Brain Mechanisms of Propofol-Induced Loss of Consciousness in Humans: a Positron Emission Tomographic Study

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The Journal of Neuroscience, July 1, 1999, 19(13):5506-5513

Brain Mechanisms of Propofol-Induced Loss of Consciousness in Humans: a Positron Emission Tomographic Study
Pierre Fiset¹^,³, Tomás Paus², Thierry Daloze¹, Gilles Plourde¹, Pascal Meuret¹, Vincent Bonhomme¹, Nadine Hajj-Ali⁴, Steven B. Backman¹^,³, and Alan C. Evans²
Departments of ¹ Anesthesiology and ² Neurology and Neurosurgery and ³ McGill University Health Center, McGill University, Montreal, Quebec, Canada, H3A 1A1, and ⁴ Faculté de Pharmacie, Université de Montréal, Montreal, Quebec, Canada H3C 3J7

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the present study, we used positron emission tomography to investigate changes in regional cerebral blood flow (rCBF) duringa general anesthetic infusion set to produce a gradual transitionfrom the awake state to unconsciousness. Five right-handed humanvolunteers participated in the study. They were given propofolwith a computer-controlled infusion pump to achieve three stablelevels of plasma concentrations corresponding to mild sedation,deep sedation, and unconsciousness, the latter defined as unresponsivenessto verbal commands. During awake baseline and each of the threelevels of sedation, two scans were acquired after injection ofan H₂¹⁵O bolus. Global as well as regional CBF were determined and correlatedwith propofol concentrations. In addition, blood flow changesin the thalamus were correlated with those of the entire scannedvolume to determine areas of coordinatedchanges.
In addition to a generalized decrease in global CBF, large regional decreases in CBF occurred bilaterally in the medial thalamus,the cuneus and precuneus, and the posterior cingulate, orbitofrontal,and right angular gyri. Furthermore, a significant covariationbetween the thalamic and midbrain blood flow changes was observed,suggesting a close functional relationship between the twostructures.
We suggest that, at the concentrations attained, propofol preferentially decreases rCBF in brain regions previously implicatedin the regulation of arousal, performance of associative functions,and autonomic control. Our data support the hypothesis that anestheticsinduce behavioral changes via a preferential, concentration-dependenteffect on specific neuronal networks rather than through a nonspecific,generalized effect on thebrain.

Key words: anesthesia; PET; arousal; consciousness; thalamus; reticular formation; cerebral blood flow; propofol

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The search for a neural substrate of consciousness has been the subject of increased scientific effort in recent years. Althoughit is difficult to provide an all-encompassing definition of theterm "consciousness," it is useful to make a distinction betweenthe level and content of consciousness: the former is generallyassociated with arousal, whereas the latter concerns the contentof subjective experience (Frith et al., 1999). In the presentpaper, the term consciousness is used in reference to the levelofarousal.

Since the pioneering work of Jasper (1949) and Moruzzi and Magoun (1949), the thalamus and the brainstem reticular formationhave been known to play a critical role in the regulation of levelsof consciousness. More recent work in nonhuman species providedevidence that neuronal oscillations in the reticular thalamicnucleus are intimately linked to the variations in sleep-wakingcycle (Steriade and Deschenes, 1984; Steriade and Llinas, 1988;Steriade et al., 1993). In particular, GABAergic cells of thereticular thalamic nucleus seem to control bursting activity ofthe thalamocortical neurons and, in turn, modulate cortical activity(Steriade et al., 1993; Destexhe et al., 1994). In humans, muchless is known about the relationship between the intrathalamicnuclei activity and consciousness. Reports on the recording ofunit activity in the human thalamus are sparse, and lesion studies(Lugaresi et al., 1986; Kinney et al., 1994) provide only a limitedstatic picture of the system. On the other hand, several brainimaging studies have shown regional cerebral blood flow (rCBF)variations in the human thalamus in relation to various statesof consciousness, including sleep (Maquet et al., 1996, 1997;Hofle et al., 1997) vigilance (Paus et al., 1997), and attention(Kinomura et al., 1996).

