical ACh release was increased by dialysis delivery of mAChR antagonists. Percentage change in ACh releaseafter antagonist delivery is shown graphically in Fig. 2A. Repeated-measuresANOVA comparing the effects of Ringer (control) and Ringer containingmuscarinic antagonists showed a significant drug main-effect onACh release (F = 100.1; df = 3, 132; P < 0.0001). Posthoc Tukey-Kramerstatistic revealed that AF-DX 116, scopolamine, and AF-DX 116plus pirenzepine significantly increased ACh release over Ringerlevels (P < 0.01). Increases in ACh release caused by the threeantagonist treatment conditions were not significantly differentfrom each other.

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Fig. 2. Effects of muscarinic antagonists on prefrontal cortical ACh release and EEG spindles. A: dialysis delivery of muscarinic antagonists to prefrontal cortex increased local ACh release. ^*AF-DX 116 (3 nM), scopolamine (10 nM), and AF-DX 116 (3 nM) plus pirenzepine (3 nM) increased prefrontal cortex ACh release above control (Ringer) levels by 15.2, 17.6, and 16.3%, respectively. B: number of 7- to 14-Hz EEG spindles/min was decreased only by dialysis delivery of AF-DX 116. Dialysis delivery of AF-DX 116 (3 nM) to prefrontal cortex caused a significant (P < 0.01) decrease ( $-$ 18.3%) in the number of 7- to 14-Hz EEG spindles/min in the contralateral prefrontal cortex. Scopolamine (10 nM) did not alter number of EEG spindles/min. Coadministration of pirenzepine (3 nM) with AF-DX 116 blocked the decrease in the number of EEG spindles induced by AF-DX 116 alone. The combination of AF-DX 116 plus pirenzepine was associated with only a 0.3% decrease in number of spindles/min.

Figure 2B summarizes the number of halothane-induced EEG spindles/min during control and drug delivery conditions for theentire recording period (75 min). A significant drug main-effectwas revealed by repeated-measures ANOVA (F = 282; df = 3, 321;P < 0.0001). Posthoc Tukey-Kramer statistic revealed that onlyAF-DX 116 caused a significant (P < 0.01) decrease in halothane-inducedEEG spindles/min compared with control dialysis. The number ofEEG spindles/min during dialysis delivery of AF-DX 116 also wassignificantly lower than during dialysis delivery of either scopolamine(P < 0.01) or AF-DX 116 plus pirenzepine (P < 0.01).

The plots of power spectral densities in Fig. 3 represent the averaged results of EEG recordings during 15 experiments. Scopolaminedid not cause a decrease in EEG power at any frequency (Fig. 3A).Analysis of variance revealed that there was a significant drugmain-effect on EEG power caused by AF-DX 116 (F = 9.78; df = 49,245; P = 0.004, Fig. 3B, gray line). Post hoc multiple comparisonstests with Bonferroni correction showed that AF-DX 116 causeda significant (P < 0.05) decrease in slow-wave EEG power at the0.5, 1.0, 1.5, 2.0, 2.5, 3.5, and 4.5 Hz frequencies. Interestingly,this decrease in EEG power included the frequencies describedas slow oscillations in feline cortex (Steriade et al. 1993b).The decrease in slow-wave EEG power caused by AF-DX 116 was blockedby the addition of pirenzepine to the microdialysis solution (Fig.3B, dashed line).

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Fig. 3. Power spectral analysis quantified activation of prefrontal cortex. A: EEG power spectral density indicates that the contralateral EEG was unchanged by microdialysis delivery of scopolamine. B: microdialysis delivery of AF-DX 116 caused a significant (P < 0.05) decrease in slow-wave EEG power (gray line) compared with Ringer control (solid black line). The simultaneous microdialysis delivery of pirenzepine and AF-DX 116 did not alter EEG slow waves (dashed black line).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The diverse regulatory roles subserved by the prefrontal cortex (Groenewegen and Uylings 2000) justify efforts to understandcontrol of prefrontal cortical excitability. The prefrontal cortexis involved in memory formation (Gabrieli et al. 1998), forwardplanning (Gaffan and Harrison 1989; Tanji and Hoshi 2001), andrelation of arbitrary associations (Toni and Passingham 1999).Cardiopulmonary control and the emotional content of perceptionare modulated by prefrontal cortical projections (reviewed inGroenewegen and Uylings 2000). The prefrontal cortex is particularlyvulnerable to the effects of anesthesia, and memory-blocking drugscommonly used during surgery disrupt prefrontal cortical function(Andrade 1996; Casele-Rondi 1996). Dysfunctions of the prefrontalcortex also are implicated in neurodegenerative diseases suchas Alzheimer's and Parkinson's, psychiatric disorders such asschizophrenia, and postoperative delirium in the elderly population(reviewed in Groenewegen and Uylings 2000).

