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The Journal of Neuroscience, November 19, 2008, 28(47):12284-12293; doi:10.1523/JNEUROSCI.1952-08.2008
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Development/Plasticity/Repair
Excitation and Inhibition Jointly Regulate Cortical Reorganization in Adult Rats
Alia Benali,1 Elke Weiler,1 Youssef Benali,3 Hubert R. Dinse,2 andUlf T. Eysel1 1Medical Faculty, Institute of Physiology, Department of Neurophysiology, and 2Institute for Neuroinformatic, Theoretical Biology, Neural Plasticity Laboratory, Ruhr University Bochum, D-44780 Bochum, Germany, and 3Department of Traumatology, Staedtische Kliniken, D-44137 Dortmund, Germany
Abstract
Top
Abstract
Introduction
The primary somatosensory cortex (SI) retains its capability for cortical reorganization after injury or differential use into adulthood. The plastic response of SI cells to peripheral stimulation is characterized by extension of cortical representations accompanied by changes of the receptive field size of neurons. We used intracortical microstimulation that is known to enforce local, intracortical synchronous activity, to induce cortical reorganization and applied immunohistochemical methods in the same individual animals to investigate how plasticity in the cortical topographic maps is linked to changes in the spatial layout of the inhibitory and excitatory neurotransmitter systems. The results reveal a differential spatiotemporal pattern of upregulation and downregulation of specific factors for an excitatory (glutamatergic) and an inhibitory (GABAergic) system, associated with changes of receptive field size and reorganization of the somatotopic map in the rat SI. Predominantly local mechanisms are the specific reduction of the calcium-binding protein parvalbumin in inhibitory neurons and the low expression of the activity marker c-Fos. Reorganization in the hindpaw representation and in the adjacent SI cortical areas (motor cortex and parietal cortex) is accompanied by a major increase of the excitatory transmitter glutamate and c-Fos. The spatial extent of the reorganization appears to be limited by an increase of glutamic acid decarboxylase and the inhibitory transmitter GABA. The local and medium-range net effects are excitatory and can facilitate receptive field enlargements and cortical map expansion. The longer-range increase of inhibition appears suited to limit these effects and to prevent neurons from pathological hyperexcitability.
Key words: plasticity; somatosensory system; receptive field; GABA; glutamate; parvalbumin
Introduction
The primary somatosensory cortex (SI) is a popular model for studies of cortical plasticity in rats. A number of different experimental manipulations, such as sensory deprivation, lesions, training, or intracortical microstimulation (ICMS), have been used to alter the cortical map or the size, position, shape, and sensitivity of receptive fields (RFs) (Merzenich et al., 1984; Recanzone et al., 1992
Based on theoretical and experimental work, it has been suggested that the maintenance of cortical maps and RFs arises from a meticulous balance of both local and global mechanisms based on feedforward and recurrent inputs (Stratford et al., 1996
Experimental work on a timescale of days to weeks reveals that cortical map expansion and RF sharpening/contraction induced by the repetitive cutaneous stimulation during nursing is associated with changes in the inhibitory and excitatory system (Rosselet et al., 2006
Previous work revealed, after eye removal, TTX injection, and monocular deprivation, a decrease in the neuronal activity that induced a decrease in the neuronal GABA and GAD expression after 4 and 5 d (Hendry and Jones, 1986
Changes in cortical maps and RF sizes after dorsal rhizotomy or unloading the hindlimb for 14 d were accompanied only by a reduction of inhibition (D'Amelio et al., 1996
Very fast changes in RF properties have been observed after direct pharmacological disruption of inhibition. A number of studies in SI have shown that blockade of GABAA receptors by iontophoretic application of GABA antagonists leads to rapid expansion of the RFs of most neurons (Hicks and Dykes, 1983
The first goal of the present study was to induce cortical plasticity by ICMS in SI and to investigate the time course and reversibility of changes in neuronal RF properties. The second goal was to study the spatiotemporal pattern of changes in the GABAergic and glutamatergic systems at the stimulation site and in the surrounding cortical areas.
