Nitric Oxide Is Necessary for Multiple Memory Processes after Learning That a Food Is Inedible in Aplysia

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The Journal of Neuroscience, November 1, 2002, 22(21):9581-9594

Nitric Oxide Is Necessary for Multiple Memory Processes after Learning That a Food Is Inedible in Aplysia
Ayelet Katzoff, Tziona Ben-Gedalya, and Abraham J. Susswein
Faculty of Life Sciences, Gonda (Goldschmied) Medical Diagnostic Research Center, Bar Ilan University, Ramat Gan 52 900, Israel

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Nitric oxide (NO) signaling was inhibited via N $omega$ -nitro-L-arginine methyl ester (L-NAME) during and after training Aplysiathat a food is inedible. Treating animals with L-NAME 10 min beforethe start of training blocked the formation of three separablememory processes: (1) short-term, (2) intermediate-term, and (3)long-term memory. The treatment also attenuated, but did not block,a fourth memory process, very short-term memory. L-NAME had littleor no effect on feeding behavior per se or on most aspects ofthe animals' behavior while they were being trained, indicatingthat the substance did not cause a pervasive modulation or poisoningof many aspects of feeding and other behaviors. Application ofL-NAME within 1 min after the training had no effect on short-or long-term memory, indicating that NO signaling was not neededduring memory consolidation. Treating animals with the NO scavenger2-phenyl-4,4,5,5-tetramethyl-imidazdine-1-oxy-3-oxide before trainingalso blocked long-term memory. Memory was not blocked by D-NAME,or by the simultaneous treatment with L-NAME and the NO donorS-nitroso-N-acetyl-penicillamine, confirming that the effect ofL-NAME is attributable to its effect as a competitive inhibitorof L-arginine for NO synthase in the production of NO rather thanto possible effects at other sites. These data indicate that NOsignaling during training plays a critical role in the formationof multiple memoryprocesses.

Key words: nitric oxide; learning; long-term memory; short-term memory; intermediate-term memory; feeding; Aplysia

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Nitric oxide (NO) is an unconventional transmitter in the nervous systems of many animals (Garthwaite and Boulton, 1995; Jacklet,1997). NO transmission is associated with memory formation invertebrates (Böhme et al., 1993; Kendrick et al., 1997) and invertebrates(Müller, 1996). Neurons using NO are found in the neural circuitcontrolling Aplysia feeding (Jacklet, 1995). This well characterizedcircuit (Weiss et al., 1986a,b; Susswein and Byrne, 1988; Plummerand Kirk, 1990; Teyke et al., 1990, 1993; Rosen et al., 1991;Morton and Chiel, 1993; Hurwitz and Susswein, 1996; Hurwitz etal., 1997; Susswein et al., 2002) is used as a model for examiningthe organization and regulation of a complex behavior (Kupfermannet al., 1991). Aplysia feeding is modified by both associativeand nonassociative learning (Susswein et al., 1986; Schwarz etal., 1988; Lechner et al., 2000; Brembs et al., 2002). Informationon the role of NO transmission in learning and memory in thiscircuit can be put into a wider context, in which cellular, circuit,and behavioral properties are allaccessible.

We have examined the role of NO in an associative learning task having affinities with instrumental learning in higher animals.In this task, Aplysia are stimulated with a food that is too toughto eat. This food elicits bites that lead to food entry into themouth. The food then elicits swallowing movements, but these areineffective because the food is too tough. The animals' responsesbecome progressively less vigorous, and they eventually stop responding.The changes in response are specific to the taste and textureof the food. The changes in behavior are dependent on the entryof food into the mouth and on the consequent failed attempts toswallow (Susswein et al., 1986; Schwarz et al., 1988). Memoryafter training is monitored by a maintained decrease in responseto the inedible food and by savings in the time to retrain animals(Schwarz et al., 1988, 1991). Four separable memory processes(very short-, short-, intermediate-, and long-term memory) areseen after training. The memory processes can be separated bypost-training procedures (Botzer et al., 1998), which block long-termmemory but leave short-term memory intact. Memory processes canalso be distinguished by a variety of training protocols. Someprotocols lead only to long-term memory, with no preceding expressionof short- or intermediate-term memory, whereas others produceboth short- and long-term memory but not intermediate-term memory(Botzer et al., 1998). The ability to achieve long-term memoryin animals that did not first display short-term memory showedthat short- and long-term memory are independent, parallel processes.Long-term memory can last for up to 3 weeks (Schwarz et al., 1991).

This research examines the effects on learning and on the various memory processes of blocking NO signaling. Blocking of NOsignaling before training had no measurable effect on Aplysiafeeding, and during learning with inedible foods, most aspectsof the training were normal. However, blocking NO signaling duringtraining attenuated very short-term memory and completely blockedshort-, intermediate-, and long-term memories. Blocking of NOsignaling immediately after training had no effect on either short-or long-term memory, indicating that NO release only during thetraining, and not during consolidation, plays a role in memoryformation.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. Experiments were performed on Aplysia fasciata and Aplysia californica. A. fasciata weighed 50-150 gm and were collectedalong the Mediterranean coast of Israel. This species is availablelocally from May through August, and experiments performed duringthis period used them. A. californica weighed 100-150 gm and werepurchased from Marine Specimens Unlimited (Pacific Palisades,CA). A. californica was used for experiments when A. fasciatawere unavailable. The choice of the species used was based onthe season during which a particular experiment was performed.Some experiments were repeated using both species, with no differencesin results. The species used in each experiment is noted below.Animals were stored five or six to a cage in plastic mesh cagesimmersed in 1300 l tanks of aerated, filtered Mediterranean seawaterat 18°C with a 12 hr light-dark cycle. The animals were fed oneor two times weekly with Ulva lactuca that was gathered alongwith A. fasciata and was storedfrozen.

One week before an experiment, animals were separated from one another. They were kept thereafter in individual cages andwere food-deprived. Twenty-four hours before an experiment, theywere transferred to 10 l experimental aquariums that were maintainedat 19-20°C. Because in A. fasciata the presence of a conspecificin the environment is needed for animals to learn that a foodis inedible (Schwarz and Susswein, 1992), a second Aplysia wasalways transferred to the experimental aquarium along with theexperimental animal. The second animal was maintained behind apartition that was not a barrier to the flow of seawater but thatprevented contact between the animals. Because A. californicaare diurnally active (Kupfermann, 1968) and A. fasciata are nocturnalanimals (Ziv et al., 1991), experiments on A. californica wereperformed during the light portion of the day, whereas those onA. fasciata were done during the dark portion, as described previously(Susswein et al., 1986).