Pharmacological studies on anesthetic effects suggest that a variety of neurochemical routes lead to the same end point, namelythe change of the level of consciousness. Thus, the currentlyused general anesthetics may act through ligand-gated ion channelsof the GABA_A (Hales and Lambert, 1991; Yeh et al., 1991; Orseret al., 1994), NMDA (Lodge et al., 1982) (Anis et al., 1983),and muscarinic (Lydic et al., 1993; Keifer et al., 1994) receptors.It is not known, however, whether these cellular events exerttheir action by affecting specific structures of thebrain.

In the present study, we manipulated the level of consciousness using propofol, an anesthetic drug widely used in clinicalpractice to induce and maintain general anesthesia. Propofol waschosen because its concentration-effect relationships are wellestablished and predictable (Dunnet et al., 1994; Forrest et al.,1994; Casati et al., 1999). We infused propofol with a computer-controlledinfusion pump (CCIP) to maintain steady-state plasma concentrationsand, in turn, a stable effect corresponding successively to lightsedation, deep sedation, and unconsciousness. At the same time,we used positron emission tomography (PET) to measure absoluteand relative values of rCBF and electroencephalography (EEG) toassess concurrent changes in the electrocortical arousal. We foundthat the thalamic blood flow decreased as a function of the propofollevel above and beyond a decrease in globalCBF.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects. The study was approved by the Research and Ethics Committee of the Montreal Neurological Institute and Hospital.Five healthy right-handed subjects (two females) participatedin the study after giving written informed consent (age, 25.4± 3.36 years). All underwent a comprehensive medical evaluationand had no history of neurological disorders or intolerance toanesthesia.

Experimental design. We did not objectively assess the component of consciousness related to the appreciation or awarenessof afferent inputs. Our definition of consciousness, i.e., responseto verbal commands, is simple yet operationally useful in thesense that it globally evaluates all the aspects of the consciousresponse to a standardstimulus.

Three different levels of sedation (mild sedation, deep sedation, and unconsciousness) were induced and maintained with propofoladministered using a computer-controlled infusion pump (CCIP).Volunteers were also studied during an awake baseline state. Thefollowing order of conditions was used: awake baseline (baseline),mild sedation (level 1), deep sedation (level 2), and unconsciousnessdefined as an absence of response to verbal commands (level 3).Thus, the subjects always received an increasing concentrationof propofol to avoid delays encountered by the elimination ofthe drug from the brain if a decreasing concentration order hadbeenused.

At each condition, two 3 min PET scans were acquired with a Scanditronix (Uppsala, Sweden) PC-2048B tomograph, and arterialblood samples were drawn to calculate the absolute values of rCBF.Blood was also drawn for determination of arterial blood gasesand propofol plasma concentrations. During the scans, the subjectswere blindfolded and EEG, electrocardiogram, systemic arterialblood pressure, and pulse oximetry were recorded. During all scansoxygen was provided through a loosely fitting face mask at a rateof 3 l/min. Between each scan the state of consciousness was assessedby asking the volunteer to move his or her toes and squeeze theinvestigator's hand. Throughout the study, the subjects were closelymonitored by an anesthesiologist (P.F., T.D., or G.P.). Resuscitationmaterial was readily available in the scannerroom.

To facilitate localization of the regional changes in CBF, we obtained high-resolution T1-weighted magnetic resonance images(MRIs; 160 contiguous sagittal slices, 1 mm thick) from a Philips(Besl, The Netherlands) Gyroscan ACS imager (1.5 T) for eachsubject.

Propofol Infusion. Propofol was infused with a CCIP; the infusion program STANPUMP (developed by Steven L. Shafer, Departmentof Anesthesiology, Stanford University, Stanford, CA) was usedto control a Harvard Apparatus (Holliston, MA) 22 pump. A targetconcentration of propofol was rapidly reached by the administrationof a bolus dose and was maintained by an infusion with an exponentiallydeclining rate. The dosage and rate of propofol infusion werebased on pharmacokinetic parameters obtained by Tackley et al.(1989) in a population with demographic characteristics similarto those of ourvolunteers.

