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The Journal of Neuroscience, March 1, 2002, 22(5):1823-1830
Long-Term Depression in the Developing Hippocampus: Low Induction Threshold and Synapse Nonspecificity
Pontus Wasling, Eric Hanse, and Bengt Gustafsson Institute of Physiology and Pharmacology, Göteborg University, SE-405 30 Göteborg, Sweden
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
It was observed that the use of paired-pulse afferent stimulation as test stimulation (0.1-0.02 Hz) in the hippocampal CA1 area in young (1-2 week) rats, but not in older ones, led to declining synaptic activity. We show that such very low-frequency stimulation leads to long-term depression (LTD) initiated by activation of NMDA receptor channels and/or T-type voltage-dependent calcium channels. The depression is initiated within three or four such stimuli, and <10 are sufficient to induce a notable long-term effect. When the paired-pulse stimulation exceeded threshold for postsynaptic spike activation, the depression was preceded by an NMDA receptor-dependent potentiation. Irrespective of whether homosynaptic potentiation or depression occurred, the paired pulse stimulation also induced depression in neighboring synapses alternately activated by single stimuli. These results point to a very high sensitivity for induction of synaptic depression during the neonatal period. They also support the notion that a brief rise in postsynaptic calcium can induce long-term potentiation (LTP) or LTD, a larger rise more likely to induce LTP, as well as that a prolonged modest increase produces selectively only LTD.
Key words: long-term depression; hippocampus; CA1; heterosynaptic; synaptic plasticity; development
INTRODUCTION
After activation, synapses alter their efficacy, even after a single stimulus. Such paired-pulse (PP) plasticity is generally attributed to an alteration in presynaptic release probability after the first stimulus (Katz and Miledi, 1968
; Zucker, 1989
In experiments using slices from young (1-2 week) rats we observed that the use of PP stimulation at low rates (0.1 Hz) as test stimulation led to difficulties in establishing a stable baseline. Thus, PP stimulation producing field EPSPs that were subthreshold for spike activation led to a decline in field EPSP magnitude. In the present report we demonstrate that this decline is caused by the development of LTD by such stimulation, not only of the PP-stimulated synapses, but also of neighboring synapses alternately activated by single stimuli.
MATERIALS AND METHODS
Slice preparation and solutions. Experiments were performed on hippocampal slices from 6- to 42-d-old rats (n = 121). The animals were anesthetized with isoflurane, decapitated, and their brains were removed to an ice-cold artificial CSF (ACSF) solution containing 6 mM Mg2+ and 0.5 mM Ca2+. Slices (400-µm-thick) were obtained with a vibratome (Campden Instruments, Loughborough, UK) and stored in ACSF at room temperature. After at least 30 min of storage, a single slice was transferred to a recording chamber where it was kept submerged in a constant flow (~2 ml/min) at 30-32°C. The perfusion fluid contained (in mM): NaCl 124, KCl 3, CaCl2 4, MgCl2 4, NaHCO3 26, NaH2PO4 1.25, and D-glucose 10 and was continuously bubbled with 95% O2 and 5% CO2, pH ~7.4. Bicuculline methiodide (10 µM) was always present, unless otherwise stated, to block GABAA receptor-mediated activity. The higher than normal calcium and magnesium concentrations were used, and a surgical cut between CA1 and CA3 regions were made, to counteract the increased excitability in the presence of bicuculline. In some of the experiments in which bicuculline was not present, the higher concentrations of calcium and magnesium were still used for direct comparison of experiments with and without GABAAergic inhibition. In other such experiments, calcium and magnesium were present at more physiological concentrations (2 mM).
Recording and analysis. Electrical stimulation of afferent fibers and recordings of extracellular synaptic potentials were performed in the CA1 hippocampal region. Stimuli consisted of 0.2 msec negative constant current pulses (15-50 µA) delivered through bipolar tungsten wires. Stimulation electrodes were positioned in the stratum radiatum on either side of the recording electrode to provide two independent afferent inputs projecting to the same dendritic region. Both inputs received a test stimulus every 10 sec, but 5 sec apart. The stimulation intensity was set not to evoke firing in the postsynaptic neurons, unless otherwise stated, as evidenced by the absence of a population spike distorting the field EPSP.
