Single-Cell Correlates of a Representational Boundary in Rat Somatosensory Cortex

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The Journal of Neuroscience, June 1, 1998, 18(11):4403-4416

Single-Cell Correlates of a Representational Boundary in Rat Somatosensory Cortex
Peter W. Hickmott and Michael M. Merzenich
Keck Center for Integrative Neuroscience, University of California, San Francisco, San Francisco, California 94143

  ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

In primary somatosensory cortex (S1), the transition from one representation to the next is typically abrupt when assayedphysiologically. However, the extent of anatomical projectionsto and within the cortex do not strictly respect these physiologicallydefined transitions. Physiological properties, such as synapticstrengths or intracortical inhibition, have been hypothesizedto account for the functionally defined precision of these representationalborders. Because these representational borders can be translocatedacross the cortex by manipulations or behaviors that change theactivity patterns of inputs to the cortex, understanding the physiologicalmechanisms that delimit representations is also an important startingpoint for understanding cortical plasticity.
A novel in vivo and in vitro preparation has been developed to examine the cellular and synaptic mechanisms that underlierepresentational borders in the rat. In vivo, a short segmentof the border between the forepaw-lower jaw representations inrat S1 was mapped using standard electrophysiological methodsand was visibly marked using iontophoresis of pontamine sky bluedye. Slices were then obtained from this marked region and maintainedin vitro. Intracellularly recorded responses to electrical stimulationof supragranular cortex were obtained from single neurons nearthe border in response to stimulation within the representationalzone or across the border. Both excitatory and inhibitory responseswere smaller when evoked by stimuli that activated projectionsthat crossed borders, as compared with stimuli to projectionsthat did not. These findings indicate that intracortical networkproperties are contributing to the expressions of representationaldiscontinuities in the cortex.

Key words: somatosensory cortex; representational boundary; horizontal connections; whole-cell recording; cortical slices; forepaw; lower jaw

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

A distinguishing characteristic of representational maps in the cerebral cortex is the presence of discrete regions that respondto a particular stimulus source. For example, in the somatosensorysystem, discrete regions of primary somatosensory cortex (S1)respond to stimulation of restricted regions of the body surface(Merzenich et al., 1978; Kaas, 1983; Chapin and Lin, 1984). Betweenthese representations are sharp representational "discontinuities"or "borders," regions of the cortex in which the responses ofthe cortical neurons change from one representation to the otherover a short distance across the cortex.

The cellular and circuit processes that underlie these sharply defined borders are not clear. The gross organization of cutaneoussomatosensory representations results primarily from the organizationof the projections to the cortex (Landry and Deschenes, 1981;Jensen and Killackey, 1987a; Rausell and Jones, 1995; Catalanoet al., 1996). However, the projection patterns of both thalamocortical(Landry and Deschenes, 1981; Jensen and Killackey, 1987a; Rauselland Jones, 1995) and intracortical (Chapin et al., 1987; Fabriand Burton, 1991; Weiss and Keller, 1994; Hoeflinger et al., 1995)projections also overlap substantially in S1 and do not strictlyrespect representational borders. Thus, the underlying anatomyis not sufficient to explain the sharpness of the transition fromone response region to another at a representational border. Somephysiological mechanism or mechanisms must be invoked to explaintheir precision.

Much of the information about representational borders has been derived from studies concerning plasticity of cortical representations.Representational maps in the adult cerebral cortex can reorganizeas a result of changes in the activity patterns of their inputsor because of behavioral training (Wang et al., 1995) (for review,see Merzenich et al., 1990; Kaas, 1991; Merzenich and Jenkins,1993; Weinberger, 1995; Buonomano and Merzenich, 1998).

Although the cellular and simple-circuit mechanisms underlying reorganization of sensory cortex are incompletely understood,it is clear that at least part of the changes observed resultfrom plasticity in the cortex itself (Kaas, 1991; Buonomano andMerzenich, 1998). Both the sprouting of new connections (Darian-Smithand Gilbert, 1994) and the strengthening or weakening of existingexcitatory or inhibitory synapses, which lead to "unmasking" ofpreviously existing subthreshold connections, have been implicatedin these reorganizations (Calford and Tweedale, 1988, 1991a,b;Donoghue et al., 1990; Nudo et al., 1990; Turnbull and Rasmussen,1990; Byrne and Calford, 1991; Chino et al., 1992; Pettet andGilbert, 1992; Recanzone et al., 1992a; Nicolelis et al., 1993).

The connections that are involved in representational plasticity in cortex are unclear. For example, in visual cortex, plasticityinduced by binocular retinal lesions appears to be mediated byintrinsic horizontal connections in V1 (Darian-Smith and Gilbert,1994, 1995; Das and Gilbert, 1995). In rat sensorimotor cortex,evidence suggests that plasticity is related to changes in boththalamocortical (Jensen and Killackey, 1987b; Armstrong-Jameset al., 1994; Rausell and Jones, 1995) and intracortical (Huntleyand Jones, 1991; Armstrong-James et al., 1994; Weiss and Keller,1994; Huntley, 1997) projections. Considering that both intracortical(Lee et al., 1991; Hirsch and Gilbert, 1993; Hess and Donoghue,1994; Hess et al., 1996) and thalamocortical (Lee and Ebner, 1992;Kirkwood et al., 1993; Crair and Malenka, 1995) connections canexhibit synaptic plasticity, either or both would be reasonablecandidates for rapid changes in representations. Recent data fromrat S1 suggest that rapid plasticity depends on changes in thestrengths of intracortical connections (Armstrong-James et al.,1994).

In this paper, a combined in vivo and in vitro preparation is described in which the effects of a representational borderon excitatory postsynaptic potentials (EPSPs) and inhibitory postsynapticpotentials (IPSPs) evoked in single cortical neurons by stimulationof supragranular horizontal connections were characterized. Thedata provide insights into possible mechanisms that allow thecortex to restrict excitation across borders between functionallydefined, cortical regions. The ultimate goal is to determine howbasic cellular phenomena account for the representational changesrecorded in the cortex after peripheral input manipulations andin learning. Some of these data have been previously presentedin abstract form (Hickmott and Merzenich, 1996).

  MATERIALS AND METHODS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

In vivo recording and production of marked slices. Using standard in vivo extracellular recording methods (Recanzone et al.,1992b; Xerri et al., 1994), a short section of the border betweenthe forepaw-lower jaw representations was mapped in rat S1. AdultSprague Dawley rats (280-350 gm) were anesthetized to an areflexiclevel with pentobarbital (50 mg/kg of body weight, i.p.) and mountedin a stereotaxic frame. Supplemental doses of anesthetic wereadministered as needed. Atropine (0.054 mg) was injected intraperitoneallyto reduce respiratory secretion. Lidocaine (2%) was injected subcutaneouslyaround wound margins and at pressure points. Rectal temperaturewas monitored and maintained at ~38°C with a heating pad. Allsurgical procedures were approved by the University of CaliforniaSan Francisco Committee on Animal Research.

