Department of Molecular and Cell Biology, University of California, Berkeley, California 94720
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ABSTRACT |
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Yang, Shao-Nian,
Yun-Gui Tang, and
Robert
S. Zucker.
Selective Induction of LTP and LTD by Postsynaptic
[Ca2+]i Elevation. Long-term
potentiation (LTP) and long-term depression (LTD), two prominent forms
of synaptic plasticity at glutamatergic afferents to CA1 hippocampal
pyramidal cells, are both triggered by the elevation of postsynaptic
intracellular calcium concentration ([Ca2+]i). To understand how one signaling
molecule can be responsible for triggering two opposing forms of
synaptic modulation, different postsynaptic
[Ca2+]i elevation patterns were generated by
a new caged calcium compound nitrophenyl-ethylene
glycol-bis(-aminoethyl
ether)-N,N,N',N'-tetraacetic acid in CA1 pyramidal cells. We found that specific patterns of [Ca2+]i elevation selectively activate LTP or
LTD. In particular, only LTP was triggered by a brief increase of
[Ca2+]i with relatively high magnitude, which
mimics the [Ca2+]i rise during electrical
stimulation typically used to induce LTP. In contrast, a prolonged
modest rise of [Ca2+]i reliably induced LTD.
An important implication of the results is that both the amplitude and
the duration of an intracellular chemical signal can carry significant
biological information.
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INTRODUCTION |
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Long-term potentiation (LTP) and
depression (LTD) are two forms of activity-dependent synaptic
plasticity that are broadly assumed to be involved in learning and
memory (Bliss and Collingridge 1993; Linden and
Conner 1995
). In LTP, brief high-frequency afferent activity
leads to a long-lasting increase in the strength of synaptic transmission, whereas prolonged low-frequency activity results in a
persistent reduction in synaptic strength. Both processes are triggered
by an increase in the level of postsynaptic intracellular calcium
concentration ([Ca2+]i). Proposals that LTD
is induced simply by a lower minimum [Ca2+]i
than LTP (the "differential threshold hypothesis") (see
Artola and Singer 1993
; Lisman 1989
) are
not supported by experiments showing that LTD and LTP have similar
probabilities of being activated by a brief rise in postsynaptic
[Ca2+]i, in the submicromolar range
(Neveu and Zucker 1996a
). One possibility is that a rise
in [Ca2+]i enables the induction of both LTD
and LTP but that other processes activated by the different patterns of
afferent stimulation are responsible for determining the outcome, for
example, activation of muscarinic (Huerta and Lisman
1995
), metabotropic (Bortolotto et al. 1994
;
Cohen and Abraham 1996
), or
N-methyl-D-aspartate (NMDA) (Huang et al.
1992
) receptors. Another possibility is that LTP and LTD are
specifically activated by different patterns of [Ca2+]i elevation.
Previous studies (Neveu and Zucker 1996a,b
) with
photosensitive Ca2+ chelators to induce LTP or LTD were
severely constrained by the limitations of available chelators.
Nitr-5 changes its Ca2+ affinity by only 30-fold so
that [Ca2+]i cannot be elevated to a very
high level. Even moderate increases in
[Ca2+]i require nearly complete photolysis of
nitr-5 so that repeated photolysis cannot be used to achieve a
prolonged rise in [Ca2+]i. Photolysis of
DM-nitrophen produces a large [Ca2+]i
rise, and repeated partial photolysis can be used to prolong a small
[Ca2+]i rise, but interaction of this
substance with endogenous cytoplasmic magnesium leads to a rise in
[Ca2+]i while filling the cell (the
"loading transient") (Neher and Zucker 1993
), which
can itself induce either LTP or LTD even before beginning the recording
session or photolysing the compound. In this study, we exploit the
properties of the recently introduced chelator nitrophenyl- ethylene
glycol-bis(
-aminoethyl
ether)-N,N,N',N'-tetraacetic acid (EGTA) (Ellis-Davies and Kaplan 1994
) to produce
either a large rise in [Ca2+]i with nearly
full photolysis or a prolonged rise in
[Ca2+]i with repeated partial photolysis
without binding magnesium ions and the complication of a loading
transient. This allows one to manipulate
[Ca2+]i levels in ways that were not
previously possible.
