Developmental Synaptic Changes Increase the Range of Integrative Capabilities of an Identified Excitatory Neocortical Connection

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The Journal of Neuroscience, March 1, 1999, 19(5):1566-1576

Developmental Synaptic Changes Increase the Range of Integrative Capabilities of an Identified Excitatory Neocortical Connection
María Cecilia Angulo¹, Jochen F. Staiger², Jean Rossier¹, and Etienne Audinat¹
¹ Neurobiologie et Diversité Cellulaire, Centre National de la Recherche Scientifique, Unité Mixte de Recherche 7637, Ecole Supérieure de Physique et de Chimie Industrielles de la ville de Paris, 75231 Paris Cedex 5, France, and ² Heinrich-Heine University, C & O Vogt Institute for Brain Research, D-40001 Düsseldorf, Germany

  ABSTRACT

Top
Abstract
Introduction
References

Excitatory synaptic transmission between pyramidal cells and fast-spiking (FS) interneurons of layer V of the motor cortexwas investigated in acute slices by using paired recordings at30°C combined with morphological analysis. The presynaptic andpostsynaptic properties at these identified central synapses werecompared between 3- and 5-week-old rats. At these two postnataldevelopmental stages, unitary EPSCs were mediated by the activationof AMPA receptors with fast kinetics at a holding potential of $-$ 72 mV. The amplitude distribution analysis of the EPSCs indicatesthat, at both stages, pyramidal-FS connections consisted of multiplefunctional release sites. The apparent quantal size obtained bydecreasing the external calcium ([Ca²⁺]_e) varied from 11 to 29 pA near resting membrane potential. Inyoung rats, pairs of presynaptic action potentials elicited unitarysynaptic responses that displayed paired-pulse depression at alltested frequencies. In older animals, inputs from different pyramidalcells onto the same FS interneuron had different paired-pulseresponse characteristics and, at most of these connections, aswitch from depression to facilitation occurred when decreasingthe rate of presynaptic stimulation. The balance between facilitationand depression endows pyramidal-FS connections from 5-week-oldanimals with wide integrative capabilities and confers uniquefunctional properties to eachsynapse.

Key words: paired recordings; pyramidal cell; interneuron; synaptic plasticity; depression; facilitation; basket cell; fast-spiking cell; glutamate release

  INTRODUCTION

Top
Abstract
Introduction
References

Activity-dependent mechanisms dynamically regulate the efficacy of synaptic transmission and the strength of a given synapselargely results from the activity it has previously experienced.Short-term changes that adjust the synaptic gain according torecent activity have been described at most synapses. After asingle action potential or a train of action potentials in thepresynaptic axon, the subsequent postsynaptic responses that occurduring the following hundreds of milliseconds can be either facilitatedor depressed. These activity-dependent modulations of synapticresponses depend largely on presynaptic mechanisms (Zucker, 1989;Stevens and Wang, 1995), the development of which, however, isalso influenced by the identity of the postsynaptic targets. Ininvertebrates (Muller and Nicholls, 1974; Davis and Murphey, 1993;Katz et al., 1993) and in the mammalian peripheral (Koerber andMendell, 1991) and CNSs (Thomson, 1997; Markram et al., 1998;Reyes et al., 1998; Scanziani et al., 1998), different terminalsfrom the same presynaptic axon may constitute either facilitatingor depressing synapses according to the target cells. The facilitatingor depressing characteristics of a synapse will greatly influencehow the firing rates and the temporal pattern of presynaptic actionpotentials are transferred to postsynaptic neurons (Tsodyks andMarkram, 1997).

Within the neocortex, information processing relies on the synaptic interactions involving pyramidal and nonpyramidal cells.Pyramidal cells are excitatory glutamatergic neurons that conveythe output signals of the neocortex but also provide most of theintracortical excitatory synaptic drive. Nonpyramidal cells aremainly inhibitory local circuit neurons using GABA as neurotransmitter.Excitatory responses at synapses between neocortical pyramidalcells are characterized by a frequency-dependent depression duringdischarges of pairs or trains of presynaptic action potentials,whereas synapses from pyramidal cells onto interneurons can displayeither facilitation or depression (Thomson et al., 1993; Deucharset al., 1994; Buhl et al., 1997; Markram et al., 1997; Thomson,1997; Galarreta and Hestrin, 1998; Reyes et al., 1998). This heterogeneityamong pyramidal-interneuron synapses is probably caused by thediversity of nonpyramidal cells, which has made difficult thecharacterization of synaptic and integrative properties of specificsubtypes of interneurons (Kawaguchi, 1993, 1995; Cauli et al.,1997; Parra et al., 1998).

We focused our attention on the excitatory synapses made by pyramidal cells onto a discrete subtype of neocortical interneuron.These interneurons, called fast-spiking (FS) cells, can be identifiedby their ability to fire fast action potentials at high nonaccommodatingfrequencies (McCormick et al., 1985; Kawaguchi, 1993; Cauli etal., 1997). Most of these cells express the calcium-binding proteinparvalbumin (Kawaguchi, 1995; Cauli et al., 1997), and their axonsform multiple axoaxonic (chandelier cells) or axosomatic (basketcells) contacts (Kawaguchi, 1995) preferentially on pyramidalcells. This morphological feature suggests a powerful role ofFS cells in regulating the neocortical output. The control ofFS cell activity and, therefore, their integration of excitatoryinputs is likely to play a major role in balancing excitationand inhibition and/or in maintaining temporal coherence in thecortical network (Cobb et al., 1995; Whittington et al., 1995;Buzsaki, 1997).