Tests of response to food. A number of experiments examined the animals' ability to respond to food, independent of learning.To test the response of animals to a pure chemical stimulus thatevokes feeding, a seaweed extract was prepared by soaking Ulvain 20 times its weight of seawater and then homogenizing thismixture for 20 min. The mixture was then filtered, and 15 ml ofthe fluid was placed in a 5 l aerated experimental chamber containingan animal. The animal had been transferred to the container 12hr before the start of the experiment. Other experiments examinedthe response to ad libitum access to food as well as to smallpieces or strips of seaweed. Techniques for examining the responseto food were as described previously (Susswein et al., 1976; Rosenet al., 1989; Blumberg and Susswein, 1998; Blumberg et al., 1998).

Training procedure. As in previous studies (Schwarz and Susswein, 1986; Susswein et al., 1986; Schwarz et al., 1988, 1991;Botzer et al., 1998), training began by touching a small pieceof Ulva wrapped in plastic net to the rhinophores of animals.Aplysia respond to this stimulus by lifting the head and centeringfood on the lips. Food on the lips initiates a biting response,which leads to entry of food into the buccal cavity. Food in thebuccal cavity leads to swallowing responses. However, becausenetted food physically cannot be swallowed, it becomes lodgedin the buccal cavity, where it produces repetitive failed swallowingresponses. Food eventually leaves the buccal cavity. The nettedfood continues to stimulate the lips, producing further bitingresponses, which again lead to failed swallows. As training proceeds,many responses fail to lead to entry of food into the buccal cavity.When food enters the buccal cavity, it stays within the cavityfor progressively shorter periods, eliciting fewer attempted swallowingresponses. Finally, animals stop responding to the netted food.The criterion for cessation of responsiveness was 3 min withoutfood entering the mouth (Botzer et al., 1998). In all experiments,biting responses and entry and exit of food into and from thebuccal cavity were observed visually, and occurrences were notedby pressing the appropriate button of a three-button mouse connectedto a computer. A computer program noted the time that a mousebutton was pressed. In addition, swallowing responses that werefelt by the experimenter as an inward pull on the netted foodwere alsonoted.

Memory is shown by testing the animals in a procedure that is identical to that in the initial training. Memory is displayedby a decrease in the responsiveness of the animals at the startof training and by a reduction in the time needed for the animalsto stop responding to the food. The measure of responsivenessto food used in this and previous studies is the time spent byfood in the buccal cavity during the first 5 min of a session(Susswein et al., 1986; Botzer et al., 1998).

All experiments testing intermediate- and long-term memory were performed using a blind procedure, in which naive animals,seawater-treated animals, or both were tested along with the experimentalanimals.

Drugs and drug treatments. NO signaling was blocked with N $omega$ -nitro-L-arginine methyl ester (L-NAME; concentration, 100 mg/kg),an inhibitor of nitric oxide synthase (NOS). This was deliveredby preparing a solution of 10 mg/ml in artificial seawater (ASW)and injecting animals with a volume that was appropriate to theanimal's weight. Most animals weighted ~100 gm, so 1 ml was injected.The composition of the artificial seawater was (in mM): NaCl,460; KCl, 10; CaCl₂, 11; MgCl₂, 55; and NaHCO₃, 5. In some experiments,D-NAME, at a concentration identical to that of L-NAME, was injectedinto animals as a control for the possible nonspecific effectsof L-NAME. In one experiment, animals were injected with 2-phenyl-4,4,5,5-tetramethyl-imidazdine-1-oxy-3-oxide(PTIO), an NO scavenger, at a concentration of 0.025 mM. Animalsof ~100 gm were then injected with 1 ml of this solution. In oneexperiment, the NO donor S-nitroso-N-acetyl-penicillamine (SNAP;1 mM) was injected immediately after the L-NAME treatment, Animalswere injected with a solution of 0.2 mg/ml prepared in ASW. Animalswere injected with these substances either 10 min before trainingor immediately (within 1 min) after training, as was needed forthe experimentalprocedure.

Statistics. Many experiments examined the effects of a drug on memory after training. The presence of memory was measuredby using paired t tests that compared the behavior before andafter training. In addition, the percentage of change in responsefor experimental animals was compared with that of seawater-treatedcontrols that were run simultaneously. For each animal, the percentageof change between the training and testing session was calculated,and a t test was used to determine whether there were significantdifferences between experimental and control groups. For someexperiments, data were not available on the parameters of theinitial training, and in these experiments, the parameters ofthe sessions testing memory were compared between experimentaland control groups, using ttests.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

L-NAME does not block feeding behavior

The aim of the study was to determine whether NO signaling has a role in learning that food is inedible or in memory afterlearning. However, before determining whether inhibiting NO signalingaffects learning or memory, it was important to examine whethersuch inhibition affects feeding behavior per se. Animals (A. fasciata)were allowed 1 hr of ad libitum access to food after 1 week offood deprivation. Animals were observed throughout this hour,and the start and end of all feeding bouts were noted. Previousstudies (Ziv et al., 1991) have shown that such observations areaccurate to within ~15 sec in judging the start and stop of feeding,and individual bouts of feeding are minutes long. The percentageof time spent feeding was then calculated in animals that weretreated with L-NAME 10 min before the start of the observationas well as in control animals that were treated with seawater.There were no obvious differences in the patterning or vigor offeeding movements between animals injected with L-NAME and thoseinjected with seawater. In both groups, 65-70% of the hour wasdevoted to feeding, and there was no significant difference inthe time devoted to feeding (p = 0.78; t₍₁₁₎ = 0.29; two-tailedt test) (Fig. 1A). These data indicate that L-NAME does not disruptfeeding behavior, although it is possible that L-NAME may causesubtle effects that require a fine-grained analysis to discern.

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Figure 1. Lack of effects of L-NAME on feeding behavior. Shaded bars, Treated with L-NAME; open bars, treated with seawater. A, Percentage of time spent feeding in 1 hr of ad libitum exposure to food (n = 7 seawater controls; n = 6 animals treated with L-NAME). B, Latency to respond to food touching the lips in previously unaroused animal (n = 7 seawater-treated animals; n = 11 L-NAME-treated animals). C, Number of bites in a 5 min period in which the lips were stimulated continuously with food (n = 8). D, Swallow amplitude. E, Swallow period (n = 10 seawater-treated animals; n = 5 L-NAME-treated animals). In this and in subsequent figures, means and SE are shown.

