Expression of Integrin-Associated Protein Gene Associated with Memory Formation in Rats

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The Journal of Neuroscience, June 1, 1998, 18(11):4305-4313

Expression of Integrin-Associated Protein Gene Associated with Memory Formation in Rats
A-Min Huang¹^,², Hai Long Wang², Yu Ping Tang¹, and Eminy H. Y. Lee¹
¹ Institute of Biomedical Sciences, Academia Sinica, Taipei, Taiwan, Republic of China, and ² Graduate Institute of Life Sciences, National Defense Medical Center, Taipei, Taiwan, Republic of China

  ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The present study has adopted the PCR differential display method to identify cDNA clones associated with memory formationin rats. The one-way inhibitory avoidance learning task was usedas the behavioral paradigm. Total RNA isolated from the hippocampusof poor-memory (<80 sec) and good-memory (600 sec) rats 3 hr aftertraining was used for comparison. Three cDNA fragments correspondingto different spliced forms of integrin-associated protein (IAP)mRNA were found to be differentially expressed in the hippocampusof good-memory rats. Quantitative reverse transcription-PCR revealedapproximately four fold higher of IAP mRNA level in good-memoryrats. This result was confirmed further by in situ hybridizationanalysis, and the major difference was in the dentate gyrus. Ithas been demonstrated that this difference in IAP mRNA expressionis not attributable to different sensitivities of individual ratsto electric shock. Rapid amplification of cDNA ends obtained thefull-length IAP cDNA, which is 1192 bp in length excluding thepoly(A⁺) tail. The IAP mRNA expression was significantly upregulatedby NMDA and amphetamine injections to the dentate gyrus of thehippocampus. On the other hand, injection of antisense oligonucleotidecomplementary to the IAP transcript markedly impaired memory retentionin rats and decreased the amplitude and slope of EPSP in the invivo long-term potentiation paradigm. These results together suggestthat IAP gene expression plays an important role in memory formationand synaptic plasticity in rat hippocampus.

Key words: PCR differential display; integrin-associated protein; inhibitory avoidance learning; memory formation; long-term potentiation; hippocampus

  INTRODUCTION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

A number of studies have revealed that there are many forms of memory. According to the temporal parameter, memory can bedivided into at least two distinct forms: short-term memory andlong-term memory. Short-term memory lasts for minutes to hours,whereas long-term memory persists for several hours to days, weeks,and even years (Goelet et al., 1986). Two lines of evidence suggestthat long-term memory, but not short-term memory, requires denovo RNA and protein synthesis. The first one is that inhibitionof protein or mRNA synthesis impairs long-term memory (Davis andSquire, 1984). The second one is that long-term memories are believedto be stored by modification of preexisting synapses or formationof new synaptic connections (Weiler et al., 1995). This evidenceindicates that the neural activities associated with learninglead to the expression of various genes, the protein productsof which play a critical role in memory formation. Extensive effortshave been made to identify specific gene expression related tolong-term memory formation. With the use of two-dimensional gelanalysis, Castellucci et al. (1988) identified several proteinsthat are related to the process of long-term sensitization forthe gill-withdrawal reflex in the sea plug Aplysia. Screeningof Drosophila mutants has yielded approximately 10 genes thatare specific to the processes of olfactory learning and memory(Tully, 1996). These methods are effective; however, they takea long time to identify and characterize the specific genes.

In the present study, we have used the PCR differential display method (Liang and Pardee, 1992) to identify gene expressionrelated to memory formation in rats. The general strategy of thismethod is to amplify partial cDNA sequences from subsets of mRNAsby reverse transcription (RT) and PCR. Pairs of primers were usedin the PCR amplification: one is a degenerate anchor primer thatanneals to the poly(A⁺) tail, and the other is arbitrary in sequence and hybridizesat different positions relative to the anchor primer. The amplifiedPCR products are then displayed on a sequencing gel, and the differentiallyexpressed genes can be rapidly identified. An inhibitory avoidancelearning task was used as the behavioral paradigm. Previous pharmacologicaland biochemical studies have shown that the hippocampus is involvedin this form of learning (Lee et al., 1993; Cammarota et al.,1995; Izquierdo et al., 1995). More related to the present study,injection of protein or mRNA synthesis inhibitors into the dentategyrus of the hippocampus significantly impaired memory consolidationin rats (Lee et al., 1992). Using the PCR differential displaymethod, we have found that one of these genes related to memoryformation encodes the rat integrin-associated protein (IAP). IAPwas first characterized in human placental tissue and hematopoeticcells (Brown et al., 1990). Subsequent analyses showed that anRh complex-related glycoprotein CD47 (Mawby et al., 1994) andan ovarian tumor marker OA3 (Campbell et al., 1992) are the sameas IAP. These observations suggest that IAP may have differentfunctions in different tissues. In the present study we providethe first evidence that IAP gene expression in the hippocampusis associated with memory consolidation and synaptic plasticityin rats.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Animals. Adult male Sprague Dawley rats (220-300 gm) bred in the Animal Facility of the Institute of Biomedical Sciences,Academia Sinica, were used. Animals were housed in a room maintainedat 23 ± 2°C and a 12 hr light/dark cycle (light on at 6:30 A.M.).Food and water were available ad libitum.

Inhibitory avoidance learning task. A one-way inhibitory avoidance learning task was used to measure retention performancein rats. The apparatus consists of a trough-shaped alley dividedby a sliding door into an illuminated safe compartment and a darkcompartment. A shock generator with facilities to vary currentis connected to the floor of the dark compartment. The behavioraltask included the training and testing procedures and was conductedbetween 10:00 A.M. and 5:00 P.M. Before experimentation, ratswere kept in a dim room for 1 hr to adjust to the environment.On the training phase, the rat was placed at the far end of theilluminated compartment facing away from the door. As the ratturned around, the door was opened. When the rat entered the darkcompartment, the door was closed and a 1.0 mA/1 sec footshockwas given. The rat was then removed from the alley and returnedto its home cage. Three hours later, the retention test was given.The rat was again placed into the illuminated compartment, andthe latency to step into the dark compartment was recorded asthe measure of retention performance. Rats that did not enterthe dark compartment and reached the ceiling score of 600 secwere removed from the alley and assigned as good-memory rats.Rats with a retention latency <80 sec were assigned as poor-memoryrats. Sixty-eight rats were trained. Eleven rats that showed poormemory and eleven rats that showed good memory were chosen forfurther experiments. The remaining rats showing a retention latencybetween 80 and 600 sec were not used in the present study. Fiveuntrained rats and four rats that received only electric shockwithout going through the training procedure were used for thecontrol experiment. In assessing the effects of IAP antisenseoligonucleotide on memory retention (see below), we subjectedthe rats to the same behavioral training and testing procedures,and the retention score for each rat was recorded.

