Increased Histone Acetyltransferase and Lysine Acetyltransferase Activity and Biphasic Activation of the ERK/RSK Cascade in Insular Cortex During Novel Taste Learning

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (34)

Citing Articles via Google Scholar

Google Scholar

Articles by Swank, M. W.

Articles by Sweatt, J. D.

Search for Related Content

PubMed

PubMed Citation

Articles by Swank, M. W.

Articles by Sweatt, J. D.

Previous Article  |  Next Article

The Journal of Neuroscience, May 15, 2001, 21(10):3383-3391

Increased Histone Acetyltransferase and Lysine Acetyltransferase Activity and Biphasic Activation of the ERK/RSK Cascade in Insular Cortex During Novel Taste Learning
Michael W. Swank and J. David Sweatt
Division of Neuroscience, Baylor College of Medicine, Houston, Texas 77030

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Changes in gene expression are thought to be involved in neuronal plasticity associated with learning and memory. Althoughacetylation of lysine residues on histones by histone acetyltransferases(HAT) is an obligatory component of transcription, HAT activityhas been largely ignored in studies of the nervous system. Wedeveloped a new model for studying novel taste learning usingnovel solid food presentation to nondeprived animals. Using thisbehavioral paradigm, we investigated short- and long-term regulationof lysine acetyltransferase activity and the ERK/mitogen-activatedprotein kinase (MAPK)/RSK cascade in insular cortex, a CNS regionknown to be crucial for the formation of novel taste memories.We observed that novel taste learning elicited biphasic (acuteand long-lasting) activation of two distinct lysine acetyltransferaseactivities along with the ERK/MAPK cascade in insular cortex.In vitro studies revealed that the ERK cascade could regulatethe lysine acetylation of a 42 kDa lysine acetyltransferase substrate,suggesting a causal relationship between ERK activation and lysineacetyltransferase activity in insular cortex. Overall, our studiesreveal an unanticipated long-lasting activation of insular cortexsignal transduction cascades in novel taste learning. Furthermore,our studies suggest the hypothesis that acute and long-term ERKactivation and lysine-histone acetyltransferase activation mayplay a role in regulating gene expression in single-trial learningand long-term memoryformation.

Key words: MAP kinase; histone acetyltransferase; protein kinase; taste aversion; insular cortex; learning; memory; gene expression

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The association between histone acetylation and transcriptional regulation has been known for many decades (Allfrey et al.,1964), and it is widely recognized that increased histone acetyltransferase(HAT) activity is an obligatory component of transcription (Davieand Spencer, 1999; Spencer and Davie, 1999; Kouzarides, 2000).Although current models suggest that changes in transcriptionalcontrol are necessary for long-term memory formation (Bailey etal., 1996; Impey et al., 1998; Silva et al., 1998; Alberini, 1999;Roberson et al., 1999; Stork and Welzl, 1999), the role of histoneacetylation has not been examined in any learning or memory paradigmtodate.

Novel taste learning presents several unique attributes that make it a compelling model for looking at gene expression duringlong-term memory formation: it is robust, long-lasting, and canoccur after only a single trial (Bures, 1998). These propertiesof novel taste learning suggest the hypothesis that altered geneexpression may be involved in the formation of thememory.

Consistent with this hypothesis, activation of the ERK/mitogen-activated protein (MAP) kinase cascade, a prototype cascadefor regulating gene expression, has been shown to occur afternovel taste experience in the insular cortex, and MAP kinase activationis necessary for novel taste memory formation (Berman et al.,1998). Furthermore, localization of phosphorylated, activatedMAP kinase by immunohistochemistry has further defined the insularcortex as being involved in novel taste learning in mice (Swank,2000a). Although a recent detailed study gave new insight intothe neurotransmitters involved in the upstream regulation of MAPkinase by novel taste (Berman et al., 2000), little work has beendone on mitogen-activated protein kinase (MAPK)-dependent eventsthat lie downstream of this pathway in insularcortex.

With this in mind, it is interesting that recent evidence suggests that MAP kinase is involved in regulation of histone acetylationand chromatin remodeling through the action of downstream effectors(Thomson et al., 1999). For example, one specific effector isthe cAMP response element-binding protein (CREB)-binding protein(CBP), an MAPK substrate with intrinsic histone acetyltransferaseactivity; when phosphorylated by MAP kinase, CBP acetyltransferaseactivity increases (Ait et al., 1999), resulting in increasedtranscription (Martinez-Balbas et al., 1998). Therefore, in thepresent studies, we were interested in evaluating whether histone-lysineacetyltransferase activity is regulated in insular cortex duringsingle-trial novel taste learning. As part of these studies, wealso undertook a characterization of the activation of the Raf/MEK/ERK/RSKcascade in insular cortex after single-trial novel tastelearning.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mice. Male Swiss Webster mice weighing 30-35 gm were housed individually, received ad libitum food and water, and were maintainedon a 12 hr light/dark schedule until training began. All procedureswere in accordance with university and National Institutes ofHealthguidelines.

To test neophobia, mice (n = 3) were given a 10 min access to a preweighed portion of blueberry bar that was then reweighedto measure consumption. On the next day mice were given a second10 min access to blueberry bar that was similarly removed andreweighed. The increase in the amount of food consumed duringthe second exposure was taken as an index of decreased neophobia,an indicator that the mice formed a long-term memory of the noveltaste.

To assess the development of a conditioned taste aversion to blueberry bar, we used a variation of the typical conditionedtaste aversion protocol, adapted to solid food in nondeprivedmice. Mice were randomly assigned to two groups (n = 5) and given10 min access to blueberry bar followed by injection of eitherLiCl or NaCl (0.15 M, 20 ml/kg, i.p.). On the next day, mice weregiven a 10 min access to blueberry bar, and intakes were recorded,with decreased consumption relative to NaCl controls taken asan indicator of conditioned tasteaversion.

Effects of MAP kinase blockade on acquisition of conditioned taste aversion. To test whether a conditioned taste aversionto a solid food is MAP kinase-dependent, as has been shown forsaccharin (Berman et al., 1998), we used the selective MEK inhibitorSL327, a blood-brain barrier-permeant compound which, when givenperipherally, has been shown to block other MAP kinase-dependentforms of learning such as fear conditioning (Atkins et al., 1998)and spatial learning (Selcher et al., 1999). Mice were randomlyassigned to one of four groups: LiCl, DMSO-LiCl, SL327-LiCl, andNaCl (n = 5 per group). Two groups of mice were injected witheither DMSO (0.1 ml, s.c.) or the MEK inhibitor SL327 (a kindgift of Dr. James Trzaskos; DuPont, Billerica, MA; 100 mg/kg in0.1 ml DMSO, s.c.). One hour later DMSO-LiCl and SL327-LiCl mice,along with two uninjected groups (LiCl and NaCl) were given 10min access to blueberry bar. Conditioning intakes were measuredand were not significantly different between groups, indicatingthat neither DMSO nor SL327, when given subcutaneously, suppressesfood intake under these conditions (data not shown). LiCl, DMSO-LiCl,and SL327-LiCl mice were then injected with LiCl (0.15 M; 20 ml/kg,i.p.), and NaCl mice were injected with NaCl (0.15 M; 20 ml/kg,i.p). The next day mice were given a 10 min test access to blueberrybar, and intakes were recorded. Increased intakes in the SL327mice relative to the LiCl-injected mice were taken as an indicatorof attenuation of conditioned tasteaversion.

