Neuronal Correlates for Preparatory Set Associated with Pro-Saccades and Anti-Saccades in the Primate Frontal Eye Field

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The Journal of Neuroscience, January 1, 2000, 20(1):387-400

Neuronal Correlates for Preparatory Set Associated with Pro-Saccades and Anti-Saccades in the Primate Frontal Eye Field
Stefan Everling and Douglas P. Munoz
Medical Research Council Group in Sensory-Motor Neuroscience, Department of Physiology, Queen's University, Kingston, Ontario K7L 3N6, Canada

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Diversity in behavioral responses to sensory stimuli has been attributed to variations in preparatory set. Variability inoculomotor responses toward identical visual stimuli has beenwell documented, but the neuronal processes underlying this variabilityare poorly understood. Here, we report evidence for set-relatedactivity for saccadic eye movements in single neurons in the frontaleye field (FEF) in monkeys trained on a task in which they eitherhad to look toward a visual stimulus (pro-saccade) or away fromthe stimulus (anti-saccade) depending on a previous instruction.A portion of FEF neurons were identified as neurons projectingdirectly to the superior colliculus (SC) with antidromic activationtechniques. Saccade-related neurons in the FEF had lower prestimulusand stimulus-related activity on anti-saccade trials comparedwith pro-saccade trials. The level of prestimulus activity correlatedwith saccadic reaction times, express saccade occurrence, anderrors in the anti-saccade task. In addition, saccade-relatedactivity in the FEF was higher for pro-saccades than for anti-saccades.These results demonstrate that the direct descending pathway fromthe FEF to the SC carries preparatory set-related activity forpro-saccades and anti-saccades. The results also provide insightsinto the neuronal basis of variations in saccadic reaction timesand in the control of the prepotent response to glance to a flashedstimulus.

Key words: frontal eye field; eye movement; anti-saccade; motor preparation; saccade; frontal lobe; superior colliculus; monkey

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

One of the most remarkable behavioral features of humans and animals is the moment to moment variability of responses to identicalsensory stimuli (Sherrington, 1910; Kupfermann et al., 1974; Wiseet al., 1996a). This flexibility, evident in the type of the responseand in its reaction time, has been attributed to variations inreadiness to make a response or in intention to perform a particulartask, both commonly referred to as preparatory set (Hebb, 1972;Evarts et al., 1984). For the oculomotor saccadic system, variabilityin reaction times is well documented. Saccadic reaction time (SRT)toward a flashed visual stimulus (pro-saccades) can range from90 to >400 msec with a mean of ~200 msec (Westheimer, 1954). Althoughthe common response is to look toward a suddenly flashed visualstimulus (Hess et al., 1946; Ingle, 1973), humans (Hallett, 1978;Hallett and Adams, 1980; Fischer and Weber, 1992) and monkeys(Schlag-Rey et al., 1997; Amador et al., 1998; Everling et al.,1998a, 1999) can be instructed in advance not to look to the stimulusbut instead to look to the opposite side, in a task that is knownas the anti-saccade task (for review, see Everling and Fischer,1998).

Neurophysiological evidence for set-related activity in the anti-saccade task has been found in the dorsolateral prefrontalcortex (DPC) and in the supplementary eye field (SEF). Many SEFneurons are more active on anti-saccade trials compared with pro-saccadetrials (Schlag-Rey et al., 1997). Furthermore, on anti-saccadetrials when the monkey failed to suppress an eye movement, theactivity of many neurons in the DPC (Funahashi et al., 1993) andin the SEF (Schlag-Rey et al., 1997) was similar to that associatedwith pro-saccades.

Another region of frontal cortex likely to display preparatory set activity for saccades is the frontal eye field (FEF) inthe rostral bank of the arcuate sulcus (for review, see Schall,1997; Schall and Thompson, 1999). A critical involvement of theFEF in the anti-saccade task has been supported by human lesion(Guitton et al., 1985) and brain-imaging studies (O'Driscoll etal., 1995; Sweeney et al., 1996; Doricchi et al., 1997). Moreover,acute inactivation of the FEF leads to a prolongation of SRTs(Sommer and Tehovnik, 1997; Dias and Segraves, 1999). In additionto visual and saccade-related responses (Bruce and Goldberg, 1985),many FEF neurons display low-frequency prestimulus activity (Bruceand Goldberg, 1985; Schall, 1991) that could be correlated withSRTs (Dias and Bruce, 1994). To address the question whether variationsin the activity of FEF neurons reflect differences in preparatoryset, we recorded the activity of single FEF neurons while monkeysperformed a task with randomly interleaved pro- and anti-saccadetrials.

Previous studies have shown that the variability in discharge of neurons in the superior colliculus (SC) reflects differencesin preparatory set (Basso and Wurtz, 1997, 1998; Dorris et al.,1997; Dorris and Munoz, 1998; Everling et al., 1999). To determinewhether the direct pathway from the FEF to the SC (Leichnetz etal., 1981; Fries, 1984; Segraves and Goldberg, 1987; Stanton etal., 1988; Lynch et al., 1994) carries set-related activity, weused antidromic activation techniques to identify corticotectalneurons in manyexperiments.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrophysiology. All experimental procedures were in accordance with the Canadian Council on Animal Care policy on the useand care of laboratory animals and approved by the Queen's UniversityAnimal Care Committee. Surgical, electrophysiological, and dataacquisition methods were described previously (Munoz and Istvan,1998; Everling et al., 1999). Briefly, two male monkeys (Macacamulatta) were implanted with scleral search coils, a head-restrainingdevice, and two recording chambers, one centered above the arcuatesulcus (right hemisphere in monkey a and left hemisphere in monkeyb) for neuron recordings in the FEF and one centered on the midlineand tilted 38° posterior of vertical for microstimulation of theSC. These were the same animals that we used for single neuronrecordings in the SC in the same paradigm (Everling et al., 1999).Single neurons were recorded in the rostral bank of the arcuatesulcus. The FEF region was first identified by low-threshold microstimulation(<50 µA at 100 msec, 300 Hz, 0.3 msec biphasic pulses) that reliablyelicited a contraversive saccade. The intermediate layers of theSC were identified by neuronal recordings and microstimulation(Everling et al., 1999). For antidromic activation of corticotectalneurons, single biphasic current pulses (0.1-0.3 msec) were passedthrough one of four chronically implanted monopolar tungsten microelectrodesinserted into the intermediate layers of the ipsilateral SC andan indifferent electrode. Electrodes were implanted in the SCfor 2-4 weeks. One electrode was placed at <2° eccentricity onthe collicular motor map; the other three electrodes were placedbetween 10 and 20° eccentricity (~45° up, approximately horizontal,~45° down) on the collicular motor map (Robinson, 1972). The responsesto SC stimulation that were recorded in the FEF were digitizedon a hard drive at 30 kHz (DataWave Technologies) for subsequentoff-line analysis. We stored the epoch spanning 5 msec beforeto 10 msec after the onset of stimulation. Single biphasic stimulationpulses were delivered while the activity of a single FEF neuronwas monitored (Fig. 1). The current threshold for antidromic excitationranged from 15 to 1500 µA, with a mean of 370 µA (median, 200µA). Antidromic responses were verified with several criteria,including fixed threshold, fixed latency, ability to follow high-frequencytwin pulses, and collision testing (Lipski, 1981). Stimulationpulses were not delivered during recordings of the behavioralparadigms.