Materials and Methods
Animals and experimental procedures. Briefly, a total of 62 adult Sprague Dawley rats (male, 300–400 g) were anesthetized by intraperitoneal injection of urethane (1.5 g/kg body weight) and kept under a constant level of anesthesia by monitoring forepaw withdrawal, corneal reflex, and respiratory rate, and, if necessary, an extra dose (10% of original dose) was administrated. Body temperature was monitored and maintained between 37 and 37.5°C.Experimental procedures were similar to those used previously (Recanzone et al., 1992
In the second (43 rats, stimulated animals) and third (six rats, sham animals) series of animals, a surgical procedure was developed to minimize possible structural artifacts induced by the craniotomy. After abrading the skull to a thin layer, local field potentials were recorded from the skull after electrical stimulation of the middle toe to localize the toe representation in the left or right somatosensory cortex (0.5 Hz, 1 min, 20–50 µA). At the location of the maximum local field potential, a small hole (0.1 ± 0.05 mm2) was carefully drilled above each hemisphere. Through this aperture, a glass microelectrode (3 M sodium acetate; 1–2 M
) was inserted, and action potentials were extracellularly recorded in layer IV in depths of 600–800 µm. For tactile stimulation, an electrically driven stimulator (Bruel & Kjaer) was used to apply computer-controlled tactile stimuli of 8 ms duration (1 Hz). The receptive field mapping was performed as described by Recanzone et al. (1992)
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Figure 1. Experimental procedure. a, The ratunculus with the hindpaw representation and the recording sites (dots) with a representative receptive field. An enlargement of the rectangle in illustration a is represented in b. It shows the place of the hindpaw representation in the map, which was electrically stimulated. c, For the investigation of the immunolabeled cells, at least nine coronal sections in a rostrocaudal extent of 2 mm with intervals of 250 µm between the sections were analyzed for each marker. Each coronal section was divided into sampling areas (five on each hemisphere) with a dorsoventral extent from the pia mater to the white matter and with a mediolateral extent of 500 µm in layer IV. HP, Hindpaw; UZ, unresponsive zone; FP, forepaw; Barrel, barrel cortex; T, tail.
Intracortical microstimulation. To induce plasticity in the somatosensory cortex, we applied intracortical microstimulation in the cortical layer IV. This method has been successfully used in studies of rapid plastic changes inducible within a few hours, in adult motor, somatosensory, and auditory cortex and thalamus, which were fully reversible (Nudo et al., 1990ICMS was applied for 2 h in one hemisphere (ICMS side). The ICMS side was stimulated via the microelectrode with charged balanced repetitive pulse trains of 40 ms duration (13 pulses, 0.2 ms duration at 300 Hz, 6 µA) for 2 h at a repetition rate of 1/s (supplemental Fig. 2, available at www.jneurosci.org as supplemental material). To exclude possible lateralization differences between the hemispheres, the ICMS was randomly applied in individual animals to the left or the right hemisphere. The sham-operated group (n = 6) received the same surgery as the ICMS-treated animals, including the insertion of a glass microelectrode (3 M sodium acetate) into each hemisphere but without electrical stimulation.
Microcoagulation. At the end of each experiment, two microcoagulations were induced anteriorly and posteriorly to the somatosensory cortex to find the electrode tracks of the control electrode and ICMS electrode in the stained sections of the cortex (supplemental Fig. 1a, available at www.jneurosci.org as supplemental material). The microcoagulation was induced through the stimulation/control electrode with direct current of 20 µA for 5 min. A Masson's trichrome staining (see below) of every tenth section allowed us to find the microcoagulations and the electrode tracks (supplemental Fig. 1b,c, available at www.jneurosci.org as supplemental material). Based on the coordinates of the three landmarks (two microcoagulations plus ICMS/control electrode position), selection of the sections and positioning of the sampling areas were possible. The position of the stimulation/control electrode was in most cases at 2.5 ± 0.5 mm lateral of the fissura longitudinalis cerebri (measured in layer IV). If the electrodes were outside this area, the animals were not included in the study. The sampling areas were aligned according to the position of the ICMS electrode.
Reversibility of the ICMS-induced plasticity. To examine the reversibility of the ICMS-induced plasticity, the animals were kept under anesthesia after the stimulation. During the recovery periods of 2, 5, 7, and 10 h (Table 1), the RFs were determined in 15–30 min intervals. After the different survival times, the animals were perfused and their brains were treated like those of the acute animals.