We used selected patterns of photolysis of nitrophenyl-EGTA to show
that, when the amplitudes and durations of
[Ca2+]i elevation are adjusted to resemble
those occurring during electrical stimulation used to induce LTP or LTD
(Otani and Connor 1996; Petrozzino et al.
1995
), LTP or LTD is selectively and exclusively produced by
such changes in [Ca2+]i.
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METHODS |
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Transverse hippocampal slices, 400 µm thick, were cut by
vibratome from brains of 11- to 22-day-old Sprague-Dawley rats after halothane anesthesia and decapitation (Neveu and Zucker
1996a). Slices were maintained
1 h in recording medium
containing (in mM) 119 NaCl, 2.5 KCl, 2.5 CaCl2, 1.3 MgSO4, 1.0 NaH2PO4, 26.2 NaHCO3, and 11 D-glucose, saturated with 95%
O2-5% CO2. They were then transferred to a
submersion chamber and perfused continuously at 2.5 ml/min at 22°C.
Whole cell recording electrodes (4-7 M
) were filled with (in mM)
117.5 Cs gluconate, 17.5 CsCl, 8 NaCl, 10 N-2-hydroxyethylpiperazine-N'-2-ethanesulfonic acid, 0.2 EGTA, 2 Na2ATP, and 0.2 GTP, pH 7.2 adjusted with CsOH.
Electrode tips were filled with this solution containing 5-8 mM
nitrophenyl-EGTA (Molecular Probes), 50% loaded with Ca2+,
and neutralized with 7.5-12 mM HCl. Excitatory postsynaptic potentials
(EPSPs) were recorded under current clamp, holding cells at a membrane
potential of
80 mV, after correction for a
6 mV junction potential,
determined by measuring the potential difference between recording
medium and pipette solution with 3 M KCl microelectrodes and a KCl agar
bridge as ground lead. We continuously monitored pipette access and
cell input resistances by recording responses to a square pulse of
hyperpolarizing current (usually 30 pA) and balancing the initial
access resistance with a bridge circuit. Access resistance ranged
between 20 and 80 M
and varied <20% during experiments. Field
recordings were made in the stratum radiatum with a glass
microelectrode (3-6 M
) filled with 3 M NaCl. Schaffer
collateral/commissural afferents were stimulated in the same layer with
bipolar stainless steel electrodes by using 100-µs pulse of 0.5 to 5 V. Stimulus electrodes were positioned to excite afferents probably
ending
150 µm of the postsynaptically recorded cell body, as judged
by the rapid rise time of postsynaptic responses and from electrotonic
calculations (Tsai et al. 1994
). Such proximal synapses
are more likely to be fully equilibrated with the pipette solution when
recordings are made 20 min after forming seals and breaking into cells.
Large responses contaminated with active membrane responses were
avoided. Responses were sampled at 10 kHz, and maximal rising slopes
were calculated on-line with the Neurophysiologia program (David Selig, San Francisco) by using a least-squares regression to cubic spline curve fits. In field recordings, postsynaptic responses were
distinguished from electrical artifacts and presynaptic signals by
observing the recruitment of a delayed negative potential after a
graded artifact as stimulus intensity was increased. Because
stimulation was optimized for minimal excitation of proximal synapses
in the recorded cell and extracellular electrodes were not repositioned after establishing whole cell recording, field potentials often had
very small postsynaptic components. The maximum slope of the rising
phase of this component after the artifact returned to baseline was
measured. Responses were normalized to average values 5-10 min before
light exposure, and every other response is plotted to enhance clarity.
In summary graphs, responses are aligned with respect to light
exposures (Fig. 2) or electrical stimulation (Fig. 3), averaged across
experiments in 40-s bins, and means plotted ± SE. Significance
was evaluated with Student's t-test (two-tailed), comparing
all points before photolysis to all points afterward.
