Reactive Oxygen Species Mediate Activity-Dependent Neuron-Glia Signaling in Output Fibers of the Hippocampus

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The Journal of Neuroscience, September 1, 1999, 19(17):7241-7248

Reactive Oxygen Species Mediate Activity-Dependent Neuron-Glia Signaling in Output Fibers of the Hippocampus
Coleen M. Atkins and J. David Sweatt
Division of Neuroscience, Baylor College of Medicine, Houston, Texas 77030

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Nonsynaptic signaling is becoming increasingly appreciated in studies of activity-dependent changes in the nervous system.We investigated the types of neuronal activity that elicit nonsynapticcommunication between neurons and glial cells in hippocampal outputfibers. High-frequency, but not low-frequency, action potentialfiring in myelinated CA1 axons of the hippocampus resulted inincreased phosphorylation of the oligodendrocyte-specific proteinmyelin basic protein (MBP). This change was blocked by tetrodotoxin,indicating that axonally generated action potentials were necessaryto regulate the phosphorylation state of MBP. Furthermore, scavengersof the reactive oxygen species superoxide and hydrogen peroxideand nitric oxide synthase inhibitors prevented activation of thisneuron-glia signaling pathway. These results indicate that, duringperiods of increased neuronal activity in area CA1 of the hippocampus,reactive oxygen and nitrogen species are generated, which diffuseto neighboring oligodendrocytes and result in post-translationalmodifications of MBP, a key structural protein in myelin. Thus,in addition to their well-known capacity for activity-dependentneuron-neuron signaling, hippocampal pyramidal neurons possessa mechanism for activity-dependent neuron-gliasignaling.

Key words: hippocampus; oligodendrocyte; glia; myelin; myelin basic protein; reactive oxygen species; superoxide; nitric oxide; hydrogen peroxide; alveus; neuron-glia signaling

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Recent progress in studies of nonsynaptic cellular communication in the nervous system has illustrated the important rolethis form of signaling has during development, synaptic plasticity,and pathogenesis. This type of cellular communication has thepower of a larger sphere of cellular influence than synaptic signaling,tends to have a long duration in its effects, and is not limitedto cell types directly coupled by synapticconnections.

Several forms of nonsynaptic signaling have functional consequences in a variety of neuronal circuits, including electrotoniccoupling by gap junctions, electric field effects, and signalingby diffusible molecules (Bach-y-Rita, 1993; Jefferys, 1995; Vanhataloand Soinila, 1998). In the developing cortex, gap junctions mediatesynchronous calcium oscillations to contribute to cortical columnarchitecture (Connors et al., 1983; Peinado et al., 1993; Dermietzel,1998). Electrical fields play a key role in synchronizing neuronalfiring during interictal epileptic discharges (Snow and Dudek,1984; Jefferys, 1995). Recently, reactive oxygen and nitrogenspecies have received considerable attention, because the diffusiblemessengers nitric oxide and superoxide have been found to modulatediverse forms of synaptic plasticity (Böhme et al., 1991; O'Dellet al., 1991, 1994; Shibuki and Okada, 1991; Haley et al., 1992;Daniel et al., 1993; Williams et al., 1993; Bito et al., 1996;Kantor et al., 1996; Son et al., 1996; Wilson et al., 1997; Gahtanet al., 1998; Klann et al., 1998).

One form of synaptic plasticity well studied in the context of nonsynaptic cellular signaling is hippocampal long-term potentiation(LTP), which is a persistent increase in synaptic efficacy elicitedby brief, high-frequency stimulation. LTP induced by modest tetanicstimulation is inhibited by nitric oxide synthase inhibitors,whereas strong LTP-inducing stimulation can mitigate this inhibition(Chetkovich et al., 1993; O'Dell et al., 1994; Williams et al.,1993; Kantor et al., 1996; Son et al., 1996; Wilson et al., 1997;Gahtan et al., 1998; Klann et al., 1998). Interestingly, an adjacentnonsynaptically connected neuron can express LTP when LTP is inducedin a neighboring neuron (Schuman and Madison, 1994). This requiresnitric oxide synthase activity, providing compelling evidencethat nitric oxide can act as an intercellular messenger duringLTP. It has been proposed that reactive oxygen and nitrogen speciesact by activating protein kinase C (PKC) and mitogen-activatedprotein kinase (MAPK) during LTP because these enzymes are requiredfor LTP and are activated by reactive oxygen species in the hippocampus(Roberson et al., 1996; Klann et al., 1998).