Slice preparation and ex vivo pharmacological experiments. We developed a method for preparing live slices through insularcortex using a variation of the typical method for preparing hippocampalslices for physiological recordings (Roberson et al., 1999). MaleSwiss Webster mice weighing 30-35 gm were killed by cervical dislocation,and brains were removed rapidly and placed into ice-cold cuttingsolution containing (in mM): 110 sucrose, 60 NaCl, 3 KCl, 1.25NaH₂PO₄, 28 NaHCO₃, 5 D-glucose, 0.5 CaCl₂, 7 MgCl₂, and 0.6 ascorbate,saturated with 95% O₂ and 5% CO₂. The rostral portion of the forebraincontaining insular cortex was mounted on a vibratome stage, and300 µm slices were transferred to ice-cold cutting solution. Sliceswere taken through the insular cortex until the striatum appeared.After equilibration in a 1:1 mix of cutting solution and aCSFcontaining (in mM): 125 NaCl, 2.5 KCl, 1.25 NaH₂PO₄, 25 NaHCO₃,10 D-glucose, 2 CaCl₂, and 1 MgCl₂, saturated with 95% O₂ and5% CO₂ at room temperature for 20 min, slices were then transferredto aCSF for another hour at room temperature. Slices were thentransferred to a 32°C water bath where they were maintained for1 hr. In slices treated with the selective MEK inhibitor U0126(Promega, Madison, WI), the inhibitor was added at the beginningof this incubation. After 1 hr of incubation, slices were treatedwith forskolin (50 µM with 100 µM Ro20-1724, a cAMP phosphodiesteraseinhibitor) for 1 hr. Slices were then removed, frozen on dry ice,and noncortical tissue was dissected away. In experiments to examinehistone acetylation, the histone deacetylase inhibitor trichostatinA (Sigma, St. Louis, MO) was added to a final concentration of500 ng/ml at the beginning of the 32°C incubation; samples werecollected 2 hr later. For all slices, sample preparation for Westernblotting was identical to that describedbelow.

Histone extraction and acid-urea gel electrophoresis. Samples were Dounce-homogenized as described below. The nuclear fractionwas pelleted by centrifugation (18,000 × g; 15 min; 4° C) andthe supernatant was saved for conventional SDS-PAGE. Histoneswere extracted from the nuclear pellet by the addition of fivevolumes 0.2 M HCl and 10% glycerol, and the insoluble fractionwas pelleted by centrifugation (18,000 × g; 30 min; 4° C). Histonesin the acid supernatant were precipitated with 10 volumes of ice-coldacetone followed by centrifugation (18,000 × g; 30 min; 4° C).The histone pellet was then resuspended in 9 M urea, and aliquotswere assayed for total protein by Coomassie assay. $beta$ -mercaptoethanoland acetic acid were added to a final concentration of 5%. Sampleswere resolved on 15% acrylamide acid-urea gels (0.9 M acetic acid,7 M urea) and then transferred to polyvinylidene difluoride (PVDF)membrane and processed for acetylated lysine immunoreactivity.Supernatant samples were processed as described below and assayedfor acetylated lysine immunoreactivity by conventional SDS-PAGEand Western blotting with an antibody to acetylatedlysine.

Novel versus familiar taste time course. Mice were randomly assigned to one of two main groups: novel mice had no previousexposure to the tastant before testing; familiar mice had threeprevious exposures to the food on three successive days followedby 2 d without access to blueberry bar. At all times animals hadad libitum access to water and their usual chow. On test day,mice were given a 10 min access to a preweighed portion of blueberrybar that was then removed and weighed to record intakes. In the"novel" group, one group of mice was not given access to blueberrybar; these mice are the naive controls, and data obtained fromthem are plotted on the zero time point. In the "familiar" group,one group of mice did not receive a fourth access to blueberrybar; these mice represent the familiar control group and are plottedat the 96 hr time point. After consumption and recording of intakes,mice were killed at the following time points: 0.5, 1, 2, 6, 12,24, and 48 hr after consumption (n = 4 per timepoint).

Sample preparation and Western blotting. Mice were killed by cervical dislocation, and brains were removed rapidly and frozenon dry ice. Brains were then dissected on a freezing stage at $-$ 12° C; briefly, a 14 ga punch was used to score a circular groovecentered over the intersection of the middle cerebral artery andrhinal fissure. A 14 ga punch with a notched end was then usedto lift out the cortical punch that fractured at the externalcapsule, leaving behind noncortical tissue. Punches were thenhomogenized in a hypotonic lysis buffer containing 10 mM Tris,pH 7.5, 1 mM EDTA, 2.5 mM sodium pyrophosphate, 1 mM $beta$ -glycerop-hosphate,1 mM sodium orthovanadate, 1 mM phenylmethylsulfonylfluoride,1% protease inhibitor cocktail (Sigma), and 1% Igepal CA-630.Protein concentration was determined by Coomassie assay (Pierce,Rockford, IL), and volumes were adjusted so that all samples were2 µg/µl. SDS-PAGE sample buffer (5×) was added to each sampleand boiled, and 30 µg/lane was loaded onto either 8 or 10% acrylamidegels, depending on the molecular weight of the protein being assayed.Samples were blotted onto PVDF membrane (Immobilon P; Millipore,Bedford, MA), blocked in 5% nonfat dry milk in Tris-buffered salinecontaining 0.05% Tween 20 (TTBS) for 1 hr, and then probed withthe following antibodies (all from Cell Signaling or the parentcompany, New England Biolabs, Beverly, MA): phospho-Raf (Ser259),phospho-MEK1/2 (Ser217/221), phospho-MAPK (Erk1/2) (Thr202/Tyr204),and phospho-p90RSK (Ser381). To examine lysine acetyltransferaseactivity, blots were probed with an antibody to acetylated lysine;this antibody recognizes not only acetylated histones, but otherHAT substrates such as p53 and PCAF when acetylated on $epsilon$ -aminogroups of lysine residues. All antibodies were diluted 1:1000in TTBS and 1% milk and incubated for either 2 hr at room temperatureor overnight at 4°C. Blots were then rinsed for 20 min in TTBS,incubated in HRP-conjugated anti-mouse or anti-rabbit (1:25,000in 1% milk and TTBS), rinsed, incubated in enhanced chemiluminescentsubstrate (SuperSignal Pico; Pierce), and exposed to film (KodakBioMax; Eastman Kodak, Rochester, NY). Films were scanned, anddensitometry performed as described previously (Roberson et al.,1999).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Solid food in nondeprived animals elicits neophobia and supports a conditioned taste aversion

Initial experiments were conducted using nondeprived mice that had ad libitum access to food and water. Mice were given accessto a variety of solid foods, and we found that they consumed variableamounts of such foods as Cheetos (Frito-Lay, Dallas, TX), FrootLoops (Kellogg's, Battle Creek, MI), pizza, and ironically, catfood. Of the extensive number of foods tested, Nutri-Grain (Kellogg's)blueberry breakfast bars were chosen because mice appeared toprefer this over other foods tested (data not shown) and consumedthis novel food even when nonfood-deprived. The availability ofseveral other flavors also makes this food useful for future experimentsdesigned to assess discrimination learning. Because these mice(n = 6) had been exposed to such a wide variety of novel tastes,they were later used to conduct an initial screening of insularcortex for changes in lysine acetylation (seebelow).

