The Contribution of Facilitation of Monosynaptic PSPs to Dishabituation and Sensitization of the Aplysia Siphon Withdrawal Reflex

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The Journal of Neuroscience, December 1, 1999, 19(23):10438-10450

The Contribution of Facilitation of Monosynaptic PSPs to Dishabituation and Sensitization of the Aplysia Siphon Withdrawal Reflex
Igor Antonov¹, Eric R. Kandel¹^,²^,³, and Robert D. Hawkins¹^,²
¹ Center for Neurobiology and Behavior, College of Physicians and Surgeons, Columbia University, New York, New York 10032, and ² New York State Psychiatric Institute and ³ Howard Hughes Medical Institute, New York, New York 10032

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

To examine the relationship between synaptic plasticity and learning and memory as directly as possible, we have developeda new simplified preparation for studying the siphon-withdrawalreflex of Aplysia in which it is relatively easy to record synapticconnections between individual identified neurons during simpleforms of learning. We estimated that monosynaptic EPSPs from LEsiphon sensory neurons to LFS siphon motor neurons mediate approximatelyone-third of the reflex response measured in this preparation,which corresponds to siphon flaring in the intact animal. To investigatecellular mechanisms contributing to dishabituation and sensitization,we recorded evoked firing of LFS neurons, the siphon withdrawalproduced by stimulation of an LFS neuron, the complex PSP in anLFS neuron, and the monosynaptic PSP from an "on-field" or "off-field"LE neuron to an LFS neuron during behavioral training. Unlikethe simplified gill-withdrawal preparation (Cohen et al., 1997;Frost et al., 1997), in the siphon-withdrawal preparation we foundno qualitative differences between the major cellular mechanismscontributing to dishabituation and sensitization, suggesting thatdissociations that have been observed previously may be attributableto transient inhibition that does not occur for this componentof the reflex. Furthermore, in the siphon-withdrawal preparation,all of the various cellular measures, including monosynaptic PSPsfrom either on-field or off-field LE neurons, changed approximatelyin parallel with changes in the behavior. These results providethe most direct evidence so far available that both dishabituationand sensitization involve multiple mechanisms, including heterosynapticfacilitation of sensory neuron-motor neuronPSPs.

Key words: facilitation; PSP; dishabituation; sensitization; Aplysia; learning

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Many theories of learning have proposed that plasticity at specific synapses in the CNS is critical for memory storage, anda number of mechanisms of synaptic plasticity have been identifiedthat might contribute to learning and memory (Hawkins et al.,1987; Ito, 1989; Antonov et al., 1991; Bliss and Collingridge,1993; Linden and Connor, 1995). However, in most cases it hasbeen very difficult to test the causal relationship between thesemechanisms and learning. The gill- and siphon-withdrawal reflexof Aplysia is advantageous for such an analysis, and previousstudies have suggested that several simple forms of learning ofthe reflex are caused in part by plasticity at synapses of thesiphon sensory neurons (for review, see Hawkins et al., 1993).However, even in this simple system it has proven surprisinglydifficult to demonstrate a direct relationship between the synapticplasticity and learning. Most previous studies of the reflex haveinvolved behavioral experiments in the intact animal and eithercellular analogs or correlates in the isolated nervous system,which are only indirectly related to the behavior. A few studieshave attempted to bridge the cellular and behavioral levels moredirectly by examining the sensory neuron synapses and behaviorin the same preparation (Byrne et al., 1978; Lukowiak, 1986; Wrightet al., 1991). However, from these and other studies (Jackletand Rine, 1977; Kanz et al., 1979; Hawkins et al., 1981; Colebrookand Lukowiak, 1988; Frost et al., 1988; Trudeau and Castellucci,1993), it has become clear that plasticity of the behavior isdetermined by multiple mechanisms of cellular plasticity at anumber of loci, so that any one mechanism may not correlate wellwith the behavior. Furthermore, the contribution of each mechanismappears to depend on the particular experimental procedures suchas the stimuli used and the response measured, making comparisonsbetween studies with different procedures problematic (Hawkinset al., 1998a).

For these reasons, it seemed desirable to be able to study cellular mechanisms and learning simultaneously in as simple abehavioral system as possible. Toward that end, we have developeda new preparation with which it is relatively easy to measurereflex contraction of the siphon while simultaneously recordingfrom one or more neurons in the ganglion with intracellular electrodesand thus to relate the cellular events to behavior. This preparationexhibits several simple forms of learning with properties generallysimilar to learning in the intact animal (Carew et al., 1981;Hawkins et al., 1998a). The reflex response is mediated in partby monosynaptic connections from the LE sensory neurons to LFSmotor neurons, which exhibit several types of plasticity, includinganalogs of these forms of learning (Hawkins et al., 1983; Mackeyet al., 1987; Wright et al., 1991). We have now been able to usethis preparation to provide the first direct evidence that heterosynapticfacilitation of the monosynaptic PSPs contributes to learningand memory for dishabituation and sensitization of the withdrawalreflex and to show that other sites and mechanisms of plasticityalsocontribute.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aplysia californica weighing 100-150 gm were obtained from Marinus (Long Beach, CA). They were housed in individual containersin a large aquarium with circulating artificial seawater (InstantOcean, Aquarium Systems, Mentor, OH) at 15°C on a 12 hr light/darkcycle and food-deprived for several days before an experimentwas begun to try to minimize variability in their motivationalstate. The animals were anesthetized by injection of 50 ml ofisotonic MgCl₂, and the siphon, tail, and CNS were dissected outin 50% MgCl₂, 50% artificial seawater. The siphon was cut partiallyin half along the longitudinal axis, and the abdominal ganglionwas dipped in 0.5% glutaraldehyde for 60 sec to kill muscle cellsin the sheath. The preparation was then pinned to the Sylgardfloor of a Lucite recording chamber filled with circulating, aeratedartificial seawater at room temperature (see Fig. 1A). One-halfof the cut part of the siphon was not pinned. Seawater was injectedinto the tail and siphon to flush out the MgCl₂, and the abdominalganglion was partiallydesheathed.