Photolysis was accomplished with a standard 100-W Hg lamp (Nikon)
fitted with a Uniblitz (Vincent Associates) shutter and aimed directly
at the slice, beginning at 20 min after starting perfusion of cells
with photolabile Ca2+ chelator from patch pipettes. In
LTP-inducing experiments, an f/1.5 75 mm focal length quartz
lens was used to increase light intensity. The light intensities with
and without the lens (1.0 and 0.13 W/cm2, respectively)
were measured with a radiometer (International Light Model IL1700) by
using a filter (Schott glass UG-1) with a transmittance spectrum
similar to the excitation spectrum of nitrophenyl EGTA, after
correcting for the reduction in intensity caused by the UG-1. Infrared
and far-ultraviolet radiation was minimized with a liquid filter
(Landò and Zucker 1989
) to minimize cytotoxic and
heating effects of light. Photolysis rate was measured in microcuvettes
(with DM-nitrophen as described by Zucker 1994
, and converting to
nitrophenyl EGTA from the known relative quantum efficiencies and
absorbances at 360 nm of the two photolabile chelators) at 87%/s with
the lens and 11%/s without it.
In calculations of postsynaptic [Ca2+]i, the
light intensity was assumed to be reduced by a factor of 2 to account
for absorbance of light at a depth of 100 µm in the slice, based on
our measurements of light absorbance at 360 nm in cortical slices of
varying thickness (360 nm is the center of the action spectrum for
photolyzing nitrophenyl-EGTA). Effects of photolysis on
[Ca2+]i were estimated from a model of
nitrophenyl-EGTA photolysis and binding kinetics in cells. The model,
written in BASIC programming language for Intel-based personal
computers, is similar to models that were previously described in some
detail (Landò and Zucker 1989; Zucker
1994
). It is a single-compartment model, appropriate for
uniform full-field illumination of a small cell where intracellular gradients in light intensity caused by self-absorption are minimal. The
model includes the binding of Ca2+ to nitrophenyl-EGTA and
its photoproduct and the effect of light on the respective levels of
photolyzed and unphotolyzed nitrophenyl-EGTA (Ellis-Davies et
al. 1996
), the binding of Ca2+ to native buffers,
assumed to be present at 1 mM concentration with 10-µM affinity and
20 mM · ms binding rate, and Ca2+ extrusion by a first
order pump, with pump rate (0.1 ms
1) adjusted to remove
Ca2+ with a time constant of 1 s without additional
exogenous buffer (Regehr and Tank 1992
). A commented
program listing and program disk are available from the authors on
request.
Given the 20-30 min we allow for equilibration of intracellular and
pipette solutions, nitrophenyl-EGTA concentration was assumed to equal
that of the patch pipette, for the following reasons. Filling of the
soma from 20- to 80-M pipettes should occur with a time constant of
from 1.8 to 7.4 min for access resistances of 20-80 M
(Eq.
18 in Pusch and Neher 1988
); equilibration of the first third
of 500-µm dendrites (Tsai et al. 1994
), where the
EPSPs we measure are likely to arise, should occur with a characteristic time of ~1 min
(x2/4D, x = 0.0015 cm, D = 10
6 cm2/s) (from
Gabso et al. 1997
); and fura-2 has been shown to reach 90% equilibration in proximal dendrites of pyramidal cells within 10 min (Helmchen et al. 1996
). Nitrophenyl-EGTA purity was
measured by Scatchard analysis at >95%. This information was used to
adjust Ca2+ loading of the chelator to leave resting
[Ca2+]i undisturbed at 100 nM. Despite these
precautions, significant uncertainties exist in the concentration,
affinity, and kinetics of native buffer, concentration and
Ca2+-loading of nitrophenyl-EGTA, light intensity at cells
recorded within a slice, and rate of Ca2+ removal by ion
pumps. Therefore simulations of the effects of nitrophenyl-EGTA
photolysis on [Ca2+]i remain only rough
order-of-magnitude estimates.