Having demonstrated that mice would consume measurable quantities of a novel solid food, we then assessed neophobia, a characteristicreluctance to consume a novel foodstuff, to determine whethermice would form a lasting memory of the novel taste; if so, theywould be expected to consume more on second exposure. We foundthat mice consumed a measurable quantity of blueberry bar duringtheir initial 10 min access and that this first exposure was characterizedby neophobia, as indicated by the observation that intakes werenearly double on the second access, a significant increase (Fig.1A). These data indicate that the mice formed a memory of thenovel taste after their first exposure, and this memory was expressedas an attenuation of neophobia on the second exposure, a resultwhich is in line with other previously described taste learningparadigms (Bures, 1998).

View larger version (14K):
[in this window]
[in a new window]
Figure 1. A, Neophobia during first access to a novel solid food is attenuated on second exposure. Mice were given 10 min access to Nutri-Grain blueberry bar, and intakes were recorded. Ten minute intakes on the second are significantly higher, demonstrating attenuation of neophobia through familiarization. (*p < 0.05 by one-way ANOVA). B, Pairing of solid novel food with LiCl produces a conditioned taste aversion. Mice injected with LiCl after a 10 min access to blueberry bar consume significantly less than NaCl-injected when tested (***p < 0.001 by one-way ANOVA).

Another attribute of taste learning is the ability to form selective robust aversions to a novel taste when it is paired witha malaise-inducing agent such as LiCl. This is a highly adaptiveform of learning that depends critically on the animal's abilityto use the memory of the novel taste so that future encounterswith a toxic and potentially lethal food can be avoided. As expected,test intakes of the novel taste that had been paired with LiClwere significantly suppressed relative to NaCl controls, demonstratingthat the solid food stimulus supports a conditioned taste aversion(Fig. 1B). Along with the demonstration of attenuation of neophobiawith familiarization, this experiment shows clearly that miceacquire a memory of the novel taste and suggests that the useof a novel solid food in nondeprived animals may be a useful toolto study mechanisms involved in novel tastememory.

Conditioned taste aversion to a solid food is MAP kinase-dependent

Because previous reports have shown that novel taste learning (Berman et al., 1998) and development of conditioned taste aversionto saccharin in water-deprived mice are MAP kinase-dependent (Swank,2000b), we wanted to confirm that this signal transduction cascadewas also involved in taste learning using a novel solid food asthe conditioned stimulus during conditioned taste aversion learning.Animals injected with LiCl developed a significant conditionedtaste aversion to the blueberry bar, as shown by the markedlysuppressed intakes relative to NaCl controls (Fig. 2). This wassignificantly attenuated by SL327 but not DMSO vehicle; only theSL327 and NaCl intakes were significantly greater than in LiClmice. These data suggest, as has been documented previously fornovel tastes in solution (Berman et al., 1998, 2000) that MAPkinase plays an important role in encoding a novel taste memoryfor a more complex solid food with additional odor and texturalcues. The lack of complete blockade of conditioned taste aversionwith MAP kinase inhibition is also consistent with previous reportsusing saccharin in solution (Berman et al., 1998).

View larger version (9K):
[in this window]
[in a new window]
Figure 2. Memory for a novel food and acquisition of a conditioned taste aversion is MAPK-dependent. LiCl, LiCl-DMSO, and LiCl-SL327 mice all received 10 min access to blueberry bar followed by injection of LiCl. NaCl mice received NaCl after blueberry bar. SL327 (100 mg/kg, s.c.) injected 1 hr before blueberry bar significantly attenuates conditioned taste aversion, as shown by test intakes. (*p < 0.05 relative to LiCl by ANOVA and Duncan interval).

Regulation of histone acetylation in insular cortex

In our first series of studies we demonstrated not only that mice form a memory for a novel solid food taste, but that thisappears also to be MAP kinase-dependent. In this next phase wefocused on histone acetyltransferase^a activity, an essential component of transcriptionalregulation.

In our first experiment, we sought to confirm the presence of histone acetyltransferase activity in insular cortex. Althoughspecific activators of histone acetyltransferases are not yetavailable, trichostatin A, a potent inhibitor of histone deacetylases(HDAC), has been shown to increase histone acetylation in a numberof systems (Yoshida et al., 1990). We are unaware of any reportsthat have examined its effect in the brain, but we predicted thatit was likely to act in a similar manner in the insular cortex.Not surprisingly, treatment of slices with trichostatin A produceda significant increase in acetylation of histones H4 and H2A,but not H2B or H3 (Fig. 3). However, we also detected three prominentacetylated proteins when we used conventional SDS-PAGE to assaythe supernatant from these samples; given their apparent molecularweights, these proteins are denoted p42AcK, p55AcK, and p70AcK.Lysine acetylation of p55AcK, but not p42AcK and p70AcK, was increasedby trichostatin A. These data suggest that the acetylation stateof p55AcK is regulated by HDAC, and by inference, histone acetyltransferases.These data suggest also that p42AcK and p70AcK are not regulatedby histone acetyltransferases; however, a differential sensitivityto HDAC could account for the lack of altered acetylation in thesetwo proteins. Taken together, our findings in this first experimentdemonstrate the existence of both histone acetyltransferase andlysine acetyltransferase activity in insular cortex, as evidencedby lysine acetylation of several proteins and a regulation ofhistone acetylation by inhibition of histone deacetylases.

View larger version (28K):
[in this window]
[in a new window]
Figure 3. Effect of the histone deacetylase inhibitor trichostatin A on histone and non-nuclear protein acetylation in insular cortex slices. A, Two hour treatment with trichostatin A produced significant increases in acetylation of histones H4, H2A, but not H2B or H3. Acetylation of an unknown protein, termed p55AcK, was also increased by trichostatin A. Acetylation of two other proteins, p42AcK and p70AcK, was not altered by trichostatin A (*p < 0.05, **p < 0.01, ***p < 0.001 relative to controls by one-way ANOVA; y-axis: IOD, integrated optical density, i.e., pixel intensity × area). B, Representative blots showing acetylated lysine immunoreactivity after Western blots of histone extracts (left) or non-nuclear proteins (right).

