NMDA Receptor and Nitric Oxide Synthase Activation Regulate Polysialylated Neural Cell Adhesion Molecule Expression in Adult Brainstem Synapses

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The Journal of Neuroscience, July 1, 2001, 21(13):4721-4730

NMDA Receptor and Nitric Oxide Synthase Activation Regulate Polysialylated Neural Cell Adhesion Molecule Expression in Adult Brainstem Synapses
Farima Bouzioukh¹^,², Fabien Tell¹, André Jean¹, and Geneviève Rougon²
¹ Laboratoire de Neurobiologie des Fonctions Végétatives, Faculté de Saint Jérôme, Centre National de la Recherche Scientifique (CNRS) Formation de Recherche en Évolution 2132-Unité Sous Contrat Institut National de la Recherche Agronomique 1147, 13397 Marseille, Cedex 20, France, and ² Laboratoire de Génétique et Physiologie du Développement, Institut de Biologie du Développement de Marseille, CNRS Unité Mixte de Recherche 6545, Parc Scientifique de Luminy, 13288 Marseille, Cedex 09, France

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Here we report that synapses in the adult dorsal vagal complex, a gateway for many primary afferent fibers, express a highlevel of the polysialylated neural cell adhesion molecule (PSA-NCAM).We show that electrical stimulation of the vagal afferents causesa rapid decrease of PSA-NCAM expression both in vivo and in acuteslices. Inhibition of NMDA receptor activity completely preventedthe decrease. Blockade of calmodulin activation, neuronal nitricoxide (NO) synthase, or soluble guanylyl cyclase and chelationof extracellular NO mimicked this inhibition. Our data providea mechanistic framework for understanding how activity-linkedstimulation of the NMDA-NO-cGMP pathway induces rapid changesin PSA-NCAM expression, which may be associated with long-termdepression.

Key words: adhesion molecules; NMDAR; NO; plasticity; dorsal vagal complex; PSA-NCAM

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The polysialylated form of the neural cell adhesion molecule (PSA-NCAM) has been implicated in many aspects of cell-cell interactions.The carbohydrate polysialic acid (PSA), which is specificallyattached to NCAM through a regulated process, can attenuate adhesionforces and modulate cell surface interactions. It thereby orchestratesdynamic changes in the shape and movements of cells and theirprocesses. A convergent set of data suggests that PSA-NCAM supportsstructural plasticity in the developing and in the adult nervoussystem (for review, see Rutishauser and Landmesser, 1996; Kissand Rougon, 1997). In the adult, PSA-NCAM expression is retainedonly in certain brain areas that undergo structural reorganizationsand synaptic plasticity, such as the hypothalamus, the olfactorybulb, and the hippocampus (Seki and Arai, 1993). In the adulthippocampus, selective removal of PSA has been associated withfunctional modifications because it totally suppresses the inductionof long-term potentiation (LTP) or long-term depression (LTD)(Muller et al., 1996). Furthermore, LTP is perturbed in mice lackingNCAM and consequently PSA (Muller et al., 1996; Cremer et al.,1998).

The dorsal vagal complex (DVC) located in the dorsal medulla comprises three structures, namely the nucleus of the solitarytract (NST), the area postrema (AP), and the dorsal motor nucleusof the vagus nerve (DMX). The DVC is a gateway for many primaryafferents from cardiovascular, respiratory, gastrointestinal,and other visceral sensory receptors (Jean, 1991; Barraco, 1994).The central control of autonomic function is far from well understood,but neuronal mechanisms for the processing and integration ofvisceral afferent signals may possess plastic properties similarto those described in the higher brain regions (Miles, 1986; Glaumand Brooks, 1996; Zhou et al., 1997). Synapses afferent to theDVC exhibit both short- and long-term plasticity. Repetitive stimulationof afferent fibers leads to short- or long-term depression ofexcitatory synapses while inhibitory inputs are potentiated (Miles,1986; Glaum and Brooks, 1996; Zhou et al., 1997). In adult animals,the DVC also expresses high levels of neuromodulin [ growth-associatedprotein-43 (GAP-43)] (Kruger et al., 1993) and PSA-NCAM (Bonfantiet al., 1992) that could subserve structural reorganizations andsynaptic plasticity in response to afferent activity. In the presentstudy, we have combined in vivo and slice work to examine howsynaptic activity modulates expression of PSA-NCAM.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In vitro experiments
Transverse brainstem slices (300 µm) from the level of the obex were prepared from 4- to 6-week-old Sprague Dawley rats, asdescribed previously (Vincent and Tell, 1997). Briefly, the animalwas craniotomized under pentobarbitone sodium anesthesia; thebrainstem and upper cervical spinal cord were removed rapidlyand glued to the cutting stage of a vibratome. Throughout thesurgical and sectioning procedure, the brainstem was immersedin chilled cutting saline saturated with carbogen (95% O₂ and5% CO₂) and contained (in mM): 60 NaCl, 3 KCl, 0.5 CaCl₂, 28 NaHCO_3,7 MgCl₂, 1.25 Na₂HPO₄, 5 D-glucose, 110 sucrose, and 0.6 L-ascorbate.After stabilization at 32°C in carbogenated artificial CSF (ACSF)[containing (in mM): 130 NaCl, 3.3 KCl, 2.45 CaCl₂, 25.6 NaHCO_3,2.4 MgCl₂, 1.25 KH₂PO₄, 10 D-glucose, 0.4 L-ascorbate, 2 pyruvate,and 3 myo-inositol], the brainstem slice was transferred to arecording chamber on a microscope stage (Axioskop; Zeiss, Oberkochen,Germany), secured with a nylon mesh, and superfused at a constantrate of 3 ml/min with carbogenated ACSF at 32°C. A bipolar electrodewas positioned under visual control onto the solitary tract (ST)for electrical stimulation. In all studies, the ST was stimulatedwith a source of constant current using pulses 500 µA intensityand 200 µsec duration. In most studies, our protocol was a trainof pulses at 30 Hz (train duration of 5 sec; train period of 10sec) for 5, 10, or 15 min. In another series, one to three high-frequencypulse trains (100 Hz) were applied to the tract. Each train wasseparated by a 5 min period. Slices were dissected 5 min afterthe end of the last train; the two halves of the DVC were separatedwith microscissors and stored in two different microtubes. Sampleswere stored at $-$ 80°C until processing for immunoblotting. Teststimuli (100 µsec) were delivered every 20 sec through bipolartungsten electrodes placed onto ST, as described previously (Zhouand Poon, 2000). Field potentials (FPs) were recorded using glassmicroelectrodes (10-20 µm tip diameter). The current intensityof test stimuli (200-300 µA) was set to produce 40-50% of themaximum evoked response. The baseline was recorded for at least10 min to ensure the stability of the response. LTD was inducedusing three high-frequency pulse trains. LTD was always attemptedin the presence of 20 µM bicuculline. At the end of experiments,tetrodotoxin (TTX) (3 µM) was routinely added into the perfusionsaline. Before the analysis, the raw FPs were corrected for bysubtracting the electrode artifacts recorded in TTX-containingsaline, as described previously (Zhou and Poon, 2000). FPs weretypically biphasic with an early and late component correspondingto the presynaptic fiber volley and excitatory postsynaptic response,respectively (Zhou and Poon, 2000). Amplitude of the early phaseand the slope of the late phase were measured as an index of thestimulus efficacy on presynaptic fibers and of the postsynapticresponses,respectively.