Recordings were made by means of a glass micropipette (filled with 3 M NaCl) in stratum radiatum. Field EPSPs were amplified with an Axoclamp-2A (Axon Instruments, Foster City, CA) and filtered at 3 kHz. Data were digitized (10 kHz sampling rate) and collected using a 486 personal computer. Evoked responses were analyzed off-line using custom-made IGOR Pro (WaveMetrics, Lake Oswego, OR) software, written by Pontus Wasling. Field EPSP magnitude was estimated by linear regression over the first 0.8 msec of the initial slope. The presynaptic volley was measured as the peak-to-peak amplitude of the initial positive-negative deflection, and it was not allowed to change by >3% over the 40-60 min stimulation period. Statistical significance for paired and independent samples was evaluated using Student's t test (p < 0.05).
Drugs used were: D-2-amino-5-phosphonopentanoate (D-AP-5) and (RS)-1-aminoindan-1,5-dicarboxylic acid (AIDA) from Tocris Neuramin (Bristol, UK), and bicuculline methiodide and NiCl2 from Sigma-Aldrich (Stockholm, Sweden).
RESULTS
When in a 4- to 5-week-old rat afferent stimulation at 0.1 Hz shifted from a single to a PP stimulus (50 msec interval) for 20 min, field EPSP slopes remained much the same during as well as after the PP stimulus epoch (Fig. 1A) (104 ± 3%; n = 6; 20 min after end of PP stimulation). However, when performing the same experiment in younger rats (6-12 d), field EPSPs started to depress during the PP stimulation and remained thereafter depressed (Fig. 1B). This depression could be followed for the duration of the recording, in some cases up to 2 hr, and is thus an LTD. It was not associated with any change in the afferent volley (see Materials and Methods) and is thus an LTD of synaptic transmission. In 6- to 12-d-old rats the field EPSPs 20 min after cessation of PP stimulation had decreased to 71 ± 2% of baseline (n = 8). Also when examined in somewhat older rats, 17-18 d, LTD, albeit smaller, could be evoked (77 ± 3%; n = 9). After two 20 min PP stimulation epochs (20 min interval) in 6- to 12-d-old rats field EPSPs were further depressed (to 48 ± 3%; n = 3). However, additional stimulation epochs did not produce more depression, indicating that the LTD was saturable.
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Figure 1. PP stimulation elicits LTD in young but not in older rats. A-C, Summary plots of normalized initial slope measurements of field EPSPs, evoked in the stratum radiatum layer of the hippocampal CA1 region. Stimulation rate is 0.1 (A, B) and 0.033 Hz (C). The horizontal bars indicate the time period during which single volley test stimulation was replaced by PP stimulation. The slope measurements are normalized with respect to the 2 min period immediately preceding the onset of PP stimulation. In A and B average values ± SEM are shown. Insets are the averages of 12 sweeps taken from representative experiments, at a time indicated by the characters in the graph. Calibration: 0.2 mV, 10 msec. A, PP stimulation is applied for 20 min at 0.1 Hz in 27- to 42-d-old rats (n = 6). B, PP stimulation is applied for 20 min at 0.1 Hz in 6-12 d old rats. Data are pooled from experiments using PP interstimulus intervals of 50 msec (n = 4), 100 msec (n = 2), and 200 msec (n = 2). C, From one experiment, using a 10-d-old rat, showing the effect of PP stimulation when the test frequency was 0.033 Hz.
When examined in the younger rats, LTD occurred using a range of test frequencies and PP intervals. Thus, stimulation at 0.033 Hz led to a LTD similar in development (per PP stimulus) to that at 0.1 Hz (Fig. 1C), and even a 0.016 Hz test frequency led to an LTD (data not shown). Similarly, when using longer PP intervals (200-1000 msec) LTD, albeit smaller (81 ± 3%; n = 6), was observed. Similar values were also found at PP intervals of 2.5 sec (80 ± 4%; n = 7).
The above experiments were performed in the presence of the GABAA receptor antagonist bicuculline to allow for the analysis of changes in the excitatory transmission alone. The presence of disinhibition was, however, not a prerequisite to observe PP-induced LTD. In fact, in the absence of bicuculline, PP stimulation led to an even larger LTD (57 ± 5%; n = 5). Neither was the use of higher than normal calcium and magnesium concentrations (4 mM; see Materials and Methods) necessary for the observation of this LTD. Thus, in the absence of bicuculline and in 2 mM calcium and magnesium in the perfusion solution, the LTD was of about similar magnitude (71 ± 3%; n = 5).
