Reduction of Pentylenetetrazole-Induced Seizure Activity in Awake Rats by Seizure-Triggered Trigeminal Nerve Stimulation

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The Journal of Neuroscience, November 1, 2000, 20(21):8160-8168

Reduction of Pentylenetetrazole-Induced Seizure Activity in Awake Rats by Seizure-Triggered Trigeminal Nerve Stimulation
Erika E. Fanselow¹, Ashlan P. Reid², and Miguel A. L. Nicolelis¹^,²
Departments of ¹ Neurobiology and ² Biomedical Engineering, Duke University Medical Center, Durham, North Carolina 27710

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Stimulation of the vagus nerve has become an effective method for desynchronizing the highly coherent neural activity typicallyassociated with epileptic seizures. This technique has been usedin several animal models of seizures as well as in humans sufferingfrom epilepsy. However, application of this technique has beenlimited to unilateral stimulation of the vagus nerve, typicallydelivered according to a fixed duty cycle, independently of whetherongoing seizure activity is present. Here, we report that stimulationof another cranial nerve, the trigeminal nerve, can also causecortical and thalamic desynchronization, resulting in a reductionof seizure activity in awake rats. Furthermore, we demonstratethat providing this stimulation only when seizure activity beginsresults in more effective and safer seizure reduction per secondof stimulation than with previous methods. Seizure activity inducedby intraperitoneal injection of pentylenetetrazole was recordedfrom microwire electrodes in the thalamus and cortex of awakerats while the infraorbital branch of the trigeminal nerve wasstimulated via a chronically implanted nerve cuff electrode. Continuousunilateral stimulation of the trigeminal nerve reduced electrographicseizure activity by up to 78%, and bilateral trigeminal stimulationwas even more effective. Using a device that automatically detectsseizure activity in real time on the basis of multichannel fieldpotential signals, we demonstrated that seizure-triggered stimulationwas more effective than the stimulation protocol involving a fixedduty cycle, in terms of the percent seizure reduction per secondof stimulation. In contrast to vagus nerve stimulation studies,no substantial cardiovascular side effects were observed by unilateralor bilateral stimulation of the trigeminal nerve. These findingssuggest that trigeminal nerve stimulation is safe in awake ratsand should be evaluated as a therapy for human seizures. Furthermore,the results demonstrate that seizure-triggered trigeminal nervestimulation is technically feasible and could be further developed,in conjunction with real-time seizure-predicting paradigms, toprevent seizures and reduce exposure to nervestimulation.

Key words: epilepsy; trigeminal nerve; seizure detection; seizure control; pentylenetetrazole; bilateral stimulation

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Seminal neurophysiological studies performed several decades ago demonstrated that stimulation of either cranial nerves orareas of the brainstem can cause desynchronization of the corticalEEG (Moruzzi and Magoun, 1949; Zanchetti et al., 1952; Magneset al., 1961; Chase et al., 1967). Such desynchronization typicallyreflects a state of arousal and full vigilance in mammals andis opposite to the high degree of EEG synchronization observedduring seizure activity. Building on these classical findings,several researchers showed that stimulation of the vagus nervecan lead to EEG desynchronization (Zanchetti et al., 1952; Chaseet al., 1966, 1967; Chase and Nakamura, 1968). More recently,several studies have demonstrated that the desynchronization inducedby vagus nerve stimulation (VNS) in dogs can be used to reducestrychnine- or pentylenetetrazole (PTZ)-induced seizure activity(Zabara, 1985, 1992). This paradigm was demonstrated subsequentlyto be effective in other animals, with other seizure models (Lockardet al., 1990; Woodbury and Woodbury, 1990; McLachlan, 1993), andhas been used with moderate success in treating humans who haveotherwise intractable epileptic seizures (Penry and Dean, 1990;Uthman et al., 1990, 1993; Ben-Menachem et al., 1994; Vagus NerveStimulation Study Group, 1995; McLachlan, 1997; Schachter andSaper, 1998). Because 0.5-2% of the population has epilepsy (Schachterand Saper, 1998; McNamara, 1999) and 10-50% of these patientsdo not respond well to antiepileptic medications and/or may notbe candidates for resective epilepsy surgery (McLachlan, 1997;Schachter and Saper, 1998), there is a substantial need for potentialalternative therapies for chronic seizures. Indeed, the VNS techniquehas recently received FDA approval and is currently being usedinpatients.

There are, however, several limiting factors of the VNS technique, which, if addressed, could greatly increase the efficacyand applicability of cranial nerve stimulation for seizure reductionin patients. First, the standard implementation of VNS in humanstypically involves stimulating the vagus nerve on a fixed, intermittentduty cycle (e.g., 30 sec on; 5 min off; 24 hr a day), independentlyof whether any seizure activity is ongoing or imminent (althoughthe use of manual patient- or caregiver-triggered stimulationvia a handheld magnet has also been used) (Terry et al., 1990;Uthman et al., 1993). This type of protocol has been used in previousstudies for two main reasons. First, although continuous stimulationmay have a greater therapeutic effect than intermittent stimulation(Takaya et al., 1996), continuous stimulation can cause nervedamage, whereas intermittent stimulation does not (Agnew et al.,1989; Agnew and McCreery, 1990; Ramsay et al., 1994). Second,the side effects associated with VNS are typically experiencedduring the stimulation (Uthman et al., 1993; Ramsay et al., 1994;McLachlan, 1997), so giving intermittent stimulation reduces theiroccurrence. However, because stimulation is delivered regardlessof whether seizure activity is present or is likely to occur,this fixed stimulation protocol has the disadvantage that thepatient may receive excessstimulation.