In vivo experiments
Rats weighing 200-300 gm were anesthetized with pentobarbitone sodium (50 mg/kg, i.p.) The trachea and the jugular vein werecannulated. One cervical vagus nerve was dissected free from thesurrounding tissues. Bipolar silver electrodes were placed onthe intact nerve, secured in the muscles, and isolated with Vaseline.Rectal temperature was maintained between 36 and 38°C. The nervewas stimulated with a repetitive train at 30 Hz (train durationof 5 sec; train period of 10 sec) for 15 min. The intensity wasset at a level such that breathing was markedly inhibited duringthe first second of stimulation. Nitroarginine (100 mg/kg in normalsaline) was injected intraperitoneally 1 hr before surgery. Ratswere injected with (+)-5-methyl-10,11-dihydro-5H-dibenzo [a,d]cyclohepten-5,10-imine maleate (MK-801) (2 mg/kg) intravascularlyin normal saline 5 min before the onset of the stimulation. Controlanimals received corresponding injections of normal saline. Animalswere decapitated at the end of the stimulation period. Brainstemslices were prepared as described above and then rapidly processedfor immunoblotting. For immunohistochemistry experiments, ratswere perfused through the heart with 4% paraformaldehyde in phosphatebuffer beforeprocessing.

Immunohistochemistry
The brains were immersed in fixative (4% paraformaldehyde in phosphate buffer; 3-5 hr; 4°C). The fixed tissues were sectionedcoronally (50 µm thickness) with a vibratome. Free-floating sectionswere permeabilized in PBS-0.3% Triton X-100 [15 min at room temperature(RT)] and then incubated (1 hr) with 5% goat serum in 0.1 M PBS,pH 7.4. Tissue sections were treated with primary antibody (overnightat 4°C). After washing, sections were incubated with biotinylatedgoat anti-mouse antibody (1:200; Jackson ImmunoResearch, WestGrove, PA), washed in PBS, and developed using the VectastainABC kit and DAB kit (Biosys Inc.). Sections were examined withan Axiophot microscope (Zeiss). Control sections treated withsecondary antibodies alone showed nostaining.
Frozen section immunohistochemistry. Fixed brains were immersed in PBS containing 30% sucrose. The brainstems were sectionedcoronally (20 µm thickness) using a cryostat. Sections were incubatedfirst with 0.01% digitonin (20 min at RT) and then (1 hr) with15% fetal calf serum in 0.1 M PBS, pH 7.4. Tissue sections weretreated with primary antibody (overnight at 4°C). After washing,sections were incubated with FITC-conjugated goat anti-mouse IgM(PSA) or Texas Red-conjugated anti-mouse IgG [GAP-43, synaptophysin,and glial fibrillary acidic protein (GFAP); 1:4000; Jackson ImmunoResearch)antibodies. In double-immunolabeling experiments, the use of onlyone primary antibody followed by the addition of both anti-mouseIgM FITC-conjugated and anti-mouse IgG Texas Red-conjugated antibodiesresulted in only singlelabeling.
Antibodies. The following antibodies were used: mouse monoclonal (IgM) anti-PSA antibody [1:2000; (Rougon et al., 1986)],mouse monoclonal (IgG) anti-GAP-43 antibody (1:20,000; Roche Products,Hertforshire, UK), mouse monoclonal (IgG) anti-synaptophysin antibody(1: 200; Roche Products), mouse monoclonal (IgG) anti-GFAP antibody(1:8,000; Sigma, St. Louis, MO), and rabbit anti-NCAM antibody[1:1000 (Rougon and Marshak, 1986)].
Quantitative analysis. PSA immunoreactivity (IR) was quantified using densitometric measurements. Image recording was performedat low magnification using a Zeiss stereomicroscope equipped witha CCD camera. All images were taken with constant field illuminationusing identical camera settings. For each region of interest,average gray levels were measured using a computer-assisted imageanalysis system (NIH Image). Confocal images were obtained byusing a Zeiss Axiovert microscope 135M with 63× oil objectiveand a Zeiss laser-scanning confocal imaging system (LSM410).

