Coincident Spiking Activity Induces Long-Term Changes in Inhibition of Neocortical Pyramidal Cells

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The Journal of Neuroscience, October 15, 2001, 21(20):8270-8277

Coincident Spiking Activity Induces Long-Term Changes in Inhibition of Neocortical Pyramidal Cells
Carl D. Holmgren and Yuri Zilberter
Karolinska Institute, Department of Neuroscience, Division of Neuroanatomy and Brain Development, S-17177 Stockholm, Sweden

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In pyramidal cells, induction of long-term potentiation (LTP) and long-term depression (LTD) of excitatory synaptic transmissionby coincidence of presynaptic and postsynaptic activity is consideredrelevant to learning processes in vivo. Here we show that temporallycorrelated spiking activity of a pyramidal cell and an inhibitinginterneuron may cause LTD or LTP of unitary IPSPs. Polarity ofchange in synaptic efficacy depends on timing between Ca²⁺ influx induced by a backpropagating train of action potentials(APs) in pyramidal cell dendrites (10 APs, 50 Hz) and subsequentactivation of inhibitory synapses. LTD of IPSPs was induced bysynaptic activation in the vicinity of the AP train (<300 msecrelative to the beginning of the train), whereas LTP of IPSPswas initiated with more remote synaptic activation (>400 msecrelative to the beginning of the AP train). Solely AP trains inducedneither LTP nor LTD. Both LTP and LTD were prevented by 5 mM BAPTAloaded into pyramidal cells. LTD was prevented by 5 mM EGTA, whereasEGTA failed to affect LTP. Synaptic plasticity was not dependenton activation of GABA_B receptors. It was also not affected bythe antagonists of vesicular exocytosis, botulinum toxin D, andGDP- $beta$ -S.

Key words: neocortex; interneuron; pyramidal cell; LTP; LTD; coincident detection

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Backpropagating action potentials (APs) in dendrites of pyramidal cells in neocortex and hippocampus evoke a transient increasein the dendritic [Ca²⁺]_i (Schiller et al., 1995; Magee and Johnston, 1997; Isomura etal., 1999; Kaiser et al., 2001), providing a general associativesignal for Hebbian plasticity in active synapses (Magee and Johnston,1997; Markram et al., 1997a). Coincidence of backpropagating APswith synaptic activity may induce either long-term potentiation(LTP) or long-term depression (LTD) in excitatory synapses dependingon a precise temporal order of APs and EPSPs in the millisecondrange (Magee and Johnston, 1997; Markram et al., 1997a; Bi andPoo, 1998; Debanne et al., 1998; Egger et al., 1999). It is possiblethat such temporal patterns of presynaptic and postsynaptic neuronspiking activity exist in vivo during learning episodes and caninduce long-term plasticity in active synaptic contacts (Buzsakiet al., 1996; Thomas et al., 1998; King et al., 1999; Paulsenand Sejnowski, 2000).

Excitability of pyramidal cells is effectively controlled by inhibitory interneurons, which can modulate the timing of a spikegeneration (Miles et al., 1996; Freund and Gulyas, 1997; Thomaset al., 1998; King et al., 1999; Larkum et al., 1999; Zilberter,2000). Despite the importance of inhibitory transmission in theregulation of pyramidal cell firing, there is a lack of information,to our knowledge, on long-term synaptic plasticity in inhibitoryconnections resulting from a temporally correlated spiking ofa pyramidal cell and aninterneuron.

