Impaired Conditioned Fear and Enhanced Long-Term Potentiation in Fmr2 Knock-Out Mice

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The Journal of Neuroscience, April 1, 2002, 22(7):2753-2763

Impaired Conditioned Fear and Enhanced Long-Term Potentiation in Fmr2 Knock-Out Mice
Yanghong Gu¹, Kellie L. McIlwain¹, Edwin J. Weeber⁴, Takanori Yamagata¹, Bisong Xu¹, Barbara A. Antalffy², Christine Reyes², Lisa Yuva-Paylor¹, Dawna Armstrong², Huda Zoghbi¹^,³^,⁵, J. David Sweatt⁴, Richard Paylor¹^,⁴, and David L. Nelson¹
Departments of ¹ Molecular and Human Genetics, ² Pathology, and ³ Pediatrics, ⁴ Division of Neuroscience, and ⁵ Howard Hughes Medical Institute, Baylor College of Medicine, Houston, Texas 77030

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

FRAXE mental retardation results from expansion and methylation of a CCG trinucleotide repeat located in exon 1 of the X-linkedFMR2 gene, which results in transcriptional silencing. The productof FMR2 is a member of a family of proteins rich in serine andproline, members of which have been associated with transcriptionalactivation. We have developed a murine Fmr2 gene knock-out modelby replacing a fragment containing parts of exon 1 and intron1 with the Escherichia coli lacZ gene, placing lacZ under controlof the Fmr2 promoter. Expression of lacZ in the knock-out animalsindicates that Fmr2 is expressed in several tissues, includingbrain, bone, cartilage, hair follicles, lung, tongue, tendons,salivary glands, and major blood vessels. In the CNS, Fmr2 expressionbegins at the time that cells in the neuroepithelium differentiateinto neuroblasts. Mice lacking Fmr2 showed a delay-dependent conditionedfear impairment. Long-term potentiation (LTP) was found to beenhanced in hippocampal slices of Fmr2 knock-out compared withwild-type littermates. To our knowledge, this mouse knock-outis the first example of an animal model of human mental retardationwith impaired learning and memory performance and increased LTP.Thus, although a number of studies have suggested that diminishedLTP is associated with memory impairment, our data suggest thatincreased LTP may be a mechanism that leads to impaired cognitiveprocessing aswell.

Key words: FRAXE syndrome; mental retardation; Fmr2; knock-out; memory; behavioral test; LTP

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mutation of FMR2 is associated with nonsyndromic and mild mental impairment. Delays in language development are particularlyprominent. Expansion and methylation of a CCG repeat in the 5'untranslated region (UTR) of exon 1 of FMR2 is the most commonlesion and results in a fragile site (FRAXE) on chromosome Xq28and the reduction of FMR2 gene expression (Knight et al., 1993;Brown, 1996). Expansion of the FRAXE CCG repeat is quite rare,with an incidence estimated to be <1:50,000 (Allingham-Hawkinsand Ray, 1995; Brown, 1996). The FRAXE phenotype is primarilycharacterized by mild mental retardation, accompanied by a numberof inconsistent symptoms, including a long, narrow face, mildfacial hypoplasia, a high-arched palate, irregular teeth, hairabnormality, angiomata, clinodactyly, thick lips, and nasal abnormalities(Hamel et al., 1994; Knight et al., 1994, 1996; Mulley et al.,1995; Carbonell et al., 1996; Murgia et al., 1996). Some FRAXEpatients also have behavioral deficits, such as attention deficit,hyperactivity, and autistic-like behavior. Two patients with internaldeletions of the FMR2 gene had similar phenotypes (Gedeon et al.,1995), supporting the notion that FMR2 is solely responsible forFRAXE mental retardation. The most abundant FMR2 transcript is9.5 kb and is expressed at high levels in adult brain, placenta,and several fetal tissues such as liver and lung (Gecz et al.,1996; Gu et al., 1996). Detailed adult brain expression studiesby Northern blot analysis showed high expression in hippocampusand amygdala (Chakrabarti et al., 1996). FMR2 consists of 22 exonsthat span ~500 kb of Xq28 and encodes a 1311-amino acid proteinwith a predicted molecular mass of 141 kDa (Gecz et al., 1997).The mouse ortholog Fmr2 has been characterized and shares 77%identity at the nucleotide level and 86% homology at the aminoacid level. In situ hybridization studies have located Fmr2 mRNAin the hippocampus, the piriform cortex, Purkinje cells, and thecingulate gyrus (Chakrabarti et al., 1998).

The function of FMR2 remains elusive. FMR2 is hypothesized to be a transcriptional activator. It shares significant homology(20-35% amino acid identity) with three autosomal genes: AF4 (Guet al., 1992), LAF4 (Ma and Staudet, 1997), and AF5Q31 (Taki etal., 1999). All proteins of the FMR2 family are rich in serineand proline residues, share several highly similar regions suggestingfunctional motifs, and exhibit features of proteins involved intranscriptional regulation. A recent study has found that AF4and LAF4 have transcriptional transactivation potential and thatLAF4 possesses no specific DNA binding capacity (Ma and Staudet,1997).

To model FRAXE mental retardation and to further understand the function and expression of Fmr2, we replaced a portion ofthe Fmr2 gene with the Escherichia coli lacZ gene under the controlof the Fmr2 promoter. This allowed study of Fmr2 expression duringembryonic development and in a variety of tissues using 5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside(X-Gal) staining. Fmr2 knock-out (KO) mice and their wild-type(WT) littermates were examined for gross anatomical structures,lacZ expression, behavioral abnormalities, and electrophysiologicalresponses in neurons of the hippocampus. We report here impairmentsin conditioned fear and hot plate analgesia, as well as enhancedlong-term potentiation (LTP) in Fmr2 KO male mice. These resultssuggest a role for FMR2 in regulating synaptic plasticity andthat its absence in humans and mice can alter neuronal functionand memoryformation.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Construction of pfmr2-Xgal and transfection
The targeting vector pfmr2-Xgal was composed of pKOScrambler V924 (Lexicon Inc., Woodlands, TX), a 6.5 kb Fmr2 BamHI-EheIfragment of the Fmr2 promoter and exon1 5' UTR, and a 4.5 kb lacZand a bacterial neomycin (neo) gene fragment, along with a 3.5kb EheI-SalI fragment of Fmr2 intron 1. A 4.8 kb SalI exon 1 regionfragment was subcloned from bacterial artificial chromosome (BAC)14637 (Genome Systems, St. Louis, MO). One SalI site was fromthe BAC vector. Another SalI site was from Fmr2 intron 1. The7.0 kb BamHI fragment containing Fmr2 exon 1 was subcloned fromBAC 14636. The blunted HindIII-SalI fragment containing the lacZand neo genes was ligated with EheI-digested pfmr2-exon 1, whichwas made by ligation of a 6.5 kb BamHI-NotI fragment derived fromthe 7.0 kb BamHI fragment, a 3.5 kb NotI-SalI fragment from a4.8 kb SalI fragment, and BamHI- and SalI-digested pKOScramblerV924. The 14.5 kb AscI-SalI fragment containing the 6.5 kb Fmr2promoter and exon 1 fragment, 4.5 kb lacZ and neo fragment, and3.5 kb intron 1 fragment from pfmr2-exon 1 was cloned back intoAscI- and SalI-digested, modified pKOScrambler V924, containinga 1.8 kb RsrII thymidine kinase fragment. This construct pfmr2-Xgalwas linearized by SalI and introduced into 129Sv ES cells by electroporation.The positive clones were selected by G418 (Mansour et al., 1988).