Positive and negative coupling of two distinct lysine acetylation pathways to the MAP kinase cascade

To continue our investigations we evaluated possible upstream regulators of lysine acetyltransferase and histone acetyltransferaseactivity in insular cortex slices. Given the differences in sensitivityto HDAC inhibitors, we were particularly interested in possibledifferential regulation of p42AcK, p55AcK, and p70AcK. BecauseERK/MAP kinase has been implicated in regulating histone acetyltransferaseactivity in other systems (Ait et al., 1999; Kawahara et al.,1999), we chose to test this pathway first. As a first experiment,we needed to examine ERK/MAPK regulation in insular cortex, andwe hypothesized that PKA might regulate MAPK in insular cortexas it does in hippocampus (Roberson et al., 1999). Presumed activationof PKA by forskolin produced a robust activation of the MAP kinasecascade, as shown by highly significant increases in phosphorylationof both the 42 and 44 kDa isoforms of MAPK (Fig. 4A). Treatmentof slices with the selective MEK inhibitor U0126 not only abolishedthe forskolin response, but also reduced basal phospho-MAPK tolevels undetectable by Western blot (Fig. 4D). These data indicatethat the cAMP cascade regulates MAPK in insular cortex.

View larger version (14K):
[in this window]
[in a new window]
Figure 4. Effects of forskolin activation of PKA on MAPK activation and lysine acetylation. A, Forskolin produces a significant activation of both p42 and p44 isoforms of MAP kinase. The selective MEK inhibitor U0126 completely abolishes phospho-MAPK immunoreactivity (D) and is not plotted here. Two-way ANOVA revealed a significant main effect of forskolin on phosphorylation of both p42ERK (p < 0.001) and p44ERK (p < 0.05); there was also a significant main effect of U0126 (p < 0.001). B, Activation of the MAPK cascade elicits an increase in lysine acetylation of p42AcK that is blocked by U0126. Two-way ANOVA revealed a significant main effect of both forskolin (p < 0.05) and U0126 (p < 0.01). Post hoc Dunnett analysis revealed that forskolin control acetylation was significantly greater than forskolin U0126 (p < 0.05). C, Inhibition of the MAPK cascade by U0126 causes increased acetylation of p55AcK. Two-way ANOVA revealed a significant main effect of U0126 (p < 0.05) but not forskolin. D, Representative Western blots of phospho-MAPK (left) and acetylated lysine (right). Note the complete absence of phospho-MAPK immunoreactivity in U0126 slices.

Our next set of experiments indicated that MAPK can regulate lysine acetyltransferase activity in insular cortex. Acetylationof p42AcK was significantly increased by forskolin-treated insularcortex slices, and this was blocked by the specific MEK inhibitorU0126 (Fig. 4B), demonstrating that acetylation of p42AcK is MAPkinase-dependent. In contrast, acetylation of p55AcK was significantlyincreased by the MEK inhibitor U0126 independent of forskolin,suggesting that the MAP kinase cascade exerts an inhibitory controlover the histone acetyltransferases responsible for acetylationof p55AcK. p70AcK was not affected by any treatment (data notshown). These data, like those obtained after treatment with trichostatinA, suggest a differential regulation of p42- and p55AcK. Importantly,they indicate a positive regulation of a novel lysine acetyltransferaseactivity by the ERK/MAPK cascade in insular cortex and a possiblenegative regulation of histone acetyltransferase activity by theERK/MAPK cascade in the insularcortex.

Previous exposure to novel tastes increases lysine acetylation of p42AcK and p55AcK in insular cortex

We next sought to determine whether novel taste learning is associated with activation of histone acetyltransferase and lysineacetyltransferase in insular cortex. An initial pilot experimentexamined insular cortices of mice that had been exposed to a varietyof novel tastes (see Results), to determine whether novel tastelearning is associated with lysine acetyltransferase activation.Western blots of acutely prepared insular cortex revealed thesame three prominent acetylated proteins of ~42, 55, and 70 kDathat were observed in insular cortex homogenates obtained fromin vitro slice experiments (Fig. 5A). Compared with naive controls,mice that had been used to screen for novel solid food preferencesshowed significant increases in lysine acetylation of p42AcK andp55AcK; p70AcK did not appear to be altered by taste experience(Fig. 5B). These pilot data compelled us to perform the followingcontrolled experiment to compare novel with familiarized tasteat a number of time points after taste exposure.

View larger version (16K):
[in this window]
[in a new window]
Figure 5. Acetylation of a 42 and 55 kDa protein, but not a 70 kDa protein, is altered by previous novel taste exposure. Mice that had been used to screen for solid food preferences were used for an initial screen for lysine acetylation in insular cortex. A, Western blot revealed three prominent acetylated proteins in both novel and naive mice. B, Lysine acetylation of both the 42 and 55 kDa proteins was shown to be increased after several previous exposures to novel foods (p < 0.05 by one-way ANOVA).

A single exposure to a novel taste produces increased lysine acetylation of p42- and p55AcK

A single 10 min exposure to novel taste produced significant increases in lysine acetylation of both p42AcK and p55AcK. (Fig.6A,B). Representative blots are shown in Figure 6C. Given thatthe slice experiments revealed two distinct lysine acetyltransferasepathways responsible for acetylating p42AcK and p55AcK, perhapsnot surprisingly the kinetics of acetylation of these two proteinswere found to be different. p42AcK showed an unusual biphasicresponse: acetylation was significantly increased relative tonaive controls at 1 and 2 hr, then decreased to control levelsfollowed by significant increases at 12, 24, and 48 hr (Fig. 6A).In contrast, p55AcK showed a more prolonged response, with acetylationbeing significantly increased at all time points out to 12 hr,followed by a return to baseline at 24 and 48 hr (Fig. 6B).

View larger version (23K):
[in this window]
[in a new window]
Figure 6. Acetylation of p42AcK (A) and p55AcK (B) after novel and familiar taste. Novel mice were given a single 10 min access to blueberry bar (denoted by arrow at t = 0 hr), and time of killing is indicated by the x-axis. The data point at t = 0 hr represents the control group of naive mice that did not receive novel food. Familiar mice received three previous exposures at 0, 24, and 48 hr (denoted by arrows) followed by an additional 48 hr before the fourth exposure at t = 96 hr. The data point at t = 96 hr represents mice with three previous exposures only and is the control group for the familiar groups. All data are expressed as integrated optical density (area × pixel intensity) normalized to the t = 0 control mice. A, Lysine acetylation of p42AcK shows a biphasic response in the novel group and a persistent increase in the familiar group. Two-way ANOVA showed significant main effects of both group (novel vs familiar; p < 0.01) and time (p < 0.05). Post hoc Dunnett analysis revealed a significant increase in p42AcK acetylation in the novel group at 1, 2, 12, and 24 hr. Relative to t = 96 hr controls, there was no significant change in the familiar group. B, Lysine acetylation of p55AcK. Two-way ANOVA revealed significant effects of both group (novel vs familiar; p < 0.001) and time (p < 0.001). Post hoc Dunnett analysis revealed significant increases in acetylation of p55AcK at all time points up to 12 hr, but not at 24 and 48 hr. There was no significant change in acetylation of the familiar group at any time points relative to t = 96 hr. C, Representative immunoblots showing changes in acetylation of p42AcK and p55AcK. Note that there is no change in the acetylation of p70AcK.