After reflecting the skin and temporalis muscle, S1 was exposed via a wide craniotomy approximately centered on bregma, thedura was removed, and the cortex was covered with silicone oil.A computer image of the brain surface was recorded using a CCDcamera and NIH Image software. Carbon-fiber electrodes (10 µmfiber diameter) designed to generate minimum damage were usedfor response mapping. The forepaw or lower jaw was stimulatedwith a fine glass probe to elicit multiunit cutaneous responsesin S1. Responses were amplified 500× or 1000× (DAM-50 amplifier,WPI Instruments, or custom-built amplifier), filtered between300 Hz and 10 kHz (Krone-Hite Inc.), and fed into an oscilloscopeand audio monitor. Responsiveness to forepaw and lower jaw stimulationwas determined subjectively by listening to the audio monitoroutput. Penetrations were introduced into the forepaw zone, 1-2mm rostral to bregma; subsequent penetrations were introducedmore laterally until regions that responded to tactile stimulationof the lower jaw were encountered. Recordings were all at an approximatedepth of 700-800 µm. The location of penetrations was recordedon the computer image of the cortex by using surface vasculaturelandmarks. Penetrations spaced <50 µm apart were then made tolocate the border more exactly. Typically, three of these rowsof penetrations were made and arranged perpendicular to the forepawand lower jaw border, which is normally oriented roughly parallelto the midline. Rows were separated by 400-500 µm (see Fig. 1A).Three or four locations on the forepaw and lower jaw border werethen marked by iontophoresis of Chicago sky blue (Sigma, St. Louis,MO) (2% in 0.5 M Na acetate; 150-200 µm below the surface for6-8 min, using <0.5 µA of ejection current; see Fig. 1A). Dyemarks typically had initial diameters of ~200 µm, but became smallerover time, reaching a final diameter of 10-50 µm after 1-2 hrin vitro.

After marking, the animal was decapitated, the brain was rapidly removed, and 400-µm-thick coronal slices were cut on a vibratomefrom the marked region of cortex. Slices with a dye mark locatingthe border that was defined previously were selected for use invitro (see Fig. 2A). The supragranular layers of the cortex werethen isolated with a cut parallel to the cortical surface aroundlayer 4 (500-700 µm from the cortical surface). These slices weremaintained in standard mammalian bicarbonate buffer (in mM: NaCl,119; KCl, 2.5; NaH₂PO₄, 1.25; MgSO₄, 1.3; CaCl₂, 2.5; NaHCO₃,26.2; and glucose, 11; saturated with 95% O₂ and 5% CO₂) for intracellularrecording. Note that these and all subsequent chemicals were obtainedfrom Sigma, unless otherwise stated. Slices were checked for viabilityand stability by recording maximal extracellular field potentialsin layer 3 in response to electrical stimulation at or above layer4 (0.05 Hz; see Fig. 2B). Field potentials so obtained closelyresembled those evoked in visual cortex by layer 4 stimulation(Kirkwood and Bear, 1994), consisting of a small rapid negativityfollowed by a main negativity at a latency of ~5 msec (see Fig.2B, asterisk). Note that the small, slow negative potential evidentafter the main negative potential in the example in Figure 2Bwas observed in the majority of cases; this slow negativity resultedfrom the relatively high-intensity stimuli presented close tothe recording site and did not reflect any unhealthiness of theslice. Electrodes for field recording were glass of ~1.5-2.5 µmtip diameter, filled with 1N NaCl (1-4 M $Omega$ resistance). Only slicesin which stable fields with a main negativity (see Fig. 2B, asterisk)of >0.6 mV were used.

Intracellular recording. Neurons for recording were obtained using blind whole-cell recording (Blanton et al., 1989) froma region near the mark (~100-200 µm) in cortical layer 2/3. Patchelectrodes were pulled on a Flaming-Brown puller to a tip diameterof 1.5-2.5 µm and filled with (in mM): Cs gluconate (Aldrich,Milwaukee, WI), 128; CsCl, 7; EGTA, 1; HEPES, 10; QX-314, 10;Mg ATP, 2; Na GTP, 0.2; and biocytin 0.3-0.5%, pH 7.0-7.4. Suchelectrodes had tip resistances of 3-8 M $Omega$ . QX-314 (Research Biochemicals,Natick, MA) was included to block action potentials so that theamplitude of large postsynaptic potentials (PSPs) could be quantified.Only neurons with initial resting potentials of less than $-$ 60mV and stable input resistances of >50 M $Omega$ were used. For recordingPSPs, positive or negative current was injected to maintain themembrane potential at $-$ 50 to $-$ 55 mV.

Recorded signals were amplified using an Axoclamp 2B amplifier (Axon Instruments, Foster City, CA), digitized at 10 kHz, andsaved to the hard disk of a Gateway 486 computer using Experimenter'sWorkbench (DataWave Inc.) data acquisition system. PSPs were recordedin these neurons in current-clamp mode by stimulating layer 2/3at the same distance from the cortical surface as the cell. Thestimulating electrode was a bipolar, parylene-coated 1 M $Omega$ tungstenelectrode with a tip separation of ~100-150 µm (FHC Inc.). Stimuliwere divided into two categories based on the horizontal distanceof the stimulation sites from the impaled neuron: the first categoryconsisted of stimuli within 300 µm of the neuron and is referredto as close stimulation; the second consisted of stimuli between450 and 800 µm and is referred to as distant stimulation. Usuallya given neuron was only stimulated in one of these categories.To examine possible effects at the border on connections withincortical layer 2/3, brief electrical stimuli (100 µsec duration,0.1 Hz) were presented in layer 2/3 at one of two locations withrespect to the impaled neuron. The first location was across theborder from the patched neuron, either at a close or distant site,and the second location was at the same horizontal distance fromthe neuron as the first site, but on the other side of the neuron.Thus, in the second case there was no border interposed betweenrecording and stimulating electrodes. Throughout this paper, thefirst case, cross border stimulation, will be referred to as "CBstimulation" and the second case, noncross border stimulation,will be referred to as "NCB stimulation". Both sites were at thesame distance from the cortical surface as the impaled neuron.This recording and stimulating configuration is schematized inFigure 2A, left, in which the locations of CB (black square) andNCB (gray square) stimulation are shown with respect to the border(open circle) and recording site (inverted triangle). Thus, onestimulus site was in the forepaw representation and one in thelower jaw representation, as determined by the in vivo mapping.To minimize variability, the same stimulating electrode at thesame polarity was used for both stimuli and was approximatelypositioned with the aid of a microscope eyepiece graticle. Theelectrode position was then more precisely adjusted to equalizethe time from stimulus to PSP initiation between CB and NCB stimulation.PSPs were evoked at both of these sites starting below the minimalintensity necessary to evoke a PSP and gradually increased toa supramaximal intensity, thus generating a complete input-output(I-O) curve for each neuron. The same stimulus intensities wereused at both sites of stimulation except when lower and higherstimuli were necessary to define the minimal and maximal responses.Because sodium-dependent spikes were blocked with intracellularQX-314, it was possible to record pure PSPs even at high stimulusintensities in most cells. However, in some cells large voltage-activatedpotentials were evoked by larger PSPs; these cells were not usedfor PSP analysis, although they were sometimes used for analysisof pure IPSPs (see below). PSPs were evoked around the reversalpotential for IPSPs, typically at $-$ 50 to $-$ 55 mV. The average ofthree to five individual PSPs was used for quantification at eachstimulus intensity (see Fig. 3).

