Impairment of Long-term Potentiation and Associative Memory in Mice That Overexpress Extracellular Superoxide Dismutase

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The Journal of Neuroscience, October 15, 2000, 20(20):7631-7639

Impairment of Long-term Potentiation and Associative Memory in Mice That Overexpress Extracellular Superoxide Dismutase
Edda Thiels¹^,², Nathan N. Urban¹^,², Guillermo R. Gonzalez-Burgos¹, Beatriz I. Kanterewicz¹, German Barrionuevo¹^,², Charleen T. Chu³, Tim D. Oury³, and Eric Klann¹^,²
¹ Department of Neuroscience and ² Center for the Neural Basis of Cognition, University of Pittsburgh, Pittsburgh, Pennsylvania 15260, and ³ Department of Pathology, University of Pittsburgh Medical Center, Pittsburgh, Pennsylvania 15261

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Reactive oxygen species, including superoxide, generally are considered neurotoxic molecules whose effects can be alleviatedby antioxidants. Different from this view, we show that scavengingof superoxide with an antioxidant enzyme is associated with deficitsin hippocampal long-term potentiation (LTP), a putative neuralsubstrate of memory, and hippocampal-mediated memory function.Using transgenic mice that overexpress extracellular superoxidedismutase (EC-SOD), a superoxide scavenger, we found that LTPwas impaired in hippocampal area CA1 despite normal LTP in areaCA3. The LTP impairment in area CA1 could be reversed by inhibitionof EC-SOD. In addition, we found that EC-SOD transgenic mice exhibitedimpaired long-term memory of fear conditioning to contextual cuesdespite exhibiting normal short-term memory of the conditioningexperience. These findings strongly suggest that superoxide, ratherthan being considered exclusively a neurotoxic molecule, shouldalso be considered a signaling molecule necessary for normal neuronalfunction.

Key words: EC-SOD; superoxide; LTP; associative memory; contextual fear conditioning; hydrogen peroxide

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Long-term potentiation (LTP) in the hippocampus is an activity-dependent increase in synaptic strength that has been hypothesizedto underlie mammalian learning and memory (Bliss and Collingridge,1993). The most intensely studied form of LTP is induced by high-frequencystimulation (HFS) of the Schaffer collateral-commissural inputto the pyramidal neurons of area CA1. The induction of LTP inarea CA1 is dependent on the activation of NMDA receptors (Collingridgeet al., 1983) followed by an influx of Ca²⁺ into the postsynaptic cell (Lynch et al., 1983; Malenka et al.,1988). The influx of Ca²⁺ results in the activation of a number of Ca²⁺-dependent enzymes, some of which produce small signaling molecules,including cAMP, nitric oxide-cGMP, and arachidonic acid (for review,see Roberson et al., 1996).

An additional class of signaling molecules likely to be produced in response to LTP-inducing HFS are reactive oxygen species(ROS), particularly superoxide. Consistent with this possibility,it was shown that superoxide is produced in response to NMDA receptoractivation in hippocampal area CA1 (Bindokas et al., 1996). Inaddition, several studies showed that removal of superoxide altershippocampal LTP in area CA1. For example, cell-permeable superoxidescavengers of superoxide were shown to block LTP (Klann, 1998),and cell-impermeable superoxide scavengers were shown to stronglyattenuate LTP (Klann et al., 1998). Finally, hippocampal slicesfrom transgenic mice that overexpress cytoplasmic superoxide dismutase(SOD-1) were found to exhibit deficient LTP (Gahtan et al., 1998).These data suggest that ROS, such as superoxide, are criticalcomponents of the signal transduction machinery necessary forLTP in hippocampal areaCA1.

On the basis of a large body of evidence that links hippocampal LTP and certain types of memory function (Martin et al., 2000),the finding that cell-impermeable scavengers strongly attenuateLTP suggests the possibility that extracellular superoxide maybe important not only for LTP but also for hippocampal-dependentmemory function. To test this hypothesis, we performed studieswith transgenic mice that overexpress extracellular superoxidedismutase (EC-SOD). Herein we report that EC-SOD transgenic miceexhibit a reversible impairment of LTP in hippocampal area CA1.Furthermore, we report that EC-SOD transgenic mice exhibit impairedlong-term but not short-term memory in contextual fear conditioning,a hippocampal-dependent memory task. Taken together, our findingssuggest that extracellular superoxide is critical for both hippocampalLTP and hippocampal-dependent memoryfunction.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

EC-SOD transgenic mice. EC-SOD transgenic mice were generated as previously described (Oury et al., 1992). Briefly, purifiedEC-SOD DNA was injected into the pronuclei of fertilized eggsisolated from mice [(C57BL/6 × C3H)F1 × (C57BL/6 × C3H)F1]. Mouseeggs surviving microinjection then were implanted into the oviductsof pseudopregnant foster mothers (CD1) following standard procedures.Mice carrying the human EC-SOD transgene were identified by Southernblot analysis of tail DNA probed with the entire human EC-SODcDNA. Transgenic founders were bred with (C57BL/6 × C3H)F1 (14-16back-crosses) to produce offspring for further studies. Heterozygotemice expressing human EC-SOD were compared with wild-type micefrom the same litter for eachexperiment.

Nissl staining. Brains from wild-type and EC-SOD transgenic mice were sectioned as described previously (Oury et al., 1999).Sections were collected sequentially in four bins of cryoprotectantand stored at $-$ 20°C until processing. One bin of tissue from eachbrain was processed for staining with cresyl violet. Sectionswere analyzed with a Zeiss (Thornwood, NY) Axioplan photomicroscopeequipped with differential interference optics. Images of immunoreactivecells were digitized with a DAGE (Michigan City, IN) video camera(MTI 3CCD) and an image analysis system (Simple 32; C-ImagingSystems).

Reverse transcription-PCR. Hippocampi were dissected from the brains of EC-SOD transgenic mice and nontransgenic littermates,and RNA was isolated using acid phenol-chloroform extractionsas previously described (Chomczynski and Sacchi, 1987). Messagefor human EC-SOD or mouse EC-SOD was detected by reverse transcription(RT)-PCR using a Geneamp rtTh PCR kit (Perkin-Elmer, Norwalk,CT) and primers specific for either mouse EC-SOD (forward, 5'-CCCATGCTCTCCGCCTCTAGAA-3';reverse, 5'-AAAGTCATTGCCTTGGCGCATG-3') or human EC-SOD (forward,5'-AGACACCTTCCACTCTGAGG-3'; reverse, 5'-GTTTCGGTACAAATGGAGGC-3').PCR products were detected after agarose gel electrophoresis byethidium bromidestaining.

Immunocytochemical staining. Wild-type and EC-SOD transgenic mice were killed by lethal injection with Nembutol. The brainwas perfused and fixed by injecting 20 ml of 4% buffered formalinthrough the left ventricle of the heart. Hippocampal sectionsthen were processed for standard paraffin embedding. Five-micrometer-thicksections were cut onto poly-L-lysine-coated slides for immunochemicallabeling using a rabbit polyclonal antibody specific to humanEC-SOD with minor variations to a previously described protocol(Oury et al., 1996). Briefly, the primary antibody was dilutedinto a wild-type mouse brain homogenate at 1:300 and allowed toincubate overnight at 4°C. The solution was centrifuged to removeparticulates and applied to tissue sections that had been treatedwith 0.1% pepsin in 0.01N HCl for 10 min for antigen retrieval.After washing, the primary antibody was detected using biotinylatedgoat anti-rabbit IgG and the Vectastain ABC reagent (Vector Laboratories,Burlingame, CA) followed by development with diaminobenzidine.As a control, serial sections were labeled with nonimmune rabbitIgG. To further control for potential nonspecific staining, sectionsfrom wild-type mice lacking human EC-SOD were labeled with thisantibody against human EC-SOD to ensure that the labeling presentin the EC-SOD transgenic mice was specific for human EC-SOD.

