Properties of Horizontal and Vertical Inputs to Pyramidal Cells in the Superficial Layers of the Cat Visual Cortex

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The Journal of Neuroscience, March 1, 2000, 20(5):1931-1940

Properties of Horizontal and Vertical Inputs to Pyramidal Cells in the Superficial Layers of the Cat Visual Cortex
Yumiko Yoshimura¹^,², Hiromichi Sato³, Kazuyuki Imamura¹, and Yasuyoshi Watanabe¹
¹ Department of Neuroscience, Osaka Bioscience Institute, Furuedai, Suita, Osaka 565-0874, Japan, ² Department of Visual Neuroscience, Research Institute of Environmental Medicine, Nagoya University, Furo-cho, Chikusa-ku, Nagoya, Aichi 464-8601, Japan, and ³ School of Health and Sport Sciences, Osaka University, Machikaneyama, Toyonaka, Osaka 560-0043, Japan

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The purpose of this study is to elucidate the integrative input mechanisms of pyramidal cells receiving horizontally projectingaxon collaterals (horizontal projection) and vertical input fromlayer IV. We performed whole-cell recordings from pyramidal cellsin layer II/III and focally activated other single pyramidal cellsmonosynaptically connected via long-distance horizontal (LH) projections(the distance between presynaptic and postsynaptic cells was 350-1200µm) in slice preparations of the kitten primary visual cortex.In addition, presynaptic single fibers in layer IV (vertical input)and/or short-distance horizontal (SH) inputs from neighboringsingle pyramidal cells (distance within 100 µm) in layer II/IIIwere activated. Unitary EPSPs evoked by the activation of LH andSH connections had smaller amplitude and larger coefficient ofvariation than those evoked by stimulating the vertical input.Paired-pulse stimulation of the LH and SH inputs caused the depressionof the second EPSP, whereas that of vertical inputs caused eitherfacilitation or depression of the second EPSP. The EPSPs evokedby simultaneous activation of LH and vertical inputs summatedlinearly at the resting membrane potential. However, the EPSPsevoked by stimulation of the two inputs were nonlinearly (supralinearly)summated when the postsynaptic membrane was depolarized to a certainlevel. Similar EPSP interaction was observed in response to simultaneousactivation of the LH and SHinputs.

Key words: horizontal connection; pyramidal cell; visual cortex; synaptic interaction; whole-cell recording; cat

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Pyramidal cells in the visual cortex, particularly those located in the superficial layers, are known to send axon collateralshorizontally for up to several millimeters (Fisken et al., 1975;Gilbert and Wiesel, 1979) and to interconnect with functionaldomains, or columns, which process similar stimulus features (Gilbert,1983; Ts'o et al., 1986; Hata et al., 1991). There is some evidenceindicating that cells in the primary visual cortex exhibit responsemodulation depending on the context of the stimuli inside andoutside the classical receptive field (Van Essen et al., 1989;Kapadia et al., 1995; Sillito et al., 1995; Polat et al., 1998;Akasaki et al., 1998). It has been suggested that long-range horizontalconnections could form the structural basis for this context-dependentintegration of visual information over a wide area in the visualfield (for review, see Gilbert, 1992).

To understand the functional role of horizontal connections, it is particularly important to clarify the precise nature ofthe synaptic interactions between the horizontal input and otherinputs on a postsynaptic cell. Previous in vitro studies havedemonstrated that stimulation of the horizontal pathway evokedweak monosynaptic and polysynaptic EPSPs followed by IPSPs inthe visual cortex (Hirsch and Gilbert, 1991; Weliky et al., 1995;Katz et al., 1997). However, Hirsch and Gilbert (1991) used massiveelectrical stimulation with metal wires to activate the horizontalconnections. Thus, axons of passage were also inevitably activatedin addition to the target axon collaterals. The combined studyusing optical imaging of the ferret visual cortex in vivo andlaser photostimulation with caged glutamate in slices has beenperformed to clarify the spatial relationships between the orientationdomains and the patterns of the aforementioned lateral connections(Weliky et al., 1995; Katz et al., 1997). Although axons of passagewere not stimulated in this method, it was impossible to isolateunitary responses derived from the identified presynapticneurons.

In the present study, we performed whole-cell recordings from a pyramidal cell in layer II/III in a slice preparation of thekitten primary visual cortex and focally activated a single presynapticpyramidal cell within layer II/III and/or a single fiber in layerIV. Subsequently, we also performed whole-cell recordings froma presynaptic cell to inject a neural tracer. By using these methods,we were able to analyze unitary EPSPs derived from horizontaland vertical inputs and visualize the synaptically connected cellpairs.

Yoshimura et al. (1999) recently reported that the number of open channels at the peak of EPSCs at pyramidal-pyramidal synapsesin layer II/III is several times smaller than that reported forsynapses between geniculocortical afferents and layer IV spinystellate cells (Stratford et al., 1996). Therefore, it is assumedthat the convergence of a significant amount of input to a pyramidalcell is necessary to cause it to fire. However, to our knowledge,no study has examined the interactions between horizontal inputsand identified single inputs using intracellular recording techniques.Therefore, we systematically investigated the precise propertiesof the spatial and temporal interactions between horizontal andverticalinputs.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

All experiments were approved by the Animal Research Committee of the Osaka Bioscience Institute and performed in accordancewith the National Institute of Health guidelines for the careand use of laboratoryanimals.

Slice preparations. Kittens [n = 14, postnatal day 29 (P29)-35] were deeply anesthetized by injections of ketamine (20 mg/kg,i.m.) followed by sodium pentobarbital (40 mg/kg, i.v.), and thenperfused transcardially with ice-cold oxygenated artificial CSF(ACSF). The composition of the ACSF was as follows (in mM): 124NaCl, 3.8 KCl, 1.2 KH₂PO₄, 1.3 MgSO₄, 2.4 CaCl₂, 10 glucose, and26 NaHCO₃, pH 7.4 when bubbled with 95% O₂ and 5% CO₂. Slicesof the primary visual cortex (300- to 350-µm-thick) were cut usinga rotor slicer (DTY7700; Dosaka EM) and then incubated with ACSFin an interface chamber for 1 hr at 32-34°C. For the recordingexperiments, the slices were transferred into a submerged recordingchamber that was continuously perfused with ACSF at 25-27°C. Recordingswere obtained from layer II/III pyramidal cells, which were identifiedby microscopic observation with Nomarski optics. The criteriafor the identification of pyramidal cells have been describedpreviously (Yoshimura and Tsumoto, 1994).