Control data. To control for possible nonspecific effects of the mapping, marking, and slicing procedures, the forepaw-lowerjaw region was mapped in vivo as above, but dye marks were placed300-500 µm medial to the border. These marks were specificallyplaced near the center of the forepaw representation at a distancefrom major representational borders. Control data were obtainedfrom neurons close to these dye marks in a manner identical tothat detailed above for neurons close to the marked border. Theresulting PSPs were also analyzed identically, as detailed below.Thus, data were obtained from these neurons as detailed above,but no representational borders were close to the neurons, onlya dye mark. As shown in Figure 2A, right, the stimulating electrodesin these control preparations were placed in two locations: eitherat a site in layer 2/3 in which the dye mark (open circle) wasbetween the recording (inverted triangle) and stimulating electrodes[cross-mark (CM) stimulation, black square], or at an equidistantsite on the opposite side of the neuron, in which there was nodye mark interposed [ non-cross-mark (NCM) stimulation, gray square].Thus, NCM stimulation was equivalent to NCB stimulation, whereasCM stimulation was analogous to CB stimulation. However, in thecontrol slices, no border intervened between the CM stimulationsite and the recording site, as opposed to the CB case, in whichthe dye mark and the border coincided. Control data were onlyobtained using close stimulation (i.e., <300 µm from the neuron).

Analysis of PSPs. For each stimulus intensity, two PSP characteristics were determined: the peak amplitude of the PSP andthe time required for the potential to fall from peak amplitudeto one-half the peak amplitude (t_1/2). This measure of fall timewas chosen as a method of quantifying later components of thePSP. From these measures, three parameters that summarize thedata across stimulus intensities were defined (see Fig. 3B). (1)The maximal peak amplitude (pk_max) and (2) the steepness of theinput-output function (Salin and Prince, 1996) were defined. Becausethe I-O plots were asymptotic, they were generally well fit bya single exponential function (see Fig. 3B, left). The steepnessof the I-O function was thus measured by fitting an exponentialto the data and calculating the value of $tau$ (I-O $tau$ ). Smaller I-O $tau$ values reflect steeper slopes of the submaximal portion of theI-O curve. Note that for one neuron in the analysis of IPSPs,the $tau$ values were not used in the analysis, because the R² value for both CB and NCB stimulation was <0.5 (see Fig. 6B).(3) The ratio of the mean of the t_1/2 values from the PSPs elicitedby the higher 50% of the stimuli (t_1/2, high) (see Fig. 3B, rightplot, squares) divided by the mean t_1/2 values from PSPs elicitedby the lower 50% of the stimuli (t_1/2, low) (see Fig. 3B, rightplot, circles) was also defined. This ratio (referred to as h/lratio) was used as a measure of the contribution of later responsesto the compound PSP (see Figs. 3, 4).

Two additional parameters were also measured: the threshold stimulus intensity required to evoke a minimal PSP and the latencyof the PSP. Because the latency decreased slightly at higher stimulusintensities, the latency was measured for relatively small PSPs(~5 mV amplitude).

To determine whether there was an effect of the representational border, parameters were compared for CB and NCB (or CM andNCM in control slices) stimulation using paired, two-tailed Student'st tests; p < 0.05 was taken to be significant.

Reversal potentials were determined in voltage-clamp mode by evoking postsynaptic currents (PSCs) at various holding potentials(typically from $-$ 80 to +20 mV). All PSCs were evoked by closestimulation (<300 µm). The reversal potential was determined atthree regions of PSCs: (1) at the peak of the PSC evoked by minimalstimulation, which estimated the contributions of EPSCs and IPSCsto monosynaptic responses; (2) at the peak of a PSC evoked atmaximal stimulation, which estimated the contributions of higher-thresholdmonosynaptic and rapid disynaptic responses; and (3) at a point20 msec after the peak of the PSC evoked at maximal stimulation,which was approximately at the peak of the IPSC and estimatedthe contribution of longer latency events.

Analysis of IPSPs. To isolate monosynaptic IPSPs, a combination of 10-15 µM 6,7-dinitroquinoxaline-2,3-dione (DNQX; ResearchBiochemicals) or 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX; ResearchBiochemicals) and 100 µM DL-2-amino-5-phosphonopentanoic acid(APV) was bath-applied via the perfusion system for >10 min. PSPsat several stimulus intensities from minimal to maximal were obtainedfor both CB and NCB sites. The peak amplitude and the t_1/2 weredetermined for the IPSP at each intensity, and the maximal peakamplitudes (ipk_max), I-O $tau$ (I-O i $tau$ ) and the average and maximalt_1/2 (it_1/2 avg and it_1/2 max, respectively) were determined forCB and NCB stimulation. Typically, IPSPs were recorded at $-$ 40to $-$ 45 mV. Values were compared using paired t tests, as for theanalysis of PSPs. Reversal potentials were also determined forthe peak of pure IPSCs in a manner similar to that described above.Note that isolated IPSPs could only be recorded reliably withclose stimulation.

Cytochrome oxidase histochemistry. After mapping and marking of the forepaw-lower jaw border, as detailed above, a small (~2mm in the rostral-caudal dimension) piece of cortex around themarked border was removed and fixed in 4% paraformaldehyde overnight.The tissue was then rinsed in 0.1 M PBS and sectioned in the coronalplane at 50 or 100 µm on a vibratome. These sections were thenreacted for cytochrome oxidase (Wong-Riley and Welt, 1980) ina solution consisting of 0.5 mg/ml diaminobenzidine, 0.3 mg/mlcytochrome C (type III), and 0.2 mg/ml catalase in 0.1 M PBS.The reaction was allowed to proceed at 37°C until staining wasclearly visible (~4 hr). Sections were then rinsed in PBS, mountedon slides in 90% glycerol and 10% PBS, and examined at low power.

Throughout this paper, values are expressed as mean ± SEM, unless otherwise indicated.

  RESULTS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

In this study, the border between the forepaw and lower jaw representations was mapped in vivo using standard extracellularmapping techniques, and the border then was visibly marked byiontophoresis of Chicago sky blue dye. Coronal slices from themarked region were maintained in vitro, and the synaptic responsesof single neurons to stimuli of infragranular cortex were comparedfor stimuli that were delivered across the border versus equidistantstimuli that were not. Differences in both excitation and inhibitionevoked by CB versus NCB stimulation were discovered.

