Functionally Independent Columns of Rat Somatosensory Barrel Cortex Revealed with Voltage-Sensitive Dye Imaging

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The Journal of Neuroscience, November 1, 2001, 21(21):8435-8446

Functionally Independent Columns of Rat Somatosensory Barrel Cortex Revealed with Voltage-Sensitive Dye Imaging
Carl C. H. Petersen and Bert Sakmann
Department of Cell Physiology, Max-Planck-Institute for Medical Research, Heidelberg D-69120, Germany

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Whisker movement is somatotopically represented in rodent neocortex by electrical activity in clearly defined barrels, whichcan be visualized in living brain slices. The functional architectureof this part of the cortex can thus be mapped in vitro with respectto its physiological input and compared with its anatomical architecture.The spatial extent of excitation was measured at high temporalresolution by imaging optical signals from voltage-sensitive dyeevoked by stimulation of individual barrels in layer 4. The opticalsignals correlated closely with subthreshold EPSPs recorded simultaneouslyfrom excitatory neurons in layer 4 and layer 2/3, respectively.Excitation was initially (<2 msec) limited to the stimulated barreland subsequently (>3 msec) spread in a columnar manner into layer2/3 and then subsided in both layers after ~50 msec. The lateralextent of the response was limited to the cortical column definedstructurally by the barrel in layer 4. Two experimental interventionsincreased the spread of excitation. First, blocking GABA_A receptor-mediatedsynaptic inhibition caused excitation to spread laterally throughoutwide regions of layer 2/3 and layer 5 but not into neighboringbarrels, suggesting that the local excitatory connections withinlayer 4 are restricted to single barrels and that inhibitory neuronscontrol spread in supragranular and infragranular layers. Second,NMDA receptor-dependent increase of the spread of excitation wasinduced by pairing repetitive stimulation of a barrel column withcoincident stimulation of layer 2/3 in a neighboring column. Suchplasticity in the spatial extent of excitation in a barrel columncould underlie changes in cortical map structure induced by alterationsof sensoryexperience.

Key words: neocortex; somatosensory cortex; barrel cortex; imaging; voltage-sensitive dye; plasticity

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The rodent somatosensory barrel cortex provides a unique opportunity to identify specific cortical locations in brain slicepreparations. Each whisker is represented in the neocortex bya barrel that can be visualized at high resolution in the livingbrain slice (Woolsey and Van der Loos, 1970; Agmon and Connors,1991; Petersen and Sakmann, 2000). The local neocortical neuronalnetwork can thus be investigated in vitro within the context ofa well defined somatotopic map. A comparison of data obtainedfrom in vitro and in vivo recordings may delineate the exact contributionof different neuronal ensembles to the in vivoresponse.

The spatiotemporal structure of whisker-evoked responses was initially inferred by repeated measurements of extracellularunit recordings (Armstrong-James et al., 1992). These measurementssuggested that cortical responses to single whisker deflectionswere initiated in a single barrel in layer 4 and then spread verticallyin a columnar manner into layer 2/3. At longer latencies, excitationwas recorded in neighboring columns. Simultaneous recordings frommultiple sites over the barrel cortex region with a multielectrodearray confirmed the initial excitation of a single barrel, followedby spread to neighboring barrels (Petersen and Diamond, 2000).The spatial resolution of extracellular unit recordings is low,and they do not measure subthreshold responses. Higher spatialresolution (but without temporal resolution) single whisker responseshas been obtained from 2-deoxyglucose uptake studies (Durham andWoolsey, 1977; Kossut et al., 1988; McCasland and Woolsey, 1988)and optical imaging of intrinsic reflectance changes of the corticalsurface (Masino and Frostig, 1996). An alternative approach isto image neuronal activity with voltage-sensitive dyes, whichcan record both the spatial and temporal structure of layer 2/3responses with high resolution. In such optical recordings, aneven larger area of cortex appears to be excited by stimulationof a single whisker (Orbach et al., 1985; Kleinfeld and Delaney,1996). Large single whisker subthreshold receptive fields havealso been reported with whole-cell voltage recordings from neuronsin layers 2-5 (Moore and Nelson, 1998; Zhu and Connors, 1999).The functional response of a large area of neocortex after singlewhisker stimulation appears to be at odds with the apparent anatomicalprecision of the wiring from single whiskers to single layer 4barrels.

To investigate the spatiotemporal dynamics of neocortical responses under more controlled conditions, we stimulated singlebarrels in vitro and imaged voltage-sensitive dye signals at highresolution. Unlike responses to single whiskers in vivo, stimulationof a single barrel evoked a response primarily limited to thewidth of a single barrel. The spread of excitation, although invariantunder many manipulations, could however be expanded by blockadeof GABA_A-mediated inhibition. The lateral extent of layer 2/3responses could also be expanded in an NMDA receptor-dependentmanner by pairing stimulation of a barrel column with stimulationof layer 2/3 in a neighboring column, a process that could underliemap plasticity induced by alterations in sensoryexperience.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Preparation of slices of somatosensory barrel cortex. Wistar rats (13-15 d old) were decapitated under deep halothane anesthesia.The brain was rapidly removed and placed in ice-cold extracellularmedium. One of three types of slices was subsequently prepared.The majority of experiments were performed on 350-µm-thick thalamocorticalslices prepared following the description of Agmon and Connors(1991), with modifications (Petersen and Sakmann, 2000). Otherexperiments were performed on 350-µm-thick slices cut to revealthe five rows (A-E) of the posterior medial barrel subfield followingthe description of Finnerty et al. (1999). The response propertiesof these two types of paracoronal slices were not different. Additionally,some experiments were performed on 250-µm-thick slices cut tangentialto the pia at a depth such that the slices contained layer 4 barrelsas described by Fleidervish et al. (1998). Slices were cut bya vibratome in ice-cold extracellular medium and were subsequentlyincubated at 35°C for 15-30 min after slicing. The slices werethen transferred to room temperature (20-23°C) until requiredfor analysis. Throughout the procedure, slices were maintainedin extracellular medium containing (in mM): 125 NaCl, 25 NaHCO₃,25 glucose, 2.5 KCl, 1.25 NaH₂PO₄, 2 CaCl₂, and 1 MgCl₂ (bubbledwith 95% O₂ and 5% CO₂).

Optical recording of voltage-sensitive dye signals. Slices were incubated at room temperature in extracellular medium with0.1 mg/ml RH155 (Molecular Probes, Eugene, OR) for 15-30 min asdescribed by Laaris et al. (2000). Slices were washed for 15 minin the experimental chamber before use to remove unbound dye.All experiments were performed at 35°C. Glass microelectrodes(similar to those used for whole-cell patch-clamp recordings,although slightly larger in tip diameter) were filled with extracellularmedium to form an extracellular stimulating electrode. Constantamplitude current pulses (200 µsec, 10-100 µA) were deliveredwith an A365 stimulus isolator (World Precision Instruments, Sarasota,FL). For slices cut normal to the pia, the tip of the stimulatingelectrode was placed at the bottom of layer 4 in the center ofa visually identified barrel. For tangential slices, the stimulatingelectrode was placed in the middle of a barrel. The slice wasilluminated with light of 700 ± 25nm wavelength (Omega Optical,Brattleboro, VT) and viewed with a Zeiss 10× water immersion lensgiving a field of view of 775 µm. Quantitative optical recordingsof changes in light transmission were made with the Deltaron HR1700(Fuji, Tokyo, Japan), which consists of an array of 128 × 128detectors; thus, each pixel receives light from a 6 × 6 µm regionof the slice. In experiments of the type shown in Figures 8 and9, a larger field of view was imaged by using a 0.5× C-mount adaptor,and, in these cases, each pixel received light from a region of12 × 12 µm. Evoked changes in light transmission measured withthis voltage-sensitive dye at low stimulation intensities were<0.1%. These small changes in light intensity could be well resolvedwith a time resolution of 0.6 msec per frame with the differentialgain of the Deltaron HR1700 camera set in the range between 60and 1000. To reduce noise, 16 consecutive stimuli were averagedwith each stimulus separated by an interval of 5 sec. Image datawere analyzed off-line by custom-written routines in IgorPro (WaveMetricsInc., Lake Oswego, OR). Differential images were divided by theprestimulus image, and voltage-sensitive dye signals are thuspresented as fractional changes in lightintensity.

