Cell Surface Expression of Polysialic Acid on NCAM Is a Prerequisite for Activity-Dependent Morphological Neuronal and Glial Plasticity

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The Journal of Neuroscience, December 1, 1999, 19(23):10228-10236

Cell Surface Expression of Polysialic Acid on NCAM Is a Prerequisite for Activity-Dependent Morphological Neuronal and Glial Plasticity
Dionysia T. Theodosis¹, Renée Bonhomme¹, Sergio Vitiello¹, Geneviève Rougon², and Dominique A. Poulain¹
¹ Institut National de la Santé et de la Recherche Médicale U378, Institut François Magendie Université Victor Segalen Bordeaux II, F33077 Bordeaux, France, and ² Centre National de la Recherche Scientifique, Unité Mixte de Recherche 6545, Parc Scientifique de Luminy, F13288 Marseille, France

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Polysialic acid (PSA) on the extracellular domain of the neural cell adhesion molecule (NCAM) reduces cell adhesion and isconsidered an important regulator of cell surface interactions.The hypothalamo-neurohypophysial system (HNS), whose glia, neurons,and synapses undergo striking, reversible morphological changesin response to physiological stimulation, expresses high levelsof PSA-NCAM throughout life. Light and electron microscopic immunocytochemistryin normal rats and rats in which cell transport was blocked withcolchicine showed that PSA-NCAM is expressed in both HNS neuronsand glia, particularly at the level of astrocytic processes thatenvelop neuronal profiles and can undergo remodeling. Moreover,we confirmed that the overall levels of PSA-NCAM were not greatlyaltered by stimulation (lactation and chronic salt ingestion).Nevertheless, PSA is essential to morphological plasticity. Usingcomparative ultrastructural analysis, we found that, after specificenzymatic removal of PSA from NCAM by microinjection of endoneuraminidaseclose to the hypothalamic magnocellular nuclei in vivo, therewas no apparent withdrawal of astrocytic processes nor any increasein synaptic contacts normally induced by lactation and dehydration.Our observations demonstrate, therefore, that expression of PSAon cell surfaces in the adult HNS is indispensable to its capacityfor activity-dependent morphological neuronal-glial and synapticplasticity. The carbohydrate PSA on NCAM can thus be considereda necessary permissive factor to allow neuronal and glial remodelingto occur whenever the proper inductive stimulusintervenes.

Key words: NCAM; neuronal-glial interactions; astrocytes; synaptic plasticity; hypothalamo-neurohypophysial system; lactation; osmotic stimulation

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The neural cell adhesion molecule (NCAM) is represented by several isoforms that differ in their protein backbone, mode ofattachment to the plasma membrane, and content of $alpha$ -2,8-linkedsialic acid residues [polysialic acid (PSA)] on their extracellulardomain. PSA constitutes up to 30% of the highly sialylated NCAMisoforms, designated as PSA-NCAM. Because of its negative chargeand large hydrated volume, PSA on NCAM attenuates cell adhesionand has become an attractive molecular candidate to intervenein dynamic cellular changes (for review, see Rougon, 1993; Fryerand Hockfield, 1996; Rutishauser and Landmesser, 1996). For example,PSA on cell surfaces would permit cells to detach from their neighbors,thereby allowing them to undergo changes in conformation relatedto motility or morphological remodeling. Much evidence supportssuch a function in the developing CNS in which PSA-NCAM has beenshown to intervene in cell migration, neurite outgrowth, and axonalfasciculation (for review, see Rutishauser and Landmesser, 1996;Yoshida et al., 1999). PSA-NCAM disappears from most of the CNSafter birth, but its continued expression in neuronal systemscapable of plasticity (Bonfanti et al., 1992) strongly suggestsa similar role in the adult. Nevertheless, most available dataare correlative, and evidence of an actual participation is scarce.Recently, electrophysiological recordings in hippocampal slicesfrom NCAM- or PSA-deficient mice revealed that the glycoproteindoes take an active part in physiological synaptic plasticity(long-term potentiation) (Muller et al., 1996; Cremer et al.,1998). On the other hand, the abnormally small olfactory bulbin NCAM-deficient mice (Cremer et al., 1994; Ono et al., 1994)has indicated that it intervenes in neurohistogenesis and migrationof PSA-NCAM-immunoreactive olfactory bulb precursors, which dividein the subventricular zone and migrate to the olfactory bulb (Bonfantiand Theodosis, 1994; Rousselot et al., 1995).

