Protein Phosphatase-1 Regulation in the Induction of Long-Term Potentiation: Heterogeneous Molecular Mechanisms

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The Journal of Neuroscience, May 15, 2000, 20(10):3537-3543

Protein Phosphatase-1 Regulation in the Induction of Long-Term Potentiation: Heterogeneous Molecular Mechanisms
Patrick B. Allen¹, Øivind Hvalby², Vidar Jensen², Michael L. Errington⁴, Mark Ramsay⁵, Farrukh A. Chaudhry³, Timothy V. P. Bliss⁴, Jon Storm-Mathisen³, Richard G. M. Morris⁵, Per Andersen², and Paul Greengard¹
¹ Laboratory of Molecular and Cellular Neuroscience, The Rockefeller University, New York, NY 10021, ² Department of Physiology and ³ Anatomical Institute, Institute of Basic Medical Sciences, University of Oslo, Blindern, N-0317 Oslo, ⁴ Division of Neurophysiology, National Institute for Medical Research, London NW7 1AA, United Kingdom, ⁵ Center for Neuroscience, University of Edinburgh, Edinburgh EH8 9LE, United Kingdom

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Protein phosphatase inhibitor-1 (I-1) has been proposed as a regulatory element in the signal transduction cascade that couplespostsynaptic calcium influx to long-term changes in synaptic strength.We have evaluated this model using mice lacking I-1. Recordingsmade in slices prepared from mutant animals and also in anesthetizedmutant animals indicated that long-term potentiation (LTP) isdeficient at perforant path-dentate granule cell synapses. Invitro, this deficit was restricted to synapses of the lateralperforant path. LTP at Schaffer collateral-CA1 pyramidal cellsynapses remained normal. Thus, protein phosphatase-1-mediatedregulation of NMDA receptor-dependent synaptic plasticity involvesheterogeneous molecular mechanisms, in both different dendriticsubregions and different neuronal subtypes. Examination of theperformance of I-1 mutants in spatial learning tests indicatedthat intact LTP at lateral perforant path-granule cell synapsesis either redundant or is not involved in this form oflearning.

Key words: synaptic plasticity; LTP; phosphoprotein phosphatase-1 (PP-1); inhibitor-1 (I-1); CA1 pyramidal cells; dentate granule cells; perforant path; spatial learning

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Stable changes in synaptic strength can be observed after a range of stimuli in both intact animals and in vitro preparations.This plasticity is a candidate mechanism for information storagethat might contribute to learning and memory formation (Blissand Collingridge, 1993). Recently, attempts have been made toprovide additional insight into the physiological significanceof synaptic plasticity by elucidating and manipulating the underlyingbiochemical mechanisms. From a wide array of studies, it has becomeapparent that enzymes controlling protein phosphorylation at thesynapse are important for the induction and maintenance of long-termchanges in synaptic strength (for review, see Tokuda and Hatase,1998). Among the enzymes involved, phosphoprotein phosphatase-1(PP-1), a serine/threonine phosphatase, has emerged as a prominentregulatory element. PP-1 is a multifunctional enzyme that controlsthe phosphorylation status and activity of a variety of downstreameffector molecules that are known to govern synaptic strength(Greengard et al., 1999). These include NMDA (Blank et al., 1997;Snyder et al., 1998) and AMPA (Yan et al., 1999) glutamate receptors,plus additional components of the calcium signaling cascade, suchas calcium-calmodulin-dependent protein kinase II (Strack et al.,1997) and cAMP response element-binding protein (Bito et al.,1996). PP-1 is highly enriched in dendritic spines and is thereforeappropriately localized for the regulation of excitatory synaptictransmission (Ouimet et al., 1995).