Whole-cell recording of membrane potential. Simultaneous whole-cell patch-clamp recordings were established with excitatoryneurons of layer 2/3 and layer 4 using Axopatch 200 amplifiers(Axon Instruments, Foster City, CA). Whole-cell recordings wereestablished using pipettes with resistances of 5 M $Omega$ filled witha solution containing (in mM): 130 potassium gluconate, 10 sodiumgluconate, 10 HEPES, 10 phosphocreatine, 4 NaCl, 4 MgATP, and0.3 Na₃GTP, adjusted to pH 7.2 with KOH. Biocytin (3 mg/ml) wasroutinely included in the intracellular solution. Excitatory neuronsin layer 2/3 were easily distinguished by the prominent apicaldendrite and pyramidal shape of somata. Within layer 4, excitatoryneurons had small round somata and were often found in clusters.These neurons were further identified as excitatory based on theirregular firing patterns to depolarizing current and broad actionpotentials (APs) (~1 msec half-width). Electrophysiological datawere collected simultaneously with the optical voltage-sensitivedye imaging, and thus 16 consecutive sweeps of extracellular stimulationwere also averaged for these electrical recordings. Data wereanalyzed and aligned with optical recordings using custom writtenroutines inIgorPro.

Morphological reconstruction of biocytin stained neurons. After filling neurons with biocytin, slices were fixed overnightat 4°C in 4% paraformaldehyde. The slices were washed with PBS(100 mM sodium phosphate, pH 7.2) five times over a period of2 hr. Endogenous peroxidases were then quenched by a 5 min incubationwith 1% H₂O₂. The slices were subsequently rinsed in PBS fivetimes over a period of 2 hr. Slices were conjugated with avidin-biotinylatedhorseradish peroxidase following the instructions of the manufacturer(ABC-Elite, Vector stains; Vector Laboratories, Burlingame, CA).Slices were then washed five times over a period of 2 hr withPBS, and subsequently biocytin-stained neurons were visualizedunder a reaction with 0.5 mg/ml DAB and 0.01% H₂O₂. When the neuronalprocesses were clearly visible, the reaction was stopped by washingwith PBS. Finally, the slices were mounted on slides using mowiol.Axonal and dendritic processes were subsequently reconstructedin three dimensions using Neurolucida software (MicroBrightFieldInc., Colchester,VT).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Voltage-sensitive dye signals report the spatiotemporal pattern of subthreshold EPSPs

Simultaneous recording of voltage-sensitive dye signals and whole-cell membrane potential
Field stimulation with a large-diameter patch electrode filled with extracellular solution placed in the lower center of alayer 4 barrel (Fig. 1A) evoked responses that could be detectedby both voltage-sensitive dye imaging and membrane potential recordingsfrom excitatory neurons. Slices were stained with the voltage-sensitivedye RH155, which inserts into the outer leaflet of cell membranesand changes the degree of absorption of light at 700 nm dependingon the potential across the membrane in which it is attached.The camera thus detects a bright-field image of the slice (Fig.1A) on which small fractional changes in transmission of the orderof 0.1% are spatially resolved in response to the field stimulus(Fig. 1D). Each pixel in the camera collected light from a regionof 6 × 6 µm, and image frames were captured at 0.6 msec intervals(Fig. 1F). The time course and relative amplitudes of voltage-sensitivedye signals quantified in regions of 50 × 50 µm around the whole-cellrecording electrodes in layer 2/3 and layer 4 were similar tothe evoked subthreshold EPSPs (Fig. 1E). Biocytin was routinelyincluded in the whole-cell pipette solution to identify the dendriticand axonal arborizations of the layer 4 and layer 2/3 excitatoryneurons in the context of the layer 4 barrel structure (Fig. 1B)and reconstructed in three dimensions (Fig. 1C).

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Figure 1. Experimental setup for simultaneous whole-cell and voltage-sensitive dye recording. A, Bright-field image of somatosensory barrel cortex from a slice stained with RH155. Dark regions correspond to the layer 4 barrels, which are outlined in cyan. Two whole-cell recording pipettes are visible, one in layer 2/3 and the other in layer 4. A large-diameter patch pipette filled with extracellular solution is used for field stimulation, with the tip positioned at the bottom of the central barrel. B, The excitatory neurons are filled with biocytin during the whole-cell recordings, allowing their structure to be visualized after fixation and staining. C, Reconstruction of the biocytin-filled layer 2/3 pyramidal neuron (red dendrite and blue axon) and the layer 4 spiny stellate (black dendrite and green axon). D, A single unfiltered differential image normalized to the bright-field transmitted light ( $Delta$ I/I₀) of the voltage-sensitive dye signal taken 12 msec after stimulation. E, Time course of voltage-sensitive dye responses (top traces) compared with the simultaneously obtained whole-cell recordings (bottom traces). The voltage-sensitive dye signals were quantified from an area of 50 × 50 µm around the location of the neurons from which the whole-cell recordings are made (layer 2/3 red traces and layer 4 blue traces). F, Optical arrangement for simultaneous whole-cell recordings and voltage-sensitive dye recordings. The slice is illuminated with 700 nm light from a halogen lamp and viewed with a 10× water immersion lens. The slice is stained with voltage-sensitive dye RH155, which increases its absorption of 700 nm light when membranes are depolarized. Small changes in the amount of light transmitted through the slice can be recorded with a Fuji Deltaron camera. With a square field of view of 775 µm obtained under these conditions, each pixel covers a region of 6 × 6 µm, and each frame has 0.6 msec duration.

Pharmacological characterization of voltage-sensitive dye signals
In the absence of voltage-sensitive dye, no changes in light transmission could be evoked; thus, the entire recorded signalis attributable to the response of the voltage-sensitive dye RH155.No phototoxicity was apparent with the use of the dye at the concentrationsand illumination intensities used in this study as assessed byresting membrane potential, AP discharge patterns, and membranepotential changes evoked by field stimulation. Optically detectedsignals were blocked by 1 µM TTX bath application (normalizedsignal amplitude at 12 msec was $-$ 0.04 ± 0.04; n = 8), suggestingthat the voltage-sensitive dye signals are entirely dependenton AP generation and conduction. Removal of extracellular Ca²⁺ or blockade of glutamatergic synaptic transmission by 10 µM NBQXand 100 µM D-APV reduced the peak signal amplitude quantifiedacross the entire field of view to similar extents [0.22 ± 0.08(n = 8) for NBQX and APV; 0.21 ± 0.08 (n = 8) for nominally Ca²⁺-free artificial CSF]. Thus, >80% of the voltage-sensitive dyesignal is attributable to the action of synaptically releasedglutamate (Yuste et al., 1997; Higashi et al., 1999; Laaris etal., 2000). The remaining 20% of the signal had a time coursesimilar to that without pharmacological manipulation and presumablyreflected direct activation of neuronal membrane near the stimulatingelectrode. Whole-cell voltage recordings made simultaneously suggestedthat the stimulation artifact was strongly enhanced during blockadeof glutamatergic transmission, showing a component with a decaytime course similar to evoked EPSPs. The larger stimulation artifactin the presence of NBQX and APV presumably results from the increasedmembrane resistance attributable to block of glutamate receptors,thus giving larger responses to the extracellular current injection.Removal of divalent cations increases membrane excitability, andsuch an effect may also account for the surprisingly large signalremaining in nominally Ca²⁺-free medium. The changes in membrane excitability complicatethe pharmacological dissection of the voltage-sensitive dye signalbut give the lower bound estimate that at least 80% of the dyesignal is caused by synaptically released glutamate acting ationotropic receptors and generating dendritic EPSPs. In supportof a major postsynaptic component to voltage-sensitive dye signals,Laaris et al. (2000) found that the removal of extracellular calciumwas able to completely block neocortical signals evoked by stimulationof the thalamus, with the remote stimulation site in these experimentspreventing direct activation of dendrites