An LE siphon mechanosensory neuron, identified by its electrophysiological properties and response to siphon stimulation (Byrneet al., 1974), was impaled with a single-barreled glass microelectrodefilled with 2.5 M KCl, and an LFS_B siphon motor neuron, identifiedby its electrophysiological properties and siphon movement (Frostet al., 1988), was impaled with a double-barreled microelectrode.In some experiments, current was passed through one barrel ofthe electrode either to hyperpolarize the motor neuron ~30 mVbelow resting potential and prevent spiking during the siphonstimulation or to depolarize the neuron and cause spiking. Mechanicalstimulation (taps) was delivered to the pinned half of the siphonwith a controlled force stimulator identical to the one used byCohen et al. (1997). The tip of the stimulator was a 1.5-mm-diameterstainless steel rod, tap duration was 500 msec, and tap pressurewas usually ~20 gm/mm² [calibrated against a strain gauge transducer (Grass Instruments,Quincy, MA)], which is considered to be relatively innocuous (Waltersand Cohen, 1997). Withdrawal of the other half of the siphon,which was not pinned, was recorded with a low mass isotonic transducer(Harvard Apparatus, South Natick, MA) connected to the siphonwith a silk suture. The component of contraction that was measuredwith this recording system would probably contribute to backwardbending or "flaring" of the siphon in the intact animal. Duringdishabituation and sensitization training, the tail was stimulatedwith a train of four 60 Hz AC electrical shocks [1.0 sec duration,2 sec interstimulus interval (ISI), 25 mA] delivered via fixedcapillary electrodes. Preparations were considered unhealthy andexcluded from the results if the shock produced a siphon withdrawalof <3 mm, which occurred in ~25% of dishabituation and sensitizationexperiments.

The preparation was rested for at least 1 hr before the beginning of dishabituation or sensitization training (see Fig. 1B).During habituation and dishabituation, the siphon was stimulatedeight times with a 5 min intertrial interval, and habituationwas measured as the decrease in responding on trial 5 comparedwith trial 1. The tail was then shocked 2.5 min after trial 5,and dishabituation was measured as the increase in respondingon trials 6, 7, and 8 compared with trial 5. During sensitization,there was a single siphon stimulation (trial 1) followed by 1hr rest to minimize habituation. The tail was then shocked, andthe siphon was stimulated again for 2.5 min (trial 2), 7.5 min(trial 3), and 12.5 min (trial 4) after the shock. Sensitizationwas measured as the increase in responding on trials 2, 3, and4, compared with trial 1. During both dishabituation and sensitization,experiments were continued only if the siphon withdrawal on trial1 was between 0.5 and 3 mm (the maximal withdrawal was usually~6 mm). On each trial, we measured the siphon withdrawal, thespikes in the LE siphon sensory neuron, and the spikes or complexPSP in the LFS siphon motor neuron in response to the siphon stimulation.In some experiments, we also fired an action potential in theLE neuron with intracellular current injection through a bridge-balancecircuit and measured the monosynaptic PSP produced in the motorneuron. The amplitudes and areas of the PSPs were measured usinga laboratory interface to a microcomputer and commercially availablesoftware (Hilal Associates, Englewood, NJ). The data on dishabituationand sensitization were analyzed with one, two, or three-way ANOVAwith one repeated measure (trial), followed by planned comparisonsof the experimental group to the appropriate pre-shock and no-shockcontrols on eachtrial.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Contribution of the CNS to the reflex

The siphon-elicited siphon withdrawal reflex is mediated in part by central motor neurons in the abdominal ganglion and inpart by peripheral motor neurons in the siphon itself (Perlman,1979). Both types of motor neurons receive monosynaptic inputfrom the LE siphon sensory neurons (Bailey et al., 1979). To estimatethe relative contributions of the central and peripheral componentsof the reflex, we compared the reflex response before and aftercutting the siphon nerve, which connects the siphon to the abdominalganglion (Fig. 1A). To measure the baseline level we first recordedthe response during five trials of siphon stimulation, which producedapproximately equal habituation in two groups of preparations(Fig. 2). We then cut the siphon nerve in one group, waited 1hr for recovery, and gave five more trials of siphon stimulation.In the control (uncut) group, the siphon reflex recovered completelyon trial 6 after the 1 hr rest (107.6 ± 13.4% of trial 1, n =9). By contrast, in the experimental (cut) group, the amplitudeof the response on trial 6 was only ~45% of the response on trial1 (44.1 ± 9.3%, n = 11). We obtained similar results when we comparedthe average responses on trials 6-10 with trials 1-5 (control,96.7 ± 8.3%; cut, 47.9 ± 8.2%). These results indicate that ~55%of the reflex is mediated through the CNS, which agrees very wellwith the estimate of 55% by Perlman (1979). When we looked atthe area (instead of the amplitude) of the response, the withdrawalon trial 6 was slightly smaller in the cut group (31.9 ± 4.7%of trial 1), suggesting that the CNS may contribute to the durationas well as the amplitude of the reflex.

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Figure 1. Experimental preparation (A) and behavioral protocols (B). See Materials and Methods for details.

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Figure 2. Contribution of the CNS to the siphon withdrawal reflex. A, Records from representative experiments showing the siphon-withdrawal reflex (SWR) in response to a siphon tap (TAP) on trials 1 and 6 in a control preparation (A₁) and a preparation in which the siphon nerve was cut between trials 5 and 6 (A₂). B, Average amplitude of siphon withdrawal in two groups of preparations, both of which received five trials of siphon stimulation with a 5 min interstimulus interval, a 1 hr rest, and then five more trials of siphon stimulation. The siphon nerve was cut immediately after trial 5 in one group (Cut). The average area of siphon withdrawal (measured during the first 1 sec after the start of the withdrawal) is also shown for trial 6 (bars). The points show the means, and the error bars show the SEM. The data have been normalized to the value on trial 1 for each preparation [average amplitude on trial 1 = 1.8 ± 0.4 mm (Control) and 2.0 ± 0.3 mm (Cut), average area = 2295 ± 559 mm × msec (Control) and 2049 ± 367 mm × msec (Cut), not significantly different).

Contribution of LFS_B siphon motor neurons to the reflex

The central component of the siphon withdrawal reflex is mediated by five types of identified motor neurons in the abdominalganglion (LFS_A, LFS_B, LBS, LDS, and RDS), each of which producesa different type of siphon movement (Perlman 1979; Frost et al.,1988; Frost and Kandel, 1995; Hickie and Walters, 1995). At thebeginning of each experiment, we searched for a motor neuron which,when fired with intracellular current injection, produced movementof the siphon that was measurable with our recording system. Thesewere predominantly LFS_B motor neurons, which receive strong excitatoryinput from tail stimulation and produce backward bending or "flaring"of the siphon in intact animals. By contrast, intracellular stimulationof either LFS_A or LBS motor neurons produced only a very weakresponse with our recordingsystem.

