Hippocampal Long-Term Potentiation Preserves the Fidelity of Postsynaptic Responses to Presynaptic Bursts

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The Journal of Neuroscience, February 15, 1999, 19(4):1236-1246

Hippocampal Long-Term Potentiation Preserves the Fidelity of Postsynaptic Responses to Presynaptic Bursts
David K. Selig¹, Roger A. Nicoll²^,³, and Robert C. Malenka¹^,²
Departments of ¹ Psychiatry, ² Physiology, and ³ Cellular and Molecular Pharmacology, University of California, San Francisco, California 94143

  ABSTRACT

Top
Abstract
Introduction
References

Hippocampal cells often fire prolonged bursts of action potentials, resulting in dynamic modulation of postsynaptic responses;yet long-term potentiation (LTP) has routinely been studied usingonly single presynaptic stimuli given at low frequency. Recentwork on neocortical synapses has suggested that LTP may causea "redistribution of synaptic strength" in which synaptic responsesto the first stimulus of a presynaptic burst of action potentialsare potentiated with later responses depressed. We have examinedwhether this redistribution occurs at hippocampal synapses duringLTP. Using prolonged bursts that result in maximal short-termdepression of later responses within the burst, we found thatLTP resulted in a uniform potentiation of individual responsesthroughout the burst rather than a redistribution of synapticstrength. This occurred both at Schaffer collateral-CA1 synapsesand at CA3-CA3 synapses, the latter being activated and monitoredusing paired recordings. Thus in the hippocampus, LTP preservesthe fidelity of postsynaptic responses to presynaptic bursts bya uniform increase rather than a redistribution of synaptic strength,a finding that suggests there are important differences betweenneocortex and hippocampus in how long-term changes in synapticstrength are used to encode newinformation.

Key words: long-term potentiation; redistribution of synaptic strength; short-term synaptic depression; short-term synaptic facilitation; presynaptic bursts; electrophysiology; hippocampus; rat

  INTRODUCTION

Top
Abstract
Introduction
References

The normal firing pattern of many neurons in the CNS consists of bursts of action potentials (Ranck, 1973; O'Keefe, 1976;Wilson and McNaughton, 1993), leading to synaptic responses thatmay undergo both facilitation and depression, often in sequence(Dobrunz and Stevens, 1997; Brenowitz et al., 1998). Facilitationmay be essential for the conversion of a temporal into a spatialcode (Buonomano and Merzenich, 1995) and may also play a rolein increasing the reliability of synaptic transmission (Dobrunzand Stevens, 1997), enabling bursts to function as the most basicelement of the neural code (Lisman, 1997). Depression may be causedby depletion of synaptic vesicles, activation of inhibitory presynapticautoreceptors, failure of action potential propagation, desensitizationof postsynaptic receptors, or a combination of these (Luscheret al., 1994; Dobrunz and Stevens, 1997; Brenowitz et al., 1998)and may serve to control synaptic gain by attenuating responsesto afferents with statically elevated firing rates (Abbott etal., 1997; Tsodyks and Markram, 1997)

In the hippocampus, bursts of action potentials are commonly observed during in vivo recordings (Ranck, 1973; O'Keefe, 1976;Wilson and McNaughton, 1993). In fact, hippocampal CA3 pyramidalcells have an intrinsic bursting capability (Kandel and Spencer,1961; Wong and Prince, 1981). Excitatory synapses made by CA3cells onto other CA3 pyramidal cells and onto CA1 pyramidal cellsare notable for exhibiting long-term potentiation (LTP), paired-pulsefacilitation, and, with longer stimulus trains, short-term depression(Dobrunz and Stevens, 1997).

Although most studies of LTP have monitored synaptic strength using single presynaptic stimuli, a recent study has demonstratedthe importance of examining the effects of LTP with more prolonged,complex stimuli (Markram and Tsodyks, 1996). Temporally pairingaction potentials in synaptically connected pairs of layer 5 pyramidalcells in the somatosensory cortex resulted in LTP, as measuredwith the response to the first action potential in presynapticbursts. However, there was no net change in synaptic strengthwhen all of the responses to the presynaptic bursts were considered;the responses to the early stimuli in the bursts were potentiated,whereas the responses to the later stimuli were depressed. Thisshift in the synaptic response pattern was termed a "redistributionof synaptic strength" (Markram and Tsodyks, 1996).

An important question is whether this redistribution of synaptic strength during LTP is a general feature of all excitatorysynapses in the mammalian brain (Zador and Dobrunz, 1997). Becausethe excitatory synapses onto CA1 pyramidal cells in the hippocampushave provided the most detailed information currently availableon the mechanisms of LTP (Bliss and Collingridge, 1993; Nicolland Malenka, 1995), we decided to address this question at thesesynapses. We used patterns of presynaptic bursts causing bothfacilitation and depression of the synaptic responses but foundno evidence of a redistribution of synaptic strength during LTP.Instead, we found that the fidelity of the synaptic responseswas preserved by a uniform potentiation to all stimuli in thebursts. We therefore conclude that LTP at hippocampal synapsesand LTP at neocortical synapses involve distinct mechanisms withdistinct functional implications for the ways in which these twostructures encode newinformation.