Recording procedures. Whole-cell recordings were made from pyramidal cells in the superficial layers. Whole-cell patch pipettes(resistance, 6-10 M $Omega$ ) were filled with a solution containing (inmM) 130 K-gluconate, 10 KCl, 10 HEPES, 3 MgATP, and 0.5 Na₂GTP,with pH adjusted to 7.2 using KOH. The osmolality of the solutionwas 280-285 mOsm. Neurobiotin (0.5%) was added to the pipettesfor intracellular staining of the recorded cells. Membrane potentialswere recorded in the current-clamp mode with a patch-clamp amplifier(Axopatch 2B; Axon Instruments, Foster City, CA). Liquid junctionpotentials were corrected. The alignment of the recording andstimulating electrodes is shown in Figure 1A. For the stimulationof individual horizontal connections, the tip of a second pipettefilled with ACSF was placed onto the soma of other pyramidal cellsin the superficial layers. The horizontal connections within layerII/III were divided into two groups according to the distancebetween the presynaptic and postsynaptic cells as long-distancehorizontal (LH) connections (cell distance of 350-1200 µm) andshort-distance horizontal (SH) connections (cell distance of <100µm). If no postsynaptic potential was recorded during 50 trialsof stimulation, the stimulating electrode was moved to anotherneuron. To detect whether the evoked EPSPs were unitary or not,the EPSP amplitudes were plotted against the stimulus intensity(Fig. 1B). In the case of unitary responses, we observed a certainthreshold of stimulus intensity below which no response was detectedand EPSPs appeared only at or above this threshold. The mean EPSPamplitude did not change significantly with further increasesin stimulus intensity beyond a certain range above the threshold(Stern et al., 1992; Yoshimura and Tsumoto, 1994). After the detectionof a monosynaptic LH connection (Fig. 1Ad,Cd), an additional stimulatingelectrode was placed on a pyramidal cell located at a distanceof <100 µm from the recorded cell in the superficial layers toactivate a SH connection with focal stimulation (Fig. 1Aa,Ca).For the activation of a vertical input from layer IV, a stimulatingglass electrode was inserted in layer IV just beneath the recordedcell to activate a single fiber by the minimal-stimulation protocol(Fig. 1A, Vertical, D) (Allen and Stevens, 1994). Each input pathwaywas stimulated at 0.33 Hz. To examine the spatiotemporal interactionsbetween the LH inputs and vertical or SH inputs, the responsesto concurrent activation at various interstimulus intervals (ISIs)of any two inputs were recorded. The ISIs used were 0, 5, 10,20, 50, 100, and 200 msec. For evaluating response summation,the summation index (SI) was defined as follows:

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Figure 1. Schematic arrangement of electrodes (A) and examples of unitary EPSPs evoked by focal stimulation of horizontal (C) and vertical (D) input pathways. When cell a or d in A was stimulated, clear EPSPs were recorded from a pyramidal cell in the superficial layers, as shown in C. No EPSP was evoked by the stimulation of cell b and c in A. The distance between the stimulated and recorded cells was 60, 350, 410, and 440 µm for cells a-d, respectively. B, The stimulus-response curve of EPSPs obtained from the cell shown in C and D. Each dot indicates the mean peak amplitude of EPSPs evoked by the stimulation of the cell d. Error bars indicate SDs. The abrupt increase of the EPSP amplitude at the stimulus intensity of 13 V suggests that the EPSPs were unitary. D, EPSPs evoked by minimal stimulation of the layer IV.

SI = (the peak amplitude of the EPSP evoked by combined stimulation)/(the peak amplitude obtained by the simple mathematicalsummation of two EPSPs elicited by the individual activation oftwo inputpathways).

To test the effects of paired-pulse stimulation, either one of the three input pathways was successively stimulated at ISIsof 20, 50, 100, 200, 500, and 1000msec.

Data acquisition and analysis. Data were digitized at the rate of 10 kHz and fed to a computer (Gateway 2000) for off-lineanalysis. Synaptic potentials were filtered at 1 kHz. Data wereanalyzed mainly with pClamp software (Axon Instruments). The risetime of the EPSP was measured as the time between the time pointscorresponding to 10 and 90% of the peak amplitude. For the analysisof spontaneous EPSPs, the threshold was manually set at 3× theSD of the mean baseline noisevalue.

Visualization of synaptic contacts. After completion of the physiological recording experiments, we replaced the stimulatingelectrode with a patch-pipette containing 0.5% neurobiotin andobtained recordings from the presynaptic cell for at least 15min while injecting neurobiotin under microscopic observation.Accordingly, both presynaptic and postsynaptic cells were histologicallyvisualized by intracellular staining with neurobiotin. Sliceswere fixed in phosphate buffer (0.1 M, pH 7.4) containing 4% paraformaldehydeand 0.1% glutaraldehyde, immersed in 30% sucrose solution, andthen resectioned into 60-80 µm section with a microtome. The sectionswere then processed by the standard method using avidin-biotinylatedhorseradish peroxidase complex (Horikawa and Armstrong, 1988).The labeled neurons were reconstructed under a light microscope(Optiphot, Nikon) using a cameralucida.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study is based on data recorded from 44 postsynaptic and 65 presynaptic pyramidal cells in the kitten visual cortex.All the recorded cells were identified as pyramidal cells in thesuperficial layers by microscopic observation using Nomarski opticsduring the recording experiments. All the cells showed typicalspike accommodation to a depolarizing current injection, a characteristicof pyramidal cells (Mason and Larkman, 1990). Furthermore, in7 of 44 pairs with LH connections and 3 of 25 pairs with SH connections,the presynaptic and postsynaptic cells were histologically ascertainedas being pyramidal cells by intracellular staining (see below).The input resistance and the resting potential of the recordedcells were 330 ± 103 M $Omega$ and $-$ 73.1 ± 4.4 mV (mean ±SD).