Tissue dissection and total RNA extraction. Animals were decapitated immediately after the retention test. Their brains wereremoved and placed in ice-cold saline for 5 min and then slicedon an ice-cold platform. Bilateral hippocampal tissues were dissectedout, frozen on dry ice, and stored at $-$ 80°C until use. Total RNAwas isolated from the hippocampus of each rat using 1 ml of theUltraspec RNA isolation solution according to the instructionof the manufacturer (Biotecx Laboratories, Houston, TX). DNasetreatments were performed to remove DNA contamination. Twentymicrograms of total RNA were incubated at 37°C for 30 min with2 U of ribonuclease inhibitor (Promega, Madison, WI), 2 U of DNaseI (Promega) in 10 mM Tris-Cl, pH 9.0, 50 mM KCl, 1.5 mM MgCl₂,and 0.1% Triton X-100. The reaction was stopped by extractionwith phenol/chloroform (3:1), and the supernatant was precipitatedwith 2 vol of ethanol in the presence of 0.25 M potassium acetate.RNA was then redissolved in an appropriate volume of DEPC-treatedwater. Optical densities of OD₂₆₀ and OD₂₈₀ were used to estimatethe quantity and purity of the isolated total RNA.

PCR differential display. PCR differential display analysis was performed according to the original method (Liang and Pardee,1992; Liang et al., 1993) with minor modifications. Total RNA(1.0 µg) was incubated at 70°C for 10 min with 2 µl of one ofthe degenerate oligo dT primers (25 µM) (T₁₂VA, T₁₂VC, T₁₂VG,and T₁₂VT; V = A, C, or G) (synthesized by Genosys Biotechnologies,The Woodlands, TX) and DEPC H₂O to a final volume of 9 µl, andsubsequently kept on ice for 5 min. Four microliters of 5× synthesisbuffer, 1 µl of 200 µM dNTP mix, 2 µl of 0.1 M dithiothreitol(DTT), 0.28 µl of RNasin (40 U/µl) (Promega), and 1 µl of SuperscriptII Moloney murine leukemia virus reverse transcriptase (200 U/µl)(Life Technologies/BRL, Grand Island, NY) were added to the mixtureand incubated at 37°C for 60 min. The reaction was terminatedby heating the sample at 80°C for 10 min. Two microliters of thereverse-transcribed products were added into 18 µl of the PCRreaction mixtures containing 50 mM KCl, 10 mM Tris-Cl, pH 8.8at 25°C, 1.0 mM MgCl₂, 0.1% Triton X-100, 4 µM dNTP, 0.5 µM [³⁵S]dATP (Amersham, Buckinghamshire, UK), and 1 U of Tag DNA polymerase(Promega). Thirty short arbitrary primers (purchased from GenosysBiotechnologies) were used for the PCR reactions. The PCR parameterswere 94°C for 30 sec, 40°C for 1 min, and 72°C for 30 sec for40 cycles followed by a final elongation at 72°C for 5 min. Analiquot of 5.7 µl of the PCR products was mixed with 2.3 µl ofsequencing loading buffer and separated on 6.0% polyacrylamidegels. Differentially expressed cDNA fragments were recovered fromthe sequencing gels, reamplified with the same set of primer pairs,and cloned into the pGEM-T vector using the TA cloning system(Promega). Plasmid DNA containing the correct inserts was sequencedusing the ABI Prism dye terminator kit and an ABI 373 sequencer(Applied Biosystems, Foster City, CA). The nucleotide sequencesobtained were compared with known sequences by searching GenBankand European Molecular Biology Laboratory databases with the FastaProgram (Genetic Computer Group).

Rapid amplification of cDNA ends cloning. Rapid amplification of cDNA ends (RACE) cloning strategy (Frohman et al., 1988)was used to obtain the full-length rat IAP cDNA. Specific oligonucleotideswere designed from the common sequence of A5, A6, and A7 fragmentsidentified by PCR differential display. RACE reactions were performedwith the Marathon cDNA amplification kit from Clontech Laboratoriesaccording to the manufacturer's instructions. One microgram ofhippocampal poly(A⁺) RNA from an untreated rat was subjected to cDNA synthesis andone-fiftieth of the RACE-ready cDNA was used as template in the5'RACE or 3'RACE PCR reactions. 5'RACE reactions were performedwith a gene-specific primer (GSP1) (see Fig. 2A) and Anchor Primer(Clontech Laboratories). Dilutions of the primary PCR amplificationwere used for secondary PCR reactions using a nested gene-specificprimer (GSP2) (see Fig. 2A) and another Anchor Primer. Productsof the secondary PCR reactions were analyzed by a 1.5% agarosegel and three cDNA fragments (~1000, 700, and 400 bp) were visualizedon the ethidium bromide-stained gel. These products were clonedinto the pGEM-T vector (Promega), and clones containing the 1000,700, or 400 bp insert were sequenced from both directions usingthe ABI373 sequencer. The 1000 or 700 bp clone contains the sequenceof A5 fragment (Fig. 1), and the 400 bp clone contains the sequenceof the A6 fragment (Fig. 1). 3'RACE reactions were performed withanother gene-specific primer (GSP3) (Fig. 2A) and Anchor Primer.A 300 bp fragment was obtained, which was identical to the sequenceof A5 fragment. The rat IAP cDNA obtained by this RACE cloningstrategy was 1160 bp in length, which did not contain the 5' untranslationregion and an initiation codon by comparison with the mouse IAPcDNA sequence (GenBank, accession number Z25524). Further cloningwas performed by using an oligonucleotide corresponding to the5' end of mouse IAP cDNA (mIAP: 5'-CCC GGG CAG CCT GGG CGG CCGCTC CTG-3') and an oligonucleotide to the 5' end of the 1160 bpcDNA (GSP4) (Fig. 2A). Oligonucleotides used for PCR analysisof the IAP gene were synthesized by Genosys Biotechnologies.

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Figure 1. PCR differential display of rat hippocampal RNA associated with retention performance of inhibitory avoidance learning. Total RNA isolated from the hippocampus of poor-memory (PM) and good-memory (GM) rats was subjected to differential display analysis using 5' oligonucleotide Ldd8 (5'-AGC CAG CGA A-3') and 3' oligonucleotide T₁₂VA as the primer set. Radiolabeled PCR products were analyzed with a 6.0% polyacrylamide gel. Differentially expressed cDNA fragments $---$ A5, A6, and A7 cDNA bands, among three poor- and three good-memory rats $---$ are illustrated.

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Figure 2. Nucleotide and deduced amino acid sequence of rat IAP cDNA. A, Nucleotide sequence of rat IAP cDNA. Nucleotides are numbered relative to the start of the initiation codon. The putative poly(A⁺) addition site (AATAAA) is underlined. The location of sites at which the 5' [nucleotide (nt) 868-877] and 3' (nt 1172-1185) PCR differential display primers hybridized are also shown. Gene-specific primers used for RACE cloning are shown. The deduced amino acid sequence is shown in a one-letter IUPAC code, starting with the initiator methionine. The splicing sites that generate form 2, form 3, and form 4 rat IAP are indicated by arrows. This sequence has been assigned accession number AF017437 by GenBank. B, Alignment of amino acid sequence among rat, mouse, and human IAP. Sequences are numbered starting with the initiator methionine. The amino acid sequences are given with gaps introduced during the alignment indicated by dots. Amino acids are shadowed where the residues of two or three sequences are identical at any given position. Potential N-linked glycosylation sites in the rat IAP are shown by asterisks above the sequence.