Generation and analysis of chimeric and knock-out mice
The positive clones were injected into a C57BL6 blastocyst, and the blastocyst was transferred to pseudopregnant female mice.Chimeric mice were crossed back with C57BL6 wild-type animals.Mice tails from offspring were digested with 0.3 mg/ml proteinaseK in 700 µl of 50 mM Tris, pH 7.5, 50 mM EDTA, pH 8.0, 100 mMNaCl, 0.5 mM spermidine, and 1% SDS solution at 55°C overnight.DNA was spooled out by adding 2 volumes of 100% ethanol into 400µl supernatant. Ten micrograms of DNA were XbaI-digested overnightand run in a 1% agarose gel for 8 hr to overnight. A Genescreennylon filter was used to transfer DNA from an agarose gel, hybridizedwith a 1.5 kb XbaI-SalI fragment probe in 1.5× SSPE, 1% SDS, and0.5% fat-free milk at 65°C overnight, and then washed with 2×SSC and 1% SDS threetimes.

Reverse transcription-PCR
Total RNA was isolated from mouse brain, lung, skeletal muscle, spinal cord, heart, spleen, liver, and kidney with TRIzol(Invitrogen, Gaithersburg, MD) according to the manufacturer'sprotocol. RNA was reverse-transcribed as described previously(Gu et al., 1996). Reverse transcription (RT)-PCR was performedwith primers mfmr2-1 (5'-GGT AAA GCT CGT TGG CTG TG-3') and mfmr2-2(5'-GAA ATC TTG CGG GAA TCT CAG-3') or mfmr2-550 (5'-GGA ATG GGAACG AAG GAA TC-3') and mfmr2-580 (5'-CTG GTG AGA TGG GAT CAT TC-3')for the Fmr2 gene. Control primers were MA8 (5'-CCG TGT ACT ACCTTG ATG CTG TAG-3') and MA11 (5'-CAA TAA TGA CTG GCA TCT CAG GC-3')for the AF5q31 mouse ortholog. PCR was performed at 95°C for a5 min initial denaturing, followed by 35 cycles of denaturationat 95°C for 45 sec, annealing at 55°C for 45 sec, and extensionat 72°C for 1 min 20 sec. The final extension was 7min.

X-Gal staining
Embryos were dissected in cold PBS, and the skin of embryonic day 15 and 17 embryos was peeled off. Newborn mice were dividedinto two sagittal sections, whereas adult mice were dissected,and their organs were removed. Embryos or adult organs were fixedin 4% paraformaldehyde in PBS at 4°C for 30 min to 2 hr, dependingon the stage of embryo, and washed with PBS three times for 10min each time at 4°C for the first time and at room temperaturefor the second and third times. The embryos or organs were equilibratedwith 0.02% NP-40 and 0.01% NaOH in PBS and incubated in PBS containing1 mg/ml X-Gal, 5 mM K₄Fe(CN)₆, 5 mM K₃Fe(CN)₆, 0.02% NP-40, and0.01% NaOH at 30°C overnight. The samples were post-fixed with4% paraformaldehyde in PBS at 4°C for 30 min with shaking. Formicroscopic examination, the fresh organs were cut on a cryostat,and sections were briefly fixed in 4% paraformaldehyde in PBSat 4°C and stained with X-Gal solution overnight. Whole mountsof embryos stained with X-Gal were embedded in paraplast and cut.All sections were counterstained with nuclear fastred.

