Potentiation of Hippocampal Synaptic Transmission by Superoxide Requires the Oxidative Activation of Protein Kinase C

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The Journal of Neuroscience, February 1, 2002, 22(3):674-683

Potentiation of Hippocampal Synaptic Transmission by Superoxide Requires the Oxidative Activation of Protein Kinase C
Lauren T. Knapp¹ and Eric Klann¹^,²^,³^,⁴
¹ Department of Neuroscience and the ² Center for the Neural Basis of Cognition, University of Pittsburgh, Pittsburgh, Pennsylvania 15260, and ³ Department of Molecular Physiology and Biophysics and ⁴ Division of Neuroscience, Baylor College of Medicine, Houston, Texas 77030

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Recent evidence suggests that reactive oxygen species (ROS), including superoxide, are not only neurotoxic but function assmall messenger molecules in normal neuronal processes such assynaptic plasticity. Consistent with this idea, we show that briefincubation of hippocampal slices with the superoxide-generatingsystem xanthine/xanthine oxidase (X/XO) produces a long-lastingpotentiation of synaptic transmission in area CA1. We found thatX/XO-induced potentiation was associated with a persistent superoxide-dependentincrease in autonomous PKC activity that could be isolated viaDEAE column chromatography. The X/XO-induced potentiation wasblocked by the inhibition of PKC, indicating that the superoxide-dependentincrease in autonomous PKC activity was necessary for the potentiation.We also found that X/XO-induced potentiation and long-term potentiation(LTP) occluded one another, suggesting that these forms of plasticityshare similar cellular mechanisms. In further support of thisidea, we found that a persistent, superoxide-dependent increasein autonomous PKC activity isolated via DEAE column chromatographyalso was associated with LTP. Taken together, our findings indicatethat X/XO-induced potentiation and LTP share similar cellularmechanisms, including superoxide-dependent increases in autonomousPKC activity. Finally, our findings suggest that superoxide, inaddition to its well known role as a neurotoxin, also can be considereda small messenger molecule critical for normal neuronalsignaling.

Key words: superoxide; long-term potentiation; hippocampus; protein kinase C; reactive oxygen species; synaptic plasticity

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Long-term potentiation (LTP) is a long-lasting form of synaptic enhancement that has been postulated to underlie learningand memory mechanisms in the mammalian hippocampus (Malenka andNicoll, 1999). The most commonly studied forms of LTP are inducedby high-frequency stimulation (HFS), typically one or more trainsof 100 Hz stimulation, of the Schaffer collateral-commissuralinput to CA1 pyramidal neurons. These forms of LTP are dependenton the activation of the NMDA subtype of glutamate receptors (Collingridgeet al., 1983), influx of Ca²⁺ into the postsynaptic pyramidal neuron (Lynch et al., 1983; Malenkaet al., 1988), and the production of small messenger moleculesthat, along with Ca²⁺, trigger the activation of a number of protein kinase signalingcascades (Roberson et al., 1996; Malenka and Nicoll, 1999).

One of the small messenger molecules produced after high-frequency stimulation that appears to be critical for LTP is thereactive oxygen species (ROS) superoxide. Evidence consistentwith this notion includes the following findings: (1) NMDA receptoractivation results in the production of superoxide in hippocampalslices (Bindokas et al., 1996), (2) cell-permeable scavengersof superoxide block LTP (Klann, 1998), (3) cell-impermeable scavengersof superoxide strongly attenuate LTP (Klann et al., 1998), and(4) hippocampal slices from transgenic mice that overexpress eithercytoplasmic superoxide dismutase (SOD-1) or extracellular superoxidedismutase (EC-SOD) exhibit impaired LTP (Gahtan et al., 1998;Thiels et al., 2000).

In addition, it has been shown that superoxide can interact directly with protein kinase C (PKC), resulting in a persistentincrease in autonomous PKC activity (Knapp and Klann, 2000). Thisis notable because persistent activation of PKC has been shownto be associated with and necessary for the expression of LTP(Klann et al., 1991, 1993; Wang and Feng, 1992; Sacktor et al.,1993; Hrabetova and Sacktor, 1996).

If a molecule such as a superoxide is to be deemed critical for LTP, then it should fulfill certain criteria (Sweatt, 1999).These criteria include the ability of the molecule to producea persistent potentiation in synaptic transmission when addedto hippocampal slices (Sweatt, 1999). Other small messenger moleculesthat have been shown to meet these criteria are arachidonic acid(Williams et al., 1989), nitric oxide (Böhme et al., 1991; Zhuoet al., 1993), carbon monoxide (Zhuo et al., 1993), and cAMP (Freyet al., 1993).

In this manuscript we show that brief exposure of hippocampal slices to xanthine/xanthine oxidase (X/XO), a superoxide-generatingsystem, results in a PKC-dependent, long-lasting potentiation.The X/XO-induced potentiation occludes LTP, which suggests thatboth types of potentiation share similar cellular signaling mechanisms.Finally, we show that both X/XO-induced potentiation and LTP areassociated with a persistent, oxidative activation of PKC. Takentogether, these data are consistent with the notion that superoxidecan function as a physiological signaling molecule and that theoxidative activation of PKC by superoxide is critical forLTP.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Materials. Xanthine (X), superoxide dismutase (SOD), catalase, and bisindolylmaleimide (Bis) were purchased from Calbiochem(La Jolla, CA). 2-Amino-5-phosphonovaleric acid (APV) and DEAE-cellulosewere purchased from Sigma (St. Louis, MO). Xanthine oxidase (XO)was purchased from Roche Molecular Biochemicals (Indianapolis,IN).