In the present work, we first characterized the basic presynaptic and postsynaptic properties at the pyramidal cell to FSinterneuron connection in layer V of the rat motor cortex. Wethen studied the paired-pulse response characteristics at thiscentral synapse. Our results show that in 3-week-old rats, pyramidal-FSidentified synapses depress at all tested frequencies. In contrast,paired-pulse depression (PPD) and paired-pulse facilitation (PPF)coexisted in connections from 5-week-old rats, indicating thatthe range of integrative capabilities largely increased afterthe third postnatalweek.

  MATERIALS AND METHODS

Brain slice preparation. Wistar rats [postnatal days 14-20 (P14-P20) and P27-P36] were anesthetized by an intraperitonealinjection of ketamine (65 mg/kg) and xylazin (14 mg/kg) and decapitated.Brains were quickly removed, and 300-µm-thick parasagittal sectionsof cerebral motor cortex were prepared as previously described(Cauli et al., 1997). The slices were incubated for 1 hr in aphysiological extracellular saline solution containing (in mM):NaCl, 121.0; KCl, 2.5; NaH₂PO₄, 1.25; CaCl₂, 2; MgCl₂, 1; NaHCO₃,26; glucose, 20; and pyruvate 5, and bubbled with a mixture of95% O₂ and 5% CO₂. For recordings, they were transferred to achamber and perfused at 1-2 ml/min with the same physiologicalextracellular saline solution at 30°C.

Paired recordings. Paired recordings from synaptically coupled pyramidal and FS neurons were obtained by using sharp intracellularand patch microelectrodes,respectively.

Postsynaptic FS cells were initially identified using videomicroscopy with Nomarski optics under infrared illumination (Stuartet al., 1993). Neurons with pyramidal or bipolar-like shapes wereexcluded from the sample. Furthermore, the kinetics of the actionpotential firing of recorded cells was analyzed to take into accountonly those with electrophysiological patterns of FS cells (seedata collection and analysis; Connors and Gutnick, 1990; Kawaguchi,1995; Cauli et al., 1997). Patch pipettes were pulled from borosilicateglass tubing and had a resistance of 3-5 M $Omega$ when filled with aninternal solution containing (in mM): 144 K-gluconate, 3 MgCl₂,0.2 EGTA, and 10 HEPES, pH 7.2-7.4, 300 mOsm. Two milligrams permilliliter biocytin was also included to study the morphologyof postsynaptic cells (see Morphology). In 20 experiments, weused 100 µM spermine and, in five experiments, we used 4 mM ATPand 0.4 mM GTP into the patch pipette. We did not observe anydifference between recordings performed with and without thesecompounds for the parameters measured in the presentwork.

Whole-cell recordings were performed from layer V FS interneurons. The holding potential was set to $-$ 60 mV on the patch-clampamplifier for all postsynaptic interneurons that gave a membranepotential of $-$ 72 mV after correction for junction potentials (Neher,1992). Only cells with resting membrane potentials more negativethan $-$ 50 mV were furtherconsidered.

Unitary EPSCs were studied in control conditions and after adding AMPA/kainate antagonists DNQX or NBQX in the external solution(10 µM; Tocris Cookson, Bristol, UK). In experiments in whichthe [Ca²⁺]_e was reduced from 2 or 3 mM to 0.5 mM, the external [Mg²⁺]_e was increased to 2.5 mM.

After whole-cell recordings were established, presynaptic neurons were impaled with a sharp microelectrode filled with 3 MKCl or 1.5 M KCl and 2% biocytin (resistance, 40-120 M $Omega$ ). Pyramidalcells were initially identified by their characteristic actionpotential firing induced by depolarizing current pulses (McCormicket al., 1985; Connors and Gutnick, 1990; Cauli et al., 1997).The identification of the presynaptic cells was further confirmedby their characteristic features obtained by biocytin labeling(see Morphology). The impaled presynaptic cells were iontophoreticallyinjected with biocytin by applying depolarizing current pulsesat the end of the experiment (2-3 nA, 5-15 min). Postsynapticresponses were induced by triggering action potentials in thepresynaptic cell with depolarizing pulses (3 msec, 1.5 nA). Thelatency of these responses was measured from the peak of the presynapticaction potential. Monosynaptic coupling between the two neuronswere considered when EPSCs were elicited with brief latencies(Table 1). The stability of the recordings during the time courseof the experiment was tested by plotting the EPSC amplitudes againsttime. A run down of the synaptic responses was rarely observed.In our experimental conditions, the peak amplitude and the probabilityof response of the EPSCs could remain stable for up to 3 hr ofrecording.


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Table 1. Action potential firing and unitary EPSC properties of postsynaptic FS interneurons at two different developmental stages

Data collection and analysis. Whole-cell current-clamp (mode I-Clamp fast) and voltage-clamp recordings of postsynaptic FScells were obtained using a patch-clamp amplifier (Axopatch 200A;Axon Instruments, Foster City, CA) and filtered at 5 and 2 kHz,respectively. Series resistances between 10 and 25 M $Omega$ were monitoredthroughout the experiments, but they were not compensated. Intracellularcurrent-clamp recordings of presynaptic pyramidal cells were obtainedusing an intracellular amplifier (Neuro Data; Instruments Corp.).Digitized data were acquired and analyzed off-line using Acquis1software (Gérard Sadoc, Centre National de la Recherche Scientifique,Gif-sur-Yvette,France).