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Table 1. Overview of the experimental groups and number of animals
Fixation and histochemistry. After ICMS and the different recovery periods, the rats were killed with an overdose of urethane, and their brains were fixed by intracardial perfusion with 0.9% NaCl, followed by 4% paraformaldehyde in 0.1 M phosphate buffer, pH 7.4. The brains were postfixed for 4 h at 4°C in the same fixative.After postfixation, the brains were either prepared for embedding in paraffin or cryoprotected in sucrose (30% in PBS). For paraffin embedding, tissue was dehydrated through graded alcohols and xylene and embedded in paraffin. Serial sections of 5 µm were cut coronally, and every 10th section was placed on gelatin-coated slides, dewaxed in xylene, transferred through a descending ethanol series into PBS, and then stained with cresyl violet (a Nissl stain) for cytoarchitectural control and a Masson's trichrome stain for microcoagulation and electrode reconstruction (Carson, 1990
Frozen sections of 30 µm were cut with a freezing microtome. The sections were rinsed in PBS, and every 10th section was stained with cresyl violet.
Immunohistochemistry. Consecutive serial sections (interval of 100 µm for paraffin sections or 300 µm for frozen sections) adjacent to Nissl-stained sections (first series) were treated immunohistochemically with antibody against glutamate (second series; 1:4000; Sigma), GABA (third series; 1:4000; Sigma), GAD (fourth series; 1:500; DakoCytomation), parvalbumin (PV) (fifth series; 1:1000; clone PA-235; Swant), calbindin D28K(CB) (sixth series; 1:250; Swant), calretinin (CR) (seventh series; 1:1000; Swant), and c-Fos (eighth series; 1:3000; Dianova). The sections were blocked with normal goat or normal horse serum [1:100 in PBS, 1 h, room temperature (RT); Vector Laboratories] and incubated with primary antibodies overnight at RT and then with the appropriate secondary antibody (Vectastain, 1:200 in PBS, 1.5 h, RT). Detection was performed with a standard ABC kit (Vectastain, 1:500, 1.5 h, RT). The immunostaining was visualized using the glucose oxidase–diaminobenzidine–nickel method (Shu et al., 1988
Data collections and data analysis. Data collection of immunolabeled neurons was performed manually (glutamate, c-Fos, CB, and CR) and automatically (GABA, GAD, PV, and Nissl) (Benali et al., 2003
To quantify the concentration of substances in the tissue, the optical density (OD) was measured by using the NIH Image system (version 1.61). According to Beer's law, the concentration is proportional to the optical density (Rees and Laurence, 1955
Data presentations. The spatial distribution of the cell numbers and ODs are presented as false-color-coded images in Figure 4. The x-axes of the distributions indicate the mediolateral position of the analyzed areas and the y-axes the rostrocaudal distance from the ICMS site (with ICMS set at zero). The color of each point encodes the local cell number or the local OD. The spatially continuous distributions were calculated by linear interpolation between the cell numbers (or optical density) of the ROIs that are discretely distributed. Data from the hemispheres of the ICMS or control animals are separate two-dimensional linear interpolations in the areas 0–4.5 mm lateral and –1 to 1 mm rostrocaudal from the stimulation or control electrode. By the interpolation, the values at the original measurement points were not changed. The implementation of the calculations were made with standard functions of Matlab version 6.0 (MathWorks).
Statistics. A nonparametric Mann–Whitney U-Test was used to determine whether there were differences in the number of cells and in the OD between the stimulated and the sham group. Quantitative differences between the hemispheres were assessed by a nonparametric paired Wilcoxon's test or by a parametric paired Student's t test. The results are given as the mean ± SD. A p value of <0.05 was considered significant.
Results
ICMS-induced enlargement of cortical and peripheral representations
Cortical representation
To verify that our application of microstimulation induced the plasticity effects that have been described previously (Recanzone et al., 1992
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Figure 2. Somatosensory mapping of the hindpaw representation before (a) and after (b) ICMS. L, Lateral; C, caudal. Dots indicate recording sites with the appending receptive field (indicated by the arrow). Bars show recording sites, which are unresponsive to tactile stimulation. Asterisks mark newly accrued receptive fields after ICMS (b). Receptive field size from both hemispheres of control (sham) and stimulated animals (c). Time course of receptive field changes before (pre ICMS) and after 2 h of electrical stimulation (post ICMS) over an interval of 10 h after stimulation compared with preconditions (d). *p < 0.05.