Preparation of hippocampal slices and extracellular recordings. Hippocampi from male Sprague Dawley rats (100-150 µg) wereremoved, and 400 µM slices were prepared with a McIlwain tissuechopper. The slices were perfused for 1-2 hr with a standard salinesolution (in mM: 124 NaCl, 4.4 KCl, 26 NaHCO₃, 10 D-glucose, 2CaCl₂, and 2 MgCl₂, gassed with 95% O₂/5% CO₂, pH 7.4) in an interfacetissue slice chamber at 30-32°C. Responses to Schaffer collateralstimulation in area CA1 were monitored for a minimum of 20 minbefore either incubation of the slices with X/XO or delivery ofLTP-inducing HFS. Test stimuli (50 µsec) were given at a current(30-50 µA) that produced 50% of the maximum initial slope of theextracellular field EPSP (fEPSP). Responses to test stimuli weremeasured every 2.5 min as an average of four individual traces(0.1Hz).

Measurement of superoxide generated from X/XO. The concentrations of superoxide produced by X/XO were determined spectrophotometrically(570 $lambda$ ) by measuring the SOD-inhibitable conversion of nitrobluetetrazolium to diformazan (Halliwell and Gutteridge, 1989). Similarconcentrations of superoxide produced by X/XO were observed whenX/XO was present in a test tube and when X/XO was added to slicesin a recordingchamber.

Application of X/XO to hippocampal slices. To determine whether X/XO exerted an effect on hippocampal synaptic transmission,we monitored baseline responses for 20 min to ensure a stablebaseline. Responses then were monitored while the slices wereperfused with X/XO, boiled X/XO, or X/XO in the presence of SODand catalase, usually for 10 min. After washout of the compoundsthe responses were monitored for an additional 45 min. In oneset of experiments the NMDA receptor antagonist APV was presentin the perfusate before, during, and after the application ofX/XO. In another set of experiments paired pulse facilitation(PPF) was measured at several time points before and after perfusionwith X/XO.

Induction of LTP. LTP-inducing HFS consisted of three 1 sec trains of stimuli (100 Hz) given 20 sec apart with the use ofa current (60-100 µA) that elicited the maximum fEPSP. Responsesto test stimuli were measured every 2.5 min as an average of fourindividual traces (0.1 Hz) for 45 min after delivery of the finaltrain of HFS. Post-HFS fEPSPs were elicited by the same test stimulationintensity as before delivery of theHFS.

DEAE column chromatography of PKC. Hippocampal slices were frozen on dry ice 2 and 45 min after the washout of either X/XOor LTP-inducing HFS. For slices that were treated with X/XO, theentire hippocampal slice was homogenized in buffer as describedpreviously (Knapp and Klann, 2000). The homogenates were separatedinto soluble and pellet fractions via centrifugation at 45,000× g at 4°C for 45 min. For homogenates from X/XO-treated slices,the soluble fraction of hippocampal homogenates was applied toa 1 ml DEAE-cellulose column. The column was washed with 3 mlof column buffer (20 mM Tris-HCl, 1 mM EDTA, 100 ng/ml leupeptin,100 ng/ml aprotinin, and 10 µg/ml benzamidine). PKC was elutedin 500 µl fractions by the stepwise addition of column buffersupplemented with 0.1 M NaCl, followed by column buffer supplementedwith 0.25 M NaCl. The fractions were concentrated and desaltedwith the use of Microcon-3 ultrafugation devices (Millipore, Bedford,MA) for 2.5 hr at 4°C.

For the slices that were given LTP-inducing HFS, the CA1 region between the stimulating and recording electrodes was dissectedand homogenized in buffer as described previously (Knapp and Klann,2000). The homogenates were separated into soluble and pelletfractions as described above, and the soluble fraction of hippocampalhomogenates was applied to a 100 µl DEAE-cellulose column. Thecolumn was washed with 300 µl of column buffer, and PKC was elutedin 50 µl fractions by the stepwise addition of column buffer supplementedwith 0.1 M NaCl, followed by column buffer supplemented with 0.25M NaCl. The fractions were concentrated and desalted via Microcon-3ultrafugation devices for 30 min at 4°C.

PKC activity assays. Autonomous and cofactor-dependent PKC activity in each preparation was determined by using the selectivePKC substrate NG(28-43) as described previously (Knapp and Klann,2000).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Xanthine/xanthine oxidase induces a superoxide-dependent, long-lasting potentiation of hippocampal synaptic transmission

To determine whether superoxide could induce a long-lasting potentiation of hippocampal synaptic transmission, we incubatedrat hippocampal slices with X/XO, a superoxide-generating system(Hille and Nishino, 1995). We found that a brief 10 min incubationof hippocampal slices with concentrations of X/XO that produced1-5 µM superoxide resulted in a slight but significant depressionof synaptic transmission while X/XO was present in the perfusate(fEPSP slope = 85 ± 9% of control, n = 10) (Fig. 1A). However,this depression was transient and was followed by a slowly risingpotentiation in the slope of the fEPSP, which reached a maximum35-45 min after the washout of X/XO (fEPSP slope = 159 ± 7% ofcontrol, n = 10) (Fig. 1A,B). The potentiation of the fEPSP slopethat was induced by X/XO persisted for at least 60 min after reachingthe maximum potentiation (data not shown). We observed a similarpotentiation in the slope of the fEPSP when hippocampal sliceswere incubated with concentrations of X/XO that produced 10 µMsuperoxide (fEPSP slope = 170 ± 5% of control, n = 8) (Fig. 1A).Incubation of hippocampal slices with higher concentrations ofX/XO that produced 50 µM superoxide resulted in a more robusttransient depression of synaptic transmission while X/XO was inthe perfusate (51 ± 7% of control, n = 6) (Fig. 1A). After thetransient depression the slope of the fEPSP recovered to baseline,but we observed no long-lasting potentiation 45 min after thewashout of X/XO (fEPSP slope = 97 ± 11% of control, n = 6) (Fig.1A). Thus, potentiation of hippocampal synaptic transmission byX/XO is a concentration-dependent phenomenon. We used concentrationsof X/XO that produce 1-5 µM superoxide for the remainder of ourstudies.