Various pharmacological agents can be used to inhibit PP-1 catalytic activity, and these drugs have been exploited to demonstratea role for PP-1 in controlling synaptic strength. In CA1 pyramidalcells, active PP-1 contributes to the induction of long-term depression(LTD) (Mulkey et al., 1994), whereas inhibition of PP-1 promoteslong-term potentiation (LTP) induction (Blitzer et al., 1995,1998). These studies also implied a physiological role for thePP-1 regulatory protein inhibitor-1 (I-1), providing support fora widely cited theoretical model that had been proposed to accountfor the observed changes in synaptic strength (Lisman, 1989).As a part of this model, calcium influx after NMDA receptor stimulationcontrols the phosphorylation state and activity of I-1; intensesynaptic stimulation is predicted to preferentially activate calcium-calmodulin-dependentadenylyl cyclase, producing an increase in cAMP levels, activationof PKA, and phosphorylation of I-1. This leads to PP-1 inhibition,thereby removing opposition to the actions of calcium-activatedkinases. In this study, we test the physiological role playedby endogenous I-1 in the PP-1-mediated regulation of LTP inductionat excitatory synapses in CA1 and in the dentate gyrus. We findthat synapses differ in their sensitivity to the contributionmade by I-1, indicating that additional PP-1 regulatory elementsare likely to be important for synapticplasticity.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Gene targeting. Murine I-1 clones were isolated from a 129SvJ strain genomic library (Stratagene, La Jolla, CA) using a ratcDNA (Elbrecht et al., 1990) as a probe. Characterization of thelocus revealed an 87 bp exon containing the initiating methionine.Using convenient restriction sites, genomic sequence surroundingthis exon was spliced into the targeting vector pPNT (Tybulewiczet al., 1991). Part of the first intron sequence (1.5 kb) and5.5 kb of the sequence upstream of exon 1 were placed on eitherside of a neo cassette. The targeting vector was transfected intothe E14 embryonic stem cell line (Thompson et al., 1989) by electroporation,followed by G418 (Life Technologies, Gaithersburg, MD) selectionof clones. Two clones identified as positive for homologous recombinationby Southern blotting were injected into blastocysts to producechimeric animals. These were mated to C57Bl/6J (The Jackson Laboratory,Bar Harbor, ME) females, and the heterozygous offspring were matedto generate mutant and wild-type mice. For the electrophysiologyexperiments, mutants derived from both targeted embryonic stemcell clones were used. In addition, one of these lines was backcrossedonto the C57Bl/6J background for three and six generations, andmice from these populations were used for further electrophysiologyand behavioral experiments, respectively. No differences wereobserved between the two lines or between the three generationsof mice used for electrophysiology. All experiments were performedon male mice according to animal careguidelines.

Anatomical studies. Wild-type and littermate mutant mice were deeply anesthetized with pentobarbital (Rikshospitalets Apotek,Oslo, Norway) and perfused through the left cardiac ventriclewith 2 ml of 150 mM NaCl, followed by 50 ml of formaldehyde (freshlydepolymerized from paraformaldehyde; TAAB, Reading, UK) in 0.1M sodium phosphate buffer, pH 7.4 (NaPi). One mutant and one wild-typemouse were perfused with 4% formaldehyde, and the brain was sectionedusing a Vibratome (Technical Products International, Oxford, UK)at 50 µm coronally; another pair was perfused with 1% formaldehydeand sectioned horizontally. Sections were processed free-floatingat room temperature (~22°C) through the following: NaPi rinse;1 M ethanolamine-HCl in NaPi (30 min); 3% newborn calf serum (NCS)in TBS (50 mM Tris-HCl, pH 8.0, and 150 mM NaCl) (30 min); affinity-purifiedantibody G-187 to I-1, final Ig concentration of 110-180 ng/ml(with 0.5% Triton X-100) or 180-280 ng/ml (without Triton) dilutedin TBS containing 1% NCS (overnight); TBS rinse; anti-rabbit Igbiotinylated species-specific whole antibody from donkey (AmershamPharmacia Biotech, Buckinghamshire, UK) diluted 1:100 in TBS (90min); TBS rinse; streptavidin-biotinylated horseradish peroxidasecomplex (Amersham Pharmacia Biotech) diluted 1:100 in TBS (90min); TBS rinse; Tris-HCl rinse; diaminobenzidine 0.5 mg/ml inTris-HCl 50 mM, pH 7.6 (6 min); same plus 0.01 mg/ml H₂O₂ (9 min);Tris-HCl rinse; and mounting in glycerol-gelatin. Triton X-100was added to the TBS for optimum penetration of antibodies toreveal the regional distribution of I-1 (see Fig. 2A,B) but wasomitted for better resolution of cytological details (see Fig.2C-E). For electron microscopy, tissue processed without Tritonwas post-fixed with OsO₄, dehydrated in ethanol, embedded in DurcupanACM (Fluka, Buchs, Switzerland), sectioned, and contrasted withlead and uranyl. The antibody was affinity-purified on recombinantI-1 coupled to Sepharose (Amersham Pharmacia Biotech, Uppsala,Sweden) via isourea linkages (Gustafson et al., 1991) and wasfound to recognize a single band of ~29 kDa by immunoblot analysisof total mouse brain homogenate (data not shown). To estimatethe difference in I-1 protein concentrations underlying the observedregional variation in staining intensity, spot tests were performedsimilar to those by Dale et al. (1986). Aliquots (0.1 µl) of serialdilutions of recombinant I-1 (13,300 down to 4 nM in 20 µM bovineserum albumin in 10 mM Tris-HCl buffer) were immobilized on Millipore(Bedford, MA) cellulose ester filter disks and processed for immunocytochemistryalong with tissue sections. I-1 spot intensities were comparedwith staining intensities from different hippocampal regions atdilutions of antibody giving submaximal staining of granule cellbodies. Because the effective light paths cannot be determined,the actual cellular concentrations of I-1 remain unknown. However,a concentration ratio of greater than 10:1 was suggested betweenthe dentate granule cells and the CA1 pyramidal cells, for dendritesas well as for perikarya. Chemicals for which the source is notspecifically mentioned were from Fluka or Sigma (St. Louis, MO)and were of the highest availablepurity.