Electrophysiological characteristics of LH, SH, and vertical connections

Focal stimuli were applied to individual presynaptic pyramidal cells with either LH or SH connections in the superficial layers,to evoke unitary EPSPs in the recorded postsynaptic cells. Foractivation of the vertical input, a single input source in layerIV was stimulated by the minimal stimulation protocol (see Materialsand Methods). Only unitary EPSPs were analyzed. The means of thepeak amplitude, rise time, half-width, and coefficient of variation(CV) of all the recorded unitary EPSPs evoked via the three differentinput pathways are summarized in Table 1. There was a statisticallysignificant difference between the peak amplitudes of the EPSPsevoked by the activation of vertical input and either LH or SHinput (p < 0.01, t test). The difference in the EPSP amplitudesbetween those evoked by the activation of the LH and SH inputswas not significant (p > 0.5, t test). The amplitudes of the recordedEPSPs, particularly of those evoked by vertical input activation(6.0 ± 2.8 mV), were larger than those reported previously (0.5± 0.5 mV for layer II/III cells, Reyes and Sakmann, 1999; 1.17± 0.23 mV for layer V cells, Markram and Tsodyks, 1996). In thesestudies in the rat neocortex, unitary EPSPs of small amplitudewere recorded using dual intracellular recordings with patch pipettes.There is the possibility that the minimal stimulation we usedactivated multiple fibers. During the recordings of the evokedEPSPs, we often observed large spontaneous EPSPs presumed to beattributable to activation of single input fibers. If the amplitudesof the large spontaneous EPSPs were comparable to those of theEPSPs evoked by the minimal stimulation of the vertical inputs,the latter could be attributable to the activation of a singleinput fiber. To check this, we collected the spontaneous EPSPsobtained in the cells identified for recording vertical input-inducedEPSPs. We analyzed 10 cells that exhibited frequent spontaneousEPSPs and accumulated >200 events from each cell. The amplitudedistribution of the spontaneous EPSPs varied from 0.4 to 9.7 mV,with a mean of 1.7 ± 1.6 mV. We calculated the mean amplitudeof the 5% of the EPSPs exhibiting the largest amplitudes in thespontaneous EPSP distribution. The mean amplitude of the largestspontaneous EPSPs (6.1 ± 1.9 mV) was not significantly differentfrom that of the unitary EPSPs evoked by vertical input stimulation(p > 0.5, t test, Table 1), suggesting that the minimal stimulationof a vertical input activated a single input pathway that evokedthe largest amplitude EPSPs. In addition, a previous study withdual intracellular recordings using patch pipettes demonstratedthat the EPSPs evoked by an action potential of a presynapticcell in the kitten visual cortex were much larger than those inthe rat visual cortex (Yoshimura et al., 1999). Therefore, weconcluded that a single axon was activated with the minimal stimulationprotocol in the present study.


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Table 1. Properties of all unitary EPSPs

Further analysis was performed to examine the correlation between the electrophysiological properties and the distance betweentwo synaptically connected cells by lateral connections. Figure2 illustrates the mean amplitude (A) and rise time (B) of theEPSPs evoked in each cell by activation of the horizontal inputpathways as a function of the distance between two cells (graphsat right). In the graphs shown on the left in Figure 2, the meanpeak amplitude (A) and rise time (B) of the EPSPs evoked by theactivation of the vertical input are plotted. In regard to thehorizontal connections, no correlation between the peak amplitudeand the distance between the cells was obvious, however, the peakamplitude of the cell group separated by a distance of >600 µm(2.3 ± 0.8 mV, n = 11) was smaller than that of the cell groupwithin 600 µm (4.0 ± 2.2 mV, n = 58, p < 0.01, t test, Fig. 2A).There was no correlation between the cell distance and the risetime of the EPSPs (r = 0.02, p > 0.5, Fig. 2B). Although the peakamplitude of the EPSPs evoked by the activation of vertical inputswas larger than that induced by the activation of horizontal inputson average (p < 0.01, t test, Table 1), there was no differencein the ranges of distribution of the peak amplitude (Fig. 2A).

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Figure 2. Relationship between the distance separating the presynaptic and postsynaptic cells in layer II/III and the electrophysiological parameters of unitary EPSPs. In the graphs on the right, the peak amplitude (A) and rise time (B) of the unitary EPSPs are plotted as a function of the distance between the recorded and stimulated cells. Each horizontal tick represents data for each pair of horizontally connected cells. The connections between cells separated by distances of <100 µm and 350-1200 µm were defined as SH and LH connections, respectively. Because of sampling bias, cell pairs separated by the distance of 100-350 µm are absent. Note the lack of correlation between the distance and the amplitude or rise time of the EPSPs. The horizontal ticks in the graphs on the left represent the mean peak amplitude (A) and rise time (B) of the EPSPs evoked by vertical input stimulation.

To visualize the contact sites between pyramidal cells, for which functional connections were identified, presynaptic andpostsynaptic cells were stained intracellularly with neurobiotinafter the electrophysiological experiments. The morphology ofapparent synaptic contacts was retrieved in 10 pairs. Two examplesof reconstructed pairs are shown in Figure 3. In these pairs,the axon collaterals from presynaptic cells (Fig. 3, red) ascendto the distal part of the apical dendrite of the postsynapticcell to give rise to putative synaptic contacts (Fig. 3, arrows).All labeled pairs separated by a distance of >350 µm (n = 7) wereassumed to make synaptic contacts on the distal parts of the apicaldendrites (Fig. 3, for example). On the other hand, axons derivedfrom more closely situated presynaptic pyramidal cells (n = 3)made contacts either on the apical dendrites (n = 2) or basaldendrites (n = 1) of the postsynaptic cells (data not shown).However, we cannot draw firm conclusions on the relation betweenthe distance separating the cells and contact sites, because theseresults were solely based on observations under a light microscope.

