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The Journal of Neuroscience, April 29, 2009, 29(17):5701-5709; doi:10.1523/JNEUROSCI.0247-09.2009
Behavioral/Systems/Cognitive
Short-Latency Visual Input to the Subthalamic Nucleus Is Provided by the Midbrain Superior Colliculus
Véronique Coizet,1,2 John H. Graham,3 Jonathan Moss,4 J. Paul Bolam,4 Marc Savasta,2 John G. McHaffie,5 Peter Redgrave,1 andPaul G. Overton1 1Department of Psychology, University of Sheffield, Sheffield S10 2TP, United Kingdom, 2Inserm U836, Grenoble Institute of Neurosciences, Joseph Fourier University, Grenoble 38042, France, 3Department of Biology, King College, Bristol, Tennessee 37620, 4Medical Research Council Anatomical Neuropharmacology Unit, University of Oxford, Oxford OX1 3TH, United Kingdom, and 5Department of Neurobiology and Anatomy, Wake Forest University School of Medicine, Winston-Salem, North Carolina 27157
Abstract
Top
Abstract
Introduction
The subthalamic nucleus (STN) is one of the principal input nuclei of the basal ganglia. Using electrophysiological techniques in anesthetized rats, we show that the STN becomes responsive to visual stimuli at short latencies when local disinhibitory injections are made into the midbrain superior colliculus (SC), an important subcortical visual structure. Significantly, only injections into the lateral, but not medial, deep layers of the SC were effective. Corresponding disinhibition of primary visual cortex also was ineffective. Complementary anatomical analyses revealed a strong, regionally specific projection from the deep layers of the lateral SC to neurons in rostral and dorsal sectors of the STN. Given the retinocentric organization of the SC, these results suggest that lower-field stimuli represented in the lateral colliculus have a direct means of communicating with the basal ganglia via the STN that is not afforded to visual events occurring in the upper visual field.
Introduction
The subthalamic nucleus (STN) occupies a central position in the functional architecture of the basal ganglia (Parent and Hazrati, 1995; Joel and Weiner, 1997
Electrophysiological studies have revealed that the STN contains neurons whose activity is related to movement and others that respond to sensory stimuli (DeLong et al., 1985
Neurons in the STN exhibit short-latency (70–120 ms) responses to the onset of phasic visual stimuli (Matsumura et al., 1992
Materials and Methods
All aspects of this study were performed with Home Office approval under section 5(4) of the Animals (Scientific Procedures) Act 1986, and experimental protocols received prior approval of the Institutional Ethics Committees.Electrophysiology
Twenty-two male Hooded Lister rats (285–620 g) anesthetized with urethane (ethyl-carbamate, 1.25 g/kg, Sigma-Aldrich) were used in the electrophysiology experiments. A contralateral approach using an angle of 35° (ML: 2.5–3.2, bregma) was used to position a parylene-C-insulated tungsten microelectrode (1–2 M, A-M Systems) into the STN (AP: 3.6–4.1 mm, bregma; DV: 7.0–8.0 mm, dura). A second tungsten electrode coupled with a 30 gauge metal injector needle filled with the GABAA receptor antagonist bicuculline methiodide (40 ng per 400 nl of saline, Sigma-Aldrich) was introduced vertically into the SC (AP: 5.8–6.3 mm, bregma; ML: 1.0–2.5 mm, bregma; DV: 3.5–5.0 mm, dura). Lateral separation between the electrode and the injector was 0.2–0.5 mm. Intracollicular injections of bicuculline (0.5 µl; 0.5 µl/min) were made with a 10 µl Hamilton syringe (Scientific Laboratory Supplies) mounted on an infusion pump, connected to the needle by a length of plastic tubing. The experimental rationale in the present study was based on the important observation of Katsuta and Isa (2003)
Multiunit spike-related potentials from the STN and SC were amplified, bandpass filtered (300 Hz to 10 kHz), digitized at 10 kHz, and recorded directly onto computer disc using a 1401+ hardware acquisition system (Cambridge Electronic Design) connected to a standard PC running CED Spike 2 software. Multiunit electrophysiological responses in the SC were used to guide the position of the SC electrode. Recordings were made while the electrode/injector assembly was lowered into the SC in the presence of a whole-field light flash (0.5 Hz, 10 ms duration) from a green LED (60 lux 570 nm) positioned 5 mm in front of the contralateral eye. Using the characteristically vigorous visual response of the SC superficial layers as a guide to position, the electrode was lowered into the subjacent intermediate layers of the medial or lateral sectors of the SC. When both the STN and SC electrodes were in place, sets of trials comprising 120 light flashes (parameters as above) were recorded. Responses were obtained during an initial baseline period before an SC injection of bicuculline. Sets of trials then were continued until the effect of the drug had worn off, typically 15–20 min.