We estimated the contribution of a single motor neuron to the reflex response in our preparation in two ways. First, we measuredthe response alternately with and without that neuron hyperpolarizedby intracellular current injection, which prevents spiking andeffectively removes the neuron from the circuit (Fig. 3). In afew experiments in which we recorded from two LFS_B neurons simultaneously,we did not detect any evidence of electrical coupling betweenthem. In two series of experiments with interstimulus intervalsof either 1 or 20 min, hyperpolarizing a single LFS_B motor neuronreduced the reflex response ~25 or 30% ( $-$ 25.1 ± 3.4%, n = 6, witha 1 min ISI; $-$ 32.5 ± 5.9%, n = 4, with a 20 min ISI).

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Figure 3. Contribution of a single LFS_B siphon motor neuron to the siphon withdrawal reflex. A, Records from a representative experiment showing the siphon withdrawal in response to a siphon tap with an LFS_B neuron alternately at resting potential (Control) or hyperpolarized to prevent it from spiking. B, Average amplitude of siphon withdrawal in two groups with interstimulus intervals of either 1 min (B₁) or 20 min (B₂). The bars in B₁ show the average withdrawal on the last five trials with the neuron either at resting potential or hyperpolarized. The average values on trial 1 (Control) were 2.9 ± 0.4 mm (B₁) and 3.2 ± 0.9 mm (B₂).

As a second method of estimating the contribution of a single LFS_B neuron to the reflex response, we compared the responseproduced by intracellular stimulation of the motor neuron withthe response produced by mechanical stimulation of the siphon(Fig. 4). There was a significant correlation between the frequencyof firing of the motor neuron and the amplitude of the evokedcontraction with either intracellular stimulation (r = 0.93, n= 25, p < 0.01) or siphon stimulation (r = 0.96, n = 17, p < 0.01).When intracellular current was used to fire the motor neuron inthe physiological range (10-20 Hz), the siphon withdrawal producedwas 24.3% of the withdrawal produced by siphon stimulation. Thisestimate agrees well with the estimate obtained by hyperpolarizingthe motor neuron (Fig. 3) and suggests that a single LFS_B motorneuron contributes ~25% of the reflex response, which agrees fairlywell with the estimate of 18% by Frost and Kandel (1995). Becausethe entire CNS was estimated to contribute ~55% of the reflexresponse (Fig. 2), these results suggest that only two or perhapsthree motor neurons mediate most of the central component of thereflex measured with our recording system. This is slightly surprisingbecause there are thought to be four LFS_B neurons (Frost et al.,1988; Frost and Kandel, 1995; Hickie and Walters, 1995). However,even the four LFS_B neurons produce somewhat different siphon movements(Hickie and Walters, 1995), not all of which may be measured equallywith our recording system.

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Figure 4. Comparison of siphon withdrawal produced by intracellular stimulation of a single LFS_B siphon motor neuron and by a siphon tap. A, Records from a representative experiment showing the siphon withdrawal produced by intracellular current injection in an LFS_B neuron (left) and a siphon tap (right). In both cases the LFS_B neuron fired 19 spikes during the first 1 sec after the start of firing. B, Group data from experiments like the one shown in A. B₁, Scatterplot of the amplitude of siphon withdrawal and the frequency of LFS firing in the first 1 sec on trial 1 in 17 experiments with siphon taps ( $open circle$ ) and on 25 trials in seven experiments with intracellular stimulation of an LFS_B neuron (). The lines indicate the linear regressions. B₂, The average amplitude of siphon withdrawal produced by LFS_B firing in the physiological range (10-20 Hz) in the two groups shown in B₁.

Firing of LFS motor neurons and LE sensory neurons during habituation, dishabituation, and sensitization

We next began an analysis of habituation, dishabituation, and sensitization of the reflex. As shown in the example in Figure5 and the average results in Figure 6A, there was significantbehavioral habituation of siphon withdrawal on trial 5, comparedwith trial 1, in two independent groups (F_(1,20) = 133.27, p <0.01). One group (n = 17), which received tail shock 2.5 min aftertrial 5, showed significant dishabituation on trial 6, 2.5 minafter the shock (F_(1,40) = 65.04, p < 0.01), and on trial 7, 7.5min after the shock (F_(1,40) = 16.65, p < 0.01) compared withtrial 5. The shocked group also showed significant dishabituationcompared with a no-shock control group (n = 5) on trials 6 and7 (p < 0.05 in each case). Similarly, another group that was notfirst habituated (n = 14) showed significant sensitization ontrial 2, 2.5 min after the shock, compared with trial 1 (F_(1,32)= 23.79, p < 0.01). That group also showed significant sensitizationcompared with a no-shock control group (n = 4) on trial 2 (p <0.05). For both dishabituation and sensitization, the effectswere largest 2.5 min after the shock and had partially declinedby 12.5 min after the shock. There was no significant differencebetween the amplitudes or time courses of dishabituation and sensitization(F_(1,36) = 0.01 for the interaction of group and shock).

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Figure 5. Records from representative experiments showing the siphon withdrawal and the firing of an LFS_B siphon motor neuron and an LE siphon sensory neuron in response to siphon stimulation during habituation, dishabituation, and sensitization (see Fig. 1B for the behavioral protocols).