  MATERIALS AND METHODS

We prepared and recorded from transverse hippocampal slices using standard procedures (Selig et al., 1995). Slices (500-600µm) from 13- to 18-d-old Sprague Dawley rats were allowed to recoverfor a minimum of 1.5 hr before being transferred to a submergedrecording chamber where they were superfused with artificial CSF(ACSF) maintained at 24-26°C and saturated with 95% O₂/5% CO₂.Our standard ACSF for these experiments contained 119 mM NaCl,2.5 mM KCl, 4.0 mM CaCl₂, 1.0 mM MgSO₄, 1.0 mM NaH₂PO₄, 26.2 mMNaHCO₃, 11 mM glucose, and 0.1 mM picrotoxin, pH 7.4. Some ofthe experiments (see Figs. 1, 2) were conducted in 4.0 mM MgSO₄.When recording from CA3, we found it necessary to double the concentrationof divalents in our standard ACSF (to 8.0 mM CaCl₂ and 2.0 mMMgSO₄) to prevent spontaneous bursting (Frankenhaeuser and Hodgkin,1957; Miles and Wong, 1983, 1987). When recording from the CA1region, we made two cuts perpendicular to the pyramidal cell layerto prevent propagation of epileptiform activity from the CA3 andsubicular regions. Perforated-patch recordings (Rae et al., 1991)were made using pipettes (1-2 M $Omega$ ) filled with a solution containing130 mM CsMeSO₃, 8.0 mM NaCl, 10 mM HEPES, and 0.2 mM EGTA, pH7.2 with CsOH (290-300 mOsm). Amphotericin B (1.2 mg/ml; Sigma,St. Louis, MO) dissolved in DMSO (0.6% final concentration) wasadded to this solution, triturated, and used to backfill pipettes.Experiments were begun only after the access resistance had stabilized(typically 12-20 M $Omega$ ). Cells were voltage clamped at $-$ 60 mV withoutcorrection for the liquid junction potential. For some experiments(see Fig. 8), whole-cell recordings from the presynaptic cellwere obtained in current clamp ( $-$ 60 mV) using pipettes (2-4 M $Omega$ )filled with a solution containing 130 mM Kgluconate, 8.0 mM NaCl,10 mM HEPES, 0.2 mM EGTA, 4 mM Mg ATP, and 1 mM NaGTP, pH 7.2with KOH (290-300 mOsm). D-AP-5 (50 µM) was obtained from Tocris.Adenosine (1-2 µM) and kynurenic acid (250 µM) were obtained fromSigma. 6-Nitro-7-sulfamoylbenzo(f)quinoxaline-2,3-dione (NBQX;5 µM) was obtained from Precision Biochemicals (Colton, CA) anddissolved in DMSO (0.05% finalconcentration).

Slices were stimulated with 100 µsec monophasic current pulses using monopolar, stainless steel stimulating electrodes placedin the stratum radiatum immediately adjacent to or within thepresumed dendritic arbor (Ishizuka et al., 1995) of the cell fromwhich the recording was being made. Slices were stimulated every30 sec in some of the experiments (see Figs. 1, 2) and every 10sec in the remaining experiments. Bursts of stimuli were givenevery 30 sec in some of the experiments (see Figs. 1, 2, 8) andevery 5 min in the remaining experiments. The rest of the stimuliwere single pulses. LTP was induced by pairing 120 stimuli at1 Hz while voltage clamping the postsynaptic cell at +10 mV. Onlycells exhibiting potentiation (>40% measured 30 min after theinduction protocol) were considered for further analysis. Responseswere amplified, low-pass filtered at 1 kHz, sampled at 2 kHz,and analyzed on-line. Response amplitude was taken as the differencebetween a 5 msec baseline and a 10 msec period surrounding thepeak of theresponse.

Control responses in the graphs include both the responses to single stimuli and the responses to the first stimuli of thebursts. Depressed responses in the graphs span the last severalresponses in the bursts (see and compare Figs. 3A, 8A). In severalexperiments (see Figs. 3-7), we have expanded the time course ofthe depressed responses of individual bursts for illustrativepurposes (see Fig. 6A₂ for example). Unless otherwise noted, bargraphs represent the average response over a period of 10 min.In some figures (see Figs. 4A₂, 5A₂), we have time aligned andaveraged the last 20 responses of successive bursts to arriveat the single traces shown. For all traces, the stimulus artifactis omitted for clarity. Summary graphs were prepared by subtractingthe isolated stimulus artifact (NBQX, D-AP-5, or picrotoxin) whenavailable from all other responses, setting the baseline periodto 100%, normalizing all responses to this baseline, averagingadjacent responses in a given experiment, and then averaging acrossexperiments. Data in the graphs and text are presented as themean ±SEM.

  RESULTS

LTP and burst-induced facilitation

In an initial set of experiments, we induced LTP in CA1 pyramidal cells while monitoring synaptic transmission with briefbursts of stimulation (25 Hz; seven stimuli) to the Schaffer collateral/commissuralafferents in the stratum radiatum. Using the perforated-patchrecording technique (Rae et al., 1991) allowed us both to achieverelatively low access resistances (12-20 M $Omega$ ) and to avoid washoutof LTP, which commonly occurs when whole-cell recordings withextended baselines are made (Malinow and Tsien, 1990).