In situ hybridization. We performed an in situ hybridization experiment to evaluate expression of the IAP mRNA in rat hippocampusafter the inhibitory avoidance learning. The in situ hybridizationprotocol used was slightly modified from the previous study (Tanget al., 1997). Three hours after the retention test, animals wereanesthetized with pentobarbital (40 mg/kg, i.p.) and perfusedintracardially with 150 ml of heparinized 0.1 M PBS, pH 7.4, followedby 150 ml of 4% paraformaldehyde in 0.1 M PBS. Brains were removedand stored at $-$ 80°C until they were sectioned. Serial sectionsat 20 µm thickness through the hippocampus from six good-memoryand four poor-memory rats were cut on a cryostat, thaw-mountedonto poly-l-lysine-coated slides, and vacuum-desiccated overnight.Slides were stored in boxes containing desiccant at $-$ 80°C untilin situ hybridization was performed. In situ hybridization wasperformed using a 46-base synthetic oligonucleotide (5'-CCA CTTCAC AAA CAT TTC ATC GGT GCT TTG GGC CTC CAC ATT AAG G-3'). Thisoligomer is complementary to the cloned rat IAP cDNA (bases 129-174)and was synthesized and purified by Genosys Biotechnologies. Theprobe (15 pmol/µl) was 3' end-labeled by incubating at 37°C for15 min with ³⁵S-dATP (Amersham) and terminal deoxynucleotidyl transferase (25U; Boehringer Mannheim, Indianapolis, IN) to a specific activityof ~10⁶ cpm/µl. Prehybridization treatment of tissue consisted of warmingthe sections to room temperature and rinsing in 20× SSC for 10min at room temperature. For hybridization, the labeled IAP oligonucleotideprobe (1 × 10⁶ cpm/slide) in 100 µg/ml yeast transfer RNA, 500 µg/ml salmonsperm DNA, and Denhardt's solution (0.02% Ficoll, 0.02% polyvinylpyrrolidone,and 0.02% bovine serum albumin) was applied to each slide. Slideswere coverslipped with parafilm, and hybridization proceeded for24 hr at 42°C. Coverslips were then removed, and sections wererinsed in 2× SSC and then in 1× SSC containing 1.0 M (DTT, 0.1%),followed by 30 min wash in 0.5× SSC containing 1.0 M DTT at 47°C.A final wash in 0.5× SSC containing 1.0 M DTT was performed atroom temperature for 30 min. The slides were dehydrated througha series of ethanols and dipped in emulsion (NTB-3, Kodak, Rochester,NY) diluted 1:1 with distilled water. After a 3 week exposureperiod, slides were developed in Kodak D-19 developer.

Quantitative RT-PCR analysis. Quantitative RT-PCR analysis was used to determine the relative amount of IAP mRNA from varioustreatments. RT reactions were performed as described above (seePCR differential display), except that 10 mM dNTP and 0.5 µg/µlof oligo d(T)₁₅ were used. The rat hypoxanthine phosphoribosyltransferase (HPRT) mRNA was used as an internal control templatethat was coamplified with the IAP mRNA. Synthetic primers 5'-CTCTGT GTG CTG AAG GGG GG-3' and 5'-GGG ACG CAG CAA CAG ACA TT-3'were used to detect HPRT mRNA (Jansen et al., 1992) and GSP1 andGSP3 primers (Fig. 2A) for IAP mRNA. One-twentieth of the RT productswas then added to a 20 µl PCR solution containing the same reactionbuffer as described above: 0.2 mM each of dGTP, dCTP, and dTTP,0.1 mM dATP, 0.1 µM HPRT primers, 0.2 µM IAP primers, 1.0 U ofTag DNA polymerase, and 0.5 µM [³⁵S]dATP (Amersham). The cycling parameters were 94°C for 30 sec,60°C for 1 min, and 72°C for 30 sec for 39 cycles followed bya final elongation at 72°C for 5 min. Eighteen microliters ofthe PCR products were analyzed on a native 9% polyacrylamide geland autoradiographed on the imaging plate of a phosphoimage analyzer(Phosphoimager, Molecular Dynamics, Sunnyvale, CA). Quantificationof the radioactivity of each cDNA band was performed accordingto the instruction manual. For establishment of the standard curve,0.125-2.0 µg of total RNA was reverse-transcribed. One-twentiethof the RT products was PCR-amplified and analyzed. For comparisonsof samples from different drug treatments, 0.5 µg of total RNAwas used.

IAP mRNA expression after intra-dentate gyrus drug administration. Pharmacological studies have shown that drugs such as amphetamineand NMDA were effective in enhancing memory performance of inhibitoryavoidance learning in rats (Lee et al., 1993; Lee and Ma, 1995).This experiment therefore was designed to examine the effectsof these drugs on IAP mRNA expression in the hippocampus. Ratswere subjected to stereotaxic surgery and drug infusions as describedpreviously (Huang and Lee, 1995). Briefly, two 23 gauge stainlesssteel thin-wall cannulae (10 mm long) were implanted bilaterallyinto the dorsal dentate gyrus of the hippocampus (3.6 mm posteriorto the bregma, 2.5 mm lateral to the midline, and 3.0 mm ventralto the skull surface). Seven to 10 d after recovery from the surgery,animals were given bilateral intra-dentate gyrus injections ofsaline, amphetamine (1.6 µg/side), NMDA (0.03 µg/side), or carbachol(0.8 µg/side). The animals were awake and gently held by the experimenterwhen they were given the injections. The injection was administeredthrough a 30 gauge injection needle connected to a 10 µl Hamiltonmicrosyringe by 0.5 m of polyethylene tubing (PE-20). The injectionneedle was bent so that when it was inserted into the cannulathe needle tip would protrude 1.5 mm beyond the tip of the cannula.Drug solutions were introduced into the PE tubing and the microsyringe,and they were delivered into the dentate gyrus manually at a rateof 0.2 µl/min with a total volume of 0.8 µl on each side. Amphetamineand carbachol were purchased from Sigma (St. Louis, MO). NMDAwas obtained from Research Biochemical (Natick, MA). Doses referto the salt form. Drugs were dissolved in 0.9% isotonic salineimmediately before use. Thirty minutes after drug infusion, bilateraldentate gyrus tissues were dissected out using a 1.5 mm punch,frozen on dry ice, and stored at $-$ 80°C until use. Total dentategyrus RNA extraction and IAP mRNA detection were performed asdescribed above.