Additional experiments examined the possible effect of L-NAME on a number of different consummatory movements. In one, theability of food to arouse animals (A. fasciata) was examined.Previous experiments (Kupfermann, 1974; Susswein et al., 1978)have shown that exposure to food arouses Aplysia, so that theybecome more responsive to food on subsequent exposures. The latencyfrom the first touch of food (the seaweed Ulva) to the head ofan animal until it bites the food is a reliable measure of itscurrent arousal state (Susswein et al., 1978). We measured thisinitial arousal latency in animals that were treated with L-NAME10 min previously and in control animals that were treated withseawater (Fig. 1B). There was no significant difference in arousallatency between these two groups (p = 0.43; t₍₁₆₎ = 0.82; two-tailedt test), indicating that L-NAME did not affect the ability offood to arouseanimals.

An additional experiment examined the possible effect of L-NAME on biting. Animals (A. californica) were injected with eitherL-NAME or seawater, and 10 min later, their lips were stimulatedwith seaweed for 5 min. Animals were not permitted to consumethe food, which was briefly pulled away from the mouth when theanimals bit. The number of bites elicited during the 5 min stimulationwas counted. Twenty-four hours later, the procedure was repeated,except that animals that had been exposed to L-NAME were injectedwith seawater and vice versa (Fig. 1C). There was no significantdifference in the number of bites when animals were treated withL-NAME or seawater (p = 0.55; t₍₇₎ = 0.63; two-tailed paired ttest).

An additional experiment examined whether L-NAME affects a second Aplysia consummatory movement, swallowing. Animals werefed strips of food (the seaweed Ulva, which was cut into 6-cm-long× 3-mm-wide strips), which elicited a single bite and a seriesof swallowing responses. The number of swallows and the time neededto consume the strip were measured in animals that were exposedto either L-NAME or seawater 10 min before being fed. This examinationprovides information on the swallow amplitude, as measured bythe length consumed per swallow, and the swallow frequency, asmeasured by the interswallow interval (Blumberg et al., 1998).There were no significant differences for either of these parametersbetween animals exposed to seawater and L-NAME (for swallow amplitude,p = 0.21, t₍₁₄₎ = 1.33; for interswallow interval, p = 0.92, t₍₁₄₎= 0.11; two-tailed paired t tests). These data indicate that swallowingis not affected by L-NAME (Fig. 1D,E).

In another gastropod, Lymnaea, blocking of NO signaling attenuates or blocks the ability of animals to respond to a purelychemical stimulus that initiates feeding movements (Elphick etal., 1995; Korneev et al., 2002). In contrast, in the experimentsabove, we found that Aplysia respond well to food, even when NOsignaling is blocked. However, in our experiments, the food stimulustouched the animals; therefore, food was sensed via both chemoreceptorsand mechanoreceptors (Rosen et al., 1982), whereas the Lymnaeaexperiments used a purely chemical stimulus. To determine whetherL-NAME blocks Aplysia feeding in response to a purely chemicalstimulus, a seaweed extract was placed in a container with ananimal (A. californica) that was treated with either L-NAME orseawater, and a number of measures of feeding were observed: (1)the latency from entry of the chemical extract into the wateruntil the lift of the head, as animals assumed the typical feedingposture (Kupfermann, 1974) (Fig. 2A); (2) the latency until thefirst bite (Fig. 2B); (3) the number of bites performed withinthe first 5 min of exposure to the seaweed extract (Fig. 2C);(4) the total time until the Aplysia stopped responding to theseaweed extract (Fig. 2D); cessation of responses (defined as180 sec without a response) presumably was caused by sensory adaptationto the chemical stimulus (Horn et al., 2001); and (5) the distributionof the amplitude of the responses (Fig. 2E), with the bite amplitudequantified using a four-point scale (Susswein et al., 1976; Rosenet al., 1989). In this scale, 1 represents the weakest amplitudebite, and 4 is the strongest amplitude. The distribution of thebite amplitudes in animals treated with L-NAME was tested againstthe distribution of seawater-treated controls. For each animal,the number of bites of each magnitude was counted, and the meansand SE of the number of bites of each magnitude were then calculatedfor all of the L-NAME- and seawater-treated animals. There wereno significant differences in any of the parameters of feedingbetween animals treated with L-NAME and seawater, indicating thatthe responses to purely chemical stimuli initiating feeding arealso not affected by blocking NO signaling.

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Figure 2. Lack of effects of L-NAME on responses to seaweed extract in n = 8 seawater-treated and n = 8 L-NAME-treated animals. Shaded bars, Treated with L-NAME; open bars, treated with seawater. A, Latency to lift of the head. There was no significant difference between L-NAME- and seawater-treated animals (p = 0.39; t₍₁₄₎ = 0.88). B, Latency to the first bite. There was no significant difference between L-NAME- and seawater-treated animals (p = 0.67; t₍₁₄₎ = 0.43). C, Number of bites in 5 min of exposure. There was no significant difference between L-NAME- and seawater-treated animals (p = 0.59; t₍₁₄₎ = 0.55). D, Time to stop responding to the seaweed extract. There was no significant difference between L-NAME- and seawater-treated animals (p = 0.39; t₍₁₄₎ = 0.90). E, Amplitude of each bite elicited by seaweed extract using a four-point scale. There was no significant difference in the relative distribution of the four levels of bite amplitude (p = 0.09; $chi$ ²₍₃₎ = 6.42).

L-NAME does not block learning that a food is inedible

Ten minutes after treatment with either L-NAME or seawater, animals (A. fasciata) were stimulated with Ulva that was wrappedin plastic netting, making it inedible. The animals can tastethe food through the holes in the net. Animals treated with L-NAME,as well as those treated with seawater, responded readily to theinedible netted food and bit and then attempted to swallow it.After a number of failed attempts to swallow the netted food,it was rejected. The food continued to stimulate the lips, andanimals bit and attempted to swallow it again. As the trainingprogressed, animals responded less to the food. The food enteredthe mouth less frequently, and when it entered, it was rejectedearlier. Eventually, animals stopped responding to the nettedfood. The changes in responses and their cessation are attributedto associative learning (Susswein et al., 1986; Schwarz et al.,1988).

Previous experiments (Susswein et al., 1986) have used the time that food spends in the mouth and the number of swallows elicitedby the food as measures of responsiveness to the food. There wereno significant differences in these parameters between animalstreated with L-NAME or seawater (time in mouth, p = 0.57, t₍₃₅₎= 0.57; number of swallows, p = 0.76, t₍₂₃₎ = 0.31; two-tailedt tests) during the first 5 min of the training, indicating thatthe initial response to the inedible food is not affected by L-NAME(Fig. 3A,B).