Behavioral testing
Animals. Behavioral testing was performed on Fmr2 mutant and wild-type mice. Mice were housed three to five per cage in aroom with a 12 hr light/dark cycle (lights on at 6 A.M. and offat 6 P.M.) with access to food and water ad libitum. In general,behavioral testing was performed between 9 A.M. and 5 P.M. Experimentswere conducted by an experimenter blind to the genotypes of themice. Fourteen KO and 11 wild-type males were tested on the fullbehavioral test battery (batch 1). Batch 1 mice were ~2-3 monthsof age when testing began. A separate batch of 11 KO and 12 WTmale mice (batch 2) was used to replicate significant effectsfrom the conditioned fear and hot plate tests. Mice from batch2 were 8-9 months of age when tested. Animals in batches 1 and2 were tested at the F2 generation (129SvEvTac × C57BL/6J F2).A third batch of 17 mutant and 18 wild-type male mice was usedto further examine whether the conditioned fear effect was delay-dependent.Mice from batch 3 were ~3-5 months old at the beginning of testing.Animals from batch 3 were backcrossed onto the C57BL/6J backgroundfor one more generation. All behavioral testing procedures wereapproved by the National Institute of Mental Health Animal Careand Use Committee and followed the National Institutes of Healthguidelines Using Animals in Intramural Research.
Neurological exam. The neurological screen was adapted from that of Irwin (1968), which is commonly used for pharmaceuticalapplications to screen for major neurological effects of new drugcompounds. This neurological screen is also similar to phase 1of the SHIRPA (SmithKline Beecham Pharmaceuticals; Harwell, MRCMouse Genome Centre and Mammalian Genetics Units; Imperial CollegeSchool of Medicine at St. Mary's; Royal London Hospital, St. Bartholomew's;and the Royal London School of Medicine Phenotype Assessment)screen used to identify behavioral phenotypes in ENU mutant mice(Rogers et al., 1997). The mouse was placed into an empty cageand observed for 1 min. Several behavioral responses were assessed(i.e., wild running, freezing, licking, jumping, sniffing, rearing,movement throughout the cage, urination, and defecation). Posturalreflexes were then evaluated by first determining whether themouse splayed its limbs in response to rapid vertical and horizontalcage movement. The righting reflex, whisker touch response, eyeblink, and ear twitch were then evaluated. Several simple motorresponses were evaluated using a wire suspension test and a verticalpole test. In the wire suspension test, the mouse was suspendedfrom a single wire (2 mm) by its forepaws, with time on the wirescored for a maximum of 60 sec. In the vertical pole test, a mousewas placed on a cloth tape-covered pole (1.9 cm diameter and 43cm long); the end of the pole was then lifted to a vertical position;and the time a mouse stayed on the pole was recorded for a maximumof 60 sec. These values are converted to the following pole testscores: fell before the pole reached a 45 or 90° angle, 0 or 1,respectively; fell in 0-10 sec, 2; 11-20 sec, 3; 21-30 sec, 4;31-40 sec, 5; 41-50 sec, 6; 51-60 sec, 7; stayed on for 60 secand climbed halfway down the pole, 8; climbed to the lower halfof the pole, 9; climbed down and off in 51-60 sec, 10; 41-50 sec,11; 31-40 sec, 12; 21-30 sec, 13; 11-20 sec, 14; and 1-20 sec,15. During each test, any abnormal behavioral responses, suchas hindlimb clutching, were recorded. The mouse was then weighed,and its body temperature was assessed using a rectal probe (ThermalertTH-5). Other physical features were recorded, including the presenceof whiskers, bald hair patches, palpebral closure, exophthalmos,andpiloerection.
Locomotor activity in the open field. One week after the neurological screen, locomotor activity was evaluated by placinga mouse into the center of a clear Plexiglas (40 × 40 × 30 cm)open-field arena and allowed to explore for 30 min. Overhead incandescentlights provided room lighting that measured ~800 lux inside thetest arenas. In addition, white noise was present at ~55 dB insidethe test arenas. Activity in the open-field was quantitated bya computer-operated Digiscan optical animal activity system [RXYZCM(16), Accuscan Electronics] containing 16 photoreceptor beamson each side of the arena, which divides the arena into 256 equallysized squares. Total distance (locomotor activity), vertical activity(rearing measured by number of photo beam interruptions), andcenter distance (distance traveled in the center of the arena)were recorded. The center distance was also divided by the totaldistance to obtain a center distance/total distance ratio. Thecenter distance/total distance ratio can be used as an index ofanxiety-related responses (Peier et al., 2000). Data were collectedat 2-min intervals over the 30 min test session. Open-field activitydata were analyzed using two-way (genotype × time) ANOVA withrepeatedmeasures.
Light/dark exploration. One week later, mice were tested in the light/dark exploration test, which consisted of a polypropylenechamber (44 × 21 × 21 cm) unequally divided into two chambersby a black partition containing a small opening. The large chamberwas open and brightly illuminated (800 lux), whereas the smallchamber was closed and dark. White noise was present in the roomat ~55 dB in the test chamber. Mice were placed into the illuminatedside and allowed to move freely between the two chambers for 10min. The time to enter the dark and the total number of transitionswere recorded. Data were analyzed using a one-wayANOVA.
Rotarod test. Motor coordination and balance were tested 1 week later using an accelerating rotarod (UGO Basile acceleratingrotarod). The rotarod test was performed by placing a mouse ona rotating drum and measuring the time each animal was able tomaintain its balance walking on top of the rod. Some mice heldon to the rotating drum as they began to fall and rode completelyaround the rod. For these mice, the latency to the first completerevolution was recorded. The speed of the rotarod acceleratedfrom 4 to 40 rpm over a 5 min period. Mice were given four trialswith a maximum time of 300 sec (5 min) and a 30-60 min intertrialrest interval. Rotarod data were analyzed using a two-way (genotype× trial) ANOVA with repeatedmeasures.
Startle and prepulse inhibition of the startle. One week after rotarod testing, prepulse inhibition of acoustic startle responseswas measured using the SR-Lab System (San Diego Instruments, SanDiego, CA) as described previously (Crawley and Paylor, 1997).A test session began by placing a mouse in the Plexiglas cylinderwhere it was left undisturbed for 5 min. A test session consistedof seven trial types. One trial type was a 40 msec, 120 dB soundburst used as the startle stimulus. There were five differentacoustic prepulse plus acoustic startle stimulus trial types.The prepulse sound was presented 100 msec before the startle stimulus.The 20 msec prepulse sounds were at 74, 78, 82, 86, and 90 dB.Finally, there were trials in which no stimulus was presentedto measure baseline movement in the cylinders. Six blocks of theseven trial types were presented in pseudorandom order such thateach trial type was presented once within a block of seven trials.The average intertrial interval was 15 sec (range, 10-20 sec).The startle response was recorded for 65 msec (measuring the responseevery 1 msec) starting with the onset of the startle stimulus.The background noise level in each chamber was ~70 dB. The maximumstartle amplitude recorded during the 65 msec sampling windowwas used as the dependentvariable.
The following formula was used to calculate percent prepulse inhibition of a startle response: 100 $-$ [(startle response onacoustic prepulse plus startle stimulus trials/startle responsealone trials) × 100]. Thus, a high percent prepulse inhibitionvalue indicated good prepulse inhibition; i.e., the subject showeda reduced startle response when a prepulse stimulus was presentedcompared with when the startle stimulus was presented alone. Conversely,a low percent prepulse inhibition value indicated poor prepulseinhibition; i.e., the startle response was similar with and withoutthe prepulse. Acoustic response amplitude data were analyzed usinga one-way ANOVAs. Prepulse inhibition data were analyzed usinga two-way (genotype × prepulse sound level) ANOVA with repeatedmeasures.
Habituation of the acoustic startle response. One week later, habituation of the acoustic startle response was measured. Onehundred startle stimuli (120 dB, 40 msec) were presented to eachmouse. The average interstimulus interval was 15 sec. The maximumresponse to each stimulus was recorded. Averages for the blocksof 10 stimuli were used for the analysis. Startle habituationdata were analyzed using a two-way (genotype × stimulus number)ANOVA with repeatedmeasures.
Pavlovian conditioned fear. Two to 3 weeks later, performance in a conditioned fear paradigm was measured using the FreezeMonitor system (San Diego Instruments). The test chamber (26 ×2 × 18 cm high) was made of clear Plexiglas and surrounded bya photo beam detection system (12 × 10 beams). The bottom of thetest chamber was a grid floor used to deliver a mild electricfoot shock. The test chamber was placed inside a sound-attenuatedchamber (Med Associates; internal dimensions, 56 × 38 × 36 cm).Mice were observed through windows in the front of the sound-attenuatedchamber. A mouse was placed in the test chamber (house lightson) and allowed to explore freely for 2 min. A white noise (80dB), which served as the conditioned stimulus (CS), was then presentedfor 30 sec, followed by a mild (2 sec, 0.5 mA) foot shock, whichserved as the unconditioned stimulus (US). Two minutes later,another CS-US pairing was presented. The mouse was removed fromthe chamber 15-30 sec later and returned to its home cage. Freezingbehavior was recorded using the standard interval sampling procedureevery 10 sec. Responses (run, jump, and vocalize) to the footshock were also recorded. If a mouse did not respond to the footshock, it was excluded from theanalysis.
Twenty-four hours (test battery and replicate batch) or 30 min (delay-dependent experiment) later, the mouse was placed backinto the test chamber for 5 min, and the presence of freezingbehavior was recorded every 10 sec (context test). Two hours later,the mouse was tested for its freezing to the auditory CS. Environmentaland contextual cues were changed for the auditory CS test: a blackPlexiglas triangular insert was placed in the chamber to alterits shape and spatial cues; red house lights replaced the whitehouse lights; the wire grid floor was covered with black Plexiglas;and vanilla extract was placed in the chamber to alter the smell.Finally, the sound-attenuated chamber was illuminated with redhouse lights. There were two phases during the auditory CS test.In the first phase (before CS), freezing was recorded for 3 minwithout the auditory CS. In the second phase, the auditory CSwas turned on, and freezing was recorded for another 3 min. Forthe delay-dependent experiment, the CS test was given 30 min afterthe context test. The number of freezing intervals was convertedto a percent freezing value. Context and CS test data were analyzedusing a one-wayANOVA.
Spatial learning in the Morris water task. Two weeks later, mice were trained in the Morris water task (Morris, 1981) to locatea hidden escape platform in a circular pool (1.38 m diameter)of water (Upchurch and Wehner, 1988). Each mouse was given eighttrials a day, in blocks of four trials for 4 consecutive days,for a total of 32 trials. The time taken to locate the escapeplatform (escape latency) and the distance traveled were determined.After trial 32, each animal was given a probe trial, during whichthe platform was removed and each animal was allowed 60 sec tosearch the pool. The amount of time that each animal spent ineach quadrant was recorded (quadrant search time). The numberof times a subject crossed the exact location of the platformduring training was determined and compared with crossings ofthe equivalent location in each of the other quadrants (platformcrossing).
Escape latency and distance traveled (data not shown) data were analyzed with two-way (genotype × trial block) ANOVAs withrepeated measures. Selective search data in the probe trial wereanalyzed by individual one-way (quadrants) repeated ANOVAs andleast squares design post hoc comparison tests. A one-way ANOVAwas used to compare the quadrant search time and platform-crossingdata for the training quadrant only between KO and wild-typemice.
Anagelsic response using the hot plate test. Two weeks later, the hot plate test was used to evaluate sensitivity to a painfulstimulus. Mice were placed on a 55.0 ± 0.3°C hot plate, and thelatency to the first hindpaw response was recorded. The hind pawresponse was either a foot shake or a paw lick. Hot plate datawere analyzed using a one-wayANOVA.