Mapping the forepaw-lower jaw border in vivo

Initially, a short segment (~1.5 mm) of the border between the forepaw and lower jaw representations was mapped using standardextracellular techniques in vivo. As observed previously in therat (Chapin and Lin, 1984; Waters et al., 1995), extracellularresponse mapping revealed a relatively sharp discontinuity betweenthe forepaw and lower jaw representations (Fig. 1A). However,in a number of animals, single penetrations that exhibited responsesto stimulation of both the forepaw and lower jaw (Fig. 1A, opencircles), typically unequally and relatively weakly, were obtained.These dual response penetrations were frequently associated witha lighter state of anesthesia. The forepaw-lower jaw responsivepenetrations could have resulted from the use of multiunit responsesto map the border, and/or from the activation of noncutaneousdeep inputs from the joints or muscles by our relatively vigorousstimulation. Also, considering that penetrations near the borderwere in perigranular cortex (Fig. 1B) and such cortex containsneurons with large receptive fields (Chapin and Lin, 1984), itis not surprising that such dual-response penetrations were obtained.Furthermore, cutaneous receptive fields are known to expand inunanesthetized animals (Chapin and Lin, 1984). Thus, the degreeof response overlap in the map of S1 should increase with lighteranesthesia. When such a penetration was obtained, the border betweenforepaw and lower jaw representations was drawn through that point.In cases in which there were no dual-response penetrations, theborder was drawn halfway between the adjacent penetrations, separatedby ~50 µm, in which exclusive forepaw and lower jaw responseswere recorded.

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Figure 1. A, Example of mapping the forepaw-lower jaw border. Inset shows a schematic of a lateral view of the rat cortex, indicating the approximate location of the "ratunculus"; dashed box indicates the approximate location of the craniotomy and the body surface map illustrated in the main figure. An outline of the rat S1 map is superimposed over the surface of the cortex (Chapin and Lin, 1984). White circles represent penetrations responding to forepaw stimulation, white squares represent lower jaw responsive penetrations, and open circles reflect penetrations responding to both. Black circles represent the dye marks that defined the border between representations. The asterisk is placed at bregma, rostral is to the right, lateral is toward the bottom. FBP, Frontal buccal pads; N, nose; RV, rostral vibrissae; UZ, unresponsive zone; FL, forelimb; HP, hindpaw. B, Cytochrome oxidase staining from a marked slice (100 µm thick). The location of the mark is indicated by the asterisk, and the arrows point to individual barrels in layer 4 in the forepaw (FP) and lower jaw (LJ) representations. Medial is to the left and the surface of the cortex is at the bottom.

Dye marks were placed along the border as indicated in Figure 1A (black circles) using low-current iontophoresis. Consideringthat intracortical microstimulation has been shown to change thesize of cortical representations in vivo (Nudo et al., 1990; Recanzoneet al., 1992a), albeit with higher intensities and longer durations,we remapped the same border after marking (n = 5, data not shown).There was no evidence of any effect of the iontophoresis on thelocation of the border. Furthermore, both bis-benzimide stainingfor nuclei (n = 3) and cresyl violet Nissl staining (n = 4) insections from the marked region showed no evidence for any lesionor other discernible damage to neurons in the region of the mark(data not shown). Dye marks decreased in size over the courseof the experiment, with a typical starting diameter of ~200 µmand a typical final diameter of ~10-50 µm.

To relate the location of the physiologically defined border to the cytoarchitectural correlates of the forepaw and lowerjaw representations, we examined sections from mapped and markedcortex that were then stained for cytochrome oxidase. This procedureallows the differentiation of granular from perigranular and agranularregions of S1 cortex (Chapin and Lin, 1984; Fabri and Burton,1991), and the cytochemically defined representations generallycorrespond to the physiologically defined (Waters et al., 1995,but see McCandlish et al., 1996). As shown in Figure 1B, the physiologicallydefined border (asterisk) falls in perigranular cortex betweenthe forepaw granular region and the lower jaw granular region.

In vitro recording

Recordings were obtained from 36 neurons in marked slices, 25 of which were used for close stimulation (<300 µm) and 11 ofwhich were used for distant stimulation (>450 µm), and from 12neurons from control slices. A schematic of the marked slice preparationis shown in Figure 2A, left, whereas a schematic of a controlslice is shown in Figure 2A, right. All neurons were recordedin superficial cortical layers (mean estimated distance from corticalsurface, 248 ± 8 µm). For the close stimulation category, themean estimated distances of the stimuli from the neuron were 210± 6 µm for CB and CM stimulation and 213 ± 7 µm for NCB and NCMstimulation. For the distant stimulation category, the mean estimateddistance was 621 ± 25 µm for CB and 626 ± 26 µm for NB stimulation.Kruskal-Wallis tests followed by planned Mann-Whitney U testsrevealed that the distances for close stimulation were not significantlydifferent (p > 0.6), whereas those from distant stimulation weresignificantly different from both the marked and control distances(p < 0.0001). The equivalence of the stimulation distances betweenCB and NCB stimulation was confirmed by examining the latencyfrom stimulus artifact to PSP onset for each stimulation site;latencies were 2.63 ± 0.1 msec for CB and CM and 2.58 ± 0.1 msecfor NCB and NCM stimulation (p > 0.4; Mann-Whitney test). Notethat the preceding latency data are presented pooled across bothcontrol and marked slices, because these values did not differsignificantly between control and marked slices (Mann-Whitneytests; p > 0.5). In marked slices, neurons ranged from 100-350µm from the mark; for close stimulation, the mean was 140 ± 5µm and for distant stimulation the mean was 179 ± 23 µm. Thesevalues were significantly different (p < 0.05; Mann-Whitney Utest). All cells were obtained randomly on either the medial (forepawzone) or lateral (lower jaw zone) side of the mark. Nonparametrictests were used to compare these data because their frequencydistributions were generally not normal (Fig. 2C).

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Figure 2. The slice preparation: stimulating and recording parameters. A, Schematic representations of coronal slices taken from rat S1 used in these studies. In both schematics, the inverted triangle represents the recording electrode, the heavy line represents the cut placed in layer 4 to isolate supragranular layers, and the dotted line represents the location of the border between the forepaw and lower jaw representations. The parallel lines represent the stimulating electrodes, with the polarities of the two electrodes indicated. Note that the same polarity configuration was used between CB and NCB stimulation, so that the same electrode of the bipolar pair was at the stimulation site. Left panel, Schematic of a slice in which the border between the forepaw and lower jaw was marked before slicing. Black square, Cross-border (CB) simulation site; gray square, noncross-border (NCB) stimulation site; open circle, dye mark, dotted line, border. Right panel, Schematic of a control slice in which the dye mark (open circle) was placed at a site in the forepaw representation of S1 away from the border (dotted line). Black square, Cross-mark (CM) stimulation site (note that no border is interposed between stimulating and recording); gray square, noncross mark (NCM) stimulation site. B, Example of a maximal amplitude field potential recorded from a slice in which the forepaw-lower jaw border was marked in vivo. The potential was recorded in cortical layer 3 in response to electrical stimulation (90 µA) above cortical layer 4. This trace is the average of 20 individual potentials. The asterisk marks the main negativity (see Materials and Methods). C, Frequency distributions of estimated stimulation distances from neurons, latencies from stimulus to PSP onset, and estimated distances of neurons from the cortical surface (i.e., depth), for close stimulation, control slices, and distant stimulation. For distances and latencies, data from both cross and noncross stimulating cases are shown. These distributions clearly demonstrate that these data are generally poorly fit by a normal distribution, and thus nonparametric statistical tests were used to compare them.