PSA-NCAM has also been implicated in synaptogenesis, but there have been no ultrastructural observations or quantitative analysesto define precisely its contribution to such structural plasticity(Rutishauser and Landmesser, 1996). A neuronal system that appearsas a good model to address this question is the hypothalamo-neurohypophysialsystem (HNS) because it expresses high levels of PSA-NCAM throughoutlife (Theodosis et al., 1991; Bonfanti et al., 1992; Kiss et al.,1993; Nothias et al., 1997) and undergoes extensive morphologicalsynaptic plasticity in response to physiological stimulation (forreview, see Theodosis and Poulain, 1993; Hatton, 1997; Theodosiset al., 1998). HNS neurons, which secrete the neurohormones oxytocinor vasopressin, are grouped in well delineated areas of the hypothalamus,the supraoptic (SON) and paraventricular (PVN) nuclei; their axonsproject to the neurohypophysis. During lactation and chronic osmoticstimulation, there is a significant reduction in glial coverageof neuronal surfaces, and they are left directly juxtaposed andcontacted by an increased number of synapses. The changes arereversible with cessation of stimulation (Theodosis and Poulain,1993; Hatton, 1997; Theodosis et al., 1998).

In the present study, therefore, we first used light and electron microscopic immunocytochemistry to visualize PSA-NCAM inthe rat HNS under basal and stimulated conditions of HNS secretion.To determine its cellular source more precisely, we also examinedthe SON of rats in which cell transport was inhibited with colchicine.We then used enzymatic removal of PSA with endoneuraminidase (endoN) (Finne and Mäkelä, 1985; Rutishauser et al., 1985) from cellsurfaces in the SON of normal and stimulated rats in vivo to seewhether PSA participates in the morphological changes. Becausethere are two bilateral SON in the hypothalamus, we were ableto microinject endo N into one SON while keeping the other intact.This approach, coupled with comparative ultrastructural analysis,thus permitted us to monitor activity-dependent plasticity notonly between groups but between two nuclei in the same animal.Finally, bilateral injections of the enzyme into two SON in lactatingrats allowed us to address the question of the consequences ofthe morphological changes to HNSfunction.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Male and female Wistar rats, at least 3 months of age and raised under controlled temperature and light conditions, were used.They were divided into the following groups according to theircondition of HNS secretion: (1) normally hydrated male and virginfemale rats, given food and water ad libitum; (2) salt-loadedmale and female rats whose drinking water had been replaced with2% NaCl for 7-10 d; (3) females on the 19th day of gestation that,after parturition, nursed a litter of 10 pups for at least 3 d;they were provided with food and water ad libitum; (4) lactatingfemales that had nursed a litter of 10 pups for at least 3 d andwere provided with food and water ad libitum; and (5) a groupof normally hydrated male and female rats (n = 8) that, underanesthesia (a mixture of equal volumes of ketamine, chloral hydrate,and xylazine), received one injection of colchicine (80 mg in2 µl) into a lateral ventricle; they were killed 24-72 hrlater.