The characteristics of the action potential discharges of postsynaptic cells were analyzed after the procedure described byCauli et al. (1997). The accommodation parameters were measuredon discharges elicited by application of 800 msec depolarizingcurrent pulses. The instantaneous discharge frequency was determinedthroughout the discharge and plotted as a function of time atthe different stimulation intensities. The instantaneous dischargefrequencies between the first two spikes (f_initial), 200 msecafter the beginning of the discharge (f₂₀₀), and at the end ofthe stimulation (f_final) were then measured at the highest intensitytested (550-1200 pA). Early and late accommodations were calculatedaccording to (f_initial $-$ f₂₀₀)/f_initial and (f₂₀₀ $-$ f_final)/f_initial,respectively. We also measured the spike amplitude (A) and duration(t_1/2), the AHP amplitude of the first and second actionpotentials of the discharges, and the resting membrane potentials(V_rmp) and input resistances (R_in), as previously described (seeCauli et al., 1997 fordetails).

Means of elicited EPSCs were obtained by averaging the traces after the first presynaptic action potential was aligned usingautomatic peak detection. Traces not showing postsynaptic responses>150% of the noise level were considered failures. The mean risetime (20-80%) of EPSCs calculated by averaging the synaptic currentswithout failures was 0.33 ± 0.06 msec (n = 29) and 0.28 ± 0.06msec (n = 15) in 3- and 5-week-old rats, respectively. No significantcorrelation was found between the mean rise time and the averagedamplitude or decay time constant of the EPSCs, indicating a lowfiltering of the elicited synaptic current in the connectionsstudied (p > 0.05; Student's ttest).

To examine the paired-pulse response characteristics of the EPSCs, pairs of single action potentials were elicited in presynapticcells by applying two short depolarizing current pulses separatedusually by 50 msec, at different frequencies of stimulation (1and 0.2 Hz). The paired-pulse response was studied by measuringthe amplitudes of the first EPSC (EPSC1) and second EPSC (EPSC2)from the baseline preceding each EPSC and by calculating the ratioamplitude EPSC2/amplitude EPSC1. We tested the recovery from depressionand the recovery from facilitation of the elicited responses byvarying the interspike interval (from 15 to 200 msec) at stimulationrates of 1 and 0.2 Hz. The coefficient of variation was calculatedafter baseline noise subtraction by dividing the SD by themean.

Statistics. The statistical significance of the difference between means of two unpaired samples was computed with the nonparametricalMann-Whitney U test. The Wilcoxon t test was used to compare themeans of two related samples, and correlations between these sampleswere tested with the nonparametrical Spearman test. For data presentingtoo many ties, the statistical significance of the means was analyzedwith a Student's t test. Statistical data are given as mean ±SD.

Morphology. The slices containing biocytin-filled cells were fixed overnight in 4% paraformaldehyde and 0.2% glutaraldehydein 0.1 M phosphate buffer (PB) at 4°C. Then, they were rinsedextensively with PB including an intermediate blocking step forendogenous peroxidase activity with 1% H₂O₂ (in PB). The nextstep was an incubation in a cryoprotectant (30% saccharose inPB) for 1 hr. Then, the slices were freeze-thawed three timesover liquid nitrogen. After three rinses in PB, the slices wereincubated with ABC (1:200; Vector Laboratories, Burlingame, CA)overnight at 4°C. Thereafter, 1 mg/ml 3,3' diaminobenzidine (Sigma,St. Louis, MO) was preincubated for 10 min, and then the peroxidasewas revealed by starting the reaction with 0.01% H₂O₂. The reactionwas stopped by rinsing with PB, and the slices were resectionedon a vibratome to sections of 50 µm thickness. These were intensifiedwith 1% OsO₄ (in PB) for 1 hr, dehydrated in an ascending seriesof ethanol (including contrasting with 1% uranyl acetate in 70%ethanol for 45 min). After immersion in propylene oxide, the sectionswere flat-embedded in Durcupan ACM (Fluka, Buchs, Switzerland).Sections were examined with a Zeiss Axioplan equipped with a drawingtube and a 100× oil immersionobjective.

  RESULTS

We studied the presynaptic and postsynaptic properties of pyramidal cell to FS interneuron connections by using paired recordingsat two different postnatal developmental stages. The excitatorysynaptic transmission at this identified central synapse was examinedin 40 pairs of cells from 3-week-old rats and in 25 pairs of 5-week-oldrats. Presynaptic pyramidal cells were impaled with sharp intracellularmicroelectrodes, and unitary EPSCs were recorded in FS cells withpatch pipettes in layer V of the motor cortex (see Materials andMethods).

Identification of the pyramidal cell to FS putative basket interneuron connections

Interneurons of the neocortex are characterized by a large morphological and functional diversity. To restrict our analysisto a single discrete subpopulation, we therefore included in thepresent study only the FS cells located in layer V that had anapparent multipolar shape as seen with infrared videomicroscopyand nonaccommodating fast-spiking discharges as a physiologicalhallmark. Figure 1B illustrates the firing behavior of the postsynapticnonpyramidal cells retained in the present study. This neuronemitted a single action potential at the beginning of a near-thresholdcurrent pulse, followed by a silent period and a discharge ofnonaccommodating fast action potentials. At higher stimulationintensities, all FS cells exhibited continuous high-frequencydischarges (Fig. 1B, top trace). The instantaneous firing frequencyduring such repetitive discharges was usually >100 Hz and showedlimited accommodation at all tested stimulation intensities (Table1; Fig. 1B, top trace; see Materials and Methods). In addition,all postsynaptic cells taken into consideration had short spikedurations (t_1/2), large afterhyperpolarizations (AHPs), smallinput resistances (R_in), and hyperpolarized resting membrane potentials(V_rmp; Table 1). These electrophysiological properties are characteristicof FS nonpyramidal cells in the neocortex (Kawaguchi, 1995; Cauliet al., 1997).