Slice electrophysiology. Adult wild-type and mutant male mice (30-40 gm) were killed with halothane (Fluothane; AstraZeneca,London, UK). The brain was removed and cooled to 0-4°C in artificialCSF (ACSF) of the following composition (in mM): NaCl 124, KCl2, KH₂PO₄ 1.25, MgSO₄ 2, CaCl₂ 2, NaHCO₃ 26, and glucose 12, bubbledwith 95% O₂-5% CO₂, pH 7.4. Transverse hippocampal slices (400µm) were cut with a vibratome in cool, bubbled ACSF and placedin an interface chamber exposed to humidified gas and maintainedat a temperature of 28-32°C. To obtain LTP in the dentate gyrus,the induction had to be enhanced by a partial block of GABA_A-mediatedinhibition with ( $-$ )-bicuculline methochloride (6 µM) (Tocris CooksonLtd., Bristol, UK). The resulting hyperexcitability was counteractedby increasing the concentration of Ca²⁺ and Mg²⁺ to 4 mM. In accordance with earlier reports (Wigström and Gustafsson,1983, 1985), a series of control experiments showed that thisprocedure facilitated the induction of LTP in CA1 without significantlychanging the magnitude of LTP. However, under these conditions,the percentage increase of the field EPSP (fEPSP) slope in thedentate is somewhat smaller than that observed in CA1. Orthodromicsynaptic stimulation was delivered alternately (0.2 Hz) throughtwo sharp monopolar tungsten electrodes placed in the outer andmiddle molecular layer in the dentate or in the distal and proximalradiatum layer in the CA1. Extracellular responses were monitoredby two glass electrodes (filled with ACSF) in the correspondingsynaptic layers. In the CA1 region, the most proximal served asthe control and the distal one as the test pathway. In the dentate,alternating between experiments, one of the pathways served asthe control, the other as the test pathway. After stable synapticresponses had been obtained in both pathways for at least 15 min,the test pathway was tetanized (100 Hz, 1 sec). The tetanic stimulationstrength was just above the threshold for generation of a populationspike in response to a single test stimulus. This procedure ensuredthe same effective tetanization strength in all experiments. Thesynaptic strength was assessed by delivering test stimuli at 10sec intervals and measuring the slope of the fEPSP in the middlethird of its rising phase. Six consecutive responses (1 min) wereaveraged and normalized to the mean value obtained 4-7 min beforetetanic stimulation. The data were pooled across animals of thesame genotype. To avoid serial accumulation of data from one genotype,experiments were performed in pairs, with animals selected fromtwo groups (mutant and wild type), and their group identitieswere revealed at the end of the experimental series. Data arepresented as mean ± SEM, and statistical significance was evaluatedusing a two-tailed ttest.