Recently, we observed an increase in myelin basic protein (MBP) phosphorylation by PKC during hippocampal CA1 LTP (Atkinset al., 1997). These results are intriguing, because MBP, a keystructural protein in myelin of the CNS, is located only in myelinatingoligodendrocytes and Schwann cells (Hartman et al., 1979). Ifwe assume that LTP is induced neuronally, then these findingssuggest that neurons and oligodendrocytes communicate nonsynapticallyduring periods of increased neuronal activity. The present studyinvestigates this novel form of nonsynaptic neuron-glia signalingin thehippocampus.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Hippocampal slice preparation. Standard hippocampal slice preparations were prepared as described previously(Roberson andSweatt, 1996). All experiments were performed in compliance withthe Baylor College of Medicine Institutional Animal Care and UseCommittee and national regulations and policies. The alveus wasstimulated antidromically, and extracellular field recordingswere made in stratum pyramidale of the CA1 region. The amplitudeof the population spike was measured. Low-frequency stimulation(LFS) (0.05 Hz) was delivered at a stimulus intensity 30-40% ofthe maximum response. High-frequency stimulation (HFS) consistedof three sets of tetani (two 100 Hz, 1-sec-long tetani, separatedby 20 sec) separated by 5 min given at the minimum stimulationintensity that elicited 75% of the maximum response. Forty-fiveminutes after delivery of the final tetani, the hippocampal sliceswere frozen on dry ice, and CA1 regions were microdissected. Forexperiments in which calcium was omitted from the saline, magnesiumconcentrations were increased to 6 mM.

MBP phosphorylation assay. To assess changes in the phosphorylation state of MBP, a back-phosphorylation assay was performedas described previously (Atkins et al., 1997). Hippocampal CA1regions were homogenized in buffer (50 mM Tris-HCl, pH 7.5, 1mM EGTA, 1 mM EDTA, 2 mM Na₄P₂O₇, 10 µg/ml aprotinin, 10 µg/mlleupeptin, and 100 µM phenylmethylsulfonyl fluoride) and boiledfor 10 min at 95°C. To back-phosphorylate MBP, exogenous PKC (purifiedaccording to the method of Huang et al., 1986), CaCl₂ (1.5 mM),l- $alpha$ -phosphatidylserine (320 µg/ml), 1,2-dioctanoyl-sn-glycerol(30 µg/ml), [ $gamma$ -³²P]ATP (20 µM, 10 µCi/reaction), and MgCl₂ (10 mM) were added tothe homogenate. Reactions were performed at 37°C for 10-60 minfor stoichiometric phosphorylation of MBP. Proteins were separatedby 15% SDS-PAGE, and phosphorylation was assessed by densitometricanalysis of autoradiographs. Changes in MBP phosphorylation andamount in experimental slices were normalized to control levelsmeasured in paired hippocampal slices from the same preparationand recording chamber. Control slices received three brief teststimulations to ensureviability.

Western blotting. Western blots and densitometric analyses were performed as described previously (Atkins et al., 1997). Thefollowing primary antibodies were used: total MBP [1:1000 (Chemicon,Temecula, CA) or 1:2000 (Boehringer Mannheim, Indianapolis, IN)]and total MAPK (1:1000; Upstate Biotechnology, Lake Placid, NY).To measure changes in MBP phosphorylation, phosphorylation levelswere normalized against total MBP amounts and then against totalprotein levels using p44 MAPK immunoreactivity or a Lowry assay.To measure changes in MBP amounts, immunoreactivity using a primaryantibody that detects MBP regardless of the phosphorylation stateof the protein was normalized against p44 MAPK immunoreactivityor a Lowryassay.

Materials. Phorbol diacetate (PDA), picrotoxin, bicuculline, 5,5-dimethylpyrroline 1-oxide (DMPO), N-nitro-L-arginine (L-NOArg),and N-monomethyl-L-arginine (L-NMMA) were from Sigma (St. Louis,MO). 6-Cyano-7-nitro-quinoxaline 2,3-(1H,4H)-dione (CNQX), DL-2-amino-5-phosphonovalerate(APV), 2-hydroxysaclofen, and RS- $alpha$ -methyl-4-carboxyphenylglycine(MCPG) were from Tocris Cookston (Ballwin, MO). Tetrodotoxin (TTX)was from Research Biochemicals (Natick, MA). Superoxide dismutase(SOD) and catalase were from Calbiochem (Pasadena, CA). This preparationof catalase has been reported previously to be free from contaminatingarginase activity (Esch et al., 1998).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Antidromic stimulation of CA1 axons in the alveus

The alveus is the final output pathway in the hippocampus, an area of the brain critical for information processing (Milneret al., 1998). In these studies, we investigated neuron-glia signalingin the alveus for several reasons. First, the hippocampal slicepreparation is easily accessible for electrically triggering actionpotentials in myelinated axons (Fig. 1A). Second, this preparationis also amenable to pharmacological manipulations. Third, thealveus is the locus for MBP-containing oligodendrocytes in areaCA1 of the hippocampus (Westrum and Blackstad, 1962; Andersen,1975; Tamamaki and Nojyo, 1991). Therefore, using this preparation,we can assay for alterations in MBP as an index of intracellularchanges in oligodendrocytes that occur in response to changesin neuronal activity elicited by stimulation of CA1 pyramidalcell axons.