Protein gel electrophoresis and immunoblots
Brain tissues were homogenized in 2% Nonidet P-40 and 0.2 M Tris-HCl buffer, pH 8, containing protease inhibitors. The homogenateswere centrifuged at 50,000 × g (1 hr at 4°C). The supernatantswere collected, and protein concentrations were determined. Insome instances, a treatment with endoneuraminidase N purifiedin our laboratory (0.2 U/mg protein; 1.5 hr at RT) was performedon homogenates in the presence of 2% Nonidet P-40. The sampleswere mixed with SDS sample buffer, and equal amounts of proteinswere fractionated by electrophoresis in 7.5% polyacrylamide gelscontaining SDS. Each sample was run twice to verify the absenceof an internal variation in the assay. After transfer onto nitrocellulose,PSA or NCAM were revealed by incubation with anti-PSA mouse IgMmonoclonal or anti-NCAM rabbit IgG polyclonal antibodies, followedby rabbit anti-mouse IgM (only for PSA), and horseradish peroxydase-conjugatedgoat anti-rabbit IgG. IR was detected with a chemiluminescencesystem. A calibration curve was established using purified recombinantfragment constant-PSA-NCAM (data not shown). Results were quantifiedby imaging densitometry (Bio Image IQ). The minimum amount ofPSA-NCAM detectable in the assay was 5 pmol, and the minimum statisticallysignificant difference between two samples was 5%.

Drugs
Drugs added to the ACSF were as follows: D-2-amino-phosphonovalerate (APV) (50 µM); 6-cyano-7-nitroquinoxaline-2, 3-dione(CNQX) (20 µM); NMDA (50 µM); 4,4,5,5-tetramethylimidazoline-1-oxyl-3-oxide(PTIO) (3 µM); 7-nitroindazole monosodium salt (7-NI) (100 µM);N-nitro-L-arginine (NNA) (1 mM); sodium nitroprusside (SNP) (100µM); S-nitroso-N-acetylpenicillamine (SNAP) (100 µM); phenylarsineoxide (PAO) (50 µM); sucrose (0.45 M); bicuculline (25 µM); 1H-[1,2,4]oxadiazolo [4,3,-a] quinoxalin-1-one (ODQ) (10 µM); and calmidazolium(200 nM).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

PSA-NCAM and GAP-43 expression in the dorsal vagal complex

A first set of experiments was performed on tissue sections prepared from rats (Fig. 1A,B,D). Figure 1 shows strong expressionof both PSA (Fig. 1C) and GAP-43 (Fig. 1E) in the DVC, in contrastwith the neighboring areas, which were negative. At a regionallevel, staining for the two molecules appeared to be superimposed.Staining was limited to the AP, the medial part of the NST (mNST),and the DMX throughout the rostrocaudal axis. Staining was weakor virtually absent in the other brainstem regions, includingthe inferior olive, the nucleus ambiguus, and the spinal trigeminalnucleus. Interestingly, staining for GFAP was also stronger inthe DVC than in the other parts of the section (Fig. 1F).

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Figure 1. Localization of PSA in the dorsal vagal complex. A, Schematic drawing of a sagittal view of the brain showing the localization of the DVC. B, Schematic drawing of a dorsal view of the dorsal vagal complex with transverse sections of the brainstem throughout the rostrocaudal axis. The three sections identify the region of the brainstem selected for the quantitative analysis of modulation of PSA expression. C, Transverse section of rat caudal medulla showing distribution of PSA immunolabeling. D, Schematic transverse section of the brainstem at the intermediate level of the DVC. E, F, GAP-43 and GFAP labelings, respectively. G, Double-staining with anti-PSA (green) and anti-GAP-43 (red) antibodies. H, Double-staining with anti-PSA (green) and anti-synaptophysin (red) antibodies. I, Confocal observation of double staining with anti-PSA (green) and anti-GFAP (red) antibodies. lNST, Lateral NST; XII, hypoglossal nucleus; SpV, spinal trigeminal nucleus; NA, nucleus ambiguus; IO, inferior olive.

Because the punctuate PSA labeling (Fig. 1G-I) was suggestive of a synaptic or perisynaptic localization, we compared thepattern of PSA IR with that of GAP-43 (Fig. 1G) and synaptophysin(Fig. 1H), a marker for presynaptic structures. The vast majorityof PSA-positive dots were closely apposed to GAP-43- and synaptophysin-positivedots. To determine whether glial cells also expressed PSA, double-labelingexperiments were performed with anti-PSA and anti-GFAP antibodies.Cells positive for GFAP exhibited a network-like organization,whereas PSA-positive elements were punctiform, and confocal lasermicroscopy indicated little if any overlap between GFAP and PSA-NCAMstaining (Fig. 1I).

Effects of electrical stimulation on PSA-NCAM expression

In vivo experiments
In vivo experiments were performed on anesthetized adult rats. Stimulation of the cervical vagus nerve (30 Hz, 15 min) induceda substantial decrease in PSA staining in the DVC on the stimulatedside compared with that in the contralateral DVC (Fig. 2A,B).Such differences were not detected in control experiments in whichthe nerve was not stimulated. Levels of PSA IR under control orstimulated conditions were recorded and quantified in differentnuclei of the DVC (Fig. 2A,B). Vagus nerve stimulation induceda significant decrease in PSA levels in DMX and mNST of the stimulatedside compared with their contralateral counterparts, and measurementsof PSA IR revealed no significant changes in control experiments(Fig. 2B).