Figure 1 shows a typical example and Figure 2 shows a summary (n = 5) of results from this experiment. After obtaining a 20min baseline, we induced LTP with 120 single stimuli given at1 Hz while holding the cells at +10 mV. The response to each stimulusin the burst potentiated (Figs. 1A, 2B) for the duration of therecordings (Figs. 1B, 2A). Moreover, although a modest differencein the level of potentiation for the first and seventh responseswas seen in the individual example, the level of potentiationfor the first and seventh responses was not significantly differentwhen all cells were considered (286 ± 42 and 256 ± 38%, respectively;n = 5; p > 0.05, paired t test; Fig. 2A,C₂). In fact, all responsesduring the burst underwent a similar potentiation (Fig. 2B, inset).Thus, the fidelity of the synaptic response to brief, facilitatorybursts of presynaptic stimuli is preserved by a uniform potentiationof responses within the burst after LTP.

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Figure 1. Example of synaptic response to short presynaptic bursts after LTP. A, Averages of 20 consecutive traces in response to short-burst stimulation (25 Hz; 7 stimuli) at the times indicted by the letters a-d in B. Calibration: 100 pA, 50 msec. B, Typical experiment in which pairing presynaptic stimulation with postsynaptic depolarization (filled arrow) results in a stable increase in the amplitude of the response to the first (B₁) as well as the seventh (B₂) stimulus in the burst. Adenosine (1 µM) was perfused during the time indicated by the horizontal bar. After wash, the amplitude of both the first and seventh response was augmented. C, Average amplitudes of the first and seventh responses immediately before pairing (Baseline), 20 min after pairing (LTP), during adenosine (Adenosine), and immediately after wash of adenosine (Wash). Absolute response amplitudes (C₁) and the first and seventh response amplitudes normalized to their respective baseline amplitudes (C₂) are shown. All values are represented as the mean ± SEM. All panels illustrate data from the same cell.

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Figure 2. Fidelity of the synaptic response to short presynaptic bursts is preserved after LTP. A, Summary graph (n = 5) showing that the amplitude of the response to the first (A₁) and seventh (A₂) stimulus in the short presynaptic bursts (25 Hz; 7 stimuli) undergoes a similar, stable potentiation with pairing (filled arrow). B, Average response amplitude to each stimulus before ( $open circle$ ) and after ( $bullet$ ) pairing normalized to the amplitude of the first response before pairing. Inset, The same data but with the amplitudes of all responses after pairing normalized to the average amplitude of the first response after pairing. C, Average amplitude of first and seventh response immediately before pairing (Baseline) and 20 min after pairing (LTP). Amplitudes are normalized to the amplitude of the first response during the baseline (C₁). The first and seventh response amplitudes are normalized separately to their respective baseline amplitudes (C₂). Potentiation of the first and seventh response amplitudes was not significantly different (286 ± 42 and 256 ± 38%, respectively; n = 5; p > 0.05, paired t test). D, The same experiments with adenosine (1-2 µM) applied after pairing. After wash, there was an increase in the amplitude of both the first and seventh responses (n = 4). All panels illustrate data from the same set of cells (n = 5).

This pattern of change in synaptic strength is very different from that seen with a redistribution of synaptic strength (Markramand Tsodyks, 1996), in which the synaptic response to the firststimulus in the burst is potentiated but the responses to stimulinear the end of the burst are relatively unaffected. Because redistributionof synaptic strength was seen in the neocortex by the use of current-clamprecordings, we considered the possibility that the responses nearthe end of the burst failed to show an increase with LTP becausethe current was shunted through voltage-gated channels that weremore strongly activated after potentiation. However, when we repeatedthese experiments in current clamp, a similar increase in theresponse to the first and seventh stimuli of the burst was stillevident (n = 3; data not shown), suggesting that shunting doesnot explain the difference between these results and those ofMarkram and Tsodyks (1996).

An important difference between the synaptic responses illustrated in Figures 1 and 2 and those observed between pairs ofneocortical cells (Markram and Tsodyks, 1996) is that the presynapticburst in CA1 was facilitatory rather than depressing. This isan important distinction because only with higher frequency stimulithat elicited short-term depression did neocortical LTP manifestitself as a redistribution rather than a uniform increase in synapticstrength (Tsodyks and Markram, 1997). We therefore asked whatconstitutes an adequate stimulus for deciding whether LTP is accompaniedby a redistribution of synapticstrength.

Two models of the synaptic responses to presynaptic bursts of stimuli are helpful in understanding the answer to this question(Abbott et al., 1997; Tsodyks and Markram, 1997). These modelspredict that with a sufficient number of presynaptic stimuli deliveredat a rate beyond a certain frequency of stimulation, termed the"limiting frequency," the amplitude of the synaptic response willbe inversely proportional to the frequency of stimulation, andthus the average postsynaptic response will be constant. Suchpresynaptic bursts therefore result in the maximal short-termdepression of the postsynaptic response. Functionally, the simplestway of conceptualizing the limiting frequency is that frequencyof stimulation at which the rate of synaptic vesicle recyclingeventually determines the synaptic response size. This will occurwhen the presynaptic burst is sufficiently long and of a sufficientlyhigh frequency such that the releasable pool of vesicles entersa depleted state (Dobrunz and Stevens, 1997). Such a burst wasrequired to observe a pure redistribution of synaptic strength(Markram and Tsodyks, 1996) and can be identified by modulatingrelease probability and by verifying that the amplitudes of theresponses near the end of the burst areunaffected.