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Figure 1. Low- and high-frequency alvear stimulation of the hippocampus was assessed to determine the forms of neuronal activity that elicit neuron-glia signaling. A, Schematic representation of the hippocampal slice preparation used in our experiments. A stimulating electrode was placed in the alveus, and action potentials were monitored with an extracellular recording electrode placed in stratum pyramidale of the CA1 region. B, To assess whether fast synaptic transmission was blocked in all our experiments, we first recorded field EPSP (fEPSP) responses in stratum radiatum in response to Schaffer collateral-commissural pathway stimulation. The fast synaptic transmission blockers CNQX (20 µM), APV (50 µM), picrotoxin (20 µM), and bicuculline (20 µM) were applied (solid bar), and the fEPSP was monitored until it was completely abolished. Traces represent the response before (a) and after (b) drug application. C, Before all physiology experiments in the alveus, we obtained an I-O curve by measuring the peak amplitude of the population spike with increasing stimulus intensity. Representative traces at 20 (a), 40 (b), and 80 (c) µA are shown. D, To study neuron-glia communication during increased firing of CA1 neurons, we delivered HFS (arrows) to the alveus after acquiring a baseline (16 min) and monitored the population spike in stratum pyramidale of the CA1 region (n = 9) for 45 min after the final tetanus. The corresponding physiology traces before (a) and after (b) tetanization are shown in the inset. Calibration: 2 msec, 4 mV.

To isolate the effects of nonsynaptic signaling, we performed all hippocampal slice experiments in the presence of fast synaptictransmission blockers (Fig. 1B). When electrical stimulation wasdelivered to the alveus and extracellular recordings were madein stratum pyramidale of area CA1, we measured a population spikewhose amplitude correlated with stimulus intensity (Fig. 1C).Thus, stimulation of CA1 pyramidal neurons in the absence of fastsynaptic transmission produced measurable back-propagating actionpotentials (Fig. 1D).

With this preparation, we assessed activity-dependent neuron-glia signaling by assaying for changes in the oligodendrocyte-specificprotein MBP. To measure MBP phosphorylation, we used a back-phosphorylationassay with PKC. Because there are no phospho-specific antibodiesagainst PKC phosphorylation sites of MBP, we used the back-phosphorylationassay, which allows for detection of the phosphorylation stateof proteins in situ. We have identified previously the 18.5 kDaisoform of MBP by amino acid sequencing, phospho-peptide mapping,Western blotting, and immunoprecipitation (Atkins et al., 1997).The identity of MBP was confirmed for this study by phospho-peptidemapping (Fig. 2A). In initial experiments, we determined whetherwe could detect changes in MBP phosphorylation with the back-phosphorylationassay after stimulating PKC activity in hippocampal slices with10 µM PDA. PDA treatment of slices resulted in a significant decreasein [³²P]phosphate incorporation into MBP with the back-phosphorylationassay (Fig. 2B), reflecting an increase in the phosphorylationstate of MBP in situ. Thus, having identified MBP and demonstratingthat we could observe changes in MBP phosphorylation in situ withthe back-phosphorylation assay, we assayed for changes in MBPphosphorylation after alveus stimulation. We investigated theeffects of two physiology paradigms, LFS and HFS, on MBP phosphorylation.