In the neocortex, pyramidal cell-interneuron pairs are frequently reciprocally connected (Buhl et al., 1997; Reyes et al.,1998; Zilberter et al., 1999; Zilberter, 2000), creating elementaryneuronal microcircuits. In these microcircuits, potentiation (ordepression) of the excitatory inputs onto a pyramidal cell maycause a backward increase (or decrease) of inhibition of the pyramidalcell by an interneuron. In a previous study (Zilberter, 2000),it was reported that trains of backpropagating dendritic APs inL2/3 pyramidal cells of the rat neocortex resulted in a short-termsynaptic depression of inhibitory transmission induced by theCa²⁺-dependent dendritic release of a retrograde messenger. Meanwhile,a long-lasting potentiation of IPSPs was often observed afterthe AP train conditioning in pyramidal neurons (Zilberter, 2000).Results of the present study demonstrate that either LTD or LTPof inhibitory transmission may be induced depending on the timeinterval between backpropagating APs in pyramidal cell dendritesand activation of inhibitorysynapses.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cortical slices (300 µm thick) were prepared from the brain of 14- to 16-d-old Sprague Dawley rats as described previously(Markram et al., 1997b). Simultaneous dual whole-cell recordingswere made in pyramidal cells synaptically connected to fast spikingnonaccommodating (FSN) interneurons (Zilberter, 2000). FSN neuronsand pyramidal cells in layer 2/3 were identified by infrared-differentialinterference contrast video microscopy and subsequent measurementsof neuron firing properties. The extracellular solution contained(in mM): 125 NaCl, 2.5 KCl, 25 glucose, 25 NaCO₃, 1.25 Na₂PO₄,2 CaCl₂, and 1 MgCl₂. All experiments were performed at 32°C inoxygenated extracellular solution. The pipette solution contained(in mM): 100 (or 115) K-gluconate, 20 KCl, 4 ATP-Mg, 10 Na-phosphocreatine,0.3 GTP, and 10 HEPES, pH 7.3 (310 mOsm/l).

Electrical signals were recorded with Axoclamp 2B and Axopatch 200B amplifiers (Axon Instruments, Foster City, CA), digitizedat 20 kHz by an analog-to-digital converter (ITC-18; InstruTech,Great Neck, NY) controlled by a program (Pulse; Heka Elektronik,Lambrecht, Germany) and analyzed off-line using commercial software(IGOR Pro; WaveMetrics Inc., Lake Oswego, OR) with custom-writtenroutines. Patch pipettes had a resistance of 3-4 M $Omega$ . Input resistanceto the postsynaptic (pyramidal) cells was in the range of 40-80M $Omega$ and was thoroughly controlled throughout the experiment. Restingmembrane potential of pyramidal cells was 74 ± 1.2 mV (n = 22)and was stable during the experiment in most cases. Small variationsin the cell resting potential (a few millivolts) were correctedby a current injection into a soma whennecessary.

Five neuron pairs were morphologically reconstructed with the aid of computerized camera Lucida system. Neurons were filledduring experiments with 2 mg/mlneurobiotin.

Conditioning protocols used for the induction of long-term changes in synaptic efficacy of inhibitory transmission betweenFSN and pyramidal cells were as follows (Fig. 1A). The conditioningtrain of 10 backpropagating dendritic APs was initiated by 5 mseccurrent injections in the soma of pyramidal cell at 50 Hz. Inthe FSN neuron, an AP was initiated at different times relativeto the beginning of the AP conditioning train in the pyramidalcell. This time is given as a subscript to the headers of thecoincidence stimulation (CS) in Figure 1A. The pattern of sequentialpostsynaptic and presynaptic stimulation was repeated every 5-7sec for 25-40 times.

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Figure 1. Conditioning protocols used for the induction of synaptic plasticity. A, A train of 10 backpropagating APs (50 Hz) was initiated in a pyramidal cell (V_m post) by 5 msec current injections in the soma, and an AP was initiated in an FSN neuron (V_m pre) at different times relative to the beginning of the AP train. B, Time distributions of synaptic plasticity observation after conditioning application in different experiments.

Figure 1B shows time distributions of observation of changes in synaptic efficacy after conditioning application in differentexperiments. In a relatively small number of experiments withIPSP depression, the observation time exceeded 20 min. However,because recovery of IPSPs from depression was never observed inour experiments, we will further refer to this process asLTD.

In control and after conditioning, the paired-pulse stimulation (100 msec interpulse interval, each 7 sec) was applied inmost experiments to evaluate the paired-pulse depression. Forother data analysis, only the first IPSP during such stimulationwas used. A paired-pulse ratio (PPR) was calculated as IPSP2/IPSP1,in which IPSP1 and IPSP2 were average IPSP amplitudes in responseto the first and second APs, respectively. The mean amplitudeof unitary IPSPs was measured from 50-100sweeps.

IPSPs were counted as potentiated or depressed if their amplitudes measured in control were significantly different to thosemeasured after conditioning (unpaired Student's t test). The minimumchange in the mean IPSP amplitude consistent with this test was8%. The absence of a tendency of IPSP amplitudes to increase ordecrease in control over time was also verified by the unpairedStudent's ttest.