Anatomy of a "normalized barrel"
Field stimulation is thought to result in the preferential excitation of axons rather than dendrites. To gain an understandingof the anatomy of some of the stimulated fibers, the axonal anddendritic arborizations of 18 layer 2/3 and layer 4 neurons werereconstructed within the context of the borders of a barrel inlayer 4. To compare the arborizations of neurons from differentexperiments, both the horizontal and vertical dimensions werenormalized. The horizontal widths of the layer 4 barrels werenormalized to each other (mean barrel width, 310 µm; range, 170-435µm), but the relative positions of the neuronal somata and barrelboundaries were maintained. The vertical dimensions were normalizedusing the pia and the layer 4/5 boundary as the fixed points (meandistance from pia to layer 4/5 boundary, 810 µm; range, 735-900µm). The normalized reconstructions of 18 excitatory layer 2/3neurons and 18 excitatory layer 4 neurons were superimposed inthe context of the barrel boundaries (Fig. 2). A field stimulusat the base of a layer 4 barrel is likely to primarily activatethalamocortical axons and axons of the layer 4 neurons, whichform a very dense network in this region. The axons from pyramidalneurons in layer 2/3 and layer 5/6 are present at a much lowerdensity at the base of a layer 4 barrel and are likely to makeonly a small contribution to evoked responses. Previous studieshave shown that individual thalamocortical axons primarily innervatesingle layer 4 barrels (Jensen and Killackey, 1987). The axonalarborization of layer 4 spiny stellate and star pyramidal neuronsis likewise primarily horizontally confined to individual barrels(Harris and Woolsey, 1983; Lorente de Nó, 1992; Bernardo et al.,1990; Lübke et al., 2000; Petersen and Sakmann, 2000). The responseobserved at the shortest latencies in both voltage-sensitive dyerecordings and whole-cell recordings (Figs. 1, 3) is thus likelyto result from the postsynaptic action of glutamate released fromthalamocortical and layer 4 axons acting on ionotropic glutamatereceptors located on the dendrites of layer 4 neurons. Each layer4 axon forms excitatory connections with approximately one-thirdof the excitatory neurons within its home barrel, with a meanEPSP amplitude of ~1 mV (Petersen and Sakmann, 2000). It wouldthus appear that, to evoke EPSPs averaging ~5 mV (Figs. 1, 3)in the excitatory layer 4 neuronal network, APs are required in<20 presynaptic neurons. An AP with an amplitude of ~100 mV anda duration of ~1 msec can only give a small signal compared withthat resulting from the released glutamate of the same AP, whichevokes a mean depolarization of ~1 mV in one-third of the severalthousand neighboring layer 4 neurons and lasting ~50 msec. Fromsuch calculations, it becomes apparent why the voltage-sensitivedye signal predominantly reports subthreshold membrane depolarizationrather than evoked APs.

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Figure 2. Morphology of excitatory neurons of layer 2/3 and layer 4 within a barrel column. A, Excitatory neurons were filled with biocytin during whole-cell recordings and subsequently stained. Axonal and dendritic arbors were reconstructed in three dimensions for 18 layer 2/3 and 18 layer 4 excitatory neurons. Two-dimensional projections into the original plane of the slice are illustrated from the pia to a depth including layer 5A. The dimensions of the reconstruction of each neuron are normalized with respect to the pia, bottom of layer 4, and the lateral width of the layer 4 barrel, thus generating a representation of a normalized barrel column. Layer 2/3 pyramidal neurons are shown with red dendrite and blue axon. Layer 4 spiny stellate neurons are shown with black dendrite and green axon. The scale bar represents the mean normalization length. B, The same reconstructed neurons are shown with the dendritic and axonal compartments separated. The layer 4 dendrites are primarily confined to the layer 4 barrel. The layer 4 axon forms an ascending column of input to the layer 2/3 pyramidal neurons. The major lateral spread of neuronal arborization derives from the axons of the layer 2/3 pyramids.

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Figure 3. Correlation of voltage-sensitive dye signal with dual whole-cell recordings of membrane potential. A, Bright-field image of somatosensory barrel cortex from a slice stained with RH155. Dark regions correspond to the barrels. Two whole-cell recording pipettes are visible, one in layer 2 (blue box) and one in layer 4 (red box). The extracellular stimulation electrode is visible at the bottom of the micrograph at the border of layer 4 and 5 in the middle of a barrel. The time series of pictures indicates the optical response of the voltage-sensitive dye after stimulation at 0 msec. The images were collected with 0.6 msec exposure time and are presented without filtering or averaging. Excitation can be observed to spread gradually from layer 4 to layer 2/3, maintaining a strict columnar excitation. Scale bar, 100 µm. B, Comparison of optical responses quantified from the 60 × 60 µm boxes indicated in A. Blue, layer 2/3; red, layer 4, with the membrane potential response of two individual neurons located within the boxes from which simultaneous whole-cell recordings were made. Three stimulus strengths are compared. As stimulus strength is increased, both the optical and the whole-cell responses increase in amplitude in a similar manner. Equally, the latency of responses in both layer 2/3 and layer 4 is similar in optical and whole-cell recordings. The decay kinetics are also similar, although in this example the voltage-sensitive dye signal decays somewhat slower. C, The amplitude of responses to the highest stimulation strength in an experiment was used to normalize the response to less intense stimuli and the relative response amplitude detected optically in a region 60 × 60 µm surrounding the soma of neurons from which the whole-cell recordings were made. The linear fit suggests a good correlation between the amplitudes of voltage signals detected optically and by whole-cell recordings. D, The latency to half-maximal response of recordings is greater in layer 2/3 (blue squares) than in layer 4 (red circles), as measured both optically and by whole-cell recordings. The dye latency, however, is somewhat slower than the latency determined by whole-cell recordings.