In three cases, an insulated silver wire was inserted into the visual cortex (with the dura carefully retracted) to record visually evoked field potentials. These were low-pass filtered (DC-1 kHz, 3 dB points), digitized at 10 kHz, and recorded directly to disk using the 1401+ acquisition system. Signal averaging over sets of 300 light flashes was performed by the Spike 2 software. After recording under baseline conditions, a Gelfoam swab soaked in a solution of bicuculline (100 µg/ml) was placed directly on the surface of the exposed cortex. Averaged field potentials were recorded for successive series of 300 flashes until the effect of the drug had worn off.
At the end of the experiments, the position of any subcortical recording sites was marked with a small lesion induced by passing a 10 µA anodal current for 2.5 min through the tungsten recording electrode. Animals then were killed by an overdose of pentobarbitone and perfused with 0.9% saline followed by 4% paraformaldehyde. The brains were taken for histological analysis.
Following the experiments, peristimulus time interval histograms (PSTHs) were constructed based on SC and STN multiunit data (bin width 1 ms). PSTHs were imported into an Excel program (Microsoft) (Peter Furness, Sheffield) which determined the following response characteristics before and after an injection of bicuculline: (1) baseline activity: the mean number of multiunit spikes occurring during the 500 1 ms bins before the light flash; (2) response latency: the time point at which poststimulation spikes exceeded 3.0 SD of the baseline mean; (3) response duration: response offset was defined as the time point at which poststimulation activity returned to 3.0 SD of the baseline mean; and (4) response amplitude: the mean number of multiunit spikes between response onset and offset minus the baseline mean. The statistical reliability of differences between response latencies for the SC and STN, and between STN baseline firing rates before and after SC injections of bicuculline, were assessed by t tests. Probabilities <0.05 (two tailed) were accepted as statistically reliable.
Anatomy
Tracer injections. For the light microscopy experiments, we used 15 male Hooded Lister rats (265–602 g) bred in the Sheffield laboratory. Animals were anesthetized with an intraperitoneal injection of a mixture of Ketaset (0.765 ml/kg) and Rompun (1.1 ml/kg). Single injections of the anterograde tracers biotinylated dextran amine (BDA: Sigma-Aldrich) and Phaseolus vulgaris leucoagglutinin (PHA-L: Vector Laboratories) were directed to different quadrants of the SC on opposite sides of the brain in the same subject (e.g., caudomedial and rostrolateral or caudolateral and rostromedial). The stereotaxic coordinates were as follows: AP: 6.0–7.3 mm, bregma; ML: 0.5–2.5 mm, bregma; DV: 3.5–5.0 mm, dura). Some injections of anterograde tracers were combined with an injection of the retrograde tracer Fluorogold (Fluorochrome) into the substantia nigra pars reticulata (AP: 5.0–5.8 mm, bregma; ML: 1.0–3.0 mm, bregma; DV: 8.0–9.0 mm, dura) to help identify the STN. BDA (10% in phosphate buffer; PB) and Fluorogold (4.0% in distilled water) were pressure ejected in volumes of 30–90 nl, while PHA-L was ejected iontophoretically (5 µA anodal current applied to a 2.5% solution in PB, 7 s on/off for 15–20 min). To identify SC neurons projecting to the STN, small (6–10 nl) pressure ejections of the retrograde tracer cholera toxin subunit B (CTb; Quadratech Epsom; 1% solution in PB) or larger injections of the fluorescent tracer True Blue (Sigma-Aldrich) (5% in distilled water) were made into the STN. After allowing 7 d for the transport of tracers, animals were reanesthetized with pentobarbitone and perfused transcardially with warm saline (40°C) followed by 4% paraformaldehyde in PB, pH 7.4. Serial coronal or sagittal sections (30 µm) were cut on a freezing microtome and collected in PB, except for tissue containing True Blue, where the sections were collected directly onto slides, allowed to dry in a light protected box, and coverslipped with DPX mountant.For electron microscopy, an additional three rats received PHA-L injections as described above. Following 7 d survival, the animals were perfused with PBS (0.01 M phosphate) followed by 3% paraformaldehyde plus 0.1% glutaraldehyde. Sagittal sections (70 µm) were cut on a vibratome and collected in PB.