In ~30% of all experiments, a rundown of IPSPs was observed. The rundown usually started soon (1-3 min) after obtaining thewhole-cell configuration. It was indicated by a gradual decreasein the amplitude of IPSPs and was not associated with a changein the cell resting potential. These experiments were not analyzedfurther.

Average data are given as mean ± SEM. Statistical significance of difference in mean IPSPs was analyzed by paired Student'sttest.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

LTP and LTD of inhibitory transmission

Conditioning by the CS₊₄₁₀ and CS₊₅₁₀ protocols in most cell pairs induced LTP of IPSPs. Figure 2A demonstratesone experiment in which considerable IPSP potentiation was evokedby the CS₊₄₁₀ conditioning. The IPSP potentiation lastedfor ~1 hr until termination of the experiment. Horizontal linesindicate the amplitudes of mean IPSPs. These mean IPSPs are alsoshown in the top panel. In 34 cell pairs tested in similar experiments,LTP of inhibitory transmission ranging from 108 to 261% of controlwas observed after conditioning. The mean IPSP amplitude was 160± 16% of control after CS₊₄₁₀ (n = 10; mean ± SEM; p < 0.01)and 142 ± 6% of control after CS₊₅₁₀ (n = 24; p < 0.01).

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Figure 2. LTP and LTD of inhibitory transmission in pyramidal cells. A, LTP of inhibitory transmission between FSN and pyramidal neurons. The mean IPSPs in control and after the CS₊₄₁₀ conditioning are shown in the top panel, and their amplitudes are indicated by horizontal lines in the bottom panel. B, LTD of inhibitory transmission. The mean IPSPs in control and after the CS₊₂₅₀ conditioning are shown in the top panel, and their amplitudes are indicated by horizontal lines in the bottom panel. C, Summary of changes in efficacy of inhibitory synaptic transmission in different experiments. Horizontal lines show the mean values. D, Variations in efficacy of inhibitory transmission (percentage of control) depending on timing between the conditioning AP train and synaptic stimulation. E, IPSPs averaged in 34 cell pairs in control and after conditioning-inducing LTP (CS₊₄₁₀ and CS₊₅₁₀). In each experiment, IPSPs were normalized to the mean IPSP amplitude in control. Then, IPSPs in all cell pairs recorded at equivalent times during the experiment protocol were averaged. Filled circles show IPSPs averaged within each minute of the experimental protocol. F, IPSPs averaged in 22 cell pairs in control and after conditioning-inducing LTD (CS₊₁₀, CS₊₂₀₅, and CS₊₂₅₀) by the same procedure as in Figure 1E.

Surprisingly, a shorter delay between the train of backpropagating APs and synaptic stimulation resulted in LTD of IPSPs.Figure 2B demonstrates one experiment in which conditioning byCS₊₂₅₀ induced a prominent long-lasting decrease of IPSPs.Horizontal lines indicate the amplitudes of mean IPSPs, whichare also shown in the top panel. Synaptic depression was observedin all five cell pairs after CS₊₁₀, and the average IPSPamplitude was 75 ± 6% of control (p < 0.01). In 9 from 15 cellpairs after CS₊₂₀₅ (n = 15; p < 0.01), the average IPSP amplitudeduring depression was 69 ± 0.05% of control. In all eight cellpairs tested after CS₊₂₅₀ (p < 0.01), the average IPSP amplitudewas 58 ± 0.06% of control. Conditioning by CS₁₀, CS₊₃₀₀,and CS₊₈₀₀ did not evoke significant changes in IPSPs (n= 8, p > 0.4; n = 9, p > 0.2; and n = 5, p > 0.8, respectively).A summary of changes in the efficacy of inhibitory synaptic transmissioninduced by different conditioning protocols is shown in Figure2C. Figure 2D illustrates variations in synaptic efficacy of inhibitorytransmission depending on timing between the conditioning AP trainand synapticstimulation.

To reveal the time course of LTD and LTP development, we averaged IPSPs in all cell pairs in control and after correspondingconditioning protocols (CS₊₁₀, CS₊₂₀₅, CS₊₂₅₀ andCS₊₄₁₀, CS₊₅₁₀, respectively). In each experiment, IPSPswere normalized to the mean IPSP amplitude in control. Then IPSPsin all cell pairs, recorded at equivalent times during the experimentprotocol, were averaged. The resulting time courses of LTP andLTD of IPSPs are shown in Figure 2, E and F, respectively. Filledcircles demonstrate IPSPs averaged within each minute of the experimentalprotocol. LTP is evident immediately after termination of conditioning,although it continues to increase over the following several minutes.LTD, however, appears to be on a steady-state level after conditioningtermination.