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Figure 6. The average siphon withdrawal and firing of LFS_B motor neurons and LE sensory neurons during habituation (HAB) and dishabituation (DIS) in experiments like the one shown in Figure 5A and during sensitization (SEN) in experiments like the one shown in Figure 5B. A, The average amplitude of siphon withdrawal in response to siphon stimulation in the group receiving tail shock () and in a no-shock control group ( $open circle$ ). *p < 0.05, **p < 0.01 compared with trial 1 for habituation and sensitization, and compared with trial 5 for dishabituation. The average values on trial 1 were 2.1 ± 0.2 mm (DIS, Shock), 2.4 ± 0.3 mm (DIS, No shock), 2.3 ± 0.3 mm (SEN, Shock), and 2.1 ± 0.2 mm (SEN, No shock); not significantly different. B, The average frequency of firing of LFS_B neurons during the first 1 sec after the start of firing measured simultaneously with the siphon withdrawals shown in A. The average values on trial 1 were 15.8 ± 0.9 Hz (DIS, Shock), 15.8 ± 1.2 Hz (DIS, No shock), 15.6 ± 0.9 Hz (SEN, Shock), and 15.0 ± 1.1 Hz (SEN, No shock); not significantly different. C, The average frequency of firing of LE neurons during the first 1 sec after the start of firing () and the average spontaneous firing of LFS neurons during the 5 sec before each siphon stimulation. The average values on trial 1 were 3.5 ± 0.7 Hz (LE, DIS), 3.1 ± 0.6 Hz (LE, SEN), 1.2 ± 0.1 Hz (LFS, DIS), and 1.0 ± 0.1 Hz (LFS, SEN).

In these experiments we recorded the firing of an LFS motor neuron and in most cases also an LE sensory neuron simultaneouslywith the siphon withdrawal. Figure 5 shows examples of the neuronalactivity, and Figure 6B shows the average evoked firing duringthe first 1 sec after the start of the response to siphon stimulation,which included the peak of the siphon withdrawal on most trials(the average time-to-peak of siphon withdrawal was 731 ± 23 msecoverall and did not change by >170 msec during habituation, dishabituation,or sensitization). There was a significant decrease in evokedfiring of the motor neuron on trial 5, compared with trial 1,in both habituation groups (F_(1,20) = 289.92, p < 0.01), whichcorrelated significantly with the decrease in siphon withdrawal(r = 0.35, p < 0.05, one-tail comparing the decreases in LFS spikesand siphon withdrawal). This correlation was more modest thanin similar studies on other preparations (Cohen et al., 1997),perhaps because a single central motor neuron contributes only~25% of the siphon withdrawal response. During dishabituation,there was a significant increase in evoked firing of the motorneuron on trials 6, 7, and 8, compared with trial 5 (p < 0.01in each case), which correlated significantly with the increasein siphon withdrawal on each trial (r = 0.45, p < 0.05 on trial6). The dishabituation group also showed a significant increasein evoked firing of the motor neuron compared with the no-shockcontrol group on each trial after the shock (p < 0.05 in eachcase). Similarly, during sensitization, there was a significantincrease in evoked firing of the motor neuron on trial 2, comparedwith trial 1 (F_(1,32) = 25.66, p < 0.01), which correlated significantlywith the increase in siphon withdrawal (r = 0.45, p < 0.05, one-tail).The sensitization group also showed a significant increase inevoked firing of the motor neuron compared with the no-shock controlgroup on trials 2 and 3 (p < 0.05 in each case). For both dishabituationand sensitization, the increases in evoked firing of the motorneuron were largest 2.5 min after the shock and had partiallydeclined by 12.5 min after the shock. There was no significantdifference between the amplitudes or time courses of the increasesduring dishabituation and sensitization (F_(1,36) = 0.03 for theinteraction of group andshock).

When the siphon tap was within the receptive field of an LE sensory neuron ("on-field"), it always caused the LE neuron tofire action potentials. Unlike the LFS motor neurons, evoked firingof the LE sensory neurons did not change significantly duringhabituation, dishabituation (n = 10), or sensitization (n = 9),although there were small and nonsignificant trends for a decreasein firing of the LE neurons during habituation and an increaseduring dishabituation and sensitization (Fig. 6C, and see Fig.15). Sensitizing stimuli have been shown to produce a much largerincrease in evoked firing of the Aplysia tail sensory neurons(Walters et al., 1983), and repeated sensitizing stimuli can alsoproduce a larger increase in firing of the LE neurons (our unpublishedobservations).

These results suggest that habituation, dishabituation, and sensitization of siphon withdrawal are attributable at least inpart to changes in evoked firing of the LFS motor neurons. Thesechanges cannot be explained by alterations in firing of the LEsensory neurons, and therefore could involve changes in synaptictransmission in the CNS. Moreover, during habituation, the percentagechange in siphon withdrawal was approximately the same as thepercentage change in evoked firing of LFS motor neurons, but duringdishabituation and sensitization the percentage change in siphonwithdrawal was larger than the change in evoked firing of themotor neurons (see Fig. 15). These results suggest that additionalmechanisms may also contribute to dishabituation andsensitization.

One possible additional mechanism is a change in the pattern of firing of the LFS motor neurons, such that the same numberof spikes produced greater siphon withdrawal. As shown in theexamples in Figure 5 and the average results in Figure 7, theevoked firing of LFS motor neurons on each trial tended to followa reproducible pattern with four components that have previouslybeen described for the gill motor neuron LDG1 (Cohen et al., 1997):an initial high-frequency burst, a sustained response during thetap, a smaller second burst around the offset of the tap, anda gradual decline in firing after the tap. The pattern of firingof the LE sensory neurons was also similar to that described previously(Byrne et al., 1974; Frost et al., 1997) and matched the firsttwo components of the pattern of firing of the LFS neurons: aninitial high-frequency burst and a sustained response during thetap, but little firing after the tap. These results suggest thatthe LE neurons contribute directly to firing of the LFS neuronsduring the tap but contribute only indirectly to LFS firing afterthe tap.

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Figure 7. The average pattern of firing of LFS motor neurons and LE sensory neurons during habituation, dishabituation, and sensitization of siphon withdrawal in the same experiments as Figure 6. A, Firing of LFS (A₁) and LE (A₂) neurons during habituation and dishabituation. B, Firing of LFS (B₁) and LE (B₂) neurons during sensitization. On each trial, the number of spikes in each 100 msec interval has been normalized to the total number of spikes on trial 1 in each experiment (average on trial 1 = 18.2 ± 0.9 in A₁, 3.5 ± 0.7 in A₂, 18.4 ± 1.2 in B₁, and 3.1 ± 0.6 in B₂). The horizontal bar below the x-axis indicates the duration of the siphon tap.