Induction of PP LTD involves both NMDA receptors and T-type calcium channels
To examine the pharmacology of the induction of this LTD, 8- to 13-d-old rats were examined, the PP interval was kept at 50 msec, and bicuculline was used to block GABAA receptor-mediated inhibition, unless otherwise stated. In the presence of the NMDA receptor antagonist D-AP-5 (50-100 µM), PP stimulation led to an LTD that was smaller, although not significantly so (78 ± 2%, n = 10; p > 0.05) (Fig. 2A). T-type voltage-gated calcium channels can be involved in the induction of LTD, in particular a form observed when synaptic inhibition is not blocked (Oliet et al., 1997
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Figure 2. Induction of LTD elicited by PP stimulation involves both NMDA receptor channels and T-type Ca2+ channels. A-C, Summary plots as described in Results and in Figure 1. All experiments were performed on 8- to 13-d-old rats. A, PP stimulation was applied in the presence of (50-100 µM) D-AP-5 (n = 10). B, PP stimulation was applied in the presence of 100 µM Ni2+ (n = 7). C, PP stimulation was applied in the presence of both D-AP-5 (50 µM) and Ni2+ (100 µM) (n = 5).
In the absence of bicuculline, both D-AP-5 and Ni2+ significantly reduced the LTD, from the 57% (± 5; n = 5) observed in control solution to 87 ± 3% (n = 8; D-AP-5) and 75 ± 3% (n = 5; Ni2+). This larger reduction of LTD by AP-5 and Ni2+ than in the disinhibited slice may be a consequence of the fact that NMDA receptor channels and voltage-gated calcium channels interact in a dual manner in that they both permeate calcium ions in a voltage-dependent manner and also produce depolarization. Blockade of one type of channel would then be expected to cause a supralinear reduction of the calcium signal because of less overall depolarization. It is not unlikely that such an effect is larger when inhibition is present, making the overall depolarization during synaptic activation less (Hanse and Konnerth, 1998
Because both D-AP-5 and Ni2+ seemed able to reduce the amount of LTD produced, it was examined whether the coapplication of these antagonists could more fully block LTD. In fact, in such experiments (in the presence of bicuculline) LTD was reduced to an almost nonsignificant level (94 ± 2%; n = 5) (Fig. 2C). On the other hand, coapplication of D-AP-5 and nifedipine led to an LTD (84 ± 4%; n = 6) not significantly smaller than that found in D-AP-5 alone. Metabotropic glutamate receptors (mGlurs) have been implicated in some forms of LTD (Bolshakov and Siegelbaum, 1994
The reduced LTD observed in the presence of D-AP-5 and Ni2+ was not secondary to reductions of field EPSP amplitude resulting from application of these drugs. In these experiments the stimulation strength was set to evoke similarly sized baseline field EPSPs, and the 10-20% reduction of the field EPSP by Ni2+ (none by D-AP-5) was thus compensated for. On average, the field EPSP peak amplitudes in control solution, in D-AP-5, in Ni2+, and in D-AP-5 combined with Ni2+ were 0.39, 0.34, 0.37, and 0.35 mV, respectively.
LTD can be preceded by an initial potentiation
When PP stimulation was strong enough to produce postsynaptic spike activity (Fig. 3A, inset), the LTD was preceded by a potentiation of the field EPSP slope (Fig. 3A). However, the final level of depression (20 min after end of PP stimulation) was much the same (75 ± 1%; n = 9) as when this potentiation did not occur. In Figure 3B are illustrated results from experiments in which only a brief episode (nine stimuli) of PP stimulation was given. In experiments in which subthreshold stimuli were used (inset b) depression resulted, whereas those in which spikes were evoked (inset a) potentiation was observed. In the presence of D-AP-5 (50 µM), such strong PP stimulation (insert) did not result in any initial potentiation, only in LTD (Fig. 3C). On the other hand, Ni2+ (100 µM) did not block this initial potentiation (Fig. 3D). PP stimulation (nine PP stimuli) thus seems capable of initiating not only LTD but also NMDA receptor-dependent potentiation. It can be noted that although being of much smaller initial magnitude, the LTD evoked by this brief PP stimulation was much more stable than the corresponding potentiation.