LTP and LTD are triggered by an increase in dendritic Ca2+

Because conditioning trains of backpropagating APs induced Ca²⁺ transients in dendrites (Isomura et al., 1999; Zilberter, 2000;Kaiser et al., 2001) and spines (Majewska et al., 2000) of L2/3pyramidal cells, an increase in dendritic [Ca²⁺]_i was suggested to be a trigger of synaptic plasticity. Indeed,in six cell pairs, 5 mM BAPTA loaded into pyramidal cells viathe pipette solution prevented induction of LTP after the CS₊₄₁₀conditioning protocol. The mean IPSP was 1.78 ± 0.12 mV in controland 1.72 ± 0.11 mV after CS₊₄₁₀ in the presence of BAPTA(p > 0.4). Interestingly, EGTA (5 mM), which has the same Ca²⁺ buffer capacity as BAPTA but much slower binding kinetics, failedto affect the LTP induction. In seven cell pairs, IPSP potentiationto 156 ± 14% of control was observed after CS₊₄₁₀ (n = 3)and CS₊₅₁₀ (n = 4) protocols in the presence of EGTA (p <0.01). Normalized IPSPs averaged in the experiments describedabove are shown in Figure 3, A and B.

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Figure 3. Induction of LTP and LTD of inhibitory transmission is Ca²⁺ dependent. A, Averaged in six cell pairs, IPSPs measured in control and after the CS₊₄₁₀ conditioning with 5 mM BAPTA loaded into pyramidal cells. BAPTA prevented the LTP induction. B, Averaged in seven cell pairs, IPSPs measured in control and after the CS₊₄₁₀ (n = 3) and CS₊₅₁₀ (n = 4) conditioning with 5 mM EGTA loaded into pyramidal cells. EGTA did not affect the LTP induction. C, Averaged in four cell pairs, IPSPs measured in control and after the CS₊₂₀₅ conditioning with 5 mM BAPTA loaded into pyramidal cells. BAPTA prevented LTD of IPSPs. D, Averaged in six cell pairs, IPSPs measured in control and after the CS₊₂₀₅ conditioning with 5 mM EGTA loaded into pyramidal cells. EGTA prevented LTD of IPSPs. Note LTP of IPSPs unmasked with the presence of EGTA . In all figures, IPSPs were averaged by the same procedure as in Figure 1E.

Meanwhile, both BAPTA and EGTA prevented the LTD initiation (Fig. 3C,D). In four cell pairs, the mean IPSP was 1.2 ± 0.5 mVin control and 1.17 ± 0.4 mV after CS₊₂₀₅ in the presenceof BAPTA. With similar conditioning, EGTA not only prevented theinitiation of LTD but also unmasked the LTP development. LTP ofIPSPs was observed in five of six cell pairs tested and was 119± 6% of control (n = 6; p < 0.05).

These results indicate that an initiating step in the induction of inhibitory transmission LTP is triggered rapidly afterCa²⁺ influx into dendrites, whereas the LTD initiation is slower.They also suggest that both processes, LTP and LTD of inhibitorytransmission, may develop in parallel: LTD predominates at shorterdelays between initiation of Ca²⁺ influx into dendrites and synaptic stimulation, whereas LTP takesover at longerones.

LTP and LTD are not induced by variations in GABA release probability

To examine the site of expression of synaptic plasticity, PPR of IPSPs was measured in most experiments. PPR was not changedsignificantly by any conditioning protocol (Fig. 4A). One possibilityis that the paired-pulse depression may be induced predominantlyby desensitization of postsynaptic GABA_A receptors. However, PPRcould be widely modulated by affecting GABA release probabilityin presynaptic terminals.

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Figure 4. GABA release probability and reversal potential of synaptic currents are not changed during LTP or LTD. A, A summary of PPR measured in different experiments. B, Change in PPR induced by lowering the extracellular Ca²⁺ concentration to 1 mM (n = 3) and by the antagonist of mGluRs, ACPD (100 µM; n = 7). C, Current-voltage relationships of synaptic currents in control (open circles) and after conditioning (filled circles) by CS₊₂₀₅ (n = 3) and CS₊₄₁₀ (n = 3) protocols. Deviations are shown upward for control and downward for data after conditioning. Dashed vertical lines indicate the Cl reversal potential, $-$ 48.6 mV.