Peripheral representation (receptive field) of the ICMS site
To minimize possible structural artifacts induced by the treatments (see above, Animals and experimental procedures), only a small craniotomy was performed for inserting the electrode. ICMS was applied to a single site of the cortical representation of toe 3. In sham-operated animals (n = 6), the average RF size at the tip of toe 3 (Figs. 1a, 2c) was 27.53 ± 11.45 mm2 in the right hemisphere and 30.74 ± 10.14 mm2 in the left hemisphere (p > 0.05, paired t test) (Fig. 2c). In the ICMS-treated animals (n = 39), the mean value of the RF size before stimulation was 39.39 ± 29.22 mm2 for the ICMS side and 56.59 ± 45.33 mm2 for the contralateral side (p > 0.05, paired t test) (Fig. 2c). After stimulation, we found a significant increase of the RF sizes on the stimulated side (221.73 ± 73.35 mm2; paired t test, p < 0.005) (Fig. 2c). The maximum increase was present for 45 min from 15 min up to 1 h after stimulation (Fig. 2d). Afterward, the RF sizes began to decrease. However, even 2–5 h after stimulation, the RF sizes were still significantly increased (t test, p < 0.001) (Fig. 2d) and returned to normal values between 5 and 10 h after stimulation offset (Fig. 2d). On the contralateral side, the RF size did not change (60.23 ± 48.41 mm2; paired t test, p = 0.81) (Fig. 2c).To investigate the underlying mechanisms of the functional changes after stimulation (RF enlargement and increase of the cortical representation), brain tissue from stimulated and sham-operated animals was evaluated with Nissl stain (we counted in the ROI the number of cells to get an overview about the total number of cortical cells and to rule out cell loss as a possible reason for changes in protein expression) and immunohistochemical markers indicative for neuronal activity and the state of the glutamatergic and GABAergic transmitter systems (Bradford, 1995
Mapping the neuronal activity by c-Fos
First we tested whether the RF enlargement at the ICMS site and the increase of the cortical map was induced by an increase of the neuronal activity. The metabolic marker c-Fos, an immediate early gene known for its powerful indication of cellular/metabolic activity, was used for mapping the neuronal activity (Morgan et al., 1987
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Figure 3. Histological changes after 2 h of ICMS compared with the contralateral side. a, b, Changes at the stimulation site in c-Fos and in PV. A dark arrow indicates the electrode track. c, Increase of the excitatory system (glutamate) after 2 h of ICMS 1 mm lateral the ICMS electrode. The small right top image shows a magnification of stained pyramidal cell. d, e, Enhancement of inhibitory system after 2 h of ICMS in GABA and GAD 500 µm rostral the ICMS electrode. In the small windows of the GAD images at a higher magnification, a nonlabeled pyramidal cell is shown, which is surrounded by labeled GAD puncta. (For magnification, see scale bar in a).
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Figure 4. Summary of the changes after 2 h of ICMS are shown in first two columns. a, b, d, e, g, h, j, k, Color-coded representations of the histological changes after ICMS. The statistical differences are marked by * (significance level of 1%) or x (significance level of 5%). Arrows indicate the location of the electrodes during ICMS or without ICMS. Note that, in controls (sham), c-Fos-IR cells are below threshold for color coding (Tables 2
Mapping of the inhibitory and excitatory systems at the stimulation site
After we revealed that, after ICMS, the RF size increase at the stimulation site is not correlated with an increase of the metabolic activity (low c-Fos labeling) and the RF size increase in the surround correlates with an increased metabolic neural activity (high c-Fos labeling), we wanted to get more insight into the possible underlying mechanisms of these different RF size enlargements. A possible assumption is that an expression of high inhibition/low excitation at the stimulation site and high excitation/low inhibition in the surround is induced by shifts in transmitter balance. Therefore, we analyzed the expression of the neurotransmitters for the excitatory (glutamate) and inhibitory (GABA plus GAD) systems.Although we had the highest receptive field enlargement at the stimulation site, we did not find differences in either transmitter system compared with controls. Neither the number of immunoreactive (IR) cells nor the OD of the labeling for glutamate and for GABA were significantly changed in this region (Table 2) (see Table 5). Furthermore, the expression of the GABA-synthesis enzyme GAD was not significantly different between the control animals and the stimulated animals at the stimulation site, but there were indications for a specific downregulation of the GABAergic system based on the expression of the calcium-binding proteins.