There was no significant change in the pattern of firing of the LE neurons during habituation, dishabituation, or sensitization.There was a small but significant change in the pattern of firingof the LFS neurons during habituation (F_(14,224) = 2.04, p < 0.05for the effect of bin), with the biggest decreases in firing occurringnear the onset of the tap (in the first three bins or 150 msec).However, there was no significant change in the pattern of firingof the LFS neurons during dishabituation or sensitization thatcould contribute to changes in siphon withdrawal during thoseforms oflearning.

Another possible mechanism that could contribute to enhanced siphon withdrawal during dishabituation and sensitization isperipheral enhancement, perhaps attributable to post-tetanic potentiation(PTP) at the neuromuscular junction. Frost et al. (1988) providedevidence that PTP at the neuromuscular junction of LFS neuronscontributed to sensitization of the siphon-withdrawal reflex insimilar experiments. Consistent with that possibility, there werechanges in spontaneous as well as evoked firing of LFS neuronsduring dishabituation and sensitization in our experiments (Fig.6C). During dishabituation, there was a significant increase inspontaneous firing measured just before trial 6, 2.5 min afterthe shock (F_(1,32) = 50.85, p < 0.01), and trial 7, 7.5 min afterthe shock (F_(1,32) = 5.31, p < 0.05). Similarly, during sensitization,there was a significant increase in spontaneous firing on trial2, 2.5 min after the shock (F_(1,26) = 53.20, p < 0.01), and trial3, 7.5 min after the shock (F_(1,26) = 4.89, p < 0.05). These changesin spontaneous firing might give rise to peripheral enhancement2.5 and 7.5 min after theshock.

Peripheral enhancement contributes to dishabituation and sensitization

We tested peripheral enhancement by measuring the siphon withdrawal produced by intracellular stimulation of an LFS neuronwith a dishabituation design (Fig. 8). There was no significantchange in the siphon withdrawal produced by LFS stimulation ontrial 5 compared with trail 1, indicating that peripheral depressionor fatigue make little contribution to habituation. By contrast,there was a modest (~10%) but significant increase in siphon withdrawalon trial 6, 2.5 min after the shock (F_(1,12) = 15.22, p < 0.01),that had worn off by trial 7, 7.5 min after the shock. These resultssuggest that peripheral enhancement makes some contribution todishabituation and sensitization 2.5 min after the shock, in agreementwith previous studies on other preparations (Jacklet and Rine,1977; Cohen et al., 1997).

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Figure 8. Siphon withdrawal produced by intracellular stimulation of an LFS_B neuron before and after tail shock. A, Records from a representative experiment showing the siphon withdrawal produced by firing an LFS_B neuron with intracellular current injection. The LFS_B neuron was stimulated on eight trials with an intertrial interval of 5 min, and the tail was shocked 2.5 min before trial 6. B, Average amplitude of siphon withdrawal () and LFS spike frequency ( $open circle$ ) in experiments like the one shown in A. The average values on trial 1 were 1.5 ± 0.3 mm (SWR) and 24.0 ± 2.1 mm (LFS spikes).

As shown in Figure 8, there was no significant change in the number of spikes produced in the LFS neuron by constant currentinjection. This result indicates that the excitability of theLFS neuron remained relatively constant after the tail shock,and therefore that changes in the number of spikes produced bysiphon stimulation during dishabituation and sensitization (Figs.5, 6B) were attributable to changes in synaptic input to the motorneuron.

Plasticity of the complex PSP in an LFS neuron during habituation, dishabituation, and sensitization

We directly tested the possibility that habituation, dishabituation, and sensitization involve changes in the synaptic inputto LFS motor neurons by hyperpolarizing the motor neuron duringthe siphon tap, preventing it from firing, and allowing measurementof the underlying complex PSP. In these experiments, we also measuredthe remaining siphon withdrawal with the LFS motor neuron hyperpolarizedand found that although the overall amplitude of the reflex wasreduced, its plasticity during habituation, dishabituation, andsensitization was normal (Figs. 9, 10A). This result suggests thatfiring of the remaining motor neurons underwent plasticity similarto that of the neuron that was hyperpolarized.

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Figure 9. Records from representative experiments showing the complex PSP produced in an LFS_B neuron by siphon stimulation during habituation, dishabituation (A), and sensitization (B). The LFS neuron was hyperpolarized to keep it from firing during each siphon tap.

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Figure 10. The average siphon withdrawal and area of the complex PSP in an LFS_B neuron during habituation, dishabituation, and sensitization in experiments like the ones shown in Figure 9. A, The amplitude of siphon withdrawal in response to siphon stimulation in experiments in which an LFS_B motor neuron was hyperpolarized and therefore did not contribute to the withdrawal response. The average values on trial 1 were 1.7 ± 0.2 mm (DIS, Shock), 1.1 ± 0.3 mm (DIS, No shock), 1.6 ± 0.2 mm (SEN, Shock), and 1.0 ± 0.2 mm (SEN, No shock). B, The average area of the complex PSP in the hyperpolarized LFS_B neuron measured simultaneously with the siphon withdrawals shown in A. PSP area was measured during the first 1 sec after the start of the PSP and normalized to the area on trial 1 in each experiment (average on trial 1 = 38,217 ± 3835 mV × msec for DIS, Shock, 41,904 ± 5389 mV × msec for DIS, No shock, 40,171 ± 4125 mV × msec for SEN, Shock, and 48,330 ± 5430 mV × msec for SEN, No shock, not significantly different).

As shown in the examples in Figure 9 and the average results in Figure 11, the complex PSP in an LFS neuron had a complicatedshape with the same four components that were described previouslyfor evoked spikes: an initial peak near the onset of the tap,a smaller sustained depolarization during the tap, a second peakaround the offset of the tap, and a gradual decline after thetap. We therefore measured the total area under the PSP in thefirst 1 sec rather than simply measuring peak amplitude (Fig.10B). During habituation, there was a significant decrease in thearea of the PSP on trial 5, compared with trial 1, in two independentgroups (F_(1,14) = 78.91, p < 0.01). During dishabituation, therewas a significant increase in the area of the PSP on each trialafter the shock (6, 7, and 8) compared with either trial 5 orthe no-shock control group (p < 0.01 in each case). Similarly,during sensitization there was a significant increase in the areaof the PSP on the first two trials after the shock (2 and 3) comparedwith either trial 1 or a no-shock control group (p < 0.01 in eachcase). For both dishabituation and sensitization, the increasesin the area of the complex PSP were largest 2.5 min after theshock and had partially declined by 12.5 min after the shock.There was no significant difference between the amplitudes ortime courses of the increases during dishabituation and sensitization(F_(1,27) = 1.28 for the interaction of group and shock).