The second main problem is that the vagus nerve is involved in, among other things, cardiovascular and abdominal visceralfunctions. Indeed, because of the pattern of vagus innervationof the heart, the vagus nerve can only safely be stimulated unilaterally(i.e., on the left side only). This is a potential limitationin the efficacy of cranial nerve stimulation because the effectsof the stimulation may be bilateral (Chase et al., 1966; Zabara,1992; Henry et al., 1998, 1999) and may, therefore, be aided byadding more stimulation sites. For these reasons, use of a nervewithout the types of visceral fibers that are found in the vagusnerve could potentially be more effective for seizurereduction.

Here, we demonstrate that trigeminal nerve stimulation reduced PTZ-induced seizures in awake rats. In addition, we show thatsuch stimulation was more effective when it was bilateral. Finally,we describe a real-time interface for automatically detectingseizure activity and eliminating it by providing stimulation onlywhen seizure activity is present. These results suggest that ifsuch techniques were implemented in human patients, they couldgreatly decrease the amount of stimulation necessary for seizurecontrol while increasing the efficacy of cranial nerve stimulationas a therapy for intractableepilepsy.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects. Eight adult female Long-Evans hooded rats weighing between 230 and 375 gm served as subjects in this study. Allprocedures and experiments were conducted in compliance with DukeUniversity Medical Center animal use policies and were approvedby the Duke University Institutional Animal Care and UseCommittee.

Induction of seizures. Seizures were induced by intraperitoneal injection of PTZ (40 mg/kg). This dose of PTZ induced generalizedseizure activity for 1-2 hr. This seizure activity was manifestedin two ways: (1) highly synchronous, large-amplitude activityin the thalamic and cortical field potential traces (see Figs.2, 3, 5-7) and (2) clonic jerking of the body and forelimbs. Thesetwo indicators of seizure activity were highly correlated at alltimes, as assessed by concurrent visual inspection of the animaland the real-time field potential traces. Occasionally, a supplementaldose of PTZ (7-10 mg/kg) was given if seizures ceased in <1hr.

Nerve cuff electrodes. The infraorbital nerve(s) was stimulated unilaterally or bilaterally via chronically implanted nervecuff electrodes. These electrodes were constructed in-house andconsisted of two bands of platinum (0.5 mm wide and 0.025 mm thick;~0.8 mm separation between bands) that ran circumferentially aroundthe infraorbital (IO) nerve (see Fig. 1, inset). The platinumbands were held in place and electrically insulated by a thinSylgard coating. Each band was connected to a piece of flexible,three-stranded Teflon-coated wire that was used to pass currentbetween the bands (Fanselow and Nicolelis, 1999).

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Figure 1. Schematic drawing of nerve cuff electrode and ASD device. Field potential signals from chronically implanted microwires in the VPM thalamus and/or SI cortex were sent to an amplifier and recording unit for collection, as well as to the ASD device. When the ASD device detected seizure activity, it sent a signal to the stimulator, which delivered a current pulse to the implanted nerve cuff electrode. Scale bar: inset, 1 mm.

Chronic implantation of microwire electrodes. Microwire electrodes (NBLabs, Denison, TX) were chronically implanted into theventral posterior medial thalamus (VPM) and/or primary somatosensorycortices (SI) for use in recording field potentials in these areas(Fig. 1). Three rats had arrays of 16 microwires implanted inlayer V of the SI cortex and bundles of 16 electrodes implantedinto the VPM thalamus, both contralateral to the stimulated nerve.Five rats had two arrays of 16 electrodes implanted, one eachinto layer V of the left and right SI cortices so that recordingscould be made both ipsilateral and contralateral to the nervebeingstimulated.

These implants were performed under pentobarbital anesthesia (50 mg/kg). Small craniotomies were performed over the areasinto which electrodes were to be implanted [coordinates from Paxinosand Watson (1986)]. Electrodes were slowly lowered into theseareas, and recordings were made throughout the implantation processto assess electrode location. After electrodes were in the correctposition, they were cemented to skull screws by the use of dentalacrylic (Nicolelis et al., 1997).

Chronic implantation of nerve cuff electrodes. After implantation of the microwires, nerve cuff electrodes were implantedeither unilaterally or bilaterally. A dorsoventral incision wasmade on the face several millimeters caudal to the caudal edgeof the whiskerpad. Tissue was dissected until the infraorbitalnerve was exposed, and the cuff electrode was positioned aroundthe nerve such that the nerve lay inside the cuff. The cuff wasthen tied around the nerve to hold it in place, and the woundwas sutured. The Teflon-coated leads from the platinum bands wererun subcutaneously to the top of the head where they were attachedto connector pins and affixed to theskull.

Recording procedures. Field potential recordings from VPM thalamus and SI cortex were made using chronically implanted microwires(Nicolelis et al., 1997). Field potentials were collected usinga Grass Model 15 amplifier and stored on a personal computer.Signals were collected at a sampling rate of 512 Hz and bandpassfiltered during collection at 1-100 Hz. During each recordingsession, 16 field potential channels were recorded, 8 from eacharea from which recordings were made in a given rat (either VPMand SI, or SI left and SI right). In addition, one channel wasrecorded for each nerve cuff being stimulated (unilateral or bilateralstimulation) to indicate when stimulation occurred. During experiments,animals were awake and allowed to move freely in a 30 cm × 30cm recordingchamber.