We next sought to determine what effect repeated presentations of the taste stimulus would have on insular cortex lysine acetylation.Similar to the response of p42 and p55AcK acetylation after asingle presentation of novel taste, repeated taste presentation(familiar) elicited significantly elevated lysine acetylationof both p42AcK and p55AcK relative to naive controls (Fig. 6A,B).These data are consistent with our observation that novel tasteelicits lysine acetylation in insular cortex, in that repeatedpresentation of the same stimulus also elicits altered lysineacetylation. Although interpretation of our findings is speculativeat present, these data may also suggest that lysine acetylationis chronically increased when a formerly novel taste has becomefamiliar, i.e., when long-term memory for that taste has beenacquired. In this scenario, the acute response to novel tasteis potentially associated with acquisition and consolidation.However, additional behavioral experiments will be needed to addresstheseissues.

Activation of the MAPK/ERK pathway by novel taste in insular cortex

Given that the in vitro studies described above demonstrated that acetylation of p42AcK is regulated by MAP kinase, we hypothesizedthat increased lysine acetylation of p42AcK was a result of MAPkinase activation in the insular cortex. This hypothesis was especiallyappealing, because MAP kinase activation in the insular cortexhas already been shown after novel taste learning (Berman et al.,1998; Swank, 2000a). Similar to results previously reported usingnovel saccharin in water-deprived rats, the ERK/MAP kinase pathwaywas activated in insular cortex after the novel solid food tastestimulus. Peak phosphorylation of p42 (Fig. 7A) and p44 MAPK (Fig.7B) occurred within 2 and 6 hr, respectively, after novel taste.Phosphorylation then dropped toward baseline at 12 hr, followedby significant increases at 24 and 48 hr. These findings demonstrateMAP kinase activation in insular cortex in response to novel solidfood taste presentation.

View larger version (21K):
[in this window]
[in a new window]
Figure 7. Phosphorylation of p42 and p44 MAP kinase after novel or familiar taste. A, B, Two-way ANOVA revealed significant main effects of both group (novel vs familiar, p < 0.001) and time (p < 0.001) for both MAPK isoforms. A, Post hoc Dunnett analysis of p42ERK revealed significant increases in phosphorylation at 1, 2, 6, 24, and 48 hr. B, p44 MAPK phosphorylation was significantly increased at 2, 6, and 48 hr. A, B, For both MAPK isoforms, phosphorylation was significantly increased at the 144 hr time point; this is 48 hr after the fourth and final exposure to the now-familiar taste. C, Total MAPK levels are unchanged in both the novel and familiar groups for both MAPK isoforms. Normalized p42 values are plotted against the left y-axis, and p44 values against the right y-axis. Two-way ANOVA revealed that there was no significant effect of either group (novel vs familiar) or time. D, E, Representative immunoblots showing phospho-MAPK and total MAPK, respectively.

Similar to the response to the novel taste, there was a significant increase, relative to naive controls, in phosphorylationof both p42 and p44 MAPK at all time points after repeated exposureto the taste, i.e., taste familiarization. However, there wasno significant additional increase in MAPK phosphorylation witha fourth exposure. These data suggest that once the mice haveretained a long-term memory of the novel taste, the now-familiartaste elicits minimal additional changes in MAPK activation. However,overall levels of MAP kinase phosphorylation in familiarized animalswere significantly increased relative to naive controls, suggestingthat persistent activation of MAPK is associated withretention.

The kinetics of MAPK phosphorylation after both single and repeated exposures to a novel taste are similar to the acetylationof p42AcK. In both cases, a single novel taste produces a biphasicactivation; the effect of repeated presentation leading to familiarizationis to elicit increased activity that it not significantly alteredby additional exposure to a familiar taste. Taken together withthe in vitro insular cortex slice experiments, these data areconsistent with the hypothesis that acetylation in vivo of p42AcKmay be regulated by MAP kinase. Additional future experimentsin vivo will be necessary to test this hypothesisdirectly.

Equally important, our data indicate an interesting long-term regulation of ERK/MAPK in insular cortex after novel taste exposure.In the next series of experiments, we sought to gain some insightinto the basis for this long-lasting activation of ERK/MAPK.

Changes in phospho-MAPK are not attributable to an increase in total MAPK

Although phospho-MAPK levels changed dramatically across the different groups, total MAPK levels were not significantly alteredby either single or repeated presentations of novel food at anytime point (Fig. 7C). These data demonstrate that the increasesin MAPK phosphorylation seen here are not attributable to changesin the total amount ofMAPK.

Activation of the entire ERK/MAPK cascade by novel taste

Regulation of ERK/MAPK activity is complex, and there are several upstream activators. We sought to determine whether thetwo upstream regulators of MAPK in the canonical MAPK cascade,MEK and Raf, were also activated in insular cortex during noveltaste learning. Both are positively regulated by phosphorylation,and inferred activity can, like MAPK, be measured by Western blotswith phosphospecificantibodies.

Phosphorylation of MEK showed similar kinetics to that of MAP kinase. In the novel group, phospho-MEK was significantly increasedat 1 and 2 hr, declined, and was then significantly increasedat 24 and 48 hr. Repeated taste presentation also produced overallsignificant increases in phospho-MEK relative to the naive controls,but again, as with MAPK, additional presentations did not elicitany further increases in MEK phosphorylation relative to the familiarcontrol (t = 96 hr) (Fig. 8A).

View larger version (19K):
[in this window]
[in a new window]
Figure 8. Phosphorylation of MAP kinase cascade elements MEK, Raf, and p90 RSK. A, phospho-MEK shows a biphasic response. Two-way ANOVA revealed a significant main effect of both group (novel vs familiar; p < 0.001) and time (p < 0.001). Post hoc Dunnett analysis revealed significant increases in phospho-MEK at 1, 2, 24, and 48 hr in the novel group but no significant effect of time in the familiar group. B, Phosphorylation of Raf does not show the biphasic response seen with p42AcK and phospho-MAPK. Two-way ANOVA revealed a significant main effect of both group (novel vs familiar; p < 0.05) and time (p < 0.001). phospho-Raf was significantly increased at 0.5, 1, 2, 6, and 12 hr, but then declined to baseline at 24 and 48 hr. Within the familiar group, phospho-Raf levels at t = 144 hr (48 hr after the fourth taste exposure) were significantly depressed relative to the t = 96 hr control. C, phospho-p90RSK also shows a biphasic response to novel taste. Two-way ANOVA revealed significant main effects of both group (novel vs familiar; p < 0.001) and time (p < 0.001). Within the novel group, phosphorylation was significantly increased at all time points, although the plot shows the characteristic biphasic response. As with other members of the MAPK cascade, there was no significant effect of time within the familiar group. D, Representative immunoblots showing phospho-MEK, phospho-Raf, and phospho-p90RSK immunoreactivity.