The layer 4 axons project in a columnar manner into layer 2/3 (Lübke et al., 2000), defining a "barrel column" and formingexcitatory contacts predominantly onto the basal dendrites ofpyramidal neurons (Feldmeyer et al., 1999). The axonal arborizationsof these layer 2/3 pyramidal neurons are not confined to the barrelcolumn structure, and although the densest axonal arborizationsare close to the soma, there are numerous collaterals that spreadhorizontally for long distances (Fig. 2). Depending on the degreeof functional activation of these layer 2/3 pyramidal neurons,they could propagate signals across different barrel columns.These anatomical reconstructions give a static representationof the excitatory neuronal network with which we can compare thefunctional spatiotemporal spread of excitation monitored withvoltage-sensitive dye imaging. Not included in this anatomicalreconstruction of a "normalized barrel" are inhibitory neurons,which are likely to regulate the degree of activity of the excitatoryneurons. The voltage-sensitive dye signals will thus differ inat least two respects from the anatomical representation. First,they will report the time course of excitation in the neuronalnetwork, and second, the voltage-sensitive dye signal will includethe effects of inhibition. Furthermore, the anatomical reconstructionof the barrel column is deduced from a selected population ofneurons from which whole-cell recordings were made. It is unknownhow well these neurons represent the ensemble local neuronal networkswithin the entire depth of the slice from which the voltage-sensitivedye signal isderived.

Spatiotemporal correlation of optical signals with simultaneous whole-cell membrane potentials
Stimulation of a slice at the lower center of a layer 4 barrel evoked voltage-sensitive dye signals initiated in layer 4,which subsequently spread to layer 2/3 (Fig. 3). To correlatethe time course and amplitude of the optically detected signals,dual whole-cell recordings were made simultaneously from excitatoryneurons in layer 4 and layer 2/3, respectively. Coincident withthe current injection (200 µsec, 10-100 µA), a small stimulationartifact appeared in both electrical and optical signals. Thissignal was small and of very short duration (a single frame of0.6 msec duration in the imaging) and was ~0.5 msec duration inwhole-cell voltage recordings. The stimulus signal was also highlylocalized in the imaging experiments to within an ~50 µm radiusof the stimulating electrode. After a latency of ~1 msec, bothoptical and membrane voltage of layer 4 neurons revealed depolarizingsignals. The latency for half-maximal responses in layer 4 was2.0 ± 0.2 msec (n = 10) measured optically, whereas the latencywas 1.5 ± 0.1 msec (n = 10) for whole-cell voltage recordings.The voltage-sensitive dye signal subsequently propagated verticallyinto layer 2/3, and EPSPs were simultaneously observed in voltagerecordings of layer 2/3 pyramidal neurons. The latency to thehalf-maximal optical signal was 3.4 ± 0.1 msec (n = 10) comparedwith 2.8 ± 0.1 msec (n = 10) in voltage recordings. The peak amplitudesof voltage-sensitive dye and membrane potential signals were similarin layer 2/3 and in layer 4. By varying the stimulation strength,we could correlate the changes in voltage-sensitive dye signaland evoked EPSPs. The amplitudes changed in a linearly correlatedmanner both comparing layer 4 and layer 2/3 and comparing opticaland whole-cell voltage recordings (Fig. 3B). Equally, the decayphase of optical and whole-cell voltage recordings appeared qualitativelysimilar [in some experiments, the voltage-sensitive dye signaldecayed more slowly (Fig. 3B), but in other experiments the electricalresponse decayed more slowly (see Fig. 6B)]. The normalized correlationof the peak amplitude of signals recorded in all experiments betweenoptical and voltage recording (Fig. 3C) shows a slope very closeto unity [wc = 1.02 * vsd $-$ 0.04; r² = 0.87; n = 10 (wc indicates whole-cell recording, and vsd indicatesvoltage-sensitive dye signal)]. The latency correlation (Fig.3D) also appears to be linear, although the dye signal latencywas longer (wc = 0.70 * vsd + 0.26; r² = 0.77; n =10).
These correlations between the time course and amplitude of the two types of signals appear remarkably close considering thatthe neurons from which the whole-cell recordings were made representa minute fraction of the population of the cell membrane areafrom which the voltage-sensitive dye signals are derived. Thevoltage-sensitive dye signal is thus able to resolve the spatiotemporalstructure of small subthreshold EPSPs in ensembles of many neuronsevoked by fieldstimulation.

Spatial extent of voltage-sensitive dye signals in relationship to anatomical barrel boundaries

Barrel boundaries can be visualized at high resolution in living brain slices (Petersen and Sakmann, 2000), allowing the spatialextent of the voltage-sensitive dye signal to be analyzed withreference to the anatomy of barrel cortex. From Figures 1 and3 it is clear that the predominant spread of excitation is limitedhorizontally to the width of the layer 4 barrel, which is clearlydistinguishable in the bright-field image. To analyze the lateralspread of excitation with respect to barrel boundaries more rigorously,the borders were measured quantitatively by fitting sigmoidalcurves to intensity plots of transmitted light within layer 4in bright-field images (Petersen and Sakmann, 2000). The borderwas defined as the location with the half-maximal intensity ofbright field transmitted light, leaving a septal area betweenneighboring barrels averaging ~100 µm in width. The superimposedlateral limits of layer 4 barrels (Fig. 4A, cyan) correspond tothis definition, and the evoked voltage-sensitive dye signal aroundthe peak of the response at 12 msec is shown with and withoutthe barrel boundaries superimposed. The voltage-sensitive dyesignal is narrowest in layer 4 and broader in both layer 2/3 andlayer 5. Only small signals are detected in neighboring barrelsat this time point, and, in addition, it appears that the largestdrop in signal amplitude occurs at the barrel boundaries. Thetime dependence of the signal at different locations within layer4 is indicated in the bottom right panel of Figure 4A. Large signalsare detected within the layer 4 barrel with nearly equal amplitudeacross the barrel. The signal in the septum dividing neighboringbarrels is strongly reduced in amplitude, and only small signalsare detected in the neighboring barrel. The largest signal inthe neighboring barrel appears after a significantly longer latency.Averaged over many experiments (n = 11), the latency for half-maximalsignals in the stimulated barrel was 2.0 ± 0.2 msec; for layer2/3, latency was 4.0 ± 0.2 msec, and for the nearest neighborlayer 4 barrel, the latency measured 10.6 ± 3.2 msec (measuredat the same distance from the stimulation electrode as the layer2/3 latency). The small signal that can be detected in neighboringbarrels thus presumably results from polysynaptic excitation.The spatial extent of voltage-sensitive dye signals at 12 msecafter stimulation normalized across experiments (n = 11) and alignedsuch that the origin occurs at the barrel boundary (Fig. 4B) indicatesa sharp drop in amplitude at the septum. A sigmoidal curve fittedto the data has a half-maximal value at 1 µm inside the home barreland 80%-20% transition length of 101 µm. Also indicated in Figure4B are the corresponding measurements for the lateral spread ofvoltage-sensitive dye signals in layer 2/3 at 12 msec after thestimulus. The voltage-sensitive dye signal in layer 2/3 also dropsin amplitude near the barrel border but it is shallower, and,importantly, >10% of the maximal signal spreads 200 µm outsidethe stimulated barrel (sigmoidal fit to the data gives a half-maximalvalue at 10 µm outside the home barrel and 80%-20% transitionlength of 131 µm). Thus, within layer 2/3, there is considerableoverlap of voltage-sensitive dye signals from neighboring barrelcolumns but very little within the barrels of layer 4. Additionalevidence that the determinant of the width of the voltage-sensitivedye signal in layer 4 is the anatomical barrel structure comesfrom the linear dependence between the bright-field barrel widthand the width at half-maximum of the voltage-sensitive dye signal(vsd width = barrel width * 0.83 + 43; r² = 0.64; n = 11) (Fig. 4C).