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RESULTS |
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According to the differential threshold hypothesis (Artola
and Singer 1993; Lisman 1989
), LTD has a low
intrinsic [Ca2+]i threshold and is
selectively induced by a modest rise in
[Ca2+]i, similar to what occurs during
induction of LTD by low-frequency afferent stimulation. LTP is
selectively induced by a greater rise in
[Ca2+]i, exceeding its higher intrinsic
[Ca2+]i threshold, as occurs during
high-frequency afferent stimulation. The problem with this hypothesis
is illustrated in Fig. 1. Whole cell
recordings were made from a CA1 pyramidal cell (Fig. 1, top traces) simultaneously with field recordings from the stratum radiatum (middle traces). The recorded pyramidal cell was
perfused for 20 min with a partially calcium-loaded solution of the
caged calcium compound nitrophenyl-EGTA (Ellis-Davis and Kaplan
1994
). The slices were exposed to two light flashes that
partially photolyzed the nitrophenyl-EGTA, calculated to elevate
postsynaptic [Ca2+]i by ~800 nM (Fig. 1,
bottom traces). This treatment caused a long-lasting
depression in afferent synaptic transmission to the cell containing
nitrophenyl-EGTA in two slices (Fig. 1, left panels, 30.0 ± 4.8% reduction in rising slope of EPSP, mean ± SD),
whereas in another experiment a long-lasting potentiation was produced (right panels, 41.6% increase in EPSP slope). Field
potentials, dominated by cells not filled with nitrophenyl-EGTA, are
unaffected by light exposures. When only a single light exposure was
used, elevating [Ca2+]i by only 130 nM, no
effects on synaptic transmission were observed.
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These results resemble more extensive results obtained with a different
caged calcium compound, nitr-5 (Neveu and Zucker 1996a), in which similar short-lasting minimal threshold
[Ca2+]i elevations were found to be
sufficient to induce LTP or LTD. In that study it was also shown that
photolytic induction of long-lasting depression occluded the induction
of LTD by low-frequency afferent stimulation, that photolytic induction
of long-lasting potentiation occluded the induction of LTP by
high-frequency stimulation, and that photolytically induced LTD and LTP
shared pharmacological sensitivities to phosphatase and calmodulin
inhibitors with electrically induced LTD and LTP respectively. Taken
together, the results indicate that LTD and LTP can both be induced by
brief submicromolar elevations in postsynaptic
[Ca2+]i, even in the absence of presynaptic
activity (Neveu and Zucker 1996b
).
To determine whether LTD and LTP can be selectively activated by
different temporal patterns of postsynaptic
[Ca2+]i elevation, we used different patterns
of light exposure to try to mimic the changes in
[Ca2+]i that typically accompany induction of
LTD and LTP by afferent stimulation (Otani and Connor
1996; Petrozzino et al. 1995
). The main results
are shown in Fig. 2. In the left
panels, slices were exposed to repeated dim flashes of the same
intensity as in Fig. 1, of durations from 2.6 to 15 s, spaced over
a 45-s interval, and designed to produce a rise in
[Ca2+]i to ~750 nM and lasting ~1 min.
The photolysis light pattern is shown in Fig. 2E,
top. The calculated temporal profile of
[Ca2+]i elevation shown in Fig.
2E, bottom, is similar in magnitude to that
occurring during 1-Hz stimulation (Otani and Connor
1996
; Petrozzino et al. 1995
), and Mulkey and
Malenka (1992)
showed that as little as 30-60 s of such stimulation
can induce measurable LTD. Effects of photolysis on EPSP rising slopes
from a typical injected cell are shown in Fig. 2A, with
field recordings in Fig. 2B. All of the responses from 20 to
30 min after photolysis were depressed below all of the responses
before photolysis (P
0.0001 by Wald-Wolfowitz
2-sample runs test), and a similar comparison in the field recordings
shows little change (P > 0.4). The EPSP reduction was
accompanied by no change in either pipette access or cell input
resistance. Sample responses to current injection are shown in Fig.
2A.
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In repetitions of this experiment, in which
[Ca2+]i was probably elevated to ~750 nM
for ~1 min, LTD was induced, or synaptic transmission was
persistently depressed, in five of six slices. The average reduction in
EPSP slope in these five slices was 25.8 ± 13.9% (measured as a
difference in all points before photolysis to all points afterward,
P < 0.02), as illustrated in Fig. 2C. Averaged changes in field recordings from these slices (Fig.
2D) show no change (reduction of 11.1 ± 10.1%,
P > 0.05). Photolysis-induced LTD often developed
slowly, as reported for LTD induced by electrical stimulation
(Cummings et al. 1996). LTP was never activated by this
protocol. Control experiments show that repeated light exposures of
this intensity and with durations
15 s have no effect on EPSPs in
cells not filled with a photolabile chelator (see Fig. 1D) (Neveu and Zucker 1996a
).
