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Previous Article | Next Article
The Journal of Neuroscience, September 15, 2002, 22(18):7892-7902
Regulation of Synaptic Plasticity Genes during Consolidation of Fear Conditioning
Kerry J. Ressler, Gayla Paschall, Xiao-liu Zhou, and Michael Davis Department of Psychiatry and Behavioral Sciences, Center for Behavioral Neuroscience, Emory University School of Medicine, Atlanta, Georgia 30322
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
In mammals, long-term memory induced by Pavlovian fear conditioning has been shown to be dependent on the amygdala during a protein and mRNA synthesis-dependent phase of memory consolidation. We have used genes identified in a kainic acid model of synaptic plasticity as in situ hybridization probes during the consolidation period after fear conditioning. We found that these genes were transcriptionally regulated in several brain areas only when stimuli were presented in a manner that supported behavioral learning and not after unpaired presentations or footshocks alone. Immediate early genes and neurofilament mRNA peaked ~30 min after conditioning, as expected. Interestingly, nurr-1,
-actinin, and 16c8 increased ~2-4 hr later, whereas neurogranin and gephyrin decreased during that time. Our results suggest that fear memory consolidation occurs within a broad neural circuit that includes, but is not limited to, the amygdala. Together, a broad array of transcriptionally regulated genes, encoding transcription factors, cytoskeletal proteins, adhesion molecules, and receptor stabilization molecules, appear to mediate the neural plasticity underlying specific forms of long-term memory in mammals.
Key words: fear conditioning; learning; consolidation; synaptic plasticity; startle; amygdala
INTRODUCTION
The early, middle, and late temporal phases of memory formation have been well described in invertebrates (Bailey et al., 1996
; Dubnau and Tully, 1998
Pavlovian fear conditioning has provided an excellent model system to study learning that occurs in a very short time frame, so that the temporal relationship between sensory stimuli can be tightly controlled (Davis; 1992
Although most studies of gene expression involved in fear conditioning have focused on single genes and generally limited time courses after learning (Campeau et al., 1991
MATERIALS AND METHODS
Animals
A total of 78 adult male Sprague Dawley rats (Charles River, Raleigh, NC) weighing between 300 and 400 gm were used. Animals were housed in group cages of four rats each in a temperature (24°C)-controlled animal colony, had ad libitum access to food and water, and were maintained on a 12 hr light/dark cycle. All behavioral procedures took place during the light cycle and were approved by the Institutional Animal Care and Use Committee.Kainic acid treatment
Methods were as described previously (Crispino et al., 1998General behavioral procedures
Animals were trained and tested in identical cages suspended between compression springs within a ventilated, sound-attenuated chamber as described previously (Cassella and Davis, 1986Fear conditioning
Animals were pre-exposed to handling and placement in the training/testing chamber for 5 d before fear conditioning. During pre-exposure, baseline startle was measured on each of 2 d by presenting 30 startle stimuli at a 30 sec interstimulus interval (ISI). Animals were then divided into matched groups having equivalent baseline mean startle amplitudes. On the day of fear conditioning, the animal was brought to the room, allowed to habituate, and placed in the chamber as before. The CS-US pairing began after a 5 min acclimation period in the chamber. Experiment 1. In the light-shock paired group, 15 light-shock pairings were given with an average intertrial interval (ITI) of 2 min (range, 1-3 min), creating a 30 min training period. The shock (US) was delivered during the last 0.5 sec and coterminated with the 4 sec light (CS). The context control group was placed in the chamber as on the previous days for 30 min also, but no stimuli were given. Two cohorts of animals were processed for experiment 1, with a total of 15 animals kept for behavioral testing 24 hr later and 21 animals killed at different time points. Experiment 2. In the light-shock paired group, 10 light-shock pairings were given with an average ITI of 4 min (range, 3-5 min), over a 40 min training session. The shock (US) was delivered during the last 0.5 sec of the 4 sec light (CS). The unpaired light-shock