Raf is an upstream activator of MEK that is also positively regulated by phosphorylation. The kinetics of Raf phosphorylationwere similar to that of MAP kinase during the first wave of activation(Fig. 8B); novel taste produced significant elevations of phospho-Rafat 0.5, 1, 2, 6, and 12 hr. However, one difference here is thelack of a second wave of activation of Raf; phosphorylation ofRaf after novel taste declined at 12 hr and was not significantlydifferent from naive controls at 24 and 48 hr. Similarly, althoughlevels of phospho-Raf were significantly increased by repeatedtaste presentation, there was a significant decline 48 hr afterthe fourth taste presentation (144 hr time point). These datasuggest the interesting possibility that the prolonged phase ofMEK/MAPK activation we observed may be attributable to a Raf-independentmechanism.

In addition to upstream activators of ERK/MAPK, we also sought to investigate the possible regulation of MAPK substrates.We focused on p90RSK because it is a MAPK substrate whose activityis regulated by phosphorylation and because p90RSK can coupleMAPK to phosphorylation of such downstream effectors as CREB.The kinetics of p90RSK phosphorylation were similar to those describedabove, although the magnitude of the response here was much greaterthan for other components of the MAP kinase cascade (Fig. 8C).Representative blots for phospho-Raf, phospho-MEK, and phospho-p90RSKare shown in Figure 8D. Novel taste produced significant increasesin phosphorylation of p90RSK at all time points; however, theresponse shows a similar biphasic response, declining at 12 hr,and then increasing at 24 and 48 hr. Repeated taste presentationsproduced significant increases in phospho-p90RSK, but there wasno significant additional increase with a fourth exposure relativeto the familiar controls (t = 96 hr). The finding that p90RSKphosphorylation followed similar kinetics as MAPK is interestingfor several reasons. As a substrate of MAPK, it allows one totrack MAPK activity and confirms the MAPK activation observedin our earlier experiments. Furthermore, as a kinase that regulatesphosphorylation of the transcription factor CREB, it providesa possible immediate link to altered gene expression mediatedby MAPkinase.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Novel taste memory is associated with long-lasting changes in lysine acetylation of p42AcK and p55AcK

A single 10 min exposure to a novel taste is sufficient to produce a memory for that taste, as shown by the attenuation ofneophobia and the capacity for acquisition of a conditioned tasteaversion to that taste. Insular cortex histone and lysine acetyltransferaseactivities were both regulated by novel taste but showed distinctlydifferent kinetics. Lysine acetylation of p55AcK showed an immediateand prolonged response up to 12 hr, and then levels declined tobaseline. Lysine acetylation of p42AcK, on the other hand, showedan unusual biphasic response which has not, to our knowledge,been reported for any biochemical marker in any learning or memoryparadigm to date. Although acetylation decreased at 6 hr, levelswere significantly elevated again even at 48 hr. The suggestionfrom these data that such a late response may be involved in long-termmemory formation is supported by the findings that acetylationis persistently elevated in the insular cortex of animals receivingmultiple presentations of the novel taste. The possibility thatthe long-lasting activation of p42AcK and p55AcK after repeatedpresentations is a result of familiarization, i.e., consolidationof the memory of the novel taste, is a tantalizing hypothesis.One important consideration to note is that the immunoreactive42 and 55 kDa bands seen here may actually represent multipleacetylation substrates that comigrate on SDS-PAGE, and the kineticsseen here may actually represent different substrates that areacetylated at different timepoints.

Novel taste memory is associated with biphasic activation of the entire ERK/MAPK cascade, and familiarization produces a persistent activation of the ERK/MAPK cascade

Although the biphasic response of p42AcK is unusual, demonstration of coupling to the MAP kinase cascade is suggested by thefinding of a similar activation of the entire ERK/MAPK cascade.Novel taste produced a biphasic increase in MAP kinase phosphorylation,and repeated taste presentation produced a persistently elevatedphosphorylation. Both the upstream activator MEK and the downstreamsubstrate p90RSK showed similar kinetics, demonstrating activationof the entire ERK/MAPKcascade.

The coordinate regulation of MEK suggests that future experiments be performed to examine the functional role of this lateractivation, along with the possible in vivo MAPK-dependent acetylationof p42Ack. These experiments might conceivably use the peripherallyadministered MEK inhibitor SL327, which has been shown here toblock conditioned taste aversion when given shortly before thenovel taste. Given the complex kinetics of MAPK, lysine acetyltransferase(KAT), and HAT activation, along with the short half-life of suchMEK inhibitors as SL327, such experiments will require that thedosing regimen is optimized to block various stages of ERK activation,including those that persist for hours or days after novel tastepresentation. At this time, both the behavioral necessity of thelater activation of the MAPK cascade, along with its role in lysineacetylation in insular cortex, remain to betested.

A dichotomy in the biphasic response of ERK/MAPK cascade components is seen when comparing phosphorylation of Raf, an immediateupstream activator of MEK, with the phosphorylation of MEK itself.Phosphorylation of Raf appears to show only the first wave ofactivation and is not significantly elevated in the novel groupafter 12 hr. This may provide a clue to the biphasic activationof MEK/MAPK, because a different MEK activator, perhaps Rap, maybe recruited for later MAPK activation. It is also plausible thatthis late phase of activation may depend on transcriptional activationby the first wave of MAPK activation. Although this has not beenreported in the brain, such a regulatory system has been seenwith MAP kinase activation in oocytes, which exhibit a biphasicactivation of MAP kinase; activation of MAP kinase stimulatestranscriptional activation of the kinase c-Mos, which can activateMAP kinase via phosphorylation of MEK, resulting in a positivefeedback loop between c-Mos and MAP kinase (Fisher et al., 2000).It will be interesting to determine whether such a self-reinforcingfeedback loop, a mnemogenic chemical reaction by the criteriaof Roberson and Sweatt (1999), exists in the insular cortex afternovel tastelearning.

This unusual biphasic response has not been previously reported for such MAP kinase-dependent learning and memory paradigmsas novel taste learning (Berman et al., 1998) spatial learning(Blum et al., 1999; Selcher et al., 1999), or fear conditioning(Atkins et al., 1998; Schafe et al., 2000). However, in none ofthese previous reports was MAP kinase examined for longer than2 or 3 hr after behavioral manipulations leading to MAPK activation,thus raising the possibility that the biphasic activation seenhere is not unique to our specific paradigm. Further examinationof the long-term kinetics of MAP kinase activation in other learningand memory paradigms will be necessary to address this intriguingpossibility.