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Figure 1. X/XO-induced potentiation is concentration- and time-dependent. A, X/XO-induced potentiation is dependent on the concentration of superoxide. Stable baseline responses of the fEPSP slope were recorded in hippocampal area CA1 for 20 min before the addition of X/XO (indicated by the bar) for 10 min. X concentrations were kept constant at 20 µg/ml for all experiments. XO concentrations were 2 µg/ml (open circles, n = 10), 15 µg/ml (open squares, n = 8), or 25 µg/ml (filled squares, n = 6). These X/XO concentrations produced superoxide concentrations of 1-5, 10, and 50 µM, respectively. Error bars indicate SEM for the indicated number of determinations. When we compared the fEPSP slope 45 min after the washout of X/XO with the fEPSP slope immediately before the addition of X/XO, statistically significant potentiation was observed for XO concentrations of 2 and 15 µg/ml (p < 0.001 by paired Student's t test). B, Representative fEPSPs before, 30 min after, and 45 min after treatment with X/XO (20 and 2 µg/ml). Calibration: 2 mV, 3 msec. C, X/XO-induced potentiation is dependent on the duration of X/XO incubation. Stable baseline responses were recorded for 20 min before the addition of X/XO (20 and 2 µg/ml) for 5 (open triangles, n = 4), 10 (open circles, n = 10), or 30 (filled triangles, n = 4) min as indicated by the bars. Error bars are SEM for the indicated number of determinations. When we compared the fEPSP slope 45 min after the washout of X/XO with the fEPSP slope immediately before the addition of X/XO, statistically significant potentiation was observed for the 5 and 10 min X/XO incubations (p < 0.01 and 0.001, respectively, by paired Student's t test).

We also determined whether the X/XO-induced potentiation in hippocampal synaptic transmission was time-dependent. A 5 minincubation of hippocampal slices with concentrations of X/XO thatproduced 1-5 µM superoxide did not result in a transient depressionof synaptic transmission while X/XO was in the perfusate (fEPSPslope = 101 ± 8% of control, n = 4) (Fig. 1C). However, similarto experiments with 10 min incubations of X/XO, we did observea slowly rising potentiation in the slope of the fEPSP that peaked35-45 min after the washout of X/XO (fEPSP slope = 136 ± 9% ofcontrol, n = 4) (Fig. 1C). In contrast, a 30 min incubation ofhippocampal slices with the same concentration of X/XO produceda transient depression of synaptic transmission while X/XO wasin the perfusate (fEPSP slope = 89 ± 6% of control, n = 4) (Fig.1B), followed by a slowly rising potentiation that peaked 35-45min after the washout of X/XO (fEPSP slope = 131 ± 9% of control,n = 4) (Fig. 1C). These results indicate that X/XO-induced potentiationof synaptic transmission can be induced with incubations of X/XOin a range of 5-30 min. We used 10 min incubations for the remainderof ourstudies.

The X/XO superoxide-generating system also produces hydrogen peroxide. Therefore, we determined whether either superoxideor hydrogen peroxide was responsible for the X/XO-induced potentiationof synaptic transmission. In a subset of experiments in whichhippocampal slices were incubated with X/XO, we added either SODor catalase to remove superoxide and hydrogen peroxide, respectively.As illustrated in Figure 2A, hippocampal slices incubated withX/XO in the presence of SOD did not exhibit a long-lasting potentiationof the fEPSP 45 min after the washout of these compounds (fEPSPslope = 107 ± 5% of control, n = 8). Hippocampal slices incubatedwith X/XO in the presence of catalase (Fig. 2A) did exhibit along-lasting potentiation of the fEPSP 45 min after the washoutof these compounds (fEPSP slope = 136 ± 4% of control, n = 8).However, this increase was not as robust as that observed whenslices were treated with X/XO alone, which suggests that hydrogenperoxide is necessary for the full X/XO-induced enhancement ofsynaptic transmission. Interestingly, the effect of catalase onX/XO-induced potentiation is very similar to the effect of catalaseon LTP in mouse hippocampal slices (Thiels et al., 2000). To ensurethat the X/XO-induced potentiation was not attributable to nonspecificeffects of XO, we treated slices with X and XO that had been inactivatedby boiling. As shown in Figure 2B, we observed neither a transientdepression while X/boiled XO was in the perfusate (fEPSP slope= 96 ± 6% of control, n = 8) nor a slowly rising potentiationafter the washout of X/boiled XO (fEPSP slope = 105 ± 5% of control,n = 8). Taken together, these data indicate that, whereas superoxideabsolutely is required for X/XO-induced potentiation, hydrogenperoxide also contributes this type of potentiation in hippocampalslices.