To determine whether the brief presynaptic bursts we used in Figure 1 were maximally depressing, because anything less couldexplain our failure to observe a redistribution of synaptic strength,we applied and washed out adenosine to modulate release probability(Prince and Stevens, 1992). To facilitate the comparison of theeffects of this pharmacological manipulation with those of LTP,we examined what happened after the washout of adenosine. Washouthad the expected effect on the first response, causing an increasein amplitude (Fig. 1B₁). However, the seventh response also increased(Fig. 1B₂). Adenosine was applied in three of the other four cellsin which brief presynaptic bursts were used to monitor LTP. Onaverage, the seventh response again increased (Fig. 2D), suggestingthat under these experimental conditions brief bursts of presynapticstimuli are not maximally depressing bursts. Therefore these experiments,as well as the results of a previous study of LTP using brieffacilitatory bursts in the hippocampus (Pananceau et al., 1998),do not eliminate the possibility that a redistribution of synapticstrength accompanies hippocampal LTP; the presynaptic bursts mayhave been insufficient to reveal any sort of redistribution. Itwas therefore important to arrange the experimental conditionsso that the presynaptic bursts we gave elicited maximally depressedsynapticresponses.

Burst-induced depression

To enhance our ability to elicit maximally depressed responses, we lowered [Mg²⁺] from 4.0 to 1.0 mM, increased the frequency of the presynapticbursts from 25 to 40 Hz, and increased the number of stimuli from7 to 80. Figure 3 shows that these prolonged bursts depressedthe response amplitude by a factor of three to four, which issimilar to the magnitude of depression observed with much shorterpresynaptic bursts in neocortical cell pairs (Markram and Tsodyks,1996). Bursts were given once every 5 min, the shortest intervalat which the burst responses remained stable, and were elicitedin the presence of D-AP-5 (50 µM), an NMDA receptor antagonist,to prevent induction of LTP (Fig. 3B₂). The last 20 responsesin each prolonged burst were grouped for analysis because theiramplitude was fairly constant (Fig. 3A,C). Interleaved with thebursts were single stimuli that allowed us to monitor the nondepressed,or control, responses (Fig. 3B₁).

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Figure 3. Prolonged presynaptic bursts of stimuli are necessary to depress the synaptic response. A, Example of the response to a prolonged presynaptic burst (40 Hz; 80 stimuli). The trace shows the average of 12 consecutive burst responses given every 5 min in the presence of 50 µM D-AP-5. Calibration: 100 pA, 100 msec. B, The amplitudes of the control (B₁) and depressed (B₂) responses, showing that these amplitudes were stable over time. Control responses (B₁) consist of responses to single stimuli (every 10 sec) as well as the first response in each burst. Depressed responses (B₂) are the last 20 responses in each burst, as shown in A. Bursts were given at the times indicated by the open arrowheads. Note the different amplitude scales in B₁ and B₂. C, Average amplitude of the control response as well as the average amplitude of each group of five successive responses (125 msec) in the 12 bursts. D, Average control and depressed response amplitudes. All panels illustrate data from the same cell.

To determine whether these prolonged bursts were in fact maximally depressing, we compared the burst responses in the presenceand absence of adenosine. Because one of the goals of these experimentswas to compare what happens during LTP with the effects of increasingthe probability of transmitter release, we again examined therecovery from the depressing action of adenosine (1-2 µM; Fig.4A,C₂). Washout resulted in an increase of 202 ± 20% (n = 10)in the amplitude of the control responses to single stimuli buthad no effect on the amplitude of the depressed responses at theend of the burst (101 ± 7%; n = 10). Therefore, these prolongedbursts satisfy the requirements for presynaptic stimulation thatelicits maximally depressed synaptic responses.

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Figure 4. Depressed synaptic responses are unaffected by adenosine. A, Depressed synaptic responses are unaffected by adenosine, a presynaptic neuromodulator, suggesting that under these conditions the burst is maximally depressing (n = 10). Control responses (A₁) increase after washing adenosine (1-2 µM), but depressed responses (A₂; last 20 responses in burst) remain unchanged. Traces are averages of 60 responses (10 min) and are centered over the time when the averages were taken. Open arrowheads designate bursts (40 Hz; 80 stimuli). B, Control responses (bars, and $black-square$ ) and responses to the burst (circles, $open circle$ and $bullet$ ) during adenosine (open symbols, and $open circle$ ) and after washing (closed symbols, $black-square$ and $bullet$ ) are shown. The effect of adenosine was evident only in the responses to the first 10-20 stimuli in the burst (each point represents the responses to five stimuli in the burst). C, Averages (10 min) of control and depressed responses in adenosine and after wash are shown. Amplitudes are normalized to the control response amplitude in adenosine (C₁) and to the average amplitudes in adenosine (C₂). All panels illustrate data from the same set of cells (n = 10).