Stimulation parameters. Stimulation of the IO nerve cuff electrodes was provided by the use of a Grass S8800 stimulator inconjunction with a Grass SIU6 stimulus isolation unit. Unimodalsquare current pulses with a duration of 500 µsec were given ata range of currents and frequencies. Current values were variedfrom 3 to 11 mA (2 mA intervals), and frequency values were variedfrom 1 to 333 Hz (1, 5, 10, 20, 50, 100, 125, 200, and 333 Hz).Animals tolerated stimulation at these levels without indicationof pain, although in some animals there appeared to be a sensationof pressure on the face at the highest current and frequency settings.This was evidenced by a tendency for the animals to back up whenthe stimulus began, in the direction away from the stimulatedside if unilateral stimulation was provided or straight back inthe case of bilateral stimulation. In addition, at lower stimulusintensities animals would occasionally scratch at the whiskerpadon the side of the face being stimulated during the first fewseconds of stimulation. However, the scratching was neither intensenorprolonged.

Automatic seizure detection device. A device was designed and built in-house to automatically detect seizure activity in realtime and immediately trigger a stimulator when a seizure was detected(Fig. 1). The automatic seizure detection (ASD) device first low-passfiltered the raw field potentials obtained from the microwirearrays at 30 Hz. Circuitry then determined whether the field potentialactivity surpassed a threshold voltage value, indicative thatseizure activity was present. When the field potential voltagecrossed the threshold, a TTL pulse was sent to the Grass S8800stimulator, which delivered a 0.5 sec train of 500 µsec pulsesat 333 Hz. The current level was dictated by the stimulation protocolfor a given trial. Trains of stimuli were presented as long asthe field potential activity remained above the threshold value(i.e., as long as seizure activity was ongoing). The train durationfor the seizure-triggered stimulation (0.5 sec) was chosen becauseit was the shortest duration that we found to be effective forstopping the seizure activity, and we wanted to keep the stimulationas short as possible to reduce the total amount of stimulationgiven. The voltage threshold was set manually for each experiment.Generally, the seizure activity was three to five times that ofthe background activity, and the threshold was set high enoughto identify seizure activity only. After the threshold was setfor a given experiment, it was not moved. The seizure activityrecorded on the field potential traces was directly correlatedwith behavioral manifestation of the seizures (clonic jerkingof the body and forelimbs). When setting the seizure detectionthreshold, we always verified that the seizure activity identifiedby the ASD device was directly correlated with this behavioralcomponent of theseizures.

Experimental protocols. The first part of this study was performed to determine whether stimulation of the IO branch of thetrigeminal nerve was capable of eliminating PTZ-induced seizureactivity in awake rats. To do this, we delivered continuous stimulationto the IO nerve during episodes of PTZ-induced seizure activityvia the nerve cuff electrode (Fig. 1) for 1 min stimulus-on periods,separated by 1 min stimulus-off periods. This protocol was performedwith both unilateral and bilateral stimulation of the IO nerve.Stimulus parameters were varied between the stimulus-on periodsas describedabove.

In the second part of this study, we assessed the effectiveness of stimulating the IO nerve only when seizure activity waspresent by using the ASD. For this protocol, the ASD device wasturned on for 1 min stimulus-on periods, separated by 1 min stimulus-offperiods, as in the first protocol, but stimulation was only providedduring the stimulus-on periods when seizure activity was detectedby the ASDdevice.

Data analysis. We measured seizure activity in the field potential recordings in three ways: seizure frequency, seizure duration,and integrated seizure activity. These parameters were quantifiedby the use of a custom-made analysis program developed using Matlab.The field potential traces were first bandpass filtered at 5-30Hz. A sliding window (1 sec window with 0.5 sec overlap) was usedto quantify the activity of the absolute values of the field potentialtraces. Within each window, the amplitude (i.e., voltage) rangeof the absolute value of the field potential activity in eachtrace was divided into 10 equal parts, and within each slidingwindow the number of voltage values falling into each of the 10divisions of the amplitude range was calculated. Then, a thresholdof 50% of the amplitude range was used to identify seizure activity.If activity within three consecutive windows was above this threshold,the activity was considered to be part of a seizure. From thesedata, the number of seizures and their durations could be calculatedby counting the number of windows during which activity was abovethe threshold. In addition, a measure we call the "integratedseizure activity" was calculated by summing all of the valuesfor all of the amplitude range intervals for a given on or offperiod of stimulation. This algorithm was applied in a uniform,blinded manner to all of our data, allowing for objective quantificationof the three measures of seizureactivity.

Statistical analyses. Using the values for seizure number, seizure duration, and integrated seizure activity, we assessedthe efficacy of IO nerve stimulation and ASD by comparing eachstimulation-on period with the stimulation-off period directlypreceding it. Thus, results are presented as ratios of seizureactivity during stimulus-on periods to seizure activity duringstimulus-off periods. We used multivariate ANOVAs (MANOVAs) toassess whether there were statistically significant changes inseizure duration, seizure frequency, or integrated seizure activitybetween periods of no stimulation and periods of stimulation foreach stimulus parameter setting. In addition, repeated measureANOVAs were used when comparing one measure with another (e.g.,number of seizures compared with seizure duration). When significantdifferences were indicated by MANOVA or ANOVA analyses, Tukey'shonestly significant difference post hoc tests were used to identifywhich effects were significant (p < 0.05).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Control experiments

In control experiments in which PTZ was administered, but no IO nerve stimulation was provided, the average number of seizuresper minute was 5.98 ± 0.45, and the average seizure duration was3.94 ± 0.23sec.