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Figure 11. The average shape of the complex PSP in an LFS_B neuron during habituation and dishabituation (A) and sensitization (B) in the same experiments as Figure 10. The PSP in each 50 msec interval has been normalized to the total area on trial 1 in each experiment (average on trial 1 = 49,627 ± 5371 mV × msec in A and 49,844 ± 5206 mV × msec in B).

These results are very similar to results on evoked firing of the motor neuron (Fig. 6B) and suggest that changes in the complexPSP can largely account for changes in evoked firing. However,there were some more subtle differences between evoked firingand the complex PSP, and also between dishabituation and sensitization,when we examined changes in the shape of the response (Fig. 11).Unlike evoked firing (Fig. 7), there was no significant changein the shape of the complex PSP during habituation. There wasalso no significant change during dishabituation. However, therewas a small but significant change in the shape of the complexPSP during sensitization (F_(29,261) = 2.31, p < 0.01 for the effectof bin), with the biggest increase in the amplitude of the PSPoccurring around the offset of the tap (in bins 7-12, during theend of the sustained depolarization during the tap and the beginningof the second peak after the offset of the tap). Moreover, thechange in the shape of the complex PSP was significantly differentduring sensitization than during dishabituation (F_(29,551) = 2.01,p < 0.01 for the interaction of group andbin).

Contribution of monosynaptic PSPs from LE sensory neurons to the complex PSP in LFS motor neurons

The complex PSP in an LFS motor neuron includes a direct contribution from sensory neurons and an indirect contribution viainterneurons, several of which have been identified (Frost andKandel, 1995). To estimate the direct contribution of LE sensoryneurons, we compared the monosynaptic PSP produced in a motorneuron by intracellular stimulation of an LE sensory neuron andthe complex PSP produced by mechanical stimulation of the siphon,measured ~10 sec apart under identical conditions (Fig. 12). Onaverage, the amplitude of the monosynaptic PSP produced by a singlespike in an LE cell was 29.1 ± 2.4% of the amplitude of the complexPSP, and the area of the monosynaptic PSP was 3.6 ± 0.2% of thearea of the complex PSP (n = 21). When the tap was within thereceptive field of the LE cell, it fired on average 3.3 ± 0.5spikes during the tap (n = 19). Taps of this strength are thoughtto activate approximately five LE cells (Byrne et al., 1974; Hickieet al., 1997). Multiplying these numbers suggests that monosynapticPSPs from the LE cells would contribute ~60% of the area of thecomplex PSP if they added linearly. Previous estimates of theaverage monosynaptic contribution based on different methods haveranged from 5% (Hickie et al., 1997), ~25% (Trudeau and Castellucci,1992; Cohen et al., 1997), to >50% (Byrne et al., 1978; Frostet al., 1997). Some of the differences in results may be explainedby differences in the siphon stimulation, because very weak, briefstimuli are able to elicit a withdrawal reflex without activatingthe LE cells at all, presumably by activating an as yet unidentifiedclass of sensory neurons with a lower threshold but otherwisesimilar properties (Frost et al., 1997).

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Figure 12. Direct contribution of monosynaptic PSPs from LE neurons to the complex PSP in LFS_B neurons. A, Examples of the monosynaptic PSP produced in an LFS_B neuron by intracellular stimulation of an LE neuron and the complex PSP produced by a siphon tap, measured ~10 sec apart under identical conditions. B, The average amplitude (left) and area (right) of the monosynaptic and complex PSPs in experiments like the one shown in A. The area of the complex PSP was measured in the interval indicated by the dotted lines in A, which is when LE neurons fire and contribute directly to the complex PSP (see Fig. 7).

Plasticity of the monosynaptic PSPs from LE neurons during habituation, dishabituation, and sensitization

To examine plasticity of the monosynaptic PSPs, we tested the PSP from an LE neuron to the motor neuron 10 sec before thefirst and fifth trials of habituation training, and before trials6, 7, and 8 of dishabituation and trials 1-4 of sensitization.As shown in the examples in Figure 13 and the average results inFigure 14, when the siphon tap was within the receptive field ofan LE cell and caused it to fire action potentials (on-field),the amplitude of the monosynaptic PSP from that LE cell underwentsignificant depression during habituation training in two independentgroups ( $-$ 39.5 ± 4.4%, n = 15; F_(1,21) = 78.43, p < 0.01 comparedwith trial 1). By contrast, when the siphon tap was outside thereceptive field of an LE cell and did not cause it to fire (off-field),the monosynaptic PSP did not undergo depression ( $-$ 3.6 ± 5.6%,n = 5; F_(1,21) = 24.34, p < 0.01 compared with on-field). Resultswere similar when we measured the area of the monosynaptic PSP[which is more directly comparable to the area of the complexPSP (Fig. 15)] instead of its amplitude [which can be measuredmore accurately when the PSP includes a late polysynaptic component(Fig. 13B)]. These results are similar to the results of previousstudies (Frost et al., 1997) and are consistent with the ideathat habituation involves homosynaptic depression of sensory neuronPSPs attributable to firing of the sensory neurons during thesiphon stimulation (Castellucci et al., 1970; Kupfermann et al.,1970; Byrne et al., 1978). Depression of the monosynaptic PSPswas of sufficient amplitude and duration to account for most orall of the behavioral habituation in these experiments, althoughother mechanisms may also contribute under some circumstances(Goldberg and Lukowiak, 1984; Stopfer and Carew, 1996; Frost etal., 1997).

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Figure 13. Records from representative experiments showing the monosynaptic PSP produced in an LFS_B neuron by intracellular stimulation of an on-field or off-field LE neuron ~10 sec before the siphon tap on trials 1 and 5 during habituation and trials 6-8 during dishabituation (A), and before each trial during sensitization (B).