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Figure 1. Electrophysiological characterization of connected pyramidal cells and FS interneurons from 18-d-old rats. A, Current-clamp recordings of a pyramidal cell during injection of current pulses with a sharp intracellular electrode. In response to near-threshold current pulses, the pyramidal cell emitted a single action potential with a slow AHP (middle voltage trace). Note the slow action potentials and the accommodation of the firing during larger depolarizing current pulses (top voltage trace) and the time-dependent rectification in response to hyperpolarizing current pulses (bottom voltage trace). Recordings are from the pyramidal cell shown in Figure 2A. B, Current-clamp recordings of a FS interneuron during injection of current pulses with a patch pipette. In response to near-threshold current pulses (middle voltage trace), this FS cell emitted a single fast action potential with a large fast AHP followed by a silent period and a late discharge of action potentials. Application of a larger depolarizing current (top voltage trace) induced a continuous discharge at high frequency. Note the low input resistance of the FS neuron as seen in response to hyperpolarizing current pulses (bottom voltage trace). Recordings are from the FS cell shown in Figure 2B-D. C, Unitary EPSCs at a pyramidal-FS connection. The top trace illustrates an action potential elicited in the pyramidal neuron by a brief depolarizing current pulse (middle voltage trace). The bottom traces are four superimposed current responses recorded in the FS interneuron at a holding potential of $-$ 72 mV during the stimulation of the pyramidal neuron. Note an apparent transmission failure and the large variation of the EPSC amplitudes. Recordings are from the connection illustrated in Figure 2B-D. D, Kinetics of unitary EPSCs at the same pyramidal-FS connection as in C. A biexponential fit of the decay of the EPSC was superimposed to the average of 203 postsynaptic responses, excluding failures. The numbers in parentheses represent the relative amplitude of the first ( $tau$ ₁) and the second ( $tau$ ₂) exponential.

All recorded FS neurons that were successfully stained by biocytin injection (n = 16; see Materials and Methods) were interneuronslocated in layer V that possessed round to ovoid somata (largestdiameter ranging from 15.3 to 23.1 µm). From the cell body 4-8smooth, partially beaded primary dendrites originated with variableorientations (Fig. 2A,B), although with a bias of ramifying moreintensely within the infragranular layers. The axon was emittedtoward the pia and branched soon and repeatedly, providing a densefield of boutons, typical of extended local plexus cells thatare regarded to be putative basket cells (Kawaguchi and Kubota,1998). In two of 16 cases we were able to identify multiple axosomaticcontacts, forming a pericellular basket around unstained cells(Fig. 2C). In most other cases only single axosomatic contactswere found to be established by the interneuron axons (putativebasket cells; Buhl et al., 1997; Tamas et al., 1997).

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Figure 2. Morphological characterization of pyramidal-FS connections from 18-d-old rats. A, Photomontage of a typical pyramidal cell (PYR) to a putative basket cell (BC) connection as recorded and stained with biocytin in the present study. Both cells have large somata located in layer V of motor cortex and possess a characteristic morphology for the respective cell class. White arrowheads mark the axon of the pyramidal cell, black arrowheads those of the interneuron. Roman numerals denominate cortical laminae. B, Camera lucida drawing showing the contact formed by another pair, also from layer V. The soma of the pyramidal cell and the skeleton of the axon until it contacts a secondary dendrite of the large multipolar putative basket cell (arrow) is traced. Axonal branch points that have not been reconstructed further are marked with an asterisk. Arrowheads indicate the axon initial segments of both cells. Stippled frame marks area shown as micrograph in D. C, Basket-like terminal formation of the axon of the interneuron shown in B. Arrowheads point to individual boutons presumably contacting the encircled soma (asterisk). D, High-power micrograph showing the pyramidal cell axon (PYR_ax), specifically the course of the recurrent collateral (arrowheads) that forms a delicate contact (arrow) with the putative basket cell dendrite (BC_den). Scale bars: A, B, 100 µm; C, D, 10 µm.

Pyramidal cells were initially identified by their characteristic action potential firing induced by depolarizing currentpulses (McCormick et al., 1985; Connors and Gutnick, 1990). Asseen in Figure 1A, pyramidal cells were mainly characterized bya strong firing accommodation (>80%), small AHPs (less than $-$ 7mV), and a long spike duration (>1.5 msec) (see Cauli et al.,1997 for details). In some experiments, biocytin was injectedin putative pyramidal cells synaptically connected to FS interneurons.The eight successfully stained presynaptic neurons were all largelayer V pyramidal cells with densely spiny dendrites (Fig. 2A).Their axons extended from the basal pole of their soma and rantoward the white matter giving off numerous recurrent collateralsforming one or two putative contacts onto primary or secondarydendrites of the FS neuron (Fig. 2A,B,D).

Functional properties of neocortical pyramidal to fast-spiking connections

For all connected pairs, action potentials elicited in the presynaptic pyramidal cell induced unitary postsynaptic responsesin the FS interneuron that had short latencies, low failure rates,and large coefficients of variation (Tables 1, 2; Fig. 1C).At a holding potential of $-$ 72 mV the average EPSC was rapidlyrising and decaying (Fig. 1D) and was almost completely abolishedby 10 µM NBQX or DNQX, two competitive antagonists of AMPA/kainatereceptors (Table 1). The decay of the average EPSC was adequatelyfitted in 37 of 54 pairs by a double exponential function (Table1, Fig. 1D). The amplitude of the second exponential representedonly a minor portion of the total current, indicating a predominanceof the fastest component (Table 1). The EPSCs of 17 connectionswere best fitted with a single exponential function (Table 1).We did not observe any significant difference between pyramidal-FSconnections from 3- and 5-week-old rats as far as the peak amplitudesand the first and second decay time constants of AMPA receptor-mediatedunitary EPSCs were concerned (Table 1; p > 0.05; Mann-WhitneyU test). In agreement with previous observations (Angulo et al.,1997), the I-V plot of the AMPA receptor-mediated unitary EPSCsshowed an inward rectification between $-$ 20 and +40 mV (M. C. Angulo,J. Rossier, and E. Audinat, unpublished observations), characteristicof calcium-permeable AMPA receptors (for review, see Jonas andBurnashev, 1995).