As an example, Figure 4B demonstrates the effects of lowered external Ca²⁺ concentration (1 mM) and an agonist of metabotropic glutamatereceptors (mGluRs), (±)-1-amino-1,3-cyclopentanedicarboxylic acid(ACPD) (100 µM), on PPR. Both the decrease in Ca²⁺ concentration and ACPD induced strong inhibition of IPSPs (to29 ± 3% of control, n = 3; and to 28 ± 3% of control, n = 7, respectively)and converted IPSP paired-pulse depression to IPSP paired-pulsefacilitation.

Stability of PPR after induction of LTD or LTP of IPSPs suggests a lack of transmitter release probability contribution tothese processes. The alternative possibility of presynaptic expressionof synaptic plasticity, that is, a change in AP propagation tothe presynaptic terminals, seems to be unlikely because LTP andLTD of IPSPs may develop in parallel (see above). These resultssuggest a postsynaptic mechanism of development of synapticplasticity.

Reversal potential of synaptic currents is not changed by conditioning

Ganguly et al. (2001) reported recently that the reversal potential of GABA-induced synaptic currents may undergo significantvariations during hippocampal cell development in culture. Suchsynaptic plasticity would result in corresponding change in IPSPamplitudes at the same cell resting potential. In our case, however,the reversal potential of synaptic currents was stable beforeand after conditioning application (Fig. 4C), indicating a differentmechanism of plasticity in inhibitorysynapses.

Synaptic activation is required for the induction of synaptic plasticity

Conditioning by the trains of backpropagating APs without synaptic stimulation did not affect synaptic transmission; in 14cell pairs, the mean IPSP amplitude was 4.12 ± 0.97 mV in controland 4.12 ± 0.95 mV after conditioning (p > 0.4). This impliesthat synaptic activation is necessary for the induction of synapticplasticity. If synaptic plasticity is expressed postsynaptically,GABA released from the interneuron axon terminals can activateeither GABA_A or GABA_B postsynaptic receptors. It was reportedpreviously (Komatsu, 1996) that, in the visual cortex L5, LTPof inhibitory transmission induced by a high-frequency stimulationof afferent fibers requires activation of postsynaptic GABA_B receptorsfor itsinduction.

In the present experiments, however, LTP and LTD of unitary IPSPs were initiated in the presence of GDP- $beta$ -S (0.6 mM), preventingG-protein activation, or under a block of GABA_B receptors by aselective antagonist, (2S)-3-{[(15)-1-(3,4-dich-lorophenyl) ethyl]amino-2-hydroxypropyl)(phenylmethyl)phosphinicacid CGP55845A (2 µM). In three cell pairs, the mean IPSP amplitudewas 148 ± 32% of control after CS₊₅₁₀ in the presence ofCGP55845A. Induction of LTP was also not affected by GDP- $beta$ -S (0.6mM) loaded into pyramidal neurons (see below). In two cell pairs,synaptic depression to 65 and 62% of control was obtained afterCS₊₂₅₀ in the presence of GDP- $beta$ -S. Presumably, in L2/3 pyramidalcells, activation of GABA_A receptors is essential for the inductionof long-term plasticity of inhibitory transmission. We tried toobtain direct evidence in favor of this hypothesis by applyingconditioning under a block of GABA_A receptors with a selectiveantagonist, bicuculline (Komatsu, 1996; Ouardouz and Sastry, 2000).Unfortunately, in three experiments, no IPSP recovery was observedeven after 30 min of bicucullinewashout.