Western blots. Equivalent amounts of hippocampal protein from wild-type and EC-SOD transgenic mice were resolved with 10%SDS-PAGE, blotted electrophoretically to Immobilon membranes (Millipore,Bedford, MA), and incubated in Tris-buffered saline with Tween20 (50 mM Tris-HCl, pH 7.5-8.0, 150 mM NaCl, and 0.1% Tween 20)containing 3% bovine serum albumin. Blots were incubated witheither an antibody specific for human EC-SOD or an antibody specifcfor mouse EC-SOD, followed by horseradish peroxidase-linked secondaryantibody, and developed using enhanced chemiluminescence (AmershamPharmacia Biotech, Arlington Heights, IL). Densitometric analysisof immunoreactivity was conducted using NIH Imagesoftware.

SOD activity. EC-SOD activity and total SOD activity (cytoplasmic SOD and mitochondrial SOD) remaining after extraction ofEC-SOD were measured by inhibition of cytochrome c reduction atpH 10 as described previously (Crapo et al., 1978).

Preparation of hippocampal slices. Hippocampi from male heterozygote EC-SOD transgenic mice and male wild-type mice 3-6 monthsold (~25-35 gm) were removed, and 400 µm slices were preparedwith a McIlwain tissue chopper. The slices were perfused for 1-2hr with a standard saline solution (in mM: 124 NaCl, 4.4 KCl,26 NaHCO₃, 10 D-glucose, 2 CaCl₂, and 2 MgCl₂, gassed with 95%O₂ and 5% CO₂, pH 7.4) in an interface tissue slice chamber at30-32°C.

Induction of paired-pulse facilitation and post-tetanic potentiation. For assessment of either paired-pulse facilitation (PPF)or post-tetanic potentiation (PTP), a pair of bipolar stimulatingelectrodes were placed into the st. radiatum of area CA1 to stimulatethe Schaffer collateral-commissural fibers, and a recording electrodewas placed into the st. radiatum of area CA1. PPF is a presynapticfacilitation revealed when two stimuli are presented in rapidsuccession; the response to the second stimulus is enhanced dependingon the interstimulus interval. The initial slope of the extracellularfield EPSP (fEPSP) for each stimulus was measured over a rangeof interstimulus intervals (25-400 msec). Facilitation was measuredby examining the ratio of the fEPSP slope to stimulus 2/fEPSPslope to stimulus 1. PTP was analyzed by measuring the fEPSP slopeevery second for the first 15 sec after HFS. To avoid the potentiallyconfounding effects of LTP on measurements of PTP, the NMDA receptorantagonist 2-amino-5-phosphonovaleric acid (APV; 100 µM) was includedin the perfusingsolution.

Induction of LTP. For induction of LTP in area CA1, a pair of bipolar stimulating electrodes was placed into the st. radiatumof area CA1 to stimulate the Schaffer collateral-commissural fibers,and a recording electrode was placed into the st. radiatum ofarea CA1. Responses to electrical stimulation in area CA1 weremonitored for at least 20 min before the delivery of LTP-inducingHFS. In most experiments, test stimuli (50 µsec duration) weregiven at a current (30-100 µA) that produced 50% of the maximuminitial slope fEPSP. Responses to test stimuli were measured every2.5 min as an average of four individual traces (0.1 Hz). Onetrain of LTP-inducing HFS consisted of 100 pulses delivered at100 Hz using a current (60-100 µA) that elicited the maximum fEPSP.Multiple trains of HFS were delivered with an intertrain intervalof 20 sec. Responses to test stimuli were measured every 2.5 minas an average of four individual traces (0.1 Hz) for 60 min afterthe final train of HFS. Post-HFS responses were elicited usingthe same test stimulation intensity as that used before HFS. LTPwas defined as a $>=$ 20% increase in the initial slope of the fEPSPcompared with pre-HFS control levels (within-slicecomparison).

For induction of mossy fiber LTP in area CA3, mouse hippocampal slices were prepared as described previously for rat hippocampalslices (Urban and Barrionuevo, 1996). Slices were transferredto an incubation chamber containing a standard saline solutioncontaining (in mM): 125 NaCl, 2 KCl, 26 NaHCO₃, 10 dextrose, 1CaCl₂, and 6 MgCl₂, gassed with 95% O₂ and 5% CO₂, pH 7.4, atroom temperature. After incubation, slices were transferred toa recording chamber and submerged in the same standard salinesolution described above, with the exception that the divalention concentrations were (in mM): 2.5 CaCl₂ and 1 MgCl₂, and thesolution contained 100 µM APV to block NMDA receptors. The temperatureof the recording chamber was 30-32°C. A bipolar stimulating electrodewas placed into the granule cell layer of the dentate gyrus tostimulate the mossy fibers; a recording electrode was placed intothe st. radiatum of area CA3. Mossy fiber LTP was induced withthree trains of HFS. Each train consisted of 100 pulses deliveredat 100 Hz with an intertrain interval of 10 sec (Urban and Barrionuevo,1996). Responses to test stimuli were measured every 2.5 min asan average of four individual traces (0.1 Hz) for 60 min afterthe final train of HFS. Post-HFS responses were elicited usingthe same test stimulation intensity as that used before HFS. LTPwas defined as a $>=$ 20% increase in the initial amplitude of thefEPSP compared with pre-HFS control levels (within-slicecomparison).

For all of the LTP experiments, n was the number of mice used in each experimentalcondition.

Whole-cell recordings. Slices were placed in a submersion recording chamber and perfused with the following external solution(in mM): 125 NaCl, 2.5 KCl, 1.25 NaH₂PO₄, 25 NaHCO₃, 2 CaCl₂,1 MgCl₂, 10 glucose, and 0.01 bicuculline, gassed with 95% O₂and 5% CO₂, pH 7.4, at 30-32°C. Whole-cell recordings were obtainedfrom CA1 pyramidal neurons identified visually by differentialinterference contrast and infrared video microscopy (Stuart etal., 1993). Gigaohm seals (>2 G $Omega$ ) were obtained with patch pipettes(3-7 M $Omega$ ) pulled from borosilicate glass and filled with the followinginternal solution (in mM): 122.5 Cs gluconate, 11.5 CsCl, 8 NaCl,10 HEPES, 0.5 EGTA, 4 ATP, 0.3 GTP, and 14 phosphocreatine, pH7.2-7.4, 290-300 mOsm. Recordings were made with an Axopatch 1Damplifier (Axon Instruments, Foster City, CA) operating in voltage-clampmode. Series resistance (12-20 M $Omega$ ) was not compensated, and recordingswere discarded for analysis if the series resistance changed >20%.EPSCs were evoked at 0.1 Hz by stimulation of the Schaffer collateral-commissuralpathway using bipolar stimulation electrodes placed in the st.radiatum 100-200 µm from the st. pyramidale. Stimulation parameterswere adjusted to elicit EPSCs with a peak amplitude of 50-150pA when recorded at $-$ 70 mV. The AMPA and NMDA components of theEPSC were measured as the mean current in 10 msec time windowsplaced at the current peak (AMPA) or 50-80 msec after the peak(NMDA). Current-voltage plots were made for each neuron aftercurrents were normalized relative to the AMPA component (measuredat $-$ 60 or +60 mV,respectively).