To determine whether pyramidal-FS connections consisted of single or multiple release sites, we manipulated the release probabilitiesby using paired-pulse stimulations of presynaptic cells and bychanging the concentration of [Ca²⁺]_e.

Figure 3 illustrates the average responses, including failures, recorded in a FS interneuron by spike pairs elicited in apyramidal cell with an interspike interval of 50 msec at a stimulationrate of 1 Hz. The comparison of the average amplitude, includingfailures, of EPSC1 to that of EPSC2 indicated that this connectionshowed a paired-pulse depression (Fig. 3A1). The paired-pulseratio (amplitude EPSC2/amplitude EPSC1) was 0.37. Failure ratesat EPSC1 and EPSC2 were 0.01 and 0.12, respectively, indicatingdifferent release probabilities at the first and second spikes.The amplitude distribution of EPSC1 and EPSC2 significantly differedwith EPSC1 amplitudes centered around larger values (Fig. 3A2,inset; p < 0.0001; Wilcoxon t test). Consequently, the mean amplitudeof EPSC1 excluding failures was larger than that of EPSC2 (datanot shown). These observations suggest that more vesicles werereleased at the first than at the second presynaptic action potential(Stevens and Wang, 1995). If no more than one vesicle is releasedat each site (for review, see Redman, 1990; Korn and Faber, 1991),then this indicates that this synapse consisted of several releasesites.

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Figure 3. Multiple quanta of transmitter released at a single pyramidal-FS connection from a 16-d-old rat. A1, B1, The bottom traces show the mean amplitude, including failures, of the postsynaptic currents (EPSC1 and EPSC2) recorded in a FS cell in response to pairs of action potentials (top traces) elicited in a presynaptic pyramidal cell with an interspike interval of 50 msec at a stimulation rate of 1 Hz in 3 mM (A1) and 0.5 mM (B1) of [Ca²⁺]_e. A marked PPD (ratio of 0.37) was observed in 3 mM [Ca²⁺]_e (A1), whereas a PPF (ratio of 1.2) was obtained when reducing [Ca²⁺]_e to 0.5 mM (B1). The response probabilities of EPSC1 and EPSC2 were, respectively, 0.99 and 0.88 in 3 mM [Ca²⁺]_e and 0.52 and 0.6 in 0.5 mM [Ca²⁺]_e. Traces are averages of 270 and 330 responses for A1 and B1, respectively. A2, B2, Amplitude distributions of EPSC1 and EPSC2, excluding failures, obtained in 3 mM [Ca²⁺]_e (A2) and 0.5 mM [Ca²⁺]_e (B2). The histograms and cumulative plots (A2, inset) show that the distribution of EPSC1 and EPSC2 were significantly different in 3 mM [Ca²⁺]_e, suggesting that multiple quanta were released at this connection. This was confirmed by the reduction in amplitude of both responses in 0.5 mM [Ca²⁺]_e (B2, inset). In low [Ca²⁺]_e, the amplitude distribution of EPSC1 and EPSC2 were identical suggesting that, under these conditions of low release probability, a single quantum was released when there was a response (B2). An apparent quantal size of $-$ 20 pA could be estimated from the current corresponding to 50% of the cumulative distribution (B2, inset).

In 44 pyramidal-FS connections from 3-week-old (n = 33) and 5-week-old (n = 11) animals, in which paired-pulse protocols wereapplied, we observed a significant difference between the averageamplitude, excluding failures, of EPSC1 and EPSC2 (Table 2; p< 0.001; Wilcoxon t test). These results suggest that, at bothinvestigated developmental stages, pyramidal-FS connections mainlyconsist of multiple functional release sites. For six connectionsfrom 3-week-old (n = 1) and 5-week-old (n = 5) rats, the amplitudes,excluding failures, and probabilities of response of EPSC1 andEPSC2 were identical, and therefore it was not possible to determinewhether they consisted of single or multiple release sites.


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Table 2. Paired-pulse response characteristics of pyramidal-FS connections at two different developmental stages

The effect of decreasing the [Ca²⁺]_e to 0.5 mM was studied on paired-pulse responses elicited at a stimulation rate of 1 Hz.As shown in the example of Figure 3B, after changing to a lowcalcium-containing bathing solution, the proportion of failuresincreased and became higher for EPSC1 than for EPSC2, leadingto a switch from depression to facilitation (Table 2). In addition,the amplitude of the EPSCs decreased as shown by the shift ofEPSC1 and EPSC2 amplitude distributions toward smaller values(Fig. 3B2, inset; p < 0.0001; Mann-Whitney U test). This decreasein response probabilities associated with a decrease of the averageamplitude without failures for both EPSC1 and EPSC2 when lowering[Ca²⁺]_e was also observed in nine other connections (Table 2; p <0.025; Wilcoxon t test). In four cases, these changes could bereversed after restoration of normal [Ca²⁺]_e (data notshown).