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Figure 2. Quantitative analysis of regulation of PSA expression. A, Enlarged section showing PSA immunoreactivity in the DVC after stimulation of the cervical vagus nerve (15 min, 30 Hz). The arrow shows the stimulated side. B, Levels of PSA IR were quantified on sections throughout the rostrocaudal axis in three selected structures: the AP, the DMX, and the mNST. The results were analyzed by calculating the ratio of the IR level recorded in the stimulated side over that of the contralateral, nonstimulated side and expressed as a percentage of increase or decrease (ipsilateral side IR/contralateral side IR). C, Example of a typical Western blot showing the expression of PSA in control and in stimulated adult rat in the DVC and in the hypoglossal nucleus (XII). D, Example of a Western blot revealed with anti-PSA (lanes 1-4) and anti-NCAM (lanes 5-8) antibodies in stimulated adult rat. The homogenates were incubated with endoneuraminidase N (Endo N; lanes 3, 4, 7, 8) to remove PSA and visualize NCAM proteins (lanes 7, 8). E, Quantification of PSA IR (black bars) and NCAM IR (white bar; n = 15) on Western blots after electrical stimulation of the vagus nerve. Rats were stimulated (15 min, 30 Hz) and killed just after the end of the stimulation (t = 0; n = 21), 5 hr (t = 5 hr; n = 5), or 24 hr later (t = 24 hr; n = 8). Mean ± SEM of the data. *p < 0.05; Wilcoxon test; stimulated versus contralateral side for each time considered; ns, not significant. **p < 0.05; ANOVA; stimulated side at the end of stimulation (15 min, 30 Hz) versus stimulated side 5 and 24 hr after stimulation. ip, Ipsilateral side to the stimulation; ct, contralateral side to the stimulation.

The decrease in PSA staining after electrical stimulation of the vagus nerve could result from either a rapid degradationof the molecule or a change of its subcellular localization, whichmight modify the access of the epitope to the antibody. To discriminatebetween these two hypotheses, we measured the amount of PSA IRin detergent-solubilized tissue samples. To this end, the DVCwas dissected from brainstem slices, at the end of the in vivostimulation session, and each half was separately collected. IndividualDVC halves were then processed for immunoblotting under strictlythe same conditions. First, we examined PSA and NCAM IR partitioningin the detergent-soluble (supernatant) and detergent-insoluble(pellet) fractions. Virtually all (>95%) of the IR was recoveredin the supernatant fraction. We also verified that stimulationdid not influence the relative distribution of PSA IR betweenthe two fractions (data not shown). Therefore, for all experiments,data shown are those for the soluble fractions (Fig. 2C-E). Asexpected, anti-PSA and anti-NCAM antibodies revealed a broad bandmigrating above 180 kDa. Removal of PSA using endoneuraminidaseN (Fig. 2D) showed that PSA was mainly linked to the 180 kDa NCAMisoform. Under both stimulation and control conditions, PSA andNCAM IR were always detected in both halves of the DVC, in contrastwith neighboring areas, which were negative for PSA (Fig. 2C)but positive for NCAM (data not shown). We then compared the quantityof PSA IR in both DVCs. In control experiments, when the vaguswas not stimulated, PSA IR levels did not differ between the DVCs.In contrast, vagus nerve stimulation (30 Hz, 15 min) induced astrong decrease in the PSA (~32%) and NCAM-180 (~25%) contentsof the ipsilateral DVC compared with the DVC on the nonstimulatedside (Fig. 2C-E). These data indicate that vagus nerve stimulationresulted in a rapid decrease in the amount of the 180 kDa PSA-NCAMisoform in the DVC. These low PSA levels persisted for at least5 hr and then recovered gradually (Fig. 2E).

In vitro experiments
To determine the molecular mechanisms controlling this rapid modulation of PSA expression, our experimental protocols wereadapted for an in vitro preparation. Fresh brainstem slices werekept in a standard perfusion chamber, and fibers afferent to DVCwere stimulated with a bipolar electrode placed on the ST (Fig.3A). Changes in PSA expression, detected on immunoblots, wereexpressed as the ratio of ipsilateral/contralateral IR. Controlswere performed as for the in vivo experiments (see above).

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Figure 3. Effects of electrical stimulation of the solitary tract on PSA expression in slices. A, Schematic representation of transverse section of brainstem at the level of the AP. The box shows the medial NST and the arrangement of the stimulating electrode. B, Typical Western blot showing PSA IR decrease in the ipsilateral side to the stimulation. This decrease was a function of time after the stimulation. C, Quantification of PSA on Western blots after electrical stimulation at 30 Hz during 5 (n = 5), 10 (n = 5), or 15 (n = 36) min (left to right). Mean ± SEM of the data. No statistical significant difference in PSA IRs between the two sides of the DVC was observed for the sham (n = 7). *p < 0.05; Wilcoxon test; stimulated side versus contralateral side for a given experimental condition. **p < 0.05; ANOVA; sham versus stimulated sides for 5, 10, and 15 min of stimulation. D, Quantification of PSA IR on Western blots after electrical stimulation of the ST with one (n = 6), two (n = 6), or three (n = 20) high-frequency (100 Hz) short-duration (1 sec) stimulation trains applied every 5 min. Mean ± SEM of the data. *p < 0.05; Wilcoxon test; stimulated side versus contralateral side for a given condition. **p < 0.05; ANOVA; sham versus stimulated sides for one, two, and three stimulation trains.