Contextual fear conditioning: unsignaled shocks. To test the animals' ability to associate neutral contextual stimuli withan aversive stimulus (foot shock) in the absence of competingdiscrete stimuli paired with shock, the animals were placed intoa standard mouse conditioning chamber (13 × 10.5 × 13 cm) equippedwith a house light (28 V), a loudspeaker, and a floor consistingof 19 equally spaced metal rods (2.8 mm diameter). The fear-conditioningchambers were housed in sound-attenuating cubicles (56 × 50 ×41 cm) equipped with a background noise-generating fan to overshadowextraneous sounds. The onset of the cubicle fan and the illuminationof the house light signaled the onset of the training session.A 2 sec scrambled foot shock (0.75 mA) was presented 120 and 240sec after session onset. The session ended 30 sec after the secondshock, as indicated by the extinguishment of the house light andthe cubicle fan. The animals were removed immediately and returnedto their home cages. To test fear conditioning to the contextualcues, the animals were returned to the training context 24 hrafter training for a 5 min test session. As previously, sessiononset and offset were indicated by the turning on and off, respectively,of the house light and the cubicle fan. No shocks were presentedduring the test session. The occurrence of freezing (no movementother than respiratory movement), an indicator of fear, was measuredevery 10 sec during training, except the two 10 sec bins duringwhich the shocks occurred, and every 10 sec throughout testing.A summary of this and the next protocol is provided in Table 1.

Contextual fear conditioning: signaled shocks. The training session was identical to the one described above, except thata 30 sec tone (80 dB, 2 kHz) preceded and terminated with theonset of each of the two shocks. Conditioning to the trainingcontext was tested either 3 min or 24 hr after training with eithera 2 min (immediate test) or a 5 min (delayed test) test sessionas described above. To test fear conditioning to the cue, theanimals were returned to their home cages for either 24 hr (immediatecontext test) or 2 hr (delayed context test) after testing conditioningto the context. The test chamber was modified with respect totactile, spatial, visual, and olfactory properties to create anovel test environment. The animals were placed into the modifiedchamber for a 6 min test session, with the tone present continuouslyduring the second 3 min of that session. The occurrence of freezingwas measured during training and test sessions, as describedabove.

Open-field behavior. To test the animals' locomotor function and exploratory behavior in a novel context, the animals wereplaced for 10 min in an open-field chamber (28 × 28 × 40 cm) whosefloor was divided into 16 equal-sized square fields, and the frequencyof the following behaviors was recorded: (1) entries into eachof the 16 fields, (2) rearing, (3) nose poking into small holes(1 cm diameter) equally spaced 2 cm above the floor along twoopposite walls of the chamber, and (4) freezing bouts, an indicatoroffear.

Pain threshold. To test the animals' sensitivity to pain, we placed the animals individually on a surface (25.5 × 25.5 cm)surrounded by Plexiglas walls and heated to 52 ± 0.1°C and recordedthe latency to (1) forepaw lick, (2) hindpaw lick, (3) hindpawshake, and (4) jumping. The animals were removed from the surfaceimmediately after the jump or after 5 min had elapsed, whichevercamefirst.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Anatomical and biochemical characterization of EC-SOD transgenic mice

The mutant mice used in these studies overexpress human EC-SOD. These transgenic animals appeared to be healthy and exhibitedno obvious neurological abnormalities. Adult brains of the micewere fixed and examined for histological abnormalities. The appearanceand size of the brains from EC-SOD transgenic mice were indistinguishablefrom those of wild-type mice from the same litter. We examinedthe gross anatomy of various brain regions with Nissl stainingand observed no obvious abnormalities in EC-SOD transgenic micecompared with wild-type mice, including the hippocampal formation(Fig. 1A). Thus, at a gross neuroanatomical level, EC-SOD transgenicmice appeared to be identical to their wild-type littermates.

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Figure 1. Anatomical and biochemical comparison of wild-type and EC-SOD transgenic mice. A, Nissl stains of sagittal sections through the hippocampus of wild-type (left) and EC-SOD transgenic (right) mice. B, RT-PCR of mouse hippocampal RNA. MW, Molecular weight marker; lane 1, RT-PCR kit positive control; lane 2, wild-type mouse hippocampal RNA; lane 3, wild-type mouse hippocampal RNA with RNase; lane 4, EC-SOD trangenic mouse hippocampal RNA; lane 5, EC-SOD transgenic mouse hippocampal RNA with Rnase. C, Western blot of hippocampal homogenates from wild-type (WT) and EC-SOD transgenic (TG) mice. The blots were probed with antibodies specific for either human EC-SOD (top) or mouse EC-SOD (bottom). D, Immunocytochemistry of either wild-type (left) or EC-SOD transgenic (right) mice showing diffuse expression of human EC-SOD in the hippocampi of EC-SOD transgenic mice. Scale bars, 200 µm. E, EC-SOD activity measured in hippocampal homogenates from wild-type and EC-SOD transgenic mice. Error bars indicate SEM for four determinations. *Statistical significance with a paired Student's t test (p < 0.05).

We proceeded to analyze EC-SOD transgenic mice at the biochemical level. RT-PCR analysis revealed that human EC-SOD mRNA washighly expressed in the hippocampus, with no effect on endogenouslevels of mouse EC-SOD mRNA (Fig. 1B). Similarly, Western blotanalysis revealed that EC-SOD transgenic mice overexpressed humanEC-SOD protein in the hippocampus without alteration of endogenouslevels of EC-SOD protein (Fig. 1C). Using immunohistochemicaltechniques, we observed that human EC-SOD was expressed diffuselythroughout the hippocampi of transgenic mice (Fig. 1D). In enzymaticassays we found that EC-SOD transgenic mice had ~10-fold morehippocampal EC-SOD activity than wild-type mice did (Fig. 1E).Taken together, these results demonstrate that the EC-SOD transgenicmice overexpress an enzymatically competent EC-SOD in thehippocampus.

Impaired LTP in hippocampal area CA1 in EC-SOD transgenic mice

We previously showed that cell-impermeable superoxide scavengers strongly attenuate LTP in area CA1 of rat hippocampal slices(Klann et al., 1998). Because of the overexpression of EC-SODin the hippocampus, we hypothesized that LTP would be impairedin EC-SOD transgenic mice. In the first set of experiments, weinduced LTP in area CA1 of hippocampal slices from wild-type andEC-SOD transgenic mice with one train of HFS (100 pulses at 100Hz). This induction paradigm produced LTP in slices from wild-typemice (fEPSP slope = 145 ± 7% of control; n = 9; Fig. 2A,B). Incontrast, the same induction protocol failed to produce LTP inslices from EC-SOD transgenic mice (fEPSP slope = 100 ± 3% ofcontrol; n = 9; Fig. 2A,B). We also performed experiments in areaCA1 using three trains of HFS. With this induction paradigm weobserved robust potentiation in slices from wild-type mice (fEPSPslope = 165 ± 5% of control; n = 10; Fig. 2C) and strongly attenuatedpotentiation in slices from EC-SOD transgenic mice (118 ± 5% ofcontrol; n = 10; Fig. 2C). Taken together, these results are consistentwith the idea that extracellular superoxide is necessary for thefull expression of LTP in hippocampal area CA1.