Preparation of hippocampal slices and electrophysiology
Hippocampal slices (400 µm) were prepared as described previously (Roberson and Sweatt, 1996). Hippocampal slices were bathed(1 ml/min) with artificial CSF (in mM: 125 NaCl, 2.5 KCl, 1.24NaH₂PO₄, 25 NaHCO₃, 10 D-glucose, 2 CaCl₂, and 1 MgCl₂) in aninterface chamber maintained at either 25 or 30°C. The Schaffercollateral synapse was stimulated, and the population EPSP (pEPSP)was recorded in the area CA1 stratum radiatum. Responses weremonitored for 20 min before high-frequency stimulation (HFS) wasgiven to ensure a stable baseline. Measurements are shown as theaverage slope of the pEPSP from six individual traces and arestandardized to 20 min of baseline recordings. Baseline stimulusintensities were adjusted to produce a pEPSP at 50% of the maximalresponse. NMDA receptor-dependent LTP was induced with one orthree sets of HFS, with each set consisting of two trains of 100Hz stimulation for 1 sec, separated by 20 sec. NMDA receptor-independentLTP was induced with three 200 Hz stimulations for 1 sec separatedby 2 min in the presence of the NMDA receptor antagonist AP-5.Stimulus intensities used for the HFS were matched to those usedin the baseline recordings. To minimize day-to-day variabilityin slice preparations and recordings, mutant and wild-type hippocampalslices were prepared simultaneously and placed side by side onthe same recordingchamber.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Creation of Fmr2 knock-out mice

To delete the Fmr2 gene, a replacement vector, pfmr2-Xgal, which carries the lacZ gene under the control of the Fmr2 promoter,was generated. This was accomplished by deleting a portion ofexon 1 of Fmr2 and fusing the 5' UTR of Fmr2 to the lacZ gene16 bp upstream of the Fmr2 ATG start codon (see Materials andMethods). Using positive and negative selection marker genes (Fig.1) 18 different correctly targeted embryonic stem (ES) cell cloneswere identified. Of the 18 clones, 11 were expanded, injectedinto C57/BL6 blastocysts, and transferred to pseudopregnant females.A total of 12 chimeric mice were produced, 11 of which were male.These chimeric mice were crossed with C57/BL6 wild-type females.Of the 11 chimeric males, 2 were infertile, 5 transmitted the129 ES cell genome to a fraction of their offspring, and 4 transmittedthe 129 ES cell genome to all of their offspring. HeterozygousF1 female mice were then crossed with wild-type C57/BL6 male mice.All subsequent progeny, which included null mutant males, heterozygousfemales, and wild-type males and females, were genotyped by Southernblot hybridization with a 1.5 kb SalI-XbaI fragment as the leftarm probe (Fig. 1). KO mice exhibit a 5 kb XbaI fragment, whereasWT mice carry a 6.7 kb XbaI fragment. Heterozygous females carryboth fragments (Fig. 2a).

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Figure 1. Map of Fmr2 knock-out construct and corresponding genomic region. a, Map of mouse Fmr2 targeting construct. The bold lines with arrows at both ends indicate genomic DNA fragments, corresponding to the bold lines with arrows at both ends in b. b, Map of Fmr2 exon 1, promoter region and intron 1 genomic region. The fine line with arrows at both ends represents the 6.7 kb XbaI-digested Southern blot band detected by 1.5 kb SalI-XbaI right probe in wild-type mice. c, Map of Fmr2 knock-out mouse genomic region after homologous recombination with the Fmr2 knock-out construct and Fmr2 promoter, exon 1 and intron 1 region. The fine line with arrows at both ends represents the 5.0 kb XbaI-digested Southern blot band detected by the 1.5 kb SalI-XbaI right probe in knock-out mice.

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Figure 2. a, Southern blot analysis of Fmr2 knock-out mouse tail DNA after digestion with BamHI and hybridization with the 1.5 kb SalI-XbaI right probe (Fig. 1). Lanes 1, 6, Knock-out male mice; lane 2, wild type; lanes 3-5, heterozygote females; lane 7, bacteriophage $lambda$ HindIII marker. b, RT-PCR analysis of Fmr2 knock-out and wild-type mouse adult brain. Lane 1, 100 bp ladder; lane 2, knock-out mouse brain RNA; lane 3, knock-out brain cDNA; lane 4, wild-type mouse brain RNA; lane 5, wild-type mouse brain cDNA. The top wells are products obtained with primer pair mfmr2-1 and mfmr2-2 from Fmr2. The bottom wells contain amplification products using a primer pair (ma8 and ma11) designed from the murine ortholog of the human gene AF5q31 as a control.

Pathological examination and phenotype

Gross and light microscopic examination of brain, kidney, heart, spleen, liver, and lung of knock-out and normal mice as newbornsand adults (8-10 months of age) revealed no differences in grossmorphology (data not shown). We paid special attention to theCNS and found no abnormal microscopic architecture in cortex,hippocampus, striatum, cerebellum, thalamus, and hypothalamus(Fig. 3). Examination of three KO males, which died at young ages,showed no obvious abnormalities in brain, heart, and other organs.Because FRAXE mental retardation has recently been characterizedin humans, and no histological data are available in human FRAXEpatients, subtle changes of organic microstructure in knock-outmice remain a possibility. Some KO mice appeared to be much smallerthan their wild-type littermates, but there was not a reproduciblesignificant difference.