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Figure 2. MBP phosphorylation during neuron-glia signaling in the alveus was assessed by back-phosphorylation (Atkins et al., 1997). A, MBP was identified on autoradiographs by comparing the phospho-peptide maps of MBP in the rat hippocampus (HIP) (shown in two lanes to facilitate comparison) with purified MBP (PUR) identified by amino acid sequencing (Atkins et al., 1997). Accordingly, if hippocampal slices were back-phosphorylated without the alveus, we observed a marked reduction in MBP amounts (data not shown). B, Activation of PKC by PDA applied for 5 min to hippocampal slices results in an observable increase in MBP phosphorylation in the back-phosphorylation assay. A representative autoradiograph is shown of a vehicle-treated (CTL, 0.01% DMSO) and a PDA-treated (PDA) hippocampal CA1 subregion subjected to back-phosphorylation. MBP is denoted by the arrow. In the back-phosphorylation assay, increases in phosphorylation are manifested as decreases in [³²P]phosphate incorporation. C, Densitometric analysis of autoradiographs revealed no significant change in MBP phosphorylation after delivery of LFS throughout the duration of the experiment (75 min; n = 13). However, a significant increase in MBP phosphorylation was observed 45 min after tetanization of the alveus (78 ± 5% of control; n = 14; p < 0.001; ANOVA). Similar results were also observed when the slow synaptic transmission blockers MCPG and 2-hydroxysaclofen were included to block metabotropic glutamate and GABA_B- mediated synaptic transmission (77 ± 13% of control; n = 3). There was no change in MBP amounts in HFS slices (116 ± 11% of control; n = 12) or LFS slices (113 ± 5% of control; n = 14). D, A representative autoradiograph is shown of a hippocampal slice that received HFS of the alveus (HFS) compared with a paired control slice (CTL) that were assayed by back-phosphorylation for changes in MBP phosphorylation in the CA1 subregion.

High-frequency stimulation is required for neuron-glia signaling

For experiments in which LFS was delivered to the alveus, we used either a low or high stimulus intensity to determine ifeither would elicit neuron-glia communication. The results obtainedusing these two stimulus intensities were not significantly different(data not shown) and were pooled (Fig. 2C). LFS had no effectMBP phosphorylation levels. Thus, action potential firing at lowfrequencies (i.e., 0.05 Hz) does not activate a neuron-glia signalingpathway that results in regulation of MBPphosphorylation.

In contrast, HFS elicited a significant increase in MBP phosphorylation in situ. Forty-five minutes after HFS of the alveus,there was a significant decrease in [³²P]phosphate incorporation into the 18.5 kDa isoform of MBP (Fig.2C,D). These results indicate that MBP phosphorylation levelsincrease as a result of high-frequency action potential firingin CA1neurons.

The back-phosphorylation assay allows for quantitative assessment of protein phosphorylation levels if absolute basal phosphorylationlevels of protein are known. In a separate series of studies todetermine the absolute stoichiometry of MBP phosphorylation, wefound that the basal level of MBP phosphorylation in the rat hippocampusis 36 ± 1% (n = 3) of total MBP phosphorylation sites. Therefore,the observed relative decrease in MBP back-phosphorylation inour HFS studies, which is a 22% relative decrease in phosphorylationat PKC sites, represents approximately an absolute 14% increasein phosphate incorporation into MBP in the cell. This suggeststhat PKC phosphorylation of MBP in situ increased from 36 to 50%of total phosphorylation sites as a consequence of high-frequencyneuronal firing. A selective inhibitor of PKC, chelerythrine (33µM) (Herbert et al., 1990), blocked the increase in MBP phosphorylation,indicating that PKC was the likely kinase phosphorylating MBPin situ (MBP phosphorylation, 119 ± 21% of control; n = 7; MBPamount, 94 ± 11% of control; n = 7). These results suggest thathigh-frequency action potentials in the alveus activate a neuron-gliasignaling pathway that leads to a long-lasting, significant regulationof MBPphosphorylation.

Necessity of action potentials

In the preceding experiments, we delivered all electrical stimulation directly to the alveus; thus direct stimulation of nearbyoligodendrocytes could possibly account for the regulation ofMBP phosphorylation. To eliminate this possibility, we determinedwhether action potentials in neurons are necessary for the changein MBP phosphorylation. We applied TTX to hippocampal slices andthen delivered HFS and assayed the CA1 subregions 45 min later.Voltage-gated sodium channels are not present on mature oligodendrocytes(Barres et al., 1988; Soliven et al., 1988; Sontheimer et al.,1989; Berger et al., 1991); therefore, TTX should block axonalfiring but leave direct stimulation of oligodendrocytes intact(Fig. 3A). Although there are proton-activated sodium channelson oligodendrocytes, these are insensitive to TTX and voltage(Sontheimer et al., 1989). As expected, TTX application blockedfiring of CA1 pyramidal neurons (Fig. 3A). The change in MBP phosphorylationwas also inhibited by TTX (Fig. 3B,C), demonstrating that directoligodendrocyte stimulation is not sufficient to explain the changein the phosphorylation state of MBP. Therefore, action potentialgeneration in axons is required for MBP to be modulated by high-frequencyfiring in the alveus.