Histone acetyltransferase and lysine acetyltransferase are positively and negatively regulated by MAP kinase

Histone and lysine acetyltransferase activity leading to lysine acetylation of p42AcK and p55AcK appear to be regulated byseparate and distinct pathways. Lysine acetylation of p42AcK wasfound to be MAPK-dependent in our in vitro insular cortex sliceexperiments. The possibility of ERK regulation of p42AcK is furthersupported by the similar kinetics of p42AcK and MAPK in vivo byboth novel and familiar taste. Lysine acetylation of p42AcK doesnot appear to be regulated by histone acetyltransferases, as shownby the lack of effect of trichostatin A on p42AcK acetylation.This finding raises the interesting possibility that in additionto histone acetyltransferases, a novel lysine acetyltransferaseactivity may be active in the brain, and whose function is toregulate, by lysine acetylation, nonhistone substrates. We canonly speculate at this point how lysine acetylation might regulatenonhistone substrates, but neutralization of positively chargedlysine residues might be considered analogous to the dramaticchanges that occur with phosphorylation: by altering the charge,conformational changes and alterations of protein-protein interactionscould have profound effects on the function of lysine acetyltransferasesubstrates. We are presently working to purify and sequence boththe p42AcK and p55AcK proteins to elucidate their potential rolesin neuronal plasticity underlying novel tastelearning.

In contrast to p42AcK, acetylation of p55AcK is regulated by histone acetyltransferases, because trichostatin A caused a coordinateincrease in acetylation of histones and p55AcK. It should be notedhere that although histone acetylation was measured in slices,because of the amount of tissue required to perform the histoneextraction, we were unable to measure this in insular cortex punchesobtained in vivo. However, given that in slices p55AcK acetylationoccurred in parallel with that of histones, this unknown substratemay provide a useful assay for histone acetyltransferase activityin vivo. Slice experiments also demonstrated that inhibition ofthe MAPK cascade with the selective MEK inhibitor U0126 elicitedsignificant increases in p55AcK acetylation, suggesting that theMAPK cascade exerts an inhibitory control over histone acetyltransferaseactivity in the insular cortex. However, we remain cautious inour interpretation of these findings, because this increase inp55AcK acetylation occurs after total obliteration of basal phospho-MAPK,an event that is unlikely to occur in vivo.

Solid food in nondeprived mice is a useful tool for studying novel taste memory

Although not used to any great extent before this report, we note the utility of a solid food stimulus in the study of molecularand biochemical mechanisms of learning and memory. This paradigmhas several features that make it desirable for taste learningstudies. First, its simplicity allows for high throughput, becauseanimals do not have to be maintained on any food or water deprivationschedule. Second, given that water deprivation produces anorexiaand results in large changes in gene expression in feeding-relatedareas of the brain (Watts, 2000), the use of nonwater-deprivedanimals may allow biochemical measurements that may be more representativeof the animal in its natural state. Furthermore, a novel solidfood stimulus may represent a reasonable reiteration of an ethologicallyrelevant stimulus that a mouse, a foraging animal, may encounter.Therefore, a novel solid food, by mimicking what the mouse evolvedto deal with in its natural environment, may elicit particularlyrobust biochemical changes in the insularcortex.

Long-lasting changes in biochemical activity during novel taste learning may represent changes in gene expression

Perhaps the most striking finding of this paper is that a single 10 min exposure to a novel taste stimulus produces dramaticbiochemical changes that persist for many hours after the initialstimulus. Activation of the entire MAP kinase pathway, lysineacetylation, and to a lesser extent, histone acetyltransferaseactivity, all show dramatic changes as a result of a novel tastestimulus. Furthermore, three previous exposures to a novel tasteare sufficient to produce persistent activation of all three pathwaysfor at least 48 hr after the last exposure. Although many differentscenarios may be posited, we believe that transcriptional activationand changes in gene expression are likely to subserve some ofthese persistent biochemical changes. Although not examined here,one likely mediator is CREB, a transcription factor implicatedin a number of learning and memory paradigms, and a substrateof the MAPK-activated kinase p90RSK. Hopefully future experimentswill allow the testing of this interestinghypothesis.

  FOOTNOTES

Received Dec. 4, 2000; revised Feb. 15, 2001; accepted March 9, 2001.

This research was supported by National Institutes of Health Grants MH18390, DC00454 (M.W.S.), and MH57014 (J.D.S.), a grantfrom the New York Obesity Research Center (M.W.S.), and a grantfrom the Texas Advanced Technology Program (J.D.S.). The kindsupport and encouragement of Dr. Gerard P. Smith are gratefullyacknowledged.
Correspondence should be addressed to Michael W. Swank, Division of Neuroscience, Baylor College of Medicine, One Baylor Plaza,Houston, Texas 77030. E-mail: mswank{at}cns.bcm.tmc.edu.