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Figure 4. Voltage-sensitive dye responses within layer 4 are primarily confined to the stimulated barrel and associated cortical column. A, Bright-field micrograph (top left) of the region of barrel cortex imaged with the voltage-sensitive dye. Cyan boxes indicate extent of individual barrels, and the stimulation electrode is visible in the center of the barrel at the layer 4/5 border. Images of the peak voltage-sensitive dye signal (12 msec after stimulation) without (top right) and with (bottom left) barrel demarcation. The optical responses at the locations indicated by dots in the top left panel are plotted (bottom right), with responses from within the stimulated barrel colored blue, from the septum in green, and from the neighboring barrel in red. The spatial extent of the response decays rapidly outside of the stimulated barrel, with very little response at short latencies detected in neighboring barrels. A small response can, however, be detected late in the neighboring barrels. Scale bar, 100 µm. B, The normalized spatial extent of the optical dye signal within layer 4 (red curve) measured at 12 msec after stimulation is confined to the stimulated barrel (barrel septum shown in black, with half-maximal barrel boundary at 0 µm). The black superimposed curve is a sigmoidal fit, with half-maximal value at $-$ 1.09 µm and a length constant of 36.4 µm. The spatial extent of the associated signals in layer 2/3 is plotted in blue, indicating that, although the response is more diffuse, it also shows a marked decay over similar distances with half-maximal value at 9.85 µm and a transition length of 47.3 µm. However, >10% of the signal remains 200 µm outside of the stimulated barrel. C, The full-width at half-maximum of the voltage-sensitive dye signal shows a close correlation with the anatomically defined width of the barrels stimulated.

To resolve the lateral borders of barrels in two dimensions, tangential slices containing layer 4 were prepared followingthe description of Fleidervish et al. (1998). These slices allowthe lateral extent of voltage-sensitive dye signals to be correlatedin two dimensions with the barrel structure. In particular, itappeared to be a stringent test of our hypothesis that the globalshape of the voltage-sensitive dye signal at times when it islargest should match that of the anatomical barrel structure.Barrels can have many shapes and sizes, and, in all cases tested,the outline of the barrel in the bright-field image could alsobe recognized in the voltage-sensitive dye signal at its largestsize (n = 12) (an example is shown in Fig. 5A). Unlike paracoronalslices, the small response that can be detected in neighboringbarrels does not occur with a much longer latency to the mainresponse in the stimulated barrel (Fig. 5A), which could resultfrom the inclusion of a small part of layer 2/3 or layer 5 inthe tangential slice preparation. However, the major decreasein the spatial profile of the voltage-sensitive dye signal wasagain observed to occur at the barrel boundaries (Fig. 5B, vsdresponse at 12 msec after stimulation). The profile was fittedwith a sigmoidal curve with a half-maximal value at 6 µm outsidethe barrel and 80%-20% transition length of 89 µm, in close agreementwith the data from the paracoronal slices. Furthermore, the widthat half-maximal of the voltage-sensitive dye signal depended linearlyon the width of the barrel quantified across a central regionof each barrel (vsd width = barrel width * 0.92 + 27; r² = 0.87; n = 12) (Fig. 5C).

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Figure 5. Barrel cortex slices cut tangential to the pia containing only layer 4 indicate that excitation is confined to the stimulated barrel. A, Bright-field micrograph (top left) of the region of tangentially sliced barrel cortex imaged with the voltage-sensitive dye. Cyan outline indicates the extent of the stimulated barrel with the stimulation electrode visible in the center. Images of the peak voltage-sensitive dye signal (12 msec after stimulation) without (top right) and with (bottom left) barrel demarcation. The optical responses at the locations indicated by dots in the top left panel are plotted (bottom right), with responses from within the stimulated barrel colored blue, from the septum in green, and from the neighboring barrel in red. The spatial extent of the response decays rapidly outside of the stimulated barrel with very little in neighboring barrels. The shape of the optical dye response matches closely the shape of the barrel viewed in bright-field microscopy. Scale bar, 100 µm. B, Quantification of the spatial extent of the voltage-sensitive dye signal with respect to the barrel border at 0 µm (red line indicates septum). The voltage-sensitive dye signal is fitted with a sigmoidal curve, with half-maximal value at 6 µm and length constant 32 µm. C, The full-width at half-maximum of the voltage-sensitive dye signal shows a close correlation with the width of the stimulated barrels, as defined by bright-field microscopy.

Modifying the spread of excitation

Having defined the dynamic pattern of the spread of the predominantly subthreshold excitation in a column of the barrel cortexafter single stimuli under control conditions, we investigatedpossible ways of altering the spatiotemporal spread ofexcitation.

Role of GABAergic inhibition in limiting spatiotemporal spread of voltage-sensitive dye signals
Inhibition mediated by synaptic release of GABA could be responsible for the limited lateral extent of excitation in a barrelcolumn. To test this hypothesis, GABA_A receptor-mediated inhibitionwas blocked by addition of 10 µM bicuculline to the superfusate,greatly enhancing both the voltage-sensitive dye signal and EPSPamplitude in whole-cell recordings (Figs. 6, 7). During bicucullineapplication, voltage-sensitive dye signals were larger, lastedlonger, and spread over a larger cortical region, in accord withthe effects of bicuculline observed with voltage-sensitive dyesin vitro (Laaris et al., 2000) and in vivo during whisker stimulation(London et al., 1989). Simultaneous whole-cell voltage recordingsindicated that amplitude and duration increased in a manner wellcorrelated to the changes in optically detected signals, for example,when comparing the local voltage-sensitive dye response and themembrane potential of the layer 2/3 neuron (Fig. 6B,C). In thepresence of bicuculline, APs are observed in whole-cell recordingsfrom neurons in both layer 4 and layer 2/3 (Fig. 6D), which wasnot the case in control conditions. Many APs were observed inresponse to single stimuli in both layer 2/3 and layer 4 excitatoryneurons, but the membrane potential always returned to the prestimulusvalue, even with 10 µM bicuculline present. Epileptic activitybetween stimuli was not observed, and sequential stimuli evokedreproducible responses (Fig. 6D). The absence of spontaneous activityand the ability of the membrane potential to recover its restingvalue quickly after stimulation might suggest that some inhibitionremains despite the presence of 10 µM bicuculline. This couldresult from the activation of GABA_B receptors or ionotropic GABAreceptors with low bicuculline sensitivity during massive excitation.

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Figure 6. Block of inhibition by bicuculline evokes equivalent enhancement of whole-cell electrophysiological and voltage-sensitive dye responses. A, Time series of optical responses to stimulation of a layer 4 barrel under control conditions (top) or after application of 10 µM bicuculline to block GABA_A receptors (below). The same stimulation strength evoked a larger response with a longer duration in the presence of bicuculline. Scale bar, 100 µm. B, The effect of bicuculline on the response measured by voltage-sensitive dye in a region (60 × 60 µm) surrounding a whole-cell recording (black box in A). C, The effect of bicuculline on the responses measured with whole-cell recording. These traces are averages of the same 16 consecutive sweeps as for the voltage-sensitive dye measurements in A and B. There is a close correspondence of the changes in amplitude and time course of responses with those of the voltage-sensitive dye. D, Consecutive individual sweeps of the whole-cell recordings under control conditions (left) and after application of bicuculline (right). No action potentials are evoked in control conditions, whereas several are evoked by each stimulus when inhibition is blocked. The responses to consecutive stimuli are similar.