group received 10 light, 10 odor, and 10 shock stimuli, in a pseudorandom order, with an average ITI of 1.5 min (range, 1-2 min), such that there was no overlap between any stimuli, over a 40 min training session. The shock-only group received 10 shocks, which each lasted 0.5 sec, with an average ITI of 4 min (range, 3-5 min), over a 40 min training session. Animals from all groups (n = 14 total) were returned after training to their home cage and were killed 2 hr later. Experiment 3. In the odor-shock paired group, five odor-shock pairings were given with an average ITI of 4 min (range, 3-5 min), creating a 20 min training session. The shock (US) was delivered during the last 0.5 sec of the 4 sec odor (CS). The unpaired odor-shock group was placed in the chamber and separately given five shock stimuli and five odor stimuli, with a 2 min ITI (range, 1-3 min), so that there was no overlap between stimuli. The context control group was placed in the chamber for 20 min without stimuli. Eight animals were kept for behavioral testing 24 hr later, and 12 animals were killed at different time points for in situ analysis. Behavioral testing. Twenty-four hours after fear conditioning, rats were returned to the test chamber for testing for fear-potentiated startle. In experiment 1, 30 initial startle stimuli were presented in darkness at a 30 sec ISI (leader stimuli), followed by 30 startle stimuli presented in darkness (startle alone) and 30 startle stimuli presented 3.5 sec after onset of the 4 sec light (light startle) in a balanced, pseudorandom order at a 30 sec ISI. During the testing for experiment 3, 30 leader stimuli were followed by a total of 40 startle stimuli presented at a 30 sec ISI. The first of every four startle stimuli was presented 3.5 sec after the onset of the 4 sec odor stimulus. The following three stimuli were presented without odor, allowing for the comparison of odor-startle versus startle-alone stimuli within the same session. Startle amplitude was averaged over all of the startle-alone or light-/odor-startle stimuli within the test session. Data are presented as the absolute level of startle and as a percentage of fear-potentiated startle [100 × (startle amplitude on light or odor startlestartle-alone trials)/startle-alone trials]. Statistical comparisons were made with ANOVA, paired, two-tailed t tests (within-group comparisons) or t tests for independent samples (between-group comparisons).
Preparation of clones and in situ hybridization
cDNA clones of c-fos and corticotrophin-releasing factor (CRF) genes were obtained as indicated. All other genes analyzed were obtained as follows: The rat coding sequence for a gene of interest [obtained from the KA plasticity data (Nedivi et al., 199390% homologous with rat coding sequence as determined by NCBI BLAST.
Animals were given a lethal dose of anesthetic (100 mg/kg Nembutal, i.p.) at various time points after fear conditioning and were perfused with 4% paraformaldehyde in PBS. After overnight fixation, brains were rinsed with PBS and allowed to equilibrate at 4°C in 20% sucrose in PBS. Brains were rapidly frozen in crushed dry ice and stored at
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Table 1. Synaptic plasticity gene expression after kainic acid and fear conditioning
RESULTS
Kainic acid induction of synaptic plasticity genes
Subtractive hybridization screens have described genes previously that are specifically induced in the hippocampus during the neural plasticity phase after KA-induced seizures (Nedivi et al., 1993
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Figure 1. In situ hybridization analyses of genes after kainic acid induction. Magnified bright-field images are shown of hippocampal sections that have been hybridized with 35S-labeled antisense riboprobe and exposed to autoradiography film. The brains were from rats that were treated with either saline (A-H) or kainic acid (a-h) and perfused 6 hr later (A, a, c-fos; B, b, zif268; C, c, neurofilament-light chain; D, d, 16c8; E, e, Rheb2; F, f, cAMP responsive element modulator; G, g, RC3/neurogranin; H, h, gephyrin).
Expression of plasticity genes after light-shock associative learning
We initially tested whether we could simply detect differences in plasticity-associated gene expression after fear conditioning versus placement in the context alone without fear conditioning. This would allow us to determine the time course and extent of gene expression change for later, more comprehensive behavioral studies.