Induction of LTP and exocytosis

Recent studies of excitatory transmission LTP imply a delivery of AMPA receptors to the active synapses by dendritic exocytosisas a possible mechanism of potentiation (Lledo et al., 1998; Lüscheret al., 1999). In these studies, the antagonist of vesicular exocytosis,botulinum toxin B (BoTx-B), prevented LTP induction (Lledo etal., 1998) and AMPA receptor cycling (Lüscher et al., 1999) inCA1 pyramidal cells. The existence of exocytotic machinery inthe dendrites of neocortical L2/3 pyramidal cells was also suggestedin a previous study (Zilberter, 2000) because dendritic Ca²⁺-dependent release of a retrograde messenger was prevented bythe antagonists of vesicular exocytosis BoTx-D (Xu et al., 1998;Schiavo et al., 2000) and GDP- $beta$ -S (Hess et al., 1993; Zilberteret al., 1999; Zilberter, 2000). However, neither BoTx-D nor GDP- $beta$ -Saffected the induction of inhibitory transmission LTP in thisstudy. Figure 5A shows one experiment in which the pyramidal cellwas loaded with the BoTx-D light chain (400 nM) added to the pipettesolution. The pyramidal and FSN cells were reciprocally connected,and EPSPs in the FSN neuron were recorded periodically to verifythe diffusion of BoTx-D to the presynaptic sites (see the toppanel), suggesting therefore that the toxin had already diffusedto the dendrites. EPSPs disappeared 22 min after the beginningof recordings, and CS₊₅₁₀ was applied thereafter, resultingin a pronounced LTP of IPSPs. LTP was observed in four (125 ±6% of control) of eight similar experiments. A lack of the effectof conditioning in half of the experiments can be explained bya prolonged waiting time before conditioning application (up to50 min), justified by the slow diffusion of BoTx-D light chainattributable to its high molecular weight (50 kDa). Presumably,some important intracellular ingredients were washed out duringthis period. It is also necessary to note that BoTx-D cannot beconsidered as a selective antagonist of vesicular exocytosis inneocortical cells because it strongly affected dendritic Ca²⁺ signaling in both L2/3 pyramidal cells (Zilberter, 2000) andinterneurons (Zilberter et al., 1999).

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Figure 5. Antagonists of exocytosis do not affect the induction of LTP. A, LTP of IPSPs induced by CS₊₅₁₀ at 400 µM BoTx-D (light chain) loaded into the pyramidal cell. Horizontal lines indicate the amplitudes of mean IPSPs. The FSN and pyramidal cells were reciprocally connected, and the top panel shows EPSPs measured in the FSN neuron in the beginning of recordings, which disappeared before conditioning (arrows indicate the time of EPSP recordings). B, LTP of IPSPs induced by CS₊₄₁₀ at 0.6 mM GDP- $beta$ -S loaded into the pyramidal cell. Horizontal lines indicate the amplitudes of mean IPSPs. C, A summary of experiments with BoTx-D and GDP- $beta$ -S.

As an alternative way of inhibiting exocytosis, we used 0.6 mM GDP- $beta$ -S loaded into pyramidal cells (Hess et al., 1993; Zilberteret al., 1999; Zilberter, 2000). Because GDP- $beta$ -S is a considerablysmaller molecule than the BoTx-D light chain, it diffused muchfaster to the inhibitory synapses on the pyramidal cell dendrites(five reconstructed cell pairs; 117 ± 13 µm from the soma; n =20). Tested in six cell pairs, GDP- $beta$ -S loaded into pyramidal cellsinhibited EPSPs measured in interneurons to 14 ± 6% of controlduring 9-15 min after establishing the whole-cell configuration.In experiments with GDP- $beta$ -S, LTP was observed in all cell pairs(n = 6; 143 ± 15% of control; CS₊₄₁₀, n = 3; CS₊₅₁₀,n = 3). Figure 5B demonstrates one of these experiments. Summaryof all experiments with BoTx-D and GDP- $beta$ -S is shown in Figure5C. These results, together with a lack of EGTA effect on theLTP induction (see Discussion), oppose the idea that dendriticexocytosis is involved in the mechanism of LTP in inhibitory synapsesbetween FSN and pyramidalcells.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although the long-term modulation of excitatory transmission was intensively studied during the last decades, much less attentionhas been paid to the inhibitory transmission. However, a lackof corresponding information on the role of inhibitory interneuronsand their contribution to the regulation of synaptic plasticityunderlies the general problem of understanding the role of LTPin the learning process (Paulsen and Sejnowski, 2000).