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Figure 1. Experimental configuration and antidromic responses. A, Lateral view of a rhesus monkey brain illustrating single-neuron recording in the FEF and stimulation of the ipsilateral SC. B, Antidromic response of an FEF neuron (arrow, top trace) and its collision with a spontaneously generated action potential (arrow, bottom trace) that triggered microstimulation. The vertical dashed line indicates the time of SC stimulation. C, Histogram of antidromic latencies for 33 identified corticotectal neurons. Hatched bars indicate saccade-related neurons.

Behavioral task. Monkeys were trained on a task with randomly interleaved pro- and anti-saccade trials. Details of the experimentalsetup and paradigms were described previously (Everling et al.,1999). Briefly, visual stimuli were back-projected onto a tangentscreen by light-emitting diodes (red and green, 0.3 cd/m²). Each trial of the pro-/anti-saccade paradigm (Fig. 2A,B) beganwith the presentation of a central fixation point (FP) on thescreen. The monkey was required to look at it and maintain fixationfor 700-900 msec. A red FP signaled a pro-saccade trial (Fig.2A), and a green FP signaled an anti-saccade trial (Fig. 2B).On half of the trials, the FP remained illuminated throughoutthe trial (overlap condition). On the other half of the trials(gap condition), the FP disappeared 200 msec (gap period) beforestimulus presentation. The gap condition was included to increasethe variability of behavioral responses (Fischer and Weber, 1992;Everling et al., 1998a; Munoz et al., 1998). An eccentric redvisual stimulus was then presented pseudorandomly with equal probabilityeither at the position that yielded the optimal saccade-relatedresponse of the neuron (response field) or at the mirror locationon the opposite side of the horizontal and vertical meridians.The monkeys received a liquid reward if they looked within 500msec to the correct position and maintained fixation there forat least 200 msec. During the recording of each neuron, 15-20trials of each of the eight conditions (pro/anti, gap/overlap,in/out response field) were presented in a pseudorandom order.

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Figure 2. Spatial and temporal representation of the behavioral paradigm. A, B, The monkey was required to look at a central FP for 700-900 msec. A red FP signaled a pro-saccade trial, and a green FP signaled an anti-saccade trial. On half of the trials, the FP disappeared 200 msec before the peripheral stimulus was presented (Gap condition). On the other half of the trials, the FP remained illuminated throughout the trial (Overlap condition). A red stimulus was then presented pseudorandomly and with equal probability either in the response field of the neuron (dashed circle) or at the mirror position. On pro-saccade trials (A), the monkey was required to look toward the stimulus (red solid arrow), whereas he had to look to the mirror position (green solid arrow) on anti-saccade trials (B). Monkeys sometimes generated incorrect responses in the gap anti-saccade condition (red dashed arrow). E, Eye position; FP, fixation point; S, stimulus. C, Cumulative distribution of SRTs of all pro-saccades (red) and anti-saccades (green) in the gap (dashed lines) and overlap conditions (solid lines) obtained while recording from neurons in the FEF. The thick dotted red line represents incorrect responses in the gap anti-saccade condition. The mean SRT ± SD (and number of responses) in each condition was pro-gap, 164 ± 130 msec (n = 5303); pro-overlap, 239 ± 142 msec (n = 5210); anti-gap, 205 ± 111 msec (n = 4455); anti-overlap, 279 ± 122 msec (n = 4532); direction errors in the anti-gap, 179 ± 233 msec (n = 1482).

To dissociate stimulus-related from saccade-related responses, we also tested most of the neurons on a delayed visual anddelayed memory saccade task (Munoz and Wurtz, 1995). Briefly,each trial started with the monkey fixating a FP in the centerof the screen. A visual stimulus was then presented either inthe center of the response field of the neuron or on the oppositeside of the horizontal and vertical meridians. The stimulus eitherremained visible throughout the trial (delayed visual task) ordisappeared after 100 msec (delayed memory task). The monkey wasrequired to maintain central fixation on the FP for an additionalperiod of 400-1000 msec, until the FP disappeared, which was thecue to look to the visible or memorized target. The monkey receiveda liquid reward if it looked to the visible or memorized targetlocation within 500 msec and maintained fixation there for atleast 300msec.