The mean resting potential of sampled neurons (pooled for all neurons) was $-$ 70 ± 0.7 mV, and the mean input resistance was114.8 ± 3.5 M $Omega$ . Because of the presence of Cs⁺ and QX-314 in the electrode filling solution, these initial valuesincreased over the course of 10-15 min, reaching mean values of $-$ 42.4 ± 1.4 mV and 147.1 ± 6.7 M $Omega$ , respectively. Only after thesevalues were unchanging for >2-3 min were data collected from theneuron.

Characteristics of PSPs and effects of the border-close stimulation category

Figure 3A shows examples of PSPs evoked with CB (left) and NCB (right) stimulation at various stimulus intensities. ThesePSPs are compound events, consisting of monosynaptic and polysynapticcontributions by both EPSPs and IPSPs. At low stimulus intensities,small and longer duration PSPs, which were depolarizing at approximately $-$ 50 mV, were typically obtained; these were initially thoughtto be relatively pure monosynaptic EPSPs. However, in some cases(5 of 33) the response to the threshold stimulus was negativeat approximately $-$ 50 mV, indicating monosynaptic IPSPs (Fig. 4;see Fig. 6). At higher stimulus intensities, larger and more rapiddepolarizing events were obtained, usually followed by a relativelylong hyperpolarization. The peak amplitudes (left) and t_1/2 values(right) of each of these PSPs are quantified across stimulus intensitiesfor CB (filled circles) and NCB (open circles) in Figure 3B. Forthe amplitude (Fig. 3B, left), there was a progressive increasewith increasing stimulus intensity until the amplitude plateaued.The lines in Figure 3B, left, represent the exponential fit tothe I-O curve; values of $tau$ for these fits were used as a measureof the steepness of the submaximal region of the curve. This increasein amplitude is apparently caused by activation of higher-thresholdexcitatory inputs to the neuron (Fig. 4).

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Figure 3. A, Examples of PSPs evoked by close stimulation (~240 µm in this example) for cross-border (CB, left) and non-cross-border (NCB, right) stimulation. Traces range from the minimal to maximal responses at each site, and each is the average of 3-5 individual responses. Corresponding shades of gray represent responses from corresponding stimulus intensities; four gray levels are used to differentiate intensities, and thus the grays repeat every fifth intensity. Membrane potential of this neuron was adjusted to $-$ 55 mV. B, Quantification of the PSPs shown in A. Filled symbols indicate CB stimulation, whereas open symbols indicate NCB. The left plot shows the amplitude at the peak of each PSP in A. The lines represent the best exponential fit of the input-output curve; the solid line is fitted to the data from NCB stimulation, and the broken line is fitted to data from CB stimulation. The right plot shows the 50% decay time (t_1/2) for each PSP. In the right plot, t_1/2 values from the lower 50% of stimuli (whose mean equals t_1/2 low) are shown by circles, whereas the t_1/2 values from the upper 50% of stimuli (whose mean equal t_1/2 high) are shown by squares. Note that when there was an odd number of stimulus intensities, the data from the centermost point were not used in the calculation of the h/l ratio (Fig. 2B, right, filled triangle).

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Figure 4. Mean current-voltage (I-V) relations for PSCs evoked by close stimulation pooled for CB and NCB cases. Each curve represents the mean peak current obtained for the indicated PSC. A, I-V curves reflecting primarily excitation. Circles are from the peak of the current evoked by minimal stimulation (n = 7). Squares are from the peak of the current evoked by maximal stimulation (n = 7). B, I-V curves reflecting primarily inhibition. Triangles are from currents measured at 20 msec after the peak of the maximal current (n = 10). Diamonds are from the peak of isolated IPSCs (n = 6).

There was also a rapid decrease in t_1/2 with increasing stimulus intensity that plateaued at a minimum (Fig. 3B, right). Toquantify the effects of increasing stimulus intensity on the longer-latencycomponent of the PSPs, the ratio of the mean t_1/2 resulting fromhigher-intensity stimuli (Fig. 3B, right, squares) to the meant_1/2 resulting from lower-intensity stimuli (Fig. 3B, right plot,circles) was calculated. This ratio is termed the h/l ratio (seeMaterials and Methods). Thus, a decrease in the h/l ratio couldeither reflect a smaller mean t_1/2 at high stimulus intensitiesor by a larger t_1/2 at low stimulus intensities, or both. Thisdecrease was apparently caused by the activation of IPSPs, bothmonosynaptic and polysynaptic, at higher stimulus intensities(Fig. 4). The values of these PSP parameters are summarized inTable 1 and Figure 5.


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Table 1. PSP parameters

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Figure 5. Quantification of the differences between parameters determined for NCB and CB (NCM and CM for control data) stimulation from PSPs evoked by close stimulation. A, Mean differences (NCB $-$ CB for marked, NCM $-$ CM for control) in pk_max (left), I-O $tau$ (left-center), h/l ratio (right-center), and threshold (right). Significance values are from unpaired, Student's t tests performed on each of the difference values from marked versus difference values from control slices. B, Individual difference scores (NCB $-$ CB for marked, NCM $-$ CM for control) from each neuron used to calculate the means in A.

To differentiate more precisely between excitation and inhibition, the reversal potentials of various parts of PSCs correspondingto the early and late components of the PSP, were determined.The mean reversal potential of PSCs evoked by minimal stimulationwas $-$ 21 ± 4 mV (Fig. 4A, circles; n = 7), indicating that eventhe threshold monosynaptic PSCs (and thus PSPs) were a mixtureof EPSCs and IPSCs. To examine the contributions of EPSCs andIPSCs to PSCs evoked by maximal stimulation, the reversal potentialsat the peak of the PSC (Fig. 4A, squares) and at a point 20 msecafter the peak (Fig. 4B, triangles) were determined. The meanreversal potential of the peak of the large PSCs was $-$ 4 ± 4 mV(n = 7), indicating that the peak of these larger PSCs primarilyreflected the recruitment of monosynaptic and polysynaptic EPSCs.At 20 msec after the peak of the maximal PSC, the reversal potentialwas $-$ 50 ± 2 mV (n = 10, Fig. 4B, triangles), indicating strongactivation of IPSCs, which caused the sharp decrease in the falltime with stronger stimulation. This value did not differ significantlyfrom the value obtained for pure, monosynaptic IPSCs obtainedin the presence of DNQX and APV ( $-$ 47 ± 6 mV, n = 6; Fig. 4B, diamonds).Generally, the current-voltage relations of EPSCs were approximatelylinear below 0 mV, an observation that differs from that observedby other investigators (Sutor and Hablitz, 1989b; Hirsch and Gilbert,1991). It is likely that the inclusion of QX-314, cesium, or bothin the filling solution blocked voltage-dependent conductancesthat have been suggested to underlie this voltage dependence (Sutorand Hablitz, 1989b; Hirsch and Gilbert, 1991).