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Figure 3. X-Gal staining of telencephalon or brains of Fmr2 knock-out mice. A, X-Gal staining of telencephalon of embryonic day 10.5. The ganglionic hillock is labeled. B, X-Gal staining of telencephalon of embryonic day 12.5. The wall of cerebra was divided into three zones: matrix zone at the ventricular lumen, intermediate zone, and marginal zone. The neuroblasts for the cerebral cortex migrate out of the inner matrix zone, where critical mitosis occurs, and enter the marginal zone, where they form the cortical plate. The neuroblasts in the cortical plate are no longer able to divide. C, X-Gal staining of cerebra (frontal cortex) at embryonic day 15. The neuroblasts and neuronal cells have not reached the outer one-third zone of cerebral cortex when neuroblasts migrate from inside matrix zone to outside zone, passing the neurons differentiated by neuroblasts migrating out early. D, X-Gal staining of the adult cerebellum. The most highly stained cells are Purkinje cells. E, X-Gal staining of adult brain, cut by coronal section. CA1, CA3, and dentate gyrus of hippocampus are strongly stained by X-Gal. The amygdala is also well stained. F, Enlargement of X-Gal staining of the hippocampus from D. G, Hematoxylin and eosin staining of adult brain by coronal section. No abnormalities are observed. H, Hematoxylin and eosin staining of adult cerebellum. These structures appear normal. GE, Ganglionic eminence; MZ, matrix zone; PP, preplate; IZ, intermediate zone; MaZ, marginal zone; CP, cortical plate; PC, Purkinje cell layer of cerebellum; AM, amygdala; DG, dentate gyrus of hippocampus.

One hundred fifteen F2 male offspring from a cross of heterozygous females with C57/BL6 males were genotyped. Fifty-sevenmice were knock-out, and 56 were wild-type, a ratio consistentwith normal Mendelian inheritance and suggesting an absence ofprenatal lethality. During 13 months of observation, we foundthat 9 of 57 male knock-out mice died, whereas all wild-type micesurvived. This indicates a mortality rate of 15% for the knock-outmice, which is statistically significant at p < 0.01 ( $chi$ ²). Of nine dead knock-out mice, four died at 4 months, three diedat 6-7 months, one died at 3 months, and one died at 10 months.We also examined the heterozygous female mice and found no lethalityin 38 heterozygotes. None of 11 chimeric male mice were dead after2 years. One of six homozygous female mice died at 6months.

Fmr2 expression

To determine whether the Fmr2 gene was inactivated by lacZ gene insertion and to assess transcription of Fmr2 in these mutantmice, different pairs of Fmr2 primers were used to examine theKO mice and normal controls by RT-PCR. No expression of Fmr2 inthe mutant mice could be detected, even with the primer pairsdistal to exon 2. An example of the RT-PCR analysis is shown inFigure 2b. Human FMR2 expression has been studied by Northernblot analysis, RT-PCR, in situ hybridization, and immunohistochemistryin human and mouse (Chakrabarti et al., 1996, 1998; Gecz et al.,1996; Gu et al., 1996; Miller et al., 1999). To study Fmr2 promoteractivation in the KO animals, we characterized expression of theinserted lacZ gene by staining for enzymatic activity. The resultsobtained from X-Gal staining in KO mice were consistent with theresults published from other methods. In addition, our X-Gal stainingprovided more detailed information about Fmr2 expression in additionalorgans and during embryonic development, Brain expression patternswere of particular interest because of the human phenotype. Atmurine embryonic day 10.5, Fmr2 expression begins at the ganglioniceminences of the telencephalon, including the lateral ganglioniceminence (LGE) and the medial ganglionic eminence (MGE), wherethe first group of neuroblasts are differentiated. Most of theother neuroepithelial cells in the telencephalon were still negativeat this time point (Fig. 3A). Some neuroblast cells in the spinalcord also started to express Fmr2 (data not shown). At embryonicday 12.5, in the innermost layer (the matrix zone or germinalventricular zone), critical mitosis of neuroepithelia occurs,and some of neuroepithelial cells differentiate into neuroblaststhat migrate into the outer layer. The outer layer becomes theprimitive plexiform layer (preplate), where neurons and migratingneuroblasts are located. The intermediate zone is composed ofhorizontal cells, neuronal support cells, neuron fibers, and afew migrating neuroblasts. In this stage, X-Gal staining was concentratedin the germinal ventricular zone and in the preplate. There werea few stained cells in the middle region (Fig. 3B). During cerebraldevelopment, the cortical plate of the cerebral cortex is formedby neurons migrating from inside to outside. At embryonic day15.5, the strongest X-Gal staining was apparent, with the entirebody staining dark blue in gross examination, especially the headand extremities. The cerebral cortex showed intensive blue stainingin the cortical plate. The outer marginal zone did not stain.In adult brain, X-Gal staining was found in hippocampus (includingCA1, CA3, and dentate gyrus), cerebral cortex, amygdala, the Purkinjecell layer of the cerebellum, olfactory bulb, striatum, caudatenucleus, epithalamus, thalamus, and entorrhinal cortex (Fig. 3;data not shown). Other tissues also stained by X-Gal includedbones, cartilage (intense), hair follicle (strong in mesenchymalcells of papilla), some alveolar cells in lung, the ciliary andconjunctiva of eye, tongue, tendons, salivary gland, cardiac muscle,and majorvessels.

Evaluation of basic neural functions of Fmr2 KO mice

Because humans with FRAXE/FMR2 deficiency have mental retardation, Fmr2 KO and age-matched wild-type littermates were comparedon a battery of behavioral tasks (see Materials and Methods) todetermine the effects of Fmr2 deficiency in mice. The data demonstratethat Fmr2 KO mice exhibit normal exploratory activity, anxiety-relatedresponses, motor coordination and skill learning, startle responses,sensorimotor gating, and spatial learning performance. Significantdifferences were detected between Fmr2 KO mice and their wild-typecontrol littermates on the conditioned fear paradigm for emotion-basedlearning and memory and the hot plate test for analgesia-relatedresponses.

For the following behavioral indices, the performance of WT and KO mice was not significantly different (p > 0.05): totaldistance traveled or rearing responses in the open field, center/totaldistance ratio measure for anxiety in the open field, total transitionnumber in the light/dark box, time spent walking on the rotarod,acoustic startle response, prepulse inhibition of the acousticstartle response, and habituation of the startle response (datanotshown).

Conditioned fear
Conditioned fear and spatial learning are included in our standard test battery to assess learning and memory performance(McIlwain et al., 2001), and given the phenotype in human FRAXEpatients, we were particularly interested in the performance ofFmr2 KO mice in these tests. During the 24 hr context test, wild-typemice displayed significantly greater levels of freezing than theFmr2 KO mice (p < 0.002; Fig. 4A). The difference between theWT and KO mice on the context test was replicated in a secondreplicate batch of mice (p < 0.004; Fig. 4B). Wild-type mice alsodisplayed significantly more freezing during the CS test comparedwith the KO mice both during the initial battery (p < 0.038) andduring the replication (p < 0.0189). The conditioned fear datademonstrate that Fmr2 KO mice have impaired contextual and auditory-cuedconditioned fear when tested after a 24 hr delay interval.

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Figure 4. Conditioned fear and hot plate analgesia test of Fmr2 knock-out mice. Knock-outs are represented by open bars; normal controls are represented by filled bars. A, First series of contextual and conditioned fear tests 24 hr after CS-US training. n (KO) = 14 males; n (WT) = 11 males. B, Second series of context and conditioned fear tests 24 hr after CS-US training. n (KO) = 11 males; n (WT) = 12 males. C, Third series of context and conditioned fear tests 30 min after CS-US training [n (KO) = 17 males; n (WT) = 18 males] and third series of context and conditioned fear tests 24 hr after CS-US training. D, Hot plate analgesia test of Fmr2 knock-out and normal controls. In the first batch, n (KO) = 14 males; n (WT) = 11 males. In the second batch, n (KO) = 11 males; n (WT) = 12 males.