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Figure 7. Block of inhibition by bicuculline potentiates the spread of excitation in L2/3 and L5 but not layer 4. A, Schematic representation of the spread of excitation in paracoronal slices at 10 (red), 15 (green), and 20 (blue) msec after stimulation. The black dashed line indicates that excitation in layer 2/3, and layer 5 often spread beyond the field of view. The spread of voltage-sensitive dye signal within layer 4 increases only a little compared with the expansion of excitation within layer 2/3 and layer 5. B, Individual example showing columnar excitation under control conditions (image at 12 msec) but large lateral spread of excitation in layer 2/3 and layer 5 after 10 µM bicuculline application (image at 50 msec). Scale bar, 100 µm. C, In tangential layer 4 slices, application of bicuculline has no obvious effect on the spatial extent of excitation detected by optical imaging (control image at 12 msec; bicuculline image at 40 msec). Scale bar, 100 µm.

The initial spatiotemporal pattern of the voltage-sensitive dye response was similar in control and bicuculline (Fig. 6A).The response was initially confined to the layer 4 barrel andthen spread in a columnar manner into layer 2/3. Under controlconditions, the response then decays, remaining columnar (as alsoshown in Fig. 3), whereas in the presence of bicuculline, theresponse increases several-fold and propagates laterally overa large region in layer 2/3. The infragranular region of layer5, which in many cases is only weakly excited by field stimulationunder control conditions, is also strongly activated by identicalstimuli but in the presence of bicuculline (Fig. 6A,B). Such increasesin spatial spread of voltage-sensitive dye signals are not observedin layer 4 (Fig. 7). In paracoronal slices (n = 10), the widthat half-maximal signal amplitude is increased only by 41 ± 6%within layer 4, whereas in layer 2/3, the half-width increasesby at least 117 ± 15% (quantified at peak response amplitudes).This number is likely to be an underestimate because, in manyexperiments (like the one shown in Fig. 7B; control response at12 msec after stimulation; response in the presence of bicucullineat 50 msec), the entire field of view (780 × 780 µm) of layer2/3 is homogeneously excited and, for quantification purposes,the half-width of such signals was given a value of the fieldof view, although its real value would be larger. The result ofthis non-uniform propagation of excitation is that the neighboringbarrels in layer 4 appear to be uniquely spared. The restrictedlateral spread of excitation in layer 2/3 under control conditionsthus appears to result from inhibition, whereas the restrictionof excitation within layer 4 to the stimulated barrel appearsto result from a lack of excitatory connections between barrels.This view is in good agreement with anatomical reconstructionof dendritic and axonal arborizations of layer 4 neurons remainingconfined to a single barrel (Fig. 2). The lateral propagationof excitation within layer 2/3 when inhibition is blocked presumablyreflects the suprathreshold activity of layer 2/3 neurons, withtheir axons projecting across to neighboring barrel columns excitingother layer 2/3 pyramidal neurons and also contacting the apicallayer 5 pyramidal dendrites, thus evoking excitation within layer5. Furthermore, it would appear that neurons of layer 2/3 andlayer 5/6 only weakly excite the barrel of layer 4 sandwichedin betweenthem.
We further tested the effect of bicuculline on tangential layer 4 slices to see whether significant extension of stimulatedareas could be evoked. After application of bicuculline, the areacontained within a half-maximal contour increased by only 9 ±12% (n = 10; quantified at peak response amplitudes). An exampleexperiment showing a hexagonally shaped barrel, with a similarlyshaped voltage-sensitive dye signal, which was barely affectedby bicuculline application, is shown in Figure 7C (control responseat 12 msec after stimulation; response in the presence of bicucullineat 40 msec). The smaller effect of bicuculline in tangential slicesof layer 4 compared with the effect within layer 4 of paracoronalslices presumably results from the lack of excitation from layer2/3 and layer 5/6 in these tangential slices. These data suggestthat, in layer 4, the barrels are functionally independent evenwhen enormous activity is evoked in all neighboring neocorticalregions.

Repetitive 10 Hz stimulation does not alter the spatiotemporal extent of voltage-sensitive dye signals
During active exploration, rodents move their whiskers rhythmically at a frequency of ~10 Hz, which, it is thought, increasesthe sampling rate of nearby space, allowing objects to be rapidlyand accurately located. It is thus of particular interest to investigatethe effects of repetitive stimulation on the spatiotemporal signalingpatterns within barrel cortex. When a barrel is stimulated at10 Hz frequency, each stimulus evokes a clear response, whichis similar to the response to the first stimulus. However, duringthe 10 Hz train of 10 stimuli, the response amplitude decreasesto 54 ± 7% within layer 4 and to 62 ± 6% in layer 2/3 (n = 13).More importantly, however, the spatial structure of the voltage-sensitivedye responses remains almost unaltered, with only slight increasesin the half-width of the evoked excitation measured 12 msec afterstimuli comparing first and last responses from 387 ± 23 to 437± 46 µm in layer 4 and 479 ± 43 to 509 ± 56 µm in layer 2/3, witha mean layer 4 barrel width of 399 ± 21 µm (n = 13). The functionalcolumns of excitation observed with single stimuli are thus preservedduring repetitive stimulation but with smaller signal amplitudes.This may be attributable to a depression of excitatory synaptictransmission and/or increasedinhibition.

Simultaneous stimulation of neighboring barrels has only a weak nonlinear effect on the spatiotemporal extent of voltage-sensitive dye signals
For the rodent to gather information concerning nearby objects, it is likely that the information concerning the movementof a single whisker is processed in concert with that from neighboringwhiskers and indeed the entire whisker array (Moore et al., 1999).One might therefore expect substantial modifications of the responseof a barrel column depending on whether or not its neighbor isstimulated or not. Indeed, in vivo both supralinear and sublinearchanges to responses from one whisker have been observed by pairingstimulation with neighboring whiskers (Simons, 1985; Kleinfeldand Delaney, 1996; Ghazanfar and Nicolelis, 1997; Shimegi et al.,2000). To address whether such interactions also occur in vitroin the neocortex, we stimulated neighboring barrel columns simultaneouslyand compared this with the sum of the responses to stimulationof the barrel columns separately. The results suggested that responsesare summated almost linearly (Fig. 8). To quantify the effect,the half-width of signals for layer 4 and layer 2/3 for the experimentalsimultaneous stimulation and the computed sum of individual responseswere compared at 12 msec after stimulation. The width of excitationin layer 4 did not change significantly (experiment, 534 ± 40µm; linear sum, 526 ± 40 µm; paired t test, p > 0.4; n = 12),whereas the width in layer 2/3 showed a slight superlinearity,with an experimental width of 722 ± 43 µm compared with the expectedvalue of 676 ± 41 µm (paired t test, p < 0.005; n = 12). Responsesin layer 4 barrels show little spatial overlap with nearest neighbors,and the combined response is entirely linear. Excitation in layer2/3 extends well into the neighboring barrel column, but nonethelessthe response is summated close to linearly. The small supralinearinteraction component within layer 2/3 could result from supralinearsummation of subthreshold EPSPs via voltage-gated channels.

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Figure 8. Activity evoked by the simultaneous stimulation of neighboring barrels is summated linearly. A, Bright-field micrograph showing stimulation electrodes placed in the lower center of neighboring barrels. Stimulation of single barrels (left or right) evoked responses in the barrel column. The response to simultaneous stimulation of neighboring barrels (labeled left and right) appears to be equivalent to the simple sum (labeled sum) of the responses evoked by stimulation of the barrels separately. The voltage-sensitive dye images are shown at 12 msec after stimulus. Scale bar, 200 µm. B, Comparison of the full-width at half-maximal for the voltage-sensitive dye signals between the experimental simultaneous stimulation of neighboring barrels and the linear sum of the individual responses. In layer 4, the width of excitation is unchanged and only a small increase of width is detected in layer 2/3.