Histology for light microscopy. To reveal the tracers (BDA, PHA-L, CTb, or Fluorogold), free-floating sections were washed with 0.1 M PB followed by 0.1 M PB containing 0.3% Triton X-100 (PB-TX) for 30 min. For animals injected with PHA-L, CTb, or Fluorogold, the sections were incubated overnight in primary antibody solution (goat anti-PHA-L, 1:800–1,000 dilution, Vector Laboratories, or goat anti-CTb, 1:4000 dilution, Quadratech, or rabbit anti-Fluorogold, 1:50,000 dilution, Fluorochrome). The next day, sections were washed with PB-TX and incubated for 2 h in biotinylated rabbit anti-goat IgG (1:100, Vector Laboratories, in PB-TX containing 2% normal rabbit serum) for PHA-L and CTb or in biotinylated goat anti-rabbit IgG (1:100, Vector Laboratories, in PB-TX containing 2% normal goat serum) for Fluorogold. After 30 min washing, all the sections were incubated in Elite Vectastain ABC reagent (Vector Laboratories, 1:100 in PB-TX) for 2 h. The peroxidase associated with the tracers was revealed by reacting tissue with H2O2 for
1 min using nickel-enhanced diaminobenzidine (DAB) as the chromogen for BDA and CTb (black reaction product) while PHA-L and Fluorogold were revealed by incubation with VIP (Vector Laboratories) chromogen (purple reaction product). Finally, sections were washed in PB, mounted on gelatin-coated slides, dehydrated in graded dilutions of alcohol, cleared in xylene, and coverslipped in DPX.
Light microscopy, data analysis. Following injections of anterograde tracers into the SC, three coronal sections through the STN approximately equivalent to 3.6, 3.8, and 4.1 mm caudal to bregma in the atlas of Paxinos and Watson (1997)
The location of retrogradely labeled neurons was plotted on four coronal sections through the SC separated by
Electron microscopy, histology and analysis. Tissue for electron microscopic analysis was treated in a similar manner, except that the sections were freeze thawed using isopentane and liquid nitrogen, and Triton X-100 was not used. PHA-L was revealed using DAB as the chromogen for the peroxidase reactions (
Results
Electrophysiology
Visually evoked activation of the SC and STN
As expected, neurons in the SC deep layers (Fig. 1Aa,Ba) and the STN (Fig. 1Ac,Bc) failed to respond to the light flash during a baseline period before the SC injection of bicuculline. However, after local injections of bicuculline, both medial and lateral parts of the SC deep layers exhibited short-latency, short-duration bursts of impulses in response to the light flash (Fig. 1Ab,Bb). In contrast, a corresponding burst of spikes was recorded from STN neurons only when bicuculline was injected in lateral parts of the SC deep layers (Fig. 1Ad). This effect was observed in all cases (13/13). Corresponding injections of bicuculline into medial SC were, however, consistently ineffective (6/6), leaving STN neurons unresponsive to the light flash (Fig. 1Bd). Systematic variations in the STN recording sites cannot account for these differences because they were similarly dispersed throughout the structure for cases receiving medial or lateral SC injections (supplemental Fig. 1, available at www.jneurosci.org as supplemental material). As the visual sensitivity of the SC was reinstated, several patterns of visually evoked activity emerged in the STN: (1) a short-latency, short-duration phasic response (Fig. 2a); (2) a short-latency response with a slower build up and a longer duration (Fig. 2b); (3) a superimposition of response types 1 and 2 (Fig. 2c); and (4) a long-latency, long-duration response (Fig. 2d). No reliable relationships were established between the various response patterns and either the loci of recording sites in the STN or the precise location of bicuculline injections into the SC (supplemental Fig. 1, available at www.jneurosci.org as supplemental material). However, in all cases the STN visual response latencies (mean latency: 86 ± 9 ms) were reliably longer than those recorded in the SC (mean latency: 53 ± 5 ms) (t = 3.679; df = 12; p < 0.01). Considered together, these results suggest that the lateral SC is an important source of short-latency visual input to the STN.