In vivo electrophysiology. Male mice, 5-7 months old, were anesthetized with urethane (1.5 gm/kg, i.p.; Sigma) and held ina semi-stereotaxic apparatus. For experiments in dentate gyrus,a glass recording pipette, filled with ACSF containing pontaminesky blue, was placed 2.0 mm posterior and 1.9 mm lateral to bregmaand advanced into the dentate gyrus. A bipolar stimulating electrode(Rhodes SNE 100; Clark Electromedical Instruments, Reading, UK)was inserted 3.0 mm lateral to lambda and advanced into the angularbundle to activate fibers of the perforant path. The depths ofthe two electrodes were adjusted to produce maximal responsesin the granule cell body layer. Constant current stimuli (50 µsecduration, intensity in the range of 70-120 µA) were deliveredat intervals of 30 sec, and the intensity was adjusted to producea population spike with an amplitude of 1-2 mV. To investigateLTP in area CA1, the recording electrode was positioned 2.0 mmposterior and 2.0 mm lateral to bregma on one side, with the stimulatingelectrode at the same coordinates on the contralateral side. Electrodedepths were adjusted to maximize the synaptic response in stratumradiatum. Test stimuli were delivered at 30 sec intervals, andtetanus parameters were those found in previous experiments tobe optimal for inducing LTP in mice: in dentate gyrus, six trainsof six stimuli at 400 Hz, at twice test intensity, with 100 msecbetween trains, repeated six times at an interval of 20 sec; inarea CA1, 50 stimuli at 100 Hz, repeated twice at an intervalof 30 sec. LTP was assessed for each animal by expressing themean of the values, obtained 45-50 min after the tetanus, as apercentage of the 10 values obtained before the tetanus. Paired-pulsefacilitation, elicited by stimuli of different intensities, deliveredover a range of interstimulus intervals, did not reveal any differencesbetween wild-type and mutant mice (data notshown).

Water maze tests. Testing was performed in an open field water maze 2 m in diameter and filled with opaque water (25 ± 1°C)in a laboratory filled with extramaze cues. Paths taken by themice were monitored with an overhead video camera connected toan image analyzer (HVS Image, Hampton, UK) and an Acorn (Framlingham,UK) computer, running software that sampled the coordinates on-lineat 10 Hz for subsequent automated data analysis. All subjectsswam normally and escaped readily onto the platform. Mice werefirst given four habituation trials without extramaze cues. A40 cm flagged platform was used and moved randomly between spacedtrials [intertest interval (ITI) of 10 min] of 60 sec before themice, if necessary, were guided to the platform by hand. A further16 habituation trials (four per day) were given with a flagged20 cm platform. Spatial training consisted of 32 trials (fourper day) during which the submerged platform remained in a constantposition for each mouse. The first 16 trials were with a 30 cmplatform, and the second 16 were with a 20 cm platform. Trialslasted a maximum of 90 sec, followed by an interval of 20 secon the platform (ITI of 10 min). Transfer tests of 60 sec swimwere given after these trials. Experimenters were blind as tothe genotype of the two animal groupsstudied.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Disruption of the murine I-1 gene

To address the role of I-1 in synaptic plasticity, we used gene targeting to prepare a mouse strain lacking I-1 protein. TheI-1 gene was disrupted in a 129/Ola-derived mouse embryonic stemcell line, using a targeting vector constructed for replacementof the first coding exon of the I-1 gene with a neo cassette (Fig.1A). Homologous recombination was detected by Southern blotting(Fig. 1B). After C57Bl/6J blastocyst injection and embryo transferinto pseudopregnant mothers, chimeric offspring were crossed toC57Bl/6J females, and those animals carrying the mutation werecrossed to generate heterozygous and homozygous mutants. Analysisof the I-1 protein by immunoblotting of hippocampal 1% SDS extractsshowed a single band migrating with an apparent M_r of ~29 kDain wild-type mice. Expression of I-1 protein was reduced by approximatelyhalf in the heterozygous mutant and abolished in the homozygote(Fig. 1C). I-1 mutant mice appeared to be normal in adult bodyand organ weights, gross behavior, longevity, and fecundity (datanot shown).

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Figure 1. A, Depiction of the mouse I-1 genomic locus and the targeting strategy used for gene disruption; a replacement vector was designed to delete a ~400 bp fragment containing the first coding exon of the I-1 gene and to replace it with a ~1.8 kb fragment containing the neomycin resistance gene. Homologous recombination was detected by a reduction in the mobility of a genomic AflII restriction fragment because of an increase in size of ~1.4 kb. B, Southern blot analysis of genomic tail DNA isolated from an I-1 mutant pedigree and digested with AflII. The probe is depicted in A. Wild type, +/+; heterozygote, +/ $-$ ; homozygote, $-$ / $-$ . C, Immunoblot analysis using anti-I-1 antibody. SDS homogenates (1%) were prepared from hippocampi taken from animals of the indicated genotype.