Animals were trained and tested as illustrated in Figure 2A. On the training day, animals received 15 light-shock pairings given over a 30 min period (light-shock pairing) or no new stimuli (context control) and were returned to the home cage. They were killed at several different time points (0, 1, 4, or 8 hr after training; n = 21 total) or were tested 24 hr later for the presence of fear-potentiated startle (n = 15 total) (Fig. 2A). Animals that had experienced light-shock pairings showed significant fear-potentiated startle as demonstrated by a 60% increase in the acoustic startle reflex in the presence of light (Fig. 2B; Light-Startle vs Startle alone; p < 0.05). Animals that had been placed in the context on the day of training but did not receive light-shock pairing showed no appreciable difference between startle in the presence or absence of light, and their difference scores were significantly different from the trained group (t test; p < 0.05).
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Figure 2. Associative light-shock and odor-shock pairings produce stable fear memory. A, Rats (n = 36) were pre-exposed to handling and the experimental chamber for 5 d. They were then exposed to 15 light-shock pairings over a 30 min period or were simply placed back in the chamber without stimuli for 30 min (Context Control). Animals were killed at time points after fear conditioning or were tested 24 hr later for the presence of fear-potentiated startle. B, Behavioral testing of the remaining animals from A. Mean amplitude ± SEM of startle response is shown on the left axis for startle presentations in the absence (Startle alone) or presence (Light-Startle) of a 4 sec light. The percentage increase (% potentiated startle ± SEM) is indicated by the black bars (scale to the right) for the light-shock paired difference versus the context control difference (*p < 0.05 between these groups). C, Rats (n = 20) were pre-exposed as in A. They were then exposed to five odor-shock pairings over a 20 min period (Odor-Shock Paired), exposed to five odor and five shock stimuli that were not paired (Odor-Shock Unpaired), or simply placed back in the chamber (Context Control). Animals were then killed or later tested. D, Results of behavioral testing after the odor-shock training experiment in C (*p < 0.05 between these groups).
Gene expression changes during consolidation
Thirteen of the 21 genes tested showed changes in expression after fear conditioning compared with the control condition. Ten of these genes showed robust expression changes (Table 1), primarily in the piriform cortex (PC) and in the medial and basolateral amygdala. Figure 3A illustrates a schematic of the frontal sections analyzed in this experiment. Figure 3B shows examples of peak changes in the temporal lobe seen with the fear-conditioned animals compared with the context control and KA-treated animals. Notice that the direction of change appears to be similar in both the KA and fear-conditioned animals, although to a different extent with different genes. Indicated are regions that show significant change with fear conditioning (Fig. 3B, arrows) as well as regions that did not change with that gene (Fig. 3B, arrowheads).
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Figure 3. Gene expression changes in the temporal lobe after kainic acid or fear conditioning. A, Schematic diagram from Paxinos and Watson (1986)
Figure 4 shows the quantitative time course of expression for a subset of the examined genes. As expected, the immediate early genes (c-fos and zif268) were induced rapidly (0-1 hr) after fear conditioning and returned to baseline within 2 hr (Fig. 4A,C). Genes encoding some structural proteins [e.g., neurofilament-light chain (NF-l)] also peaked early (Fig. 4B), but other genes, including NMDA receptor (NMDAR) stabilization protein and
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Figure 4. Temporal changes in gene expression after light-shock associative learning. The relative levels of expression of mRNA (in arbitrary units ± SEM) are shown for each of the indicated genes in the indicated region of interest. Levels are shown for the context control at the 1 hr time point compared with the light-shock paired animals that were killed immediately (0 hr) or 1, 4, or 8 hr after the 30 min fear training paradigm described in Figure 2A. PCtx, Piriform cortex; Nf-L, neurofilament-light chain;
Changes in expression of plasticity genes are caused by associative CS-US pairing
The previous experiments suggested that there were temporally and anatomically specific changes in plasticity gene expression after light-shock pairing. However, it was not clear whether the effects were specific to the associative learning process or caused by general activation or other nonspecific effects. To address this, we performed another set of studies with additional animals at a single time point. The time course experiments suggested that the optimal time to observe changes in most of the genes examined is 2 hr after the fear-conditioning procedure (Fig. 4 and our unpublished results). Therefore, after 5 d of habituation to handling and placement in the experimental chamber, animals were subjected to 10 presentations of footshock alone (n = 4), 10 footshocks explicitly unpaired with light (n = 4), or 10 trials in which light and footshock were paired as in the previous experiments (n = 6). Animals were killed 2 hr after the conditioning or control procedure, and brains were prepared for in situ hybridization analysis with the probes described above.