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Figure 14. Average amplitude (left) and area (right) of the monosynaptic PSP produced in an LFS_B neuron by intracellular stimulation of an on-field or off-field LE neuron during habituation and dishabituation (A) and sensitization (B). The average values on trial 1 were 12.0 ± 1.5 mV and 659 ± 104 mV × msec (Dishabituation, on-field), 12.0 ± 1.9 mV and 824 ± 155 mV × msec (Dishabituation, off-field), 9.8 ± 2.0 mV and 629 ± 144 mV × msec (Dishabituation, no shock control), 9.0 ± 1.1 mV and 703 ± 114 mV × msec (Sensitization, on-field), 10.9 ± 1.4 mV and 880 ± 115 mV × msec (Sensitization, off-field), 13.9 ± 3.5 mV and 874 ± 247 mV × msec (Sensitization, control); not significantly different.

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Figure 15. Summary of habituation, dishabituation, and sensitization of the siphon withdrawal reflex at different levels of analysis. For comparative purposes, all responses are expressed as percentage of trial 1 (T1).

We then went on to conduct similar studies of dishabituation and sensitization. During dishabituation training, there wassignificant facilitation of monosynaptic PSPs from on-field sensoryneurons on the first trial after the shock (trial 6) comparedwith either trial 5 (F_(1,42) = 64.04, p < 0.01) or a no-shockcontrol group (F_(1,42) = 26.70, p < 0.01). Unlike habituationtraining, during which depression was restricted to PSPs fromon-field sensory neurons, during dishabituation training therewas also significant facilitation of monosynaptic PSPs from off-fieldsensory neurons on trial 6, compared with trial 5 (F_(1,42) = 20.66,p < 0.01). Similarly, during sensitization training there wassignificant facilitation of monosynaptic PSPs from either on-fieldor off-field sensory neurons on the first trial after the shock(trial 2) compared with either trial 1 (p < 0.01 in each case)or a no-shock control group (p < 0.05). During both dishabituationand sensitization training, facilitation of the monosynaptic PSPwas largest 2.5 min after the shock and had partially declinedby 12.5 min after the shock. There was no significant differencebetween the amplitudes or time courses of facilitation of on-fieldPSPs during dishabituation and sensitization (F_(1,24) = 0.76 forthe interaction of group and shock). These results are consistentwith the idea that dishabituation and sensitization involve heterosynapticfacilitation of sensory neuron PSPs attributable to firing offacilitator interneurons during the tail shock (Castellucci etal., 1970; Kupfermann et al., 1970; Walters et al., 1983; Mackeyet al., 1989; Wright et al., 1991; Trudeau and Castellucci, 1993).Moreover, the observation that facilitation of the monosynapticPSPs was approximately the same during dishabituation as duringsensitization suggests that dishabituation involves the same basicmechanism as sensitization (heterosynaptic facilitation) superimposedon homosynaptic depression. Carew et al. (1971) came to similarconclusions based on an analysis of complex PSPs during neuralanalogs of dishabituation andsensitization.

Plasticity of the on-field monosynaptic PSPs was approximately equal to plasticity of the complex PSPs and firing of the LFSmotor neurons during habituation, dishabituation, and sensitization(Fig. 15). Plasticity of LFS firing was in turn approximately equalto plasticity of the behavior during habituation. However, duringdishabituation and sensitization, the increase in siphon withdrawalwas somewhat larger than the increase in LFS firing, in part becauseof peripheral enhancement (Fig. 8). Thus, these three mechanisms(homosynaptic depression and heterosynaptic facilitation of monosynapticPSPs, and peripheral enhancement) appear to be sufficient to explainmost of the changes in siphon withdrawal during habituation, dishabituation,andsensitization.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

To try to test the relationship between synaptic plasticity and learning and memory in a more rigorous fashion than was previouslypossible, Cohen et al. (1997) first developed a simplified gill-withdrawalpreparation in which most of the reflex response is mediated througha single identified motor neuron. Frost et al. (1997) then usedthat preparation to provide direct evidence that homosynapticdepression of monosynaptic PSPs from LE siphon sensory neuronscontributes to habituation of the reflex response. However, itwas difficult to record monosynaptic PSPs during dishabituationand sensitization in the gill-withdrawal preparation. We thereforedeveloped the simplified siphon-withdrawal preparation and havebeen able to use it to provide direct evidence that plasticityof monosynaptic PSPs from LE sensory neurons contributes to habituation,dishabituation, and sensitization of the reflex response. We havefound that monosynaptic PSPs from LE sensory neurons to LFS motorneurons make a substantial contribution to the behavioral responsein the siphon-withdrawal preparation and that there is a goodfit between both the amplitude and duration of plasticity of themonosynaptic PSPs and plasticity of the behavior during habituation,dishabituation, andsensitization.

Although encouraging, the fit between plasticity of the PSPs and behavior is in fact somewhat surprising. We have estimatedthat monosynaptic PSPs from LE sensory neurons contribute 60%of the complex PSP in LFS motor neurons and that LFS neurons (andall central neurons) in turn contribute 55% of the behavioralresponse, so that the monosynaptic PSPs should contribute approximatelyone-third of the behavioral response. These results imply thatthe other central and peripheral components of the reflex undergoplasticity similar to that of the monosynaptic PSPs from LE toLFS neurons. We have found that tail shock produces peripheralenhancement that is roughly similar to plasticity of the monosynapticPSPs during dishabituation and sensitization (Fig. 8). Frost etal. (1997) earlier found that plasticity of monosynaptic PSPsfrom other as yet unidentified sensory neurons also appears tobe similar to plasticity of PSPs from the LE sensory neurons duringhabituation, dishabituation, and sensitization in the gill-withdrawalpreparation. Furthermore, plasticity of PSPs from LE neurons toperipheral motor neurons is similar to plasticity of PSPs to centralmotor neurons during a neural analog of habituation (Bailey etal., 1979). Plasticity of the polysynaptic component of the reflexmight also be similar if it were primarily attributable to plasticityof the monosynaptic input from sensory neurons to interneurons.However, although plasticity of the monosynaptic PSPs, complexPSPs, motor neuron firing, and behavior were similar during habituation,dishabituation, and sensitization overall (Fig. 15), there weresome more subtle differences between motor neuron firing and thecomplex PSP, and between dishabituation and sensitization, whenwe examined changes in the shapes of the responses (Figs. 7, 11).These more subtle differences are probably attributable to differencesin plasticity of excitatory and inhibitory interneurons in thepolysynaptic component of the reflex, which would thus also contributeto plasticity of thebehavior.