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Figure 1. Effects of local intracollicular injections of bicuculline on visually evoked multiunit responses in the SC and STN. The graphs present raster displays and peristimulus histograms of single-case data aligned on the presentation of 120 light flashes (0.5 Hz) delivered to the contralateral eye (vertical dotted line). A represents data from a case where bicuculline was injected into the lateral deep layers. B is from a case where bicuculline was injected into medial SC. In both cases, before the injection of bicuculline, neither the SC (Aa, Ba) nor the STN (Ac, Bc) was responsive to the light flash. Following the injection of bicuculline into both lateral and medial SC, local neurons in the SC became responsive to the visual stimulus (Ab and Bb, respectively). In contrast, only when visual sensitivity was restored to the lateral SC did STN neurons become visually responsive (compare Ad with Bd).
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Figure 2. Peristimulus histograms showing individual cases of different types of short-latency visually evoked responses in the STN. The dashed vertical line indicates the onset time of the visual stimulus. The n associated with each histogram indicates the number of cases exhibiting that class of response; total n = 13. a, Short-latency (<70 ms), very-short-duration (10–15 ms) response. b, Short-latency (<70 ms), but slower-onset and longer-duration (
Effect of SC disinhibition on spontaneous activity in STN
General disinhibition of neural activity within the SC also induced a significant increase of the tonic firing rate of STN neurons measured in the 500 ms before each light flash. Thus, the mean prestimulus spike rate of STN multiunit activity increased from 26.62 ± 2.4 Hz to 45.17 ± 3.86 Hz following injections of bicuculline into the lateral SC (t = –4.19; df = 12; p < 0.01). In contrast, no comparable changes were found in the baseline firing rate of STN neurons following corresponding injections into the medial SC (mean number of multiunit spikes recorded before and after bicuculline were 27.24 ± 1.7 Hz and 35.00 ± 2.6 Hz, respectively; t = –2.3; df = 5; p > 0.05). These data provide further support for a regionally specific functional link between the lateral SC deep layers and the STN.Disinhibition of visual cortex
To determine whether enhanced activity in the visual cortex might also influence STN visual activity, bicuculline was applied to the primary visual cortex to increase its responsiveness to visual stimuli. Although the application of bicuculline significantly potentiated local cortical visually evoked activity (Fig. 3a,b), in all cases (3/3), the population response of STN neurons remained insensitive to the light flash (Fig. 3c,d). Once again, the STN recording sites were among those from which clear visual responses had been recorded following disinhibition of the lateral SC (supplemental Fig. 1b, available at www.jneurosci.org as supplemental material). Local disinhibition of the visual cortex also failed to influence the baseline firing rate of STN neurons (mean multiunit spikes recorded before and after bicuculline 26.16 ± 2.85 Hz and 30.77 ± 2.79 Hz, respectively; t = –0.925; df = 2; p > 0.05). These data indicate that comparable disinhibition of cortical visual activity was unable to influence either the baseline activity or restore visual sensitivity to STN neurons in the anesthetized preparation.
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Figure 3. Local application of bicuculline disinhibited visually evoked potentials (VEPs) in visual cortex (compare a and b, noting the change of scale in the inset in a) but failed to restore visual sensitivity to the subthalamic nucleus (c and d).
Together, the electrophysiological data suggest that the presence of short-latency visually evoked activity in the STN is critically dependent on input from the lateral SC deep layers but not from the medial SC or visual cortex. This degree of functional segregation within the SC was at odds with current descriptions of direct connections between the SC and the STN in rodents (Tokuno et al., 1994Anatomy
Anterograde tract tracing: light microscopy
Injections of the anterograde tracers PHA-L (n = 4) and/or BDA (n = 8) into the SC revealed a more robust direct pathway to the STN than was previously reported (Tokuno et al., 1994
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Figure 4. A robust tectosubthalamic projection was evident. Photomicrograph of a parasagittal section of rat brain illustrating the location of a large injection of the anterograde tracer PHA-L in the deep layers of the superior colliculus. Dense labeling of fibers and terminal boutons can be seen in dorsal and rostral STN (see inset) as well as in the parafascicular nucleus of the thalamus (PF) and substantia nigra pars compacta (SNc). ic, Internal capsule; SNr, substantia nigra pars reticulata; ZI, zona incerta.