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Figure 3. Reconstruction of a pair of connected pyramidal cells in the superficial layers of the kitten visual cortex. A, B, Two examples of pairs connected via long-distance horizontal axon collaterals. The soma and dendrites are shown in black. The axons of the presynaptic and postsynaptic cells are shown in red and blue, respectively. Boutons of axon collaterals of the presynaptic cell are closely apposed to the apical dendrites (arrows) of the postsynaptic cell. Electrophysiological data of the pairs in A and B are shown in Figures 7 and 10A-C, respectively. Scale bars, 100 µm.

Paired-pulse stimulation of a single input pathway

When two successive inputs came from a single cell via an LH pathway within a certain time interval, the second input wasincapable of eliciting the full EPSP amplitude in the postsynapticcell. Typical examples of such paired-pulse depressions observedfor LH inputs are shown in Figure 4, A and B. In these cases,the LH input was activated twice at an ISI of 100 msec, and theamplitudes of the second EPSPs were smaller compared to thoseof the first one. Paired-pulse depression at the synapses forSH input was also observed (Fig. 4C,D) To compare the resultsof the paired-pulse experiments at ISI of 100 msec among LH, SH,and vertical inputs, the mean amplitudes of the first EPSPs wereplotted against those of the second EPSPs for individual cellpairs (Fig. 5). In 9 of 11 cells for the LH connections and allof the 8 cells for the SH connections, the average amplitude ofthe second EPSPs was significantly smaller than that of the firstone (p < 0.05, t test), that is, paired-pulse depression was noted(Fig. 5A,B). On the other hand, among the 15 cells tested forthe effects of paired-pulse stimulation of the vertical inputs,the second EPSPs were significantly larger than the first onesin six cells (paired-pulse facilitation, p < 0.05, t test) andsmaller in seven cells (paired-pulse depression, p < 0.05, t test,Figs. 4E,F, 5C). This analysis revealed that paired-pulse depressionwas the more common outcome of paired-pulse stimulation of eitherLH or SH inputs, whereas paired-pulse stimulation of verticalinputs resulted in either facilitation or depression of the secondEPSPs (p < 0.05, $chi$ ² test).

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Figure 4. Effects of paired-pulse stimulation in six experiments. Successive stimulations at an ISI of 100 msec were applied to LH (A, B), SH (C, D), and vertical (E, F) input pathways. Each graph illustrates the data from one pair of cells. Diagonal lines indicate that the amplitudes of the first EPSPs are the same as those of the second. Insets show three individual EPSPs and the average (20-30 trials).

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Figure 5. A summary of paired-pulse experiments on the three different input pathways. Each dot denotes the average value from one experiment. Horizontal and vertical bars show the SD of the amplitudes of the first and second EPSPs, respectively. Dashed diagonal lines indicate that the amplitudes of the first EPSPs are the same as those of the second. The second EPSPs were significantly depressed compared to the first in 9 of 11 cell pairs for paired-pulse stimulation of LH input and in all eight pairs for that of SH input. Paired-pulse stimulation of vertical input resulted in either significant facilitation (6 of 15) or depression (7 of 15) of the second EPSPs.

The average ratio of the amplitude of the second EPSPs to the first EPSPs tested with various ISIs are summarized in Figure6. Paired-pulse depressions for LH and SH input pathways wereobserved for ISIs of $<=$ 100 msec.

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Figure 6. ISI dependence of paired-pulse depression and facilitation. The mean ratios (± SD) of the amplitudes of the second EPSPs to those of the first EPSPs are plotted against the tested ISIs for LH (n = 7), SH (n = 6), and vertical (n = 6) connections. Paired-pulse stimulations with ISIs of <100 msec, on average, induced second EPSP depressions for LH inputs and SH inputs and facilitation for vertical inputs.

Interaction between LH and SH or vertical inputs

Under physiological conditions in vivo, excitatory input to the pyramidal cells in the superficial layers of the visual cortexwould be expected from both horizontal and vertical input pathways.Therefore, we assessed the mechanism for interaction between theLH inputs and the vertical or SH inputs. An example of combinedstimulation of an LH input and a vertical input is shown in Figure7. Unitary EPSPs were recorded after minimal stimulation of aLH or vertical input at the resting membrane potential ( $-$ 71 mV,Fig. 7A, top two traces). The EPSPs evoked by simultaneous activationof the two inputs (A, third trace) showed a similar amplitudeand time course to the traces predicted by the mathematical summationof the two individual EPSPs (A, bottom). These results indicatethat the EPSP evoked by concurrent activation of the two inputscorresponded to a linear summation of the two individual EPSPsat the resting membrane potential. To mimic the condition of strongexcitation, corresponding to the abundant excitatory inputs tothe postsynaptic cell, the membrane potential was depolarizedto $-$ 50 mV by the injection of current (Fig. 7B). Under this depolarizedcondition, the EPSP evoked by the activation of an individualinput pathway was smaller than that evoked without this depolarization,because of the decrease in driving force (Fig. 7B, top two traces).Under this condition, when two inputs were driven simultaneously,the evoked EPSP (B, thick line of third trace) was larger thanthe mathematical summation (B, bottom trace) of the two individualEPSPs. This indicates the presence of a multiplicative, supralinearsummation of EPSPs caused by simultaneous activation of LH andvertical inputs under the depolarized condition.

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Figure 7. Interaction between EPSPs elicited by activation of LH and vertical inputs. A, Recordings at the resting membrane potential ( $-$ 71 mV). B, Recordings under the depolarized condition ( $-$ 50 mV). Single stimulation applied to LH inputs (top traces) or vertical inputs (second traces) induced unitary EPSPs. EPSPs were recorded after simultaneous stimulation of LH and vertical inputs (third traces). Predicted EPSPs (bottom traces) were calculated as a simple mathematical sum of the top two traces. EPSPs evoked by concurrent activation of the two inputs was found to be a linear sum of the two individual EPSPs at the resting membrane potential (A). However, supralinear summation was observed under the condition of a depolarized membrane (B). The EPSP induced by simultaneous stimulation of the two inputs (thick line) and the predicted EPSP (dotted line) were superimposed in the third trace in B. The morphology of this cell pair is shown in Figure 3A.