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Figure 3. PP stimulation producing population spike activity elicits an initial NMDA receptor-dependent potentiation preceding the depression. A-D, Summary plots as described in Results and in Figure 1. Insets are averages of three sweeps taken from representative experiments, at the time indicated by the characters. Calibration: 0.2 mV, 10 msec. A, PP stimulation (interstimulus interval 10-50 msec) associated with evident population spikes leading to an initial potentiation (n = 9). B, Data from experiments in which PP stimulation did (a; n = 5), and did not (b; n = 5) give rise to population spike activity are shown superimposed. Only nine consecutive PP stimulations (interstimulus interval 10 msec) were given. C, Nine consecutive PP stimulations (interstimulus interval 10 msec) associated with population spike activity were given in the presence of 50 µM D-AP-5 (n = 7). Note the absence of an initial potentiation. D, The same but in the presence of 100 µM Ni2+ (n = 2). Note the large initial potentiation.
LTD, but not initial potentiation, is synapse-nonspecific
In the present experiments, stimulation was alternated between two electrodes positioned in the dendritic layer on either side of the recording electrode, the stimuli being 5 sec apart. When PP stimulation was initiated at one of these stimulation sites, the field EPSP, but not the afferent volley, produced by stimulation at the other site also started to become depressed (Fig. 4A). Twenty minutes after the cessation of PP stimulation, the control input was still depressed to 88 ± 4% (n = 8) of baseline value, i.e., demonstrating an LTD of approximately one-third of that of the conditioned input. When stimulation was such that an initial potentiation occurred, this potentiation was not seen in the control input (Fig. 4B). Thus, depression of the control input is not secondary to overlap between the fiber populations activated by the two stimulation electrodes. That is, the LTD, in contrast to the potentiation, is not specific for the PP-activated synapses.
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Figure 4. PP stimulation induces a synapse specific potentiation, but a synapse nonspecific depression. A-D, Summary plots as described in Results and in Figure 1. The two afferent inputs projecting to the same dendritic region were alternately stimulated at 0.1 Hz. A, Top, Field EPSP changes occurring in one of the inputs (heterosynaptic), when the other input (homosynaptic) was subjected to PP stimulation (n = 8). Bottom, Same but for the presynaptic volley. B, Experiments in which PP stimulation was associated with population spike firing (n = 6). Note that the initial potentiation observed in the homosynaptic input (closed circles) is absent in the heterosynaptic one (open circles). C, Same as in A, but in the presence of 50 µM D-AP-5. Note that each plotted value is the average of three consecutive field EPSPs (n = 7). D, Same as in C, but in the presence of 100 µM Ni2+ (n = 7). Note that the error bars are within the symbols.
This heterosynaptic LTD was observed in the presence of D-AP-5 (50 µM) (Fig. 4C) as well as in the presence of Ni2+ (100 µM) (Fig. 4D). Thus, activation of both NMDA receptor channels and T-type calcium channels can support the spread of LTD to unconditioned synapses. After coapplication of D-AP-5 and Ni2+, no LTD was observed (98 ± 4%; n = 4).
Onset of LTD
As can be noted in Figures 1-4, field EPSPs started to depress within the first minute of PP stimulation. Because PP stimulation per se did not produce field EPSP changes (Fig. 2C), it would appear that LTD is rapidly induced, as also indicated by the stability of the depression after interruption of PP stimulation after a few stimuli (Fig. 3B,C). In Figure 5 are shown, on an expanded time scale, LTDs evoked in the test input at subthreshold PP stimulations (A), in the control input (B), and in the test input in the presence of D-AP-5 to ascertain the absence of an initial potentiation component (C). On balance, these curves would suggest an onset of LTD within three or four stimuli, i.e., within ~30 sec.
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Figure 5. Onset of LTD induced by PP stimulation. A-C, Summary plots as described in Results and in Figure 1. A, Data from experiments in which PP stimulation produced no initial potentiation (n = 23). B, Same as in A, but for a heterosynaptic input (n = 26). C, Same as in A, but in the presence of D-AP-5 (50-100 µM) (n = 17). The vertical lines denote the time of PP stimulation onset, and 1 min thereafter, respectively. Note in A-C that the depression is initiated already within ~30 sec, i.e., within three or four stimuli.