NMDAR-dependent expansion of the spread of excitation can be induced by pairing high-frequency stimuli
Both the development and plasticity of the neocortex have been suggested to be regulated in part by electrical activity-dependentprocesses. Changes in synaptic efficacy of inputs onto layer 2/3pyramidal neurons have been proposed recently to underlie someof the major changes in receptive fields induced by alterationsin sensory experience (Diamond et al., 1994; Finnerty et al.,1999; Feldman, 2000). To investigate whether expansion of thespatial extent of excitation in layer 2/3 can be observed in vitro,we stimulated neighboring barrels simultaneously using a pairingprotocol similar to one that causes NMDA receptor-dependent potentiationbetween layer 2/3 pyramidal neurons (Egger et al., 1999). Neighboringbarrels were stimulated simultaneously every 5 sec with a trainof five stimuli separated by 50 msec for a total of 100 stimuliseparated into 20 bursts. The effects of this pairing procedurewere measured 10-15 min later, well beyond the period of short-termplasticity or posttetanic potentiation. Each barrel was subsequentlystimulated separately, and the spatial extent of the evoked voltage-sensitivedye signal was compared with the prepairing response. There wasa no obvious change to the spatial extent of the voltage-sensitivedye signal in layer 4. In some experiments, there appeared tobe a clear enhancement of the response in layer 2/3 above theneighboring barrel with which it had shared the pairing stimulation,but there was no significant change when all experiments wereincluded (paired t test, p = 0.076; n =16).
In view of the relatively small supralinear effect in layer 2/3 of stimulating neighboring barrels (Fig. 8), it is likelythat this stimulation protocol causes only a weak coincidence(pairing) of activity in layer 2/3 pyramidal neurons. To evokea stronger pairing of excitation in layer 2/3 neurons, the stimulationof a barrel in layer 4 was paired with simultaneous stimulationof a layer 2/3 region in the neighboring barrel column. One stimulationelectrode was placed in the lower center of a barrel and evokedexcitation limited to a barrel column as described previously(Fig. 9A). The second stimulation electrode was placed in layer2/3 within 200 µm of the right-hand lateral extent of the barrelcolumn. It evoked voltage-sensitive dye signals, which were strongestin the region immediately surrounding the stimulation electrode(Fig. 9A). The same pairing protocol was used as before, and againthe effects were measured 10-15 min later to avoid measuring effectsof short-term plasticity or posttetanic potentiation. This pairingprotocol induced a significant asymmetric expansion in the lateralextent of the layer 2/3 voltage-sensitive dye signal evoked bystimulation of the barrel column (Fig. 9, quantified at 12 msecafter stimulation). The amplitude of the voltage-sensitive dyesignal evoked by stimulation of a layer 4 barrel is more thandoubled in the region close to the stimulation electrode in layer2/3. Quantified over an area of 200 × 200 µm located in the middleof layer 2/3 and laterally 500 µm from the center of the barrelcolumn toward the stimulating electrode in layer 2/3, the signalincreased after pairing by 133 ± 47% (n = 13; paired t test, p< 0.01). Measured at the same lateral distance from the spatialpeak of the voltage-sensitive dye response but on the oppositeside of the barrel column response, on average there is a slightdecrease in the signal strength (Fig. 9D). This is probably attributableto a slight rundown of the responses, because an equal changeis observed after the high-frequency pairing protocol in the presenceof the NMDA receptor antagonist D-APV (100 µM). However, the asymmetricalexpansion of the spatial extent of the voltage-sensitive dye signalclose to the layer 2/3 pairing stimulation is completely blockedby D-APV (n = 9; p > 0.1). If identical stimuli are deliveredbut the trains of stimuli are separated by 500 msec instead ofsimultaneously, then no potentiation is induced. After such unpairedprotocols, the amplitude of the evoked signals decreased by 23± 4% (n = 10), quantified as before near the layer 2/3 stimulatingelectrode. To further test that the potentiation of voltage-sensitivedye responses after pairing was not attributable to changes inoptical properties of the slice, whole-cell recordings were madefrom excitatory neurons near the layer 2/3 stimulating electrode.After the pairing protocol, EPSPs evoked by stimulation of thelayer 4 barrel increased in amplitude by 79 ± 44% (n = 7). Duringthe pairing protocol, action potentials were often evoked in theneuron by the simultaneous stimulation in layer 4 and layer 2/3.The potentiation observed here may thus share a common mechanismwith the increases in synaptic efficacy associated with EPSPspaired with action potentials evoked by somatic current injection(Markram et al., 1997; Egger et al., 1999; Feldman, 2000); however,changes in excitability or inhibition may also contribute. Thus,several molecular mechanisms could be involved in generating theexpansion of the spread of excitation after the pairing protocol.

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Figure 9. Pairing stimulation of a barrel column with a neighboring region of layer 2/3 induces an NMDA receptor-dependent expansion of excitation. A, The experimental arrangement and stimulation protocol used to induce a spatial expansion of responses (top left). Stimulation of the electrode in layer 2/3 placed to the right of the barrel column evoked a local response (top right). Stimulation of the electrode at the lower center of a barrel evoked a columnar response (bottom left). Both electrodes were then stimulated simultaneously five times at 50 msec intervals, and this was repeated at 5 sec intervals for a total of 20 pairing bursts. Responses were then tested 15-20 min after this pairing protocol, and the area within layer 2/3 excited by stimulating a barrel was found to have expanded toward the layer 2/3 stimulating electrode located on the right (bottom right). The voltage-sensitive dye images are shown at 12 msec after stimulus. Scale bar, 200 µm. B, The voltage-sensitive dye signal across the lateral extent of layer 2/3 after the pairing is selectively enhanced on the right of the barrel column at which the layer 2/3 stimulating electrode was located. A region at equal distance from the peak response but to the left shows no potentiation. The difference between left and right regions shows that the spatial extent of the layer 2/3 signal can be asymmetrically changed. Same experiment as shown in A. C, Subtracting the lateral voltage-sensitive dye signal after pairing from the control signal shows that the signal is increased on the right after pairing within layer 2/3, but within layer 4 there is no asymmetrical change. Same experiment as shown in A and B. D, Across all experiments, the changes at equal distances to the left and to the right of the peak are plotted. On average, only a small rundown of responses is observed after pairing in the presence of APV, but under control conditions, there is a significant selective enhancement of responses to the right of the peak, which is the region close to the layer 2/3 stimulating electrode. E, A schematic drawing of the changes induced by pairing the response of a barrel column with excitation of a neighboring region of layer 2/3 on the right.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Functional neocortical column

The pattern of the spread of excitation initiated in a barrel of layer 4 provides a new, dynamic view of a neocortical column.The early response (~2 msec) to a single stimulus is limited tothe stimulated barrel in layer 4, and it is only later (~5 msec)that the close correspondence to the anatomically defined barrelcolumn develops. This correspondence remains during the decayphase of the response, lasting ~50 msec after the stimulus. Thisspatiotemporal pattern of the propagation of excitation in a columnarmanner also remains invariant during repetitive stimulation andis only weakly affected by stimulation of a neighboring barrelcolumn. The functional confinement of the spread of excitationto a column was controlled by GABAergic inhibition. Even in theabsence of inhibition, however, the initial milliseconds of thespread of excitation is unchanged, showing the stereotypical columnarpropagation of the axonal projection of layer 4 excitatory neurons.Later (~25 msec) excitation spreads laterally in layer 2/3 andreaches layer 5/6, presumably through recurrent excitatory synaptictransmission of pyramidalneurons.