IAP antisense oligonucleotide administration. To specifically inhibit the expression of the IAP gene, an antisense phosphorothioatederivative of the 18 mer 5'-CGC CGC CAA GGG CCA CAT-3' was synthesizedcomplementary to nucleotides 1-18 of the sequence of rat IAP cDNA(Fig. 2A). A random 18 mer sequence 5'-TGA GAA GAG TGA TGA CAA-3'was synthesized as a control. The phosphorothioate oligonucleotideswere synthesized and purified by Genosys Biotechnologies. Forthe memory retention experiment, rats were randomly divided intothree groups (n = 11 or 9) (see Fig. 6). Rats in all groups weresubjected to stereotaxic surgery and intra-dentate injectionsas described above. For this experiment, 1 nmol of IAP antisenseor random sequence oligonucleotide in 1.0 µl was injected intoeach rat four times, with 12 hr between injections, at a rateof 0.2 µl/min. Rats were trained 12 hr after the last injection,and memory retention was measured 3 hr after training. For thelong-term potentiation (LTP) experiment, the IAP antisense orthe random sequence was similarly injected into one side of thedentate area at a position 1.0 mm above the gyrus. Two injections(1 nmol) were given, with the first injection 16 hr and the secondinjection 2 hr before the electrophysiological recording. Foreach injection, 1.0 µl of 1.0 nmol antisense or random sequencewas administered at a rate of 0.2 µl/min.

Electrophysiology. The in vivo LTP recording was adopted to test the effect of IAP antisense oligonucleotide on synaptic plasticityin rats. The method used was according to that of Wayner et al.(1993) with minor modifications. Rats (250-350 gm) were anesthetizedwith urethane (1.4 gm/kg, i.p.) and placed on a stereotaxic instrument.Throughout the surgery and experiment, core body temperature wasmonitored and maintained at 35 ± 1°C with a feedback control system.The skull was exposed, and electrodes were implanted through burrholes in the skull. Stimulating electrodes were platinum concentricbipolar electrodes with a tip diameter of 25 µm and were positionedunilaterally to the dorsomedial perforant path at stereotaxiccoordinates of 8.5 mm posterior and 4.4 mm lateral to the bregma.Recording electrodes were prepared from single-barrel glass micropipettes(1.2 mm outer diameter × 0.6 mm inner diameter), pulled on a Narishigevertical puller, and filled with 3 M NaCl. Resistance ranged from1 to 3 M $Omega$ . The recording electrodes were implanted ipsilaterallyinto the dentate gyrus, 3.5 mm posterior to the bregma and 2.0mm lateral to the midline. The stereotaxic coordinates were adjustedfor variation in rat body weights and to maximize the monosynapticresponses of the population EPSPs (pEPSPs) produced by the granularcells in response to stimulation of the perforant path. Once boththe recording and stimulating electrodes were positioned, 5% agardissolved in 0.9% NaCl was applied over the exposed skull to preventsurface drying and reduce movement artifacts. Stimulation consistedof 50 µsec duration monophasic constant current pulses deliveredonce every 10 min. Stimulus intensities ranged from 50 to 250µA and produced averaged pEPSP amplitudes of 3-5mV. Once determined,stimulus current remained constant throughout the experiment.To induce LTP, four sets of stimulus trains in a 10 min periodwere delivered after a 30 min baseline recording. Each set containedfive trains, 10 pulses per train at 400 Hz, delivered at a rateof one train/sec for 5 sec. The pulse widths in the trains were50, 100, 150, and 200 µsec, respectively. The population spikeamplitude, slope, and amplitude of the pEPSPs were recorded onceevery 10 min.

Statistical analysis. Student's t test or one-way ANOVA followed by Dunnett's t test were used for comparisons between groupsfor the IAP mRNA level and for the amplitude and slope of pEPSP.Because the distribution of the retention score was uneven andwas truncated at 600, nonparametric Mann-Whitney U test was usedto analyze the data for retention performance.

  RESULTS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

PCR differential display analysis

Total RNA samples extracted from the hippocampus of poor- and good-memory rats tested 3 hr after inhibitory avoidance learningwere subjected to PCR differential display analysis. Four 3'-endprimers (T₁₂VA, T₁₂VC, T₁₂VG, and T₁₂VT) in combination with 305'-end arbitrary 10-mers were used for screening. Most of thecDNA bands were identical among individuals; however, three cDNAbands, designated as A5, A6, and A7, were differentially expressedbetween poor-memory and good-memory rats when the T₁₂VA and Ldd8(5'-AGCCAGCGAA-3') were used as primer pairs (Fig. 1). Sequencecomparison revealed that these three cDNA bands are identicalin their 3'-end cDNA sequences. However, at the 5'-end, A5 is25 bp longer than A6, and A6 is 33 bp longer than A7. Their sequenceswere 80 and 70% homologous to the 3'-end region of the mouse IAPcDNA (accession number Z25524) and human IAP cDNA (accessionnumber Z25521), respectively. It appears that A5, A6, and A7cDNAs correspond to different alternative splicing forms of ratIAP mRNA. Differences among these three forms are identical tothe alternative splicing forms found in human and mouse (Campbellet al., 1992; Reinhold et al., 1995). A5 corresponds to the form4 IAP, A6 to the form 3 IAP, and A7 to the form 2 IAP (Reinholdet al., 1995).

RACE cloning

To obtain a full-length transcript of the rat IAP, the RACE cloning strategy was performed as described in Materials and Methods.Results indicated that the IAP cDNA is 1192 bases in length, excludingthe poly(A⁺) tail (Fig. 2A). The predicted encoded polypeptide is 321 residuesin length, which corresponds to the human or mouse form 4 IAP.Figure 2B shows the identity in amino acid sequence among rat,mouse, and human IAP. There is 93% identity between rat and mouseIAP and 72% identity between rat and human IAP. The predictedmolecular mass of IAP is 35 kDa, considerably lower than the apparentmolecular mass of 50 kDa determined for native human IAP by SDS-PAGE(Brown et al., 1990). The presence of six putative N-linked glycosylationsites (AsnXSer/Thr) (Fig. 2B) suggests that extensive glycosylationmay account for the size discrepancy.

In situ hybridization

Results of in situ hybridization analyses indicated that the IAP mRNA is expressed in both the pyramidal cell layer and thedentate gyrus of the hippocampus. Although the IAP mRNA levelwas higher in both subdivisions of the hippocampus in good-memoryrats when compared with the poor-memory controls, but the effectwas more prominent in the dentate gyrus (Fig. 3).

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Figure 3. In situ hybridization showing a higher expression of IAP mRNA signal in the hippocampus of good-memory rats. Coronal sections through the hippocampus from (A) poor-memory rats (n = 4) and (B) good-memory rats (n = 6) were subjected to in situ hybridization analyses. CA1, CA1 cell body layer; CA3, CA3 cell body layer; DG, dentate gyrus. Scale bar, 500 µm.

IAP mRNA level determined by quantitative RT-PCR analysis

To further confirm the expression of hippocampal IAP in relation to memory consolidation, quantitative RT-PCR analysis wasused to estimate the IAP mRNA level. Oligonucleotides correspondingto the common sequence of A5, A6, and A7 cDNAs were used as primers,and the PCR product is 209 bp in length (Fig. 4A). Linear relationshipwas established between serial amounts of hippocampal total RNA(6.25-100 ng) and the optical densities of the cDNA bands (Fig.4B). Statistical analyses revealed that the IAP mRNA level wassignificantly higher in good-memory rats when compared with thepoor-memory rats (t = 8.11; p < 0.01) (Fig. 4C,D).