The tectosubthalamic projection originates almost exclusively in the lateral SC. Thus, injections of either PHA-L or BDA into lateral regions (n = 6) were associated with high densities of labeled axons and terminals in ipsilateral STN (Figs. 4, 5a–c). In contrast, the STN was virtually devoid of terminal labeling when injections (n = 6) were directed to the medial SC (Fig. 5d–f). Moreover, tectosubthalamic axons and terminals were differentially distributed within specific subregions of the STN. In the caudal aspects of the STN, anterogradely labeled axons and terminals were largely confined in a dorsal sheet (Fig. 4) that extended across the entire mediolateral dimension of the nucleus (Fig. 5c). Rostrally, terminating fibers filled the entire mediolateral and dorsoventral area of the STN (Fig. 5b). There were many instances where anterogradely labeled boutons were seen in close apposition to STN soma and dendrites (Fig. 5g–j).
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Figure 5. The tectosubthalamic pathway is regionally specific. A coronal section illustrating a biotinylated dextran amine (BDA; anterograde tracer) injection site in the lateral deep layers of the SC (a), associated with dense labeling of terminals in the rostral (b) and central (c) STN. A corresponding injection of BDA into the medial SC (d) produced virtually no anterograde labeling at the same rostrocaudal levels of the STN (e, f). In the latter case, neurons of the STN marked with purple dye were retrogradely labeled by an injection of Fluorogold in substantia nigra (SN) and reacted with Vector VIP chromogen (d). g–j, Examples of terminals and boutons anterogradely labeled from the lateral SC in close apposition with STN neurons retrogradely labeled from SN. Scale bar in f applies to b–d, whereas scale bars in photomicrographs g–j = 25 µm. cp, Cerebral peduncle; MG, medial geniculate nucleus; PAG, periaqueductal gray; ZI, zona incerta.
Anterograde tract tracing: electron microscopy
To determine whether the appositions between terminals labeled from the SC and neuronal elements in the STN established direct synaptic contacts, an electron microscopic analysis was performed on tissue from three rats that received PHA-L injections into the lateral SC. A total of 85 labeled structures were examined, of which 27 were identified as synaptic boutons. These were found to form synaptic contacts with 32 postsynaptic elements within the STN. In each case, the synapse was of the asymmetrical type (Gray's type 1). The labeled terminals made synaptic contact either with dendritic shafts (53%, 17/32) (Fig. 6a) or spines (47%, 15/32) (Fig. 6b) of STN neurons, with a small population of boutons making contact with both (19%, 5/27). These results demonstrate that there is a direct synaptic connection between the SC and the STN and the type of synapse formed suggests that the projection is predominantly excitatory.
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Figure 6. Synaptic boutons (bt) anterogradely labeled with PHA-L from the superior colliculus, forming asymmetrical synapses (arrows) in the STN. a, Synaptic contact with a dendritic shaft (d); b, Synaptic contacts with dendritic spines (s). Scale bars, 0.5 µm.
Retrograde tract tracing: light microscopy
To identify the regional distribution and morphology of tectosubthalamic projection neurons, labeled neurons in the SC were plotted following injections of retrograde tracers CTb (n = 3) or True Blue (n = 3) into the STN. Retrogradely labeled neurons were mainly located in lateral sectors of the SC deep layers (Fig. 7). This impression was confirmed by a three-factor (layers—five levels; medial/lateral—two levels; rostral/caudal—four levels) repeated-measures ANOVA (interaction between the layers and medial/lateral factors: F = 5.254, df = 3, p < 0.05). Collicular neurons retrogradely labeled by STN injections typically were small-to-medium-sized multipolar neurons (Saito and Isa, 1999
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Figure 7. Collicular neurons retrogradely labeled from the STN are concentrated in the lateral deep layers. a, A photomicrograph of a CTb (retrograde tracer) the injection site confined to the STN. b, A photomicrograph of retrogradely labeled neurons (arrows) concentrated in the deep layers of the SC. c, A quantitative plot of labeled neurons at different anterior–posterior levels of the SC (numbers associated with each section indicates its location caudal to bregma in millimeters). cp, Cerebral peduncle; f, fornix; mt, mammillothalamic tract; PAG, periaqueductal gray; ZI, zona incerta.