I-1 is enriched in dentate granule cells

Mutant mice showed no staining for I-1 in immunohistochemical analyses of hippocampus (CA1-CA3) and dentate gyrus (Fig. 2A).Nissl staining revealed no overt structural abnormality in themutants (data not shown). In wild-type mice, strong staining forI-1 was seen in dentate gyrus, and much lower levels were detectedin the hippocampus (Fig. 2B); this is consistent with previousreports of I-1 distribution in the rat and primate (Gustafsonet al., 1991; Barbas et al., 1993) (but see Sakagami et al., 1994;Lowenstein et al., 1995). I-1 immunoreactivity in both regionsdecreased gradually from the septal to the temporal pole. Usingantibody concentrations that were supersaturating for dentategyrus, I-1 staining was also detectable in pyramidal cells, includingthose of CA1. I-1 immunoreactivity in the granule cells was concentratedin the cytoplasm of perikarya, avoiding the nuclei of stainedcells. The dendrites and mossy fiber terminal boutons of granulecells were also intensely stained (Fig. 2C,D). Electron microscopyrevealed staining in spines protruding from the granule cell dendritesbut no staining of afferent boutons in the dentate molecular layer(Fig. 2E), indicating that I-1 is predominantly postsynaptic atthese synapses.

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Figure 2. Immunoperoxidase labeling of I-1 in the hippocampal formation (see large box in Fig. 3A) of I-1 homozygous mutant and wild-type mice. A, In the mutant, there is no immunoreactivity. The darkness in the alveus (A) and the stratum lacunosum-moleculare (LM) is attributable to light scattering by the myelinated fibers abundant in these zones; to be visible, the photomicrograph of A was printed at twice the exposure time for wild type. B, In the wild type, the staining in the dentate gyrus, mossy fiber layer in CA3 (MF) terminal zones and LM is much stronger than in other regions. The cellular localization of I-1 in the dentate gyrus dorsal blade is shown by differential interference contrast (C, D) and electron microscopy (E). Granule cell perikarya (g), dendrites (arrows), and mossy fiber boutons (arrowheads) are strongly immunoreactive. E, A labeled spine (s) protruding from an immunopositive dendrite (arrow) receives an asymmetric synapse from an immunonegative nerve ending. A, Alveus; H, hilus; O, stratum oriens; P, stratum pyramidale; R, stratum radiatum; LM, stratum lacunosum-moleculare; MF, mossy fiber layer in CA3; G, stratum granulare; Mi, Mm, Mo, inner, middle, and outer thirds of stratum moleculare of the dentate gyrus. R contains the Schaffer collateral terminals, and Mo and Mm contain the terminals of the lateral and medial perforant path, respectively. Asterisks mark the obliterated hippocampal fissure. Scale bars: A, B, 200 µm; C, 50 µm; D, 10 µm; E, 0.5 µm.

I-1 mutants display a synapse-selective deficit in LTP induction

In view of the regional differences in the pattern of I-1 expression, we examined electrophysiological responses in hippocampusand dentate gyrus of wild-type and I-1 mutant mice (3A,B). Neuronalviability in slices prepared from animals of both genotypes wasequivalent, and there were no differences in either the stimulationstrength necessary to elicit excitatory responses or in the formof evoked responses. The perforant path can be subdivided intoa lateral and a medial component, originating in the lateral andmedial part of the entorhinal cortex, respectively. The lateralperforant path (lpp) makes excitatory synaptic contacts onto dentategranule cell dendrites in the outer third, whereas the medialperforant path (mpp) forms synapses in the middle third of themolecular layer (Hjorth-Simonsen, 1972; Hjorth-Simonsen and Jeune,1972). Physiologically, these two pathways can be distinguishedin slices, because lpp-granule cell synapses show paired-pulsefacilitation, whereas paired stimulation of mpp-granule cell synapsespredominantly causes depression (McNaughton, 1980; Hanse and Gustafsson,1992; Colino and Malenka, 1993; Min et al., 1998). The paired-pulsefacilitation in the outer molecular layer and the paired-pulsedepression in the middle molecular layer, tested at 50 msec interstimulusinterval, were not significantly different in the two groups ofanimals (wild type vs I-1 mutants in lpp, mean ± SEM, 129 ± 5%,n = 7 vs 134 ± 6%, n = 14, p = 0.60; wild type vs I-1 mutantsin mpp, 92 ± 4%, n = 6 vs 85 ± 3%, n = 13, p = 0.11).