In contrast to studies of VNS in rats (Woodbury and Woodbury, 1990) and dogs (Zabara, 1992), we did not observe any substantialcardiovascular side effects during IO nerve stimulation (Fig.2). We recorded electrocardiogram (EKG) signals in anesthetizedrats while stimulating the IO nerve and did not observe any substantialchange in heart rate during stimulation.

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Figure 2. EKG activity is not significantly altered during IO nerve stimulation. a, b, Two examples of EKG activity during IO nerve stimulation (stim; horizontal bars) in an anesthetized rat. Calibration: vertical, 100 µV; horizontal, 1 sec. c, The EKG traces and instantaneous heart rate (Inst. rate) over a 15 min period during which stimulation was twice provided continuously for 1 min, as well as five times for shorter bursts. Small changes in the EKG can be seen when stimulation is provided, but they are minor and rapidly stabilize, even during ongoing stimulation. i, ii, The traces that are shown at a faster time scale in a and b, respectively. Calibration: vertical, 100 µV for the EKG traces, 200 beats/min for the instantaneous heart rate; horizontal, 10 sec. The stimulus parameters in these traces were 50 Hz, 11 mA, and 0.5 msec pulse duration.

Stimulation of the infraorbital nerve reduces seizure activity

Stimulation of the infraorbital nerve by the use of the periodic stimulation paradigm substantially reduced PTZ-induced seizureactivity compared with that of control periods (Figs. 3, 4, 5).This effect was dependent on both the current and the frequencyof the stimulation. There were no significant differences betweenthe cortex and thalamus on any of the measures [Rao R(3,134) =0.33; p > 0.8].

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Figure 3. Stimulation of the IO nerve reduces seizure activity in a current-dependent manner. a1-a3, Filtered field potential traces showing seizure activity during three sequential 1 min periods (a1, no stimulus; a2, stimulus on; a3, no stimulus). The stimulus parameters for this figure were 11 mA, 333 Hz, and 0.5 msec pulse. b $---$ d, The amount of seizure activity during 1 min periods of stimulation at different current levels compared with the period of no stimulation directly preceding each stimulus-on period. Values are presented as a percent of the average stimulus-off period measurements. b, Integrated seizure activity. c, Number of seizures. d, Seizure duration. Error bars represent ±SEM. A solid line connects stimulation-off values; a dashed line connects stimulation-on values. Stimulation-on values significantly different from stimulation-off values are designated by an asterisk. Thick, black horizontal lines at 100% denote the level of no change in seizure activity. Calibration: vertical, 200 µV; horizontal, 10 sec.

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Figure 4. Effect of varying stimulus frequency using the periodic stimulation paradigm. a, Number of seizures. b, Seizure duration. Labeling conventions are described in Figure 3 (note the change in the scale of the y-axis in b).

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Figure 5. Effects of bilateral stimulation versus unilateral stimulation. a1 $---$ a3, Filtered field potential traces showing seizure activity during three sequential 1 min periods (a1, no stimulus; a2, bilateral stimulation; a3, no stimulus). The stimulus parameters were 9 mA, 333 Hz, and 0.5 msec pulse duration. b $---$ d, Values presented as ratios of stimulus-on/stimulus-off measurements. b, Integrated seizure activity. c, Number of seizures. d, Seizure duration. A solid line connects responses contralateral to the stimulation site; a line with long dashes connects responses ipsilateral to the stimulation site; a line with short dashes connects responses to bilateral stimulation. Responses to bilateral stimulation that are significantly different from those to ipsilateral and contralateral stimulation are represented by an asterisk. Other labeling conventions are described in Figure 3.

As expected from previous studies, the seizure reduction effect of IO nerve stimulation was greater with increasing currentlevels (Fig. 3b-d). For these experiments, pulse duration andfrequency were held constant at 0.5 msec and 333 Hz, respectively,while current was varied between 3 and 11 mA, in 2 mA increments.At currents of 3 and 5 mA, there were no differences between periodsof IO nerve stimulation and periods of no stimulation. However,at 7, 9, and 11 mA, nerve stimulation caused a significant decreasein overall seizure activity (Fig. 3b, 7 mA, 43.2 ± 7.0%; 9 mA,65.5 ± 4.7%; 11 mA, 77.5 ± 4.3%; p < 0.001) and in the numberof seizures initiated (Fig. 3c, 7 mA, 36.4 ± 5.8%; 9 mA, 50.5± 4.6%; 11 mA, 58.7 ± 6%; p < 0.0001). There was also a significantdecrease in the seizure duration at 9 mA (Fig. 3d, 52.5 ± 3.7%;p < 0.0001).

Different stimulus frequencies had different effects on the seizure activity (Fig. 4). For these experiments, pulse durationand current were held constant at 0.5 msec and 9 mA, respectively.Stimulation at high frequencies (100, 125, 200, and 333 Hz) causeda significantly smaller number of seizures than did periods ofno stimulation (Fig. 4a; p < 0.05), as described above. Stimulationfrequencies of 50 Hz and lower did not cause any significant changesin the number of seizures initiated (Fig. 4a; p = 1.0), but seizuresdid tend to be longer than those during control periods at thesefrequencies (Fig. 4b; 10 Hz; p < 0.02).