As expected, the immediate early genes had returned to baseline by 2 hr and were not significantly different in their levels of expression from the control groups (data not shown). However, the other genes examined were significant when comparing the paired light-shock group with the footshock alone or with the unpaired CS -US presentations at the 2 hr time point. Figure 5 illustrates changes that were found to be significant with seven of these genes in several different brain areas. NF-l, nurr-1,
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Figure 5. Only associative CS-US pairing alters gene expression. The relative levels of expression of mRNA (in arbitrary units ± SEM) are shown for regions in which there is no change (first region shown) or in regions with significant change for each of the indicated genes. Gene expression was analyzed at the 2 hr time point after light-shock associative learning (Paired Lgt-shk, black bars), unpaired presentations of lights and shocks (Unpaired Lgt-shk, hatched bars), or shock only controls (Shock Only Ctrl, white bars). **p 0.01, *p
Consistent with the previous experiments, RC3/neurogranin and gephyrin were significantly decreased during the same time period (Fig. 5E,G) [RC3 medial amygdala (MeA), F(2,13) = 4, p < 0.05; RC3 piriform cortex, F(2,13) = 4.3, p < 0.05; gephyrin BLA, F(2,13) = 7.2, p < 0.01]. This experiment confirms that at a relatively late time period after the presentation of the paired CS and US, there are significant changes in the expression level of genes that may be involved in the long-term storage of conditioned fear memory. These changes occur only if the animals experience the pairing of lights and shocks and not if they receive shocks alone or the same number of lights and shocks in an unpaired manner.
To rule out the possibility of a general increase in multiple areas as opposed to a specific increase in limited areas, we also examined expression levels in regions that showed a basal level of expression that did not seem to change after fear conditioning. The first region shown with each of the genes in Figure 5 illustrates these data. In each of these regions (hypothalamus, thalamus, hippocampus, and perirhinal cortex), no significant change was seen in level of expression with the gene indicated, although significant changes may be seen in some of these areas with other genes. This demonstrates that the increases or decreases in expression described were specific for the time of expression, gene, and region of interest.
Gene expression changes with odor-shock associative learning
The previous experiment suggests that the association between light and shock led to the gene expression changes observed. To rule out the possibility that these findings were related to sensory modality or to the possible aversive properties of light itself, we examined the expression of the same 21 genes during the consolidation phase of an odor-shock training paradigm after paired and unpaired odor-shock presentations. We have shown previously that after only a small number of training trials, a neutral odor paired with mild footshock leads to robust fear conditioning (Paschall and Davis, 2002
In situ hybridization revealed that the set of genes induced with odor-shock pairing was similar to that induced with light-shock pairing. In most cases, gene expression at 2 hr after unpaired odor-shock presentation was indistinguishable from the context control condition (t tests; p > 0.5). Furthermore, the time course of induction of the genes that showed robust changes with light-shock pairing was similar to the time course of induction after odor-shock pairing. Again, the immediate early genes (c-fos and zif268) and NF-l showed rapid increases in gene expression at the first time point examined (30 min). nurr-1 and
Plasticity gene expression changes occur in unexpected brain areas
From studies of immediate early genes in fear conditioning and evidence from amygdala inactivation, we expected to find changes in synaptic plasticity genes within the basolateral amygdala complex. However, we also found that these and other genes examined showed significant changes in expression in several nonamygdala areas. Figure 3B illustrates that many of the genes examined showed learning-induced changes within the piriform cortex in addition to the neighboring amygdala. Figure 6A shows the time-dependent changes of c-fos and nurr-1 expression in the associative somatosensory, perirhinal, and insular cortices along with the endopiriform nucleus (see Fig. 3A for schematic). These are areas that project extensively to the amygdala, suggesting that much of the synaptic plasticity during the consolidation phase of fear conditioning may occur in the afferent neurons presynaptic to the amygdala.