In addition to the awake baseline condition (baseline, 0.0 µg/ml of propofol in plasma), the following three levels of propofolwere targeted: level 1, 0.5 µg/ml plasma when the volunteer isawake and mildly sedated and readily follows commands; level 2,1.5 µg/ml plasma when the volunteer is deeply sedated, his orher speech is sluggish, and reactions to verbal orders are slow;and level 3, 2.5-3.0 µg/ml plasma when the volunteer is unconsciousand does not respond to verbal orders but breathesspontaneously.

The plasma concentration of propofol was assessed with HPLC (Plummer, 1987) using arterial blood samples obtained at least5 min after the target effect site concentration was reached and4 min before the commencement of eachscan.

EEG. Brain electrical activity was recorded using Ag/AgCl electrodes placed over the left hemisphere (F₄, P₄, and O₂) andat the vertex (C_z) and referenced to the right earlobe (A₂) (ElectrodeNomenclature Committee, 1994). A horizontal electro-oculogramwas obtained from two electrodes placed at the outer canthi ofeach eye, and an electromyogram (EMG) was recorded from an electrodeplaced on the chin. The electrodes were filled with conductivegel and glued to the scalp with collodion and a piece of gauze.The electrode impedance was considered acceptable if <10 k $Omega$ .

Brain electrical activity was amplified (bandpass, 0.3-100 Hz) and sampled at 256 Hz with Monitor software (Stellate Systems,Montreal, Quebec, Canada) and stored on disk for subsequent analysis.For each 3 min epoch corresponding to a CBF scan, the EEG activitypresent at various frequency bands was determined using fast Fouriertransform (Rhythm software, Stellate Systems). The following frequencybands were used: $delta$ , 1.5-4.0 Hz; $theta$ , 4.5-8.0 Hz; $alpha$ , 8.5-11.5 Hz; $sigma$ , 12.0-15.0 Hz; $beta$ , 18.0-30.0 Hz; and $gamma$ , 30.5-57.0 Hz. For thepresent analysis, only data from F₄-A₂ wereused.

EEG epochs containing obvious muscle activity or eye blinks were rejected. Data from F₄-A₂ were subjected to an ANOVA forrepeated measures to evaluate the effect of propofol level (baselineand levels 1-3) on the total and relative power at each frequencylevel ( $alpha$ , $delta$ , $theta$ , $sigma$ , $beta$ , and $gamma$ ). The Greenhouse-Geisser procedurewas used to adjust the degrees of freedom. Tukey's honestly significantdifference test was used for post hoc tests (Kirk, 1982).

Measurement and analysis of rCBF. Values of rCBF were measured with a Scanditronix PC-2048B eight-ring 15-slice tomograph.The axial view of this scanner is 9 cm, and in this study, thesubjects were placed in the scanner so that the brain was scannedfrom approximately z = 48 to z = $-$ 44 mm. The distribution of rCBFwas measured during each 3 min scan using the ¹⁵O-labeled H₂O bolus method (Raichle et al., 1983). For each scan,30 mCi of ¹⁵O-labeled H₂O was injected into the left antecubital vein. Arterialblood samples were taken from a catheter placed in the right radialartery. The sinograms were reconstructed using an 18 mm Hanningfilter.

Absolute rCBF. Arterial blood samples were collected manually at 5 sec intervals and assayed in a well counter calibratedwith respect to the tomograph. CBF was calculated using the two-compartment,weighted integration method of Ohta et al. (1996). Cerebral perfusionmaps (K1 maps) were generated for each scan using the sum of thenative PET image across all frames. Mean whole-brain CBF valueswere then obtained by averaging the K1map.

The averaging of masked K1 maps allowed calculation of mean CBF values in the gray and white matter. The masks were standardprobabilistic maps of gray or white matter co-registered witheach K1 map by means of an automatic registration program (Woodset al., 1993). A probability of 0.6 was chosen as the cutoff pointfor a voxel to be of gray or of white matter,respectively.

The mean CBF of the regions of interest was calculated. The coordinates of significant peaks observed after statistical analysisof the relative CBF images were back-transformed into the coordinatesof each individual K1 map and served as the center of a 7 mm radiusvolume of interest. The average CBF value in that region was thenextracted.