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Figure 2. Characterization of X/XO-induced potentiation. A, X/XO-induced potentiation is superoxide-dependent. Stable baseline responses were recorded for 20 min before the slices were incubated with X/XO and antioxidant enzymes for 10 min (indicated by the bar). Open circles are ensemble averages from slices incubated with X/XO (20 and 2 µg/ml) and SOD (25 µg/ml). Filled circles are ensemble averages from slices incubated with X/XO and catalase (25 µg/ml). Error bars are SEM for eight determinations. When we compared the fEPSP slope 45 min after the washout of X/XO with the fEPSP slope immediately before the addition of X/XO, statistically significant potentiation was observed in the presence of catalase (p < 0.001). B, Specificity of X/XO-induced potentiation. Filled squares are ensemble averages from slices incubated with X (20 µg/ml) and boiled XO (2 µg/ml). Error bars are SEM for eight determinations. C, X/XO-induced potentiation is downstream of NMDA receptor activation. Stable baseline responses were recorded for 20 min before the slices were incubated with X/XO (20 and 2 µg/ml) for 10 min either with (filled triangles) or without (open triangles) the NMDA receptor antagonist APV (50 µM) in the perfusate (indicated by the bars). Error bars are SEM for six determinations. There was no statistically significant difference in the potentiation between the groups 45 min after the washout of X/XO (p > 0.05 by paired Student's t test).

Interestingly, the transient depression in synaptic transmission that we observed when hippocampal slices were treated withX/XO alone was blocked in the presence of either SOD or catalase(Fig. 2A). These data suggest that superoxide and hydrogen peroxideare necessary for the transient depression in synaptic transmissionthat is induced by X/XO.

If an ROS such as superoxide acts as a cellular messenger in LTP, then its actions should be independent of NMDA receptoractivation because the application of exogenous superoxide wouldbe downstream of this step in the pathway. Therefore, we examinedthe effect of APV, an NMDA receptor antagonist that blocks theinduction of LTP (Collingridge et al., 1983), on X/XO-inducedpotentiation. When hippocampal slices perfused with 50 µM APVwere incubated with X/XO for 10 min, we observed a transient depressionof synaptic transmission while X/XO was in the perfusate (fEPSPslope = 92 ± 5% of control, n = 6) (Fig. 2C), followed by theslowly rising potentiation of synaptic transmission (fEPSP slope= 148 ± 13% of control, n = 6) (Fig. 2C). The potentiation inducedby X/XO in the presence of APV was not different from those slicestreated with X/XO alone (fEPSP slope = 158 ± 7% of control, n= 6). These results are consistent with the notion that superoxidemight act as a cellular messenger downstream of NMDA receptoractivation inLTP.

Cell-impermeable scavengers of superoxide have been shown to attenuate LTP (Klann et al., 1998), suggesting that superoxidemay need to enter the extracellular space after LTP-inducing stimulation.In addition, the incubation of hippocampal slices with X/XO hasbeen shown to result in a superoxide-dependent increase in therelease of glutamate (Pellegrini-Giampietro et al., 1988). Takentogether, these data suggest the possibility that X/XO-inducedpotentiation is expressed presynaptically. Therefore, we examinedthe effects of X/XO on PPF, a well characterized presynaptic processin which facilitation is revealed when the second of two presynapticaction potentials results in increased neurotransmitter releaserelative to the response of the first action potential. Therefore,we measured PPF before and after slices were incubated with X/XO.We observed a small but significant increase in PPF (117 ± 6%of control, n = 6) immediately after the washout of X/XO (Fig.3, top) that coincided with the transient depression induced byX/XO (Fig. 3, bottom). Interestingly, we observed small but significantincreases in PPF that coincided with the slowly rising potentiationboth 20 (92 ± 3% of control, n = 6) and 30 min (90 ± 4% of control,n = 6) after the washout of X/XO (Fig. 3). However, PPF returnedto control levels by the time that potentiation stabilized 40min after the washout of X/XO (Fig. 3). Taken together, theseresults suggest that the cellular mechanisms underlying both thetransient depression and the initial potentiation induced by X/XOare at least partially presynaptic.

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Figure 3. Effect of X/XO on PPF. PPF was examined every 10 min with four sets of paired pulses, with an interpair interval of 20 sec and an interpulse interval of 50 msec. The change in PPF was expressed as the percentage of PPF at 0 min (the ratio of the second response to the first response). There was no alteration in PPF until immediately after the washout of X/XO (20 and 2 µg/ml), when we observed a increase in PPF that coincided with transient depression induced by X/XO. We also observed decreases in PPF 20 and 30 min after the washout of X/XO that coincided with the slowly rising potentiation induced by X/XO. Error bars are SEM for six determinations. *Statistical significance with a paired Student's t test (p < 0.05).

X/XO induces a persistent superoxide-dependent increase in autonomous PKC activity in hippocampal slices

Previously, we have observed a persistent increase in autonomous PKC activity in hippocampal slices exposed to X/XO, whichcan be isolated via DEAE-cellulose chromatography (Knapp and Klann,2000). Once again, we treated hippocampal slices for 10 min withX/XO; 45 min after the washout of X/XO the slices were homogenizedand subjected to DEAE-cellulose column chromatography. As hasbeen reported previously, we observed two fractions of cofactor-dependentPKC activity that eluted from the DEAE columns with 0.1 and 0.25M NaCl salt washes after an application of the soluble fractionof hippocampal homogenates in both control (X/boiled XO) and X/XO-treatedslices (data not shown). In addition, we observed a unique peakof autonomous PKC activity that could be eluted with 0.25 M NaClin X/XO-treated slices, but not in the control slices treatedwith X/boiled XO (Fig. 4). We did not observe this peak of autonomousPKC activity when X/XO-treated slices were incubated with SOD(Fig. 4). The unique peak of autonomous PKC activity induced byX/XO was not affected by incubation with catalase (Fig. 4). Takentogether, these data indicate that X/XO induces a persistent increasein autonomous PKC activity in hippocampal slices that is dependenton superoxide but that is not dependent on hydrogen peroxide.