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Figure 3. Lack of effects of L-NAME on training. Three parameters of the training were measured. Shaded bars, Treated with L-NAME; open bars, treated with seawater. A, Time that food is in the mouth during the first 5 min of training. B, Number of attempted swallowing responses performed during the first 5 min of training. C, Length of training needed for the animals to stop responding to the inedible food.

There was also no significant difference between animals treated with L-NAME or seawater in the time needed to stop respondingto the inedible netted food (p = 0.56; t₍₃₅₎ = 0.59; two-tailedt test), indicating that L-NAME does not affect this parameterof the initial learning that a food is inedible (Fig. 3C).

Block of NO signaling affects short- and long-term memory

Previous studies have identified a number of separable phases of memory (Botzer et al., 1998). A single training session continueduntil Aplysia stop responding to food elicits short-term memory,which is maintained for up to 0.5 hr, and long-term memory, whichis present from 1 to 7 d after training (Schwarz et al., 1991;Botzer et al., 1998). However, such a training session does notlead to intermediate-term memory, measured from 1 to 12 hr aftertraining. A series of experiments were performed to determinethe effects of L-NAME on memory processes that are elicited bya single training session that is continued until animals stopresponding to inedible nettedfood.

L-NAME before training blocks short-term memory
After training, memory was examined by re-exposing the animals to the same inedible food for a second time. As in previousstudies (Botzer et al., 1998; Schwarz et al., 1998), two parameterswere used to quantify memory: (1) the initial responsiveness tothe food (as measured by the time that food is in the mouth inthe first 5 min) and (2) the time needed to stop responding tothe inedible food. Memory is demonstrated by a decrease in theseparameters when animals are retrained, with respect to the valuesmeasured in the originaltraining.
The possible effect of L-NAME on short-term memory was examined by treating animals (A. fasciata) with either L-NAME or seawater,training them 10 min later, and then testing the animals 0.5 hrafter the end of the initial training (Fig. 4). Previous data(Botzer et al., 1998) have shown that robust short-term memoryis seen at this time. Decreases in both the time to stop respondingto food as well as in the time that food spent in the mouth duringthe first 5 min were seen 0.5 hr after training in seawater-treatedcontrol animals, indicating that these animals displayed short-termmemory. However, in animals that had been injected with L-NAMEbefore the training, there were no significant differences betweenthe initial training and the test of memory for either the timeto stop responding to food or for the time that food was in themouth during the first 5 min. There were also significant differencesin the percentage of changes in responses between the trainingand testing sessions between animals treated with L-NAME and seawaterfor both parameters of memory. Values in animals that had beeninjected with L-NAME were similar to those observed in previouslyuntreated, naive animals that were run as controls in tandem withthe previously trained animals. These data indicate that the formationof short-term memory is blocked in animals injected with L-NAMEbefore training.

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Figure 4. L-NAME treatment before training blocks short-term memory. Animals were treated before training with L-NAME (n = 7) or seawater (n = 6). Open bars, Data from the initial training session; shaded bars, data from a second session that measured memory after 30 min. Memory is indicated by a decrease in a value from the first to the second session. Experiments showing a significant decrease in this and in subsequent figures are marked with asterisks. An additional group of previously untreated naive animals (Naive; n = 6) was examined in a blind procedure along with the previously trained animals. A, There was a significant decrease in the time for animals to stop responding to inedible food between the training and testing session for the seawater-treated controls (p < 0.001; t₍₅₎ = 14.16) but not for the L-NAME-treated animals (p = 0.340; t₍₆₎ = 1.035; 2-tailed paired t tests). There was also a significant difference in the percentage of change in response between the training and testing session between L-NAME- and seawater-treated animals (p < 0.001; t₍₁₁₎ > 100; 2-tailed t test). B, There was a significant decrease in the time that food was in the mouth during the first 5 min between the two session for the control animals (p < 0.001; t₍₅₎ = 7.57) but not for animals treated with L-NAME (p = 0.227; t₍₆₎ = 1.35; 2-tailed paired t tests). In addition, there was a significant difference in the percentage of change in response between training and testing between L-NAME- and seawater-treated animals (p < 0.001; t₍₁₁₎ = 9.48; 2-tailed t test).

Short-term memory is preserved when L-NAME is injected after training
Injecting L-NAME before training potentially could interfere with short-term memory formation either during the training periodor during the 0.5 hr interval between the training and the test.To differentiate between these possibilities, either L-NAME orseawater was injected into animals (A. californica) immediately(within 1 min) after training, and memory was examined 0.5 hrlater (Fig. 5). Both the animals injected with L-NAME and thoseinjected with seawater displayed significant decreases in thetime to stop responding and in the time that food spent in themouth during the first 5 min, indicating that blocking NO synthesisafter training does not eliminate short-term memory. In addition,there were no significant differences in the percentage of changein responses between the training and testing sessions betweenanimals treated with seawater and with L-NAME. Thus, the blockof memory by L-NAME is the result of the effect of the drug beforeor during the training and not subsequent to it.

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Figure 5. L-NAME treatment immediately after training does not affect short-term memory. The experiment was identical to that in Figure 4, except that animals were treated with L-NAME or seawater immediately after the training. For animals treated with L-NAME, n = 8; for animals treated with seawater, n = 6; for naive animals, n = 7. A, There was a significant decrease in the time to stop responding between the training and testing session for the control animals (p < 0.001; t₍₅₎ = 8.28) and for the animals treated with L-NAME (p < 0.001; t₍₇₎ = 11.77; 2-tailed paired t tests). In addition, there was no significant difference in the percentage of change in response between the training and testing session between animals treated with L-NAME and with seawater (p = 0.94; t₍₁₂₎ = 0.07; 2-tailed t test). B, There was a significant decrease in the time that food was within the mouth during the first 5 min between the training and testing session for animals treated with seawater (p = 0.002; t₍₅₎ = 5.74) and for animals treated with L-NAME (p < 0.001; t₍₇₎ = 7.19; 2-tailed paired t tests). In addition, there was no significant difference in the percentage of change in response between the training and testing session (p = 0.56; t₍₁₂₎ = 0.60; 2-tailed t test).

L-NAME before training blocks long-term memory
Previous studies (Botzer et al., 1998) indicated that short- and long-term memory after learning that a food is inedible areindependent processes, because each can be obtained in the absenceof the other. The independence of short- and long-term memoriesraises the possibility that L-NAME specifically blocks short-termbut not long-term memory. To examine this possibility, animals(A. fasciata) were treated with either L-NAME or seawater 10 minbefore training, and memory was tested 24 hr later (Fig. 6). Forthe seawater-treated controls, during the test of memory therewere significant decreases in both the time to stop respondingto food and in the time that food was in the mouth during thefirst 5 min with respect to the values seen during the initialtraining. However, there were no significant differences betweenthe training and testing sessions in animals that had been treatedwith L-NAME before the training. There were also significant differencesbetween animals treated with L-NAME and with seawater in the percentageof changes in response between the training and testing sessionsfor both the time to stop and for the time spent in the mouth.Values during the 24 hr test in animals that had been treatedwith L-NAME were similar to those observed in naive animals thatwere run as controls in tandem with the previously trained animals.These data indicate that the formation of long-term memory isblocked in animals injected with L-NAME before training.