We verified that mechanical stress from the stimulation electrode did not influence PSA IR levels by showing that placingthe electrode onto the ST of one hemi-slice for 15 min withoutstimulation caused no differences between the two sides (Fig.3B,C).
ST stimulation (30 Hz for 15 min) in vitro as in vivo induced a decrease in PSA expression (Fig. 3B). The clear downregulationof PSA IR in the ipsilateral side in 31 of 36 slices tested averaged23% when ipsilateral and contralateral sides were compared 15min after the end of the stimulation (Fig. 3B,C). We then investigatedthe effects of stimulation duration. For 30 Hz stimulation, PSAIR decreased as a function of time. The decrease reached 15% after5 min and 20% after 10 min of stimulation (Fig. 3B,C). A singlehigh-frequency (100 Hz) short-duration (1 sec) stimulation trainalso induced a significant decrease in PSA IR as soon as 5 minafter the end of the stimulation (Fig. 3D). A greater reductionwas induced by additional second or third trains applied 5 and10 min, respectively, after the first. Thus, the decrease in PSAIR occurs rapidly (<5 min) and is sensitive to the number andduration of the stimulationtrains.

Activation of NMDA receptors is a prerequisite to PSA decrease

Peripheral information conveyed by vagal afferent fibers activates predominantly glutamate receptors (Saha et al., 1995; Schaffaret al., 1997). Using a pharmacological approach, we investigatedthe role of glutamate receptor subtypes in the regulation of PSAexpression on brainstem slices. All drugs were tested using the15 min duration, 30 Hz frequency stimulation paradigm. Figure4A shows that coapplication in normal saline of CNQX, an AMPAreceptor antagonist, and APV, an NMDA receptor (NMDAR) antagonist,inhibited the stimulation-induced PSA IR decrease; the IR ratiofrom the two DVCs was similar to that of unstimulated controls.When used separately in normal saline, the drugs yielded similarresults. However, in a magnesium-free medium, which removes themagnesium blockade of NMDA receptors at resting potential (Nowaket al., 1984), ST stimulation induced a reduction in PSA IR thatwas insensitive to CNQX but sensitive to APV. In normal saline,blockade of NMDA receptors by APV also blocked the decrease inPSA IR induced by three trains of stimulation at high frequency(Fig. 4A).

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Figure 4. Regulation of PSA expression requires NMDA receptors. A, Glutamate receptor antagonists affect the percentage decrease of PSA IR after 30 Hz stimulation (15 min) or a high-frequency stimulation (100 Hz, 1 sec, 5 min). Preincubation of slices with both CNQX (20 µM, 10 min) and APV (50 µM, 10 min) together (n = 10) or separately (n = 10) inhibits the decrease in PSA IR. ST stimulation of slices perfused with CNQX (n = 5) in a magnesium-free ACSF (60 min), which removes the magnesium blockade of NMDA receptors, still induces a reduction of PSA IR but not in the presence of APV (n = 5). Bath application of NMDA (50 µM, 7.5 min) (n = 8) results in a similar PSA IR downregulation. Mean ± SEM of the data. *p < 0.05; Wilcoxon test; stimulated side versus contralateral side for a given condition. **p < 0.05; ANOVA; stimulated side (30 Hz, 15 min) versus stimulated and treated sides according to described experimental conditions. B, Addition of bicuculline (25 µM, 10 min; n = 4) does not prevent the effects of ST stimulation. High-K⁺ ACSF (30 mM, 7.5 min; n = 10) results in a decrease of PSA IR that is sensitive to APV (n = 6). Mean ± SEM of the data. *p < 0.05; Wilcoxon test; stimulated side versus contralateral side for a given condition. **p < 0.05; ANOVA; stimulated side (30 Hz, 15 min) versus stimulated and treated sides according to described experimental conditions.

The involvement of NMDA receptors in the reduction of PSA expression was further confirmed by direct NMDA receptor stimulation.Medullary slices were cut into two halves along the midline. Onehalf was perfused with ACSF containing NMDA and the other withnormal saline. The PSA IR of the half superfused with NMDA wasalways lower than that in the control hemi-slice (Fig. 4A). Insimilar experiments raising K⁺ concentration to 30 mM in the ACSF for 7.5 min also downregulatedPSA IR. This effect completely vanished when APV was added tothe high-K⁺ saline (Fig. 4B). The effect of ST stimulation on PSA (Fig. 4B)was not abolished by addition of bicuculline to the perfusingsaline, suggesting that GABA_A receptors do not contribute to PSAregulation.

Nitric oxide-cGMP pathway regulates the expression of PSA-NCAM

Activation of NMDA receptors may cause nitric oxide (NO) release and cGMP formation (East and Garthwaite, 1991). We thereforetested whether the PSA IR decrease induced by ST stimulation wasdependent on the activation of the NO pathway. All drugs weretested as previously with stimuli at 30 Hz applied for 15 min.In a first series of experiments, we used NNA, an inhibitor ofboth neuronal NO synthase (nNOS) and endothelial NOS. Incubationof the slices in the presence of NNA prevented the stimulation-induceddecrease in PSA IR (Fig. 5A,B). A similar result was obtainedwith 7-NI. To further confirm the role of NO in the reductionof PSA IR, we checked on halves separated from their control counterpartswhether NO donors mimicked ST stimulation. As shown in Figure5B, bath application of SNP or SNAP for 7.5 min reproduced thedecrease in PSA IR seen after ST stimulation.