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Figure 4. Effect of X/XO on autonomous PKC activity isolated from slices with DEAE column chromatography. Slices were incubated with X/boiled XO (open squares, n = 5), X/XO (open circles, n = 5), X/XO + SOD (filled squares, n = 5), or X/XO + catalase (filled circles, n = 5) for 10 min, and the incubations were followed by perfusion with normal saline solution for 45 min. Then the slices were frozen on dry ice and homogenized; the soluble fraction of the homogenates was applied to a DEAE column. PKC was eluted from the column with either 0.1 or 0.25 M NaCl (arrows), and autonomous PKC activity was measured in each fraction as described in Materials and Methods.

X/XO-induced potentiation in hippocampal slices is PKC-dependent

Because X/XO can induce a persistent, superoxide-dependent increase in autonomous PKC activity in hippocampal slices in amanner similar to that previously observed in electrically inducedLTP (Klann et al., 1998), we hypothesized that the X/XO-inducedpotentiation observed in Figure 1 was PKC-dependent. To test thishypothesis, we added X/XO to hippocampal slices in the presenceof 500 nM bisindolylmaleimide I (Bis), a highly selective PKCinhibitor that acts on the catalytic domain of PKC (Toullec etal., 1991). As shown in Figure 5A, we observed that Bis blockedthe X/XO-induced potentiation in synaptic transmission (fEPSPslope = 111 ± 5% of control, n = 8). Therefore, activation ofPKC is necessary for X/XO-induced potentiation. It is interestingto note that the transient depression induced by X/XO still wasobserved in the presence of Bis (Fig. 5A), which suggests thatthis type of plasticity is not a manifestation of superoxide-inducedstimulation of PKC.

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Figure 5. Effect of the PKC inhibitor Bis on X/XO-induced potentiation and X/XO-induced increase in autonomous PKC activity. A, X/XO-induced potentiation is PKC-dependent. Stable baseline responses of the fEPSP slope were recorded for 20 min before the slices were incubated with X/XO (20 and 2 µg/ml) for 10 min in the presence of the PKC inhibitor Bis (500 nM) as indicated by the bars. Error bars are SEM for eight determinations. When we compared the fEPSP slope 45 min after the washout of X/XO with the fEPSP slope immediately before the addition of X/XO, no statistically significant potentiation was observed (p > 0.05 by paired Student's t test) B, X/XO-induced persistent increase in autonomous PKC activity is present after the washout of Bis. Slices were incubated with either normal saline (open circles, n = 5) or X/XO (filled circles, n = 5) in the presence of Bis as described in A. At the end of the experiment the slices were frozen and homogenized. The soluble fraction of the homogenates was applied to a DEAE column, and PKC was eluted from the column with either 0.1 or 0.25 M NaCl (arrows). Autonomous PKC activity was measured in each fraction as described in Materials and Methods.

Previously, we have investigated the modification of PKC induced by superoxide and determined that the regulatory domain ofPKC is required because PKM, the free catalytic domain of PKC,was not stimulated by superoxide (Knapp and Klann, 2000). If superoxidestimulates PKC by acting on the regulatory domain, then we wouldexpect to observe the superoxide-stimulated peak of autonomousPKC activity eluted from a DEAE column from slices exposed toX/XO in the presence of Bis. As shown in Figure 5B, we observedthe expected unique peak of autonomous PKC activity from DEAEcolumns from slices treated with X/XO in the presence of Bis.This finding suggests that a block of the X/XO-induced potentiationby Bis cannot be attributable to interference with the superoxide-inducedstimulation ofPKC.

To ensure that Bis could inhibit oxidatively activated PKC, we performed in vitro assays to determine whether Bis could inhibitX/XO-induced increases in autonomous PKC activity. Purified PKCwas treated with X/XO as described previously (Knapp and Klann,2000) in the presence and absence of 500 nM Bis. Treatment ofpurified PKC with X/XO resulted in increased autonomous enzymeactivity (control = 4.23 ± 0.34 pmol/min; X/XO = 18.34 ± 1.67pmol/min; n = 4) that was inhibited completely by Bis (controlplus Bis = 0.19 ± 0.02 pmol/min; X/XO = 0.25 ± 0.07 pmol/min;n = 4). Thus, Bis is able to inhibit oxidatively activatedPKC.

X/XO-induced potentiation and LTP share similar cellular mechanisms

If the potentiation induced by superoxide contributes to LTP, then that potentiation should occlude LTP. To test this possibility,we treated slices with X/XO; 60 min after the washout of the X/XOthe stimulation intensity was reduced to obtain a new baseline,and HFS was delivered to the slices. Figure 6A shows that, afterpotentiation by X/XO, HFS did not result in a significant enhancementof synaptic transmission (fEPSP slope = 108 ± 9% of control, n= 6). However, if X/XO-induced potentiation was blocked by SOD,then HFS elicited LTP (fEPSP slope = 168 ± 8% of control, n =6) (Fig. 6B). We also determined whether LTP could occlude X/XO-inducedpotentiation. LTP was induced with HFS; 30 min after the lasttrain the stimulation intensity was reduced to obtain a new baseline.Figure 6C shows that, after the establishment of LTP, the applicationof X/XO to the slices did not enhance synaptic transmission significantly(fEPSP slope = 110 ± 10% of control, n = 6). However, if LTP wasblocked by APV, then the application of X/XO to the slices resultedin potentiation (fEPSP slope = 148 ± 8% of control, n = 6). Takentogether, the findings in Figure 6 suggest that the X/XO-inducedpotentiation and LTP share similar cellular mechanisms.