A final experiment shows that the context impairment is delay-dependent. For this last experiment, F2 generation mice hadbeen backcrossed one generation to C57BL/6 mice. Hemizygous malemice from this N1 backcross generation were tested for contextualand auditory-cued fear conditioning either 30 min or 24 hr aftertraining. Figure 4C shows that, consistent with the previous findings,wild-type mice displayed significantly more freezing during thecontext test compared with Fmr2 KO mice after the 24 hr delay(p < 0.001), but there was no difference in levels of freezingafter the 30 min delay (p > 0.6). In contrast to the previousdata, there were no differences between WT and KO mice duringthe CS test either after the 24 hr or 30 min delay intervals (p> 0.2). Taken together, the conditioned fear data indicate thatFmr2 KO mice have impaired contextual fear conditioning that isdelay-dependent.
The reason that Fmr2 KO mice did not show auditory-cued conditioned fear impairment in this last experiment is unclear butis likely attributable to differences in genetic background. Behavioraldifferences on various tasks after one generation of backcrossinghave been observed before in our research group (R. Paylor, unpublishedobservations).

Hot plate test
The latency to the first hindlimb response in the hot plate test (Fig. 4D) was significantly longer in wild-type comparedwith Fmr2 KO mice (p < 0.0005). This difference in the hot platetest was replicated with another batch of mice (p < 0.00001).These results suggest that Fmr2 KO mice are more sensitive topainful stimuli compared with their wild-type littermates (Fig.4D) and that Fmr2 may be involved innociception.

Spatial learning performance
Data acquired during the probe trial is the best indicators of mice using a spatially biased search strategy to locate theplatform during training. Thus, data acquired during trainingare less informative and are often dissociated from the performanceduring the probe trial (Paylor et al., 1998; Tecott et al., 1998).In the Morris spatial learning task, the time and distance tofind the platform were significantly different between Fmr2 KOand WT mice (p < 0.035; Fig. 5A,B). However, during the probetrials, Fmr2 KO and WT mice selectively searched the area of thepool (p < 0.005) where the platform was located during training,as measured by the number of times they crossed the exact positionof the platform compared with the equivalent site in the otherthree quadrants (Fig. 5C). These data indicate that although KOmice take longer to locate the platform during training, bothKO and WT mice use a spatially biased search pattern.

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Figure 5. Performance of Fmr2 knock-out and wild-type mice on the hidden platform version of the Morris water task. The escape latency in seconds (A) and swim distance in centimeters (B) to locate the hidden platform during training are shown. C, Number of platform crossings for knock-out and wild-type mice during the probe trial. n (KO) = 11 males; n (Wild-type) = 12 males. Data are plotted as the mean ± SEM.

Enhanced long-term potentiation in Fmr2 KO mice

Our behavior data suggest a derangement of normal synaptic function or of synaptic plasticity as a basis for the learningand memory deficits we observed. We therefore undertook characterizationof the physiologic responses of Fmr2 KO animals using the hippocampalslice preparation. We detected no deleterious effects of Fmr2deficiency on baseline hippocampal CA1 synaptic transmission.No significant change was observed in Fmr2 KO mice for the input-outputfunctions for CA1 presynaptic fiber volley amplitudes at increasingintensities of stimulation of the Schaffer collateral inputs (Fig.6A). In addition, paired-pulse facilitation, a form of short-termsynaptic plasticity, was normal in Fmr2 KO mice at interpulseintervals of 20-300 msec (Fig. 6B).

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Figure 6. Electrophysiological responses at Schaffer collateral synapses in area CA1 of hippocampus. A, Loss of Fmr2 had no effect on baseline synaptic transmission in stratum radiatum of the CA1 region of the hippocampus measured in Fmr2 knock-out mice (open squares; n = 14, male) or wild-type mice (closed squares; n = 9, male). B, Paired-pulse facilitation was likewise unaffected in Fmr2-knock-out (n = 14, male) compared with wild-type (n = 11, male) mice.

To study whether loss of the Fmr2 gene affected long-term synaptic plasticity, we performed a series of experiments to evaluateNMDA receptor-dependent and NMDA receptor-independent forms ofLTP at Schaffer collateral synapses. First, we studied LTP inducedusing HFS consisting of two trains of 100 Hz for 1 sec, each trainseparated by 20 sec, to induce NMDA receptor-dependent LTP. Forthis experiment, the temperature of the slices within the interfacechamber was maintained at 25°C, because it has been shown previouslythat electrophysiologic examination at 25°C can potentially revealLTP deficits not normally seen at higher temperatures. Applicationof HFS produced robust and long-lasting potentiation in the pEPSPfrom WT mice. Surprisingly, we observed enhancement of potentiationin the Fmr2 KO mice (Fig. 7A). The observed increase in potentiationwas long-lasting and detectable for up to 3 hr after tetanization(data not shown).

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Figure 7. Enhanced LTP in Fmr2 knock-out mice. A, Fmr2 knock-out hippocampal slices showed enhanced LTP compared with wild types after a modest LTP-inducing protocol consisting of a single set of tetani while maintaining slices at 25°C [60 min after tetanus: n (KO, male) = 9, 167 ± 9%; n (WT, male) = 14, 132 ± 6%; p = 0.003]. B, Enhanced LTP in Fmr2 knock-out hippocampal slices is present after a single set of tetani stimulation while maintaining slices at 32°C [60 min after tetanus: n (KO, male) = 6, 170 ± 11%; n (WT, male) = 6, 150 ± 5%; p = 0.14]. C, Fmr2 knock-out mice maintain the enhanced LTP after three sets of HFS at 32°C [60 min after tetanus: n (KO, male) = 7, 244 ± 18%; n (WT, male) = 5, 189 ± 20%; p = 0.020]. D, In the presence of the NMDA receptor antagonist AP-5 (50 µM), Fmr2 knock-out mice showed enhanced NMDA-independent LTP compared with wild types after three trains of 200 Hz stimulation for 1 sec separated by 4 min at 32°C [60 min after tetanus: n (KO, male) = 6, 155 ± 8%; n (WT, male) = 6, 135 ± 4%; p = 0.038].

To determine whether the enhancement in KO LTP was attributable to a lowering in the threshold for LTP induction, we changedtwo parameters in our LTP induction paradigm. In control slices,increasing the temperature or the amount of HFS delivered to theslice is known to increase the amount and duration of CA1 potentiation(Chetkovich et al., 1993). Increasing the temperature of the interfacechamber from 25 to 32°C resulted in an expected increase in potentiationin wild-type slices to ~150 ± 5% at 60 min after tetanus (Fig.7B). Moreover, increasing from one set to three sets of HFS at32°C increased WT potentiation to 189 ± 20% at 60 min after thefirst tetanus. However, the Fmr2 KOs still exhibited enhancedLTP with both the single set of HFS (170 ± 11% at 60 min) andthe three sets of HFS at 32°C (244 ± 18% at 60 min) (Fig. 7C).These data indicate that the enhancement of LTP is not specificto a particular LTP induction paradigm. Moreover, the data suggestthe interesting possibility that the Fmr2 gene product is somehowinvolved in limiting the magnitude of LTP induced by a given LTP-inducingstimulus.