LTP in the dentate gyrus was elicited in slices by tetanization of either the mpp or lpp fibers. In the mutants, we observeda striking difference in the ability to produce LTP in these twopathways. Tetanization of mpp gave substantial and equally welldeveloped LTP in wild-type and mutant animals (Fig. 3C). At 45min after tetanization, the values for the slope of the fEPSPin relation to the pretetanic value were 132 ± 10% for wild-type(n = 11) and 132 ± 7% for mutant animals (n = 21). When the lateralperforant path was tetanized, the picture was dramatically different(Fig. 3D). Whereas fEPSP measured 137 ± 5% in wild-type mice (n= 17), the mutants showed only 109 ± 5% (n = 32). This remainingvalue was, however, significantly different from the control input,which showed 98 ± 2% (p = 0.03). In an attempt to confirm theregulatory role of I-1 during LTP induction in the lpp-granulecell synapses, we tried to re-establish LTP by loading granulecells from mutant mice with I-1 or with thiophosphorylated I-1.However, this approach, with both sharp electrodes and patch electrodes,was abandoned because of technical difficulties associated withinjection into the small mouse granule cells.

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Figure 3. I-1 regulates synaptic plasticity at a subset of synapses. A, Schematic of a hippocampal slice. The large box shows the region from which the immunohistochemical section in Figure 2 is taken. The small box indicates the part of CA1 and dentate gyrus in which LTP was studied. B, Diagram of stimulating and recording electrode arrangement in the CA1 (top panel) and in the upper blade of the dentate gyrus (bottom panel). C-E, Pooled data of the extracellular fEPSP slopes evoked in the wild-type (filled circles) and mutant (open circles) mice in the medial perforant path (C), in the lateral perforant path (D), and in the CA1 region (E). For the sake of clarity, nontetanized control pathway responses are not shown. Arrow indicates the time of tetanic stimulation. Vertical bars indicate SEM.

Tetanization of stratum radiatum fibers and recording the fEPSP of CA1 pyramidal cells revealed that LTP at these synapseswas equally strong in wild-type and I-1 mutant mice (Fig. 3E).The radiatum-CA1 fEPSP in wild-type animals measured 154 ± 12%(n = 14) of the pretetanic control value 45 min after tetanization.In slices from I-1 mutant mice, the corresponding fEPSP valuewas 153 ± 9% (n =11).

To corroborate these findings, in vivo recordings were made in anesthetized mice. This preparation gave results that werequalitatively similar to those obtained in slices; recordingsin CA1 did not reveal any significant difference in LTP [wildtype, 120 ± 5% (n = 4); mutant, 122 ± 4% (n = 4), measured at45-50 min after tetanus]. In the perforant path (Fig. 4), LTPof the fEPSP in dentate gyrus was greatly reduced in I-1 mutantmice, becoming insignificant (p = 0.2) at 50 min [wild type, 115.1± 4.1% (n = 7); mutant, 103.6 ± 2.5% (n = 7), measured at 45-50min after tetanus]. The difference in paired-pulse facilitationseen in vitro cannot be exploited to help distinguish betweenthe two pathways in vivo because both lpp and mpp exhibit paired-pulsefacilitation in the intact animal (M. L. Errington, unpublishedobservations; McNaughton and Barnes, 1977). We cannot rule outthe possibility that both mpp and lpp contribute significantlyto test input responses. However, the magnitude of the plasticitydeficit observed in vivo indicated that LTP induction in wholebrain preparations is at least as sensitive to PP1 activity asit is in slices.

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Figure 4. In vivo LTP of the fEPSP in dentate gyrus. After tetanization of the perforant path, LTP in the wild-type group shows significant potentiation, whereas LTP in the mutants declines to baseline over the course of the experiment. Arrow indicates the time of tetanic stimulation. Vertical bars indicate SEM.