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Figure 4. Quantitative RT-PCR analysis of rat IAP mRNA. A, Autoradiograph of the IAP and HPRT cDNA bands. Serial quantities (6.25, 12.5, 25, 50, and 100 ng) of total hippocampal RNA were reverse-transcribed and amplified by PCR. The template of HPRT was used as an internal control. RT-PCR products were analyzed by a 9% polyacrylamide gel, visualized by a phosphoimager machine, and quantitated. B, Linear relationship between the optical density of the cDNA bands and the quantity of total RNA. C, Autoradiography of the IAP and HPRT cDNA bands from the poor-memory (PM) and good-memory (GM) rats. D, Higher expression of IAP mRNA level in good-memory rats (n = 11 in each group). **p < 0.01 by Student's t test. E, IAP mRNA expression in control animals and animals that received electric shock only. The control rats (n = 5) were placed in the chamber for 5 sec, returned to the home cage, and killed 3 hr later. Rats in the shocked group (n = 4) received a single electric shock, were returned to the home cage, and were killed 3 hr later.

To demonstrate that the observed effects are not attributable to differences in the sensitivity of individual rats to electricshock, hippocampal RNA from five untrained rats and from fourrats that received electric shock but not the training procedurewas analyzed. Results indicated that there was not a significantdifference in IAP mRNA level between these two groups of rats(t = 0.11; p > 0.75) (Fig. 4E). These results indicate that thedifference in IAP mRNA level is not attributable to the differencein the sensitivity of the animals to electric shock.

Regulation of IAP mRNA by drugs

If IAP mRNA expression is specifically associated with memory processing, then drugs that facilitate memory performance arelikely to alter IAP mRNA expression. We tested this hypothesisby directly injecting amphetamine, NMDA, and carbachol into thedentate gyrus in rats. Animals were killed 30 min after drug infusion,and their dentate gyrus tissues were dissected out and subjectedto RT-PCR analysis of IAP mRNA expression. As shown in Figure5, one-way ANOVA revealed an overall significant effect of drugtreatment (F = 4.06; p < 0.05). Further Dunnett's t test indicatedthat both amphetamine and NMDA contributed to this main effect(t_D = 2.32, p < 0.05, and t_D = 2.70, p < 0.05, respectively).Carbachol was without a significant effect (t_D = 0.11, p > 0.05).

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Figure 5. Drug effects on IAP mRNA level. Saline (SAL), amphetamine (AMPH), NMDA, or carbachol (CARB) was infused into rat dentate gyrus bilaterally at a rate of 0.2 µg/min and a total volume of 0.8 µl on each side. The number in each column indicates the number of rats in each treatment group. Thirty minutes after drug infusion, rats were decapitated, and the bilateral dentate gyrus tissues were dissected out. Total RNA was isolated and subjected to quantitative RT-PCR analysis identical to the procedure in Figure 4. Both amphetamine and NMDA significantly increased IAP mRNA level in the hippocampus (*p < 0.05; Dunnett's t test).

Effects of IAP antisense oligonucleotide on memory retention in rats

To demonstrate that IAP mRNA expression is indeed involved in the memory process, we have assessed the effects of IAP antisenseoligonucleotide treatment on memory retention in rats. As shownin Figure 6, results indicated that IAP antisense oligonucleotideadministration significantly impaired retention performance inrats (Mann-Whitney U test; U = 18.5, Z = 2.35, p < 0.05 when comparedwith the controls). Injection of random sequence oligonucleotidedid not produce a marked effect on memory retention (Mann-WhitneyU test; U = 58.5, Z = 0.13, p > 0.05 when compared with the controls).

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Figure 6. Effects of IAP antisense oligonucleotide on memory retention of one-way inhibitory avoidance learning in rats. The distribution of the retention score for each individual rat after saline (n = 11), IAP antisense oligonucleotide (n = 9), or random sequence (n = 11) treatment is shown. Four injections at intervals of 12 hr were given before the training procedure (for details, see Materials and Methods). For each injection, 1.0 µl of saline or the oligonucleotide (1 nmol) was injected directly into the dentate gyrus of the hippocampus bilaterally. There was a significant difference between the control group and the IAP antisense group when evaluated by the Mann-Whitney U test (p < 0.05).

Effects of IAP antisense oligonucleotide on hippocampal LTP

To further verify that the observed increase in IAP mRNA expression is associated with memory processing, we have adoptedthe LTP paradigm, an electrophysiological model for learning andmemory (Collingridge and Bliss, 1995), and the same antisensemanipulation for the present investigation. Results indicatedthat IAP antisense oligonucleotide injection to the dentate gyrusmarkedly decreased the expression of in vivo LTP in both the amplitude(41% decrease on the average; t_D = 3.61, p < 0.01; Dunnett's ttest) (Fig. 7A) and slope (37% decrease on the average; t_D = 3.28,p < 0.01) (Fig. 7B) of pEPSP in the hippocampus when comparedwith the tetanization group. There was not a marked differencebetween the tetanization group and the random sequence controlgroup regarding the amplitude of pEPSP (t_D = 0.91, p > 0.05) andslope of pEPSP (t_D = 0.52, p > 0.05).

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Figure 7. Effects of IAP antisense oligonucleotide on LTP in rat hippocampus. Percentage change in the (A) mean amplitude and (B) slope of pEPSPs and SEMs was presented as a function of time after IAP antisense oligonucleotide injection (n = 5) and the random sequence injection (n = 5) versus the tetanization controls (n = 5). The tetanus stimulations that yielded LTP (indicated by arrows) were given at 30, 40, 50, and 60 min. Each stimulation contains five trains at 400 Hz. The duration of stimulation was 50 µ sec at 30 min, 100 µsec at 40 min, 150 µsec at 50 min, and 200 µsec at 60 min, respectively.

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

IAP was first identified as a 50 kDa glycoprotein in the human placenta and hematopoetic cells (Brown et al., 1990) and predictedas a membrane protein containing three domains: an extracellulardomain, a multiple membrane-spanning domain, and an alternativelyspliced intracellular domain (Lindberg et al., 1993). The beliefthat the cDNA cloned in this study is the rat counterpart of humanor mouse IAP is based on two explanations. First, the amino acidsequence of the rat IAP is 93% identical to the mouse IAP and72% identical to the human IAP. Second, the alternative splicingforms for the cytoplasmic tail of the rat IAP are identical tothose of mouse and human. The three forms (A5, A6, and A7 in thisstudy) of IAP identified by PCR differential display in the rathippocampus correspond to form 4, form 3, and form 2 of the mouseor human IAP, respectively. This evidence suggests that form 2,form 3, and form 4 IAP express in the rat brain.