Both LTP (Morishita and Sastry, 1991; Kano et al., 1992; Komatsu and Iwakiri, 1993; Komatsu, 1994; McLean et al., 1996; Aizenmanet al., 1998; Shew et al., 2000) and LTD (Komatsu and Iwakiri,1993; McLean et al., 1996; Morishita and Sastry, 1996; Aizenmanet al., 1998) of inhibitory transmission in different mammalianbrain regions have been reported. Despite the limited number ofthese papers, a variety of mechanisms have been proposed for theinduction of synaptic plasticity. In all of these studies, synapticresponses were evoked by stimulation of afferent fibers. Witha high-frequency stimulation, LTD of inhibitory transmission wasobserved in CA3 pyramidal cells (McLean et al., 1996) and in L5of visual cortex (Komatsu and Iwakiri, 1993), although LTP occurredwhen NMDA receptors were blocked. Afferent tetanization inducedLTP of IPSCs in deep cerebellar nuclei (DCN) neurons (Ouardouzand Sastry, 2000), whereas a 10 Hz stimulation initiated LTD (Morishitaand Sastry, 1996). A unique property of DCN cells is a prominentrebound depolarization and associated spike bursting after theIPSP-induced membrane hyperpolarization. Depending on the numberof spikes during the rebound depolarization and on the correspondingCa²⁺ influx into a postsynaptic DCN cell, either LTD or LTP of IPSPscould be initiated (Aizenman et al., 1998).

The present study demonstrates that AP generation in presynaptic and postsynaptic neurons, correlated in time, may inducelong-term plasticity of synaptic efficacy in inhibitory contacts.The polarity of these variations in synaptic efficacy dependson timing between spike generation in a pyramidal cell and FSNinterneuron. Both LTP and LTD of inhibitory transmission are triggeredby an increase in postsynaptic dendritic Ca²⁺ concentration induced by backpropagating APs in the pyramidalcell but also require GABAergic synapse activation for theirinduction.

In most studies available on long-term plasticity of inhibitory synaptic transmission, LTP and LTD were also initiated byan increase in postsynaptic [Ca²⁺]_i (Kano et al., 1992; Komatsu and Iwakiri, 1993; Komatsu, 1996;McLean et al., 1996; Morishita and Sastry, 1996; Aizenman et al.,1998; Caillard et al., 1999; Ouardouz and Sastry, 2000). Synapticplasticity could be induced solely by the postsynaptic membranedepolarization and subsequent Ca²⁺ influx (Llano et al., 1991; McLean et al., 1996; Morishita andSastry, 1996; Aizenman et al., 1998; Caillard et al., 1999; Ouardouzand Sastry, 2000). Moreover, transition between LTD and LTP wassuggested to be directly dependent on the level of increase in[Ca²⁺]_i (Aizenman et al., 1998; Ouardouz and Sastry, 2000).

In our study, postsynaptic membrane depolarization with a corresponding Ca²⁺ influx mediated by backpropagating APs (Zilberter, 2000; Kaiseret al., 2001) failed to affect the efficacy of inhibitory transmissionunless accompanied by the activation of inhibitory synapses. Itis unlikely that polarity of synaptic plasticity (LTD or LTP)during coincidence of the increase in dendritic [Ca²⁺]_i and synaptic activation was determined by the level of [Ca²⁺]_i for the following reasons. The time constant of Ca²⁺ transient decay in the pyramidal cell dendrites is ~150 msecon average (Kaiser et al., 2001); thus, the [Ca²⁺]_i level is much higher during synaptic stimulation inducing LTDof IPSPs (CS₊₁₀, CS₊₂₀₅, and CS₊₂₅₀). However,LTP of IPSPs was not prevented by EGTA, in contrast to LTD. Thisindicates that (1) after elevation of [Ca²⁺]_i, the LTP process is initiated faster than the LTD one, and(2) the level of [Ca²⁺]_i at the moment of synaptic stimulation is not significant forthe development of synaptic plasticity. Besides, eliminating theLTD initiation in the presence of EGTA (Fig. 3D) unmasked LTPof IPSPs induced by the same conditioning (CS₊₂₀₅). Thissuggests that both processes, LTD and LTD of IPSPs, may coexist,developing inparallel.

What may be a mechanism of plasticity in inhibitory synapses? Although the present study does not answer this question, itsuggests that the dendritic exocytotic machinery is most likelynot involved in this process. First, the antagonists of vesicularexocytosis, BoTx-D (Xu et al., 1998; Schiavo et al., 2000) andGDP- $beta$ -S (Hess et al., 1993; Zilberter et al., 1999; Zilberter,2000), did not prevent development of IPSP LTP. Note, however,that neither GDP- $beta$ -S nor BoTx-D are selective inhibitors of exocytosisand thus cannot provide the direct evidence against its involvementin LTP. In neocortical bitufted interneurons (Reyes et al., 1998),BoTx-D decreased the amplitude of dendritic Ca²⁺ transients to 66% of control (Zilberter et al., 1999), althoughit increased Ca²⁺ transients to 182% of control in dendrites of L2/3 pyramidalcells (Zilberter, 2000).