LTP and burst-induced depression

Having verified that this prolonged stimulation is maximally depressing, we returned to the question of whether hippocampalLTP results in a redistribution of synaptic strength. A typicalexample of this experiment is shown in Figure 5. After obtaininga 20 min baseline during which prolonged presynaptic bursts weregiven every 5 min and at the end of which D-AP-5 was washed out(Fig. 5A₁,A₂), we induced LTP. D-AP-5 was then reapplied, andbursts were restarted. Figure 5, B₁ and B₂, illustrates that thedepressed responses at the end of the burst exhibited an increasein amplitude that was equivalent to that of the control responses(control responses, 272 ± 6%; depressed responses, 290 ± 16%).To ensure that in this cell these prolonged bursts were indeedmaximally depressing, we applied adenosine (2 µM) that, consistentwith the experiment illustrated in Figure 4, dramatically decreasedthe control responses but had no effect on the depressed responses.These two manipulations (LTP and adenosine) performed on the sameset of synapses strongly suggest that a redistribution of synapticstrength does not occur during hippocampal LTP. As an additionalcontrol, we also applied kynurenic acid (250 µM), a low-affinityglutamate receptor antagonist. This had the expected effect inthat, like LTP, both the control and depressed response amplitudeschanged in parallel after washout of the drug (control responses,241 ± 5%; depressed responses, 228 ± 17%; Fig. 5A,B₂). At theend of the experiment we applied NBQX, a specific AMPA receptorantagonist, which abolished both the control and the depressedresponses (Fig. 5A,B₁).

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Figure 5. Example of the synaptic response to prolonged bursts after LTP, adenosine, and kynurenic acid. A, Typical experiment in which the induction of LTP with pairing (filled arrow) results in a stable potentiation of the control responses (A₁) as well as the depressed responses elicited by the prolonged presynaptic bursts (A₂; 40 Hz; 80 stimuli). Adenosine (2 µM), kynurenic acid (Kyn; 250 µM), and NBQX (5 µM) were perfused during the times indicated by the horizontal bars. Adenosine depressed the control responses without affecting the depressed responses. Kynurenic acid depressed both responses. Traces are averages of 60 responses and are centered over the time when the averages were taken. Calibration: A₁, A₂, 200 pA, 20 msec. Note, however, the different amplitude scales in A₁ and A₂. B, Averages of control and depressed response amplitudes with LTP, adenosine, kynurenic acid, and NBQX. Absolute amplitudes are summarized (B₁). Control and depressed response amplitudes are normalized to their respective amplitudes during the baseline, in adenosine, and in kynurenic acid (B₂). All panels illustrate data from the same cell.

LTP was obtained in seven additional cells in which prolonged bursts were given (Fig. 6). Although there was a tendency forthe control responses to undergo more potentiation than the depressedresponses, on average the increase in the two was not significantlydifferent (control responses, 275 ± 30%; depressed responses,215 ± 32%; n = 8; p > 0.05, paired t test; Fig. 6A,C₂). In fact,the increases in response amplitudes throughout the burst weresimilar (Fig. 6B, inset), indicating that the fidelity of thesynaptic response, even with these prolonged bursts, is preservedduring LTP.

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Figure 6. Fidelity of the synaptic response to prolonged bursts is preserved after LTP. A, Summary graph (n = 8) showing that the control responses (A₁) and the depressed responses (A₂) undergo a similar, stable potentiation after the induction of LTP with pairing (filled arrow). Bursts were given at the times indicated by the open arrowheads (40 Hz; 80 stimuli). B, Control responses (bars, and $black-square$ ) and responses to burst (circles, $open circle$ and $bullet$ ]) during the baseline (open symbols, and $open circle$ ) and after pairing (closed symbols, $black-square$ and $bullet$ ). Inset, The same data but with the amplitudes of all responses after pairing normalized to the average amplitude of the control response after pairing (each point represents the responses to five stimuli in the burst). It is evident that the potentiation during LTP was uniform for responses to all stimuli of the burst, thus maintaining fidelity of the synaptic burst response. C, Averages of control and depressed response amplitudes during the baseline and after LTP. Amplitudes are normalized to the control response amplitude during the baseline (C₁). Control and depressed response amplitudes (C₂) are normalized to their respective ampli-tudes during the baseline and are not significantly different after LTP (275 ± 30 and 215 ± 32%, respectively; n = 8; p > 0.05, paired t test). All panels illustrate data from the same set of cells (n = 8).

In six of the eight cells we also applied adenosine (Fig. 7A-C) at a concentration (1-2 µM) that, after washout, gave us anincrease in the control response amplitude similar to that obtainedduring LTP. Again, consistent with the example shown in Figure4, when we washed out adenosine, the control response amplitudeincreased dramatically, whereas the depressed response amplitudewas unaffected (control responses, 280 ± 42%; depressed responses,104 ± 14%; n = 6; Fig. 7A,C₂). Thus in the same cells in whichLTP caused an equivalent increase in responses throughout theburst (i.e., failed to result in a redistribution of synapticstrength), we were able to demonstrate that depressed responseswere unaffected by a presynaptic manipulation of transmitter release,thus proving that the bursts were maximally depressing. In thesesame cells we also applied and then washed out kynurenic acidto assess how a pure postsynaptic manipulation would affect theresponses to prolonged bursts (Fig. 7D-F). Again, we chose a concentrationof kynurenic acid (250 µM) that, after washout, gave us an increasein the control response similar to that obtained during LTP. Aswould be expected, these results closely paralleled the LTP resultsobtained earlier in the same cells (Fig. 6). The increase in theamplitude of the control and depressed responses was similar (controlresponses, 223 ± 8%; depressed responses, 250 ± 30%; n = 6; Fig.7D,F₂) as was the increase for all responses in the bursts (Fig.7E, inset).