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Figure 2. Impaired LTP in hippocampal area CA1 of EC-SOD transgenic mice. A, Stable baseline responses were recorded in hippocampal area CA1 of slices from either wild-type (WT) or EC-SOD transgenic (EC-SOD TG) mice for 20 min. LTP-inducing HFS consisted of one train of HFS (100 pulses at 100 Hz). Error bars indicate SEM for 10 determinations. B, Representative fEPSPs recorded in area CA1 before and 60 min after delivery of HFS to slices from either WT or EC-SOD TG mice. Calibration: 2 mV, 3 msec. C, Similar to A, except LTP-inducing HFS consisted of three trains of HFS (100 Hz) delivered 20 sec apart. Error bars indicate SEM for 10 determinations. D, Stable baseline responses were recorded in area CA3 of slices from either WT or EC-SOD TG mice for 10 min. LTP-inducing HFS consisted of three trains of HFS delivered 10 sec apart. Error bars indicate SEM for five determinations.

To determine whether extracellular superoxide also was necessary for LTP hippocampal area CA3, we induced LTP at the mossyfiber $right-arrow$ CA3 pyramidal cell synapse in slices from wild-type andEC-SOD transgenic mice with three trains of HFS. In contrast tothe forms of LTP examined in Figure 2, A and C, mossy fiber LTPis NMDA receptor-independent (Harris et al., 1984). As illustratedin Figure 2D, we observed no difference in mossy fiber LTP betweenslices from wild-type mice (fEPSP amplitude = 153 ± 15% of control;n = 5) and EC-SOD transgenic mice (fEPSP amplitude = 165 ± 19%of control; n = 5). These data suggest that extracellular superoxideis not necessary for mossy fiber LTP in area CA3, and that superoxideproduction in the hippocampus is likely to be coupled to NMDAreceptor activation (Bindokas et al., 1996).

EC-SOD transgenic mice exhibit normal synaptic transmission, post-tetanic potentiation, and paired pulse facilitation

We performed several experiments to determine whether the impairment of LTP in hippocampal area CA1 of EC-SOD transgenic micewas attributable to alterations in either synaptic transmissionor NMDA receptor function. First, we tested the synaptic input-outputrelation in area CA1 by using a range of stimulus intensities(10-70 µA) to elicit synaptic responses and comparing either thefiber volley amplitude versus the stimulus intensity (Fig. 3A)or the fEPSP slope versus the fiber volley amplitude (Fig. 3B).We observed no significant differences between wild-type and EC-SODtransgenic mice with either comparison (Fig. 3A,B). Using whole-cellrecordings we similarly detected no differences between wild-typeand EC-SOD transgenic mice in the amplitude and time course ofsynaptic currents at various voltages (data not shown). Furthermore,the current-voltage relationships for the non-NMDA component (Fig.3C) as well as the NMDA component (Fig. 3D) of the synaptic currentswere indistinguishable between wild-type and EC-SOD transgenicmice (Fig. 3C,D). Finally, there were no significant differencesin high-frequency synaptic transmission between slices from wild-typeand EC-SOD transgenic mice, measured as either total depolarizationduring HFS [integrating the entire response to HFS: wild-type,106 ± 8% of control; n = 4; EC-SOD transgenic (TG), 103 ± 5% ofcontrol; n = 4] or the steady-state depolarization produced duringHFS (averaged over the last 50 msec of the HFS: wild-type, 99± 7% of control; n = 4; EC-SOD TG, 104 ± 6% of control; n = 4).Overall, these results indicate that the LTP deficit in EC-SODtransgenic mice cannot be attributed to alterations in eithersynaptic transmission or NMDA receptor function.

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Figure 3. Baseline synaptic transmission and synaptic currents are normal in EC-SOD transgenic mice. A, Plot of fiber volley amplitude across stimulation intensities. There was no significant difference between wild-type (WT) and EC-SOD transgenic (EC-SOD TG) mice. Error bars indicate SEM for seven determinations. B, Plot of fEPSP slope across fiber volley amplitudes. There was no significant difference between WT and EC-SOD TG mice. Error bars indicate SEM for seven determinations. C, Averaged amplitudes of AMPA receptor-mediated responses. D, Averaged amplitudes of NMDA receptor-mediated responses. Error bars in C and D indicate SEM for five determinations. The AMPA-mediated component was measured 5 msec after onset of the EPSC; the NMDA component was determined from the averaged response 50-100 msec after the stimulus.

We examined two short-lasting forms of presynaptic plasticity to determine whether the blockade of LTP in EC-SOD transgenicmice was attributable to abnormal presynaptic function. We firstexamined PTP in hippocampal slices from wild-type and EC-SOD transgenicmice. For that purpose, we analyzed the enhancement of synapticresponses during the first 15 sec after HFS (Zucker, 1989; Chapmanet al., 1995). To avoid potential confounding effects of LTP onPTP measurements, we performed the experiments in the presenceof APV (50 µM), an NMDA receptor antagonist. As shown in Figure4A, PTP in area CA1 was indistinguishable between hippocampalslices from wild-type and EC-SOD transgenic mice. Next, we examinedPPF in hippocampal slices from wild-type and EC-SOD transgenicmice. PPF is a presynaptic facilitation revealed by the enhancedmagnitude of the response evoked by the second pulse of a pairof pulses delivered at short intervals (McNaughton, 1982; Hesset al., 1987; Muller and Lynch, 1989). We observed no significantdifference in PPF between slices taken from wild-type and EC-SODtransgenic mice (Fig. 4B). Taken together, these data suggestthat the blockade of LTP in EC-SOD transgenic mice cannot be attributedto abnormal presynaptic function.

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Figure 4. Post-tetanic potentiation and paired-pulse facilitation are normal in EC-SOD transgenic mice. A, Post-tetanic potentiation in wild-type (WT) and EC-SOD transgenic (EC-SOD TG) mice. The graph includes 2 responses measured before HFS, 15 responses measured every second immediately after HFS, and 2 additional responses measured 5 min after HFS. Error bars indicate SEM for seven determinations. B, Paired pulse stimulation in WT and EC-SOD TG mice. The graph represents responses to paired pulses in which the fEPSP slope of the response to the second stimulus is expressed as a percentage of the fEPSP slope of the response to the first stimulus versus the interpulse interval of paired pulses. Error bars indicate SEM for five determinations.

Blockade of LTP in EC-SOD transgenic mice is reversible

EC-SOD is a Cu- and Zn-dependent enzyme (Marklund et al., 1982). Therefore, we determined whether the copper chelator diethyldithiocarbamate(DDCA) could reverse the blockade of LTP observed in hippocampalarea CA1 of EC-SOD transgenic mice. For that purpose, we deliveredone train of LTP-inducing HFS to slices from either wild-typeor EC-SOD transgenic mice in either the presence or absence of5 mM DDCA. We observed that DDCA reversed the blockade of LTPin slices from EC-SOD transgenic mice ( $-$ DDCA, fEPSP slope = 99± 7% of control; n = 6; +DDCA, fEPSP slope = 145 ± 7% of control;n = 6; Fig. 5A) but had no statistically significant effect onLTP in slices from wild-type mice ( $-$ DDCA, fEPSP slope = 156 ±6% of control; n = 6; +DDCA, fEPSP slope = 165 ± 8% of control;n = 6; Fig. 5A). These results show that the blockade of LTP inEC-SOD transgenic mice can be reversed by inhibition of EC-SOD.In addition, these results suggest that the underlying signalingcascades responsible for the induction and expression of LTP remainintact in the hippocampi of EC-SOD transgenic mice.