Normalized rCBF. To identify the brain regions where propofol induced changes in blood flow beyond those observed globally,we analyzed the effects of propofol on normalized rCBF. This analysiswas limited to the initial 60 sec period of the 3 min scan. First,between-scan and between-subject differences in global CBF wereremoved by proportional normalization: in each scan, count valuesin all voxels were multiplied by a constant, based on the meancount value of all gray matter voxels for the given scan, so thatthe resulting global mean had a value of 50 in all scans and subjects.The gray matter voxels were defined by a probabilistic gray mattermask (gray matter p > 0.5). The use of the gray matter mask ensuresthat the global changes in CBF in the area of greatest neuronalactivity are removed. Second, PET images were co-registered withthe individual MRIs (Woods et al., 1993) and transformed intostereotaxic space (Talairach and Tournoux, 1988) by means of anautomated feature-matching algorithm (Collins et al., 1994).

To assess the significance of the linear relationship between the plasma level of propofol and normalized rCBF, a propofolregression map was calculated. The following calculations wereperformed for each of the three-dimensional volume elements (voxels)constituting a volume. The data set consisted of normalized rCBFobtained in five subjects, each scanned twice during each of thethree propofol conditions, yielding a total of 30 CBF volumes.Because of excessive movements during scanning, however, fourscans obtained at levels 2 and 3 in one of the subjects had tobe excluded, leaving us with a total of 26 volumes. The effectof propofol on CBF was assessed by means of an analysis of covariance(ANCOVA) (Sokal and Rohlf, 1981), with subjects as a main effectand the plasma level of propofol as a co-variate. The subjecteffect was removed, and the parameter of interest was the slopeof the propofol effect on normalized rCBF. An estimate of theslope, $beta$ _PROP, and its SD, s, were obtained by least-squares fittingof the model (ANCOVA) at each voxel. A total of 26 values of theco-variate were used, corresponding to the 26 volumes in the dataset. The degrees of freedom (df) of the estimate of the SD (s)were increased from 20 (26 $-$ 5 $-$ 1) by pooling s across all voxels,and this replaced a voxel s in the denominator of the t statistic,t = $beta$ _PROP/pooled s, so that its distribution was normal. The resultingt statistic map tested whether, at a given voxel, the slope ofthe regression was significantly different from zero; the presenceof a significant peak was tested by a method based on three-dimensionalGaussian random-field theory, which corrects for the multiplecomparisons involved in searching across a volume (Worsley etal., 1992). Values equal to or exceeding a criterion of t = 3.5were considered significant (p < 0.0004, two-tailed, uncorrected),yielding a false-positive rate of 0.5 in 200 resolution elements(each of which has dimensions 7.7 × 18 × 18 mm), which is approximatelythe volume of brain graymatter.

In addition to the above propofol regression map, a regional regression map was generated to assess the significance of therelationship between CBF values in the thalamus and those obtainedat each voxel of the entire scanned volume. This was done to revealbrain regions that showed a coordinated blood flow response inthe thalamus and in other regions to the changing plasma levelsof propofol. CBF values in the thalamus were first derived bypositioning a spherical volume of interest (radius, 8 mm) at thecenter of the peak defined by the propofol regression. Subsequently,the same statistical procedures were used when calculating thepropofol regression map: subject effect was removed, and the parameterof interest was the slope $beta$ _THAL of the effect of CBF in the thalamuson CBF. Assessment of significance for this parameter (i.e., generationof a t map) was performed in the same manner as for the propofolregression.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Propofol concentration

HPLC analysis of plasma demonstrated that the concentrations achieved were very similar to those targeted. The measured concentrationswere as follows (mean ± SD): level 1, 0.445 ± 0.070 µg/ml (target,0.5 µg/ml); level 2, 1.35 ± 0.11 µg/ml (target, 1.5 µg/ml); andlevel 3, 2.67 ± 0.5 µg/ml (target, 2.5-3.0 µg/ml). The mean andmedian absolute errors of propofol plasma concentrations in allsubjects were 12 and 8%, respectively, of the values predictedby theCCIP.