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Figure 7. Synaptic responses to prolonged bursts are altered by adenosine but not by kynurenic acid. A, After LTP, control responses (A₁) increase after washing adenosine (1-2 µM), but depressed responses (A₂; last 20 responses in burst) are unaffected (n = 6). Open arrowheads designate bursts (40 Hz; 80 stimuli). B, Control responses (bars, and $black-square$ ) and responses to burst (circles, $open circle$ and $bullet$ ) during adenosine (open symbols, and $open circle$ ) and after washing (closed symbols, $black-square$ and $bullet$ ) are shown. Each point represents the responses to five stimuli. C, Averages of control and depressed response amplitudes in adenosine and after wash are shown. Amplitudes are normalized to the control response amplitude in adenosine (C₁) and to the average amplitudes in adenosine (C₂). D, After LTP, both control (D₁) and depressed responses (D₂; last 20 responses in burst) increase after washing kynurenic acid (Kyn; 250 µM; n = 6). Open arrowheads designate bursts (40 Hz; 80 stimuli). The break in the graphs represents 5-10 min. E, Control responses (bars, and $black-square$ ) and responses to burst (circles, $open circle$ and $bullet$ ) during kynurenic acid (open symbols, and $open circle$ ) and after washing (closed symbols, $black-square$ and $bullet$ ) are shown. Inset, The same data are shown but with the amplitudes of all responses after washing normalized to the average amplitude of the control response after washing (each point represents the responses to five stimuli in the burst). It is evident that the responses to bursts underwent a uniform increase in gain. F, Averages of control and depressed response amplitudes in kynurenic acid and after wash. Amplitudes are normalized to the control response amplitude in kynurenic acid (F₁) and to the average amplitudes in kynurenic acid (F₂). All panels illustrate data after LTP from the same cells (n = 6), a subset of those shown in Figure 6.

These experiments strongly suggest that LTP at excitatory synapses on CA1 pyramidal cells is fundamentally different fromthe LTP observed in the neocortex (Markram and Tsodyks, 1996).However, it is conceivable that because we stimulated extracellularlyand recorded population synaptic responses, rather than stimulatingthe presynaptic cell directly as is done in paired recordings,a redistribution of synaptic strength may have occurred in ourexperiments without our detecting it because of inconsistent extracellularstimulation of the afferent fibers during the bursts. To addressthis issue, we attempted to record from connected pairs of hippocampalpyramidalcells.

LTP and burst-induced depression at synapses between pairs of hippocampal pyramidal cells

Recording from connected pairs of hippocampal pyramidal cells in slices is a difficult undertaking for many reasons, mostnotable of which is the low level of synaptic connectivity (MacVicarand Dudek, 1979; Miles and Wong, 1986; Sayer et al., 1990; Fosterand McNaughton, 1991; Malinow, 1991; Smith et al., 1995). We werefurther handicapped by the need to record from the postsynapticcell using the perforated-patch technique to obtain an adequatebaseline of burst responses for analysis. We first attempted torecord from connected CA3-CA1 pyramidal cell pairs. We examined29 cell pairs but did not observe a single connection. We thereforeturned our attention to CA3 pyramidal cell pairs in which thebasic properties of LTP are indistinguishable from those of LTPbetween CA3 and CA1 pyramidal cells (Zalutsky and Nicoll, 1990;Pavlidis and Madison, 1997; Debanne et al., 1998).

We recorded from a total of 209 pairs of CA3 pyramidal cells, finding 26 pairs that were synaptically connected. Initiallywe used the same experimental conditions that were used for theCA1 experiments. However, the CA3 region exhibited spontaneousbursting. This was prevented by doubling the concentrations ofthe divalent cations to reduce overall excitability (Frankenhaeuserand Hodgkin, 1957). It was also necessary to reduce the numberof stimuli in each burst, because we found the unitary responseswere generally depressed to a stationary level after three tofour stimuli. We therefore shortened the bursts to 10 stimuli(at 40 Hz) and gave them every 30 sec. The last six unitary responsesin the burst were designated as the depressed responses. The controlresponses consisted of the unitary responses to the first stimulusin each burst combined with unitary responses to interleaved singlestimuli.

Figure 8 shows the results from the four pairs of CA3 pyramidal cells in which it was possible to complete the experiment.As was the case for the population synaptic responses recordedin CA1 pyramidal cells, the unitary control response amplitudeand the unitary depressed response amplitudes exhibited a similarpotentiation after the induction of LTP (205 ± 42 and 234 ± 39%,respectively; n = 4; Fig. 8B,D₂). Indeed the amplitude of allunitary responses in the burst underwent a similar potentiation(Fig. 8C, inset). Thus, even though the presynaptic burst stimulationnecessary to elicit depressed responses in these CA3 cell pairswas similar to that used in the neocortical cell pairs (Markramand Tsodyks, 1996), these CA3-CA3 synapses exhibited a form ofLTP distinct from the redistribution of synaptic strength seenwith neocortical LTP.