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Figure 6. X/XO-induced potentiation and LTP occlude each other. A, X/XO-induced potentiation occludes LTP. Stable baseline responses of the fEPSP slope were recorded for 20 min before the slices were incubated with X/XO (20 and 2 µg/ml) as indicated by the bar. At 60 min after the washout of X/XO the stimulus intensity was reduced (indicated by the down arrow) to match the fEPSP slope before exposure to X/XO. LTP-inducing HFS (indicated by the up arrow) then was delivered to the slices as described in Materials and Methods. Additional incubations of the slices with X/XO before HFS did not produce additional potentiation, indicating that the X/XO-induced potentiation was saturated (data not shown). Error bars are SEM for six determinations. B, LTP can be induced after a blockade of X/XO-induced potentiation by SOD. Slices were incubated with X/XO and SOD (25 µg/ml) as indicated by the bar. At 60 min after the washout of X/XO and SOD, LTP-inducing HFS (indicated by the arrow) was delivered to the slices. Error bars are SEM for six determinations. C, LTP occludes X/XO-induced potentiation. Stable baseline responses in hippocampal slices were recorded for 20 min before the delivery of LTP-inducing HFS as indicated by the up arrow. At 30 min after the last train of HFS the stimulus intensity was reduced (indicated by the down arrow) to match the fEPSP slope before the HFS. Slices then were incubated with X/XO (20 and 2 µg/ml) as indicated by the bar. Additional delivery of HFS before incubation of the slices with X/XO did not produce additional potentiation, indicating that LTP was saturated (data not shown). Error bars are SEM for six determinations. D, X/XO can induce potentiation after a blockade of LTP by APV. HFS (indicated by the arrow) was delivered to the slices in the presence of APV (indicated by the bar). At 30 min after HFS the slices were incubated with X/XO as indicated by the bar. Error bars are SEM for six determinations.

Because X/XO-induced potentiation and LTP are likely to share similar cellular mechanisms, we determined whether LTP was associatedwith superoxide-stimulated PKC. We delivered HFS to the Schaffercollateral input to area CA1, which resulted in LTP (for 2 minexperiments, fEPSP slope = 181 ± 5% of control, n = 5; for 45min experiments, fEPSP slope = 158 ± 7% of control, n = 5) (Fig.7A). We observed a typical elution profile of cofactor-dependentPKC activity from DEAE columns from LTP slices at both 2 and 45min after the last train of HFS that was not different from controlslices (Fig. 7B,C). However, we detected a unique peak of autonomousPKC activity in LTP slices both 2 and 45 min after the last trainof HFS that was not detected in control slices (Fig. 8A,B). Thesedata are consistent with the idea that superoxide-induced stimulationof autonomous PKC activity is a biochemical mechanism involvedin the induction and expression of both X/XO-induced potentiationand LTP.

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Figure 7. No alteration in the DEAE column elution profile of cofactor-dependent PKC activity after the induction of LTP. A, Induction of LTP. Stable baseline responses of the fEPSP slope were recorded in hippocampal slices for 20 min before the delivery of HFS as indicated by the arrow. Responses were recorded for either 2 min (filled circles, n = 5) or 45 min (open squares, n = 5) after the final train of HFS. Error bars are SEM for the indicated number of determinations. B, C, Elution profile of cofactor-dependent PKC activity from either control slices (open circles in B, open squares in C) or slices taken 2 min (filled circles in B) and 45 min (filled squares in C) after the final train of LTP-inducing HFS. Either 2 or 45 min after the final train of HFS the slices were frozen, and the area between the stimulating and recording electrodes was dissected and homogenized. The soluble fraction of the homogenates was applied to mini-DEAE columns, and PKC was eluted with either 0.1 or 0.25 M NaCl (arrows). Cofactor-dependent PKC activity was measured as described in Materials and Methods.

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Figure 8. LTP is associated with a unique peak of autonomous PKC activity that elutes from DEAE columns. Shown are elution profiles of autonomous PKC activity from either control slices (open circles in A; open squares in B) or slices taken 2 min (filled circles in A) and 45 min (filled squares in B) after the final train of LTP-inducing HFS. Either 2 min (n = 5) or 45 min (n = 5) after the final train of HFS the slices were frozen, and the area between the stimulating and recording electrodes was dissected and homogenized. The soluble fraction of the homogenates was applied to mini-DEAE columns, and PKC was eluted with either 0.1 or 0.25 M NaCl (arrows). Autonomous PKC activity was measured as described in Materials and Methods.

We performed control experiments to ensure that the unique peak of superoxide-stimulated autonomous PKC activity was specificto LTP. First, we delivered test stimulation to slices with thesame number of stimuli as given during HFS, but at low frequency(0.1 Hz). When the soluble fraction of homogenates from theseslices was applied to DEAE columns, we did not observe the uniquepeak of autonomous PKC activity (Fig. 9A). In addition, we deliveredHFS to slices in the presence of either the NMDA receptor antagonistAPV or SOD and applied the soluble fraction of homogenates fromthese slices to DEAE columns. Once again, we did not observe theunique peak of autonomous PKC activity (Fig. 9B,C). These resultsindicate that the LTP-associated appearance of superoxide-stimulatedPKC that eluted from the DEAE columns cannot be elicited by eitherlow-frequency stimulation or HFS in the absence of LTP. The resultsof the APV and SOD experiments also indicate that NMDA receptoractivation and the subsequent production of superoxide are necessaryto trigger the oxidative activation of PKC.

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Figure 9. The LTP-associated unique peak of autonomous PKC activity is NMDA- and superoxide-dependent. Shown are elution profiles of autonomous PKC activity from control slices and slices that were given test pulses (A), slices in which HFS was delivered in the presence of APV (B), and slices in which HFS was delivered in the presence of SOD (C). In each panel, n = 5.