Immunocytochemistry
Tissue fixation. Animals were deeply anesthetized with urethane, injected intracardially with heparin (0.5 ml, 2500 IU), andperfused with fixative composed of freshly prepared 4% paraformaldehydeand 0.1% glutaraldehyde in phosphate buffer (0.1 M, pH 7.4; 300ml during 20 min). After post-fixation in 4% paraformaldehydeovernight at 4°C, brains were removed and cut on a vibratome toobtain frontal slices (50-75 µm), which underwent immunolabelingfor light and electronmicroscopy.
Light microscopy. For single immunostaining, standard immunofluorescence and immunoperoxidase techniques were performed onthe free-floating brain sections, according to procedures describedin detail in our earlier studies (Bonfanti et al., 1992; Oliveet al., 1995). Briefly, after incubation in casein (0.5% in PBS)for 1 hr to block nonspecific sites, they were incubated in amonoclonal mouse IgM antibody that specifically recognizes PSAon NCAM. The production and characterization of the antibody aredescribed in detail previously (Rougon et al., 1986). It is amouse monoclonal IgM recognizing specifically $alpha$ -2,8-linked PSAwith chain length greater than 12 residues. The absence of PSAin NCAM-deficient mice has provided the most compelling evidencethat NCAM is indeed the major carrier of PSA in the CNS (Cremeret al., 1994; Ono et al., 1994). The antibody was used at a dilutionof 1:4000-1:6000 (24-48 hr at 4°C). Affinity-purified anti-mouseIgM immunoglobulins (Igs) conjugated to fluorescein isothiocyanate(FITC) (Immunotech, Marseille, France) (diluted 1:400) or to horseradishperoxidase (HRP) (1:50; Sigma, Les Ulis, France) were used asimmunolabels. HRP reaction product was revealed either with 3,3'-diaminobenzidine(DAB) (0.1%) and 0.01% H₂O₂ or with a more sensitive method usingglucose oxidase-nickel-DAB as substrate (Shu et al., 1988). Thesections were examined with light microscopy (Leica, Paris, France),using bright- and dark-field optics for the HRP-containing sectionsand epifluorescence with appropriate filters for FITC-treatedsections.
Controls included omitting the primary antibody or its substitution by diluted mouse ascites fluid containing IgM irrelevantantibodies. No specific labeling was visible on thesepreparations.
In some cases, double immunolabeling was performed on free-floating sections incubated for 48 hr at 4°C in mixtures of primaryantibodies containing anti-PSA (diluted 1:4000) and mouse monoclonalIgs raised against glial fibrillary acidic protein (GFAP) (diluted1:500; Sigma). After careful rinsing, the sections were incubatedfor 2 hr at room temperature in a mixture of fluorescent conjugates(Immunotech). Rat FITC-conjugated anti-mouse IgM Igs (diluted1:500) were used to identify PSA immunoreactivity, whereas goatanti-mouse Igs conjugated with Texas Red (diluted 1/500) wereused to visualize GFAP immunoreactivities. All preparations wereexamined with standard epifluorescencemicroscopy.
Immunoelectron microscopy. Blocks containing the SON were dissected from vibratome slices of brains obtained from differentgroups of rats that underwent immunoperoxidase labeling for PSA-NCAM,as described above (see also Theodosis et al., 1991). HRP reactionproduct was revealed with DAB and H₂O₂. After osmication, dehydration,block staining in uranyl acetate, and flat embedding in Epon resin,ultrathin sections were cut from selected areas and mounted onnickel grids. They were examined without any further contrastwith a CM10 Philips electronmicroscope.

In vivo endo N treatment
Unilateral injections. Stereotaxy was used to make a single microinjection of endo N in the vicinity of one SON (coordinates:anteroposterior,1.4 mm; lateral, 17.5 mm in relation to the interauraland sagittal lines; depth, 8 mm from the surface of the skull).The enzyme was diluted 1:5000 in 2 µl of artificial CSF from astock solution containing 1 mg/ml protein. The activity of theenzyme was titrated to be 3500 U/mg. The enzyme had been purifiedfrom phage K1 (Wang et al., 1994); it degrades rapidly and specificallylinear polymers of sialic acid with $alpha$ -2,8-linkage with a minimumlength of seven to nine residues (Rutishauser et al., 1985), characteristicof sialic acid residues associated with NCAM (Finne and Mäkelä,1985). The injections were performed in groups of normally hydratedvirgin (n = 3), salt-loaded (n = 5), and gestating (n = 3) ratsthat had been anesthetized with ketamine, chloral hydrate, andxylazine. Another group of salt-loaded rats received a similarinjection of CSF alone (n = 4). The normally hydrated rats werefixed 6 d later, as were the salt-loaded rats that had been given2% saline to drink for 6 d starting on the day of endo N injection.The gestating females were killed 12 d later, after they had undergonea successful parturition and had nursed a litter of 10 pups for6-10 d. All experimental procedures were approved by our institution'sAnimal Care and UseCommittee.
After fixation as described above, the brains were cut on a vibratome to obtain frontal slices (50-75 µm) that underwent immunofluorescenceor immunoperoxidase labeling for PSA-NCAM to control the efficacyof endo N removal of PSA. Blocks containing the SON were dissectedunder microscopic control from slices of animals in which theenzyme had diffused properly (see Fig. 4). They were processedfurther for electron microscopy, which included post-fixationin 1% OsO4 in phosphate buffer, dehydration with increasing concentrationsof ethanol, and embedding in Epon resin. To enhance contrast,they were block-stained with 1.5% uranyl acetate in 50% ethanolduring dehydration. After identification of the SON in semithinsections, ultrathin sections were cut, mounted on nickel grids,contrasted with lead citrate, and examined with a Philips CM10electron microscope. The SON on the side contralateral to theendo N injections was dissected and processedconcomitantly.
Bilateral injections. In one group of gestating rats (n = 4), we used stereotaxy to make two bilateral injections of endoN (diluted 1:5000) in the vicinity of each SON. A group of controlgestating rats (n = 4) that underwent no treatment were examinedconcurrently. The weight and water intake of the pregnant damswas recorded daily. After they gave birth, they were allowed tosuckle litters of 10 pups whose weight was recorded daily. Pupsand mothers were killed 8 d after parturition. The mothers werefixed as described above, and their brains were removed and cuton a vibratome to obtain sections that underwent immunolabelingfor PSA to control the efficacy of endo N removal of PSA fromNCAM.