These results raise the question of whether the enhanced LTP magnitude is selective for the NMDA receptor-dependent componentof LTP. To test this, we induced NMDA receptor-independent LTPwith three trains of 200 Hz stimulation for 1 sec, separated by4 min at 32°C in the presence of the NMDA receptor antagonistAP-5. Wild-type slices showed an increase in potentiation of 135± 4% at 60 min after then first tetanus. Again, the Fmr2 KO micerevealed enhanced potentiation (155 ± 8% at 60 min after the firsttetanus; Fig. 7D). This suggests that the enhanced potentiationin the Fmr2 KO mice is not simply attributable to an augmentationin HFS-induced NMDA receptoractivation.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this study, we successfully generated Fmr2 gene KO mice to model the human FRAXE mental retardation syndrome by replacinga fragment containing parts of the Fmr2 exon 1 and intron witha bacterial lacZ gene. The lacZ gene was controlled by the Fmr2promoter through fusing the 5' UTR of Fmr2 to the lacZ gene. Thetranscript carries the Fmr2 5'UTR and lacZ and produces the $beta$ -galactosidaseenzyme.

The absence of RT-PCR products for Fmr2 after exon 1 in the KO mice demonstrates that replacement of a portion of exon 1 withlacZ and neomycin genes effectively disrupted normal transcriptionand translation of Fmr2, extinguishing its expression. Comparisonof the X-Gal staining pattern in KO male mice with RT-PCR datafrom the normal controls illustrates that X-Gal expression isunder the control of the Fmr2 promoter, and the use of the X-Galstain to study expression patterns has provided more informationabout the temporal and spatial patterns of Fmr2 expression. Forexample, Fmr2 is highly expressed in both ganglionic eminences(LGE and MGE) of the ventral telencephalon at embryonic day 10.5.In contrast, little or no Fmr2 can be found in the dorsal telencephalonat this time. This pattern correlates well with Fmr2 expressioncoincident with differentiation of neuroblasts. The LGE and MGEeventually generate the striatum and the pallidum, componentsof basal ganglia. Recent studies also indicate that a significantnumber of LGE- and MGE-derived neurons migrate tangentially intothe cerebral cortex, becoming a large fraction of the GABAergicinterneurons of the neocortex (de Carlos et al., 1996; Tamamakiet al., 1997; Lavdas et al., 1999; Zhu et al., 1999). The structureof basal ganglia in Fmr2 KO mice is normal, but the distributionof GABAergic interneurons in the neocortex is not known. LTP datafrom hippocampal slices showed that the enhanced LTP is more obviousin KO mice compared with normal control LTP when LTP was examinedin the presence of the GABA receptor blocker bicuculline and suggestedthat the number of GABAergic neurons is not reduced in neocortexor at least inhippocampus.

In the dorsal subdivision of the telencephalon, the postmitotic neuroblasts migrate in a radial manner out of the neuroepitheliumand form the first recognizable cortical layer, the primordialplexiform layer, or preplate (Super et al., 1998). Both the preplateand the ventricular zone express the Fmr2 gene. The ventricularzone, before the neuroepithelial cells begin to differentiateinto neuroblasts, does not express Fmr2. The preplate is thensplit into the superficial zone (marginal zone) at the pial surfaceand the subplate below the cortical plate (CP). These neuronsin the cortical plate take their positions in an "inside-out"sequence, with newly differentiated neurons migrating throughthe existing cells of the CP (Berry and Rogers, 1965; Rakic, 1974).The deeper, more differentiated neurons in the CP strongly expressFmr2. We conclude that Fmr2 expression is strongly associatedwith differentiation of neuroepithelial cells into neuroblastsand neurons (Fig. 3C). We hypothesize that loss of Fmr2 in thesehighly expressing neuroblasts may alter their function, leadingto the behavioral and physiologic effects found in human patientswith FRAXE mental retardation and the mice described here. Itis possible that some of the potential phenotypes are not completelyrevealed because of functional compensation by FMR2 paraloguessuch as AF5Q31, AF4, andLAF4.

The findings from the behavioral and electrophysiological studies confirm that Fmr2 plays a role in CNS function. Fmr2 KOmice displayed a delay-dependent deficit in contextual fear conditioning.In the first set of experiments, contextual and auditory-cuedconditioned fear were impaired in the Fmr2 mutant mice. However,when we studied the delay dependency of the conditioned fear impairment,we observed that the CS impairment was not replicated. Importantly,the contextual fear impairment was replicated in each experiment.These findings suggest that the CS impairment is not necessarilya reliable phenotype. We believe that the CS impairment is dependenton genetic background, because the mice in the final experimentin which the CS impairment was not replicated were backcrossedone generation onto a C57BL/6 genetic background. On the otherhand, the contextual fear impairment appears to be robust andpresent in both mixed F2 generation mice and N1 backcrossedmice.

The contextual fear impairment is delay-dependent. In each experiment, Fmr2-deficient mice displayed significantly less conditionedfear during the 24-hr delay context test. However, the levelsof contextual fear conditioning were similar between Fmr2-deficientand wild-type control mice when the test occurred 30 min afterthe initial training session. These findings indicate that theFmr2-deficient mice learn to associate the shock with the trainingcontext and can remember the context over a short delay interval.Therefore, Fmr2-deficient mice have impaired conditioned fearthat is delay-dependent, which indicates that the Fmr2 proteinplays a role in the memory processes for contextual informationover longerperiods.

Hippocampal and amygdala dysfunction can lead to abnormal conditioned fear (Kim and Fanselow, 1992; Phillips and LeDoux, 1992).Although it is unclear what neural circuits are mediating thebehavioral effects of Fmr2 deficiency, the electrophysiologicalfindings demonstrate that there is abnormal hippocampal functionin the Fmr2-deficient mice. Basic hippocampal synaptic functionappears to be normal in Fmr2-deficient mice. However, LTP is significantlyincreased in the Fmr2 mutant mice. Although an increase in LTPmight appear to be contradictory to mental retardation in thehuman disease, there are at least two other reports showing anincrease in LTP and impaired learning and memory, studies involvingloss of postsynaptic density 95 (PSD95) and loss of protein-tyrosinephosphatase $delta$ (PTP $delta$ ; Migaud et al., 1998; Uetani et al., 2000).The present findings, however, represent the first example ofan animal model of human mental retardation with impaired learningand memory performance and increased LTP. Thus, our data and thatof others suggest that increases in LTP may be fundamental mechanismsthat lead to impaired cognitiveprocessing.