The supralinear summation of EPSPs was also observed after simultaneous stimulation of LH and SH inputs (Fig. 8). At the restingmembrane potential, simultaneous activation of LH and SH inputsevoked an EPSP with an amplitude equal to the linear summationof two individually evoked EPSPs (Fig. 8A). Under the conditionin which the cell was depolarized to $-$ 55 mV, the interaction betweenthe two inputs switched between two states, that is, between linearand nonlinear summation (Fig. 8Ba,Bb). We calculated the SI (seeMaterials and Methods) for each of the EPSPs evoked after simultaneousactivation of two inputs under the condition in which the cellswere depolarized to $-$ 55 mV (Fig. 8C). The distribution of SI showedtwo clear peaks, suggesting a threshold mechanism for the supralinearsummation of EPSPs. This switching between the two summation patternswas not observed in the case of simultaneous stimulation at theresting membrane potential, suggesting that it is not an artifactresulting from occasional stimulation of more than two input sources.

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Figure 8. Interaction between unitary EPSPs evoked by activation of LH (720 µm) and SH (60 µm) inputs. The data shown in A-C were obtained from one cell. A, EPSPs evoked by simultaneous activation of the two inputs were found to be linearly summated at the resting membrane potential ( $-$ 72 mV). B, Linear (a) and supralinear (b) summations were observed under the condition of a depolarized membrane ( $-$ 55 mV). In Bb, the recorded EPSP (thick line) and the predicted EPSP (dotted line) were superimposed. C, The distribution of the summation index calculated from the EPSPs recorded at $-$ 55 mV; data represent those from the experiment shown in B. Note the two clear peaks, the ones on the left and right correspond to linear and nonlinear summation, respectively. Other conventions are the same as in Figure 7.

The SI for the average EPSP amplitude of each recorded cell was calculated and plotted against the membrane potential of thepostsynaptic cell (Fig. 9). The simultaneous activation of twoinputs often evoked somatic action potentials, although the stimulationof a single input pathway never did. We deleted the data of cellsthat exhibited these action potentials because we were unableto measure the exact amplitude of the EPSPs in the presence ofaction potential. In Figure 9, the incidence of the supralinearaugmentation of EPSPs evoked by simultaneous activation of LHinput and either vertical (filled circles) or SH input (open circles)is clearly shown to be dependent on the extent of depolarizationof the membrane. For the cases in which the combined stimulationof the two inputs resulted in supralinear summation of the EPSPswith an SI >1.10, the average membrane potential was $-$ 62.5 ± 6.8mV (average SI = 1.45 ± 0.22, n = 10), whereas for the cases oflinear summation where the SI was <1.10, it was $-$ 73.7 ± 3.3 mV(average SI = 0.93 ± 0.07, n = 32). The membrane potential betweenthese two groups was significantly different (p < 0.01, t test).Therefore, depolarization of the postsynaptic cell is necessaryfor reliable supralinear summation after simultaneous activationof two inputs. There was no significant difference in the meanSI of supralinear interaction observed under a depolarized conditionbetween LH and vertical input interaction (SI = 1.47 ± 0.28) andLH and SH input interaction (SI = 1.43 ± 0.19, p > 0.5, t test).The mean SIs of the linear interaction at the resting membranepotential were 0.95 ± 0.05 for LH and vertical input interaction(n = 21) and 0.89 ± 0.08 for LH and SH input interaction (n =11), and the difference was statistically significant (p < 0.05,t test).

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Figure 9. Induction of nonlinear interaction by concurrent activation of two inputs depends on the depolarization of membrane potential. Summation indices of cells were plotted against the membrane potential of postsynaptic cells. When two inputs are summated linearly, the SI takes the value of 1. Each point represents data from one cell (n = 26 for LH and vertical input interaction, n = 16 for LH and SH input interaction). For the interaction between LH and SH inputs, linear (or slightly sublinear) summation was observed at the resting membrane potential. Induction of supralinear summation is clearly dependent on the depolarization of the postsynaptic cell for both input interactions.

To assess the temporal nature of the interaction between the two inputs via different pathways, the ISI for two successivestimulations was varied between 0 and 200 msec (Fig. 10). The EPSPsevoked by simultaneous or successive activation of LH and verticalinputs were linearly summated for all the tested ISIs at the restingmembrane potential (Fig. 10A-C, D, filled circles). The averageSIs of the LH and SH input interaction were <1.0 for ISIs of <20msec (Fig. 10, open circles). Thus, two inputs coming via differentpathways interacted linearly at all tested ISIs, whereas thosearriving from a single pathway exhibited nonlinear interactionin the case of an ISI of <100 msec (Fig. 6).

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Figure 10. Temporal interaction between LH and vertical or SH inputs. EPSPs evoked by individual stimulation (A, B) and concurrent stimulation of the two inputs (C). C, EPSPs were linearly summated by concurrent stimulation of both LH and vertical inputs with all tested ISIs. V_m = $-$ 77 mV. The morphology of this pair is shown in Figure 3B. D, The mean SIs (± SD) were plotted against the tested ISIs. The graph shows pooled data from six cells for LH and vertical inputs and six cells for LH and SH inputs. The SIs of the interaction between LH and SH inputs are <1 for ISIs of <50 msec.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The primary objective of this study is to describe the synaptic interactions between horizontal and vertical connections inthe superficial layers of the kitten visual cortex. It is quiteimportant to understand exactly what happens in cells when particularinput pathways are activated for the understanding of the corticalstrategies for informationprocessing.