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Table 2. Summary of the number of IR cells in the suppression zone immediately after the ICMS (Fig. 4)
Mapping the expression of calcium-binding proteins at the stimulation site
Several types of GABAergic neurons can be differentiated by their expression of the calcium-binding proteins (CaBPs) PV, CB, and CR. Each of these three CaBPs is mostly colocalized with GABA in distinct subpopulations of nonpyramidal cells (Hendry et al., 1989
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Table 3. Summary of the number of IR cells in the excitation zone immediately after the ICMS (Fig. 4)
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Table 4. Summary of the number of IR cells in the inhibition zone immediately after the ICMS (Fig. 4)
Mapping excitatory neurotransmitter system outside the stimulation site
Adjacent to the SZ, the OD of glutamate staining was significantly enhanced 250 µm caudal to the stimulation site in an area extending from the fissura longitudinalis cerebri up to 4 mm toward lateral. This area includes the motor cortex, the hindlimb region, forelimb region, and the dysgranular region of S1.The number of glutamate-IR cells was significantly increased 250 µm rostral to the stimulation site in the hindpaw and forepaw region and 750 µm anterior to the stimulation site in the motor cortex (Fig. 4d). Also, an increase in the number of cells expressing glutamate occurred 1 mm lateral to the stimulation site in the forepaw representation in an area of 1.250 mm anteroposterior extent (Fig. 4d). At 1 mm posterior to the stimulation site, an increase of the number cells expressing glutamate was observed in the motor cortex and the somatosensory hindlimb and dysgranular region of S1 (see Fig. 6b), which are highly interconnected (Hoover et al., 2003
This zone, which is characterized by positive changes in the excitatory transmitter system, will be further called excitation zone (EZ). Within the EZ, for example in the hindpaw representation, the electrophysiological recordings revealed an enlargement of the cortical area and increased RFs (Fig. 2) that lasted up to 5 h. The glutamate staining observed at different time points (2, 5, 7, and 10 h after stimulation) showed a similar time course and lasted up to 5 h after stimulation (Fig. 5a).
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Figure 5. Optical density of glutamate (a), GABA (b), and GAD (c) at different time points after ICMS from the different zones (Fig. 4c,f,l). For comparison, see time course of changes in RF size (Fig. 2d). Because the OD of the immunoreactivity of animals differ, the data were standardized, to compare among animals. The OD of each individual measure was divided by the average value of all stained sections from the same animal and same marker. IZ, Inhibition zone.
In parts of the EZ, an upregulation of the inhibitory system was found as well (Figs. 4g,j, 6b).
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Figure 6. Cortical topography surrounding the ratunculus in primary somatosensory cortex (a). VC, Visual cortex; fl, forelimb; hl, hindlimb; SI, primary somatosensory cortex; MC, motor cortex; cg, cingulate cortex; OB, bulbus olfactorius; RAG, retrosplenial cortex; TE, temporal cortex; CR, cerebral cortex; SII, secondary somatosensory cortex; Ins, insular cortex; PIR, piriform cortex. Classification of the zones attributable to the specific changes of the transmitters and proteins immediately after two hours of ICMS and overlay these to the cortical representation (b). FP, Forepaw; HP, hindpaw; IZ, inhibition zone; UZ, unresponsive zone.
Mapping the inhibitory neurotransmitter system outside the stimulation site
The changes in the inhibitory transmitter system displayed a different spatial distribution compared with the excitatory system (Figs. 4f,i–l, 6b).The OD of the GABA and GAD staining was significantly changed outside the EZ (Fig. 4h,k; Table 5). The OD of GAD staining was increased 500 µm caudal/3.5 mm lateral of the stimulation site and 750 µm rostral extending from the fissura longitudinalis cerebri up to 1.5 mm lateral (Fig. 4k). The OD of the transmitter GABA was increased medial to the stimulation site in the agranular frontal cortex (Fig. 4h) and extended into the contralateral side (data not shown).