Bilateral versus unilateral stimulation

Bilateral stimulation was significantly more effective at reducing seizures than was unilateral stimulation either contralateralor ipsilateral to the recording site (Fig. 5). This effect wassignificant for the integrated seizure activity measure (Fig.5b) at a current level of 7 mA (75.7 ± 5.7%; p < 0.002), as wellas for the number of seizures (Fig. 5c) at 7 and 9 mA (7 mA, 63.7± 5.3; 9 mA, 78.1 ± 3.7%; p < 0.01). It is important to pointout that the superior effect of bilateral stimulation was onlyevident for the middle range of stimulation intensities used inthis study. That is, if the current was too low, presumably belowthe threshold for seizure reduction, there was no advantage instimulating both nerves, and if the current was high enough, stimulatingunilaterally was as effective as stimulating bilaterally. Howeverin the middle range of stimulation intensities, bilateral stimulationallowed us to use less current per nerve while still maintaininga high degree of seizurereduction.

Automatic detection of seizure activity and termination of seizures

Use of the ASD device to stimulate the IO nerve only when seizure activity was detected successfully reduced the amount ofseizure activity relative to control periods. Figure 6 shows thatwhen the seizure detector identified seizure activity in the fieldpotential traces and triggered the stimulator, the seizure stopped.As in the experiments described above, the degree of seizure reductionwas dependent on the current level (Fig. 7). For this set of experiments,we held the pulse duration constant at 0.5 msec, and the frequencyat 333 Hz. Current was varied from 3 to 11 mA in 2 mA increments.Figure 7b shows that the integrated seizure activity level wassignificantly reduced at 9 and 11 mA (9 mA, 55.2 ± 7.2%; p < 0.03;11 mA, 56.6 ± 8.0%; p < 0.01). The number of seizures was significantlydecreased at 7 and 9 mA (Fig. 7c, 7 mA, 19.3 ± 5.8%; p < 0.05;9 mA, 22.5 ± 6.1%; p < 0.0001). In addition, the seizure durationwas decreased at 7, 9, and 11 mA (Fig. 7d, 7 mA, 40.2 ± 3.3%;9 mA, 45.2 ± 3.6%; 11 mA, 49.4 ± 4.0%; p < 0.0001 for all). Tocompare the efficacy of the ASD device with that of the periodicstimulation paradigm, we calculated the ratio of the percent ofseizure reduction to stimulus-on time (Fig. 8). By comparing theseratios between ASD stimulation and periodic stimulation protocols,we observed that, at least in the acute seizure model (PTZ) usedin this study, delivering stimulation only when seizure activitywas detected was up to 39.8 times more effective at seizure reductionper second of stimulation than was periodic stimulation not relatedin any way to seizure activity.

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Figure 6. Seizure-specific stimulation stops synchronous activity. When the field potential amplitude reached a threshold value, the seizure detector (ASD device) triggered IO nerve stimulation. a $---$ c, Traces correspond to the roman numerals i-iii, respectively (see Fig. 7). Note that the stimulation outlasts seizure activity because pulses were provided in 500 msec trains. Also note that the traces indicating seizure detection and stimulation are only indicators and are not indicative of stimulation current or frequency. Calibration: vertical, 200 µV; horizontal, 500 msec.

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Figure 7. Seizure reduction using the ASD device. a1-a3, Filtered field potential traces showing seizure activity during three sequential 1 min periods (a1, no stimulus; a2, stimulus on; a3, no stimulus). The stimulus parameters were 9 mA, 333 Hz, and 0.5 msec pulse duration. Within each segment, the trace labeled seizure detector indicates where the ASD device detected seizure activity; the trace labeled stimulus on indicates where the ASD device sent a TTL pulse to trigger the IO nerve stimulator when it detected such activity. The roman numerals i-iii and arrows indicate parts of the traces that were enlarged to create Figure 6. b, Integrated seizure activity. c, Number of seizures. d, Seizure duration. Labeling conventions are described in Figure 3.

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Figure 8. Comparison of the amount of seizure reduction versus the amount of stimulation provided. Stimulation was provided by the use of the periodic stimulation paradigm (dashed line) or the ASD device (solid line). The y-axis represents the ratio of seizure activity reduction to seconds of stimulation in a given stimulus-on period. Asterisks designate the ratios of ASD seizure reduction to seconds of stimulation that were significantly higher than those obtained by the use of the periodic stimulation protocol. a, Integrated seizure activity. b, Number of seizures. c, Seizure duration.

There was an important difference between the nature of the seizure reduction effect using the ASD device and that observedusing the periodic stimulation paradigm described above. Withthe periodic stimulation paradigm, the number of seizures andthe seizure durations were reduced by approximately the same amountat each current level (Fig. 3, compare c, d). However, when theASD device was used, the seizure durations were reduced significantlymore than the number of seizures (Fig. 7, compare c, d; p < 0.000001).