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Figure 5. Impaired LTP in EC-SOD transgenic mice is rescued by DDCA but not by catalase or bicuculline. A, Rescue of impaired LTP by DDCA. Responses recorded from slices from either wild-type (WT) or EC-SOD transgenic (EC-SOD TG) mice given LTP-inducing HFS in the presence of 5 mM DDCA were compared with responses recorded from control slices from the same animal (in an adjacent recording chamber) given LTP-inducing HFS in the absence of the compound. Error bars indicate SEM for six determinations. B, Impaired LTP is not reversed by catalase. Responses recorded from slices given LTP-inducing HFS in the presence of catalase (260 U/ml) were compared with responses recorded from control slices from the same animal (in an adjacent recording chamber) given LTP-inducing HFS in the absence of the compound. Error bars indicate SEM for six determinations. C, Slices from either WT or EC-SOD TG mice were given LTP-inducing HFS in the presence of 10 µM bicuculline. Error bars indicate SEM for four determinations.

EC-SOD converts superoxide to hydrogen peroxide and oxygen (Halliwell, 1992). Because hydrogen peroxide has been shown toinhibit LTP (Pellmar et al., 1991; Auerbach and Segal, 1997),it is possible that the blockade of LTP in EC-SOD transgenic micewas caused by altered hydrogen peroxide metabolism. To examinethe potential involvement of altered hydrogen peroxide metabolismin the impairment of LTP in EC-SOD transgenic mice, slices fromwild-type and EC-SOD transgenic mice were given LTP-inducing stimulationin either the presence or absence of catalase (260 U/ml), an enzymethat scavenges hydrogen peroxide (Halliwell, 1992). Catalase hadno effect on the blockade of LTP in slices from EC-SOD transgenicmice ( $-$ catalase, fEPSP slope = 99 ± 7% of control; n = 6; +catalase,fEPSP slope = 96 ± 5% of control; n = 6; Fig. 5B). Interestingly,in experiments with slices from wild-type mice, we observed thatcatalase caused a small but statistically significant decreasein the magnitude of LTP ( $-$ catalase, fEPSP slope = 166 ± 10% ofcontrol; n = 6; +catalase, fEPSP slope = 144 ± 7% of control;n = 6; Fig. 5B). These results indicate that blockade of LTP inEC-SOD transgenic mice is not caused by overproduction of hydrogenperoxide. Furthermore, these results indicate that productionof hydrogen peroxide may be necessary for the full expressionof LTP in area CA1 of wild-typemice.

Mice that overexpress cytoplasmic SOD (SOD-1) exhibit impaired LTP that has been attributed to upregulation of GABAergic neurotransmission(Levkovitz et al., 1999). To determine whether a similar mechanismwas involved in the blockade of LTP in EC-SOD transgenic mice,we delivered one train of LTP-inducing HFS to slices from wild-typeand EC-SOD transgenic mice in the presence of bicuculline (10µM), a selective GABA_A receptor antagonist. Bicuculline had noeffect on the blockade of LTP in slices from EC-SOD transgenicmice (fEPSP slope = 105 ± 3% of control; n = 4; Fig. 5C) or onLTP in slices from wild-type mice (fEPSP slope = 162 ± 8% of control;n = 4; Fig. 5C). These results indicate that the lack of LTP inEC-SOD transgenic mice cannot be attributed to upregulation ofGABAergicneurotransmission.

EC-SOD transgenic mice exhibit deficient hippocampal-dependent associative memory

Under the assumption that hippocampal LTP underlies hippocampal-dependent memory, our observations of compromised LTP in areaCA1 of hippocampal slices from EC-SOD transgenic mice lead tothe prediction that hippocampal-dependent memory function alsois compromised in these mice. To test this prediction, we usedtwo versions of the contextual fear-conditioning paradigm (Kimand Fanselow, 1992; Phillips and LeDoux, 1992). In the first paradigm,which involved conditioning with unsignaled shocks (Table 1),wild-type and EC-SOD transgenic mice received two 2 sec foot shocksduring a 5 min training session (2 min intershock interval) andwere tested 24 hr later for conditioning to the training context.Figure 6A shows that whereas both groups of animals exhibitedcomparably low levels of freezing during training, EC-SOD transgenicmice exhibited significantly less freezing (19 ± 6% freezing;n = 11) than did wild-type mice (42 ± 7% freezing; n = 11) duringtesting. In the second paradigm, which involved conditioning withsignaled shocks, wild-type and EC-SOD transgenic mice similarlyreceived two 2 sec foot shocks; however, the shocks were precededby a 30 sec tone. Animals trained in this paradigm were testedfor conditioning to the training context either 3 min after training,to assess short-term memory of the conditioning experience, or,similar to the first paradigm, 24 hr after training, to assesslong-term memory of the conditioning experience. Figure 6B showsthat wild-type and EC-SOD transgenic mice exhibited comparablylow levels of freezing during training irrespective of delay totesting. When tested for conditioning to the context 3 min aftertraining, both wild-type and EC-SOD transgenic mice exhibitedelevated levels of freezing, with the freezing level being comparablebetween the two groups (wild-type mice, 33 ± 10% freezing; n =6; EC-SOD transgenic mice, 29 ± 13% freezing; n = 8; Fig. 6B).In contrast, when tested for conditioning to the context 24 hrafter training, EC-SOD transgenic mice exhibited significantlylower levels of freezing to the context than did wild-type mice(wild-type mice, 58 ± 9% freezing; n = 8; EC-SOD transgenic mice,17 ± 6% freezing; n = 8), similar to the pattern observed withthe first paradigm. Collectively, these data indicate that theinitial acquisition and short-term memory of contextual fear conditioningis normal in EC-SOD transgenic mice, but that consolidation ofcontextual fear conditioning over a long retention interval issignificantly impaired in EC-SOD transgenic mice.


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Table 1. Contextual fear conditioning protocols for assessing associative memory in wild-type and EC-SOD transgenic mice

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Figure 6. Impaired associative memory in EC-SOD transgenic mice. A, Group data of the percentage of time engaged in freezing to the training context during training (train) and testing (test) for wild-type mice (WT; open bars) and EC-SOD transgenic mice (EC-SOD TG; filled bars). Animals were conditioned with unsignaled shocks and tested 24 hr after training. Error bars indicate SEM for 11 determinations per group. B, Group data of freezing behavior as shown above, except that animals were conditioned with signaled shocks and tested either 3 min or 24 hr after training. Error bars indicate SEM for eight determinations per group, except for the group of wild-type animals tested 3 min after training, for which the number of determinations was six. C, Group data of freezing behavior to the tone during training (train) and testing (test) for wild-type mice (open bars) and EC-SOD transgenic mice (filled bars). All animals were tested for conditioning to the tone 26 hr after training. Data on the left show results for animals that received a context test trial 3 min after training (with immediate context test); data on the right show results for animals that received a context test trial 24 hr after training (with delayed context test). The trend toward stronger conditioning to the tone by wild-type mice compared with EC-SOD transgenic mice failed to reach statistical significance regardless of whether animals received the immediate, 2 min context test or the delayed, 5 min context test. The trend, however, raises the possibility that conditioning to the tone may also have been affected by the overexpression of EC-SOD, albeit to a considerably lesser extent than conditioning to the context. Error bars indicate SEM for eight determinations per group, except for the group of wild-type animals with the immediate context test, for which the number of determinations was six. *Statistically significant difference (p < 0.01) between wild-type and EC-SOD transgenic mice determined with Tukey's HSD method for post hoc comparisons after a repeated measures ANOVA with one within factor (trial) and one between factor (group).