IAP was originally named for its association with the $beta$ ₃ class of integrins on placenta and platelets (Brown et al., 1990).Integrins were named for their links between the extracellularmatrix protein and cytoskeleton (Tamkun et al., 1986). In thenervous system, integrins are involved in anatomical organizationduring development and neurite growth in tissue cultures (Reichardtand Tomaselli, 1991; Defreitas et al., 1995). The possible involvementof integrin-like proteins in neuroplasticity was first examinedby Lynch and colleagues (Staubli et al., 1990; Xiao et al., 1991),who found that antagonists for integrin-binding sites and integrinantibodies block LTP in rat hippocampal slices. Results obtainedin the present study imply that the function of integrin involvedin LTP and neuronal plasticity is possibly regulated by IAP. IfIAP is involved in synaptic modification that occurs during memoryformation through the integrin signaling pathway, there shouldbe integrins on the synaptic plasma membrane (SPM) of the hippocampus.However, antibodies to $alpha$ _v $beta$ ₃ or $alpha$ ₅ $beta$ ₁ integrins did not label anyconventional integrin in the hippocampal SPM (Bahr et al., 1991a,b;Bahr and Lynch, 1992). These observations suggest three possiblemodels for the involvement of hippocampal IAP in the process ofmemory formation. First, the association between hippocampal IAPand conventional integrins is not present in the synaptic area.Interactions between IAP and conventional integrins may affectfasciculation of neurites, which is proposed to be needed forsynapse rearrangement during memory formation (Glanzman et al.,1989; Keller and Schacher, 1990). Second, hippocampal IAP mayregulate the functions of a new class of integrin that is requiredfor the process of memory formation. In the hippocampal SPM, matrixreceptors with smaller molecular weights than conventional integrinsand containing integrin epitopes were identified (Bahr et al.,1997). For example, a 55 kDa synaptic protein was eluted fromaffinity columns by integrin antagonists and labeled by antibodiesto the integrin $alpha$ ₅ $beta$ ₁ (Bahr et al., 1997). IAP may be involvedin regulation of the physiological functions of these unconventionalintegrins. Further evidence suggesting a possible associationbetween the function of integrin and IAP comes from a recent studythat a Drosophila mutant, Volado, which showed impaired memory,is also deficient in $alpha$ -integrin (Grotewiel et al., 1998). Whetherthere is a parallel increase in integrin expression of good-memoryrats in the present study is currently under investigation. Thethird possibility is that a direct interaction between IAP andthe extracellular matrix proteins that is independent of integrinmay exist. This speculation is not surprising because IAP is expressedin some cells with no known integrins, such as erythrocyte (Brownet al., 1990). In this regard, IAP may be viewed as a kind ofcell adhesion molecule the expression of which is enhanced bythe process of memory formation. Some structural features conferon IAP the properties of a cell adhesion molecule. First, theextracellular domain of IAP has a single immunoglobulin variable(IgV)-like structure (Lindberg et al., 1993). The IgV-like structureis the common feature of many cell adhesion molecules in the nervoussystem (Yoshihara et al., 1991). One of the natural ligands forIAP was shown to be the thrombospondin-1 matrix protein, suggestingthat IAP may be directly involved in cell adhesion to matrix proteins(Gao et al., 1996). Second, there are several potential glycosylationsites in IAP. Glycosylation is an important characteristic ofcell adhesion molecules. In addition to being regulated at thetranscriptional and translational levels (Rose, 1995; Schmidt,1995), cell adhesion molecules modified at the post-translationallevel were also found to be related to the process of memory formation(Doyle et al., 1992; Fox et al., 1995; Murphy et al., 1996). Hence,glycosylation of IAP may facilitate adhesion of cell surface tothe matrix. Third, the cytoplasmic tail of IAP possesses alternativesplicing forms. In the cytoplasmic portion, form 4 IAP is eightamino acids longer than form 3, and form 3 is 11 amino acids longerthan form 2. If the cytoplasmic tail is involved in the interactionbetween IAP and the cytoskeleton, differential expression of differentforms of IAP may suggest the reorganization of cytoskeletons requiredfor synaptic modification during memory formation.

In this study, we found that the IAP mRNA level was higher in good-memory rats 3 hr after the avoidance learning. One wouldsuspect that the high IAP mRNA level could be related to individualdifferences in the sensitivity of the animal to electric shock.We then examined this possibility by comparing the expressionof IAP mRNA from untreated rats and rats that received electricshock only with the same parameters as used in training. No differencein IAP mRNA expression between these two groups was found, suggestingthat the IAP mRNA expression in good-memory rats is not attributableto individual differences in their sensitivities to electric shock.The other possibility is that good-memory rats have constitutivelyhigher levels of IAP. Although in the present study we have demonstratedthat IAP antisense injection impaired memory retention and hippocampalLTP in rats, these results do not provide direct evidence regardingthe cause-effect relationship between IAP and memory processing.Ideally, it is best to compare hippocampal IAP mRNA levels beforeand after training in the same animals or to compare IAP mRNAlevels between trained and untrained individuals. However, thefirst suggestion is apparently impossible to implement. The secondis also unfeasible because shock stimulus is an essential componentof the training procedure. It is difficult to distinguish thetrained and untrained groups without including the shock stimulus,although in the control study we have demonstrated that the IAPmRNA level was not different between the shocked animals and theunshocked controls. To overcome this difficulty, we have now consideredan alternative approach for the IAP overexpression design, andthese studies, along with other control experiments, are currentlyunder investigation. On the other hand, we have chosen animalswith retention scores of 600 sec and <80 sec for the present study.This cutoff provides the advantage of assuring good retentionversus poor retention rats. It does not necessarily mean thatthose animals with a retention score falling between 80 and 600sec did not learn; instead, it is most likely that these animalswere in a state of an approach-avoidance conflict (dark vs shock)during the retention test. This suggestion is made on the basisof the finding that the memory retention of the animal improvesas the shock intensity increases within a moderate intensity range(Riess, 1970). Accordingly, the number of animals showing middleretention scores decreases. Moreover, there were no apparent differencesin other behavioral aspects between the good-memory and poor-memoryrats, such as their responses to handling stress (our unpublishedobservations).

To further demonstrate the relationship between IAP mRNA expression and memory function, we have conducted the IAP regulationstudy. NMDA is known as an agonist for the NMDA type of glutamatereceptors. Activation of NMDA receptors has been shown to be involvedin many forms of learning and memory (Izquierdo, 1991) as wellas LTP (Collingridge and Bliss, 1995). At the subcellular level,activation of the NMDA receptor induces a number of biochemicalevents, including Ca²⁺ influx, protein phosphorylation, nitric oxide synthesis, andimmediate-early gene expression (Connor et al., 1988; Cole etal., 1989; Bading and Greenberg, 1991; Chetkovich et al., 1991;Nei et al., 1996). Recently, the effect of NMDA receptor activationat the intercellular level is emerging. Fazeli and colleagues(Fazeli et al., 1994; Wang et al., 1992) have demonstrated thatthe NMDA-dependent increase in neuronal cell adhesion moleculesand amyloid precursor protein follows the induction of LTP inthe dentate gyrus of rats. The induction of IAP mRNA by NMDA inthe present study together with the above results further supportsthe role of IAP gene expression in memory processing. In additionto NMDA, both amphetamine and carbachol are well known to facilitatememory processing. Amphetamine was suggested to improve memoryretention through activation of the adrenergic receptors, andpossibly finally via activation of NMDA receptors in the hippocampus(Lee et al., 1993; Cammarota et al., 1995; Izquierdo et al., 1995).Carbachol should act directly on muscarinic cholinergic receptorsto facilitate memory. In the present study, we found that, similarto the effect of NMDA, amphetamine markedly increased the IAPmRNA level in the hippocampus. However, carbachol injection waswithout such an effect. These results together suggest that NMDAand amphetamine may act through the enhancement of cell adhesionto extracellular matrix proteins to facilitate memory formation,whereas the effect of carbachol is not mediated through the IAPsignaling pathway. Last, application of the IAP antisense oligonucleotideimpaired memory retention and hippocampal LTP in rats. Althoughthe distribution of antisense oligonucleotide in the dentate gyrusis not directly examined in the present study, in another reportSchmidt et al. (1995) demonstrated a successful diffusion of labeledantisense oligonucleotide in the endomeningeal cell layer afterintraperimeningeal cavity injection in goldfish. The pattern ofantisense penetration and distribution in the mammalian brainshould be examined further.