Data analysis. During off-line analysis, trials with reaction times <80 msec were excluded as anticipations and trials withreaction times >500 msec as no-response trials. For all analyses,only neurons with at least five trials for each condition wereincluded. A Gaussian activation function (Richmond and Optican,1987) with a SD of 20 msec was used to construct continuous spikedensity waveforms and to obtain the levels of neuronal activitywith a binwidth of 1 msec. Smaller SDs (4 and 10 msec) did notchange the overall shape of the activation waveform, but resultedin a higher scatter caused by the relatively low discharge rateof cortical neurons. For comparing the neuronal activity duringthe instruction period (visible fixation point: red, pro-saccade;green, anti-saccade), we determined the mean activity during theperiod 400-200 msec before stimulus presentation for correct pro-saccadeand anti-saccade trials. Gap and overlap trials were combinedfor this analysis. For comparing the neuronal prestimulus activity,we determined the mean activity in the period 40-50 msec afterstimulus presentation. This period reflected the level of activationof the neuron before the visual signal arrives in the FEF (>70msec for our sample; see also Schmolesky et al., 1998). For comparingstimulus-related responses, we determined the mean activity inthe interval ±5 msec around the peak of neuronal activation ina time window from 70 to 140 msec after stimulus appearance, andthe prestimulus activation in the interval 40-50 msec after stimuluspresentation was subtracted as the baseline activity from thisvalue. This analysis was performed on trials collected in theoverlap condition only with the exclusion of all saccades withSRTs <150 msec to avoid a contamination of the stimulus-relatedresponse with saccade-related activity. For comparing saccade-relatedresponses, we determined the largest peak of activity in the intervalfrom 20 msec before to 40 msec after saccade initiation for eachneuron in the overlap condition. Then, the average activity wasmeasured in a 10 msec interval extending from 5 msec before to5 msec after the peak. For this analysis, only saccades that landedwithin a radius that deviated less than ±25% of the optimal vectorof the saccade were included. Comparisons were performed witha paired Student's t test or, if a test of normal distributionfailed (Kolmogorov-Smirnov test), with the nonparametric Wilcoxonsigned-ranktest.

Neuron classification. We used the classification scheme of Bruce and Goldberg (1985) and Segraves and Goldberg (1987) toclassify FEF neurons based on their discharge. After isolatinga single neuron in the FEF for recording, it was tested for acorticotectal projection with antidromic stimulation of the SC.We then recorded its activity in the combined pro-/anti-saccadetask (Fig. 2). The delayed visual and memory saccade tasks werethen used to dissociate stimulus-related and saccade-related responses.Only neurons that increased their discharge transiently for saccadesinto their response field were classified as saccade-related.If we could not maintain stable recording long enough to run thedelayed visual and memory saccade tasks, we classified the neuronon the basis of its discharge behavior during the anti-saccadecondition. Only neurons that increased their discharge transientlyfor anti-saccades in their response field were classified as saccade-related.For all analyses, we only included saccade-related neurons thatincreased their discharge >20 spikes/sec for visually guided saccades.Of these saccade-related neurons, we classified neurons as visuomovementneurons if they also increased their discharge >20 spikes/secafter the appearance of a visual stimulus in their receptive field.Saccade-related neurons that increased their discharge <20 spikes/secafter the appearance of a visual stimulus were classified as movementneuronsonly.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Behavior

Figure 2C shows the cumulative distribution of SRTs obtained from the two monkeys in the combined pro-/anti-saccade paradigmduring experiments in which we recorded from FEF neurons. Consistentwith our previous observations, anti-saccades had longer SRTsthan pro-saccades, and saccades in the overlap condition had longerSRTs than saccades in the gap condition. Furthermore, anti-saccadesin the gap condition had shorter SRTs than pro-saccades in theoverlap condition. The shortest SRTs were observed for directionerrors in the anti-saccade gap condition. Figure 2C also illustratesthe broad distribution of SRTs for all types ofsaccades.

Identification of corticotectal neurons

The antidromic identification of a corticotectal visuomovement neuron is shown in Figure 1B, and its activity in the combinedpro-/anti-saccade task is illustrated in Figure 3. Stimulationof the SC led to activation of an action potential in the neuronafter a fixed delay of 1.7 msec (Fig. 1B, top trace). When theSC stimulation immediately followed an orthodromic action potential(Fig. 1B, bottom trace), the response to SC stimulation was annihilated,verifying that the response was caused by antidromic activation(Lipski, 1981). In the combined pro-/anti-saccade task, the neuronincreased its discharge shortly after the visual stimulus appearedin its response field (Fig. 3A,C, left panels, all rasters). Onpro-saccade trials, the neuron then discharged for saccades intoits response field, whereas the activity was suppressed beforean anti-saccade was generated away from the response field (Fig.3A,C, right panels, bottom rasters). The neuron also increasedits discharge for all saccades into its response field (Fig. 3A,C,right panels, top rasters; B,D, right panels, bottom rasters).Therefore, the neuron was classified as a corticotectal visuomovementneuron. The peak in saccade-related discharge, however, was laterfor anti-saccades than for pro-saccades. This discharge patternis similar to SC neurons (Everling et al., 1999). The neuron alsohad a lower activity during the instruction period before stimulusappearance on anti-saccade trials compared with pro-saccade trials(green traces below red traces). The neuron increased its activityduring the gap period on pro-saccade and anti-saccade trials (Fig.3C,D).

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Figure 3. Activity of a corticotectal neuron (same as Fig. 1B) recorded in the FEF during the pro-/anti-saccade paradigm. Activity in the left panels is aligned on appearance of the eccentric stimulus (S on), and activity in the right panels is aligned on the beginning of the saccade (Saccade onset). A, Activity of the neuron on overlap trials when the stimulus was presented in its response field (RF, dashed circle) on pro-saccade trials (red) and anti-saccade trials (green). Each dot indicates the time of an action potential, and each row represents one trial. The trials are sorted according to saccadic reaction times (indicated by vertical tickmarks). The bottom panel shows the average activation waveforms for pro-saccades (red, thick) and anti-saccades (green, thin). B, Same as in A but for stimulus presentations at the mirror position of the response field of the neuron. C, Same as in A but for the gap condition in which the FP disappeared 200 msec before stimulus appearance. D, Same as in C but for stimulus presentations at the mirror position of the response field of the neuron in the gap condition.

In a total of 85 experimental sessions, we recorded from 176 neurons in the FEF. Eighty neurons displayed saccade-relatedactivity (32 visuomovement and 48 movement) and provided sufficientdata for this report. In 25 of these sessions, the monkeys wereimplanted with stimulation electrodes inserted into the intermediatelayers of the SC for antidromic identification. During these sessions,we identified 33 neurons as corticotectal (Fig. 1). Of these 33neurons, 18 (54%) neurons were identified as saccade-related (12visuomovement and 6 movement neurons). The remainder comprisedother classes of FEF neurons (Bruce and Goldberg, 1985). The distributionof antidromic latencies is illustrated in Figure 1C. The meanantidromic latency ± SD for all 33 antidromic neurons was 2.49± 1.08 msec (range, 0.8-5.0 msec) and for the 18 saccade-relatedneurons (described in this report) it was 2.13 ± 0.93 msec (range,0.8-4.0 msec). Antidromic neurons that did not fulfill our criteriafor saccade-related neurons had slightly longer latencies (2.93± 1.12 msec; range, 1.2-5.0 msec; unpaired t test, t = 2.27; df= 32; p = 0.031). The range of values we report (Fig. 1C) is comparableto the antidromic latencies described previously for corticotectalneurons in the FEF (Segraves and Goldberg, 1987: mean, 2.25 msec,range, 1.2-6.0 msec; Sommer and Wurtz, 1998: mean, 2.1 ± 1.5 msec,minimum, 0.7msec).