In addition, analysis of the data revealed that in control experiments where PTZ was administered but no stimulation was provided,the average time between the end of one spontaneously occurringseizure and the beginning of the next was 6.1 sec (calculatedfrom the average number of seizures and the average seizure duration).We also measured the latency between the end of a stimulus andthe next spontaneous seizure (i.e., in the epoch after a stimulus-onperiod), which was 7.59 ± 1.29 sec. Thus, the average delay betweenthe end of a period of stimulation and the next spontaneouslyoccurring seizure is an average of 24% longer than the interseizureinterval during control experiments where no stimulation waspresent.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The results of this study demonstrate three substantial advances in the use of cranial nerve stimulation for the treatmentof seizures. First, we showed that stimulation of the trigeminalnerve can reduce PTZ-induced seizure activity in rats. This indicatesthat the seizure reduction effect of cranial nerve stimulationis not limited to stimulation of the vagus nerve but instead maybe mediated by a more nonspecific arousal mechanism that can berecruited by stimulation of a number of cranial nerves. Second,we showed that bilateral trigeminal nerve stimulation could havethe same seizure reduction effect as unilateral stimulation butrequired much less current to do so. This finding is therapeuticallyrelevant, because it suggests that multisite stimulation couldhelp maximize the seizure reduction effect of any technique usingcranial nerve stimulation, while using the lowest current levelspossible. Finally, we showed that in the acute seizure model usedin this study (PTZ), automatic, real-time seizure-triggered stimulationreduces seizures more effectively per second of stimulation thandoes periodic stimulation that is unrelated to seizure onset.This means that the use of a real-time brain-device interfacethat would automatically detect seizure activity and trigger anerve stimulator only when such activity was present could providea high degree of seizure control while potentially reducing theoverall amount of stimulation presented to a patient. We proposethat these findings may significantly improve the efficacy ofcranial nerve stimulation as a therapy for patients with intractableepilepticseizures.

Mechanism of seizure reduction by cranial nerve stimulation

The mechanism by which cranial nerve stimulation causes desynchronization of thalamic and cortical activity and reduces seizureactivity is unknown. However, one theory is that such stimulationactivates the midbrain reticular formation and that this activationresults in generalized arousal via the reticular-activating system.In support of this view, Gellhorn (1960) showed that stimulationof the midbrain reticular formation suppresses focal strychninespikes in cats. In addition, several methods of eliminating seizure-relatedactivity by activating multiple sensory modalities have been demonstrated.These include the reduction of absence seizures by acoustic stimuli(Rajna and Lona, 1989) and the reduction of interictal focal activityor absence seizures by motor or mental activity (Jung, 1962; Ricciet al., 1972) or by thermal stimulation (McLachlan, 1993). Becausesuch a wide range of manipulations can reduce seizure-relatedactivity, it is reasonable to suggest that seizure reduction inthese cases is caused by a generalized effect on arousal mediatedby the brainstem reticular formation. This is supported by theclassical work of Moruzzi and Magoun (1949) demonstrating thatstimulation of the midbrain reticular formation causes EEG desynchronization.This hypothesis is consistent with our finding that seizure reductioneffects are not specific to the vagus nerve but can instead beachieved by stimulation of multiple cranial nerves that conveyinformation to the reticularformation.

One important factor to consider with regard to both the mechanism of seizure reduction by trigeminal nerve stimulation andits applicability to long-term use in humans is the nature ofthe fiber types that must be activated to cause the seizure reductioneffect. Multiple studies of the VNS technique have shown thatthe level of stimulation, in terms of stimulus frequency and intensity,must be high enough to activate slowly conducting c-fibers (Chaseet al., 1967; Woodbury and Woodbury, 1990). The frequency rangewe found to be therapeutic in the present study was somewhat differentfrom that typically used in animal and human VNS studies. In animalstudies the usual therapeutic range was generally 10-30 Hz (Woodburyand Woodbury, 1990; Zabara, 1992; Takaya et al., 1996), althoughLockard et al. (1990) used higher stimulation frequencies (50-250Hz) in monkeys. In human studies the range used for stimulationwas typically 20-30 Hz (McLachlan, 1997). This difference betweenVNS studies and ours may be caused by the difference in the relativenumbers of fiber types between the vagus nerve and the infraorbitalnerve. In cat, the vagus nerve is composed of 65-90% unmyelinatedfibers (Foley and DuBois, 1937; Agostoni et al., 1957), whereasthe rat IO nerve contains ~33% slowly conducting, unmyelinatedfibers (Klein et al., 1988). However, it is not clear what therelationship is between fiber composition and the stimulus frequency/intensityrequired for seizure reduction, so interpreting these differencesis difficult. A complicating factor is that although it has beenshown that for seizure reduction the level of stimulation mustbe sufficient to activate c-fibers, it has not been demonstratedthat these fibers are necessary for the seizure reduction effect.Finally, it is important to note that according to studies byTorebjork and colleagues (Torebjork, 1974; Torebjork and Hallin,1974), c-fibers do not conduct if electrical stimuli are presentedat frequencies above ~10 Hz. This means that although high stimulationfrequencies were required for the seizure reduction effect observedhere, it is likely that at such frequencies the c-fibers werenot activated or were activated to a lesser degree than otherfibers in thenerve.

Furthermore, it is possible that cells in the trigeminal nucleus were not able to follow with sustained responses at the highrates of stimulation we provided. For example, Andresen and Yang(1995) demonstrated using a slice preparation of the rat medullathat neurons in the nucleus of the solitary tract (NTS) respondedwith lower EPSP amplitudes as the frequency of solitary tractstimulation was increased. These results may also be relevantto trigeminal nerve stimulation. If this is the case, it is unclearwhy our results show that higher frequency stimulation is moreeffective for seizure elimination than are lower stimulation rates.However, the study by Andresen and Yang (1995) also demonstratedthat bursts of high-frequency stimulation resulted in less EPSPattenuation than did continuous high-frequency stimulation, suggestingthat an optimal stimulation protocol could involve short burstsof high-frequency stimulation rather than continuoustrains.