Quantitative ultrastructural analysis
A comparative ultrastructural analysis was performed on tissue obtained from rats under different conditions of HNS secretion,which had received an injection of endo N or vehicle into thearea of one SON. The analysis was performed only on tissue fromanimals in which the cannula had not entered the SON and in whichthe enzyme had diffused properly and removed all PSA immunoreactivityfrom inside and around the nucleus (see Fig. 4). The contralateralSON was analyzed concurrently. The analysis was performed on electronmicrographs of the ventral [including the ventral glia lamina(VGL)], middle, and dorsal portions of the SON. The micrographshad a final magnification of 13,000×, a magnification high enoughto ensure unambiguous visualization of synapses and cell surfacesand low enough to ensure a large section area in each photograph.The profiles photographed were selected at random with referenceto their position in the grid space, a type of sampling that preventedthe same area from being photographed twice (see also Theodosisand Poulain, 1984). For each group, each composed of a minimumof three animals, at least nine photographs of each SON were examined,and the following parameters were obtained: (1) total number ofneuronal soma and dendritic profiles; (2) number of soma and/ordendritic profiles in juxtaposition (without glial interposition)to other somata and/or dendrites; and (3) number of soma and/ordendrites contacted by the same axonal terminal simultaneously("double" synapse). The investigator was unaware of the experimentalconditions during both the photography and quantitative analysis.Raw data were analyzed using $chi$ ² analysis. Statistical differences were considered significantif p $<=$ 0.05.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

PSA-NCAM is expressed by both HNS neurons and glia

Using an antibody that specifically recognizes PSA on NCAM (Rougon et al., 1986), we confirmed that high levels of PSA-NCAMimmunoreactivity are visible in all parts of the adult rat HNS(see also Theodosis et al., 1991; Bonfanti et al., 1992; Kisset al., 1993). With light microscopy, the immunoreaction in theSON and PVN was characterized by an intense, discontinuous labelingaround immunonegative neuronal somata (Fig. 1A). Electron microscopyshowed that such a perineuronal distribution was essentially attributableto accumulation of PSA immunoreactivity on the surface and inthe cytoplasm of astrocytic processes surrounding neuronal elementswhose cytoplasm was free of reaction (Fig. 1B-E). PSA immunoreactivitywas detected on the surface of some rare axonal and dendriticprofiles, especially in the VGL (Fig. 1E). In the neurohypophysis,immunoreaction covered the surface of all neurosecretory axonsand pituicytes, the astrocytic-like glia of the gland (Fig. 1F).

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Figure 1. PSA immunoreactivity in the adult HNS under basal conditions of neurosecretion. Light microscopy of the SON (A) shows an intense, discontinuous immunoreaction in the neuropile (arrowheads), around immunonegative neuronal somata (S). Electron microscopy (B-E) reveals that this is essentially attributable to the presence of reaction product in astrocytic processes (arrowheads) that surround immunonegative somata (B and at higher magnification in B₁), dendrites (d) (C), and synapses (D). In addition, PSA immunoreaction is visible on the surface of dendritic and axonal (a) profiles, especially in the ventral region of the nucleus (E). In the neurohypophysis, the surfaces of all neurosecretory axons (a) are immunopositive (F). A, Immunofluorescence; B-F, immunoperoxidase labeling.