The homology of the rodent prefrontal cortex to human prefrontal cortex has been questioned (Preuss 1995). Alternatively,brain regions in rodents that have not evolutionarily differentiatedinto highly complex structures may indeed be homologous to brainregions in primates (Uylings and van Eden 1990). When the prefrontalcortex is defined by the major projection field of the mediodorsalthalamus and by interconnectivity with other brain regions (Groenewegenand Uylings 2000; Öngür and Price 2000), these anatomical criteriasuggest that the mouse prefrontal cortex is homologous to primateprefrontal cortex. All of the present results were from the prefrontalcortex of B6 mouse (Fig. 1, A and B) as verified by histologicalexamination. The results provide the first evidence that endogenousACh in one prefrontal cortex activates the EEG in the contralateralprefrontal cortex via postsynaptic M1receptors.

Pre- and postsynaptic muscarinic mechanisms modulate ACh release and excitability in prefrontal cortex

Numerous studies substantiate the present in vivo pharmacological approach for identifying mAChR subtypes (Baghdoyan et al.1998; Baghdoyan and Lydic 1999; Billard et al. 1995; Douglas etal. 2001, 2002). Recent studies of B6 mouse found that scopolamineand AF-DX 116 are equipotent for increasing ACh release and thatpirenzepine is 100-fold less potent than scopolamine or AF-DX116 (Douglas et al. 2001). Those data supported the interpretationthat M2 mAChRs function as presynaptic autoreceptors in prefrontalcortex of B6 mouse (Douglas et al. 2001). A subsequent study (Douglaset al. 2002) found that one functional consequence of enhancingACh release in ipsilateral prefrontal cortex is activation ofthe contralateral prefrontal cortical EEG. No data were availableto identify the postsynaptic receptors through which endogenousACh could activate EEG in contralateral prefrontal cortex. Thereforethe present study evaluated the hypothesis that the postsynapticM1 receptor is one site at which ACh activates prefrontal corticalEEG.

Characterizing brain neurochemistry relative to various mouse strains and other species is an important goal for mouse phenotyping.Previous work on feline EEG analysis has shown a fast componentin the gamma (30-40 Hz) range (Steriade and Amzica 1996). Thereforeadditional FFT analyses were performed in the present study acrossthe EEG frequency spectrum $<=$ 60 Hz. These analyses did not revealany prominent power in the 30- to 40-Hz range. This lack of gammaactivity may be one reason most studies of mouse EEG have focusedon frequencies ranging from 0 to 25 Hz (Franken et al. 1998; Huberet al. 2000; Tobler et al. 1997; Veasey et al. 2000; Zhang etal. 1996).

When delivered to prefrontal cortex by microdialysis, 3 nM AF-DX 116 increased ipsilateral cortical ACh release (Fig. 2A)and activated the EEG in the contralateral prefrontal cortex (Figs.2B and 3B). Cortical activation was quantified by a reductionin the number of EEG spindles (Fig. 2B) and by a decrease in EEGslow waves as determined by FFT analysis (Fig. 3B, solid grayline). AF-DX 116 has higher affinity for M2 and M4 subtypes thanfor M1, M3, or M5 subtypes (Billard et al. 1995; Caulfield andBirdsall 1998; Jones et al. 1992). Taken together, these findingsindicate that contralateral EEG activation (Figs. 2B and 3B) wasmediated by a non-M2/M4 mAChRsubtype.

The present results suggest that nicotinic cholinergic receptors did not cause EEG activation. Scopolamine is a cholinergicantagonist that blocks all five mAChR subtypes (Jones et al. 1992).Microdialysis delivery of scopolamine increased ipsilateral AChrelease (Fig. 2A) but did not activate the contralateral EEG (Figs.2B and 3A). The increased ACh release caused by scopolamine wouldbe expected to activate nicotinic cholinergic receptors. Therewas no contralateral prefrontal cortical activation associatedwith scopolamine-evoked ACh release. The present data thereforeare consistent with the interpretation that the contralateralcortical activation associated with increased ACh release wasmediated by muscarinic, and not nicotinic, AChreceptors.

Dialysis delivery of pirenzepine was used to test the hypothesis that M1 mAChRs mediate ACh-induced activation of contralateralcortex. Previous studies have shown that 3 nM pirenzepine doesnot alter ACh release when delivered by microdialysis to prefrontalcortex (Douglas et al. 2001). At a concentration of 3 nM, pirenzepineshould block M1 and M4 receptors (Jones et al. 1992). In the currentstudy, 3 nM pirenzepine was added to Ringer containing 3 nM AF-DX116 for dialysis delivery to prefrontal cortex. The combinationof antagonists increased ACh release at the dialysis site (Fig.2A) but no more effectively than did 3 nM AF-DX 116 alone (Fig.2A). A key finding was that pirenzepine blocked the AF-DX 116-inducedactivation of the contralateral prefrontal cortical EEG (Figs.2B and 3B). Microdialysis delivery of AF-DX 116 plus pirenzepinefailed to decrease the number of EEG spindles/min (Fig. 2B) andlikewise failed to decrease EEG slow waves (Fig. 3B, dashed line).The only change resulting from the addition of pirenzepine tothe AF-DX 116 was antagonism of M1 receptors. Therefore the AF-DX116 plus pirenzepine data are consistent with the interpretationthat postsynaptic M1 mAChRs contribute to cholinergically enhancedEEG activation in contralateral prefrontalcortex.