^aThe term histone acetyltransferase (HAT), although it would appear to refer specifically to the lysine acetylation of histones,is commonly used in the literature to refer also to lysine acetyltransferaseactivity responsible for acetylation of a rapidly growing listof other nonhistone substrates such as p53, CBP, and PCAF. Webelieve that the use of the term lysine (K) acetyltransferase(KAT) may be a more reasonable description of lysine acetyltransferasesinvolved in acetylation of nonhistone substrates such as p42AcKdescribed in this report, and we reserve the use of the term histoneacetyltransferase (HAT) for instances in which histones are demonstratedto be among the substrates that areacetylated.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ait SA, Carlisi D, Ramirez S, Upegui-Gonzalez LC, Duquet A, Robin P, Rudkin B, Harel-Bellan A, Trouche D (1999) Phosphorylation by p44 MAP Kinase/ERK1 stimulates CBP histone acetyltransferase activity in vitro. Biochem Biophys Res Commun 262:157-162[ISI][Medline].
Alberini CM (1999) Genes to remember. J Exp Biol 202:2887-2891[Abstract].
Allfrey VG, Faulkner R, Mirsky AE (1964) Acetylation and methylation of histones and their possible role in the regulation of RNA synthesis. Proc Natl Acad Sci USA 61:786-794.
Atkins CM, Selcher JC, Petraitis JJ, Trzaskos JM, Sweatt JD (1998) The MAPK cascade is required for mammalian associative learning. Nat Neurosci 1:602-609[ISI][Medline].
Bailey CH, Bartsch D, Kandel ER (1996) Toward a molecular definition of long-term memory storage. Proc Natl Acad Sci USA 93:13445-13452[Abstract/Free Full Text].
Berman DE, Hazvi S, Rosenblum K, Seger R, Dudai Y (1998) Specific and differential activation of mitogen-activated protein kinase cascades by unfamiliar taste in the insular cortex of the behaving rat. J Neurosci 18:10037-10044[Abstract/Free Full Text].
Berman DE, Hazvi S, Neduva V, Dudai Y (2000) The role of identified neurotransmitter systems in the response of insular cortex to unfamiliar taste: activation of ERK1-2 and formation of a memory trace. J Neurosci 20:7017-7023[Abstract/Free Full Text].
Blum S, Moore AN, Adams F, Dash PK (1999) A mitogen-activated protein kinase cascade in the CA1/CA2 subfield of the dorsal hippocampus is essential for long-term spatial memory. J Neurosci 19:3535-3544[Abstract/Free Full Text].
Bures JB-RFYT (1998) In: Conditioned taste aversion. Memory of a special kind. Oxford: Oxford UP.
Davie JR, Spencer VA (1999) Control of histone modifications. J Cell Biochem [Suppl] 32-33:141-148.
Fisher DL, Mandart E, Doree M (2000) Hsp90 is required for c-Mos activation and biphasic MAP kinase activation in Xenopus oocytes. EMBO J 19:1516-1524[ISI][Medline].
Impey S, Smith DM, Obrietan K, Donahue R, Wade C, Storm DR (1998) Stimulation of cAMP response element (CRE)-mediated transcription during contextual learning. Nat Neurosci 1:595-601[ISI][Medline].
Kawahara K, Watanabe S, Ohshima T, Soejima Y, Oishi T, Aratani S, Nakata M, Shibata M, Inoue K, Amano T, Fujii R, Yanai K, Hagiwara M, Fukamizu A, Maruyama I, Nakajima T (1999) Hypernuclear acetylation in atherosclerotic lesions and activated vascular smooth muscle cells. Biochem Biophys Res Commun 266:417-424[Medline].
Kouzarides T (2000) Acetylation: a regulatory modification to rival phosphorylation? EMBO J 19:1176-1179[ISI][Medline].
Martinez-Balbas MA, Bannister AJ, Martin K, Haus-Seuffert P, Meisterernst M, Kouzarides T (1998) The acetyltransferase activity of CBP stimulates transcription. EMBO J 17:2886-2893[ISI][Medline].
Roberson ED, Sweatt JD (1999) A biochemical blueprint for long-term memory. Learn Mem 6:381-388[Abstract/Free Full Text].
Roberson ED, English JD, Adams JP, Selcher JC, Kondratick C, Sweatt JD (1999) The mitogen-activated protein kinase cascade couples PKA and PKC to cAMP response element binding protein phosphorylation in area CA1 of hippocampus. J Neurosci 19:4337-4348[Abstract/Free Full Text].
Schafe GE, Atkins CM, Swank MW, Bauer EP, Sweatt JD, LeDoux JE (2000) Activation of ERK/MAP kinase in the amygdala is required for memory consolidation of Pavlovian fear conditioning. J Neurosci 20:8177-8187[Abstract/Free Full Text].
Selcher JC, Atkins CM, Trzaskos JM, Paylor R, Sweatt JD (1999) A necessity for MAP kinase activation in mammalian spatial learning. Learn Mem 6:478-490[Abstract/Free Full Text].
Silva AJ, Kogan JH, Frankland PW, Kida S (1998) CREB and memory. Annu Rev Neurosci 21:127-148[ISI][Medline].
Spencer VA, Davie JR (1999) Role of covalent modifications of histones in regulating gene expression. Gene 240:1-12[ISI][Medline].
Stork O, Welzl H (1999) Memory formation and the regulation of gene expression. Cell Mol Life Sci 55:575-592[Medline].
Swank MW (2000a) Phosphorylation of MAP kinase and CREB in mouse cortex and amygdala during taste aversion learning. NeuroReport 11:1625-1630[ISI][Medline].
Swank MW (2000b) Pharmacological antagonism of tyrosine kinases and MAP kinase in brainstem blocks taste aversion learning in mice. Physiol Behav 69:499-503[Medline].
Thomson S, Mahadevan LC, Clayton AL (1999) MAP kinase-mediated signalling to nucleosomes and immediate-early gene induction. Semin Cell Dev Biol 10:205-214[ISI][Medline].
Watts AG (2000) Understanding the neural control of ingestive behaviors: helping to separate cause from effect with dehydration-associated anorexia. Horm Behav 37:261-283[Medline].
Yoshida M, Kijima M, Akita M, Beppu T (1990) Potent and specific inhibition of mammalian histone deacetylase both in vivo and in vitro by trichostatin A. J Biol Chem 265:17174-17179[Abstract/Free Full Text].

Copyright © 2001 Society for Neuroscience 0270-6474/01/21103383-09$05.00/0

This article has been cited by other articles:

W. B. Chwang, J. S. Arthur, A. Schumacher, and J. D. Sweatt
The Nuclear Kinase Mitogen- and Stress-Activated Protein Kinase 1 Regulates Hippocampal Chromatin Remodeling in Memory Formation
J. Neurosci., November 14, 2007; 27(46): 12732 - 12742.
[Abstract] [Full Text] [PDF]

W. B. Chwang, K. J. O'Riordan, J. M. Levenson, and J. D. Sweatt
ERK/MAPK regulates hippocampal histone phosphorylation following contextual fear conditioning.
Learn. Mem., May 1, 2006; 13(3): 322 - 328.
[Abstract] [Full Text] [PDF]

P. Trifilieff, C. Herry, P. Vanhoutte, J. Caboche, A. Desmedt, G. Riedel, N. Mons, and J. Micheau
Foreground contextual fear memory consolidation requires two independent phases of hippocampal ERK/CREB activation
Learn. Mem., May 1, 2006; 13(3): 349 - 358.
[Abstract] [Full Text] [PDF]

G. M. Sutton, L. M. Patterson, and H.-R. Berthoud
Extracellular Signal-Regulated Kinase 1/2 Signaling Pathway in Solitary Nucleus Mediates Cholecystokinin-Induced Suppression of Food Intake in Rats
J. Neurosci., November 10, 2004; 24(45): 10240 - 10247.
[Abstract] [Full Text] [PDF]

C. Crosio, E. Heitz, C. D. Allis, E. Borrelli, and P. Sassone-Corsi
Chromatin remodeling and neuronal response: multiple signaling pathways induce specific histone H3 modifications and early gene expression in hippocampal neurons
J. Cell Sci., December 15, 2003; 116(24): 4905 - 4914.
[Abstract] [Full Text] [PDF]

M. Fornage, M. W. Swank, E. Boerwinkle, and P. A. Doris
Gene expression profiling and functional proteomic analysis reveal perturbed kinase-mediated signaling in genetic stroke susceptibility
Physiol Genomics, September 29, 2003; 15(1): 75 - 83.
[Abstract] [Full Text] [PDF]

S. K. Sharma, C. M. Sherff, J. Shobe, M. W. Bagnall, M. A. Sutton, and T. J. Carew
Differential Role of Mitogen-Activated Protein Kinase in Three Distinct Phases of Memory for Sensitization in Aplysia
J. Neurosci., May 1, 2003; 23(9): 3899 - 3907.
[Abstract] [Full Text] [PDF]

This Article