To establish whether neural activity in the FEF reflected variations in preparatory set and influenced the ensuing behavioralperformance, we performed correlations between FEF neural activityand behavioral responses and between FEF neural activity and taskcondition. In the subsequent sections, we contrast the dischargeof all FEF saccade-related neurons in the pro-/anti-saccade paradigm(1) during the instruction period before stimulus appearance,(2) during the gap period, (3) between prestimulus activity andSRT, (4) between prestimulus activity and express saccades, (5)between prestimulus activity and anti-saccade errors, (6) in themagnitude of stimulus-related activity, and (7) in the magnitudeof saccade-related activity. For each analysis, at least fiveresponses were required in each category. Therefore, the numberof neurons tested in each analysis varied. In each analysis wesummarize the results for all saccade-related neurons (Table 1)and the subset of neurons antidromically activated from the SC(Table 1, bracketed values; Figs. 4, 5, 7-11, filled squares).


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Table 1. Comparison of activity in pro-saccade versus anti-saccade trials

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Figure 4. Activity during the instruction period. The mean discharge rate of individual neurons in the period 400-200 msec before stimulus presentation on pro-saccade trials is plotted against the mean activity on anti-saccade trials. Filled squares indicate antidromically activated corticotectal neurons. Dashed line is the unity line (slope, 1).

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Figure 5. Prestimulus activity on overlap and gap trials. A, Mean spike density on pro-saccade trials (thick lines) and anti-saccade trials (thin lines) in the overlap (solid lines) and gap (dashed lines) conditions. B, The mean discharge rate of individual neurons in the period 40-50 msec after stimulus presentation (A, shaded region) on overlap pro trials (mean, 11.7 ± 1.1 spikes/sec) is plotted against the mean activity on gap pro trials (mean, 19.8 ± 1.6 spikes/sec). Filled squares indicate antidromically activated neurons. Dashed line is the unity line (slope, 1). C, Same as in B but for the comparison of anti-saccades between the gap (mean, 15.7 ± 1.1 spikes/sec) and overlap condition (mean, 9.0 ± 1.4 spikes/sec). D, Same as in B but for the comparison between pro- and anti-saccades in the gap condition.

Instruction period-related neuronal activity

Monkeys were instructed by the color of the initial FP at the beginning of each trial, whether they were required to generatea pro-saccade or an anti-saccade after peripheral stimulus presentation(Fig. 2A,B). Therefore, if the activity of FEF neurons reflectspreparatory set, neurons should show differential activation patternsbetween pro-saccade and anti-saccade trials during the instructionperiod (red FP, pro-saccade; green FP, anti-saccade). We quantifiedthe activity during the instruction period for the populationof saccade-related neurons in the interval 200-400 msec beforestimulus presentation (Table 1, Fig. 4). A lower activity onanti-saccade trials was found in the majority of neurons (51 of80, or 64%). These differences were significant for 31% (25 of80) of the neurons (t test, p < 0.05) and for the population.This finding revealed that FEF saccade-related neurons do indeedmodulate their activity during the instruction period, beforethe stimulus ispresented.

Gap-related neuronal activity

To examine whether the activity of FEF neurons represents a neuronal correlate for the reduction of SRTs in the gap saccadetask (Saslow, 1967; Fischer and Boch, 1983; Forbes and Klein,1996; Paré and Munoz, 1996), half of the trials in the paradigmincluded a gap of 200 msec between FP disappearance and stimulusappearance. Consistent with a previous report (Dias and Bruce,1994), we observed an increase in discharge during the gap periodin the majority of FEF saccade-related neurons (68 of 80, or 85%).Figure 5A illustrates the activity of the 80 neurons as it evolvedin the time leading up to appearance of the eccentric stimulus.There was an increase in activity ~100 msec after FP disappearanceon both pro-gap and anti-gap trials. Significant differences (ttest, p < 0.05) between gap and overlap pro-saccade trials wereobtained for 58% (46 of 80) of the neurons (Fig. 5B) and for thepopulation (Wilcoxon signed rank test, p < 0.0001). Increasesin discharge during the gap period compared with the overlap taskon anti-saccade trials were found in 77% (61 of 79) of the neurons(Fig. 5C). These differences were significant (t test, p < 0.05)in 44% (35 of 79) of the neurons and for the population (Wilcoxonsigned rank test, p < 0.0001).

The level of neuronal activity at the end of the gap period was significantly different between pro-saccade trials and correctanti-saccade trials (Table 1, Fig. 5A,D). A significantly higherlevel of prestimulus activity on pro-saccade trials was observedin 30% (24 of 79) of the neurons. However, five neurons FEF neuronswere significantly more active at the end of the gap period foranti-saccades than for pro-saccades.