State of consciousness

All volunteers were conscious but mildly sedated at level 1, such that they responded to verbal commands and reported beingslightly drowsy. At level 2, four subjects were deeply sedated,as indicated by their slurred speech and slow responses to verbalcommands, whereas one volunteer was unconscious. At level 3, allfive volunteers wereunconscious.

Cardiovascular parameters

Heart rate and P_CO₂ did not change at levels 1-3 compared with baseline. There was a significant drop in systolic and diastolicblood pressure at level 3 compared with the baseline and withlevel 1, as illustrated in Table 1. A small nonsignificant increasein P_CO₂ was observed at levels 2 and 3 compared with baseline.


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Table 1. Vital signs: mean ± SD for all subjects during baseline and levels of sedation

Electroencephalogram

Table 2 shows the effect of propofol on EEG. There was a significant increase in total power during level 3 compared withbaseline and level 1. There was a significant increase in $sigma$ relativepower during levels 2 and 3 compared with baseline. There wasfinally a significant decrease in $gamma$ power during level 3 comparedwith baseline. This effect remained significant when the $gamma$ relativepower from the chin EMG was used as a time-varying covariate.


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Table 2. EEG values (µv²/sec) for total power and percent of total (relative) power for frequency bands

Absolute CBF

Figure 1 shows a 20.2% decrease in global CBF, from 40.1 to 32.1 ml · 100 gm¹ · min¹, between baseline and level 3. The ANOVA showed a significantmain effect of level (F = 4.63; p = 0.0226), and a post hoc pairedt test comparing each of the levels showed a statistically significantdifference between baseline and level 3 (p < 0.05) and a borderlinedifference between levels 1 and 3.

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Figure 1. Absolute cerebral blood flow changes as a function of the baseline and the three levels of propofol expressed as the mean concentration of propofol ± SD. *Statistically significant difference (p < 0.05).

The white and gray matter compartments were defined with the aid of the respective probabilistic maps. The two-way repeatedmeasures ANOVA revealed a significant main effect of tissue type(F = 4.52; p = 0.0477) but no significant interaction betweenlevel and tissuetype.

Normalized rCBF

The results of the regression of propofol levels versus rCBF are summarized in Table 3. As the plasma concentration of propofolincreased, normalized rCBF decreased in the thalamus (Figs. 2,3A) and in the parieto-occipital cortices, cuneus, precuneus,and posterior cingulate (Fig. 3A).


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Table 3. Stereotaxic coordinates

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Figure 2. Normalized thalamic blood flow as a function of propofol levels. There is significant negative correlation with a peak in the medial thalamus (t = 5.62).

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Figure 3. A, The merged rCBF-MRI images indicate the location of the negative correlation of the regression between normalized rCBF and propofol concentration. The range of negative t values for the PET data is coded by the color scale. B, Positive covariation between the thalamic rCBF and other brain structures. The range of positive values for the PET data is coded by the color scale.

On the other hand, significant positive correlations between propofol and rCBF were observed in the cerebellum, the medialfrontal cortex, and the left temporalpole.

The thalamus-based regional regression revealed a positive correlation between the thalamic CBF and the midbrain, upper midbrain,and left orbitofrontal cortex (Table 3, Fig. 3B).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Propofol induced a decrease in absolute CBF throughout the white and gray matter. Using the normalized rCBF data, we foundthat this effect is particularly pronounced in the medial thalamus,the cuneus and precuneus, the posterior cingulate and orbitofrontalgyri, and the right angular gyrus. The propofol-related variationsin the thalamic blood flow were statistically linked with thosein the midbrain reticular formation, thus suggesting a close functionalrelationship between the two brainstructures.

Propofol and global cerebral blood flow

Our finding that propofol produces a decrease in the global CBF is consistent with the results of several animal studies thatused a variety of techniques, including cerebral venous outflowmeasurement (Langerkranser et al., 1997), labeled tracer injection(Werner et al., 1993; Todd and Weeks, 1996), and ¹³³Xe (Van Hemelrijck et al., 1990). A global decrease in CBF, measuredby middle cerebral artery Doppler (Eng et al., 1992) and ¹³³Xe (Pinaud et al., 1990; Newman et al., 1995), has also been reportedin humansubjects.