The lack of a short-term memory deficit by EC-SOD mice suggests that the long-term memory deficit cannot be attributed toa difference between the groups in exploratory behavior or sensorimotorfunction. Nevertheless, to rule out such an alternative explanationof the findings, we performed two additional behavior analyses.First, we observed exploratory behavior of wild-type and EC-SODtransgenic mice in an open-field chamber for 10 min, recordingthe frequency of entries into equal-sized square fields drawnonto the floor of the chamber, rearing, nose poking into holesin the chamber walls, and freezing. We found no systematic differencesbetween the two groups of mice with respect to any of the measures,including the percentage of entries into the center fields ofthe chamber (Table 2). Second, we tested the pain threshold ofwild-type and EC-SOD mice by placing the animals on a heated platform.We observed no differences in the latency to lick the forepaw,lick the hindpaw, shake the hindpaw, or jump off the hot platform(Table 2). Taken together, these observations render it unlikelythat the long-term memory deficit in EC-SOD transgenic mice canbe explained in terms of altered sensorimotor function.


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Table 2. Open-field behavior and pain threshold are indistinguishable between wild-type and EC-SOD transgenic mice

This conclusion was strengthened by our tests of conditioning to the tone in animals trained in the fear-conditioning paradigmwith signaled shocks (Table 1). To assess fear conditioning tothe tone, a hippocampal-independent conditioning paradigm (Kimand Fanselow, 1992; Phillips and LeDoux, 1992), we modified theconditioning chamber with respect to spatial, tactile, olfactory,and visual properties to render the test context novel. Animalswere tested in the novel context 26 hr after training, with thetone being presented during the second 3 min of the 6 min test.Analysis of freezing during the first 3 min of the test revealedthat none of the mice generalized from the training to the noveltest context. Figure 6C depicts fear conditioning to the tonefor mice that received a context test trial 3 min after training(with immediate context) and animals that received a context testtrial 24 hr after training (with delayed context). Irrespectiveof the context test protocol, wild-type and EC-SOD transgenicmice showed comparably low levels of freezing to the tone duringtraining and significantly enhanced levels of freezing to thetone during testing (with immediate context: wild-type mice, 70± 6% freezing; n = 6; EC-SOD transgenic mice, 56 ± 9% freezing;n = 8; with delayed context: wild-type mice, 74 ± 9% freezing;n = 8; EC-SOD transgenic mice, 43 ± 10% freezing; n = 8). Thesedata show that EC-SOD transgenic mice can consolidate associativerepresentations over a long retention interval provided that theassociations involve simple stimulus relations whose mnemonicprocessing is relatively independent of the integrity of thehippocampus.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

A growing body of evidence suggests that ROS, such as superoxide, are necessary to induce the full expression of LTP in hippocampalarea CA1. For example, cell-permeable superoxide scavengers havebeen shown to prevent the induction of LTP (Klann, 1998), andtransgenic mice that overexpress the superoxide-scavenging enzymeSOD-1, a cytoplasmic SOD, exhibit impaired LTP (Gahtan et al.,1998). In addition, cell-impermeable scavengers of superoxidehave been shown to strongly attenuate LTP (Klann et al., 1998).Similarly, we found that, depending on the LTP induction paradigm,LTP was either blocked or strongly attenuated in area CA1 of hippocampalslices from EC-SOD transgenic mice (Fig. 2A,B). These findingsare consistent with the idea that superoxide is a critical moleculein the biochemical milieu necessary for LTP in hippocampal areaCA1.

In contrast to LTP, synaptic transmission appeared to be normal in EC-SOD transgenic mice (Fig. 3). In addition, we observedno deficit in either PTP or PPF in EC-SOD transgenic mice (Fig.4). These data are important because they indicate that the overexpressionof EC-SOD in the transgenic mice interferes with neither presynapticnor postsynaptic function. The blockade of LTP in these mice,therefore, is unlikely to be attributable to nonspecific effectsof EC-SOD. Furthermore, we were able to reverse the LTP deficitby inhibiting EC-SOD (Fig. 5A), which suggests that there areno fundamental differences in the biochemical machinery in areaCA1 between wild-type and EC-SOD transgenicmice.

Interestingly, we found that mossy fiber LTP in EC-SOD transgenic mice was indistinguishable from mossy fiber LTP in wild-typemice (Fig. 2C), which suggests that superoxide does not play acritical role in this form of synaptic plasticity. The inductionof mossy fiber LTP is NMDA receptor-independent; instead, itsinduction is dependent on the activation of voltage-gated Ca²⁺ channels (Jaffe and Johnston, 1990; Castillo et al., 1994). Inrat hippocampal slices, glutamate receptor (AMPA, kainate, andNMDA) activation has been shown to result in the production ofsuperoxide, whereas membrane depolarization that activates voltage-gatedCa²⁺ channels did not (Bindokas et al., 1996). Thus, superoxide productionin the hippocampus is likely to be more closely coupled to NMDAreceptor activation than to the activation of voltage-gated Ca²⁺ channels. It will be of interest to determine whether other NMDAreceptor-dependent forms of LTP in the hippocampus, such as atthe perforant path $right-arrow$ dentate granule cell synapse, are also dependenton production ofsuperoxide.

The enzymatic action of EC-SOD is to convert superoxide to hydrogen peroxide and oxygen (Halliwell, 1992), and long incubationsof hippocampal slices with hydrogen peroxide have been shown toprevent the full expression of LTP (Pellmar et al., 1991; Auerbachand Segal, 1997). Furthermore, mice that overexpress SOD-1 haveimpaired LTP that can be reversed partially by the hydrogen peroxidescavenger catalase (Gahtan et al., 1998). In contrast to thesestudies, catalase did not reverse the impaired LTP observed inEC-SOD transgenic mice (Fig. 5B). Moreover, hydrogen peroxidemay be necessary for the full expression of LTP, because we foundthat catalase slightly attenuated LTP in slices from wild-typemice (Fig. 5B), a finding consistent with previous observations(Katsuki et al., 1998). One way to reconcile these apparentlycontradictory findings is to hypothesize that hydrogen peroxideis necessary for the full expression of LTP, and that prolongedexposure to exogenous hydrogen peroxide, in addition to endogenoushydrogen peroxide, is deleterious to the full expression of LTP.This hypothesis remains to betested.

Our findings are consistent with the hypothesis that superoxide is produced in response to LTP-inducing stimulation. If thishypothesis is correct, then several questions arise. One questionis the cellular action of superoxide. It is possible that superoxideacts as a signaling molecule. Superoxide can activate severalprotein kinases in the hippocampus, including protein kinase C(PKC; Knapp and Klann, 2000) and extracellular signal-regulatedkinase 2 (Kanterewicz et al., 1998), that are necessary for LTP(Malinow et al., 1989; English and Sweatt, 1997). In addition,superoxide scavengers have been shown to block LTP-associatedincreases in PKC activity (Klann et al., 1998). Alternatively,superoxide can inactivate the calcium/calmodulin-dependent phosphatasecalcineurin (Wang et al., 1996). Such an inactivation has beenshown to occur with electrical stimulation of cultured hippocampalneurons (Bito et al., 1996) and might serve to enhance the phosphorylationof critical proteins involved in LTP. It also is possible thatsuperoxide interacts with nitric oxide. The role of nitric oxidein LTP is controversial (Holscher, 1997); however, there is evidencethat nitric oxide is produced via NMDA receptor activation afterLTP-inducing stimulation (Chetkovich et al., 1993). Superoxideand nitric oxide are known to interact rapidly to form peroxynitrite,a very reactive oxidant that can also nitrate target proteins(Torreilles et al., 1999). It remains to be determined whetherperoxynitrite either oxidizes or nitrates proteins after LTP-inducingstimulation.