It has been proposed that LTD is associated with enhanced phosphatase activity (Lisman, 1989). This proposal was supportedby the observation that pharmacological blockade of PP-1 activityin rat slices prevents NMDA receptor-dependent LTD induction inCA1 (Mulkey et al., 1994). A priori, the I-1 mutants might beexpected to exhibit well developed LTD (unless depression wasalready maximal under basal test conditions). In preliminary experiments,LTD induction in CA1 was similar in wild-type and I-1 mutants(R. Mulkey and R. Malenka, personal communication). We attemptedto elicit perforant path LTD in slices using reported stimulationparadigms (1 Hz for 15 min) (Trommer et al., 1996). In wild-typeanimals, LTD failed to appear in two separate groups of animals:postnatal day 16-19 (n = 12) and adult (n = 4). In the young andthe adult groups, the fEPSP slope measured 92 ± 5 and 109 ± 12%,respectively, relative to control levels, 15 min after cessationof 1 Hz stimulation. Similar results were observed in mutant animalsin which the fEPSP slope after the low-frequency train in thetwo age groups measured 106 ± 6 (n = 11) and 115 ± 7% (n = 7),respectively, relative to control values. In neither the youngnor the adult group was the fEPSP slope significantly differentbetween the wild-type and the mutant animals (p = 0.08 and p =0.72, respectively). There was no observable difference betweenexperiments performed with 2 mM Ca²⁺ and 2 mM Mg²⁺ or in solutions with higher calcium concentration (2.5 mM Ca²⁺ and 1.3 mM Mg²⁺) or 4 mM Ca²⁺ and 4 mM Mg²⁺ with the addition of 6 mM bicuculline to partially block GABA_A-mediatedinhibition.

I-1 mutants perform normally in water maze tests

The rodent hippocampus plays a critical role in the acquisition and retention of spatial memory (O'Keefe and Nadel, 1978).Projection neurons in the entorhinal cortex provide the main excitatoryinput to the hippocampus via the perforant path (Hjorth-Simonsen,1972; Hjorth-Simonsen and Jeune, 1972), and lesions in this relaydisrupt spatial learning in both rats (Schenk and Morris, 1985;Whishaw, 1987; Skelton and McNamara, 1992) and mice (Hardman etal., 1997). We therefore examined the spatial learning performanceof I-1 mutant and wild-type mice in a reference memory task trainedin a 2 m diameter water maze (Morris, 1981). Training was separatedinto two stages with a smaller platform used for the second stageto increase the difficulty of the task and thus the spatial accuracyrequired of the mice. Learning occurred over the first 4 d oftraining in both mutant and wild-type groups. The second set oftrial blocks using the smaller platform produced a similar patternof results but with a more pronounced effect of trial block andagain no difference between mutant and wild-type groups (Fig.5A). The platforms were removed after both training sets, andanimals were examined for any learned preference for the quadrantin which the platform had previously been located. A spatial biasdeveloped for the trained quadrant, and this bias was acquiredat a similar rate for mutant and wild-type mice (Fig. 5B). Therefore,both groups of mice learned the water maze task, indicating thatintact LTP in the lateral perforant pathway is not a requirementfor spatial learning in the water maze.

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Figure 5. Performance in a water maze test. A, Mean escape latencies for mutant and wild-type mice. Initial training was performed using a 30 cm platform (left). ANOVA revealed an effect of blocks of four trials (F_(3,84) = 2.76; p < 0.05), indicating that learning occurred over the 4 d of training, whereas no difference was seen between mutant and wild type (F < 1; p > 0.5). After transfer test 1, subsequent trial blocks were performed using a 20 cm platform (right), and this produced a similar pattern of results: a more pronounced trial effect (F_(3,84) = 7.61; p < 0.001) and again no difference between mutant and wild-type groups (F < 1; p > 0.5). B, Percentage time spent in each of the pool quadrants during transfer tests. After the first training set (top panel), an effect of quadrant was seen (F_(3,84) = 4.63; p < 0.05), but a t test revealed that this was between the adjacent left-training and the adjacent right-training quadrants (p < 0.05). No difference was found between the training quadrant and the adjacent right quadrant. This suggested that the spatial bias was not yet directed toward the training quadrant alone. No genotype group difference between any of the quadrants was seen (F < 1; p > 0.3). Transfer tests performed after the second set of trials with the 20 cm platform (bottom panel) indicated that performance had substantially improved. Again, an effect of quadrant was seen (F_(3,84) = 8.53; p < 0.001). The percentage time spent in the training quadrant was significantly greater relative to both adjacent quadrants (t test: 0.001 < p < 0.05). However, no genotype group difference was found (F = 1; p > 0.3).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Abnormalities in hippocampal LTP have been detected in a large number of genetically manipulated mice, and accompanying deficitsin spatial learning are most consistently associated with electrophysiologicallesions in CA1 (Goda and Stevens, 1996), although this correlationis incomplete (Zamanillo et al., 1999). In I-1 mutant mice, thelpp LTP deficit might be compensated for by intact plasticityin the medial perforant path and/or altered activity at downstreamhippocampal synapses. Therefore, a postulated role for lpp LTPin spatial learning cannot be ruled out. Further tests are beingperformed to analyze the possible contribution of I-1 to additionalbehavioralparameters.