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Figure 6. L-NAME treatment before training blocks long-term memory. The experiment was identical to that in Figure 4, except that the test of memory was performed after 24 hr. For animals treated with L-NAME, n = 7; for animals treated with seawater, n = 4; for naive animals, n = 6. A, There was a significant decrease in the time to stop responding to the inedible food between the training and testing session for the control animals (p < 0.001; t₍₃₎ = 25.37) but not for the L-NAME-treated animals (p = 0.32; t₍₆₎ = 1.08; 2-tailed paired t tests). In addition, there was a significant difference in the percentage of change in response between the training and testing session between animals treated with L-NAME and seawater (p < 0.001; t₍₉₎ = 10.13; 2-tailed t test). B, There was a significant decrease in the time that food was in the mouth during the first 5 min from the training and testing session for the control animals (p = 0.005; t₍₃₎ = 7.19) but not for the L-NAME-treated animals (p = 0.33; t₍₆₎ = 1.06; 2-tailed paired t tests). In addition, there was a significant difference between L-NAME- and seawater-treated animals in the percentage of change in response from the training to the testing session (p = 0.002; t₍₉₎ = 4.14; 2-tailed t test).

Long-term memory is preserved when L-NAME is injected after training
The inhibition of long-term memory by L-NAME could be explained by effects that occur after the training, during the periodof memory consolidation. To test this possibility, animals (A.fasciata) were treated with either L-NAME or seawater immediatelyafter training, and memory was tested 24 hr later (Fig. 7). Boththe animals treated with L-NAME and those treated with seawaterdisplayed significant decreases between the training and testingsessions in the time to stop responding to food and in the timethat food spent in the mouth during the first 5 min, indicatingthat blocking NO synthesis after training does not eliminate long-termmemory. There were also no significant differences in the percentageof change in response between the training and testing sessionsbetween animals treated with L-NAME and seawater for both parametersof memory.

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Figure 7. L-NAME treatment immediately after training does not affect long-term memory. The experiment was identical to that in Figure 6, except that animals were treated with L-NAME or seawater immediately after the training rather than preceding it. For animals treated with L-NAME, n = 7; for animals treated with seawater, n = 5; for naive animals, n = 5. A, There was a significant decrease in the time to stop responding to the inedible food between the training and testing session for the control animals (p = 0.002; t₍₄₎ = 12.13) and for the L-NAME-treated animals (p = 0.001; t₍₆₎ = 5.80; 2-tailed paired t tests). In addition, there was no significant difference between these groups in the percentage of change in response from the training and testing session (p = 0.11; t₍₁₀₎ = 1.77; 2-tailed t test). B, There was a significant decrease in the time that food was within the mouth during the first 5 min between the training and testing session for the control animals (p = 0.013; t₍₄₎ = 4.22) as well as for the L-NAME-treated animals (p = 0.019; t₍₆₎ = 3.16; 2-tailed paired t tests). In addition, there was no significant difference in the percentage of change in response between the training and testing session (p = 0.52; t₍₁₀₎ = 0.67; 2-tailed t test).

Lip stimulation alone is not sufficient to establish long-term memory
Previous studies have shown that stimulation of the lips with food is not sufficient to cause long-term changes in feedingbehavior. Long-term memory also requires food entry into the mouthand the subsequent failure of swallowing responses to convey thefood into the gut. The experience of food in the mouth and failedswallows must be temporally associated with the lip stimulation(Susswein et al., 1986). An additional experiment was performedto verify the previous finding that long-term memory requiresthe temporal association of exposure to food with the subsequententry of food into the mouth and the failure to swallow the food.This experiment also examined the possible effect of L-NAME onthe need for food entry into the mouth on long-termmemory.
Animals (A. californica) were treated with either L-NAME or seawater. Half of the L-NAME-treated animals and half of the seawater-treatedanimals were trained with inedible food until they stopped responding.In the other half, the lips were stimulated with netted food,but the food was not permitted to enter the mouth. Animals thatwere treated with lip stimulation were yoked to the animals thatreceived normal training with the food entering the mouth; ineach stimulated animal, the lip stimulus was continued for a periodthat was yoked and was therefore identical to that required forcessation of responses in a matched experimental animal. Thus,the duration of the lip stimulation was determined by the timeto stop in the trained animal; therefore, the means and SD forthe trained and stimulated animals are the same. The yoked procedurewas performed for both L-NAME- and seawater-treated animals. Twenty-fourhours after training or lip stimulation, all of the animals weretested in a blind procedure, with inedible food that entered themouth and elicited failed swallows, to test long-term memory (Fig.8).

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Figure 8. Lip stimulation alone is insufficient for memory formation. L-NAME-treated (n = 8) and seawater-treated (n = 7) animals were trained with inedible food. Each trained animal was yoked to an animal whose lips were stimulated (for L-NAME-treated, n = 8; for seawater-treated, n = 7) for a period equivalent to that of the training. Twenty-four hours later, both the trained and the yoked animals were tested with inedible netted food that entered the mouth and produced failed swallows. For animals treated with seawater, significant differences were observed between the animals that had been trained with food entering the mouth and those in which the lips were stimulated for both the time to stop responding to food (p < 0.001; t₍₁₃₎ = 5.68) and the time that food was in the mouth during the first 5 min of the test (p < 0.01; t₍₁₃₎ = 3.10; 2-tailed t tests). However, for animals treated with L-NAME, no significant differences were observed between the trained animals and the yoked controls (for the time to stop, p = 0.22, t₍₁₅₎ = 1.28; for the time that food was in the mouth, p = 0.73, t₍₁₅₎ = 0.36; 2-tailed t tests).

For animals treated with seawater, significant differences were observed between the animals that had been trained with foodentering the mouth and those in which the lips alone were stimulatedfor both the time to stop responding to food as well as for thetime that food was in the mouth during the first 5 min of thetest. For the animals that had received lip stimulation alone,values were comparable with those during the initial trainingwith inedible food entering the mouth. In contrast, there wereno significant differences in L-NAME-treated animals between thosethat had been trained previously with food entering the mouthand with food stimulating the lips. Values in both groups werecomparable with those in the initial training sessions. Thesefindings confirm that food must enter the mouth and initiate failedswallowing responses to produce long-term memory, and this requirementis not affected in animals treated with L-NAME.