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Figure 5. The nitric oxide-cGMP pathway regulates PSA expression. A, Typical Western blots probed with anti-PSA antibody. B, Preincubation of slices with NNA (1 mM, 60 min; n = 6) or 7-NI (100 µM, 10 min; n = 6), two inhibitors of NOS, prevents stimulation-induced PSA IR decrease. Application of the two NO donors SNP (100 µM, 7.5 min; n = 9) and SNAP (100 µM, 7.5 min; n = 6) mimics the PSA IR decrease observed after ST stimulation. Mean ± SEM of the data. *p < 0.05; Wilcoxon test; stimulated side versus contralateral side for a given condition. **p < 0.05; ANOVA; stimulated side (30 Hz, 15 min) versus treated and stimulated sides according to described experimental conditions. C, Typical Western blot probed with anti-PSA antibody. D, Blockade of calmodulin with calmidazolium (200 nM, 20 min; n = 8) or soluble guanylyl cyclase with ODQ (10 µM, 60 min; n = 6) inhibits the stimulation-induced PSA IR decrease. Chelation of diffusible NO with PTIO (3 µM, 5 min) results in an increase in PSA IR after ST (n = 9) or NMDA (n = 5) stimulation. Mean ± SEM of the data. *p < 0.05; Wilcoxon test; stimulated side versus contralateral side for a given condition. **p < 0.05; ANOVA; stimulated side (30 Hz, 15 min) versus stimulated and treated sides according to described experimental conditions. E, Typical Western blot probed with anti-PSA antibody. F, Incubation of slices with PAO (50 µM, 10 min; n = 6) or sucrose (0.45 M, 20 min; n = 6) reduces PSA IR decrease after stimulation with the NO donor SNAP. Mean ± SEM of the data. *p < 0.05; Wilcoxon test; side treated with NO donor versus contralateral side for a given condition. **p < 0.05; ANOVA; NO donor-stimulated side versus corresponding sides treated according to described experimental conditions.

In NOS-containing neurons, glutamate-induced elevations of Ca²⁺ activate calmodulin and induce NO production by activating NOS(Snyder, 1992). Blockade of calmodulin by perfusion of sliceswith calmidazolium prevented the decrease in PSA IR induced byST stimulation (Fig. 5C,D). NOS activation induces cGMP productionin the hippocampus (East and Garthwaite, 1991). Thus, we askedwhether production of cGMP via activation of soluble guanylylcyclase was involved in the pathway regulating PSA expression.Bath application of ODQ, a potent and selective inhibitor of thisenzyme (Garthwaite et al., 1995), suppressed the effects of STstimulation (Fig. 5C,D).

Because NO can act as a transcellular messenger, we chelated extracellular NO using PTIO (Fig. 5C,D) or carboxy-PTIO (datanot shown), two membrane-impermeable NO scavengers (Ko and Kelly,1999), to test whether NO diffusion was involved. We verifiedthat, in the absence of stimulation, the PSA IR of PTIO-treatedand untreated separated halves was not statistically different(data not shown). In the presence of the NO scavengers, the STstimulation resulted in an increase in PSA IR. Furthermore, inall experiments, NO chelation caused instead an increase of PSAIR on the stimulated side (Fig. 5C,D). This result suggests thatdiffusible and intracellular NO may have opposing influences onthe changes on PSA expression induced by ST stimulation. To furtherascertain that NMDA receptor activation occurred upstream of NOSactivation in the pathway, we tested the effects of NMDA additionin the presence of PTIO. For these experiments, DVCs were separatedin two halves, one side being used as control. Here again, PSA-NCAMexpression was upregulated in the NMDA-PTIO-treated half comparedwith the control hemi-slice (Fig. 5C,D).

This decrease in PSA IR is rapid and probably involves synaptic endocytosis of PSA, followed by its degradation. PAO and sucrose,two reagents reported to interfere with mechanisms involved inclathrin-dependent endocytosis (Frost and Lane, 1985; Heuser andAnderson, 1989), strongly reduced the decrease in PSA IR resultingfrom stimulation with the NO donor SNAP (Fig. 5E,F).

The stimulation-induced PSA IR decrease is associated with NMDAR-dependent LTD

To search for a possible link between the modulation of PSA expression by stimulation and plasticity occurring in the DVC,we recorded extracellular FPs in adult rat brainstem slices withinthe mNST. We showed (Fig. 6A,B) that a 100 Hz stimulation, whichinduced a PSA IR decrease, also induced LTD. The slope of fieldpotentials was maximally reduced within 20 min after stimulationand remained depressed for the duration of the experiment. The100 Hz stimulation did not change the amplitude of the presynapticvolley recorded extracellularly (100 ± 1% of control value; n= 6), indicating that the stimulation excites the same numberof fibers during the experiment (Fig. 6C). Twenty minutes afterthe 100 Hz stimulation, the average depression was 28 ± 3% (n= 8; p < 0.001; Mann-Whitney U test). We further demonstratedthat NMDAR activation was required during the induction by applyingthe NMDAR antagonist APV. Loading slices with APV blocked theability to induce LTD (9 ± 5%; n = 5) (Fig. 6A) and in additionrevealed a nonsignificant increase in the response. Therefore,NMDARs are likely to be involved in both triggering this formof synaptic plasticity and regulating PSA-NCAM expression, suggestinga link between LTD and PSA-NCAM endocytosis.

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Figure 6. NMDAR-dependent LTD. A, Time course of changes in FP slope after 100 Hz stimulation. LTD is induced by 100 Hz stimulation (; n = 8), and 50 µM APV blocks LTD ( $open circle$ ; n = 5). The arrow indicates the time of stimulation. FPs are normalized to baseline set at 100% ± SEM. B, No presynaptic changes could be detected. The amplitude of the presynaptic volley remained stable for the duration of the experiment.

The NMDA-NO pathway regulates PSA-NCAM expression in vivo

We confirmed the physiological relevance of the activation of the NMDA-NO pathway after ST stimulation by showing that itwas also functional in vivo. Cervical vagus nerve stimulationin anesthetized rats induced an ipsilateral reduction in PSA IR(Fig. 2). When the rats received systemic injections of MK-801to block NMDA receptors or intraperitoneal injections of NNA toinhibit NOS activity, the stimulation-induced PSA IR decreasewas significantly lower than it was in untreated animals (Fig.7A,B).