The delay between the onset of seizure-triggered stimulation and the end of the seizure activity might shed some light onthe mechanism by which trigeminal stimulation reduces seizureactivity. The average time between the onset of the seizure-triggeredstimulus and the end of the seizure was 529.9 ± 40.3 msec (notethat Fig. 6 demonstrates some of the shortest delays). It is interestingthat this value is similar to the minimum effective stimulus trainduration (500 msec) that we determined empirically. However, itshould be noted that there was a wide range of delays, and thismay be caused by at least two factors. First, the phase of thesynchronous oscillations during which the stimuli occur may havea profound impact on the efficacy of the stimulation. Second,it is possible that the ability to abort a seizure varies dependingon the amount of time the seizure has been ongoing before a sufficientstimulus arrives. Thus, differences in the phase of the oscillatoryseizure activity at which the stimuli occur or the threshold usedfor seizure detection may affect the efficacy of the stimulation.These mechanisms could explain the variation in the amount oftime required to abort aseizure.

Another important mechanism-related issue is whether the trigeminal stimulation was merely able to stop seizure activity duringthe stimulation itself or whether it also had an effect on thenumber of seizures initiated. In control files where PTZ was administeredbut no stimulation was provided, the average time between theend of one spontaneously occurring seizure and the beginning ofthe next was 6.1 sec (calculated from the average number of seizuresand the average seizure duration, as reported in Results). Wealso measured the latency between the end of a period of stimulationand the next spontaneous seizure (i.e., in the epoch after a stimulus-onperiod), which was 7.59 ± 1.29 sec. Thus, the average delay betweenthe end of a period of stimulation and the first spontaneous seizureafter the stimulus ends is actually, on average, 24% longer thanthe interseizure interval during control files with no stimulationpresent. These results are supported by results from other laboratories(Zabara, 1992; Takaya et al., 1996) showing that the seizure reductioneffect of vagus nerve stimulation can outlast the stimulusduration.

Bilateral versus unilateral IO nerve stimulation

The fact that bilateral stimulation can be more effective than unilateral stimulation in the middle of the therapeutic-currentrange has implications for how such stimulation could be usedto most effectively reduce seizure activity. Specifically, becausebilateral stimulation at 7 mA was just as effective as unilateralstimulation at 11 mA (Fig. 5), the use of bilateral nerve cuffelectrodes would reduce the amount of current delivered to eachnerve, while still maintaining the same seizure reduction effectas higher stimulation current at a single site. This would bebeneficial because it would reduce the potential for damage tonerve fibers at the stimulation site (Agnew et al., 1989; Agnewand McCreery, 1990), and it would reduce the intensity of anypossible side effects associated with the stimulation. Bilateralstimulation is a further improvement over VNS, because the vagusnerve cannot be safely stimulated bilaterally without substantialrisk of cardiovascular side effects (Schachter and Saper, 1998).

It is important to point out that our finding that bilateral stimulation of the IO nerve was more effective than unilateralstimulation is in contrast to two previous studies reporting thatbilateral stimulation of the vagus nerve was no more effectivethan unilateral stimulation (Chase et al., 1966; Zabara, 1992).This discrepancy is likely either caused by differences in fibercomposition between the vagus nerve and the IO nerve or causedby the fact that the stimulus parameters used in those studieswere beyond those for which bilateral stimulation is superiorto unilateral stimulation. Details about the stimulus parametersused for assessing the efficacy of bilateral stimulation in thosetwo studies were notprovided.

Another important point to consider is that we have tested the effect of bilateral stimulation with the PTZ seizure model,which involves generalized, tonic-clonic seizures (Fisher, 1989).Further testing with focal seizure models such as localized applicationof alumina gel (Lockard et al., 1990) or penicillin (McLachlan,1993) to the cortex will be necessary to determine whether thereis an advantage to bilateral stimulation in eliminating thesetypes of seizures as well. Evidence to support an advantage inusing bilateral stimulation to treat focal seizures is that, inour study, unilateral stimulation eliminated seizure activityin both hemispheres at the same time, suggesting that the effectof the stimulation is not restricted to one hemisphere. Such resultshave also been found for VNS in cats (Chase et al., 1966), dogs(Zabara, 1992), and humans (Henry et al., 1998, 1999). These resultssuggest that because each nerve being stimulated can reduce seizuresbilaterally, the effect of stimulating both nerves could be additivewithin a givenhemisphere.

A brain-device interface for automatic, real-time detection and reduction of seizure activity

This study showed that triggering trigeminal nerve stimulation only when a seizure began is a much more effective method forreducing seizure activity than is providing stimulation on a fixedduty cycle, as has been used in past studies. This finding isan important advancement in the use of cranial nerve stimulationtherapies in epilepsy for severalreasons.

First, stimulating only when seizure activity occurs would, for many patients, reduce the overall amount of stimulation requiredfor maintaining seizure control. Thus, the amount of potentiallyunnecessary stimulation usually occurring between seizure periodswould be reduced, decreasing the possibility of damage to thenerve (Agnew et al., 1989; Agnew and McCreery, 1990; Ramsay etal., 1994). It is important to note, however, that several researchershave demonstrated a prophylactic effect of vagus nerve stimulationsuch that after stimulation, seizures are less likely for a periodof time related to the duration of the preceding stimulation (Zabara,1992; Takaya et al., 1996). This implies that perhaps the bestoverall treatment stimulation protocol might involve the use ofseizure-triggered stimulation combined with intermittent prophylacticnonseizure-triggeredstimulation.