D-NAME does not block memory
L-NAME blocks NO production by acting as a competitive inhibitor of L-arginine for NOS, the enzyme that produces NO. However,L-NAME may cause a number of additional, nonspecific effects (Buxtonet al., 1993; Moroz et al., 1998). A number of experiments weredesigned to determine whether the effects of L-NAME occur viaits inhibition of NO production or via nonspecificeffects.
The first such experiment examined the effects of D-NAME, the chemically identical enantiomer of L-NAME, which does not interactwith NOS and inhibit NO production. Animals (A. californica) weretreated with D-NAME 10 min before the training. Memory was testedeither 0.5 or 24 hr after the training, to test the possible effectsof D-NAME on short- and long-term memory, respectively. Becausethe previous experiment showing that short- and long-term memoriesare blocked by L-NAME were performed on A. fasciata, we also replicatedthese finding using A. californica, to be certain that L-NAMEis also effective in thisspecies.
As was found in previous experiments, no significant differences were seen between the initial training and the test in animalstreated with L-NAME before the training, after either 0.5 or 24hr, using either measure of memory (Fig. 9). In contrast, theanimals treated with D-NAME showed significant savings when testedeither 0.5 or 24 hr after the training. D-NAME-treated animalswere run along with controls treated with seawater (data not shown).The percentage of savings were significantly larger in D-NAME-treatedanimals than for animals treated with seawater for the time spentin the mouth 24 hr after the training. There were no other significantdifferences between these D-NAME- and seawater-treated animals.Thus, D-NAME does not block either short- or long-memory, indicatingthat the effects of L-NAME are likely to be results of its specificactions on NOS.

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Figure 9. D-NAME does not block memory. A, Effects of L- and D-NAME application before training on short-term memory. L-NAME blocked short-term memory, as shown by no significant differences between training and testing (for the time to stop responding to food, p = 0.53, t₍₉₎ = 0. 69; for the time that the food was in the mouth during the first 5 min, p = 0.21, t₍₉₎ = 1.49; 2-tailed paired t tests). In contrast, D-NAME did not affect short-term memory, as shown by significant savings between training and testing (for time to stop responding, p < 0.001, t₍₇₎ = 9.73; for time in the mouth, p < 0.001, t₍₇₎ = 7.97; 2-tailed paired t test). B, Effects of L- and D-NAME before training on long-term memory. L-NAME blocked long-term memory, as shown by no significant difference in the time to stop responding to food (p = 0.59; t₍₆₎ = 0.56) and in the time that the food was in the mouth during the first 5 min (p = 0.88; t₍₆₎ = 0.15; 2-tailed paired t tests). In contrast, D-NAME did not affect long-term memory, because there were significant differences in both the time to stop responding to food (p < 0.001; t₍₆₎ = 17.28) and in the time in the mouth (p < 0.001; t₍₆₎ = 10.06; 2-tailed paired t tests). D-NAME-treated animals were run in a blind procedure with seawater-treated controls. There was no significant difference in the percentage of savings between D-NAME- and seawater-treated animals for the time to stop responding (p = 0.24; t₍₁₀₎ = 1.18), and for the time spent in the mouth, there was a significantly larger percentage of savings for D-NAME-treated animals than for seawater-treated animals (p = 0.4; t₍₁₀₎ = 2.42; 2-tailed t tests).

PTIO blocks long-term memory
An additional way to demonstrate that the effects of L-NAME occur via inhibition of NO production would be to block NO activityby using another compound, which has a different mode of activity.Accordingly, we examined the effects on learning and long-termmemory of PTIO, an NO scavenger (Park et al., 1998). Animals (A.californica) were treated with either PTIO or seawater 10 minbefore training, and memory was tested 24 hr after training. Theeffects of PTIO were similar to those of L-NAME (Fig. 10). Foranimals treated with PTIO, there was no significant differencein the time to stop responding to food between the training andtesting sessions, and there was also no significant differencein the time that food was in the mouth in the first 5 min of thetraining and test sessions. In contrast, control animals treatedwith seawater showed significant decreases in the time to stopresponding to the food and in the time in the mouth during thefirst 5 min. However, there were no significant differences inthe percentage of savings between PTIO- and seawater-treated animalsfor either the time to stop responding or the time that food wasin the mouth. Nonetheless, these data are consistent with thehypothesis that blocking NO signaling blocks memory formation.

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Figure 10. PTIO blocks long-term memory. Animals were treated with PTIO (n = 9) or seawater (n = 7) before training, and memory was measured after 24 hr. A, There was a significant decrease in the time to stop responding between the training and testing session for the control animals (p = 0.025; t₍₆₎ = 2.95) but not for animals treated with PTIO (p = 0.492; t₍₈₎ = 0.71; 2-tailed paired t tests). However, there was no significant difference in the percentage of change in response between the training and testing session between animals treated with PTIO and seawater (p = 0.09; t₍₁₃₎ = 1.82; 2-tailed t test). B, There was a significant decrease in the time that food was within the mouth during the first 5 min of a session between the training and testing session for the control animals (p = 0.016; t₍₆₎ = 3.33) but not for animals treated with PTIO (p = 0.085; t₍₈₎ = 1.97; 2-tailed paired t tests). However, there was no significant difference in the percentage of change in response between PTIO- and seawater-treated animals between the training and testing session (p = 0.07; t₍₁₄₎ = 1.93; 2-tailed t test).

The NO donor SNAP restores long-term memory
An additional way to demonstrate that L-NAME affects memory by blocking NO release is to show that memory can occur even inthe presence of L-NAME if an exogenous source of NO is present.To examine whether exogenous NO can overcome the effects of L-NAME,the NO donor molecule SNAP (Park et al., 1998) was injected intoanimals (A. californica) immediately after L-NAME was injected.In control animals, seawater was injected in place of SNAP. Animalswere then trained, and long-term memory was examined after 24hr. Our expectation was that animals treated with SNAP would displaylong-term memory, whereas animals treated with seawater wouldnot. This expectation was confirmed (Fig. 11). In animals treatedwith SNAP, there were significant differences between the initialtraining and the test 24 hr after training, using as criteriaboth the time to stop responding and the time that food spentin the mouth for the first 5 min, whereas animals treated withseawater did not display memory, as measured by no significantchanges between the training and the testing in the time to stopresponding to the food or in the time spent in the mouth duringthe first 5 min.