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Figure 7. The NMDA-NO pathway regulates PSA expression in vivo. A, Typical Western blot. B, In anesthetized rats, systemic injection of MK-801 (2 mg/kg, 5 min before stimulation; n = 9) or intraperitoneal injections of NNA (100 mg/kg, 60 min before stimulation; n = 8) reduces the stimulation-induced PSA IR decrease. Mean ± SEM of the data. *p < 0.05; Wilcoxon test; stimulated versus contralateral side for a given condition. **p < 0.05; ANOVA; stimulated side at the end of stimulation (15 min, 30 Hz) from control rats versus corresponding stimulated sides from treated rats.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The first finding of this study is that the expression of PSA-NCAM within the DVC of adult rats is dynamic and controlledby synaptic activity. Our study extends a previous report (Bonfantiet al., 1992) on mapping of PSA expression in adult rats by demonstratinga precise regional and cellular localization. Interestingly, PSA-NCAMexpression is not observed in all NST subregions but only in themedial part of the NST, which is implicated in the regulationof visceral function. We show that, in the DVC, PSA is mainlyassociated with the NCAM 180 kDa isoform, which is often expressedin postsynaptic membranes (Persohn et al., 1989; Persohn and Schachner,1990). In agreement, PSA labeling was punctuate and closely apposedto synaptophysin- or GAP-43-immunoreactive dots. However, thisanalysis did not allow us to determine the precise localizationof PSA within the synapse. In the DVC, PSA did not colocalizewith the astrocyte marker GFAP. This contrasts with its expressionin axons and glia of the adult hypothalamo-hypophyseal system,a structure that undergoes profound structural remodeling afterphysiological stimulation (Theodosis et al., 1991). The PSA expressionpattern in the DVC is reminiscent of that reported in the striatumand hippocampus. In the adult striatum, electron microscopy showedthat PSA expression is confined to presynaptic and postsynapticsites (Uryu et al., 1999). In the hippocampus, PSA-positive smallboutons were found to make synaptic contacts with PSA-positivedendrite outgrowths (Seki and Arai, 1999). Such a localizationstrongly suggests that, in the DVC, PSA could contribute to structuralremodeling ofsynapses.

Activity-dependent regulation of adhesion molecules has been reported previously in several systems (Fields and Itoh, 1996).The anatomy of the DVC, which allowed both access to slice preparationsand the comparison of PSA IR levels in treated and control hemi-slices,was particularly suitable for experiments on the regulation ofPSA expression. We provide here the first evidence for a rapiddownregulation of PSA-NCAM levels induced by synaptic activation.Although in vivo stimulation probably activated both afferentand efferent fibers of the vagus nerve, it is unlikely that thedecrease in PSA resulted from an antidromic activation of dorsalmotor vagal neurons. Immunohistological observations showed thatPSA IR was decreased throughout the DVC. In addition, in vitrostimulations of the ST (which contains only afferent fibers) gavesimilar results, and our pharmacological data strongly suggestthat synaptic activation was crucial to induce changes in PSAexpression. The modulation of PSA expression in the NST likelydepends on ST stimulation, and those observed in the DMX may beattributable to the activation of local circuit interneurons andcollaterals of second-order NST neurons, which establish localreflex arc with the DMX (Whitehead, 1988). Indeed, visceral afferentinputs have their first synaptic relay in the NST. There is someevidence that the first-order afferents make some monosynapticcontacts on the dorsally directed dendrites of the DMX (Rinamanet al., 1989).

Our evidence suggests that changes in PSA expression (1) resulted from increases in intracellular Ca²⁺, (2) required activation of NMDA receptors, and (3) involvedthe NO-cGMP signaling pathway. Downregulation of PSA was morepronounced when the duration of the 30 Hz stimulation or the numberof high-frequency trains were increased. A 100 Hz frequency stimulationfor 1 sec was as efficient as 30 Hz frequency stimulation for5 min. High-frequency stimulation is likely to cause a rapid depolarizationof the postsynaptic membrane, allowing a brief but intense Ca²⁺influx.

The vast majority of vagus nerve sensory afferents liberate glutamate (Sykes et al., 1997). Accordingly, we observed thatblockade of glutamate but not GABA receptors prevented the stimulation-inducedPSA IR decrease. The effects of glutamate may depend on actionsat different ionotropic receptors. Ionotropic receptor subtypeshave been described within the DVC and can be activated by STstimulation on brainstem slices (Tell and Jean, 1991; Travagliet al., 1991; Yen et al., 1999). In our model, activation of NMDAreceptors is required to produce the observed PSA IR decrease.Finally, exogenous application of NMDA resulted in a decreasein PSA IR. Under physiological conditions, extracellular Mg²⁺ blocks the NMDA receptor channel at the resting membrane potential.High-frequency stimulation of presynaptic fibers should activatenon-NMDA receptor channels sufficiently to depolarize the postsynapticcell, remove the Mg²⁺ blockade, and permit Ca²⁺ entry via NMDA receptor channels (Nowak et al., 1984). Experimentswith a high-K⁺ saline further confirm the pivotal role of NMDA receptors. Inthis protocol, the decrease in PSA IR was entirely suppressedby APV, suggesting a negligible role in this effect for Ca²⁺ influx through voltage-dependent Ca²⁺channels.

We examined the possible involvement of NO and cGMP, one of several signaling pathways that might be activated by a postsynapticrise in Ca²⁺. Activation of NMDA receptors causes NO release in the cerebellarcortex and formation of cGMP through activation of NOS in hippocampus(East and Garthwaite, 1991). NOS is present in presynaptic andpostsynaptic sites and cell bodies within the DVC of adult rats(Krowicki et al., 1997; Lin et al., 1998). In addition, NMDA-induceddepolarization on DVC neurons is partly mediated by the activationof the NO-cGMP pathway (Travagli and Gillis, 1994). Our data clearlyindicate that the decrease in PSA IR by afferent stimulation involvesNO production and cGMP synthesis. Alteration of PSA expressionwas reproduced by directly adding NO donors into the perfusionmedium. Interfering with NO production by blocking NOS activitywith NNA and 7-NI prevented changes in PSA IR. Activation of nNOSrequires activation of calmodulin by Ca²⁺ (Moore and Handy, 1997). Accordingly, inhibition of calmodulinsuppressed the effects induced by ST stimulation. Finally, blockadeof the soluble form of guanylyl cyclase by ODQ also suppressedthe decrease in PSA IR. These conclusions are not limited to theslice preparation, because we confirmed in vivo that blockadeof NMDA receptors by MK-801 and interfering with NO productionwith NNA prevented the decrease in PSAIR.