In the present study, we report a decrease in the mean systemic arterial blood pressure with increasing concentrations ofpropofol. When autoregulation of the cerebral vasculature is intact,changes in systemic arterial blood pressure ranging between 50and 150 mmHg do not result in variations of CBF. It has been shownin animals (Van Hemelrijck et al., 1990; Werner et al., 1993;Langerkranser et al., 1997) and in humans (Salord et al., 1995)that autoregulation is preserved when propofol is administeredin concentrations similar to those used in our study. Therefore,we suggest that the changes in CBF reported here do not resultfrom the variation in blood pressure but instead are a reflectionof the decreased cerebral metabolic requirements induced byanesthesia.

Propofol effects on the reticulothalamic system

The strong negative correlation between rCBF in the medial thalamus and propofol concentration suggests that propofol actson the reticulothalamic system when loss of consciousness is induced.We have since replicated this finding in another group of subjects(Fiset et al., 1997). The observed covariation between the thalamicand midbrain blood flow is consistent with the role of the thalamusand the ascending reticular activating system (ARAS) in the regulationof wakefulness (Steriade et al., 1990; Paus et al., 1997). Electrophysiologicalstudies in animals have shown that a progression from awake slow-wavesleep is associated with a decreased firing of neurons in thebrainstem reticular activating system and a disfacilitation ofthalamocortical relay neurons (Steriade et al., 1990; Jones, 1994).Furthermore, thalamocortical interactions expressed, for example,as 40 Hz oscillations are decreased in natural sleep (Llinásand Paré, 1991) and during general anesthesia (Plourde and Picton,1990; Plourde and Boylan, 1991; Plourde et al., 1998). Our resultssuggest that the reticulothalamic system plays a central rolein the modulation of consciousness by general anesthetics. Itis important to note that similar variations in the thalamic CBFwere also observed during natural transitions between waking andslow-wave sleep (Hofle et al., 1997; Maquet et al., 1997), betweenhigh and low vigilance levels (Paus et al., 1997), and betweenhigh and low alertness (Kinomura et al., 1996).

It is believed that neural effects of propofol are mediated at least in part by the activation of the GABA_A-ionophore receptorcomplex (Concas et al., 1991; Pedutto et al., 1991; Tanelian etal., 1993). The interaction between the GABAergic cells of thereticularis and the perigeniculate nuclei and the excitatory thalamocorticalrelay neurons is responsible for the generation of spindle waveactivity recorded during slow-wave sleep (von Krosigk et al.,1993). This suggests that the thalamic deactivation we reportin association with propofol-induced modulation of consciousnessmay result from a direct effect on the GABA_A receptor complexof that circuit. This explanation is consistent with the decreasesin CBF resulting from the pharmacological stimulation of GABA_Areceptors, suggesting that inhibitory postsynaptic neurotransmissionmay be associated with decreases in rCBF (Gjedde, 1997; Rolandand Friberg, 1988).

Propofol effects on cortical activity

In the present study, we found an overall decrease of absolute CBF in the gray matter, which may reflect an overall decreasein cortical neuronal activity. Direct inhibitory effects of propofolon cortical layers II, IV, V, and VI have been reported (Angel,1993) and could underlie the cortical deactivation. Alternatively,a decreased cortical activity may be secondary to decreased activityin the ARAS and thalamocorticalsystems.

In addition to the overall decrease in cortical CBF produced by propofol, we observed particularly pronounced effects in severalcortical regions. The medial parieto-occipital cortex was oneof the regions particularly affected. It includes the cuneus,precuneus, posterior cingulate cortex, and right angular gyrus.These areas are implicated in visual associative activities, integrationof sensory information, processing of spatial information, andevaluation sensory inputs in the service of spatial orientationandmemory.