Barrels are functionally independent
Our anatomical reconstruction of a normalized barrel is in accord with previous studies showing that both the axonal and dendriticarbors are confined to the barrel in which the soma is located(Woolsey et al., 1975; Harris and Woolsey, 1983; Simons and Woolsey,1984; Lübke et al., 2000; Petersen and Sakmann, 2000). Mappingthe connectivity of pairs of excitatory neurons within layer 4has furthermore shown that barrels are functionally independent(Petersen and Sakmann, 2000). However, such studies were limitedto the few neurons selected for whole-cell recording and cannotaddress what occurs when a much larger ensemble of neurons arestimulated. Voltage-sensitive dye signals show that the excitatoryneuronal network of barrels in layer 4 is functionally independent,even during massive excitation evoked by stimulation in the presenceof bicuculline. This not only implies that the network withineach barrel is independent of neighboring barrels but also thatactivity in supragranular and infragranular cortical laminas areonly able to weakly excite layer 4. This inability of excitationinitiated in one barrel to spread into another in vitro may explainthe lack of effect on unit responses to surround whisker stimulationin vivo after lesions to neighboring barrels (Goldreich et al.,1999).

Spread of excitation in layer 2/3
The maximal response in layer 2/3 is primarily confined to a region with a similar width to the layer 4 barrel, thus defininga "functional" barrel column. Whereas the layer 4 response showslittle overlap with the neighboring barrel, the signal evokedsomewhat later in layer 2/3 is significantly broader (26 ± 4%)than the layer 4 signal. A large fraction of the lateral decayof excitation occurs close to the boundary of the barrel column,but nonetheless significant excitation is detected in layer 2/3of the neighboring barrel column. This overlap between barrelcolumns is also reflected in the supralinearity of the summedlayer 2/3 responses evoked by stimulation of two neighboring columns.We thus conclude that sensory signals from the thalamus wouldbe processed separately in layer 4 barrels, but within layer 2/3there are significant excitatory interactions between columns.The lateral extent of excitation within layer 2/3 is stronglyregulated by inhibition, and thus the activity of GABAergic interneuronsmay determine whether the processing of whisker movement relatedcortical signals occurs at a local (single-column) or a global(multicolumn) scale in layer 2/3.

Comparison with in vivo data

Optical imaging of voltage-sensitive dyes in vivo has yielded maps of whisker-evoked activity in somatosensory cortex (Orbachet al., 1985; Kleinfeld and Delaney, 1996). Stimulation of a singlemystacial whisker can evoke voltage-sensitive dye signals overan area of several square millimeters of the cortical surface.The spread of excitation measured in vivo thus appears to be considerablymore extensive than what we observe in vitro in layer 2/3 fromthe stimulation of a single layer 4 barrel. The larger excitationarea observed in vivo is likely to result from a number offactors.

The receptive field of both thalamic ventroposterior medial neurons (Ito, 1988; Simons and Carvell, 1989; Armstrong-Jamesand Callahan, 1991; Diamond et al., 1992; Brecht and Sakmann,2001) and layer 4 neurons (Moore and Nelson, 1998; Zhu and Connors,1999) are considerably broader than might be expected from theapparent precision of the primary anatomical connections specificallywiring the sensory neurons of a given whisker to its homologousbarrel. Thus, deflection of a single whisker evokes EPSPs andeven APs in neurons located in many layer 4 barrels and septalregions. The large receptive fields of layer 4 neurons could contributeto the large spatial extent of responses in layer 2/3 evoked bysingle whisker stimulation measured in vivo by voltage-sensitivedye. This contrasts with our selective stimulation of a singlebarrel allowing a simpler analysis of the functional architectureof synapticconnections.

The width of layer 2/3 signals observed in vitro by stimulation of a single layer 4 barrel depended strongly on the stateof inhibition. Blocking inhibition with 10 µM bicuculline causedexcitation to spread laterally over much larger regions of layer2/3, in closer agreement with the size of the spread of excitationobserved in vivo. The balance between excitation and inhibitionin vivo may thus be shifted in favor of excitation compared within vitro. That this is the case is suggested by the much higherlevels of both subthreshold and suprathreshold spontaneous activityof neurons recorded in vivo. Additional support for this explanationcomes from a comparison of the duration of the voltage-sensitivedye signals in vivo and in vitro. Whereas under control conditionsin vitro voltage-sensitive dye signals last ~50 msec, in vivoa single deflection of a single whisker can evoke responses lastingup to 500 msec (Kleinfeld and Delaney, 1996), suggesting thatinhibition in vivo does not prevent prolonged excitation. Thelarger neocortical area excited in vivo as recorded by voltage-sensitivedye imaging may thus result from propagating activity within layer2/3 mediated by local recurrent excitatory collaterals of thelayer 2/3 pyramidal neurons. In support of such a conclusion,high temporal resolution imaging of responses to single whiskerdeflections result in an initial excited region that is littlelarger than a layer 4 barrel, but which subsequently rapidly expandsto cover a much larger region over the next milliseconds (Petersenet al., 2001).

NMDA receptor-dependent plasticity of barrel column responses

Previous studies of NMDA receptor-dependent plasticity in neocortical slices have focused on the increases in local fieldpotentials or responses in individual neurons (Kirkwood et al.,1993; Castro-Alamancos et al., 1995; Markram et al., 1997; Feldman,2000). Because of the very localized nature of such measurements,there has been no information about changes in the spatial patternof excitation associated with stimulation protocols that inducepotentiation of individual synaptic responses. The spatial correlateof synaptic potentiation of many synapses in the ensemble neocorticalcircuit would be an expansion in the area excited. By imagingvoltage-sensitive dye signals, we observed NMDA receptor-dependentchanges in the spatial extent of excitation induced by pairinglarge ensembles of neurons in layer 2/3. Of particular interestis the asymmetry of the spatial extension of the voltage-sensitivedye response toward the simultaneously stimulated area. Responsesthus extend toward simultaneously active regions. Such large-scalealterations in the spatiotemporal profile of responses may representan in vitro correlate of map plasticity induced by alterationsin sensory input to the neocortex (for review, see Buonomano andMerzenich, 1998). The most obvious comparison is with studiesof cortical response plasticity after whisker trimming, althoughthis plasticity develops over a period of days, whereas the plasticitywe describe here is induced within a couple of minutes and theeffects were analyzed 10-15 min later. The plasticity that wedescribe might thus represent the early steps induced by whiskertrimming protocols, which leave only two whiskers intact. In theseso-called "whisker pairing" experiments, the response of neuronsin one spared barrel to stimulation of the neighboring sparedwhisker are greatly potentiated (Diamond et al., 1994). Such changesare in accord with the data presented here. If neighboring regionsare stimulated strongly in the absence of other input, then thefunctional barrel column will extend toward the simultaneouslyactive region in layer 2/3. That changes in the spatial extentof voltage-sensitive dye signals can be induced by pairing protocolssuggests that voltage-sensitive dye imaging may also be usefulto assess in vivo plasticity of cortical maps induced by alterationsin sensoryexperience.

  FOOTNOTES

Received June 1, 2001; revised Aug. 6, 2001; accepted Aug. 9, 2001.

C.C.H.P. was supported by a Marie Curie fellowship from the European Commission. We thank Dr. Asaf Keller for critical readingof an earlier version of this manuscript and Dr. Amiram Grinvaldfor technical help and usefuldiscussions.
Correspondence should be addressed to Carl C. H. Petersen, Department of Cell Physiology, Max-Planck-Institute for MedicalResearch, Jahnstrasse 29, Heidelberg D-69120, Germany. E-mail:petersen{at}mpimf-heidelberg.mpg.de.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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