Comparison with the gill-withdrawal preparation

Having two simplified preparations has allowed us to compare plasticity of the gill- and siphon-withdrawal components of thereflex. Such comparisons have revealed a number of similaritiesbut also some important differences between the two preparations.In both preparations, habituation appears to be attributable primarilyto homosynaptic depression of monosynaptic PSPs from siphon sensoryneurons. Also, in both preparations, dishabituation and sensitizationinvolve facilitation of the monosynaptic component of the PSPthat is maximal 2.5 min after the shock, as well as peripheralenhancement that is also maximal 2.5 min after the shock and isassociated with an increase in spontaneous firing of the motorneurons.

Although in the siphon-withdrawal preparation the facilitation of monosynaptic PSPs has approximately the same amplitude andduration as facilitation of complex PSPs, increased firing ofmotor neurons, and increased siphon withdrawal, in the gill-withdrawalpreparation there are dissociations between facilitation of themonosynaptic component of the PSP and the other response measures(Cohen et al., 1997). First, although maximal facilitation ofthe monosynaptic PSP occurs 2.5 min after the shock, in the gill-withdrawalpreparation the maximal increases in withdrawal, evoked firingof the motor neuron, and the complex PSP all occur 12.5 min afterthe shock and are therefore thought to involve an important contributionfrom plasticity in interneurons. The time of maximal dishabituationor sensitization has similarly ranged from 2 or 3 min to >20 minin studies on intact animals (Pinsker et al., 1970; Mackey etal., 1987; Marcus et al., 1988; Hawkins et al., 1998a).

Second, in the gill-withdrawal preparation when facilitation of the monosynaptic PSP is maximal, there are relatively smallincreases or no change in the behavior and firing of the motorneuron and an actual decrease in the complex PSP (Cohen et al.,1997). Wright et al. (1991) observed similar dissociations betweenmonosynaptic and complex PSPs and suggested that they could beattributable to the contribution to the complex PSP of unidentifiedsensory neurons with different plasticity than the LE sensoryneurons. However, the monosynaptic component of the PSP in thegill-withdrawal preparation was measured by stimulating the siphonwith the abdominal ganglion bathed in high divalent seawater (whichreduces the polysynaptic component) and therefore included thecontribution of any unidentified sensory neurons (Cohen et al.,1997). Thus, the dissociation between the monosynaptic and complexPSP was more likely caused by transient inhibition of interneuronsinvolved in the polysynaptic component. Such transient inhibitionhas also been observed behaviorally for some components of thegill- and siphon-withdrawal reflex (Mackey et al., 1987; Marcuset al., 1988) but not for others (Hawkins et al., 1998a), andin particular does not occur for the "flaring" response that isthought to be measured in the siphon-withdrawal preparation (Illichet al., 1994). Thus, the simpler pattern of behavioral and cellularresults in the siphon-withdrawal preparation may be attributablein part to the lack of transient inhibition of interneurons involvedin the particular response measured in thatpreparation.

Similarly, although in the siphon-withdrawal preparation increases in monosynaptic PSPs, complex PSPs, firing of the motorneurons, and behavior were all approximately the same during dishabituationas during sensitization (Fig. 15), in the gill-withdrawal preparationthere were dissociations between dishabituation and sensitization(Cohen et al., 1997). In particular, facilitation of the complexPSP in the gill motor neuron was larger (or transient inhibitionwas smaller) during dishabituation than during sensitization.Similar dissociations have been observed at both the behavioraland cellular levels for some components of the gill- and siphon-withdrawalreflex (Mackey et al., 1987; Marcus et al., 1988; Wright et al.,1991), and these dissociations as well as other lines of evidence(Hochner et al., 1986; Rankin and Carew, 1988) have suggestedthat dishabituation and sensitization might involve differentunderlying mechanisms. However, such dissociations have not beenobserved for other components of the reflex in intact animals(Hawkins et al., 1998a) or in the siphon-withdrawal preparation,indicating that they are not universal. Moreover, the dissociationsbetween dishabituation and sensitization have only been observedunder circumstances when transient inhibition was also observed,suggesting that they may be attributable, at least in part, toan interaction between habituation and inhibition rather thana fundamental difference between dishabituation and sensitization.In the siphon-withdrawal preparation, there appears to be no transientinhibition and also no difference between the major cellular mechanismscontributing to dishabituation and sensitization insofar as wehave examined them, although such a difference cannot be excluded.There were some more subtle differences between dishabituationand sensitization, and also between motor neuron firing and thecomplex PSP, when we examined changes in the shapes of the responses(Figs. 7, 11). However, these were the reverse of similar changesobserved in the gill-withdrawal preparation (Cohen et al., 1997),suggesting that learning in the two preparations involves differentplasticity in interneurons participating in the two componentsof thereflex.

These differences between the gill- and siphon-withdrawal preparations illustrate that the withdrawal is not unitary but hasdistinguishable components that make different contributions tothe observed behavior depending on the experimental circumstancesand undergo different plasticity during learning. Similar resultshave been observed in intact animals (Hawkins et al., 1998a).These findings demonstrate the importance of examining cellularmechanisms of learning under the same circumstances and preferablyat the same time as the behavior. The simplified gill- and siphon-withdrawalpreparations have made it possible for us to do that. Our studiesof these preparations have provided the first direct evidencethat plasticity of monosynaptic PSPs contributes to learning andmemory for habituation, dishabituation, and sensitization of thereflex, and they have shed new light on the relationship betweendishabituation and sensitization. It will now be interesting toexamine how plasticity of the gill- and siphon-withdrawal componentsof the reflex are integrated during these forms of learning andto perform a similar analysis of classic conditioning in thesepreparations (Hawkins et al., 1998b; our unpublishedobservations).

  FOOTNOTES

Received June 7, 1999; revised July 30, 1999; accepted Sept. 13, 1999.

This work was supported by a grant from the National Institute of Mental Health (MH26212). We thank J. Koester, I. Kupfermann,and C. Rankin for their comments, H. Ayers and M. Pellan for typingthis manuscript, and C. Lam for preparing thefigures.
Correspondence should be addressed to Dr. Robert D. Hawkins, Center for Neurobiology and Behavior, Columbia University Collegeof Physicians and Surgeons, 722 West 168th Street, New York, NY10032. E-mail: rhawkins{at}pi.cpmc.columbia.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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[Abstract] [Full Text] [PDF]

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