Changes in activation of the medial occipital area have been reported in other PET studies concerned with the mechanisms modulatingthe level of consciousness. Hofle et al. (1997) in a sleep study,Paus et al. (1997) in a vigilance study, and Rainville et al.(1997) in a hypnosis study reported increases an activation inprecuneus and cuneus area concurrent with a decrease in arousaland medial thalamic activity. In contrast, in the present study,thalamic deactivation is paralleled by medial occipital deactivation.We suggest that this is the reflection of a difference in themechanism in play, namely the effect of naturally occurring changesin the level of arousal versus direct pharmacological effectsofpropofol.

GABA_A receptors are distributed widely throughout the CNS, but Hendry et al. (1987) have reported that the primary visualcortex contains 50% more GABA-immunoreactive neurons than othercortical areas. This is a reflection of the overall higher densityof neurons in the primary visual cortex and, therefore, a higherabsolute number of GABA neurons compared with other cortical regions.It is possible that some cortical areas are more sensitive tothe GABAergic inhibition caused by propofol on the basis of theirnetwork of corticocortical connections. Localized patterns ofdeactivation, like the one we report in the medial occipitotemporalarea, might be enhanced on the basis of their connectivity network.Supportive evidence to this argument is given in a recent studyby Chabli et al. (1998), who have shown that the inactivationof area 17 cells produces a decline of the evoked discharges inarea 18 cells with the same orientationtuning.

We also report a significant decrease in rCBF in the orbitofrontal cortex bilaterally. This area of the frontal lobe is implicatedin the modulation of emotional behavior and in the control ofautonomic responses linked to generalized arousal reactions (Neafsey,1990; Oppenheimer et al., 1992). It is part of a network thatsends descending connections to the solitary nucleus of the brainstem(Neafsey et al., 1986). We speculate that the changes in rCBFin the orbitofrontal region during anesthesia might be relatedto a modification of autonomic outflow that contributes to a decreasein arterial blood pressure. However, further studies are requiredto provide evidence for thathypothesis.

Finally, we report an increase in rCBF in the cerebellum. This finding might be related to the initial increase in muscletone and jerking movements frequently seen at early stages ofpropofol-induced generalanesthesia.

Electroencephalographic activity recorded when consciousness was lost was characterized by high-amplitude, low-frequency $delta$ waves and a decrease in $gamma$ activity, an EEG pattern very similarto stage IV sleep. These findings are in accordance with the viewthat $gamma$ activity is a property of the thalamocortical system associatedwith consciousprocessing.

Conclusion

The findings from the present study show that propofol induces concentration-dependent effects in the medial thalamus, cuneus,precuneus, and posterior cingulate and orbito-frontal cortices.This suggests that, at the concentrations attained (between 0.5and 3.5 µg/ml plasma), propofol preferentially decreases rCBFin areas linked to the control of consciousness, associative functions(especially those related to visual inputs), and autonomic control.These changes have not been reported in previous studies concernedwith the metabolic effects of propofol (Dam et al., 1990; Cavazzutiet al., 1991; Alkire et al., 1995).

The thalamic deactivation and its covariation with the midbrain reticular formation are consistent with the role of thesestructures in the control of consciousness. Moreover, they suggestthat the rCBF changes reported in this study are linked to thespecific effects of propofol on neuronal activity and are notthe result of a nonspecific regional effect on CNS vasculature.In this context, the deactivation pattern in specific corticalregions suggests that some neuronal circuits are more sensitiveto the effects of propofol and offers new avenues ofinvestigation.

  FOOTNOTES

Received Feb. 2, 1999; revised April 16, 1999; accepted April 19, 1999.

This study was supported by the Canadian Medical Research Council, le Fonds de la Recherche en Santé du Québec (G.P.), leCentre Hospitalier Universitaire de Liège, Belgium (V.B.) andthe Associated Anesthetists of the Royal Victoria Hospital. Wethank Drs. Barbara E. Jones and M. Catherine Bushnell for theirinput in thismanuscript.
Correspondence should be addressed to Dr. Pierre Fiset, Department of Anesthesiology, Royal Victoria Hospital, 687 Pine AvenueWest, Room S5.05, Montreal, Quebec, Canada H3A1A1.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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