Because the PKC inhibitor Bis was able to block X/XO-induced potentiation (Fig. 5A), we asked whether this inhibitor was ableto block LTP. As shown in Figure 10, delivery of HFS in the presenceof 500 nM Bis significantly attenuated LTP (fEPSP slope = 122± 6% of control, n = 6) compared with control slices from thesame animal in which HFS was delivered in the presence of saline(fEPSP slope = 167 ± 5% of control, n = 6). These results areconsistent with the idea that the oxidative activation of PKCplays a role in both forms of potentiation.

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Figure 10. The PKC inhibitor Bis attenuates LTP. Open circles are ensemble averages from control LTP experiments. Filled circles are ensemble averages from slices given LTP-inducing HFS with 500 nM Bis in the perfusing solution (indicated by the bar). Responses recorded from slices given LTP-inducing HFS in the presence of Bis were compared with responses recorded from a control slice from the same animal (in an adjacent recording chamber) that received HFS in the absence of the inhibitor. Error bars are SEM for six determinations. When we compared the fEPSP slope 45 min after HFS with the fEPSP slope immediately before HFS, small but statistically significant potentiation was observed in the presence of Bis (p < 0.05 by paired Student's t test).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The results presented herein demonstrate that superoxide is necessary for X/XO-induced potentiation in area CA1 of rat hippocampalslices and that this type of potentiation requires superoxide-inducedstimulation of autonomous PKC activity. In addition, we have shownthat we can isolate superoxide-stimulated PKC not only from slicesthat were incubated with X/XO but also from slices in which LTPwas induced. Finally, we have shown that X/XO-induced potentiationand LTP occlude one another. Taken together, these data suggestthat X/XO-induced potentiation and LTP share similar cellularmechanisms, including the oxidative activation ofPKC.

Previous results from studies on the effects of ROS on synaptic transmission indicate that the role of ROS in modulating synaptictransmission is complex, depending on numerous factors that contributeto the stringency of oxidation. Various ROS with divergent oxidativestrengths have been shown to affect synaptic transmission. Forexample, hydroxyl radical is a stronger oxidant than hydrogenperoxide, which, in turn, is stronger than superoxide (Rice-Evansand Burdon, 1994). In previous studies strong oxidizing conditionsthat promote hydroxyl radical production were found to inhibitsynaptic transmission (Pellmar, 1987; Auerbach and Segal, 1997).Another factor that influences the stringency of oxidation isthe length of oxidant exposure. For example, prolonged (>55 min)exposure of hippocampal slices to superoxide inhibits synaptictransmission (Pellmar and Lepinski, 1992). In the studies presentedherein, slices were exposed briefly (10 min) to low concentrations(Knapp and Klann, 2000) of ROS. Thus, we have characterized aphysiological role for ROS in promoting a long-lasting enhancementin synaptictransmission.

We recently showed that superoxide-dependent stimulation of autonomous PKC activity is achieved via interaction of superoxidewith the cysteine-rich zinc finger motif in the regulatory domainof the enzyme (Knapp and Klann, 2000). In a series of biochemicalstudies we showed that superoxide stimulates autonomous PKC activityvia thiol oxidation and the release of zinc from the cysteine-richzinc finger motifs. Based on the elution profiles of autonomousPKC activity from LTP samples (Fig. 8), it is reasonable to proposethat LTP-inducing HFS induces a similar release of zinc from PKC.An obvious question arises: Which PKC isoform is stimulated bysuperoxide during LTP? PKC isoforms from each PKC subfamily (classical,novel, and atypical) can be stimulated by superoxide (Knapp andKlann, 2000), and numerous PKC isoforms are present in the superoxide-stimulatedDEAE column fraction that elutes with 0.25 M NaCl (our unpublishedobservations). Thus, the identity of the PKC isoform(s) stimulatedby superoxide after the induction of LTP will need to be determinedin the future by othermeans.

In the current studies we focused on the participation of superoxide-stimulated PKC in the potentiation of hippocampal synaptictransmission. However, it is not our intention to imply that PKCis the only signaling enzyme that is affected by ROS such as superoxideduring either X/XO-induced potentiation or LTP. There are a numberof other effector molecules that are known to be important forsynaptic plasticity and that are likely to be modulated by superoxide.For instance, activation of extracellular signal-regulated kinase(ERK) is necessary for LTP (English and Sweatt, 1997), and ERKactivity in hippocampal slices is stimulated by ROS, includingsuperoxide (Kanterewicz et al., 1998). Tyrosine kinase activityhas been shown to be necessary for LTP (O'Dell et al., 1991; Grantet al., 1992; Kang and Schuman, 1995; Lu et al., 1998), and manytyrosine kinases have been shown to exhibit increased activityin response to ROS (Chan et al., 1986; Scheiven et al., 1993;Guyton et al., 1996). In addition, superoxide inhibits the activityof the protein phosphatase calcineurin in vitro (Wang et al.,1996) and in cultured hippocampal neurons after electrical stimulation(Bito et al., 1996). Therefore, it is reasonable to propose thatboth X/XO-induced potentiation and LTP involve superoxide-dependentincreases in ERK activity and/or inhibition of calcineurin inaddition to stimulation of autonomous PKCactivity.