For four of the 10 connections from 3-week-old (n = 3) and 5-week-old (n = 1) animals for which we lowered the [Ca²⁺]_e to 0.5 mM, as in the example of Figure 3, we observed no statisticaldifferences between the cumulative amplitude distributions ofEPSC1 and EPSC2 in low [Ca²⁺]_e (Fig. 3B2, inset), although the probabilities of the two responsesdiffered (p > 0.05; Mann-Whitney U test). This suggested thatin these conditions only one quantum of transmitter was releasedon the average when there was a response. The mean amplitude ofthe EPSCs without failures recorded at these four connectionsin low [Ca²⁺]_e corresponded to the postsynaptic response to one quantum oftransmitter, i.e., the apparent quantal size, which varied from11 to 29 pA with a mean of 19 ± 8 pA (n = 4). These values arewithin those reported by Bolshakov and Siegelbaum (1995) and Geigeret al. (1997) at excitatory synapses in the hippocampus. The ratioof the mean amplitude of EPSC1 without failures in normal [Ca²⁺]_e over the apparent quantal size obtained in low [Ca²⁺]_e, gives a quantal content of 1.8, 1.9, 2.5, and 3.1 (mean, 2.3± 0.6).

These results indicate that the average number of release sites active at each response decreased when lowering [Ca²⁺]_e and confirm that pyramidal-FS connections in slices of both3- and 5-week-old rats consist of multiple functional releasesites.

Postnatal development of the activity-dependent properties of synaptic transmission at pyramidal-FS connections

As mentioned above, most of the pyramidal-FS connections examined at a stimulation rate of 1 Hz displayed PPD when pairs ofpresynaptic action potentials were elicited with an interspikeinterval of 50 msec (in 2 or 3 mM [Ca²⁺]_e). The pooled data from connections from 3-week-old (n = 38)and 5-week-old (n = 21) rats indicated, however, that the depressionwas more marked at connections obtained in slices from youngerrats (Table 2; p < 0.01; Mann-Whitney U test). Larger PPD alsooccurred in connections of the young compared with the older animalswhen interspike intervals of 15, 100, and 200 msec were used (Fig.4E). For both developmental stages, PPD decreased between intervalsof 15 and 200 msec (Fig. 4E) but this decrease of PPD was onlysignificant at connections from 3-week-old animals (p < 0.025;Mann-Whitney U test).

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Figure 4. Paired-pulse response characteristics at pyramidal-FS connections at two different developmental stages. A, B, Paired-pulse responses elicited with a presynaptic interspike interval of 50 msec (top traces) at stimulation rates of 1 (A1, B1) and 0.2 Hz (A2, B2) in FS interneurons from 19- and 35-d-old rats. The bottom traces correspond to the mean amplitudes, including failures, of the postsynaptic currents. For the connection in A, the response probabilities of EPSC1 and EPSC2 were, respectively, 0.96 and 0.93 at a stimulation rate of 1 Hz (A1) and 1 and 0.98 at a stimulation rate of 0.2 Hz (A2). For the connection in B, the response probabilities of EPSC1 and EPSC2 were, respectively, 0.99 and 1 at a stimulation rate of 1 Hz (B1) and 1 at a stimulation rate of 0.2 Hz (B2). Note that in A the connection showed a PPD at stimulation rates of 1 Hz (ratio of 0.64) and 0.2 Hz (ratio of 0.73), whereas in B the connection showed a PPD at a stimulation rate of 1 Hz (ratio of 0.89) and a PPF at 0.2 Hz (ratio of 1.2). Traces are averages from 69 to 131 responses. C, Average of the paired-pulse ratios at connections from 3-week-old rats (black bars) and 5-week-old rats (white bars). Only pairs tested at both stimulation rates were included. There was a statistical difference between the ratios obtained at 1 and 0.2 Hz for pairs from 5-week-old rats (p < 0.001; n = 11) but not for pairs from younger animals (n = 8). Note that the PPD was more marked at connections from younger animals. D, Plot of the paired-pulse ratio of all individual connections as a function of the age of the preparation at stimulation rates of 1 Hz (crosses; n = 57) and 0.2 Hz (circles; n = 23). Note the large variability of responses at pairs from 5-week-old animals. E, Recovery from depression. Average paired-pulse ratios at connections from 3-week-old (n = 5) and 5-week-old (n = 6) rats obtained at presynaptic interspike intervals of 15, 100, and 200 msec at a stimulation rate of 1 Hz. F, Recovery from facilitation. Average paired-pulse ratios at connections from 5-week-old rats (n = 5) obtained at presynaptic interspike intervals of 15, 100, and 200 msec at a stimulation rate of 0.2 Hz.

We then investigated the effects of spike pairs elicited at two different stimulation rates (1 and 0.2 Hz). Figure 4A illustratesthe responses to paired-pulse stimulations elicited at 1 Hz (Fig.4A1) and 0.2 Hz (Fig. 4A2) at a pyramidal-FS connection from a19-d-old animal, using an interspike interval of 50 msec. In bothcases a depression of the second response was observed with apaired-pulse ratio of 0.64 and 0.73 at 1 and 0.2 Hz, respectively.For eight tested connections from 3 week-old rats, there wereno significant differences in the paired-pulse ratio obtainedat the two frequencies (Fig. 4C; p > 0.05; Wilcoxon t test). Theresponse probability of EPSC1 and of EPSC2 was, however, largerat a low rate of stimulation (Table 2; p < 0.01; Wilcoxon ttest).