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Figure 8. Fidelity of the synaptic response to presynaptic bursts is preserved after LTP when recording from pairs of CA3 pyramidal cells. A, Individual example showing averages of 40 consecutive unitary responses (lower traces) to presynaptic bursts (upper traces; 40 Hz; 10 stimuli) given at the times indicted by the letters a-d in B. Calibration: 100 mV, 10 pA, 50 msec. B, Summary graph (n = 4) showing that the unitary control responses (B₁) and the unitary depressed responses (B₂; last six responses in burst) undergo a similar, stable potentiation after induction of LTP with pairing (filled arrow). Bursts were induced in the presynaptic cell every 30 sec at the times indicated by the open arrowheads. C, Unitary control responses (bars, and $black-square$ ) and unitary responses to burst (circles, $open circle$ and $bullet$ ) during the baseline (open symbols, and $open circle$ ) and after pairing (closed symbols, $black-square$ and $bullet$ ). Inset, The same data but with the amplitudes of all responses after pairing normalized to the average amplitude of the control response after pairing (each point represents the responses to two stimuli in the burst). It is evident that the unitary responses to bursts underwent a uniform potentiation, thus maintaining fidelity to the original synaptic response. D, Averages of unitary control and unitary depressed response amplitudes during the baseline and after LTP. Amplitudes are normalized to the control response amplitude during the baseline (D₁). Control and depressed response amplitudes are normalized to their respective amplitudes during the baseline (D₂). They underwent a similar degree of potentiation (205 ± 42 and 234 ± 39%, respectively; n = 4). B-D, Data from the same set of connected CA3 cell pairs (n = 4), including the pair whose responses are illustrated in A.

  DISCUSSION

It is well established that the firing pattern of neurons in the CNS varies dramatically over time, ranging from single isolatedspikes to prolonged high-frequency bursts of action potentials(Ranck, 1973; Connors and Gutnick, 1990; Lisman, 1997). It isalso well documented that the probability of release and thusthe strength of synaptic transmission are markedly influencedby the pattern of presynaptic firing (Magleby, 1987; Zucker, 1989).Therefore a fundamental issue in understanding the neural encodingof information is to determine the consequences, if any, thatlong-lasting changes in synaptic strength might have on short-termsynaptic dynamics. We have examined this issue by asking whetherNMDA receptor-dependent LTP in the hippocampus involves a redistributionof synaptic strength with a presynaptic burst, as has been observedat neocortical synapses (Markram and Tsodyks, 1996), or insteadinvolves a uniform potentiation of responses to the stimuli oftheburst.

To address this issue we first recorded synaptic responses in CA1 pyramidal cells in response to brief presynaptic burststhat elicited facilitated responses. After the induction of LTP,the responses exhibited a uniform potentiation rather than a redistributionof synaptic strength, a finding that differs from that obtainedat neocortical synapses (Markram and Tsodyks, 1996). These resultsare in complete agreement with a recent study that examined theeffects of LTP on the synaptic responses to brief (80-200 msec),facilitatory bursts (Pananceau et al., 1998). There, it was alsofound that all of the responses to the stimuli of the train werepotentiated equally during LTP (i.e., no redistribution took place).Both sets of results using brief presynaptic bursts are consistentwith and follow from previous studies, which have found a lackof interaction between LTP at CA1 synapses and paired-pulse facilitation(McNaughton, 1982; Manabe et al., 1993; Asztely et al., 1996;but see Schulz, 1997; Sokolov et al., 1998). However, prolongedbursts of presynaptic stimuli result in short-term synaptic depression,which clearly uses processes not evoked by either paired pulsesor brief, facilitatory bursts (Dobrunz and Stevens, 1997). Thatthe processes resulting in synaptic depression may be affectedby LTP is supported by the observation that at neocortical synapses,the extent of redistribution of synaptic strength is positivelycorrelated with the extent of synaptic depression (Markram andTsodyks, 1996). Thus a conclusive test of whether LTP at hippocampalsynapses causes redistribution of synaptic efficacy requires thatthe presynaptic stimuli elicit synaptic responses that, like thosein the neocortical experiments, are maximally depressed by theend of thetrain.

We therefore extended the length of the burst and modified the recording conditions to elicit maximal depression of the responses.After confirmation that the responses were indeed maximally depressed,we again found that LTP was accompanied by a uniform potentiationof successive responses to the stimuli of the burst. Finally,because of the possibility that a redistribution of synaptic strengthwas overlooked because of inconsistent extracellular stimulationof afferents, we examined LTP between pairs of hippocampal pyramidalneurons. Yet again, LTP was associated with a uniform potentiationof successive responses to the stimuli of the burst. Thus, incontrast to LTP in the neocortex (Markram and Tsodyks, 1996),NMDA receptor-dependent LTP in the hippocampus involves a uniformpotentiation of responses to all patterns of stimulation, includingboth brief, facilitatory bursts and prolonged depressingbursts.

It should be noted that the burst response patterns between CA1 pyramidal cells (Figs. 1-7) and CA3 pyramidal cells (Fig. 8)differed. Although intrinsic differences in the properties ofthe presynaptic boutons contacting CA1 versus CA3 pyramidal cellsor inconsistent stimulation of afferent fibers when extracellularstimulation was used (but see Allen and Stevens, 1994) may havecontributed to this difference, we think that the different extracellular[Ca²⁺]/[Mg²⁺] ratio in the two experiments is an important factor. Regardlessof the differences in the burst responses from the two sets ofsynapses, however, the important finding was that both synapsesunderwent LTP in which the individual synaptic responses wereuniformly increased rather than redistributed. The similarityof these results may not be surprising because CA3-CA3 and CA3-CA1synapses exhibit similar forms of NMDA receptor-dependent synapticplasticity (Zalutsky and Nicoll, 1990; Pavlidis and Madison, 1997;Debanne et al., 1998).