The mean values of several PSP parameters for both CB and NCB stimulation (or CM and NCM stimulation for control slices) arepresented in Table 1. In Figure 5A, the mean differences betweenresponses to NCB and CB stimulation in marked slices (hatchedbars) and between responses to NCM and CM stimulation in controlslices (solid bars) are presented and compared (unpaired t tests)for some of these parameters. In Figure 5B, the individual differences(NCB $-$ CB, or NCM $-$ CM for control) used to generate the meansin Figure 5A for each neuron are presented. Note that the datain Figure 5 is from PSPs evoked by close stimulation. In controlslices, there were no significant differences in any measuredparameters between NCM and CM stimulation. However, in markedslices, in which a representational border intervened betweenCB stimulation and the neuron, there were significant differencesbetween NCB and CB stimulation for Pk_max, I-O $tau$ , h/l ratio, andthreshold (Table 1, Fig. 5). Furthermore, for pk_max, I-O $tau$ andh/l ratio these differences were significantly different fromthe corresponding NCM versus CM differences for control slices(Fig. 5A, unpaired t test). The positive NCB $-$ CB differencesfor pk_max, $tau$ , and threshold indicate that excitation, probablyboth monosynaptic and polysynaptic, was smaller with CB than withNCB stimulation. One alternative possibility, that there was moreinhibition with CB stimulation, was rejected because inhibition,as measured by IPSPs, was also weaker with CB stimulation (Fig.6).

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Figure 6. Examples of monosynaptic IPSPs and quantification of differences between NCB and CB stimulation. A, Examples of direct IPSPs recorded in the presence of 12 µM DNQX and 100 µM APV; the membrane potential was adjusted to $-$ 45 mV. These IPSPs were recorded from the same neuron as were the PSPs shown in Figure 2. Corresponding shades of gray represent responses from corresponding stimulus intensities as in Figure 3. Top traces, averages of 3-5 IPSPs evoked from minimal to maximal stimulus intensities, CB stimulation. Bottom traces, IPSPs evoked with NCB stimulation in the same cell. B, Effects of 50 µM CGP35348 (second from bottom trace) and bicuculline (top traces) on IPSPs. Note the residual EPSP in the presence of bicuculline in some cases. Each trace is the average of three potentials, and the membrane potential was adjusted to $-$ 45 mV. C, Mean differences (NCB $-$ CB) in ipk_max (left), I-O i $tau$ (center), it_1/2 avg and it_1/2 max (right). Significance values are from paired, Student's t tests performed on each of the parameters from NCB stimulation versus those from CB stimulation, n = 11 neurons. *p < 0.05; **p < 0.01. D, Individual difference scores from each neuron used to calculate the means in B.

From the reversal potential data in Figure 4, it is clear that the later components of the PSP are dominated by IPSPs, particularlyat higher stimulus intensities. Thus, the h/l ratio is a reasonablemeasure of the amount of inhibition that is activated by higher-intensitystimuli. Examination of the data in Table 1 indicates that t_1/2high, t_1/2 low, and h/l ratio were all larger with CB stimulationthan these parameters were for NCB, CM, or NCM stimulation. Thesedata suggest that there was less inhibition contributing to PSPsevoked by CB stimulation than there was contributing to thoseevoked by NCB stimulation. The difference in the amount of inhibitionwas particularly apparent at higher stimulus intensities in whichinhibition of the PSPs was strongest.

Effects on IPSPs

The suggestion that inhibition might also be weaker with CB stimulation led us to examine IPSPs directly. Monosynaptic IPSPswere isolated by bathing slices in 10-15 µM DNQX (or CNQX) plus100 µM APV. Bath application of 10-25 µM bicuculline methiodideblocked these IPSPS (n = 6; Fig. 6B). In four of six neurons,there was a small residual PSP of unknown type, even in the presenceof CNQX, APV, and bicuculline (Fig. 6B). This remnant potentialcould be similar to the slow excitatory PSP detected in rat layerV neurons, which has been shown to be a combination of cholinergicand noradrenergic PSPs (Benardo, 1993). Furthermore, GABA_B-mediatedPSPs were not observed because of the block of the K⁺ channel activated by the GABA_B receptor by Cs⁺ and QX-314 in the electrode (Otis et al., 1993). The lack ofany GABA_B response was confirmed in a few cells (n = 4) by bathapplication of the general GABA_B antagonist, CGP35348 (CIBA, Suffren,NY) (Fig. 6B). Examples of monosynaptic IPSPs evoked by CB (toptraces) and NCB (bottom traces) stimulation are shown in Figure6A.

These IPSPs were quantified in a similar manner to the compound PSPs: the amplitude at the peak and the 50% fall time weredetermined for the IPSP evoked at each stimulus intensity, andthe maximal peak amplitude (ipk_max), I-O i $tau$ , threshold, and themaximal and mean t_1/2 values (it_1/2 max and it_1/2 mean) were determinedfor the neuron. The mean values of these parameters for CB andNCB stimulation are presented in Table 2. The mean of the differencescores (NCB $-$ CB) for these parameters for each neuron is shownin Figure 6C, and the individual differences used to generatethese means are shown in Figure 6D. Monosynaptic IPSPs had smalleramplitudes (ipk_max; I-O i $tau$ ) and durations (it_1/2 max and it_1/2avg) with CB stimulation than with NCB stimulation, confirmingthe relative weakness of inhibition with CB stimulation that wassuggested by the data from the compound PSPs.


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Table 2. IPSP parameters

PSPs evoked by distant stimulation

The PSPs discussed so far were evoked with stimuli within 300 µm of the impaled neuron. Even with the cut to isolate layer2/3, the circuitry activated by such stimuli is complex and couldinclude both orthodromic and antidromic activation of horizontalconnections, axons and their recurrent collaterals, isolated thalamocorticalarbors, and processes of the impaled neuron. PSPs were thereforeevoked with more distant stimulation (between 450 and 800 µm)in which there would be a relatively greater contribution to thePSPs by the activation of layer 2/3 horizontal connections. Examplesof PSPs evoked by distant stimulation from CB (top traces) andNCB (bottom traces) sites are presented in Figure 7A; the PSPsshown were evoked using minimal to maximal stimulus intensities.The same parameters were measured for these PSPs as were measuredfor PSPs evoked by close stimulation, and are summarized in Table1. PSPs evoked by distant stimulation were qualitatively similarto those evoked by close stimulation. Their peak amplitudes increasedwith increasing stimulus intensity until a plateau was reached,reflecting increasing activation of excitatory inputs, and werewell fit by a single exponential. Their fall times tended to beshorter at higher stimulus intensities. However, late hyperpolarizationswere less frequently observed (4 of 11 cells). This observationindicates that inhibition played a weaker role in the late componentsof these PSPs, which were more strongly dominated by excitation.This observation is unsurprising, because the range of monosynapticinhibitory connections in rat S1 slices has been determined tobe ~400 µm (Salin and Prince, 1996), which leaves only polysynapticinhibition to suppress excitation in the distant stimulation case.Furthermore, PSPs evoked by distant stimulation had significantlysmaller amplitudes (Pk_max and I-O $tau$ ; Table 1), and larger falltimes and thresholds (t_1/2 low, t_1/2 high, and threshold; Table1) than those evoked by close stimulation.