At pyramidal-FS connections from 5-week-old rats, the response probability of EPSC1 was not affected by the rate of stimulation,but for EPSC2 the response probability increased significantlywhen the stimulation rate decreased from 1 to 0.2 Hz (Table 2;p < 0.01; Wilcoxon t test). This modification induced an increasein the paired-pulse ratio in all 15 tested connections from 5-week-oldrats (Fig. 4C; p < 0.001; Wilcoxon t test) leading in eight casesto a switch from a PPD at a stimulation rate of 1 Hz, to a PPFwhen the spike pairs were delivered at a stimulation rate of 0.2Hz (Fig. 4B1,B2). The plot of all individual data shown in Figure4D illustrates the large variability of the paired-pulse responsesand the predominance of facilitation at lower stimulation ratesat connections from 5-week-old rats. For five connections thatfacilitated at a stimulation rate of 0.2 Hz, pairs of action potentialswere applied at different interspike intervals (Fig. 4F). PPFwas large at intervals of 15 msec (average paired-pulse ratioof 1.74 ± 0.8) but was not observed at intervals of 200 msec (Fig.4F; p < 0.05; Mann-Whitney Utest).

Differential functional maturation of pyramidal-FS connections

The modifications of the activity-dependent short-term effects at pyramidal-FS connections observed between the third andfifth postnatal week occurred without significant changes of thekinetics of the AMPA receptor-mediated unitary EPSCs (see aboveand Table 1). At a stimulation rate of 0.2 Hz, there were nosignificant differences either in the response probabilities orin the average amplitude of EPSC1 with or without failures betweenthe two developmental stages (Table 2; p > 0.05; Mann-WhitneyUtest).

The restricted distribution of the paired-pulse ratios in our sample of connections in young animals (Fig. 4D) suggested thatall pyramidal cell inputs to FS cells have similar paired-pulsecharacteristics. However, the large distribution observed in thesample of connections in 5-week-old animals may imply that differentpyramidal cell inputs onto the same FS cell evolved differently.This has been directly tested by comparing the synaptic propertiesof two different presynaptic pyramidal cells impinging onto thesame postsynaptic FSinterneuron.

Figure 5A illustrates the paired-pulse responses of a single postsynaptic FS cell from a 33-d-old rat elicited by two differentpresynaptic pyramidal neurons at a stimulation rate of 0.2 Hz.The first connection onto this postsynaptic cell showed a depression(ratio of 0.64), whereas the second one showed a facilitation(ratio of 1.4). In two of three other sequential paired recordingsin slices of 5-week-old rats, the input from one pyramidal celldisplayed a PPD, whereas the input from another pyramidal cellwas characterized by a PPF (Fig. 5B). In contrast, when sequentialpaired recordings were performed in four postsynaptic young FScells (eight connections), we always observed a PPD (Fig. 5B).

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Figure 5. Paired-pulse responses elicited by two different presynaptic pyramidal cells onto single postsynaptic FS interneurons. A, Paired-pulse responses of a FS interneuron elicited by two presynaptic pyramidal cells recorded sequentially in a slice from a 33-d-old rat. A PPD (ratio of 0.64; traces are averages of 50 responses) was observed at the first connection (Pyr 1-FS) at which the response probabilities of EPSC1 and EPSC2 were 0.94 and 0.86, respectively. A PPF (ratio of 1.4; traces are averages of 76 responses) was observed at the second connection (Pyr 2-FS) with response probabilities of 0.7 and 0.87 for EPSC1 and EPSC2, respectively. B, Comparison of the paired-pulse ratios of two different presynaptic inputs onto single FS interneurons. Vertical lines link the two data points corresponding to the paired-pulse ratios of the two connections studied for each of the eight FS cells recorded in 3-week-old (n = 4) and 5-week-old (n = 4) animals. Note that PPD was obtained at all young connections, whereas different inputs onto three of four single FS cells from 5-week-old rats could display either PPD or PPF. It is noteworthy that, at older connections, the presence of PPD or PPF was independent of the order in which the sequential connections were obtained.

These results show that, at the end of the first postnatal month, inputs from different pyramidal cells onto the same FS interneuronhave different paired-pulse response characteristics, suggestingthat the regulation of glutamate release mechanisms differs amongpyramidalcells.

  DISCUSSION

Paired recordings in neocortical slices indicate that pyramidal-FS connections consist of multiple release sites at whichAMPA receptors mediate most of the postsynaptic current near restingmembrane potentials. These synapses always display PPD at earlystages of postnatal development. At later stages of development,short-term adjustments in the synaptic gain during repetitiveactivity can lead to either depression or facilitation accordingto the presynaptic firing rate. These results indicate that criticalsynaptic parameters for short-term plasticity at this excitatoryneocortical connection mature relatively late during postnataldevelopment.

Basic properties of pyramidal-FS connections

We found that transmitter release fluctuated randomly at pyramidal-FS connections and that the amplitude distribution of unitarysynaptic responses was modified by manipulations affecting theprobability of release such as paired-pulse protocols or changesin [Ca²⁺]_e. This therefore suggests that single presynaptic action potentialstrigger the release of several quanta of glutamate at pyramidal-FSconnections. Our morphological estimation of the number of synapticjunctions (one or two putative contacts; n = 4) is comparablewith the study reported by Buhl et al. (1997) at pyramidal-basketcell connections in the adult visual cortex of the cat. Thesenumbers of morphological contacts are of the same order of magnitudeas the number of quanta released that can be estimated from ourphysiological data by comparing the quantal size obtained in low[Ca²⁺]_e to the amplitude of the control EPSC (2.3 quanta on average;n = 4). Both methods probably lead to an underestimation of thenumber of release sites because, on the one hand, some contactscan be obscured during morphological analysis (e.g., by axonsundercrossing dendrites) and, on the other hand, the probabilityof release at each site is probably <1 at physiological [Ca²⁺]_e. All together, these observations show that pyramidal-FS connectionsconsist of multiple releasesites.