Relationship between SRT and neuronal activity

Neurons that modulate their discharges during the gap period could account for the reduction of SRTs in the gap task as observedpreviously in the SC (Dorris et al., 1997; Dorris and Munoz, 1998;Everling et al., 1999). To test this hypothesis for FEF neurons,we computed the trial-by-trial correlation coefficient (Pearson'sproduct-moment correlation coefficient r) between the level ofprestimulus activity in 10 msec bins beginning from 200 msec beforeto 100 msec after stimulation presentation with SRT in the gapcondition for pro-saccade and anti-saccade trials. For this analysis,we selected neurons that had significant differences in prestimulusactivity between the gap condition and the overlap condition onpro-saccade trials and for which we obtained at least 10 trialsin each condition. For pro-saccades and anti-saccades, the correlationcoefficients between SRT and the level of neuronal activity contralateralto the subsequent saccade became more negative the closer thecorrelation window moved to the onset of visual responses (>70msec) (Fig. 6A). The distribution of correlation coefficientsbetween prestimulus activity in the interval 40-50 msec afterstimulus appearance and SRT is shown in Figure 6, B and C, respectively,for pro-saccades and anti-saccades. For pro-saccades, the meancorrelation coefficient was $-$ 0.18 for saccades into the responsefield of the neuron (one sided t test against 0, p = 0.0003) and $-$ 0.03 for saccades opposite to the response field of the neuron(one-sided t test against 0, p = 0.33). For anti-saccades, themean correlation coefficient was $-$ 0.20 for saccades into the responsefield of the neuron (one sided t test against 0, p < 0.0001) and $-$ 0.07 for saccades opposite to the response field of the neuron(one sided t test against 0, p = 0.12). This finding is consistentwith the hypothesis that the prestimulus activity of FEF neuronsreflects the monkey's preparatory state. The higher the levelof prestimulus activity of a neuron is immediately before thearrival of the visual signal in the frontal eye field, the fastera saccade into the response field of the neuron will be initiated.Thus, the variability of SRTs is partly related to the variabilityof low-frequency prestimulus activity in FEF saccade-related neurons.

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Figure 6. Relationship between neuronal activity and saccadic reaction times in the gap condition. A, Mean correlation coefficients between neuronal activity and saccadic reaction times in 10 msec bins from 200 msec before to 100 msec after stimulus presentation for pro-saccades (thick lines) and anti-saccades (thin lines) in the response field of the neuron (solid lines) and to opposite position (dashed lines). B, C, Distribution of correlation coefficients between the mean activity from 40-50 msec after stimulus presentation (A, shaded area) and saccadic reaction time for pro-saccades and anti-saccades, respectively. The filled bars represent neurons with statistically significant correlations (p < 0.05).

Neuronal activity and express saccades

We have shown that FEF saccade-related neurons increase their discharge during the gap period and that the level of pre-saccadeneuronal activity correlated with SRT for contraversive saccades.A class of saccades with very short-latency SRTs that are favoredby the gap condition, express saccades (Fischer and Boch, 1983),are thought to be generated by a direct route from the visualcortex via the intermediate layers of the SC to the saccade generatorin the brainstem (Fischer, 1987; Schiller et al., 1987; Edelmanand Keller 1996; Dorris et al., 1997). This hypothesis is basedon the short latency of express saccades that approach the minimalafferent and efferent conduction times of this pathway (Carpenter,1981) and on the experimental finding that lesions of the SC inmonkey abolish express saccades, whereas lesions of the FEF inmonkeys do not have long-term effects on the proportion of expresssaccades (Schiller et al., 1987).

To investigate the role of the FEF in express saccade generation, we separated pro-saccade trials in the gap condition intoexpress saccade (SRTs, 80-125 msec) and regular saccade trials(SRTs, $>=$ 125 msec). Figure 7A illustrates the discharge of an FEFneuron during both express and regular saccade trials. The neuronhad a higher discharge rate at the end of the gap period on expresssaccade trials than on regular saccade trials. It then dischargeda saccade-related burst of action potentials for both expresssaccades and regular saccades. A higher prestimulus activity onexpress saccade trials was found for the population of FEF neurons(Fig. 7B,C; paired Student's t test, df = 15; t = 2.88; p = 0.01).These findings demonstrate that a high level of activity in theFEF before stimulus presentation is associated with the generationof saccades with latencies in the range of express saccades.

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Figure 7. Neural activity for express and regular saccades in the gap pro-saccade condition. A, Activity of a FEF neuron aligned on the presentation of the visual stimulus. Each dot indicates the time of an action potential relative to stimulus presentation, and each row represents one trial. The trials are sorted according to saccadic reaction times (indicated by vertical tickmarks). The bottom panel shows the average activation waveforms for express (thick) and regular (thin) saccades. B, Same as in A but aligned on the beginning of the saccade. C, Mean spike density of the sample of FEF neurons on express saccade trials (thick line) and regular saccade trials (thin line) for saccades into the response field of the neurons. D, Activity levels in the time 40-50 msec after stimulus presentation (B, shaded area) are plotted before express saccades (mean, 30.6 ± 5.7 spikes/sec) against the activity levels before regular saccades (mean, 20.8 ± 3.9 spikes/sec). The oblique dashed line represents the unity line (slope, 1). Filled squares indicate antidromically activated neurons.

Hanes and Schall (1996) have demonstrated that, in an oculomotor countermanding paradigm, saccades are elicited when the activityof saccade-related FEF neurons reaches a certain level of neuronalactivity. This threshold trigger level remained constant for allsaccadic latencies. Based on this finding, Hanes and Schall (1996)proposed a fixed saccade threshold for individual FEF neurons.To test this hypothesis for express saccades, we compared thepre-saccadic neuronal activity between express saccades and regularsaccades. For this analysis, we determined the mean level of neuronalactivity in the interval 20-10 msec before saccade initiation(Fig. 8A, hatched bar). This interval encompassed the activitythat can influence saccade initiation (Hanes and Schall, 1996).Figure 8B shows that the population of saccade-related neuronshad a similar pre-saccade activity for express and regular saccades(paired Student's t test, df = 15; t = 1.832; p = 0.087).

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Figure 8. Comparison of saccade-related activity on express and regular saccade trials. A, Mean spike density of the sample of neurons on express saccade trials (thick line) and regular saccade trials (thin line) for saccades into the response field of the neurons. B, The pre-saccade activity in the interval 20-10 msec before saccade onset (A, hatched area) of individual neurons on express saccade trials (mean, 48.0 ± 7.7 spikes/sec) is plotted against the pre-saccade activity on regular saccade trials (mean, 56.8 ± 10.9 spikes/sec). The oblique dashed line represents the unity line (slope, 1). Filled squares indicate antidromically activated neurons. C, The saccade activity (A, shaded area) of individual neurons on express saccade trials (mean, 97.1 ± 16.9 spikes/sec) is plotted against the saccade activity on regular saccade trials (mean, 98.2 ± 19.4 spikes/sec).