In contrast, Fig. 2, right panels, illustrate effects of single brighter exposures lasting 10 s that probably elevated [Ca2+]i to >10 µM (Fig. 2J) but only for a few seconds (calculated half-height width of [Ca2+]i rise is 2.5 s). In 10 of 28 slices, LTP, or a persistent enhancement of synaptic transmission, was induced shortly after photolysis of nitrophenyl-EGTA in the cell where [Ca2+]i was elevated to higher levels by intense photolysis (49.3 ± 12.4% increase in EPSP slopes, comparing all responses before and after photolysis, P < 0.001, Fig. 2H). Fig. 2F plots responses from a typical cell showing LTP, and Fig. 2G presents simultaneous field recordings. There was no significant change (increase of 2.7 ± 10.9%, P > 0.1) in slices where EPSPs were potentiated in the recorded cell (Fig. 2I). Control experiments show that, when unfilled cells are exposed to the bright illumination used to rapidly photolyze nitrophenyl-EGTA, there was no effect on EPSP amplitude (Fig. 3A).
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In the remaining 18 slices, photolysis induced no significant change in the recorded EPSP slope (7.7 ± 28.6% increase, P > 0.05) or the field EPSP slope (0.8 ± 10.8% increase, P > 0.15). Figure 3, B and C, shows the results from a typical cell and the averaged responses of the 18 nonresponding cells. These records also demonstrate the stability of our responses for prolonged recording periods and the absence of deleterious effects of photolysis photoproducts, confirming that the LTD generated by a more modest but prolonged [Ca2+]i elevation (Fig. 2, A and C) is due neither to drift in baseline response amplitude nor to photoproduct toxicity. A clear instance of LTD was never activated by this intense light protocol. Apparently, LTD and LTP are selectively and exclusively activated by the two patterns of [Ca2+]i elevation, LTD by a prolonged low increase in [Ca2+]i and LTP by a brief larger increase in [Ca2+]i.
Although a prolonged modest rise in [Ca2+]i
almost always induced LTD, a brief intense rise in
[Ca2+]i produced what clearly appeared to
resemble LTP, defined as a significant and persistent increase in EPSP
in the absence of significant changes in field potential responses, in
fewer than one-half the slices. This is not because the cells are
incapable of exhibiting LTP. In seven of eight slices in which the
LTP-inducing light exposure protocol failed to induce LTP (3.6 ± 8.3% decrease, P > 0.05), a subsequent afferent
tetanus (3 1-s trains, 100 Hz, with 1-s pauses) still generated LTP in
the recorded cell (65.6 ± 21.6%, P < 0.001) as
well as in the rest of the slice as indicated by the field recordings
(Fig. 4, left panels). In
contrast, in six slices in which nitrophenyl-EGTA photolysis did induce
LTP (65.9 ± 23.6% increase, n = 6, P < 0.01), subsequent tetanic afferent stimulation was
without further effect (2.0 ± 15.1% further increase, P > 0.05), except for a transient increase reflecting
posttetanic potentiation (Fig. 4, middle panels). Moreover,
like electrically induced LTP (Mulkey and Malenka 1992),
photolysis-induced LTP (52.6 ± 12.6% increase, n = 6, P < 0.001) could be reversed (to within
3.1 ± 9.8% of initial levels, P > 0.05) by
subsequent low-frequency stimulation (1 Hz for 10 min; Fig. 4,
right panels). Thus the long-lasting potentiation of
synaptic transmission evoked by a brief strong
[Ca2+]i elevation in 36% of our experiments
appears to be genuine LTP. We are unable to elevate
[Ca2+]i to high levels for more than ~2 s
before exhaustion of nitrophenyl-EGTA, and it was previously found that
[Ca2+]i must remain elevated for >2 s to
reliably induce LTP (Malenka et al. 1992
). Even a 1-s
tetanus at 100 Hz only evokes LTP if [Ca2+]i
is permitted to remain elevated for ~2-3 s. Therefore our LTP inducing protocol would be expected to induce LTP only some of the
time, just as we observed. The important result is that it never
induced LTD, whereas a prolonged small
[Ca2+]i increase almost always did.