Although the differences found between hippocampal and neocortical LTP are most likely indicative of a fundamental differencein the mechanisms responsible for LTP in these two brain regions,several differences in the experimental conditions between thetwo studies should be noted. These include the recording technique(perforated patch vs whole cell), the temperature at which experimentswere conducted, the presence or absence of GABA_A receptor-mediatedinhibition, and the extracellular divalent cation concentration.However, it seems unlikely that differences in these experimentalparameters could account for the presence or absence of a redistributionof synaptic strength duringLTP.

The simplest explanation for our results is that hippocampal synapses express a form of LTP that is primarily caused by somepostsynaptic modification of glutamate receptor function and/ornumber. This would cause the observed uniform increase in thesynaptic responses throughout the burst. In contrast, the moststraightforward explanation for the redistribution of synapticstrength observed at neocortical synapses is that they expressa form of LTP that involves significant alterations in presynapticmechanisms controlling transmitter release (Markram and Tsodyks,1996). For instance, an increase in the probability of transmitterrelease would enhance the responses to the early stimuli of theburst but would have minimal effects on depressed responses atthe end of theburst.

What are some of the functional implications of the uniform potentiation of responses to bursts shown here? Abbott et al.(1997) hypothesize that depression serves to control synapticgain by attenuating responses to afferents with statically elevatedfiring rates. If afferents exhibit a broad range of firing rates,some level of attenuation is obviously important. However, a redistributionof synaptic strength has no effect on the average postsynapticcontribution of an afferent input (Tsodyks and Markram, 1997).Thus at afferent rates of firing in which temporal summation andsynaptic attenuation are significant factors, LTP in the formof redistribution will have little effect on either the actionpotential timing or firing rate of the postsynaptic cell. On thebasis of our results, hippocampal LTP may serve to override synapticattenuation under such circumstances so that the important inputs(those that are potentiated) can drive the postsynaptic cell moreeffectively. Separately, Lisman (1997) hypothesizes that at agiven synapse only one of the stimuli in a burst result in a quantalresponse and that therefore bursts are the fundamental unit ofthe neural code. Under such circumstances, the response at a singlesynapse can be characterized by the conditional probability thata given stimulus in the burst will result in quantal release whenall the previous stimuli fail to cause quantal release. LTP inthe form of redistribution will serve to increase the probabilitythat the single release event occurs early in the burst, therebydecreasing the probability that it will occur later. Thus thetiming of the postsynaptic response to a burst (i.e., the timingof the single quantal release) will be advanced after the redistributionassociated with neocortical LTP. The quantal size will be unaffected.As mentioned above, our results with hippocampal LTP are mosteasily explained by an increase in the postsynaptic response.Therefore, in Lisman's model the single quantum will be releasedwith the same timing (defined by the series of conditional probabilities)but will be of a greater magnitude. In this context, therefore,the effects of a redistribution of synaptic strength will be significantwhere the precise timing of the inputs affects the firing of thepostsynaptic cell, whereas the effects of hippocampal LTP willbe significant where the synaptic weights most affect the firingof the postsynapticcell.

We have considered the interaction between LTP and short-term plasticity manifested in responses to bursts of stimuli. Wehave found that NMDA receptor-dependent LTP in the hippocampusinvolves an unconditional potentiation entirely independent ofthe temporal pattern of the input, thus preserving the fidelityof responses to dynamically modulated stimuli. Current evidencesupports the hypothesis that LTP may be one of the biologicalsubstrates of learning and long-term memory (Stevens, 1998). Ithas recently become apparent that both burst-induced depressionand burst-induced facilitation may also serve functional rolesin the neural coding of information (Buonomano and Merzenich,1995; Abbott et al., 1997; Lisman, 1997; Tsodyks and Markram,1997). This study of the interaction between LTP and short-termplasticity should therefore help in understanding how synapsesin the hippocampus undergo meaningful modifications that can beused for the encoding of newinformation.

  FOOTNOTES

Received Sept. 2, 1998; revised Nov. 25, 1998; accepted Dec. 1, 1998.

D.K.S. is supported by a National Institutes of Health National Research Service Award Postdoctoral Training Fellowship. R.A.N.is a member of the Keck Center for Integrative Neuroscience andthe Silvio Conte Center for Neuroscience Research and is supportedby grants from the National Institutes of Health. R.C.M. is amember of the Center for the Neurobiology of Addiction and theCenter for Neurobiology and Psychiatry and is supported by grantsfrom the National Institutes of Health, by an Investigator Awardfrom the McKnight Endowment Fund for Neuroscience, and by a grantfrom the Human Frontier Science Program. We thank Antonello Bonciand other members of the Malenka and Nicoll laboratories for manyuseful comments and discussions during the course of theseexperiments.
Correspondence should be addressed to Dr. R. Malenka, Department of Psychiatry, Langley Porter Psychiatric Institute, Box0984, University of California, San Francisco, CA94143.

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Abstract
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