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Figure 11. Effects on long-term memory of treating animals with the NO donor SNAP. All animals were treated with L-NAME before training. One group of animals (n = 8) was then immediately treated with SNAP, and another was treated with seawater (n = 5). Memory was examined after 24 hr. A, There was no significant decrease in the time to stop responding between the training and testing session for the animals treated with seawater (p = 0.85; t₍₄₎ = 0.20). In contrast, animals treated with SNAP displayed a decrease in the time to stop responding to food (p = 0.002; t₍₆₎ = 5.44; 2-tailed paired t tests). There was also a significant difference between the animals receiving SNAP and seawater in the percentage of change in response (p = 0.005; t₍₁₁₎ = 3.44; 2-tailed t test). B, There was no significant decrease in the time that food was within the mouth during the first 5 min of a session between the training and testing session for the control animals (p = 0.50; t₍₄₎ = 0.75). However, animals treated with SNAP showed significant savings using this parameter (p < 0.001; t₍₇₎ = 16.69; 2-tailed paired t tests). There was also a significant difference in the percentage of change in response between the animals receiving SNAP and seawater (p = 0.007; t₍₁₁₎ = 3.24; 2-tailed t test).

Block of NO signaling also affects memory after spaced training

A single training session continued until animals stop responding to food induces short-term memory, which is measured 0.5hr after training, and long-term memory is measured after 24 hr.However, from 1-12 hr after training, no memory is exhibited (Botzeret al., 1998). Intermediate-term memory that is measured 4 hrafter training can be elicited as a result of a spaced trainingprocedure.

L-NAME before training blocks intermediate-term memory
The findings that L-NAME injected before training blocks short- and long-term memory raised the possibility that this procedurealso blocks intermediate-term memory. This possibility was examinedby treating animals (A. californica) with either L-NAME or seawater10 min before the start of spaced training, which consisted ofthree short training sessions of 5 min each. The three sessionswere separated by 0.5 hr intervals. During these three intervals,the time that food spent in the mouth was measured. Four hoursafter the third session, the animals were tested by allowing themto attempt to eat inedible food until they stopped responding(Fig. 12).

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Figure 12. Effects of L-NAME using spaced training. A, Animals were trained with three 5 min training sessions after being treated with artificial seawater (n = 7) or L-NAME (n = 8). For each of the three training sessions, the time that food was in the mouth was measured. Note that the data shown preceded the test of intermediate memory shown in B. Data on spaced training preceding long-term memory were similar to those shown (see Results). B, Four hours after spaced training, animals were retrained in a single session until they stopped responding to food. The three groups whose data are shown with shaded bars were tested in a blind procedure (for Naive; n = 7). Animals treated with L-NAME showed no memory, whereas memory was seen in seawater-treated controls. C, In a separate population of animals that received spaced training, memory was examined 24 hr after the training. Data on retention were gathered in a blind procedure, with n = 6 naive animals. Animals treated with L-NAME (n = 6) showed no memory, whereas memory was seen in seawater-treated controls (n = 6).

In the control, seawater-treated animals, there was a progressive decrease in the time that food spent in the mouth over thethree training sessions (p < 0.001; F_(2,18) = 10.64). In contrast,there was no significant change in this parameter over the threesessions in animals that had been injected with L-NAME (p = 0.55;F_(2,21) = 0.61; one-way ANOVA) (Fig. 12A). These data suggest thatthe effects of the L-NAME treatment were still present for >1hr after the treatment, when animals received the third trainingsession.
Four hours after the training (Fig. 12B), animals that had been treated with L-NAME displayed significant increases in responsivenessto food (time spent in mouth at the start of training, p < 0.001;t₍₁₄₎ = 7.45) and also took significantly longer to stop respondingto the netted food (time to stop responding, p < 0.001, t₍₁₄₎= 6.26; two-tailed t tests) than did animals that were treatedwith seawater. Values of animals treated with L-NAME were similarto those in naive, untreated animals. These data indicate that,in addition to blocking short- and long-term memories, L-NAMEalso blocks intermediate-termmemory.

L-NAME before training blocks long-term memory after spaced training
Previous studies in the honeybee have shown that both massed and spaced training cause long-term memory processes, but theseprocesses are separable by blocking NO signaling during training.Such a block specifically interferes with long-term memory afterspaced training but not after massed training (Müller, 1996).The effects of spaced training on long-term memory after learningthat a food is inedible in Aplysia have not been examined previously.To examine whether long-term memory after spaced training thatfood is inedible is also sensitive to L-NAME, animals (A. fasciata)were trained as above with three 5 min training sessions. Thesessions were separated by 0.5 hr. Memory was examined 24 hr afterthe training (Fig. 12C).
As in the above experiment, animals in which seawater was injected before spaced training displayed a progressive decreasein the time that food spent in the mouth over the three trainingsessions (p < 0.001; F_(2,15) = 10.61). In contrast, there wasno significant change in this parameter in animals that were treatedwith L-NAME (p = 0.42; F_(2,15) = 0.98; one-way ANOVA; data notshown). Twenty-four hours after the training, there was a significantincrease in the scores of the animals that had been treated withL-NAME with respect to the values observed in the seawater-treatedanimals (for the time to stop responding, p < 0.001, t₍₁₀₎ = 5.82;for time in the mouth, p = 0.002, t₍₁₀₎ = 4.15; two-tailed t tests).Values of animals treated with L-NAME were similar to those innaive, untrained animals. These data indicate that L-NAME blockslong-term memory after spaced training, as it does after a singletraining until the animals stopresponding.

L-NAME before training partially blocks very short-term memory

Previous data (Botzer et al., 1998) have identified four separable memory processes after the training that food is inedible.The data above showed that three of these processes, short-, intermediate-,and long-term memories, are blocked by injecting L-NAME into Aplysia.It was of interest to examine whether the fourth form of memory,previously termed very short-term, is also affected. This memoryis displayed during the initial training itself. When animalsare trained with inedible food, their responses during the first5 min of training are more vigorous than during the second 5 min.However, allowing animals 15 min of rest after a 5 min trainingleads to a recovery of responsiveness. Thus, a 5 min trainingleads to a very short-term memory that decays within 15 min. Thismemory can be assessed by comparing the responsiveness in successiveperiods during the initial training to stop responding to inediblefood. To examine the effects of the very short-term memory, weexamined the data on the initial training session in animals thatwere treated with either L-NAME or seawater. It is important tonote that the time to stop responding is not significantly affectedby L-NAME (Fig. 3C), and the responsiveness to food at the startof training is not affected by L-NAME (Fig, 3A,B). The presentanalysis was designed to determine whether animals treated withL-NAME are more responsive to food during the latter portion ofa training session, despite a similar time to stop and despitesimilar responsiveness at the start oftraining.