To address the question whether the motor discharge of FEF neurons is different for express and regular saccades, we alsocompared the saccade-related activity of both saccade types (Fig.8A, shaded area). Figure 8C shows that FEF neurons had the samemotor discharge for both express and regular saccades (pairedStudent's t test, df = 15; t = 0.31; p = 0.76). These resultsdemonstrate that in intact primates the FEF is active before andduring expresssaccades.

Anti-saccade errors

Humans and monkeys sometimes fail to suppress a reflexive saccade toward the stimulus in the gap condition when instructedto generate an anti-saccade (Everling et al., 1998a; Fischer andWeber, 1992; Munoz et al., 1998). These errors are especiallyhigh in young children (Munoz et al., 1998) and certain neurologicalor psychiatric disorders that involve in the frontal cortex and/orbasal ganglia (for review, see Everling and Fischer, 1998). Todetermine whether neural processes in the FEF could account forperformance in the anti-saccade task, we measured the activitylevel of neurons at the end of the gap period in the gap anti-saccadetask and compared between correct trials and error trials. Forthis analysis, we measured the level of neuronal activity in theperiod 40-50 msec after stimulus presentation in those neuronswith a least five correct and five incorrect gap anti-saccadetrials (35 neurons for stimulus presentations into the responsefield and 17 neurons for stimulus presentations at the mirrorposition). Figure 9A shows the activity of an identified corticotectalneuron for gap anti-saccade trials in which the stimulus was presentedin the response field of a neuron. The neuron increased its dischargeduring the gap period on correct trials and error trials, however,the activity was significantly higher on error trials (t test,p < 0.05). We could confirm this observation for the populationof FEF neurons (Fig. 9B,C; t test, p = 0.0002). The neuron thendisplayed an increase in discharge that was higher for error trials.The same observation was made for the population of FEF neurons(Fig. 9B,C). The magnitude of this discharge on error trials waslower when the activity was aligned on saccade onset (data notshown). This finding indicates that this activity is primarilystimulus-related. No differences in the level of prestimulus activitywere found between correct and error trials when the stimuluswas presented at the mirror position of the response field ofthe neuron (Fig. 9D,E; Wilcoxon signed rank test, p = 0.31). Thus,a high level of prestimulus activity of FEF neurons at the locationwhere the visual stimulus was represented was associated withthe generation of a reflexive saccade toward the stimulus (error)in the anti-saccade task.

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Figure 9. Activity on correct and error anti-saccade trials. A, Activity of an antidromically activated corticotectal neuron on correct trials (solid line) and error trials (dashed line) for stimulus presentations in the response field of the neuron (dashed circle). B, Mean spike density of the sample of FEF neurons on correct trials (thin solid line) and error trials (thick dashed line) for stimulus presentations into the response field of the neurons. C, Activity levels in the time 40-50 msec after stimulus presentation (B, shaded area) are plotted before correct anti-saccades (mean, 16.7 ± 1.9 spikes/sec) against the activity levels before errors (mean, 22.4 ± 2.3 spikes/sec). The oblique dashed line represents the unity line (slope, 1). Filled squares indicate antidromically activated neurons. D, Same as in C but for correct anti-saccades (mean, 18.2 ± 2.9 spikes/sec) and errors (mean, 13.8 ± 2.5 spikes/sec) for stimulus presentations at the mirror position.

Stimulus-related neuronal activity

Visuomovement neurons in the FEF increase their discharge after the presentation of a visual stimulus in their response field(Bruce and Goldberg, 1985; Thompson et al., 1996). The magnitudeof this visual response is greater in a saccade task in whichthe stimulus is the target for a saccade compared with a fixationtask in which the animal must maintain fixation (Wurtz and Mohler,1976; Goldberg and Bushnell, 1981; Thompson et al., 1997). Noenhancement of the stimulus-related activity was found when asaccade was made away from the response field of a neuron (Goldbergand Bushnell, 1981). In the anti-saccade task, the stimulus actsas both a distractor that can trigger an incorrect pro-saccadeand as a landmark for the anti-saccade. To determine the effectof these task demands on the stimulus-related activity of visuomovementneurons, we compared the magnitude of the stimulus-related responsebetween pro-saccade trials and anti-saccade trials. All visuomovementneurons exhibited a stimulus-related response only when the stimuluswas presented in their response field, independent of the directionof the subsequent saccade (Fig. 3A,C). Figure 10A shows the activityfor the population of saccade-related neurons with visual responses.Many neurons (19 of 32, or 60%) had already a lower prestimulusactivity on anti-saccade trials compared with pro-saccade trials(Table 1, Fig. 10B). This difference was significant for the populationof FEF neurons. Therefore, we subtracted the prestimulus activityfrom the stimulus-related activity for the analysis of the magnitudeof the stimulus-related response. Despite the identical propertiesof the stimulus, the majority of visuomovement neurons (28 of32, or 87%) had reduced visual responses on anti-saccade trials(Table 1, Fig. 10A,C). These differences were significant in 52%(20 of 32) of the neurons and for the population. Thus, the reducedvisual response of FEF neurons on anti-saccade trials is the resultof both a reduced level of prestimulus activity and a reducedstimulus-related activity.

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Figure 10. Stimulus-related activity. A, Mean spike density of the sample of visuomovement neurons on pro-saccade trials (thick line) and anti-saccade trials (thin line) for stimulus presentations into the response field of the neurons. B, The prestimulus activity (A, hatched areas) of individual neurons on pro-saccade trials is plotted against the prestimulus-related activity on anti-saccade trials. C, The stimulus-related activity (A, shaded area) of individual neurons on pro-saccade trials is plotted against the stimulus-related activity on anti-saccade trials after subtracting the prestimulus level of activity (A, hatched area). The oblique dashed lines represent the unity line (slope, 1). Filled squares indicate antidromically activated neurons.

Saccade-related neuronal activity

Saccade-related neurons in the FEF increased their discharge for both pro-saccades and anti-saccades (Fig. 3). A comparisonof the levels of pre-saccade activity before saccade initiation(Table 1, Fig. 11A, B) shows that FEF neurons had a lower pre-saccadeactivity before anti-saccades compared with pro-saccades. Thisfinding indicates that, among individual neurons, there may bedifferent saccade thresholds for pro- and anti-saccades.