Limitations and conclusions

The mouse is an important model for mechanistic studies relevant to human disease (Behringer 2001; Hock and Lamb 2001; Skradskiet al. 2001), and it has been noted that "every human gene hasa mouse homologue" (O'Brien et al. 1999). The present resultsare limited to B6 mouse and additional data will be needed todetermine the extent to which these results are generalizableto other mammalian brains. The present studies do not addressthe issue of connectivity between the two hemispheres of prefrontalcortex. Although most likely, it is not known for certain thatthe putative M1 receptor mediating cortical EEG activation resideson processes innervating the contralateral cortex through thecorpus callosum. The present data also do not address the questionof which transmitter or receptor in the contralateral cortex mediatedcortical activation. Close inspection of Fig. 3 reveals that EEGspindles do not appear as a prominent feature of the EEG powerspectra. Available data suggest that the lack of a 7- to 14-Hzpeak reflects limitations of FFT analysis (Douglas et al. 2002).FFT analysis assumes that the signal being analyzed does not changefrequency content during the epoch being analyzed. This assumptionis violated by biological signals such as EEG. Furthermore, EEGspindles comprised <8.5% of the total EEG, therefore contributingrelatively little to total EEG power. This interpretation is supportedby FFT analyses that were focused on EEG frequencies in the 7-to 14-Hz range (data not shown). FFT analyses of the 7- to 14-Hzfrequency range did not unmask peaks in EEG amplitude. Thereforenumber of EEG spindles/min (Fig. 2B) provided an additional quantitativeindex of EEGactivation.

In conclusion, the present study is the first to provide evidence that one functional consequence of increased cortical AChrelease, activation of contralateral cortical EEG, is mediatedpartly by postsynaptic M1 receptors (Fig. 4). Thus enhancing therelease of ACh by blocking M2 autoreceptors and/or by activatingpostsynaptic M1 receptors may help to alleviate deficits in cholinergicneurotransmission characteristic of dementing diseases (Careyet al. 2001; Kitaichi et al. 1999). The present results also arerelevant for efforts to understand the similarities and differencesin the neuronal mechanisms regulating sleep and anesthesia. Duringsleep, EEG spindles block sensory input to cortex (Steriade 2000).During halothane anesthesia, EEG spindle generation is enhancedin B6 mouse (Figs. 1C and 2B), cat (Keifer et al. 1996), and human(Yli-Hankala et al. 1989). During sleep and halothane anesthesia,EEG spindles are suppressed by increasing cholinergic neurotransmissionat the level of the brain stem (Keifer et al. 1996; Steriade 2000)and, as shown here, by activating M1 mAChRs in the cortex.

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Fig. 4. One proposed mechanism modulating prefrontal cortical EEG and ACh release. The main source of ACh in mouse cortex arises from cortically projecting neurons of the substantia innominata (SI) and basal nucleus of Meynert (B) (Kitt et al. 1994

). Data from several studies (Douglas et al. 2001

, 2002

; Zhang et al. 2002

) support the conclusion that release of ACh in the cortex is modulated by M2 autoreceptors (inset) residing on terminals originating from substantia innominata and basal nucleus of Meynert. Recent data demonstrated that, in B6 mouse, increased ACh in one prefrontal cortex (PFC) causes EEG activation in the contralateral PFC (Douglas et al. 2002

). The present results suggest for the first time that one functional consequence of increasing ipsilateral PFC ACh release is activation of contralateral PFC EEG via postsynaptic M1 receptors (inset).

	ACKNOWLEDGMENTS

We thank M. A. Norat for expert technical assistance and statistician K. Welch at the University of Michigan Center for StatisticalConsultation andResearch.

Support was provided by National Institute of Health Grants HL-65272, HL-57120, HL-40881, and MH-45361, and the Departmentof Anesthesiology. AF-DX 116 was a gift from Boehringer-Ingelheim.

	FOOTNOTES

Address for reprint requests: R. Lydic, Department of Anesthesiology, University of Michigan, 7433 Med Sci I, 1150 W. MedicalCenter Drive, Ann Arbor, Michigan 48109 (E-mail: rlydic{at}umich.edu).

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TOP
ABSTRACT
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METHODS
RESULTS
DISCUSSION
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