In summary, with use of the PCR differential display method we have identified, cloned, and sequenced the IAP gene in therat hippocampus. Both quantitative RT-PCR and in situ hybridizationanalyses have demonstrated a higher expression of IAP mRNA levelin rats showing good retention performance. Both NMDA and amphetamine,which are known to facilitate memory retention in rats, also significantlyincreased IAP mRNA level in the hippocampus. On the other hand,the IAP antisense oligonucleotide markedly impaired memory retentionand decreased the magnitude of LTP. This has been the first studyto identify specific genes associated with memory formation ofinhibitory avoidance learning in mammals. Other candidate genesare currently under investigation.

  FOOTNOTES

Received Dec. 8, 1997; revised March 5, 1998; accepted March 10, 1998.

This work was supported by a research fund from the Institute of Biomedical Sciences, Academia Sinica, Taipei, Taiwan, Republicof China.
Correspondence should be addressed to Dr. Eminy H. Y. Lee, Institute of Biomedical Sciences, Academia Sinica, Taipei 115,Taiwan, Republic of China.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Bading H, Greenberg ME (1991) Stimulation of protein tyrosine phosphorylation by NMDA receptor activation. Science 253:912-914[Abstract/Free Full Text].
Bahr BA, Lynch G (1992) Purification of an Arg-Gly-Asp selective matrix receptor from brain synaptic plasma membranes. Biochem J 281:137-142.
Bahr BA, Sheppard A, Lynch G (1991a) Fibronectin binding by brain synaptosomal membranes may not involve conventional integrins. NeuroReport 2:13-16[Web of Science][Medline].
Bahr BA, Sheppard A, Vanderklish PW, Bakus BL, Capaldi D, Lynch G (1991b) Antibodies to the alpha v beta 3 integrin label a protein concentrated in brain synaptosomal membranes. NeuroReport 2:321-324[Web of Science][Medline].
Bahr BA, Staubli U, Xiao P, Chun D, Ji ZX, Esteban ET, Lynch G (1997) Arg-Gly-Asp-Ser-selective adhesion and the stabilization of long-term potentiation: pharmacological studies and the characterization of a candidate matrix receptor. J Neurosci 17:1320-1329[Abstract/Free Full Text].
Brown E, Hooper L, Ho T, Gresham H (1990) Integrin-associated protein: a 50 kDa plasma membrane antigen physically and functionally associated with integrins. J Cell Biol 111:2785-2794[Abstract/Free Full Text].
Cammarota M, Izquierdo I, Wolfman C, Levi de Stein M, Bernabeu R, Jerusalinsky D, Medina JH (1995) Inhibitory avoidance training induces rapid and selective changes in ³[H]AMPA receptor binding in the rat hippocampal formation. Neurobiol Learn Mem 64:257-264[Web of Science][Medline].
Campbell IG, Freemont PS, Foulkes W, Trowsdale J (1992) An ovarian tumor marker with homology to vaccinia virus contains an IgV-like region and multiple transmembrane domains. Cancer Res 52:5416-5420[Abstract/Free Full Text].
Castellucci VF, Kennedy TE, Kandel ER, Goelet P (1988) A quantitative analysis of 2-D gels identifies proteins in which labeling is increased following long-term sensitization in Aplysia. Neuron 1:321-328[Web of Science][Medline].
Chetkovich DM, Gray R, Johnston D, Sweatt JD (1991) N-methyl-D-aspartate receptor activation increases cAMP levels and voltage-gated Ca²⁺ channel activity in area CA1 of hippocampus. Proc Natl Acad Sci USA 88:6467-6471[Abstract/Free Full Text].
Cole AJ, Saffen DW, Baraban JM, Worley PF (1989) Rapid increase of an immediate early gene messenger RNA in hippocampal neurons by synaptic NMDA receptor activation. Nature 340:474-476[Medline].
Collingridge GL, Bliss TVP (1995) Memories of NMDA receptors and LTP. Trends Neurosci 18:54-56[Web of Science][Medline].
Connor JA, Wadman WJ, Hockberger PE, Wong RK (1988) Sustained dendritic gradients of Ca²⁺ induced by excitatory amino acids in CA1 hippocampal neurons. Science 240:649-653[Abstract/Free Full Text].
Davis HP, Squire LR (1984) Protein synthesis and memory: a review. Psychol Bull 96:518-559[Web of Science][Medline].
DeFreitas MF, Yoshida CK, Frazier WA, Mendrick DL, Kypta RM, Reichardt LF (1995) Identification of integrin alpha 3 beta 1 as a neuronal thrombospondin receptor mediating neurite outgrowth. Neuron 15:333-343[Web of Science][Medline].
Doyle E, Nolan PM, Bell R, Regan CM (1992) Hippocampal NCAM180 transiently increases sialylation during the acquisition and consolidation of a passive avoidance response in the adult rat. J Neurosci Res 31:513-523[Web of Science][Medline].
Fazeli MS, Breen K, Errington ML, Bliss TV (1994) Increase in extracellular NCAM and amyloid precursor protein following induction of long-term potentiation in the dentate gyrus of anaesthetized rats. Neurosci Lett 169:77-80[Web of Science][Medline].
Fox GB, O'Connell AW, Murphy KJ, Regan CM (1995) Memory consolidation induces a transient and time-dependent increase in the frequency of neural cell adhesion molecule polysialylated cells in the adult rat hippocampus. J Neurochem 65:2796-2799[Web of Science][Medline].
Frohman MA, Dush MK, Martin GR (1988) Rapid production of full-length cDNAs from rare transcripts: amplification using a single gene-specific oligonucleotide primer. Proc Natl Acad Sci USA 85:8998-9002[Abstract/Free Full Text].
Gao AG, Lindberg FP, Finn MB, Blystone SD, Brown EJ, Frazier WA (1996) Integrin-associated protein is a receptor for the C-terminal domain of thrombospondin. J Biol Chem 271:21-24[Abstract/Free Full Text].
Glanzman DL, Kandel ER, Schacher S (1989) Identified target motor neuron regulates neurite outgrowth and synapse formation of aplysia sensory neurons in vitro. Neuron 3:441-450[Web of Science][Medline].
Goelet P, Castellucci VF, Schacher S, Kandel ER (1986) The long and the short of long-term memory-a molecular framework. Nature 322:419-422[Medline].