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Figure 6. Gene expression changes in the cortex and habenula with fear conditioning. A, Pseudocolor images of in situ hybridization with the genes indicated in the associative somatosensory (S2), parietal, perirhinal, and insular cortices as outlined in Figure 3A by the blue box. The color palette is the same as in Figure 3B, with black showing no signal, blue showing the least mRNA expression, and yellow to white showing the most mRNA expression. Sections are shown after in situ hybridization with the indicated genes for the context (ctxt) and unpaired controls and at 30 min and 2, 4, and 8 hr time points after odor-shock pairing. B, Pseudocolor images as in A from the habenula as outlined in Figure 3A by the green box. C, Pseudocolor images as in A from the caudate (act) or hippocampus (nurr) showing that
Another area found to have extensive levels of synaptic plasticity gene induction is the habenula. Figure 6B illustrates the time-dependent changes in expression of c-fos,
Figure 6C illustrates that
For all described experiments, sections of brains from two regions were examined. Anteriorly, brain regions examined were in coronal sections containing the anterior commissure and included areas of frontal and piriform cortices, septum, hypothalamus, striatum, and bed nucleus of stria terminalis. Posteriorly, the coronal sections were focused on the amygdala, including the centromedial, basolateral, and cortical nuclei, hypothalamus, thalamus, hippocampus, habenula and parietal, insular, perirhinal, and piriform cortices (the posterior region is that schematized in Fig. 3A). Table 2 describes the brain regions in which altered gene expression was found. This suggests that plasticity after fear conditioning may depend on a broader neural circuit that includes, but is not limited to, the amygdala.
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Table 2. Synaptic plasticity genes are induced in a distributed neuronal circuitry
DISCUSSION
These studies demonstrate that several genes appear to be regulated at the level of transcription during the consolidation phase of fear memory formation. Twenty-one KA-inducible genes were characterized during the consolidation phase after the presentation of CS-US pairings. These changes in gene expression were shown to occur only when the CS and US were associatively paired, not after US alone or unpaired US presentations. Furthermore, we found that fear conditioning using an olfactory CS activated a similar set of genes in similar areas as fear conditioning using a visual CS. This suggests that the findings are related to the process of associative learning rather than because of the particular CS modality or the US alone. The gene expression changes described occurred with different time courses (Fig. 7A). The IEGs and neurofilament were induced early and decayed within 1-2 hr after fear learning. Genes encoding other transcription factors, structural proteins, and receptor-associated proteins were expressed in similar areas as the IEGs but with later and longer-lasting time courses. Genes whose products are thought to exert a negative regulatory role on neuronal excitability (RC3/neurogranin and gephyrin) showed decreased expression but in a similar temporally restricted manner. Thus, fear conditioning may involve the early and late expression of genes involved in different aspects of the structural and functional plasticity that contributes to LTM formation (schematized in Fig. 7B).
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Figure 7. Summary of time course and possible function of gene regulation during the consolidation period of fear conditioning. A, Schematized time courses of the more robust changes in gene expression after fear conditioning in several brain regions, including the amygdala and areas afferent to it. The line graphs represent the percentage of maximal expression (normalized to 100% for each gene) from the odor-shock experiments (0 = context control at 30 min and 2, 4, and 8 hr after conditioning). The top graph represents the genes that show rapid early increases in gene expression. The middle graph represents the genes that show a more delayed and sustained increase. The bottom graph represents the two genes that have a prolonged decrease in expression after fear conditioning. B, The putative cellular location and function of these gene products based on current literature. NMDA R, NMDA receptor; GABA R, GABA receptor; Gly R, glycine receptor; Ca/Calm, calcium/calmodulin; immed-early, immediate early.