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Figure 3. The increase in MBP phosphorylation requires action potentials in CA1 axons. A, When TTX (500 nM) was applied to hippocampal slices, the population spike in stratum pyramidale was completely abolished (TTX). A representative control response is shown for comparison (CTL). Calibration: 2 msec, 4 mV. B, Tetanization of the alveus in the presence of TTX abolished the increase in MBP phosphorylation as shown by the representative autoradiograph. C, This was confirmed by the corresponding densitometric analysis (HFS) (n = 7). We did not observe any changes in MBP amount with this protocol (91 ± 8% of control; n = 11). Thus, action potentials generated in CA1 axons are necessary for neuron-glia signaling.

Four MBP isoforms are regulated by neuron-glia signaling

The low molecular weight, classical MBPs exist as a family of isoforms ranging from 14 to 21.5 kDa (Monuki and Lemke, 1995).In the previous experiment, we choose to assay for the 18.5 kDaisoform because we have identified previously this protein byamino acid sequencing, phospho-peptide mapping, Western blotting,and immunoprecipitation (Fig. 2A) (Atkins et al., 1997). To determinewhether other isoforms of MBP are regulated during increased neuronalfiring, we also assayed for changes in the 14, 17, and 21.5 kDaisoforms. To identify each isoform, we compared the apparent molecularweights of the MBP isoforms on autoradiographs with Western blotsthat detected all four isoforms (Atkins et al., 1997). We foundthat all four MBP isoforms were regulated by phosphorylation asa consequence of HFS of the alveus (Fig. 4). This finding strengthensour assertion that these biochemical changes elicited by neuronalactivity are occurring in oligodendrocytes. All further experimentsentailed analysis of the 18.5 kDa isoform because we have conclusivelyidentified this protein in previous experiments (Atkins et al.,1997).

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Figure 4. Four isoforms of MBP (14, 17, 18.5, and 21.5 kDa) are regulated by phosphorylation during periods of increased activity of CA1 neurons. Each isoform was identified by comparison of Western blots with autoradiographs, with the exception of the 18.5 kDa isoform, which was identified by amino acid sequencing and phospho-peptide mapping (Atkins et al., 1997). Densitometric analysis of autoradiographs from hippocampal slices that received HFS of the alveus compared with control slices demonstrates increased phosphorylation of all four MBP isoforms (14 kDa, n = 6; p < 0.01; 17 kDa, n = 9; p < 0.001; 18.5 kDa, n = 14; p < 0.001; 21.5 kDa, n = 9; p < 0.001; ANOVA).

Identification of the transcellular messenger(s)

Several observations in the literature suggested that the signaling molecule mediating the communication between neurons andoligodendrocytes in the alveus could be a diffusible messenger,such as nitric oxide or superoxide. First, neuronal activity-dependentgeneration of reactive oxygen and nitrogen species has been observedin the hippocampus (Chetkovich et al., 1993; Bindokas et al.,1996; Bito et al., 1996). Second, nitric oxide and superoxidemodulate the induction of LTP in the CA1 region of the hippocampus,suggesting that these diffusible messengers are intercellularmessengers during periods of increased neuronal activity (Böhmeet al., 1991; O'Dell et al., 1991, 1994; Haley et al., 1992; Chetkovichet al., 1993; Williams et al., 1993; Kantor et al., 1996; Sonet al., 1996; Wilson et al., 1997; Gahtan et al., 1998; Klannet al., 1998). Third, the change in MBP phosphorylation is mediatedby PKC, and reactive oxygen species increase the activity of PKCin vitro (Gopalakrishna and Anderson, 1989; Larsson and Cerutti,1989; Palumbo et al., 1992) and during hippocampal LTP (Klannet al., 1998). As an initial test of the hypothesis that a reactiveoxygen or nitrogen species was the signal mediating neuron-gliacommunication, we applied a combination of SOD (a superoxide scavengingenzyme), catalase (a hydrogen peroxide scavenger), and L-NOArg(a nitric oxide synthase inhibitor) to hippocampal slices. Forty-fiveminutes after HFS of the alveus, the CA1 subregions were assayedfor changes in MBP phosphorylation (Fig. 5A). We found that SOD,catalase, and L-NOArg applied together blocked the increase inMBP phosphorylation and, in fact, decreased MBP phosphorylationlevels (Fig. 5B). These results demonstrate that the activity-dependentchanges in oligodendrocytes are blocked by reactive oxygen speciesscavengers and a nitric oxide synthase inhibitor. In addition,because MBP phosphorylation levels are decreased, this resultsuggests that protein phosphatase activation or protein kinaseinhibition during neuron-glia signaling is unmasked by inhibitionof these reactive oxygen and nitrogen species. Thus, the reactiveoxygen and nitrogen species superoxide, hydrogen peroxide, ornitric oxide (or all three) could be the transcellular signalbetween neurons and glial cells.