Grotewiel MS, Beck CDO, Wu KH, Zhu XR, Davis RL (1998) Integrin-mediated short-term memory in Drosophila. Nature 391:455-460[Medline].
Huang AM, Lee EHY (1995) Role of hippocampal nitric oxide in memory retention in rats. Pharmacol Biochem Behav 50:327-332[Web of Science][Medline].
Izquierdo I (1991) Role of NMDA receptors in memory. Trends Pharmacol Sci 12:128-129[Medline].
Izquierdo I, Fin C, Schmitz PK, Da Silva RC, Jerusalinsky D, Quillfeldt JA, Ferreira MB, Medina JH, Bazan NG (1995) Memory enhancement by intrahippocampal, intraamygdala, or intraentorhinal infusion of platelet-activating factor measured in an inhibitory avoidance task. Proc Natl Acad Sci USA 92:5047-5051[Abstract/Free Full Text].
Jansen JG, Vrieling H, van Zeeland AA, Mohn GR (1992) The gene encoding hypoxanthine-guanine phosphoribosyltransferase as target for mutational analysis: PCR cloning and sequencing of the cDNA from the rat. Mutat Res 266:105-116[Web of Science][Medline].
Keller F, Schacher S (1990) Neuron-specific membrane glycoproteins promoting neurite fasciculation in Aplysia californica. J Cell Biol 111:2637-2650[Abstract/Free Full Text].
Lee EHY, Ma YL (1995) Amphetamine enhances memory retention and facilitates norepinephrine release from the hippocampus. Brain Res Bull 37:411-416[Web of Science][Medline].
Lee EHY, Hung HC, Lu KT, Chen WH, Chen HY (1992) Protein synthesis in the hippocampus associated with memory facilitation by corticotropin-releasing factor in rats. Peptides 13:927-937[Web of Science][Medline].
Lee EHY, Lee CP, Wang HI, Lin WR (1993) Hippocampal CRF, NE, and NMDA system interactions in memory processing in the rat. Synapse 14:144-153[Web of Science][Medline].
Liang P, Pardee AB (1992) Differential display of eukaryotic messenger RNA by means of the polymerase chain reaction. Science 257:967-971[Abstract/Free Full Text].
Liang P, Averboukh L, Pardee AB (1993) Distribution and cloning of eukaryotic mRNAs by means of differential display: refinements and optimization. Nucleic Acids Res 21:3269-3275[Abstract/Free Full Text].
Lindberg FP, Gresham HD, Schwarz E, Brown EJ (1993) Molecular cloning of integrin-associated protein: an immunoglobulin family member with multiple membrane-spanning domains implicated in alpha v beta 3-dependent ligand binding. J Cell Biol 123:485-496[Abstract/Free Full Text].
Mawby WJ, Holmes CH, Anstee DJ, Spring FA, Tanner MJ (1994) Isolation and characterization of CD47 glycoprotein: a multispanning membrane protein which is the same as integrin-associated protein (IAP) and the ovarian tumour marker OA3. Biochem J 304:525-530.
Murphy KJ, O'Connell AW, Regan CM (1996) Repetitive and transient increases in hippocampal neural cell adhesion molecule polysialylation state following multitrial spatial training. J Neurochem 67:1268-1274[Web of Science][Medline].
Nei K, Matsuyama S, Shuntoh H, Tanaka C (1996) NMDA receptor activation induces glutamate release through nitric oxide synthesis in guinea pig dentate gyrus. Brain Res 728:105-110[Web of Science][Medline].
Reichardt LF, Tomaselli KJ (1991) Extracellular matrix molecules and their receptors: functions in neural development. Annu Rev Neurosci 14:531-570[Web of Science][Medline].
Reinhold MI, Lindberg FP, Plas D, Reynolds S, Peters MG, Brown EJ (1995) In vivo expression of alternatively spliced forms of integrin-associated protein (CD47). J Cell Sci 108:3419-3425[Abstract].
Riess D (1970) Sidman avoidance in rats as a function of shock intensity and duration. J Comp Physiol Psychol 73:481-485[Web of Science][Medline].
Rose SP (1995) Cell-adhesion molecules, glucocorticoids and long-term-memory formation. Trends Neurosci 18:502-506[Web of Science][Medline].
Schmidt R (1995) Cell-adhesion molecules in memory formation. Behav Brain Res 66:65-72[Web of Science][Medline].
Schmidt R, Brysch W, Rother S, Schlingensiepen KH (1995) Inhibition of memory consolidation after active avoidance conditioning by antisense intervention with ependymin gene expression. J Neurochem 65:1465-1471[Web of Science][Medline].
Staubli U, Vanderklish P, Lynch G (1990) An inhibitor of integrin receptors blocks long-term potentiation. Behav Neural Biol 53:1-5[Web of Science][Medline].
Tamkun JW, DeSimone DW, Fonda D, Patel RS, Buck C, Horwitz AF, Hynes RO (1986) Structure of integrin, a glycoprotein involved in the transmembrane linkage between fibronectin and actin. Cell 46:271-282[Web of Science][Medline].
Tang YP, Kashon ML, Sisk CL (1997) Brain regional-specific regulation of luteinizing hormone-releasing hormone messenger ribonucleic acid in the male ferret: interactions between pubertal maturation and testosterone. Endocrinology 138:4740-4747[Abstract/Free Full Text].
Tully T (1996) Discovery of genes involved with learning and memory: an experimental synthesis of Hirschian and Benzerian perspectives. Proc Natl Acad Sci USA 93:13460-13467[Abstract/Free Full Text].
Wang S, Lees GJ, Bock E, Hamberger A, Haglid KG (1992) Biphasic changes in NCAM level after an NMDA lesion to the hippocampal formation: a quantitative dot-immunobinding assay. J Neurosci Res 33:626-630[Web of Science][Medline].
Wayner MJ, Armstrong DL, Polan-Curtain JL, Denny JB (1993) Role of angiotensin II and AT₁ receptor in hippocampal LTP. Pharmacol Biochem Behav 45:455-464[Web of Science][Medline].
Weiler IJ, Hawrylak N, Greenough WT (1995) Morphogenesis in memory formation: synaptic and cellular mechanisms. Behav Brain Res 66:1-6[Web of Science][Medline].
Xiao P, Bahr BA, Staubli U, Vanderklish PW, Lynch G (1991) Evidence that matrix recognition contributes to stabilization but not induction of LTP. NeuroReport 2:461-464[Web of Science][Medline].
Yoshihara Y, Oka S, Ikeda J, Mori K (1991) Immunoglobulin superfamily molecules in the nervous system. Neurosci Res 10:83-105[Web of Science][Medline].

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