Another question raised by our findings concerns the source of superoxide production. Superoxide can be a product of the actionsof lipoxygenase on arachidonic acid (Kukreja et al., 1986), andlipoxygenase inhibitors have been shown to block LTP (Lynch etal., 1989). Although, as mentioned above, the role of nitric oxidesynthase in LTP is controversial (Holscher, 1997), this enzymehas been shown to produce superoxide (Pou et al., 1999). Finally,NMDA receptor activation in hippocampal slices has been shownto increase production of superoxide via the mitochondrial electrontransport chain (Bindokas et al., 1996). It will be interestingto determine whether LTP-inducing stimulation produces superoxidevia any of the aforementionedmechanisms.

Our studies suggest that superoxide is necessary not only for LTP but also for associative memory. We found that EC-SOD transgenicmice exhibited a pronounced deficit in contextual fear conditioningwith both unsignaled and signaled shocks when there was a delayof 24 hr between training and testing (Fig. 6A,B). This learningdeficit appears to be caused by impairment in long-term memory,i.e., information consolidation rather than information acquisition,because EC-SOD transgenic mice exhibited similar levels of contextualfear conditioning as did wild-type mice when the delay betweentraining and testing was short (Fig. 6B). The long-term memorydeficit appears to be relatively specific to hippocampal-mediatedlearning, because EC-SOD transgenic mice did not exhibit a significantdeficit in fear conditioning to the cue despite a 26 hr delaybetween training and testing. However, there was a trend for EC-SODtransgenic mice to freeze less to the tone than wild-type mice(Fig. 6C), which in light of the role of the amygdala in mediatingthis type of learning (Phillips and LeDoux, 1992; Maren et al.,1996) suggests the intriguing possibility that superoxide is involvedin synaptic plasticity in the amygdala (Rogan and LeDoux, 1995).

In addition to the role that superoxide plays in the type of associative memory documented herein, superoxide appears to benecessary for other types of learning. For example, EC-SOD transgenicmice were shown to exhibit deficits in the acquisition of theeight-arm radial maze task (Levin et al., 1998), a hippocampal-dependentspatial memory task. In addition, transgenic mice that overexpressSOD-1 were found to be deficient in their ability to acquire thespatial version of the Morris water maze task (Gahtan et al.,1998). This finding is particularly intriguing, because in Down'ssyndrome, the phenotypic manifestation of trisomy 21, the activityof SOD-1 is elevated. The learning deficit observed in SOD-1 transgenicmice has been attributed to a defect in ROS metabolism (Gahtanet al., 1998); however, given the role of superoxide as a signalingmolecule, it is possible that removal of superoxide by eitherSOD-1 or EC-SOD interferes with signaling cascades critical forlearning.

Our studies demonstrate that superoxide is necessary for hippocampal synaptic plasticity and consolidation of associativememories. Although traditionally superoxide has been considereda neurotoxic molecule, our data suggest that improper scavengingof superoxide could be involved in the pathogenesis of a widevariety of neurodegenerative diseases of learning and memory,including Alzheimer's disease (Maulthaup et al., 1997). Whereasprevious studies have suggested that scavenging of superoxideshould limit neuronal degeneration, a growing body of evidencesuggests that we consider superoxide and similar molecules aspart of the biochemical signaling necessary for normal neuronalfunction (Lander, 1997; Klann and Thiels, 1999).

  FOOTNOTES

Received June 8, 2000; revised July 27, 2000; accepted July 31, 2000.

This work was supported by National Institutes of Health Grants NS36180 (E.T.), NS24288 (G.B.), and NS34007 (E.K.). We thankLisa M. Schaefer and Kimberly D. Palangio for technical assistance,Dr. Lauren T. Knapp for helpful comments on this manuscript, Dr.J. Patrick Card for help with Nissl and immunocytochemical stainingof sections, and Dr. Jerry W. Rudy for invaluable advice concerningthe behavioralexperiments.
Correspondence should be addressed to Dr. Eric Klann, Department of Neuroscience, University of Pittsburgh, 446 Crawford Hall,Pittsburgh, PA 15260. E-mail: eklann+{at}pitt.edu.