Fmr2 KO mice took more time and longer swim paths to locate the hidden platform during the training phase of the Morris watertask. However, as noted above, for mice, escape latency and escapedistance often do not accurately reflect the search strategy subjectsare using to locate the hidden platform (Paylor et al., 1998;Tecott et al., 1998). Data obtained during a probe trial are criticalfor mice to determine whether they are locating the platform usinga spatially biased search strategy. Fmr2 KO and WT mice displayedsearch patterns that were spatially biased for the training quadrant,suggesting that both genotypes were using a spatially based searchstrategy.

Like the contextual fear-conditioning task, spatial learning also is known to depend on normal hippocampal function. It isunclear at this point why Fmr2 KO mice have impaired contextualfear conditioning but normal spatial learning. It would be prematureto speculate as to the reason for these performance differences.Future investigations evaluating Fmr2 KO mice on a series of learningand memory tasks will be necessary to further study the natureof the learning and memorydysfunction.

The Fmr2-deficient mice also have increased sensitivity to heat stimulus, suggesting that Fmr2 regulates sensory and centralpathways that regulate responses to painful stimuli. Althoughit is unclear how and where Fmr2 is playing its role in regulatingsignals of aversive heat stimuli, these findings suggest thatthe Fmr2 protein plays a role important for sensoryprocessing.

It is important to note that differences in response to painful stimuli could lead to behavioral differences in the conditionedfear test. However, there are several reasons why we do not believethat differences in "pain" sensitivity account for the behavioralimpairments observed in the conditioned fear test. First, Fmr2KO mice have impaired conditioned fear, but they have an increased(not decreased) sensitivity to the heat source in the hot platetest. Therefore, if the reason that Fmr2 KO mice have poor conditionedfear is related to differences in sensitivity to shock, then theresponse of the Fmr2 KO mice on the hot plate test is oppositeof what might have been predicted. Second, the impaired conditionedfear response present in Fmr2 KO mice is delay-dependent. If thereason that Fmr2 KO mice have impaired fear conditioning is relatedto a difference in the sensitivity to shock, then one might havepredicted that they would have had impaired conditioned fear thatis not delay-dependent. Third, the CS test impairment may be relatedto genetic background, because Fmr2 KO mice were not impairedon the CS test when the mutation was backcrossed onto a C57BL/6background. However, the differences on the hot plate test werepresent regardless of the genetic background. Fourth, althoughwe did not present the data, Fmr2 KO mice have similar responsescompared with the WT mice on the tail flick test, suggesting thatFmr2 KO mice do not have a general sensory-processing abnormality,Finally, although we did not perform a shock threshold test todetermine the lowest shock intensity that produces a reliablebehavioral response (i.e., run, jump, and vocalize), all miceincluded in this study were required to exhibit two of these responsesto be included in the analyses. Taken together, we believe thatthe data do not support the hypothesis that the impaired conditionedfear response of Fmr2 mice is related to an attenuated sensoryresponse to the shock stimulus. Further studies will be necessaryto fully understand the nature and mechanisms for both the conditionedfear response and the enhanced sensitivity on the hot platetest.

Reduction of LTP in hippocampus and impairment of the Morris water maze tests have been reported in mice deficient for the $alpha$ isoform of Ca/calmodulin kinase II (Silva et al., 1992) andthe fyn gene (Grant et al., 1992). Enhancement of LTP in hippocampushas been found in mice deficient in the AMPA receptor Glu receptor2 (GluR2; Jia et al., 1996), CB1 (cannabinoids) receptor KO mice(Bohme et al., 2000), and mice deficient in the nociceptin receptor(Manabe et al., 1998). Mice deficient in the CB1 receptor andmice deficient in the nociceptin receptor showed improved memory,whereas mice lacking the AMPA receptor GluR2 displayed severalbehavioral abnormalities, including impaired novelty-induced exploratoryactivity in open-field and object exploration, decreased self-directedbehaviors, and disrupted motor coordination (Jia et al., 1996).These results, taken with those reported here and results fromPSD95 and PTP $delta$ knock-out mice, indicate that enhancement of LTPin the CA1 region of the hippocampus can be associated with avariety of different alterations in behavioraltests.

The mechanism of enhanced LTP in Fmr2 knock-out mice is not clear at this moment. Our results indicate that the enhancementof LTP in Fmr2 KO mice is not selective for NMDA receptor-dependentLTP. Most of the mice with abnormal LTP have been created by knock-outof postsynaptic receptors in neuronal junctions or proteins inpostsynaptic dendrites, whereas Fmr2 is a nuclear protein, a memberof a new family of putative transcription factors, including AF4,LAF4, and AF5q31. Evidence has shown that the late stage of LTPrequires transcription (Nguyen et al., 1994); thus, it is possiblethat Fmr2 is a component of the receptor signal transduction pathwayin the nucleus that connects the initial ion channel change atthe early stage of LTP with the new transcription in the nucleusduring the late stage of LTP. However, this model does not explainthe enhancement of early, transcription-independent phases ofLTP. Overall, at this point the only conclusion we can draw fromour data is that the Fmr2 gene product appears to be somehow involvedin limiting the magnitude ofLTP.

It is interesting to note that there is an increased mortality rate in all four knock-out mice that display enhancement ofLTP in the CA1 region associated with learning and behavioraldefects (AMPA receptor GluR2 knock-out, PSD95 knock-out, and PTP $delta$ and Fmr2 knock-out). PSD95 knock-out mice have a distortion ofthe expected Mendelian ratio between homozygotes and the wild-typeanimals at weaning, demonstrating that some of the homozygotesdie at a very early age, possibly as embryos (Migaud et al., 1998).In mice lacking AMPA receptor GluR2, 20% of the mutants die at2-3 weeks of age (Jia et al., 1996). Sixty percent of PTP $delta$ -deficientmice die at 35 d (Uetani et al., 2000). In Fmr2 knock-out mice,15% of mutants die between 3 and 9 months of age. Although themechanism of early death in these four knock-out mouse modelsis not completely understood and possibly different, connectionsamong them mayexist.

In summary, the Fmr2 KO model suggests that Fmr2 is important for maintenance of the normal function of the CNS. Loss of Fmr2in mice causes learning and memory impairment and abnormalitiesin sensory perception. It is interesting that the phenotypes ofFRAXE patients and Fmr2 null mice both involve higher corticalfunction. At this time, we cannot ascertain the relationship betweenthe behavioral abnormalities seen in humans and those detectedin the mice. Mechanisms causing these phenotypes need furtherstudy. Abnormal LTP (enhancement) in Fmr2 KO mice may partiallyexplain the learning and memory defects, and the Fmr2 KO modelis the first mouse model in which abnormal LTP is associated witha defect in a nuclear protein. Whether similar abnormalities canbe found in human FRAXE patients remains to be investigated, butinvestigations into these phenotypes will be greatly facilitatedby the availability of the Fmr2 KOmodel.

  FOOTNOTES

Received Aug. 29, 2001; revised Jan. 10, 2001; accepted Jan 15, 2001.

This work was supported in part by National Institutes of Health Grants HD38038 and HD29256 and Mental Retardation ResearchCenter Grant HD24064. We thank J. Morales for assistance in producingthefigures.

Correspondence should be addressed to Dr. David L Nelson, Department of Molecular and Human Genetics, Room 902E, Baylor Collegeof Medicine, Houston, TX 77030. E-mail: nelson{at}bcm.tmc.edu.

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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