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The striking differences in effectiveness of the protocols illustrated
in Fig. 2, left and right panels, in selectively
inducing LTD and LTP are revealed by analysis of the results in the
form of a two-way classification table. The LTD-inducing protocol
reduced transmission in five cells and had no effect in one. The
LTP-inducing protocol increased transmission in 10 cells and had no
clear persistent effect in 18. These patterns differ at the
P 0.0001 level of significance (
22 = 27.5).
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DISCUSSION |
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When the results of Figs. 1 and 2 are considered together, they
demonstrate that neither a difference in the amplitude of [Ca2+]i elevation nor a difference in
duration is sufficient by itself to determine the response of synapses
to this chemical signal. A modest brief
[Ca2+]i elevation induces LTP or LTD with
equal probability (Neveu and Zucker 1996a).
Substantially increasing the amplitude of the [Ca2+]i trigger selectively activates LTP,
whereas substantially increasing the duration of this signal
selectively activates LTD. Thus both amplitude and duration of the
[Ca2+]i signal are important in determining
the neuron's response. Furthermore, the results show that both forms
of synaptic plasticity can be reliably and selectively induced by
different patterns of [Ca2+]i elevation,
without the need to invoke any other Ca2+-independent
signaling or triggering process. This is reminiscent of the
differential activation of transcription factors by specific patterns
of [Ca2+]i elevation (Dolmetsch et al.
1997
).
It might be thought that the variable responses to a brief modest
[Ca2+]i elevation are due to a spatial
nonuniformity in [Ca2+]i in response to
modest photolysis. We do not deny that the elevation in
[Ca2+]i is likely to be higher in more
superficial dendrites than in deeper processes. Nevertheless, the
straightforward differential minimal threshold hypothesis predicts
that, as the level of photolysis is gradually increased, LTD induction
will always be observed first. This is the result we originally
expected, and it is in particular exactly what we did not observe
(Neveu and Zucker 1996a).
Likewise, global spatial [Ca2+]i nonuniformity across the entire dendritic tree is likely to be present during the intense photolysis that elicits only LTP and to prolonged weak photolysis that induces only LTD. However, within the restricted regions of a cell activated by one or a few neighboring inputs, there is likely to be little variation in local light intensity and the degree of photolysis and hence little variation in the rise in [Ca2+]i. If such variation were a prominent feature of the [Ca2+]i rises in our experiments, we would not expect our two stimulus paradigms to selectively activate opposite responses.
It might be argued further, however, that a local spatial gradient in endogenous Ca2+ buffering exists. For example, there might be more buffering in dendritic shafts than spines, resulting in a larger [Ca2+]i elevation in spines than shafts, and such local [Ca2+]i gradients might be essential for the reliable induction of LTP or LTD. However, any such differences in buffering would be present in all our experiments and would always lead to the same gradient in [Ca2+]i, for example, between spines and shafts. Despite such postulated gradients, we find that a prolonged modest photolyzing light reliably induces LTD, while a more intense brief photolysis only induces LTP. Thus the possible existence of such gradients cannot explain the differential responses we find to our two stimulus paradigms.
It is surprising that a brief modest rise in [Ca2+]i can elicit either LTD or LTP, whereas a larger but still brief rise in [Ca2+]i triggers LTP 36% of the time, but never LTD. The larger [Ca2+]i increase appears to actively suppress LTD induction. Similarly, prolonging a modest rise in [Ca2+]i appears to selectively inhibit LTP induction. We explored only a small subset of the two-dimensional space of magnitude and duration of [Ca2+]i elevation. It would be interesting to map out this space more extensively. What are the boundaries delimiting LTP and LTD induction? What effect would a prolonged intense rise in [Ca2+]i have? Limitations of the current methodology prevent addressing the latter question.
Although we often observe LTP or LTD in response to a postsynaptic
[Ca2+]i elevation, we never induced the more
transient short-term potentiation (STP) sometimes observed in response
to briefer or less intense tetanic stimulation or to repeated
postsynaptic depolarization (Colino et al. 1992;
Huang et al. 1992
; Kullmann et al. 1992
; Malenka 1991
; Malenka et al. 1992
).