Dr. Urban's present address: Max-Planck-Institut für Medizinische Forschung, Abteilung Zellphysiologie, 29 Jahnstrasse, D-69120Heidelberg,Germany.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Auerbach JM, Segal M (1997) Peroxide modulation of slow onset potentiation in rat hippocampus. J Neurosci 17:8695-8701[Abstract/Free Full Text].
Bindokas VP, Jordan J, Lee CC, Miller RJ (1996) Superoxide production in rat hippocampal neurons: selective imaging with hyrdoethidine. J Neurosci 16:1324-1336[Abstract/Free Full Text].
Bito H, Deisseroth K, Tsien RW (1996) CREB phosphorylation and dephosphorylation: a Ca²⁺- and stimulus duration-dependent switch for hippocampal gene expression. Cell 87:1203-1214[Web of Science][Medline].
Bliss TVP, Collingridge GL (1993) A synaptic model of memory: long-term potentiation in the hippocampus. Nature 361:31-39[Medline].
Castillo PE, Weisskopf MG, Nicoll RA (1994) The role of calcium channels in hippocampal mossy fiber synaptic transmission and long-term potentiation. Neuron 12:261-269[Web of Science][Medline].
Chapman PF, Frenguelli BG, Smith A, Chen C-M, Silva AJ (1995) The $alpha$ -Ca²⁺/calmodulin kinase II: a bidirectional modulator of presynaptic plasticity. Neuron 14:591-597[Web of Science][Medline].
Chetkovich DM, Klann E, Sweatt JD (1993) Nitric oxide synthase-independent long-term potentiation in area CA1 of hippocampus. NeuroReport 4:919-922[Web of Science][Medline].
Chomczynski P, Sacchi N (1987) Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. Anal Biochem 162:156-159[Web of Science][Medline].
Collingridge GL, Kehl SJ, McClennan H (1983) Excitatory amino acids in synaptic transmission in the Schaffer collateral-commissural pathway of the rat hippocampus. J Physiol (Lond) 334:33-46[Abstract/Free Full Text].
Crapo JD, McCord JM, Fridovich I (1978) Preparation and assay of superoxide dismutases. Methods Enzymol 53:382-393[Medline].
English JD, Sweatt JD (1997) A requirement for the mitogen-activated protein kinase cascade in hippocampal long-term potentiation. J Biol Chem 272:19103-19106[Abstract/Free Full Text].
Gahtan E, Auerbach JM, Groner Y, Segal M (1998) Reversible impairment of long-term potentiation in transgenic Cu/Zn-SOD mice. Eur J Neurosci 10:538-544[Web of Science][Medline].
Halliwell B (1992) Reactive oxygen species and the central nervous system. J Neurochem 59:1609-1623[Web of Science][Medline].
Harris EW, Ganong AH, Cotman CW (1984) Long-term potentiation in the hippocampus involves activation of N-methyl-D-aspartate receptors. Brain Res 323:132-137[Web of Science][Medline].
Hess G, Kuhnt U, Voronin LL (1987) Quantal analysis of paired-pulse facilitation in guinea pig hippocampal slices. Neurosci Lett 77:187-192[Web of Science][Medline].
Holscher C (1997) Nitric oxide, the enigmatic neuronal messenger: its role in synaptic plasticity. Trends Neurosci 20:298-303[Web of Science][Medline].
Jaffe D, Johnston D (1990) Induction of long-term potentiation at hippocampal mossy fiber synapses follows a Hebbian rule. J Neurophysiol 64:948-960[Abstract/Free Full Text].
Kanterewicz BI, Knapp LT, Klann E (1998) Stimulation of p42 and p44 mitogen-activated protein kinases by reactive oxygen species and nitric oxide in hippocampus. J Neurochem 70:1009-1016[Web of Science][Medline].
Katsuki H, Noguchi K, Matsuki N (1998) Modulation of synaptic plasticity by hydrogen peroxide in the hippocampus. Soc Neurosci Abstr 24:1070.
Kim JJ, Fanselow MS (1992) Modality-specific retrograde amnesia of fear. Science 256:675-677[Abstract/Free Full Text].
Klann E (1998) Cell-permeable scavengers of superoxide prevent long-term potentiation in hippocampal area CA1. J Neurophysiol 80:452-457[Abstract/Free Full Text].
Klann E, Thiels E (1999) Modulation of protein kinases and protein phosphatases by reactive oxygen species: implications for hippocampal synaptic plasticity. Prog Neuropsychopharmacol Biol Psychiatry 23:359-376[Medline].
Klann E, Roberson ED, Knapp LT, Sweatt JD (1998) A role for superoxide in protein kinase C activation and induction of long-term potentiation. J Biol Chem 273:4516-4522[Abstract/Free Full Text].
Knapp LT, Klann E (2000) Superoxide-induced stimulation of protein kinase C via thiol modification and modulation of zinc content. J Biol Chem 275:24136-24145[Abstract/Free Full Text].
Kukreja RC, Kontos HA, Hess ML, Ellis EF (1986) PGH synthase and lipoxygenase generate superoxide in the presence of NADH or NADPH. Circ Res 59:612-619[Abstract/Free Full Text].
Lander H (1997) An essential role for free radicals and derived species in signal transduction. FASEB J 11:118-124[Abstract].
Levin ED, Brady TC, Hochrein EC, Oury TD, Jonsson LM, Marklund SL, Crapo JD (1998) Molecular manipulations of extracellular superoxide dismutase: functional importance for learning. Behav Genet 28:381-390[Medline].
Levkovitz Y, Avigonne E, Groner Y, Segal M (1999) Upregulation of GABA neurotransmission suppresses hippocampal excitability and prevents long-term potentiation in transgenic superoxide dismutase-overexpressing mice. J Neurosci 19:10977-10984[Abstract/Free Full Text].
Lynch G, Larson K, Kelso S, Barrionuevo G, Schottler F (1983) Intracellular injections of EGTA block induction of hippocampal long-term potentiation. Nature 305:719-721[Medline].
Lynch MA, Errington ML, Bliss TVP (1989) Nordihydroguariaretic acid blocks the synaptic component of long-term potentiation and the associated increases in release of glutamate and arachidonate: an in vivo study in the dentate gyrus of the rat. Neuroscience 30:693-701[Web of Science][Medline].
Malenka RC, Kauer JA, Zucker RS, Nicoll RA (1988) Postsynaptic calcium is sufficient for potentiation of hippocampal synaptic transmission. Science 242:81-84[Abstract/Free Full Text].
Malinow R, Schulman H, Tsien RW (1989) Inhibition of postsynaptic PKC and CaMKII blocks induction but not expression of LTP. Science 245:862-866[Abstract/Free Full Text].
Maren S, Aharonov G, Stote DL, Fanselow MS (1996) N-Methyl-D-aspartate receptors in the basolateral amygdala are required for both acquisition and expression of conditional fear in rats. Behav Neurosci 110:1365-1374[Web of Science][Medline].
Marklund SL, Holme E, Hellner L (1982) Superoxide dismutase in extracellular fluids. Clin Chim Acta 126:41-51[Web of Science][Medline].
Martin SJ, Grimwood JD, Morris RGM (2000) Synaptic plasticity and memory: an evaluation of the hypothesis. Annu Rev Neurosci 23:649-711[Web of Science][Medline].
Maulthaup G, Ruppert T, Schlicksupp A, Hesse L, Beher D, Masters CL, Beyreuther K (1997) Reactive oxygen species and Alzheimer's disease. Biochem Pharmacol 54:533-539[Web of Science][Medline].
McNaughton BL (1982) Long-term synaptic enhancement and short-term potentiation in rat fascia dentata act through different mechanisms. J Physiol (Lond) 324:249-262[Abstract/Free Full Text].
Muller D, Lynch G (1989) Evidence that changes in presynaptic calcium currents are not responsible for long-term potentiation in hippocampus. Brain Res 479:290-299[Web of Science][Medline].
Oury TD, Ho Y-S, Piantadosi CA, Crapo JD (1992) Extracellular superoxide dismutase, nitric oxide, and central nervous system toxicity. Proc Natl Acad Sci USA 89:9715-9719[Abstract/Free Full Text].
Oury TD, Day BJ, Crapo JD (1996) Extracellular superoxide dismutase in vessels and airways of humans and baboons. Free Radic Biol Med 20:957-965[Web of Science][Medline].
Oury TD, Card JP, Klann E (1999) Localization of extracellular superoxide dismutase in adult mouse brain. Brain Res 850:96-103[Web of Science][Medline].
Pellmar TC, Hollinden GE, Sarvey JM (1991) Free radicals accelerate the decay of long-term potentiation in field CA1 of guinea-pig hippocampus. Neuroscience 44:353-359[Web of Science][Medline].
Phillips RG, LeDoux JE (1992) Differential contribution of amygdala and hippocampus to cued and contextual fear conditioning. Behav Neurosci 106:274-285[Web of Science][Medline].
Pou S, Keaton L, Surichamorn W, Rosen GM (1999) Mechanism of superoxide generation by neuronal nitric-oxide synthase. J Biol Chem 274:9573-9580[Abstract/Free Full Text].
Roberson ED, English JD, Sweatt JD (1996) A biochemist's view of long-term potentiation. Learn Mem 3:1-24[Abstract/Free Full Text].
Rogan MT, LeDoux JE (1995) LTP is accompanied by commensurate enhancement of auditory-evoked responses in a fear conditioning circuit. Neuron 15:127-136[Web of Science][Medline].
Stuart GJ, Dodt HU, Sakmann B (1993) Patch-clamp recordings from the soma and dendrites of neurons in brain slices using infrared video microscopy. Pflugers Arch 423:511-518[Web of Science][Medline].
Torreilles F, Salman-Tabcheh S, Guerin M, Torreilles J (1999) Neurodegenerative disorders: the role of peroxynitrite. Brain Res Rev 30:153-163[Medline].
Urban NN, Barrionuevo G (1996) Induction of Hebbian and non-Hebbian mossy fiber long-term potentiation by distinct patterns of high-frequency stimulation. J Neurosci 16:4293-4299[Abstract/Free Full Text].
Wang X, Culotta VC, Klee CB (1996) Superoxide dismutase protects calcineurin from inactivation. Nature 383:434-437[Medline].
Zucker RS (1989) Short-term plasticity. Annu Rev Neurosci 12:13-31[Web of Science][Medline].

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[Abstract] [Full Text] [PDF]

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