Cell separation and amplitude of EPSPs

We used young animals (P29-P35) at the peak of the critical period for cortical plasticity (Hubel and Wiesel, 1970). Morphologicalstudies have demonstrated that the horizontal axons at this ageare already fully elongated and adopt a clustered appearance inthe cat visual cortex (Callaway and Katz, 1990; Galuske and Singer,1996). Indeed, we found that the horizontal inputs were functionaland interacted with other inputs reasonably well. Analysis ofthe relationship between the cell distance and the peak amplitudeof the EPSPs after horizontal input activation (Fig. 2) revealedthat the EPSP amplitudes for cell pairs located within 600 µmshowed diverse values of between 0.6 and 9.3 mV (average, 4.0± 2.2 mV), whereas those for pairs located >600 µm apart wererelatively small (2.3 ± 0.8 mV). This result suggests that lateralexcitatory inputs originating from single cells more than 600µm away are less influential than those from cells within 600µm. One possible explanation is that the synapses of the horizontalinputs that arose from cells more than 600 µm apart were targetedto remote sites on the dendritic tree of the postsynaptic cells,and passive dendritic filtering reduced the amplitudes of theEPSPs. However, we found no significant difference in the risetime of the EPSPs between cell pairs separated by distances of<600 µm and those separated by distances of >600 µm. Therefore,there seems to be no difference in the dendritic filtering effectsbetween these two groups, because the rise time is one of theelectrophysiological parameters reflecting differences in electrotonicfiltering. Another possibility is that the number of synapticconnection between remote pyramidal cells is smaller than thatbetween nearby cells and/or that the synaptic conductance of remoteinputs is relatively small compared to that from closer cells.Further studies are necessary to assess thesepossibilities.

Source of vertical inputs

In the present study, we focally stimulated layer IV precisely underneath the recorded postsynaptic cell with a stimulus intensitycapable of eliciting a unitary EPSP. We were unable to determinethe source of vertical input in the individual cases tested, however,they were considered as mainly reflecting the inputs from layerIV spiny stellate cells to the superficial pyramids, because theaxons of layer IV spiny neurons project densely into the superficiallayers (Gilbert and Wiesel, 1979; Lund et al., 1979; Martin andWhitteridge, 1984), whereas thalamic afferents rarely projectin the superficial layers (Garey and Powell 1971; LeVay and Gilbert,1976).

Integration of excitation evoked by two different input pathways

When two inputs arrived at a pyramidal cell via different pathways, linear or nonlinear summation of the evoked EPSPs wasnoted depending on the membrane potential (Figs. 7-9). In the interactionbetween the two inputs, particularly that between LH and SH inputs,the summation indices of a majority of cases tested at the restingmembrane potential were slightly smaller than 1.0 (Fig. 9). Therefore,it might be more appropriately called a slight sublinear summationthan a linear summation. Such sublinear summation is also reportedfor two input interactions at the distal apical dendrites of CA1pyramidal cells in rat hippocampal slices (Cash and Yuste, 1999).In that study, the shunting caused by activation of transientA-type potassium-ion channels in dendrites was suggested to bethe underlying mechanism of the sublinear summation. We observedtransient sublinear summation when two inputs arrived at a postsynapticcell within a short interval (ISI < 50 msec, Fig. 10). Therefore,a similar transient increase in conductance may be responsiblefor thisphenomenon.

Under the depolarized condition, the EPSPs evoked by simultaneous activation of either the LH and SH inputs or the LH andvertical inputs were larger than the simple sum of the two EPSPsevoked by individual activation of either. Although the mechanismresponsible for the supralinear summation of membrane responsesis not yet clear, our results suggest that a threshold mechanismunderlies the switching from the linear to supralinear EPSP summation(Figs. 8, 9). Supralinear interaction may possibly be mediatedby the NMDA receptors (Thomson, 1997; Cash and Yuste, 1999) and/orvoltage-dependent conductance in dendrites (Cash and Yuste, 1999;Larkum et al., 1999). Hirsch and Gilbert (1991) previously reportedthat a voltage-dependent enhancement of EPSPs could be evokedby massive stimulation of horizontal pathways in the superficiallayers. Such an enhancement was reported to be mediated by voltage-sensitiveNa⁺ channels (Hirsch and Gilbert, 1991), although there is also evidencefor NMDA receptor-mediated enhancement of EPSPs (Thomson, 1997).More recently, Larkum et al. (1999) reported that an axonal actionpotential facilitates the initiation of voltage-dependent Ca²⁺ action potentials in dendrites when it coincides with dendriticinputs in rat somatosensorycortex.

We found that the voltage-dependent enhancement of EPSPs could be observed in a very simple scheme that included only a pyramidalcell and two single input pathways. It is, therefore, suggestedthat the observed nonlinear summation is attributable to the intrinsicmembrane properties of the pyramidal cells or the synaptic propertiesof the inputs, rather than the properties of the global neuronalcircuitry. This augmentation capacity of horizontal input suggestsan important role of horizontal connections in information processingin the visual cortex based on the after argument. In our results,horizontal inputs interacted synergistically with vertical inputs.Because horizontal projections are known to connect neurons whichshare similar functional properties, such as orientation or chromaticpreference for visual stimuli (Ts'o and Gilbert, 1988; Gilbertand Wiesel, 1989), their activation might have a function in theselection of cell assemblies suitable for the analysis of a specificfeature of visual stimuli. When abundant excitatory vertical inputsare present in the superficial layers, the augmentation of EPSPsin a particular group of pyramidal cells caused by horizontalinputs will accentuate the output of the cell assembly relatedto the specific stimulusfeature.

Comparison of properties between horizontal and vertical inputs

We observed paired-pulse depression in the transmission between proximal pyramidal cells in the kitten visual cortex (Figs.4C,D, 5B), with results similar to those reported for the ratvisual cortex (Thomson et al., 1993; Thomson and West, 1993; Markramand Tsodyks, 1996). Additionally, we found that such depressionwas also induced in the LH input pathway (Figs. 4A,B, 5A). However,Reyes and Sakmann (1999) reported that paired-pulse stimulationof connections between layer II/III pyramidal cells situated close-byin P28 rats induced facilitation of the second EPSP, whereas itinduced weak depression or no significant effect in younger (P14)rats. There is a discrepancy between their results and ours, becausewe found only paired-pulse depression for SH inputs. There mightbe a species difference in the mechanism of this short-term modification,or, alternatively, the visual cortex of kittens of P29-P35 mightbe less mature than that of P28 rat in this respect. Unfortunately,we did not test high-frequency stimulation of individual inputpathways and could not describe the depression during trains dependingon the frequency (Markram and Tsodyks, 1996; Abbott et al., 1997).However, we tested two successive stimulations at several differentISIs (Fig. 6). Paired-pulse depression was more consistently observedfor the horizontal connections than for the vertical connectionfor ISIs of <100 msec (Figs. 4-6).