Function of transcriptionally regulated genes during consolidation
The genes chosen for this screen were identified previously with the KA model of neuronal plasticity. It is surprising that a large number of these genes are temporally and spatially regulated after fear learning, a much more limited and behaviorally relevant form of synaptic plasticity. The majority of evidence for early transcription regulation after learning has involved invertebrate studies and in vitro studies of long-term potentiation (LTP) (Nguyen et al., 1994
NF-l is transcriptionally induced rapidly after associative fear conditioning. Its transcription is regulated by protein kinase A, and it contains a CREB-binding site in its promoter (White et al., 1997
nurr-1 is a nuclear transcription factor that is involved in regulation of the dopaminergic phenotype (Saucedo-Cardenas et al., 1997
We found temporal regulation of several genes encoding molecules involved in ECM reorganization. The protease inhibitor 16c8 has been shown to be dynamically regulated with neural plasticity and cell growth (Edwards et al., 1986
Two of the genes we examined were actively inhibited with both KA plasticity and after fear learning. RC3/neurogranin is a cytosolic protein that appears to negatively regulate calcium-calmodulin (Ca/Cam)-dependent learning (Pak et al., 2000
Function of brain areas involved in the consolidation of fear
We have demonstrated that multiple brain areas, primarily the amygdala and regions afferent or efferent to it, show significant changes in gene expression during fear consolidation. We have attempted to prove that these expression changes, although complex, are limited in terms of genes, time courses, and regions of interest. Figures 3, 5, and 6 illustrate that there are also regions with basal levels of expression of a gene that do not show temporal changes during fear consolidation. Thus, we believe that the reproducible changes we see with certain genes in certain areas are meaningful and specific for the consolidation of fear learning.
It is generally accepted that the amygdala, specifically the basolateral amygdala, is critically involved in the formation of fear memories (Davis, 1992
Multiple plasticity genes were temporally regulated in the piriform cortex in these experiments. Although the piriform cortex receives a large amount of direct olfactory information, it has also been shown to receive inputs from other cortical areas, and it receives multimodal sensory inputs by way of the lateral amygdala (Pitkanen, 2000
The medial, and to a lesser extent the lateral, habenula were found to have marked changes in gene expression during consolidation (Fig. 6B). The habenula receives inputs from a variety of limbic structures, including the central amygdala, bed nucleus of stria terminalis, septum, and cortical areas (Pitkanen, 2000
Implications for learning and memory
A debate exists within the literature regarding the storage of fear memories. Connectivity and lesion experiments of the BLA have led to the hypothesis that fear memories are stored within the BLA complex (Fanselow and LeDoux, 1999
Our data imply that several genes that have not been implicated previously in fear conditioning are involved in its consolidation. The data also suggest that brain regions not known previously to be involved in this process may be important. Confirmatory studies, such as region-specific inhibition of gene expression or protein function, will need to be performed to definitively conclude the role of these genes and brain areas in the consolidation of fear conditioning. In summary, our data suggest that the early molecular events necessary for consolidation, the post-translational modification and translational regulation of protein products, are supplemented by complex temporal changes in gene expression. Together, these changes mediate both the early and eventually late phases of long-term memory consolidation in mammals.
FOOTNOTES Received Feb. 12, 2002; revised May 24, 2002; accepted July 3, 2002.
This work was supported by National Institute of Mental Health Grants MH 47840 and MH 57250, the Woodruff Foundation, the Science and Technology Center Program (Center for Behavioral Neuroscience) of the National Science Foundation under Agreement IBN-9876754, a Pfizer Postdoctoral Fellowship Award (K.J.R.), and a Rockefeller Brothers Fund Culpeper Scholarship (K.J.R).
Correspondence should be addressed to Kerry J. Ressler, Department of Psychiatry and Behavioral Sciences, Center for Behavioral Neuroscience, Emory University School of Medicine, Atlanta, GA 30322. E-mail: kressle{at}emory.edu.
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