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Figure 11. Saccade-related activity. A, Mean spike density of the sample of neurons on pro-saccade trials (thick line) and anti-saccade trials (thin line) for saccades into the response field of the neurons. B, The pre-saccade activity in the interval 20-10 msec before saccade onset (A, hatched area) of individual neurons on pro-saccade trials is plotted against the pre-saccade activity on anti-saccade. The oblique dashed line represents the unity line (slope, 1). Filled squares indicate antidromically activated neurons. C, The saccade activity (A, shaded area) of individual neurons on pro-saccade trials is plotted against the saccade activity on anti-saccade trials.

To determine the role of FEF neurons in anti-saccade generation, we compared the magnitude of the saccade-related activityof the sample of neurons for pro-saccades and anti-saccades (Fig.11A,C). The population of saccade neurons in the FEF had a lowersaccade-related activity for anti-saccades compared with pro-saccades(Table 1). However, a subset of neurons (11 of 46, or 24%), exhibitedslightly higher discharges for anti-saccades than for pro-saccades.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study is the first to provide evidence that the direct descending pathway from the FEF to the SC carries set-relatedactivity for saccades. Many saccade-related FEF neurons increasedtheir activity significantly during the gap period, they had higherlevels of prestimulus neuronal activity before express saccadescompared with regular saccades, they had higher levels of prestimulusneuronal activity on anti-saccade trials when monkeys made errors,and they had significantly lower discharges during the instructionperiod, the gap period, and reduced visual responses on anti-saccadetrials compared with pro-saccade trials. These correlations betweenneuronal activity and behavior are similar but weaker to thoseobserved previously in SC neurons (Dorris et al., 1997; Everlinget al., 1998a, 1999). The similar discharge pattern of SC andFEF neurons suggests that the preparatory set-related activityin SC neurons on pro-saccade and anti-saccade trials is mediated,at least in part, by direct descending projections from the FEFto the SC (Segraves and Goldberg, 1987).

Prestimulus activity and SRTs

The results described here demonstrate that the level of FEF neuronal activity immediately before stimulus presentation influencesthe reaction time of contralateral saccadic eye movements. Thehigher the activity, the shorter the subsequent SRT. Negativecorrelations between the level of prestimulus activity of singleneurons and reaction times have been found for saccades in theSC (Dorris et al., 1997; Dorris and Munoz, 1998; Everling et al.,1999) and for limb movements in the primary motor cortex (Lecaset al., 1986; Riehle and Requin, 1993). Event-related potentialsin humans have also shown differences in the prestimulus activationbetween fast and slow responses (Gratton et al., 1988; Everlinget al., 1998b). In an oculomotor countermanding task, Hanes andSchall (1996) did not find significant differences in the levelof prestimulus activity between saccades with short and long SRTsin FEF neurons. Instead, these authors reported that the stochasticgrowth rate of the activity of individual neurons toward a fixedthreshold correlated with SRTs. It should however be noted thata byproduct of the countermanding task used by Hanes and Schall(1996) is that SRTs were always >200 msec. Although we have notexplicitly investigated this hypothesis, our finding of similarlevels of presaccadic activity between express and regular pro-saccadesdoes support the fixed-threshold hypothesis for FEF neurons forshort-latency (<200 msec) responses. It is quite likely that prestimulusactivity plays an important role in dictating SRT for short-latencyresponses typical in the gap condition, whereas poststimulus activationis more important in determining SRT for the longer-latency responsesobtained in an oculomotor countermandingtask.

Role of the FEF in the generation of express saccades

Previous studies have demonstrated that monkeys can still generate express saccades after FEF lesions, whereas lesions ofthe SC abolish express saccades (Schiller et al., 1987). Thisobservation suggested that FEF activation is not required forexpress saccade generation. In fact, it has been proposed thatin humans express saccade generation may be facilitated afterFEF lesions (Guitton et al., 1985). This hypothesis was supportedby the finding that humans with lesions of the frontal cortexthat included the FEF, showed an increased percentage of expresssaccades in a gap saccade task (Braun et al., 1992). A later study,however, observed the opposite saccade behavior in humans withlesions restricted to the FEF (Rivaud et al., 1994). The authorsreported a bilateral increase in SRTs in the overlap task anda decreased number of express saccades in a gap saccade task inthe patients with FEFlesions.

We observed that saccade-related neurons in the FEF had a higher prestimulus activity before express saccades compared toregular saccades (Fig. 7). Moreover, we found that FEF neuronswere active during both express- and regular-latency saccades(Figs. 7, 8). How can the discrepancy between these findings andthe finding of a clear lack of any effect of FEF lesions on theoccurrence of express saccades (Schiller et al., 1987) be explained?We have suggested here that the similar discharge pattern of FEFand SC neurons on pro- and anti-saccade trials is partly the resultof a descending projection from the FEF to SC (Segraves and Goldberg,1987). However, the ascending disynaptic connection between theSC and the FEF via the mediodorsal thalamus (Lynch et al., 1994)leaves open the possibility that the differential activity ofFEF neurons before express and regular saccades may in fact bedriven at least in part by the SC. By examining the activity ofFEF neurons that were likely to receive inputs from the SC, Sommerand Wurtz (1998) recently suggested that the SC sends visual-relatedand saccade-related activity to the FEF. If this hypothesis istrue, then it is possible that the saccade-related activity ofFEF neurons for express saccades may reflect the saccade-relatedactivity in the SC for express saccades (Edelman and Keller, 1996;Dorris et al., 1997).

It has been hypothesized that in the case of an express saccade, the visual stimulus is capable of directly eliciting a saccadeif saccade neurons in the SC have already a high prestimulus activityat the time of stimulus presentation (Sommer, 1994; Edelman andKeller, 1996; Dorris et al., 1997). In this case, the visual burstof these neurons can pass a certain saccade threshold, and itbecomes functionally transformed into a motor burst. AlthoughFEF lesions have no long-term effect on express saccade generation,we hypothesize that the prestimulus activity in the FEF in intactmonkeys participates in the generation of express saccades byincreasing the excitation of SC neurons. The absence of long-termeffects of FEF lesions on express saccade generation may resultfrom post-lesion-induced neural plasticity that increases theexcitability of SC neurons to compensate for the reduced corticalexcitation.