PP-induced LTD is associated with changes in PP facilitation
The use of PP stimulation to induce LTD also allowed for the estimation of possible changes in PP plasticity during the development of LTD. Because there was no baseline PP stimulation, changes occurring in PP facilitation (PPF) during the development of LTD were normalized with respect to the average PPF during the first 10 PP stimulations. As can be noted in Figure 6, the development of LTD is paralleled by an increase in PPF that reached 16 ± 3% (n = 6) at the end of PP stimulation. A reduction of the EPSP by a decrease in stimulation strength (to 64% of control i.e., to approximately the same as an LTD) did not alter the PP ratio (101% of control; n = 7). The increase in PPF in association with LTD was thus not merely a consequence of the reduction in field EPSP magnitude. An increase of PPF was observed both for the LTD observed in the presence of D-AP-5 (9 ± 3%; n = 7) as well as of Ni2+ (19 ± 6%; n = 8). In a few experiments PP stimulation was repeated after ~20 min, demonstrating that the increase in PPF remained throughout this period.
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Figure 6. PP-induced LTD is associated with an increase in PPF. A, Summary plot, as described in Results and in Figure 1 (n = 6). B, PPF, normalized with respect to the average value obtained during the first 100 sec of PP stimulation, is plotted for the experiments illustrated in A. C, Averaged field EPSPs (n = 5) from a representative experiment taken at the times indicated by the characters (a; thick line, b; thin line). Calibration: 0.2 mV, 5 msec. D, Field EPSPs in C are shown after normalization with respect to the first EPSP.
DISCUSSION
It has been a common observation that LTD is most easily generated in young rats (Dudek and Bear, 1993
Activation of both NMDA receptor channels and Ni2+-sensitive channels was found to initiate the induction of this LTD, the homosynaptic as well as the heterosynaptic one. Considering the small requirement for postsynaptic activity for the induction the Ni2+-sensitive channels are likely to be T-type voltage-gated calcium channels. This notion is supported by the observation that a greater amount of LTD was observed when postsynaptic inhibition was intact, a result likely explained by a larger possibility for deinactivation of such channels. Moreover, the involvement of low-voltage-activated calcium channels of L-type is less likely because nifedipine had little effect on this LTD.
The PP-induced LTD appears, with respect to its calcium sources for induction, not to resemble any previously described LTD. The limited effect of NMDA receptor antagonism (by itself), the dependence also on T-type calcium channels, and the heterosynaptic nature, sets the PP-induced LTD apart from low-frequency (1-2 Hz) induced LTD (Dudek and Bear, 1992
PP-induced LTD and potentiation: differential thresholds
LTD is most commonly induced by prolonged (10 min) low-frequency activation, leading to the notion that its induction depends on a small but prolonged increase of postsynaptic calcium. However, brief high-frequency tetanization during partial NMDA receptor blockade can also produce LTD (Cummings et al., 1996
A second finding is that stronger PP stimulation that led to postsynaptic spike activity elicited an NMDA receptor-dependent potentiation rather than LTD. As for the LTD, this potentiation became initiated within the very first few stimuli. This result is then in line with the above notion that "a brief rise in postsynaptic calcium can induce either LTP or LTD, a larger rise more likely to induce LTP." Interestingly, this potentiation was not reduced by Ni2+ and was fully blocked by an NMDA receptor antagonist. This result agrees with the idea that potentiation is more discriminative with respect to its calcium source than is depression (Hanse and Konnerth, 1998
Finally, if the strong PP stimulation was interrupted after a few stimuli, the potentiation slowly (10-20 min) decayed back toward baseline values, a decay that can be seen when tetanic stimulation is too brief or too weak to elicit LTP (Hanse and Gustafsson, 1994
Prolongation of a 5 Hz train can affect the LTP observed using a briefer train (Thomas et al., 1996
Input nonspecificity
What seems also particular with this LTD is its lack of synapse specificity. LTDs previously reported, using stimulation subthreshold for postsynaptic spike generation, have been described as being input specific (Dudek and Bear, 1992
Which is the implication of the associated changes in PPF?
Hippocampal LTD is generally thought to have a postsynaptic expression based on a reduction in AMPA receptor number (Malenka and Nicoll, 1999
FOOTNOTES Received Aug. 13, 2001; revised Nov. 27, 2001; accepted Dec. 18, 2001.
This project was supported by the Swedish Medical Research Council (Project Numbers 05180 and 12600).
Correspondence should be addressed to Pontus Wasling, Institute of Physiology and Pharmacology, Göteborg University, Box 432, SE-405 30 Göteborg, Sweden. E-mail: pontus.wasling{at}physiol.gu.se.
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