The second advantage of this technique is that it would reduce the side effects experienced by patients when the stimulusis on. For example, patients undergoing VNS treatment report hoarseness,coughing, and throat pain as the most common side effects of thestimulation (Ramsay et al., 1994; McLachlan, 1997; Schachter andSaper, 1998). These side effects are generally only experiencedwhen the stimulation is on. However, if stimulation were onlypresented in response to the detection of seizure activity (oroccasionally prophylactically, as described above), these sideeffects would be experienced as infrequently aspossible.

In the future, the type of real-time, automatic seizure detector described here could be implemented in humans by buildingon and combining a number of existing technologies. First, seizuredetection could be performed by a computer microchip programmedwith a seizure detection algorithm and carried by the patient,similar to the Holter monitors used for continuous EKG monitoring.Input would be delivered to this microchip from multiple scalpEEG electrodes that would be able to pick up and amplify extracranialEEG signals. Finally, when the microchip detected seizure activityin the EEG signals, it would trigger an implanted stimulator similarto those used in the VNS technique (Terry et al., 1990), whichwould stimulate one or more trigeminal nerve cuff electrodes.This device would function in a manner analogous to cardiac pacemakers,commonly used to treat heart arrhythmia, and would require a minimumof invasive procedures. In essence, this device would constitutea "brain pacemaker" for seizure monitoring andcontrol.

The application of nonlinear computational methods for detection of seizure activity (Gabor et al., 1996; Webber et al., 1996)could be extremely beneficial if incorporated into the seizuredetector described here. Such seizure detection algorithms wouldallow for more accurate identification of seizure activity thanthe rather simple amplitude-based algorithm we used in thisstudy.

Another substantial advance could be in the implementation of seizure prediction algorithms that can identify seizures secondsor minutes before the behavioral onset (Martinerie et al., 1998;Le Van Quyen et al., 1999). There is evidence that the soonerstimulation is provided after a seizure begins, the more effectivelythe seizure can be stopped (Uthman et al., 1993); also stimulationis more likely to prevent seizure activity if it is presentedbefore rather than after a seizure has begun (Woodbury and Woodbury,1990). Therefore, it is possible that providing stimulation beforethe clinically defined onset of a seizure may prevent seizuresbefore they begin or become behaviorally relevant to the patient.Such a technique could dramatically improve the efficacy of thecranial nerve stimulationtherapy.

Application to human patients

Further studies in other animals and with other seizure models will be needed to determine whether it is appropriate to applythe techniques described here to human patients and what the bestmethods for doing so wouldbe.

The results presented here apply to seizures caused by systemic administration of PTZ, which is a model of acute, generalized,tonic-clonic seizures. It will be important to determine whetherthe results also apply to chronic seizure models, as well as toother seizure types, such as focal seizures (e.g., temporal lobeseizures) and absence seizures, if the described techniques areto be applicable tohumans.

Because the cellular mechanisms involved in different seizure types may not necessarily be similar, it is vital to ask whetherthe seizure reduction effects from trigeminal nerve stimulationwould apply to different seizure types. If the effects of trigeminalnerve stimulation are spatially restricted or only affect certaintypes of cellular excitation or inhibition, then this techniquemay be of limited use in treating multiple seizure types. If,however, as proposed in the current paper, the mechanism by whichtrigeminal nerve stimulation reduces seizure activity is, indeed,a generalized, widespread effect on cortical arousal level, perhapsmediated by the brainstem reticular-activating system, it is possiblethat this technique would be useful in treating a wide range ofseizures. In support of this view, the VNS technique has provento be effective in multiple seizure models including intraperitonealinjection of PTZ (Zabara, 1985, 1992; Woodbury and Woodbury, 1990),intraperitoneal injection of 3-mercaptopropionate (Woodbury andWoodbury, 1990), maximal electroshock (Woodbury and Woodbury,1990), topical application of penicillin to the cortex (McLachlan,1993), and chronic local application of alumina gel (Lockard etal., 1990).

Another issue that will need to be addressed before this technique is applied to humans is that because the trigeminal nerveis involved in transmitting both somatosensory and pain informationfrom the head, it is vital that the level of stimulation be belowthat that might cause discomfort such as facial pain or headaches.It is not known what stimulus parameters would be required toachieve seizure reduction without resulting in painful sensationssuch as these. However, such side effects could be substantiallyreduced by using the lowest effective stimulus parameters, whichwould be aided by the use of bilateralstimulation.

Finally, it would also be possible to develop an effective therapy by combining the VNS technique, which is currently in usein human patients, with the automatic seizure detection techniquedescribed in thispaper.

Conclusions

The results described in this study could serve to substantially increase the efficacy of cranial nerve stimulation as a techniquefor reducing or eliminating seizures in patients who suffer fromintractable epilepsy. Further development and testing of trigeminalnerve stimulation for patients with epilepsy is justified on thebasis of the results presented here. In addition, our findingssuggest that in the future, it will be feasible to develop a completelyimplantable and relatively noninvasive brain-device interfacecapable of automatically detecting seizure activity and triggeringstimulation of cranial nerves to safely and efficiently reduceseizureactivity.

  FOOTNOTES

Received May 19, 2000; revised Aug. 7, 2000; accepted Aug. 11, 2000.

This work was funded by a grant from the Klingenstein Foundation to M.A.L.N. and by National Institute of Dental ResearchGrant DE-11121-01 to M.A.L.N. We thank Dr. James O. McNamara forhelpful comments on thismanuscript.
Correspondence should be addressed to Erika E. Fanselow, Department of Neurobiology, Duke University Medical Center, Durham,NC 27710. E-mail: efanse{at}neuro.duke.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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