Interestingly, scavenging diffusible NO by PTIO or carboxy-PTIO had an effect opposite to afferent stimulation or to NMDAapplication on PSA IR, whereas blocking NO synthesis simply preventedits occurrence. In the DVC, NO may act primarily as a transcellularmessenger, inducing a strong endocytosis of PSA through productionof cGMP. The increase in PSA IR upon extracellular applicationof NO scavengers may result from the postsynaptic action of NOand cGMP. Indeed, we observed that NOS or guanylyl cyclase inhibitionprevented changes in PSA expression. A recent study on hippocampalsynaptic transmission demonstrated that NO may serve as both aretrograde messenger and a postsynaptic intracellular signalingmolecule (Ko and Kelly, 1999). However, our results also suggestthat another mechanism not involving NO could participate in theregulation of PSA expression after STstimulation.

PSA expression can be controlled at both transcriptional and post-transcriptional levels (Bruses et al., 1995; Bruses andRutishauser, 1998), and differential regulation of PSA expressionby activity is not unprecedented. During development, activityincreases PSA expression in muscle but decreases it in nerve (Rutishauserand Landmesser, 1996). In addition, PSA can be externalized onthe cell surface by differential delivery of intracellular storesin response to changes in intracellular Ca²⁺. Indeed, Ca²⁺ influx induces PSA-NCAM exocytosis in pancreatic cells (Kisset al., 1994), whereas intracellular Ca²⁺ rise triggered by NMDA receptor activation have similar effectsin oligodendrocyte precursors (Wang et al., 1996). Exocytosisand endocytosis are two complementary mechanisms suited to performregulations in defined, restricted areas, such as synaptic sites.Here, we provide the first evidence for a rapid downregulationof PSA at central synapses. Both the kinetics of the changes inexpression and their sensitivity to endocytosis blockers stronglysupport an involvement of PSA-NCAM endocytosis and rapid degradationof PSA. Our experimental conditions produced a strong and globaldecrease in PSA IR, which might obscure more subtle variationsoccurring at the synaptic level. Nevertheless, we have providedevidence that PSA expression in the DVC is synaptically regulatedand that this event might be linked toLTD.

This rapid modulation of adhesion molecule expression at the cell surface is reminiscent of that reported for the NCAM homolog(apCAM) in Aplysia, fasciclin II in Drosophila (Schuster et al.,1996), and the mammalian neural cell adhesion molecule L1 (Kamiguchiet al., 1998).

PSA-NCAM, as well as NO, has an important role in synaptic plasticity in the mature brain. NO is required for the NMDA-dependentform of synaptic plasticity in different brain regions (Lev-Ramet al., 1997; Calabresi et al., 1999). Removal of PSA from NCAMimpairs long-term changes in synaptic efficacy in hippocampalorganotypic slice cultures (Muller et al., 1996). Similar resultswere obtained by using antibodies raised against NCAM on acutehippocampal slices (Luthl et al., 1994). Our study has identifieda functional link between NO production and PSA-NCAM regulation,integrating several observations on the involvement of NO andPSA-NCAM in synaptic plasticity. In Aplysia, serotonin-inducedretrieval of apCAM from the presynaptic membrane, which shouldpromote a less adhesive environment, is linked to LTP and synaptogenesis(Bailey et al., 1992; Mayford et al., 1992). If PSA has an anti-adhesivefunction (Rutishauser and Landmesser, 1996), then in our modelit might facilitate morphological changes, whereas its endocytosisshould increase adhesion and stabilize the synapses. Several experimentshave failed to demonstrate LTP at excitatory synapses within theDVC (Glaum and Brooks, 1996). Recently , Zhou et al. (1997) presentedinstead direct evidence for LTD in 3- to 21-d-old NST neurons,dependent on activation of NMDA receptors, and a rise in intracellularCa²⁺. Here, we also observed an NMDAR-dependent synaptic plasticityin the adult NST neurons with the same stimulation as the oneused to induce a decrease in PSA-NCAM expression. Although otherexperiments are needed to demonstrate it, these results suggestthat these two events may belinked.

In conclusion, our data provide strong evidence for a rapid modulation of PSA by synaptic activation in a mammalian model.The dynamic of PSA expression suggests that it plays a finelytuned role in the integration of afferent information within theDVC and so participates in the cellular mechanisms by which thisstructure contributes to the homeostatic regulation of visceralfunction.

  FOOTNOTES

Received Jan. 24, 2001; revised March 26, 2001; accepted April 6, 2001.

This work was supported by institutional grants from CNRS to A.J. and G.R. and by European Community Quality of Life GrantEC QLRT 99-02187 to G.R. F.B. was supported by a student fellowshipfrom Direction Générale des Armées.
Correspondence should be addressed to Geneviève Rougon, Laboratoire de Génétique et Physiologie du Développement, Institutde Biologie du Développement de Marseille, Centre National dela Recherche Scientifique Unité Mixte de Recherche 6545, ParcScientifique de Luminy, 13288 Marseille, Cedex 09, France. E-mail:rougon{at}ibdm.univ-mrs.fr

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