The notion that multiple signaling cascades must be modulated by ROS for X/XO-induced potentiation is supported by the findingsshown in Figure 5. We found that the PKC inhibitor Bis could blockX/XO-induced potentiation (Fig. 5A). Because superoxide interactswith the regulatory domain of PKC (Knapp and Klann, 2000) andBis inhibits PKC by interacting with the ATP-binding site in thecatalytic domain (Toullec et al., 1991), we hypothesized thatsuperoxide-stimulated PKC activity still should be present inhippocampal slices after the washout of Bis. This hypothesis wasfound to be correct (Fig. 5B), indicating that Bis did not interferewith the interaction of superoxide with PKC. Interestingly, weobserved no potentiation in synaptic transmission after the washoutof Bis (Fig. 5A). This result suggests that the superoxide-dependentstimulation of PKC activity alone is not sufficient for X/XO-inducedpotentiation. It is possible that X/XO-induced potentiation requireseither the concomitant activation of PKC and ERK or the activationof PKC coupled with the inhibition of a protein phosphatase suchascalcineurin.

We have shown that X/XO-induced potentiation is dependent on superoxide (Fig. 2A) and is occluded by LTP (Fig. 6A). Takentogether, these findings suggest that LTP, like X/XO-induced potentiation,is dependent on superoxide. This idea is supported further byprevious findings showing that cell-permeable scavengers of superoxideblock LTP (Klann, 1998), cell-impermeable scavengers of superoxidestrongly attenuate LTP (Klann et al., 1998), and slices from micethat overexpress either SOD-1 (Gahtan et al., 1998) or EC-SOD(Thiels et al., 2000) exhibit deficient LTP. Thus, it is now criticalto determine the source of superoxide production after LTP. Possiblesources of LTP-dependent superoxide production that have beensuggested include arachidonic acid metabolism, nitric oxide synthase,and the mitochondrial electron transport chain (Thiels et al.,2000). Another possibility is endogenous XO. There is evidencefor XO activity being present in brain tissue (Markley et al.,1975) and from synaptosomal preparations (Deliconstantinos andVilliotou, 1996). However, we found that the incubation of hippocampalslices with X/boiled XO did not result in long-lasting potentiation,which suggests that endogenous XO is not capable of producingsufficient superoxide for LTP in hippocampal slice preparations.This finding also indicates that nonspecific effects of xanthinecannot account for X/XO-inducedpotentiation.

Another candidate enzyme for superoxide production during LTP is NADPH oxidase. This enzyme is a heterotetramer of cytosolicand membrane-associated proteins that can be activated by thesmall G-protein Rac1 (Shatwell and Segal, 1996). The expressionof NADPH oxidase originally was characterized in phagocytic neutrophilsof the immune system (Shatwell and Segal, 1996). However, thereis evidence that NADPH oxidase and Rac1 also are expressed inthe brain and, in particular, the hippocampus (Olenik et al.,1997; Mizuki et al., 1998). Interestingly, Rac1 is one of theproteins that has been shown to be associated with NMDA receptormultiprotein complexes (Husi et al., 2000), making it a candidatefor regulation after the induction of LTP. It remains to be determinedwhether the cytosolic and/or membrane-associated NADPH oxidaseproteins also are associated with NMDA receptor multiproteincomplexes.

In addition to the role that superoxide plays in hippocampal LTP, superoxide also appears to be necessary for hippocampus-dependentlearning and memory. For example, mice that overexpress EC-SODwere shown to have deficits in their ability to execute the eight-armradial maze task (Levin et al., 1998) and in contextual fear conditioning(Thiels et al., 2000). Moreover, mice that overexpress SOD-1 wereshown to have deficits in their ability to learn the spatial versionof the Morris water maze task (Gahtan et al., 1998). Overall,these findings are consistent with superoxide signaling beinga necessary component of hippocampus-dependent learning and memory.It will be of great interest to determine whether the superoxide-stimulatedautonomous PKC activity associated with X/XO-induced potentiationand LTP also can be isolated in hippocampal lysates from ratsthat have acquired either contextual fear conditioning or varioustypes of spatialtasks.

A number of our findings suggest that X/XO-induced potentiation and LTP share similar cellular mechanisms. This is supportedby the following findings: (1) X/XO-induced potentiation and LTPocclude one another; (2) X/XO-induced potentiation and LTP areassociated with superoxide-dependent increases in autonomous PKCactivity; (3) the magnitudes of X/XO-induced potentiation andLTP are reduced by the PKC inhibitor Bis. However, several ofour findings point to differences in these forms of potentiation.First, the onset of X/XO-induced potentiation is much slower thanLTP (compare Figs. 1A, 7A), similar to previous experiments withother small messenger molecules that can induce potentiation (Zhuoet al., 1993). Second, PPF is altered during the initial, slowlyrising phase of X/XO-induced potentiation (Fig. 3), a result thatis not observed consistently with LTP (for review, see Malenkaand Nicoll, 1999). Finally, the PKC inhibitor Bis blocked X/XO-inducedpotentiation (Fig. 5A) but only attenuated LTP (Fig. 10). Takentogether, these results suggest that cellular signaling mechanismsunderlying X/XO-induced potentiation and LTP are similar, butnotidentical.

In closing, our studies demonstrate that superoxide can produce a persistent potentiation in synaptic transmission when addedto hippocampal slices and that this potentiation shares similarcellular mechanisms with LTP. Thus, superoxide should be addedto the list of small messenger molecules that are necessary forhippocampalLTP.

  FOOTNOTES

Received Sept. 21, 2001; revised Nov. 7, 2001; accepted Nov. 7, 2001.

This work was supported by National Institutes of Health Grant NS34007 (E.K.) and National Research Service Award MH 18273(L.T.K.). We thank Dr. Edda Thiels, Dr. Eric D. Norman, and BeatrizI. Kanterewicz for helpful comments throughout these studies andDr. J. David Sweatt for critically reading thismanuscript.
Correspondence should be addressed to Dr. Eric Klann, Department of Molecular Physiology and Biophysics, Baylor College ofMedicine, One Baylor Plaza, Houston, TX 77030. E-mail: eklann{at}bcm.tmc.edu.

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