The aforementioned results suggest that the depression of horizontal input with short ISI could be involved in the suppressivemodulation of visual responses by stimuli outside of the receptivefield (Blakemore and Tobin, 1972; Nelson and Frost, 1978; VanEssen et al., 1989; Li and Li, 1994; Sengpiel et al., 1997) orthe response adaptation to high-contrast visual stimuli (Movshonand Lennie, 1979; Ohzawa et al., 1982, 1985; Carandini and Ferster,1997). Stimulus specificity of such suppressive phenomena in thevisual cortex in vivo could be explained by stimulus-specifichorizontalconnection.

The EPSPs evoked by stimulation of vertical input exhibited different properties from those evoked by stimulation of horizontalinput, that is, the former were relatively larger in amplitudeand showed smaller fluctuations from trial to trial (Table 1).Because vertical inputs from layer IV to the superficial layerscarry information of the primary stage, the reliability of synaptictransmission might be more secure than in other synapses in thevisual cortex. Partly in support of this notion, it has been reportedthat a much larger number of channels are involved in unitaryEPSPs at geniculocortical synapses than at synapses between pyramidalcells in layer II/III (Stratford et al., 1996; Yoshimura et al.,1999), and also in the present study, the paired-pulse stimulationof vertical inputs led to paired-pulse depression less often thandid paired-pulse stimulation of horizontal inputs (Figs. 4-6).

On the other hand, a single excitatory connection between pyramidal cells in layer II/III may elicit a relatively small excitationin a postsynaptic cell and, consequently, the pyramidal cell inlayer II/III requires the convergence of several excitatory inputsto fire. This, in turn, means that pyramidal cells have a widedynamic range for the modulation of responses to vertical inputsaccording to the activity of the surrounding neuronal networks.Thus, the activity of pyramidal cells in layer II/III seems tobe controlled by the activity of many horizontally connected cells,which may form the basis for context-dependent modulation of theresponses of cortical neurons (Van Essen et al., 1989; Kapadiaet al., 1995; Sillito et al., 1995; Akasaki et al., 1998; Polatet al., 1998).

  FOOTNOTES

Received July 26, 1999; revised Nov. 30, 1999; accepted Dec. 10, 1999.