Postnatal development of activity-dependent properties of synaptic transmission at pyramidal-FS connections

Conflicting results concerning the modifications of synaptic strength that occur in response to paired-pulse protocols orshort trains of presynaptic action potential at pyramidal-FS orpyramidal-basket cell connections have been published previously.Thomson et al. (1993, 1995) first showed a profound frequency-dependentfacilitation at pyramidal cell inputs onto interneurons, includingFS cells, in the adult rat neocortex. More recently, Buhl et al.(1997) reported PPD at pyramidal-to-basket cell synapses in theadult cat visual cortex, and Reyes et al. (1998) also describeddepression at synapses between pyramidal cells and FS putativebasket cells in the young rat neocortex. These data can be simplyreconciled, in light of our present results, by taking into accountthe differences in the stimulation rates and the ages of the animalsused by the different authors. Indeed, our results clearly showthat PPD is predominant in young animals within a large rangeof stimulation rates. At the fifth postnatal week, most pyramidal-FSconnections of our sample can display PPF at low stimulation rates(0.2 Hz) and PPD at higher rates (1 Hz). It is not excluded, however,that conflicting results between authors rely also on differentexperimental protocols and conditions. In particular, trains ofpresynaptic action potentials have been used by some authors (Thomson,1997; Reyes et al., 1998), whereas others have quantified theeffects of paired-pulse protocols (Buhl et al., 1997).

Postnatal changes of paired-pulse response characteristics of neocortical excitatory synapses have never been reported previously.At excitatory synapses between CA3 and CA1 hippocampal pyramidalcells, Bolshakov and Siegelbaum (1995) showed a decrease in theprobability of release without postsynaptic modifications betweenthe first and third postnatal weeks. At inhibitory synapses betweeninterneurons and Purkinje cells in the cerebellar cortex, thedecrease of the average unitary synaptic current amplitude observedbetween the second and the fifth postnatal weeks seemed to involveboth presynaptic and postsynaptic modifications (Pouzat and Hestrin,1997). In both cases, a switch from PPD to PPF accompanied thesedevelopmental changes of synaptic transmission. We did not observesignificant modifications of the unitary EPSC kinetics and amplitudesbetween the third and fifth postnatal weeks that could suggesta change in the properties of the postsynaptic AMPA receptors.The switch from PPD to PPF at low stimulation rates (0.2 Hz) duringthe postnatal development at pyramidal-FS connections stronglysuggests the occurrence of presynapticmodifications.

The observation that, in 3-week-old rats, all pyramidal cell inputs onto single FS interneurons always displayed PPD is inagreement with recent data showing that the different naturesof the target neurons underlie the early development of presynapticproperties determining the facilitating or depressing characteristicsof hippocampal or neocortical synapses (Markram et al., 1998;Reyes et al., 1998; Scanziani et al., 1998). Our results indicatethat the homogeneity of presynaptic properties in young animals,as determined by these target-specific mechanisms, evolves towarda more complex situation during later stages of development. Indeed,inputs from different pyramidal cells onto the same FS interneuronhad different paired-pulse response characteristics that differednot only quantitatively (Markram et al., 1998) but also qualitativelybecause some inputs could display PPD and others PPF. This suggeststhat the postnatal development and more recent activity endoweach pyramidal-FS connection with unique functional propertiesin the neocortical network at the end of the first postnatal month.We cannot exclude, however, that the heterogeneity of the paired-pulseresponses observed at 5-week-old animals indicates that pyramidal-FSconnections are still on the course ofdevelopment.

Physiological implications

At most pyramidal-FS connections from 5 week-old rats, the paired-pulse ratio resulting from the coexisting facilitation anddepression mechanisms will vary within a wider range than at youngerconnections, endowing older connections with large integrativecapabilities. This balance between facilitation and depressionis determined by the activity of the presynaptic pyramidal cellswhich in vivo can adopt a wide range of frequencies, often irregular(for references, see Softky and Koch, 1993). Pyramidal cell inputsto FS cells in vivo are therefore likely to consist of sequencesof single spikes and small bursts of spikes delivered at a largerange of frequencies. Our results predict that the number of presynapticpyramidal cell inputs needed to activate a FS cell will vary withthe overall activity that those inputs had experienced duringthe preceding seconds. Because of the high reciprocal connectivitybetween pyramidal cells and FS cells (Reyes et al., 1998), itis likely that a single FS cell is involved in an extremely largenumber of recurrent inhibitory loops. The observation that synaptictransmission at pyramidal-FS connections is facilitated or depresseddepending on the presynaptic firing rate suggests that the relativeweight of the recurrent inhibition mediated by a given FS cellin different loops is dynamicallyadjusted.

  FOOTNOTES

Received Oct. 8, 1998; revised Dec. 7, 1998; accepted Dec. 9, 1998.

This study was supported by Centre National de Recherche Scientifique (France), European Union Grants 96-0589 and 96-0382,and Deutsche Forschungsgemeinschaft Grant STA 431/2-1. M.C.A.was supported by a fellowship from Instituto Colombiano de Cienciay Tecnología (Colciencias; Colombia). We thank Samia Ben Ammouand U. Opfermann-Emmerich for technical assistance and Drs. SergeCharpak and James T. Porter for helpful comments on thismanuscript.
Correspondence should be addressed to Dr. Etienne Audinat, Neurobiologie et Diversité Cellulaire, Centre National de la RechercheScientifique, Unité Mixte de Recherche 7637, Ecole Supérieurede Physique et de Chimie Industrielles, Paris, 10 rue Vauquelin,75231 Paris Cedex 5,France.

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