Second, the lack of EGTA effect on the development of LTP favors our suggestion. EGTA inhibited exocytosis in endocrine cells(Neher and Marty, 1982), dorsal root ganglion neuron somata (Huangand Neher, 1996), and dendrites of cultured hippocampal neurons(Maletic-Savatic and Malinow, 1998). In CNS nerve terminals, EGTAalso inhibited evoked release, although less effectively thanBAPTA (Borst and Sakmann, 1996; Ohana and Sakmann, 1998; Rozovet al., 2001).

As a possible mechanism of synaptic plasticity, we hypothesize the upregulation or downregulation of the active conformationof GABA_A receptors by their phosphorylation by Ca²⁺-dependent protein kinase(s) (Kano et al., 1996) or dephosphorylationby protein phosphatases(s) (Morishita and Sastry, 1996). Thisassumption, however, should be tested in futureexperiments.

Pyramidal cells and FSN interneurons are reciprocally connected in most cases (Zilberter, 2000). This type of synaptic connectivitywas also found between pyramidal cells and bitufted interneuronsin L2/3 of neocortex (Reyes et al., 1998; Zilberter et al., 1999),as well as between pyramidal cells and multipolar interneuronsin L2/3 (Reyes et al., 1998) (see also Buhl et al., 1997), suggestingthat such microcircuits represent a general case in neocortex.Both excitatory and inhibitory connections in a microcircuit consistingof the pyramidal and FSN cells are usually reliable and efficient.This is indicated by a negligible probability of synaptic failuresduring EPSP or IPSP recordings and by the normally big amplitudeof EPSPs and IPSPs. Thus, both the FSN interneuron and pyramidalcell in the microcircuit can effectively control excitabilityof each other. Namely, variations in the efficacy of inhibitorytransmission may modulate the temporal pattern of APs in the outputof pyramidalcell.

Let us assume, for example, that during a hypothetical learning episode a temporal pattern of APs is repeatedly generatedin the axonal output of the pyramidal cell. These APs may initiateLTP of the corresponding excitatory transmission because the APswill also propagate back to the dendrites reaching the excitatorysynapses with some delay (in the order of a millisecond) withrespect to the initiating EPSPs (Magee and Johnston, 1997; Markramet al., 1997a; Bi and Poo, 1998; Debanne et al., 1998; Egger etal., 1999). LTP of excitatory transmission onto the pyramidalcell, on the other hand, would also induce an increased backwardinhibition by the interneuron. However, the mechanisms of synapticplasticity in inhibitory synapses onto the pyramidal cell limitits suppression by the interneuron. First, the efficacy of inhibitorysynapses onto the pyramidal cell will undergo a short-term depressionduring backpropagating AP trains attributable to the Ca²⁺-dependent dendritic release of a retrograde messenger (Zilberteret al., 1999; Zilberter, 2000). Second, the repeated pattern ofbackpropagating APs in the pyramidal cell will induce LTD of IPSPsin the temporal vicinity of the pattern, thus creating a long-lastingfavorable background for the pattern generation. Finally, thesame repeated AP pattern will induce LTP of more temporally distantIPSPs causing increased inhibition of pyramidal cell spikes asynchronouswith the pattern. Thus, the AP patterns formed during learningepisodes are defined by several mechanisms of synaptic plasticityin this elementary neuronalmicrocircuit.

  FOOTNOTES

Received May 7, 2001; revised July 10, 2001; accepted July 27, 2001.

This study was supported by Swedish Medicine Research Council Grant 2001/Z0710 and a grant from the Wallenberg Foundation.We thank Drs. N. Burnashev, G. Innocenti, S. Grillner, and A.Marty for critically reading this manuscript. We also thank Dr.G. Innocenti for financial support of this work by his Grant 12594from the Swedish Medicine ResearchCouncil.
Correspondence should be addressed to Dr. Yuri Zilberter, Karolinska Institute, Department of Neuroscience, Division of Neuroanatomyand Brain Development, Retzius väg 8, B2-2, S 17177 Stockholm,Sweden. E-mail: yuri.zilberter{at}neuro.ki.se.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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