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Figure 7. Examples of PSPs evoked by distant (~700 µm in this example) stimulation and quantification of differences between NCB and CB stimulation. A, Examples of PSPs evoked by distant stimulation for CB (top traces) and NCB (bottom traces) stimulation. Each trace is the average of 3-5 individual responses; corresponding shades of gray represent responses from corresponding stimulus intensities as in Figure 3. The membrane potential of the neuron was adjusted to $-$ 50 mV. B, Mean differences (NCB $-$ CB) in pk_max (left), I-O $tau$ (left-center), h/l ratio (right-center) and threshold (right). Significance values are from paired, Student's t tests performed on each of the parameters from NCB stimulation versus those from CB stimulation, n = 11 neurons. C, Individual difference scores (NCB $-$ CB) from each neuron used to calculate the means in B.

Differences in these parameters between NCB and CB stimulation are summarized in Figure 7, B and C: mean difference scores(NCB $-$ CB) are shown in Figure 7B and individual difference scoresare shown in Figure 7C. The mean difference scores from PSPs evokedby distant stimulation (Fig. 7B) were qualitatively similar tothose from close stimulation (Fig. 5) for Pk_max, I-O $tau$ , and threshold,indicating that excitation was smaller with CB stimulation thanwith NCB stimulation. For the distant stimulation case, the meanh/l ratio was smaller for CB stimulation than for NCB stimulation,although the difference was not significant. This finding wasopposite to that observed for close stimulation, in which theh/l ratio was smaller for NCB stimulation. This difference inh/l ratio between distant and close stimulation was expected,as inhibition in general was weaker with distant stimulation,leading to generally larger t_1/2 values (Table 1). The positiveNCB $-$ CB difference in h/l ratio therefore probably reflects asmaller amount of late (presumably polysynaptic) excitation withCB stimulation.

Thus, the data from PSPs evoked by both close and distant stimulation support the conclusion that excitation is significantlyweaker when evoked by CB stimulation as compared with NCB stimulation.The conclusion that inhibition is also smaller with CB stimulationis strongly supported by the data from short stimulation, butcannot be effectively assayed for distant stimulation caused bythe relatively small contribution of inhibition to these PSPs.

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

In these studies, it has been demonstrated that a "representational discontinuity" or "border" between two cortical representationsin rat S1 marks a relative barrier for effective excitatory andinhibitory transmission onto supragranular neurons close to theborder. This reduction in effectiveness only depended on the synapticand local circuit properties of neurons in supragranular layers,because the reduction was observed in an in vitro preparationin which the supragranular layers were physically isolated fromdeeper cortical layers. These data indicate that the reductionof information transfer across representational borders does notsolely result from feedforward intracortical inhibition preventingthe activation of neurons across the border. On the contrary,inhibitory projections across the border are actually weaker thanthose that do not cross.

Mapping the forepaw-lower jaw border

The approximate location and orientation of the forepaw and lower jaw regions observed in this study correspond to those previouslyobserved using more detailed mapping procedures (Chapin and Lin,1984; Waters et al., 1995). The border between forepaw and lowerjaw representations was generally quite distinct. However, wealso (at least one site in ~40% of maps) observed penetrationsnear the border that responded to both forepaw and lower jaw stimulation,usually unequally. These dual-response penetrations often seemedto be associated with lighter states of anesthesia, but were alsodetected in animals that appeared to be more deeply anesthetized.Such penetrations probably reflected the use of multiunit recording,relatively high-intensity skin stimulation, and location of thesepenetrations in perigranular regions of S1 in which receptivefield sizes tend to be large (Fig. 1B), and neuronal responsestend to be higher threshold (Chapin and Lin, 1984). The maps thatwere derived were stable over the course of the mapping and markingand showed no change after iontophoretic deposition of dye. Therewas no evidence of any toxic effect of the dye or of the iontophoresisprocedure on the tissue at or near the marked sites. Thus, thetissue obtained for in vitro analysis was healthy, and appropriatecontrols demonstrated the observed effects of the border werenot an artifact of damage to or experimental alteration of thesuperficial cortex.

PSPs in marked slices

The PSPs evoked in this preparation resembled those evoked by stimulation of layer 2/3 in undercut slices from cat visualcortex (Hirsch and Gilbert, 1991), or by activation of horizontalpathways in rat motor cortex (Hess et al., 1996). These connectionsarise from layer 2/3 pyramidal neurons that form excitatory synapseslocally and at longer distances (Chapin et al., 1987; Hoeflingeret al., 1995) and from nonpyramidal neurons that form inhibitorysynapses, primarily locally (Salin and Prince, 1996). For bothexcitation and inhibition, additional polysynaptic events canbe relayed over much longer distances at longer delays (Sutorand Hablitz, 1989a,b). The PSPs shown in Figures 3, 6, and 7 clearlyexhibit these characteristics. Judged by the reversal potentialof PSCs (Fig. 4), the compound PSPs recorded were typically combinationsof EPSPs and IPSPs. At maximal stimulation, the peak of the PSPappeared to be dominated by EPSPs, because the reversal potentialwas ~0 mV (Fig. 4A), whereas the later components of the PSPswere dominated by inhibition (Fig. 4B). The amount of inhibition,however, decreased dramatically with greater stimulation distance(Fig. 7), as previously demonstrated (Salin and Prince, 1997).

Is this study, we believe that all the PSPs observed primarily reflect activation of intrinsic horizontal connections. However,the circuitry of layer 2/3 is complex; thus, the relatively largeelectrical stimuli used in this study would be expected to activatemany different circuitry elements, including horizontal connections,axon collaterals, thalamocortical terminals, and possibly theprocesses of the impaled neuron. The last two possibilities wouldbe most likely in the close stimulation category because of theclose proximity of the stimulating and recording sites. However,blocking synaptic transmission with 0 Ca²⁺ and high Mg²⁺ buffer revealed that there was negligible direct activation ofneurons, even with this close stimulation. Large contributionsby activation of thalamocortical terminals would be unlikely,because only small, isolated remnants of these terminals wouldremain after undercutting layer 2/3. Furthermore, minor directactivation of either the neuron, itself, or of thalamocorticalterminal remnants did not appear to bias our results, becausesimilar differences between PSPs evoked by NCB and CB stimulationwere observed with distant stimulation (Fig. 7) in which directactivation would be minimal.

Activation of horizontal fibers of passage and collaterals from layer 2/3 neurons undoubtedly occurred, causing antidromicactivation of more distant supragranular neurons. Thus, both CBand NCB stimulation could have activated neurons on both sidesof the border, reducing the specificity of stimulation. Nevertheless,differences in both EPSPs and IPSPs with CB versus NCB stimulationwere routinely observed, even at maximal stimulus intensities.Therefore, this nonspecific antidromic activation appears to havemade only a minor contribution to the PSPs observed.