Preparatory set for anti-saccades

Primates are not constrained to react to sensory stimuli with reflexive movements, but rather they can acquire almost arbitrarystimulus-response associations (Wise et al., 1996a). The prefrontalcortex is thought be essential for the formations of these arbitraryassociations (Passingham, 1993; Wise et al., 1996b). Several neurophysiologicalstudies have shown that the activity of neurons in the frontalcortex reflects the formation of stimulus-response associations(Chen and Wise 1995a,b, 1996; Assad et al., 1998). Lesions ofthe prefrontal cortex, however, do not only lead to difficultiesin learning new associations, but also result in an inabilityto suppress inappropriate behavior (Fuster, 1991). This becomesevident in the anti-saccade task in which patients with damageto the prefrontal cortex often fail to suppress a reflexive saccadetoward the stimulus before generating the anti-saccade (Guittonet al., 1985; Pierrot-Deseilligny et al., 1991).

The results of this study provide insights into how this executive control of the frontal cortex is expressed. The findingthat saccade-related FEF neurons have lower discharges duringfixation of the instruction cue on anti-saccade trials than onpro-saccade trials seems to reflect a neuronal correlate for differentpreparatory sets necessary for the different task requirements.The finding of a decreased prestimulus activity in FEF neuronson anti-saccade trials seems to support the hypothesis that thecorrect performance of this task is dependent on a top-down controlof the SC. Indeed, it has been shown that reflexive saccades (errors)in the anti-saccade task were preceded by a high prestimulus activityin a subset of SC saccade neurons and that they were associatedwith a vigorous burst of action potentials in response to stimuluspresentation (Everling et al., 1998a). Therefore, to avoid reflexiveunwanted saccades in the anti-saccade task, the activity of saccadeneurons in the SC must be reduced until the motor signal for theanti-saccade is generated, which can only occur after stimuluspresentation. The present results suggest that the brain may accomplishthis task at least in part by reducing the excitatory drive fromsaccade-related FEF neurons to the SC during anti-saccade trials.We have shown recently that not only saccade-related neurons inthe SC have a lower discharge during the instruction period butthat fixation neurons in the SC have a higher discharge on anti-saccadetrials compared with pro-saccade trials (Everling et al., 1999).It remains to be determined whether this increased activationof collicular fixation neurons is the result of a reduced inhibitionfrom saccade-related neurons mediated by intracollicular inhibition(Munoz and Istvan, 1998) or whether fixation neurons receive anincreased prestimulus excitation on anti-saccade trials from otherneurons in the frontal cortex. One possible source may be SEFneurons that display an increased discharge on anti-saccade trialscompared with pro-saccade trials (Schlag-Rey et al., 1997).

Role of the FEF in the generation of anti-saccades

This study has also demonstrated that saccade-related FEF neurons provide a movement signal for the anti-saccade. However,in contrast to SEF neurons (Schlag-Rey et al., 1997), the majorityof FEF neurons had lower discharges for anti-saccades comparedwith pro-saccades. This finding is surprising. First, brain-imagingstudies in humans have consistently demonstrated an increasedactivation of the FEF during anti-saccade tasks compared withpro-saccade tasks (O'Driscoll et al., 1995; Sweeney et al., 1996;Doricchi et al., 1997). Our data indicate that the populationof saccade-related FEF neurons has a higher activity for pro-saccadesthan for anti-saccades during all task periods (instruction, stimulus,and saccade). One possible explanation for this discrepancy maybe that the increased activation observed in imaging studies doesnot arise from an increased activation of saccade-related neurons,but from an increased activation of inhibitory interneurons withinthe FEF that suppress saccade-related neurons. Second, the FEFis generally regarded as being involved in the generation of purposivevoluntary saccades, whereas the SC is regarded as primarily involvedin the generation of reflexive visually driven saccades (Guittonet al., 1985; Fischer, 1987; Schiller et al., 1987; Guitton, 1991;Dias et al., 1995; Forbes and Klein, 1996; Sommer and Tehovnik,1997; Dias and Segraves, 1999). Our data, however, demonstratethat saccade-related neurons in the SC and in the FEF share manyattributes, including a higher saccade-related motor burst forpro-saccades compared with anti-saccades.

Based on the finding that saccade-related SC neurons have a lower level of neuronal pre-saccade activity for anti-saccadescompared with pro-saccades, we have recently suggested that theFEF or SEF may provide additional signals for anti-saccades thatbypass the SC (Everling et al., 1999). Although we have not attemptedto identify corticopontine neurons in this study, it is knownthat half of the FEF neurons that project to the pons are movementneurons (Segraves, 1992). Therefore, given the likelihood thatseveral neurons in our sample projected to the pons, it is unlikelythat visuomovement or movement neurons in the FEF can compensatefor the reduced input from the SC to the brainstem saccade generatorfor anti-saccades. This negative finding may support an importantrole of the SEF in the initiation of anti-saccades (Schlag-Reyet al., 1997).

Our study has demonstrated significant differences in the level of preparatory neuronal activity of FEF neurons between pro-saccadeand anti-saccade trials. Like in the SC, the task to suppressthe prepotent response to look toward a flashed visual stimulusis accomplished in the FEF by a decrease of preparatory saccade-relatedactivity. We hypothesize that an imbalance in favor of motor preparationover motor inhibition could lead to the high error rates in theanti-saccade task in various disorders with an underlying frontallobe pathology (for review, see Everling and Fischer, 1998).

  FOOTNOTES

Received July 13, 1999; revised Sept. 20, 1999; accepted Oct. 14, 1999.

This work was supported by the Medical Research Council of Canada and the EJLB Foundation. S.E. was supported by a postdoctoralfellowship from the Deutsche Forschungsgemeinschaft. D.P.M. isa research scholar of the EJLB foundation and a Medical ResearchCouncil of Canada Scientist. We are grateful to I. T. Armstrong,B. D. Corneil, J. Dafoe, M. D. Dorris, and M. A. Meredith forhelpful comments. We thank A. H. Bell for participating in partof the data collection. We are especially grateful to A. Lablansfor her excellent assistance in training and care ofanimals.
Correspondence should be addressed to Dr. Douglas P. Munoz, Department of Physiology, Queen's University, Kingston, OntarioK7L 3N6, Canada. E-mail: doug{at}eyeml.queensu.ca.

Dr. Everling's present address: Department of Experimental Psychology, Oxford University, South Parks Road, Oxford OX1 3UD,UK.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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