In this analysis, for each animal (A. fasciata), the data were divided into 5 min intervals, and the percentage of the 5 minthat food was in the mouth was calculated (Fig. 13). We then determinedwhether there was a significant change in the percentage of timespent in the mouth over the first three 5 min intervals, whetherthere were significant differences between L-NAME- and seawater-treatedanimals, and whether there was a significant interaction betweenthese variables.

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Figure 13. Effects of L-NAME on very short-term memory. Very short-term memory was measured by comparing the percentage of time that food was spent in the mouth over three successive 5 min periods during the initial training. Normalized data were used in this experiment, because some animals (4 of 16 L-NAME-treated and 3 of 14 seawater-treated) reached the criterion to stop responding to the food before the end of the 15 min. To compensate, the time that food was in the mouth during each 5 min period was normalized by dividing it by the total number of minutes that the animals responded to food during the 5 min period (the full 5 min for all animals during the first and second 5 min periods as well as for all animals that also responded throughout the third 5 min period; for animals that stopped during the last 5 min period, the time in the mouth was divided by the time during this period that had already gone by before the experiment was stopped).

There was a significant decrease in the responsiveness of the animals over the training period, as measured by the percentageof time that food was in the mouth (p < 0.001; F_(1,26) = 141.57).There was also a significant difference between animals treatedwith L-NAME and with seawater (p < 0.001; F_(1,26) = 156.68). Therewas also a significant interaction between these variables (p= 0.001; F_(1,26) = 14.87; two-way ANOVA with repeatedmeasures).

The data above indicated that animals treated with L-NAME are more responsive than are animals treated with seawater duringthe latter portion of the training. To quantify this difference,the time that food was in the mouth was calculated for all animalsfrom the period 5-15 min after the start of training. For animalstreated with L-NAME, food was in the mouth for 28.6% (SD, 16.9%)of the time, whereas for seawater-treated animals, food was inthe mouth for 16.6% (SD, 11.3%) of the time (p = 0.03; t₍₂₈₎ =2.26; two-tailed t test). These data confirm that animals treatedwith L-NAME are more responsive to food in the latter portionof training than are the seawater-treated controls. This findingis consistent with the idea that the decrease in responses duringthe latter part of training represents a form of very short-termmemory, and this memory is affected by L-NAME. It is importantto note that L-NAME did not completely block the very short-termmemory but, rather, significantly weakened it, as shown by thesignificant interaction between the treatments and the successiveperiods and by the fact that the response of L-NAME-treated animalsdid decrease during the training. Thus, some component of veryshort-term memory is not dependent on a process blocked by L-NAME.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Treatment with L-NAME before training that food is inedible but not after training blocked the expression of short-, intermediate-,and long-term memories and also attenuated very short-term memorywithout completely blocking it. L-NAME had little effect on feedingbehavior per se or on the initial training. Thus, L-NAME doesnot cause pervasive modulation or poisoning of feeding and otherbehaviors. L-NAME interfered with memory because it is a competitiveinhibitor of L-arginine, a substrate of Nitric Oxide Synthase(NOS). Treatment with D-NAME, the enantiomer of L-NAME that doesnot interact with NOS, did not affect short-term or long-termmemory. In addition, long-term memory was blocked by PTIO, anNO scavenger. Finally, long-term memory was restored in L-NAMEtreated animals by SNAP, a releaser ofNO.

Timing of NO modulation

Inedible netted foods elicit a mixture of feeding movements. It is unlikely that memory formation depends on NO release contingentto a particular type of movement or to a particular time duringtraining, because SNAP would cause an increase in NO throughouttraining. NO is unlikely to function as a reinforcer that mustbe timed to the success or failure of a particular bite or a swallowand is likely to function as a modulator allowing reinforcingstimuli to beeffective.

Different effects of NO blocking and gut denervation

Aplysia feeding is initiated, organized, and effected by circuitry within the buccal and cerebral ganglia (Kupfermann, 1974),which contain few NOS-containing somata but contain many NOS-positiveneurites (Jacklet and Gruhn, 1994; Meulemans et al., 1995; Moroz,2000; Jacklet and Koh, 2001). Some neurites may be processes ofperipheral neurons, perhaps from lip chemoreceptors, which areNOS-positive in other gastropods (Elphick et al., 1995; Moroz,2000), or from the gut, which contains many peripheral neurons(Schwarz and Susswein, 1986). If the block of memory arising fromblocking NO has its origin in the block of transmission from thegut, denervating the gut and blocking NO should have similareffects.

Gut denervation (Schwarz and Susswein, 1986) and blocking of NO signaling (Fig. 6) are similar in that both interfere withlong-term memory when performed before training but not after(Schwarz et al., 1991) (Fig. 7). However, gut denervation andNO blocking differ in their effects on the initial learning. Gutdenervation blocks the initial learning, as shown by a lengthenedtraining session, with little decrease in responsiveness beforeanimals stop responding. This pattern is explained by sensoryadaptation or habituation arising from sustained lip stimulation(Schwarz and Susswein, 1986). These studies suggested that gutstimuli provide reinforcement for learning (Schwarz and Susswein,1986). This suggestion was strengthened by evidence that electricalstimulation of the esophageal nerves innervating the gut is areinforcer in a neural analog of learning (Nargeot et al., 1997)and in feeding of intact animals (Brembs et al., 2002). In contrast,blocking of NO signaling causes no change in the time to stopresponding and maintains the graded decrease in feeding responses(although the decrease is less pronounced) (Fig. 13). These differencessuggest that blocking of NO and gut denervation affect learningand memory via different pathways and are consistent with thesuggestion above that block of NO does not block reinforcement.However, we cannot eliminate the possibility that cutting theesophageal nerve interrupts axons in addition to those using NOas a transmitter, and the additional neurons account for the behavioraldifferences.

Different effects of NO blocking and isolation

Isolation from conspecifics also affects learning and memory that food is inedible in A. fasciata (Schwarz and Susswein, 1992;Schwarz et al., 1998). Isolation affects many aspects of feedingand other behaviors (Blumberg and Susswein, 1998; Blumberg etal., 1998) in a manner suggesting that isolation is a stressfulstimulus in Aplysia (Schwarz et al., 1998), as it is in otheranimals (Boissy and Le Neindre, 1997). Stress can modulate learningand memory (Schacter, 1996), and it has been proposed that theeffects of isolation on learning that a food is inedible are explainedby such modulation (Schwarz et al., 1998). The beh