All of the current-voltage relationships in Figure 4 are approximately linear; the presence of QX-314 in the electrode isknown to block a sodium current that is responsible for most ofthe nonlinearity in horizontally evoked EPSPs (Hirsch and Gilbert,1991) and in EPSPs evoked by white matter stimulation (Sutor andHablitz, 1989a,b), although there is some contribution of NMDAreceptor activation to the nonlinearities observed in those studies.

Anatomical and physiological correlates of the border

The border between forepaw and lower jaw representations was selected for these experiments because there is little overlapof these two representations (Chapin and Lin, 1984). In the rat,the region between the forepaw and lower jaw granular (layer 4)zones consists of an ~100-500 µm wide region of relatively agranularcortex, referred to as a perigranular or intercalated zone (Chapinand Lin, 1984; Fabri and Burton, 1991) (Fig. 1B). The granularregions are thought to reflect the termination zones of thalamocorticalafferents (Killackey and Belford, 1979; Dawson and Killackey,1987) and have been hypothesized to be analogous to primate area3b. Primarily on the basis of their physiological response properties,the perigranular and intercalated zones have been hypothesizedto be analogous to primate area 1 and 2, respectively (Chapinand Lin, 1984; Fabri and Burton, 1991). There is a relativelyclose correspondence between the cellular organization of theforepaw representation (i.e., the forepaw barrel subfield) andthe physiological map of the forepaw in the normal rat (Waterset al., 1995). Thus, there is an observable morphological borderbetween the forepaw and lower jaw representations. However, anatomicalsubstrates cannot account for the precision of the representationalborder because the transition between forepaw and lower jaw representationassayed physiologically occurs over an ~50-75 µm interval in thepentobarbital-anesthetized rat, which is much more abrupt thanthe separation between the anatomically distinct zones of theforepaw and lower jaw (separated by ~100-500 µm). Thus, thereis a clear discrepancy between the anatomical and physiologicalmaps.

There are several other anatomical substrates that do not precisely reflect functionally defined representational borders.(1) The terminals of thalamocortical axons have been shown tooverlap extensively in adult rat (Jensen and Killackey, 1987a)and primate (Garraghty et al., 1989; Garraghty and Sur, 1990;Rausell and Jones, 1995). In the cat (Landry and Deschenes, 1981;Snow et al., 1988) and primate (Rausell and Jones, 1995) thisoverlap can span representational borders. (2) The basilar dendritesof supragranular neurons in perigranular zones of rat S1 can extendup to 500 µm into adjacent granular zones (Chapin et al., 1987).(3) Intracortical horizontal projections extend for long distancesthroughout the cortex. These projections extend locally for ~500-600µm in all regions and for longer distances (millimeters) particularlywithin and between perigranular and dysgranular regions. However,the relative density of these horizontal connections is not uniform:injections of anterograde and retrograde tracers into rat S1 typicallyyield a "halo" of short range (approximately <500 µm) horizontalprojections which have a relatively even radial distribution.At longer distances, the density of horizontal connections withina cytoarchitectonic region is greater than the density betweensuch regions (Chapin et al., 1987; Fabri and Burton, 1991; Hoeflingeret al., 1995). Overall, it is not surprising that subthresholdEPSPs can be detected for inputs that cross representational boundaries(Zarzecki et al., 1993; Istvan and Zarzecki, 1994; Li and Waters,1996).

Corticocortical projections of parietal regions of neocortex terminate in discrete columns or bands in rats (Isseroff et al.,1984) and primates (Jones et al., 1975). Such columnar organizationhas been suggested to be a distinctive feature of cortical functionaland anatomical organization (Mountcastle, 1997). Surprisingly,the widths of these columns are approximately equal across species(~400-750 µm). The precise relationship of these columns withthe physiological borders between representations is not certain,although previous studies in rat suggest that perigranular orintercalated regions in S1 may correspond to the width of a column(Chapin and Lin, 1987), implying that our borders would generallybe near the center of a column. Therefore, our close stimulationcategory would most likely be within the same column as the impaledneuron, and would thus strongly activate intrinsic intracolumnarconnections, as well as some longer-range intercolumnar connections.Our distant stimulation category suggests that the effects ofthis representational border also apply to intercolumnar horizontalconnections, as well.

The relative weakness of excitation across representational borders could be because: (1) cross-border excitation is too weakto cause neurons to reach firing threshold; (2) cross-border inhibitionprevents neurons from reaching threshold; or (3) both of theseprocesses occur. Our data support the first of these possibleexplanations, that cross-border excitation is weaker than excitationwithin a representation. The data in Figures 3, 5 and 7, and inTable 1 clearly show that the Pk_max, I-O $tau$ , and threshold aresmaller for CB stimulation. Because these parameters primarilyreflect activation of EPSPs (Fig. 4), net cross-border excitationis weaker than same-side excitation. No evidence was found forstronger inhibition with CB stimulation. In fact, monosynapticIPSPs were smaller in amplitude and shorter in duration (Fig.6, Table 2) for CB stimulation. Furthermore, with close stimulationin which a significant amount of inhibition was activated, theh/l ratio was larger with CB stimulation, reflecting a smallercontribution of later IPSPs to the PSPs evoked by stronger stimuli.Our data only apply to corticocortical connections, because thalamocorticalprojections were severed by the cut in layer 4 (Fig. 2A). Thus,it is possible that feedforward inhibition driven by thalamocorticalprojections could drive cross-border inhibition and further contributeto the suppression of EPSPs in the intact animal.

Our data are consistent with and do not differentiate between there either being a smaller number of excitatory and inhibitoryprojections that cross the border, or that the synapses that thesecross-border projections make are weaker than those made by noncross-borderprojections, or both. Because the density of horizontal projectionstends to be greater within as opposed to between representations,the first alternative would seem likely. However, over the distancesbetween stimulating and recording used in these studies for closestimulation (<300 µm), horizontal projections are quite evenlydistributed (Chapin et al., 1987; Fabri and Burton, 1991; Hoeflingeret al., 1995). Further studies are necessary to resolve theseissues.

This in vivo and in vitro preparation provides a novel system in which to study the basic cellular and synaptic events thatunderlie the establishment of dynamic representational bordersand their plasticity. Clear correlates of a representational bordercan be detected at the level of single cortical neurons by comparingthe responses of intracortical connections that must cross a representationalborder to those that do not. By examining these cellular propertiesin relation to a representational border that has been reorganizedby some peripheral manipulation, we hope to further probe thebasic mechanisms that are responsible for representational plasticityof the cortex.

  FOOTNOTES

Received June 4, 1997; revised Feb. 26, 1998; accepted March 23, 1998.

This work was supported by National Institutes of Health Grants NS10414 and NS09859. We thank Drs. E. Ahissar, D. V. Buonomano,and P. A. Steen for helpful comments on various versions of thismanuscript.
Correspondence should be addressed to Peter W. Hickmott, Keck Center for Integrative Neuroscience, University of California,San Francisco, P.O. Box 0732, San Francisco, CA 94143.