Earlier reports have emphasized the different anatomical (Hjorth-Simonsen, 1972; Hjorth-Simonsen and Jeune, 1972; Steward,1976), physiological (McNaughton, 1980; Hanse and Gustafsson,1992; Colino and Malenka, 1993; Min et al., 1998), and pharmacological(Dahl and Sarvey, 1989; Kahle and Cotman, 1989) characteristicsof the mpp and lpp synapses on dentate granule cells. Here, wedemonstrate distinct biochemical characteristics underlying synapticplasticity in the two pathways. LTP induction at both sets ofsynapses is NMDA receptor-dependent (Hanse and Gustafsson, 1992;Colino and Malenka, 1993; Min et al., 1998), and we show thatI-1 is postsynaptically localized in granule cells at both proximaland distal dendrites. However, the development of LTP in the twopathways, targeting the same population of cells, exhibits a differentialrequirement for protein phosphatase regulation; I-1 is not requiredin the medial perforant path under the conditions of stimulationused but is important in the lateral perforant path. Unfortunately,attempts to rescue lpp LTP by intracellular injection of dentategranule cells were not successful, mainly because of the difficultyin maintaining a constant and low access resistance with the relativelythin patch pipettes required for such small neurons, in particularwith protein-containingelectrodes.

What might be the mechanistic basis of the observed mpp-lpp distinction? One possibility would be that in the medial perforantpath, synaptic strength is not regulated by PP-1. This seems unlikelygiven the sensitivity of synaptic plasticity in this pathway tophosphatase inhibition (Wang et al., 1997). A second possibilityis that excitability in the more distal dendritic subregions isdifferentially sensitive to a given phosphatase substrate(s) andthus differentially sensitive to PP-1 regulation via I-1. Forexample, consider the differential distribution and activity ofion channels found in the apical dendrites of CA1 pyramidal neurons(for review, see Johnston et al., 1999); sodium channels displayan increase in the magnitude of slow inactivation with distancefrom the soma, whereas the density of transient, A-type potassiumchannels increases along the dendrite. Furthermore, the electrophysiologicalproperties of these channels, and hence dendritic excitability,are modulated by protein phosphorylation cascades. A similar heterogeneityin ion channel function may be present in the dendritic tree ofdentate granule cells, with I-1-mediated PP-1 regulation becomingcritical in the distaldendrites.

A third possibility that may account for the differential requirement for I-1 at the different synapses may be the involvementof additional PP-1 regulatory subunits. This possibility appliesequally to Schaffer collateral-CA1 synapses in which an obligatoryrole for I-1 in LTP induction appears unlikely, both in view ofthe relatively weak I-1 expression in these cells and the absenceof interference with LTP seen in the I-1 mutants. Several additionalPP-1 regulatory candidates exist: the PP-1 targeting protein spinophilinis highly enriched in dendritic spines and mediates the controlof AMPA channel activity in striatal neurons (Allen et al., 1997;Yan et al., 1999); neurabin is a structurally related PP-1 bindingprotein that is also present at synapses (Nakanishi et al., 1997;McAvoy et al., 1999). In addition, the NMDA receptor binding proteinyotiao targets both PP-1 and PKA to the NMDA receptor, therebymodulating receptor activity (Westphal et al., 1999). The currentchallenge is to identify the means by which calcium influx mightbe coupled to alterations in the activity of PP-1 as mediatedby these newly characterized regulatory subunits. Preliminarystudies indicate that the association of PP-1 with neurabin maybe regulated by the cAMP pathway (McAvoy et al., 1999).

  FOOTNOTES

Received Dec. 10, 1999; revised Jan. 28, 2000; accepted Feb. 25, 2000.

This work was supported by United States Public Health Service Grants MH 40899 and DA 10044. We thank Peter Ingrassia forassistance with the mousecolony.
Correspondence should be addressed to Patrick B. Allen, Laboratory of Molecular and Cellular Neuroscience, The RockefellerUniversity, 1230 York Avenue, New York, NY 10021. E-mail: allenp{at}rockvax.rockefeller.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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