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Figure 8. Morphology of retrogradely labeled collicular neurons following an injection of CTb into the STN. a, A concentration of small (b and c), with a few medium-sized (d and e), multipolar neurons was located in the lateral deep layers of the SC. Scale bar in d also applies to b, c, and e.
In summary, our tracing experiments demonstrated a substantial anatomical projection between the SC and the STN that originates from small-to-medium-sized neurons concentrated in the far lateral aspects of the deep SC layers. Tectosubthalamic fibers preferentially target dorsal and rostral parts of the STN where they make asymmetric, presumed excitatory, synaptic contacts.
Discussion
The main findings of the present study are as follows: (1) local pharmacological disinhibition of the lateral, but not medial SC deep layers, nor comparable disinhibition of the visual cortex, leads to a short-latency visual activation of the STN; (2) the direct projection from the SC to the STN is more substantial than previously proposed (Tokuno et al., 1994We have demonstrated that STN neurons respond at short latency to visual stimuli and that this response derives from the SC. A close association was observed between the location within the SC where local pharmacological disinhibition was required for visual stimuli to elicit short-latency activation of the STN and tectosubthalamic cells of origin. Thus, the tectosubthalamic projection arises mainly from small-to-medium-sized neurons in the lateral deep layers of the SC, where pharmacological disinhibition was effective. Virtually no anterogradely labeled fibers and/or terminals were observed in the STN following tracer injections into the medial SC deep layers and bicuculline injections into the medial SC left the STN visually unresponsive, despite the presence of robust visually evoked population responses from medial deep SC layer neurons.
A second point of correspondence between the electrophysiological and anatomical data concerns the potential excitatory nature of the tectosubthalamic projection. Unlike our previous electron-microscopic analysis of the projection from the SC to dopaminergic neurons in the ventral midbrain (the tectonigral projection), where both asymmetric (presumed excitatory) and symmetric (presumed inhibitory) synaptic contacts were reported (Comoli et al., 2003
An interesting observation in the present study was that, while visually evoked responses could be recorded from locations throughout the STN, our anterograde tracing data showed that injections of tracer into the lateral SC consistently produced dense terminal labeling confined to a specific region of the STN (rostral and dorsal). There could be several reasons for this apparent inconsistency. First, in the rat, STN neurons typically have large dendritic arbors that can extend over half the length of the nucleus (Kita et al., 1983
Functional implications
Both the SC and the basal ganglia are phylogenetically ancient systems that have been highly conserved throughout vertebrate evolution (Medina and Reiner, 1995Clues to the function(s) of the STN have been gleaned by examining its impact on basal ganglia target structures such as the SC. The STN provides a major input to the basal ganglia output nuclei, including the substantia nigra pars reticulata, which contains the cells of origin of the nigrotectal projection to the SC. Because the subthalamonigral projection is excitatory (Smith et al., 1998
However, additional results in the present study raise problems for both suggestions. The ecology of the rodent is such that threatening stimuli (i.e., predators), presumably requiring the interruption of behavior, are most commonly detected in the upper visual field, which according to the retinocentric map is represented in the medial SC (Dean et al., 1989
Footnotes
Received Dec. 11, 2008; revised Feb. 27, 2009; accepted April 2, 2009.This work was funded by grants from the Biotechnology and Biological Sciences Research Council (to P.G.O.: 062742), Wellcome Trust (to P.R.: WT080943), Medical Research Council, UK (to J.P.B. and J.M.), and National Institutes of Health (to J.G.M.: NS35008). We are grateful to Natalie Kennerley for her excellent histological assistance and to Peter Furness for the provision of software to analyze the electrophysiological data.
Correspondence should be addressed to Paul G. Overton, Department of Psychology, University of Sheffield, Western Bank, Sheffield, South Yorkshire S10 2TP, UK. Email: p.g.overton{at}sheffield.ac.uk
Copyright © 2009 Society for Neuroscience 0270-6474/09/295701-09$15.00/0
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