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Figure 5. Reactive oxygen species scavengers and a nitric oxide synthase inhibitor block the increase in MBP phosphorylation during neuron-glia signaling. A, Hippocampal slices were perfused with SOD (120 U/ml), catalase (260 U/ml), and L-NOArg (50 µM) in the recording saline throughout the experiment. After 16 min of baseline recording, the alveus was tetanized (arrows), and then 45 min after the final tetanus, the CA1 subregion was assayed for changes in MBP phosphorylation and amount. Inset traces were obtained before (a) and after (b) tetanization. Calibration: 2 msec, 4 mV. B, Representative autoradiograph of a control and HFS slice demonstrates an increase in [³²P]phosphate incorporation in the HFS slice, indicating decreased phosphorylation of MBP in situ. Densitometric analysis confirmed these results. There was a small but significant decrease in MBP phosphorylation when reactive oxygen species scavengers and a nitric oxide synthase inhibitor was applied to slices (n = 6; p < 0.01; Student's t test) with no change in MBP amounts (96 ± 21% of control; n = 6).

To determine which reactive oxygen or nitrogen species was necessary for neuron-glia signaling, we applied each of these scavengersand inhibitors separately to hippocampal slices and assayed forchanges in MBP phosphorylation (Fig. 6). Application of SOD orcatalase alone blocked the increase in MBP phosphorylation whereasboiled, inactivated SOD or catalase had no effect. Another superoxidescavenger, DMPO (10 mM), also blocked the increase in the phosphorylationstate of MBP (98 ± 16% of control; n = 6). The nitric oxide synthaseinhibitors L-NOArg or L-NMMA blocked the increase in MBP phosphorylationas well (Fig. 6). The inactive enantiomers of these inhibitorshad no effect. From these results, we conclude that superoxide,hydrogen peroxide, and nitric oxide each are required for neuron-gliasignaling during high-frequency action potential firing.

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Figure 6. Superoxide, hydrogen peroxide, and nitric oxide each can mediate the signal between CA1 neurons and oligodendrocytes in the alveus during periods of increased action potential firing. Application of each scavenger or inhibitor alone (solid bars) blocked the increase in MBP phosphorylation (SOD, 120 U/ml; n = 6; catalase, 260 U/ml; n = 6; L-NOArg, 50 µM; n = 9; L-NMMA, 30 µM; n = 4). However, application of the inactive forms of these inhibitors (hatched bars) did not block the increase in MBP phosphorylation after tetanization of the alveus (boiled SOD, 120 U/ml; n = 5; p < 0.001; Student's t test; boiled catalase, 260 U/ml; n = 6; p < 0.01; ANOVA; D-NOArg, 50 µM; n = 5; p < 0.001; ANOVA; D-NMMA, 30 µM; n = 6; p < 0.05; ANOVA). There was a small increase in MBP amounts in slices administered boiled catalase or D-NMMA (boiled catalase, 120 ± 6% of control; n = 6; p < 0.01; Student's t test; D-NMMA, 117 ± 6% of control; n = 6; p < 0.05; Student's t test) but not with any other drug treatment (SOD, 114 ± 19% of control; n = 6; boiled SOD, 106 ± 6% of control; n = 6; catalase, 94 ± 9% of control; n = 6; L-NOArg, 112 ± 11% of control; n = 9; D-NOArg, 117 ± 9% of control; n = 5; L-NMMA, 100 ± 9% of control; n = 4).

Given these results, we propose that the source of reactive oxygen species in axons could be nitric oxide synthase. Nitricoxide synthase produces nitric oxide, as well as superoxide ina calcium-calmodulin-dependent manner (Pou et al., 1992; Xia etal., 1996, 1998). Furthermore, the interconvertability of superoxidewith hydrogen peroxide may account for the observation that inhibitorsof either of these reactive oxygen species blocked neuron-gliasignaling (Halliwell, 1992). Nitric oxide synthase has been reportedto be found in axons (Dinerman et al., 1994; Wendland et al.,1994; De Vente et al., 1998); thus, we hypothesized that high-frequencyaction potential propagation resulted in activation of axonalnitric oxide synthase. As an initial test of this hypothesis,we determined whether extracellular calcium was necessary forneuron-glia signaling by omitting extracellular calcium from thesaline. When CA1 subregions were assayed for changes in MBP phosphorylationafter HFS of the alveus, there was no change in the phosphorylationstate of MBP (103 ± 21% of control; n = 7) or amount (93 ± 18%of control; n = 7). This result indicates that extracellular calciumis necessary for neuron-glia signaling in thealveus.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In these studies, we have discovered a signaling pathway between neurons and glial cells in the hippocampus that is activatedduring periods of increased neuronal activity. Our studies suggestthat high-frequency action potential propagation in the outputfibers of the hippocampus generates a reactive oxygen or nitrogenspecies that diffuses to the surrounding myelin sheath and activatesPKC to regulate MBP phosphorylation. The effects of high-frequencyaction potential firing are long-lasting, at least 45 min beyondthe period of increased neuronal activity. Thus, the hippocampuspossesses not only a mechanism to elicit long-lasting activity-dependentchanges in neurons by synaptic signaling (i.e., LTP), it alsopossesses a mechanism for long-lasting activity-dependent changesin glia by reactive oxygen species-mediatedsignaling.