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Table 5. Summary of the optical density in the three zones for GABA, GAD, and glutamate immediately after the ICMS (Fig. 4)
Significant changes in the number of GABA- and GAD-immunoreactive cells in the ROI are located 750 µm caudal and 500 µm rostral to the stimulation site (Fig. 4g,j). Caudal, the number of IR cells was increased for GABA at 3.5 mm lateral and for GAD from 1.5 up to 2.5 mm lateral to the fissura longitudinalis cerebri. Rostral, the number of GABA-IR cells was increased from 2.5 up to 4.5 mm lateral to the fissura longitudinalis cerebri, and the number of GAD-IR cells was increased at 2.5 mm lateral. In addition, GABA-IR cells are significantly increased 1000 µm rostral and 0.5, 1.5, and 3.5 mm lateral. In summary, the upregulation of GABA and GAD seems to represent an inhibitory surround that could functionally limit the increase of glutamatergic excitation (Fig. 6b). This zone, which is characterized by positive changes in the inhibitory transmitter system, will be further called inhibition zone (Fig. 4l).
Discussion
Our histological and electrophysiological results indicate that cortical reorganization and RF enlargement after ICMS are characterized by a specific spatiotemporal pattern of changes in transmitter systems and proteins. In the SZ, which was located immediately around the stimulation site, we found no changes of the transmitter systems and a moderate increase of the neural activity (c-Fos) but a reduction of the calcium-binding protein parvalbumin. A second asymmetric zone surrounded the SZ. In this zone (excitation zone), we found an increase of the excitatory transmitter glutamate and an increase of the neural activity (c-Fos). A third zone (inhibition zone) with an upregulation of the GABAergic inhibitory system (GABA and GAD) and the neural activity (c-Fos) seems to enclose the preceding zones.Suppression zone
The immunohistochemistry of the calcium-binding protein parvalbumin showed a decrease of IR cells at the stimulation site after ICMS. A decline of parvalbumin is also observed after epileptic seizure (Kamphuis et al., 1989We assume that the decrease of parvalbumin is dependent on the electrophysiological properties (fast-spiking vs regular firing) of the cells that are involved in synchronizing the neuronal activity (McBain and Fisahn, 2001
Differences between the CaBP-containing neurons exist in their cortical distribution and their morphology (Markram et al., 2004
The chandelier neurons can be multipolar or bitufted and are targeting the initial axon segment in which they can control the generation of action potentials (Zhu et al., 2004
ICMS has been shown to produce a small RF enlargement already after 30 min of stimulation and RF size additional increases with longer application time (Dinse et al., 1993
ICMS seems to "reset" the excitatory and inhibitory balance and to induce a state as found in the precritical period during development (Morishita and Hensch, 2008
Excitation zone
Direct synaptic projections are supposed to activate neurons within a range of 125–600 µm (Stoney et al., 1968After partial deafferentation of the hindlimb, granular cortex of the rat by nerve transection neurons in the cortical hindlimb area were more readily depolarized by glutamate (Lamour and Dykes, 1988
Inhibition zone
The third and outermost zone induced by ICMS in the somatosensory cortex was characterized by an increase of markers for the GABAergic system. The increased activity of the inhibitory system in the inhibition zone probably represents a compensatory reaction to the increased activity in the EZ. It could serve to prevent a propagation of the excitation over the whole cortex as seen during epileptic seizures (Prince and Wilder, 1967
Footnotes
Received Sept. 8, 2008; accepted Oct. 4, 2008.This work was supported by Deutsche Forschungsgemeinschaft (DFG) Grant Sonderforschungsbereich (SFB) 509 TP C4 (U.T.E.), FORUM F108/00 M122/13 (E.W.), and DFG Grant SFB 509 TP C5 (H.R.D.). We thank Dr. M. A. Giese for his comments on this manuscript and help with the statistical and data analysis, and Ute Neubacher and Gabriele Bomholt for their technical help.
Correspondence should be addressed to Dr. Alia Benali, Medical Faculty, Institute of Physiology, Department of Neurophysiology, Ruhr University Bochum, D-44780 Bochum, Germany. Email: alia.benali{at}rub.de
Copyright © 2008 Society for Neuroscience 0270-6474/08/2812284-10$15.00/0
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