Equally surprising is that in none of the studies on STD was LTD ever
induced. This apparent discrepancy may be due to the ages of rats used.
The STD studies were all done on slices from 2- to 8-wk-old rats,
whereas our experiments were done on slices from 11- to 22-day-old
rats. LTD is much more readily observed in the younger animals
(Dudek and Bear 1993
), where it may replace STD as the
primary response to a modest rise in [Ca2+]i.
In some ways these results might have been anticipated from
previous findings. For example, electrical induction of LTD of ~13%
results from low-frequency afferent stimulation lasting for 30 s
(Mulkey and Malenka 1992), and 1 min of stimulation
produces depression of ~25%, similar to what we produced (25.8%)
when [Ca2+]i was elevated for ~1 min. LTP
is elicited by tetanic stimulation raising
[Ca2+]i to significantly higher levels
(Otani and Connor 1996
; Petrozzino et al.
1995
), but the [Ca2+]i must remain
elevated for a few seconds (Malenka et al. 1992
). Our
LTP-inducing protocol probably elevates
[Ca2+]i to sufficient levels but for just
barely long enough to induce LTP. There seems to be a minimum rise in
[Ca2+]i that is essential for inducing LTP
reliably, without inducing LTD. For example, pairing low-frequency
afferent stimulation with postsynaptic depolarization results in LTP
rather than LTD (Gustafsson et al. 1987
), presumably
because of the greater elevation in [Ca2+]i
resulting from unblocking NMDA receptors by depolarization. Repetitive
afferent stimulation can elicit LTP or LTD, depending on the phase
relationship between the stimulation and
-burst oscillations
(Huerta and Lisman 1995
); at least part of this phase dependency is related to postsynaptic potential changes that can sensitize or suppress activation of Ca2+ influx through
NMDA receptors. Moreover, a short postsynaptic depolarization alone can
induce LTD (Cummings et al. 1996
); presumably this
treatment does not elevate postsynaptic
[Ca2+]i sufficiently to reliably induce LTP.
Brief afferent tetanic stimulation that normally induces LTP can be
made to induce LTD when postsynaptic depolarization is prevented,
presumably because of reduction in Ca2+ influx
(Cummings et al. 1996
). Thus it is clear that a brief rise in postsynaptic [Ca2+]i can induce
either LTP or LTD and that larger rises are more likely to induce LTP.
In contrast, a prolonged modest [Ca2+]i
elevation selectively induces only LTD.
How might different amplitude and temporal patterns of postsynaptic
[Ca2+]i elevation selectively activate LTD
and LTP? At least two classes of mechanism come to mind. One
possibility is that the target molecules sensing
[Ca2+]i and responsible for inducing LTD and
LTP, thought to be Ca-dependent phosphatases and kinases, respectively
(Bliss and Collingridge 1993; Linden and Conner
1995
), are preferentially activated by different patterns of
[Ca2+]i elevation. Such a
[Ca2+]i pattern sensitivity was reported in
biochemical studies of calcium- and calmodulin-dependent kinase type II
(De Koninck and Schulman 1998
). Another possibility is
that the phosphatase and kinase cascades that underlie LTD and LTP,
respectively, may not only operate linearly to ultimately phosphorylate
or dephosphorylate one or more final targets; rather the two cascades
may interact and inhibit each other at one or more intermediate stages.
Such a scheme of enzyme interactions resembles the multilayered and mutually inhibitory neural circuits involved in pattern recognition (Bishop 1995
). The mechanisms of pattern recognition in
"enzyme circuits" may be similar to those of neural circuits.
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ACKNOWLEDGMENTS |
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We thank Dr. Roger Nicoll for critical discussion. S.-N. Yang and Y.-G. Tang contributed equally to this work.
This work was supported by National Institute of Neurological Disorders and Stroke Grant NS-15114.
Present address of S.-N. Yang: Dept. of Molecular Medicine, Karolinska Institutet, Karolinska Hospital, S-171 76 Stockholm, Sweden.
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FOOTNOTES |
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Address for reprint requests: R. Zucker, Neurobiology Division, 111 Life Sciences Addition, University of California, Berkeley, CA 94720-3200.
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Received 11 May 1998; accepted in final form 7 October 1998.
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