This work was supported in part by the Research for the Future Program (RFTF) Grant JSPS-RFTF 98L00201 from the Japan Societyfor the Promotion of Science (JSPS), and in part by JSPS fellowshipsfor Japanese Junior Scientists and Kanehara Memorial Foundation(Y.Y.). We thank Dr. K. Fox for critical reading of this manuscript,Dr. Y. Komatsu for helpful discussions, and Mr. T. Shiomitsu fortechnicalassistance.
Correspondence should be addressed to Dr. Yumiko Yoshimura, Department of Visual Neuroscience, Research Institute of EnvironmentalMedicine, Nagoya University, Furo-cho, Chikusa-ku, Nagoya, Aichi,464-8601, Japan. E-mail: yyumiko{at}riem.nagoya-u.ac.jp.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Abbott LF, Varela JA, Sen K, Nelson SB (1997) Synaptic depression and cortical gain control. Science 275:220-224.
Akasaki T, Yoshimura Y, Sato H (1998) Modulation of visual response properties by stimulus outside of the classical receptive field in cat area 17. Neurosci Res 22:S180.344.
Allen C, Stevens CF (1994) An evaluation of causes for unreliability of synaptic transmission. Proc Natl Acad Sci USA 91:10380-10383[Abstract/Free Full Text].
Blakemore C, Tobin EA (1972) Lateral inhibition between orientation detectors in the cat's visual cortex. Exp Brain Res 15:439-440[ISI][Medline].
Callaway EM, Katz LC (1990) Emergence and refinement of clustered horizontal connections in cat striate cortex. J Neurosci 10:1134-1153[Abstract].
Carandini M, Ferster D (1997) A tonic hyperpolarization underlying contrast adaptation in cat visual cortex. Science 276:949-952[Abstract/Free Full Text].
Cash S, Yuste R (1999) Linear summation of excitatory inputs by CA1 Pyramidal neurons. Neuron 22:383-394[ISI][Medline].
Fisken RA, Garey LJ, Powell TP (1975) The intrinsic, association and commissural connections of area 17 on the visual cortex. Proc R Soc Lond B Biol Sci 272:487-536.
Galuske RA, Singer W (1996) The origin and topography of long-range intrinsic projections in cat visual cortex: a developmental study. Cereb Cortex 6:417-430[Abstract/Free Full Text].
Garey LJ, Powell TP (1971) An experimental study of the termination of the lateral geniculo-cortical pathway in the cat and monkey. Proc R Soc Lond B Biol Sci 179:41-63[Medline].
Gilbert CD (1983) Microcircuitry of the visual cortex. Annu Rev Neurosci 6:217-247[ISI][Medline].
Gilbert CD (1992) Horizontal integration and cortical dynamics. Neuron 9:1-13[ISI][Medline].
Gilbert CD, Wiesel TN (1979) Morphology and intracortical projections of functionally characterised neurones in the cat visual cortex. Nature 280:120-125[Medline].
Gilbert CD, Wiesel TN (1989) Columnar specificity of intrinsic horizontal and cortico-cortical connections in cat visual cortex. J Neurosci 9:2432-2442[Abstract].
Hata Y, Tsumoto T, Sato H, Tamura H (1991) Horizontal interactions between visual cortical neurones studied by cross-correlation analysis in the cat. J Physiol (Lond) 441:593-614[Abstract/Free Full Text].
Hirsch JA, Gilbert CD (1991) Synaptic physiology of horizontal connections in the cat's visual cortex. J Neurosci 11:1800-1809[Abstract].
Horikawa K, Armstrong WE (1988) A versatile means of intracellular labeling: injection of biocytin and its detection with avidin conjugates. J Neurosci Methods 25:1-11[ISI][Medline].
Hubel D H, Wiesel TN (1970) The period of susceptibility to the physiological effects of unilateral eye closure in kittens. J Physiol (Lond) 206:419-436[Abstract/Free Full Text].
Kapadia MK, Ito M, Gilbert CD, Westheimer G (1995) Improvement in visual sensitivity by changes in local context: parallel studies in human observers and in V1 of alert monkeys. Neuron 15:843-856[ISI][Medline].
Katz L, Weliky M, Dalva M (1997) Relationships between local synaptic connections and orientation domains in primary visual cortex. Neuron 19:871-880[ISI][Medline].
Larkum ME, Zhu JJ, Sakmann B (1999) A new cellular mechanism for coupling inputs arriving at different cortical layers. Nature 398:338-341[Medline].
LeVay S, Gilbert CD (1976) Laminar patterns of geniculocortical projection in the cat. Brain Res 113:1-19[ISI][Medline].
Li C-Y, Li W (1994) Extensive integration field beyond the classical receptive field of cat's striate cortical neurons: classification and tuning properties. Vision Res 34:2337-2355[ISI][Medline].
Lund JS, Henry GH, Macqueen CL, Harvey AR (1979) Anatomical organization of the primary visual cortex (area 17) of the cat. A comparison with area 17 of the macaque monkey. J Comp Neurol 184:599-618[ISI][Medline].
Markram H, Tsodyks M (1996) Redistribuion of synaptic efficacy between neocortical pyramidal cells. Nature 382:807-810[Medline].
Martin KAC, Whitteridge DJ (1984) Form, function and intracortical projections of spiny neurones in the striate visual cortex of the cat. J Physiol (Lond) 353:463-504[Abstract/Free Full Text].
Mason A, Larkman A (1990) Correlations between morphology and electrophysiology of pyramidal neurons in slices of rat visual cortex. II. Electrophysiology. J Neurosci 10:1415-1428[Abstract].
Movshon JA, Lennie P (1979) Pattern-selective adaptation in visual cortical neurones. Nature 278:850-852[Medline].
Nelson JI, Frost BJ (1978) Orientation-selective inhibition from beyond the classic visual receptive field. Brain Res 139:359-365[ISI][Medline].
Ohzawa I, Sclar G, Freeman RD (1982) Contrast gain control in the visual cortex. Nature 298:266-268[Medline].
Ohzawa I, Sclar G, Freeman RD (1985) Contrast gain control in the cat's visual system. J Neurophysiol 54:651-667[Abstract/Free Full Text].
Polat U, Mizobe K, Pettet MW, Kasamatsu T, Norcia AM (1998) Collinear stimuli regulate visual responses depending on cell's contrast threshold. Nature 391:580-584[Medline].
Reyes A, Sakmann B (1999) Developmental switch in the short-term modification of unitary EPSPs evoked in layer 2/3 and layer 5 pyramidal neurons of rat neocortex. J Neurosci 19:3827-3835[Abstract/Free Full Text].
Sengpiel F, Sen A, Blakemore C (1997) Characteristics of surround inhibition in cat area 17. Exp Brain Res 116:216-228[ISI][Medline].
Sillito A M, Grieve KL, Jones HE, Cudeiro J, Davis J (1995) Visual cortical mechanisms detecting focal orientation discontinuities. Nature 378:492-496[Medline].
Stern P, Edwards F, Sakmann B (1992) Fast and slow components of unitary EPSCs on stellate cells elicited by focal stimulation in slices of rat visual cortex. J Physiol (Lond) 449:247-278[Abstract/Free Full Text].
Stratford KJ, Tarczy-Hornoch K, Martin KAC, Bannister NJ, Jack JJB (1996) Excitatory synaptic inputs to spiny stellate cells in cat visual cortex. Nature 382:258-261[Medline].
Thomson AM (1997) Activity-dependent properties of synaptic transmission at two classes of connections made by rat neocortical pyramidal axons in vitro. J Physiol (Lond) 502:131-147[ISI][Medline].
Thomson AM, West DC (1993) Fluctuations in pyramid-pyramid excitatory postsynaptic potentials modified by presynaptic firing pattern and postsynaptic membrane potential using paired intracellular recording in rat neocortex. Neuroscience 54:329-346[ISI][Medline].
Thomson AM, Deuchars J, West DC (1993) Large, deep layer pyramid-pyramid single axon EPSPs in slices of rat motor cortex display paired pulse and frequency-dependent depression, mediated presynaptically and self-facilitation, mediated postsynaptically. J Neurophysiol 70:2354-2369[Abstract/Free Full Text].
Ts'o DY, Gilbert CD (1988) The organization of chromatic and spatial interactions in the primate striate cortex. J Neurosci 8:1712-1727[Abstract].
Ts'o DY, Gilbert CD, Wiesel TN (1986) Relationships between horizontal interactions and functional architecture in cat striate cortex as revealed by cross-correlation analysis. J Neurosci 6:1160-1170[Abstract].
Van Essen DC, De Yoe EA, Olavarria JF, Knierim JJ, Fox JM, Sagi D, Julesz B (1989) Neural responses to static and moving texture patterns in visual cortex of the macaque monkey. In: Neural mechanisms of visual perception (Lam DM-K, Gilbert CD, eds), pp 137-154. Woodlands, TX: Portfolio.
Weliky M, Kandler K, Fitzpatrick D, Katz L (1995) Patterns of excitation and inhibition evoked by horizontal connections in visual cortex share a common relationship to orientation columns. Neuron 15:541-552[ISI][Medline].
Yoshimura Y, Tsumoto T (1994) Dependence of LTP induction on postsynaptic depolarization: a perforated patch-clamp study in visual cortical slices of young rats. J Neurophysiol 71:1638-1645[Abstract/Free Full Text].
Yoshimura Y, Kimura F, Tsumoto T (1999) Estimation of single channel conductance underlying synaptic transmission between pyramidal cells in the visual cortex. Neuroscience 88:347-352[ISI][Medline].

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