Reactive oxygen and nitrogen species as neuron-glia messengers

Our experiments demonstrate that superoxide, hydrogen peroxide, and nitric oxide are all involved in neuron-glia communicationin the hippocampus. An interesting finding was that applicationof SOD, catalase, or DMPO blocked the changes in MBP phosphorylation.These reactive oxygen species scavengers are membrane-impermeant,suggesting that they blocked the signaling of a diffusible moleculethat traversed the extracellular space to signal from axons tooligodendrocytes. Because SOD and DMPO are extracellular scavengersof superoxide, we must hypothesize that superoxide, a negativelycharged species, diffused from axons across the extracellularspace and into the myelin sheath. Studies have found that superoxideis permeant to biological membranes (Lynch and Fridovich, 1978;Rumyantseva et al., 1979; Mao and Poznansky, 1992). Alternatively,it is possible that superoxide may have dismutated to form hydrogenperoxide (Halliwell, 1992) and traversed the membrane in thisform, or reacted with nitric oxide to form peroxynitrite, whichdecomposed to a membrane-permeant species with hydroxyl radicalcharacter (Beckman et al., 1990; Radi et al., 1991; Halliwell,1992; Huie and Padmaja, 1993). Transition metals, such as copperor iron, convert superoxide and hydrogen peroxide into the highlyreactive hydroxyl radical (Halliwell, 1992). Iron in the brainis typically bound to ferritin and transferrin and is found inhigh concentrations in oligodendrocytes (Gerber and Connor, 1989;Connor et al., 1992). Thus, once superoxide or hydrogen peroxidecross into the oligodendrocyte, they have the potential of becomingeven more reactive by conversion into the hydroxyl radical. Becausethe chemistry of these reactive oxygen species is so tightly interwoven,it is difficult to definitively identify the biochemical natureof the reactive oxygen species involved in this signalingpathway.

Reaction oxygen species generation by neuron-glia signaling

In our model, we propose that the reactive oxygen and nitrogen species are generated from axonally located nitric oxide synthase,a calcium-calmodulin-sensitive enzyme (Dinerman et al., 1994;Wendland et al., 1994; De Vente et al., 1998). Calcium can enteraxons through sodium channels or reversal of the sodium-calciumtransporter (Mullins et al., 1985; DiPolo and Beauge, 1987; Waxmanand Ritchie, 1993; Stys and Lopachin, 1998). Sodium channels arevery abundant at the node of Ranvier (~1000 µm²), and their permeability ratio of P_Ca/P_Na is between 1:10 and1:7 (Meves and Vogel, 1973; Waxman and Ritchie, 1993). The sodium-calciumexchanger removes calcium intracellularly in exchange for sodiumusing the electrochemical gradient of sodium (Mullins et al.,1985; DiPolo and Beauge, 1987; Stys and Lopachin, 1998). Whenthe sodium gradient across the membrane diminishes or reverses,the gradient can reverse, transporting calcium intracellularlyand removing sodium from the cytoplasmic space. Thus, calciumflux through either of these pathways could be involved in activatingnitric oxidesynthase.

Although nitric oxide synthase is one potential source for the generation of the reactive oxygen species in this pathway,there are several other potentially relevant sources. These includearachidonic acid metabolism, xanthine oxidase, and the mitochondrialelectron transport chain. Arachidonic acid metabolism has alreadybeen implicated in hippocampal signaling as a lipoxygenase inhibitor,nordihydroguaiaretic acid, inhibits LTP (Lynch et al., 1989; Williamsand Bliss, 1989; O'Dell et al., 1991), and arachidonic acid metabolismincreases during LTP (Lynch et al., 1989, 1991). Xanthine oxidase,another potential source of superoxide, catalyzes the conversionof xanthine to uric acid, reducing molecular oxygen, which generatessuperoxide (McCord, 1985). Xanthine oxidase can be proteolyticallygenerated by a calcium-activated protease (McCord, 1985), consistentwith the requirement for extracellular calcium. Alternatively,a rise in mitochondrial respiration may increase the leakage ofelectrons, producing superoxide (Fridovich, 1978, 1989). Interestingly,glutamate receptor agonists produce superoxide in hippocampalslices, and this increase in superoxide was visualized to be nearmitochondria (Bindokas et al., 1996). In summary, axonally locatednitric oxide synthase, arachidonic acid metabolism, proteolyticconversion of xanthine oxidase, and the mitochondrial electrontransport chain are all potential sources of reactive oxygen andnitrogen species during neuron-glia signaling. Further experimentsare required to conclusively determine the source of the reactiveoxygen species that is generated during neuron-gliasignaling.

What is the redox-sensitive protein in oligodendrocytes that results in regulation of MBP phosphorylation? One possibilityis PKC because the increase in MBP phosphorylation was blockedby chelerythrine. In support of this, reactive oxygen speciesincrease the activity of PKC in vitro (Gopalakrishna and Anderson,1989; Larsson and Cerutti, 1989; Palumbo et al., 1992) and duringhippocampal LTP (Klann et al., 1998). Interestingly, the PKC isoformsidentified in myelin, $alpha$ , $beta$ II, and $epsilon$ , have been shown to be activatedby reactive oxygen species in vitro (Knapp and Klann, 1997). Alternatively,reactive oxygen species could activate a protein upstream of PKC.Voltage-gated calcium channels are possible candidates becausethese are found in oligodendrocytes and regulated by reactiveoxygen species in a variety of cells (for review, see Verkhratskyand Kettenmann, 1996; Kourie, 1998). Thus, the reactive oxygenspecies could act by direct effects on PKC or by increasing calciumlevels to activatePKC.

Neuron-glia signaling in the CNS

Classically considered inert, glial cells are becoming increasingly appreciated as active members of the signaling systemsused in the nervous system. Neuronal activity has been found tohave a variety of effects on glial cells. In the optic nerve,repetitive axonal activity triggers calcium spikes in the surroundingglial cells (Kriegler and Chiu, 1993; Chiu and Kriegler, 1994).MBP phosphorylation has also been found to be regulated by PKCduring prolonged high-frequency action potential propagation inthe optic nerve (Murray and Steck, 1983, 1984). In hippocampalslices, low-frequency stimulation of the mossy fiber pathway orthe Schaffer collateral-commissural pathway elicits calcium oscillationsthat propagate among astrocytes (Dani et al., 1992; Porter andMcCarthy, 1996; Verkhratsky and Kettenmann, 1996). A variety ofneurotransmitters applied to oligodendrocytes increase intracellularcalcium (Takeda et al., 1995), and neuronal activity can leadto depolarization of oligodendrocytes (Orkand et al., 1966). Axon-gliacommunication is also an element of development. During myelinogenesis,myelin sheath thickness and internodal length are regulated byaxon caliber (Waxman and Black, 1995). Moreover, suppression ofinternodal sodium channels in axons requires myelin ensheathement(Salzer, 1997). Thus, the pathway delineated in these studies,neuron-glia signaling in area CA1 of the hippocampus, is one exampleof the numerous conversations between neurons and glial cellsthat begins during development and lasts through maturity of thenervoussystem.

Nonsynaptic communication is a dialogue between two cells to accomplish a physiological goal that cannot be achieved throughstandard synaptic transmission. Mature oligodendrocytes have arelative scarcity of receptors and ion channels and are not synapticallycoupled to neurons (Verkhratsky and Kettenmann, 1996). Intercellularmessengers, such as reactive oxygen and nitrogen species, providea viable alternative means of communication between neurons andoligodendrocytes for integrative cellular functioning in an efficientand effective manner. Thus, neuron-glia signaling in the hippocampusduring periods of increased neuronal activity may provide a dynamicintercellular communication network in the final output fibersof thehippocampus.

  FOOTNOTES

Received March 30, 1999; revised May 24, 1999; accepted June 9, 1999.

This work was supported by National Institutes of Health Grant MH 57014 (J.D.S.) and a Williams Stamps Farish graduate fellowship(C.M.A.). We thank J. P. Adams, A. E. Anderson, C. M. Kondratick,B. Mirnikjoo, and J. C. Selcher for critical reading of thismanuscript.
Correspondence should be addressed to J. David Sweatt, Division of Neuroscience, Baylor College of Medicine, One Baylor Plaza,Houston, TX77030.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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