In accord with our earlier studies (Theodosis et al., 1991; Bonfanti et al., 1992), we found that PSA immunoreactivity didnot vary greatly in its intensity or distribution in the differentparts of the HNS in relation to varying conditions of neurosecretion(Fig. 2).This relative stability of PSA-NCAM expression differsconsiderably from the activity-dependent changes undergone byother molecules colocalized in secretory vesicles in HNS neurons.For example, during lactation and osmotic stimulation, oxytocinand vasopressin accumulate in the hypothalamic somata and decreasein neurohypophysial axons. Levels of colocalized molecules, suchas chromogranins (El Majdoubi et al., 1996) or another cell adhesionmolecule of the Ig superfamily, the F3 glycoprotein (Pierre etal., 1998), also increase in the hypothalamus and decrease inthe neurohypophysis during strong stimulation. In the presentstudy, we found that the only consistent modification in PSA-NCAMexpression in relation to HNS activity was a reduction in labelingwithin clusters of neuronal somata in the nuclei of the dehydratedand lactating rats (Fig. 2A). As clearly shown with electron microscopy,these clusters consist of neuronal profiles whose surfaces arefree of glial processes (Fig. 2B,C; see Fig. 5A), an ultrastructuralfeature that characterizes the stimulated SON and PVN (Theodosisand Poulain, 1993). In these clusters, we never detected any PSAimmunoreactivity at the level of directly juxtaposed neuronalmembranes (Fig. 2B,C).

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Figure 2. PSA immunoreactivity in the HNS under stimulated conditions of neurosecretion. As shown in this example from a lactating rat, the light microscopic distribution (A) in the SON is basically similar to that in unstimulated animals (compare with Fig. 1A). There is, nonetheless, some diminution of labeling associated with clusters of magnocellular somata (arrows). As seen with electron microscopy (B, C), such clusters contain dendritic (d₁, d₂) (B) and somatic (S₁, S₂) (C) profiles whose surfaces are directly juxtaposed, with no glial interposition (between arrows). Note that PSA immunoreactivity is not associated with juxtaposed neuronal membranes, although it continues to be visible in adjacent astrocytic profiles (astro., arrowheads). A, Immunofluorescence; B, C, immunoperoxidase reaction.

To determine the cellular source of PSA-NCAM with more certainty, we examined tissue from animals that had been treated withcolchicine, a drug often used to block axonal transport. Its actionon microtubules, however, is far more extensive, and it inducesa rapid blockade of newly formed material from the rough endoplasmicreticulum to the Golgi and from the Golgi to the cell surface(Malaisse and Orci, 1979; Alonso, 1988). We recently used thisapproach to visualize, in all HNS glia, immunoreactivity for tenascinC, an extracellular matrix molecule that is rapidly secreted byastrocytes and usually detected only in extracellular spaces andon cell surfaces (Theodosis et al., 1997). In the present study,the distribution of PSA-NCAM in the magnocellular nuclei was visiblyaltered as early as 24 hr after a single microinjection into alateral ventricle. As seen with light and electron microscopy(Fig. 3), PSA immunolabel thus diminished in the neuropile andaccumulated heavily in the cytoplasm of astrocytic cell bodiesand processes. In addition, reaction product was now visible,albeit to a lesser and more variable extent, in the cytoplasmof neuronal somata. It is noteworthy that the levels of PSA immunoreactivityappeared unaltered in the neurohypophysis, even 72 hr after intracerebralcolchicine administration.

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Figure 3. PSA immunoreactivity in the SON after cell transport block. Light (A) and electron (B) microscopy shows that, 48 hr after one intraventricular injection of colchicine, there is less PSA immunoreaction in the neuropile. It is now heavily distributed in the cytoplasm of astrocytic cell bodies and processes (astro.) and to a variable degree in that of neuronal somata (N). Note that neurosecretory granules (sg) in the magnocellular soma (N) are unlabeled (B). Immunoperoxidase labeling.

In vivo endo N treatment of the SON

To examine whether the expression of PSA-NCAM by HNS astrocytes and neurons is of consequence to their capacity to undergomorphological remodeling, we performed a comparative ultrastructuralanalysis of the SON in rats under normal (virgin) and stimulatedconditions of HNS secretion known to induce plasticity (lactationand chronic salt ingestion) (Theodosis and Poulain, 1993; Hatton,1997). Concurrent to the onset of stimulation, the animals receiveda single intracerebral injection of endo N in the vicinity ofone SON; the contralateral, untreated SON served as control. Afterrecovery from anesthesia, all animals appeared normal. For example,gestating females that had received an injection of endo N orvehicle gave birth as expected and then lactated in an apparentlynormal manner. The animals were killed, and their tissues wereprepared for light and electron microscopy 6 (virgin and saltloaded groups) or 12 (lactating) d after enzymeinjection.

As judged by light microscopy, endo N diffused in a relatively large volume of tissue around and within the SON (~2 mm³) and removed the punctate, neuropile reaction characteristicof PSA immunolabeling in this part of the brain (Fig. 4). Thecontralateral, uninjected side displayed the usual immunolabeling(Fig. 4). The absence of PSA immunoreactivity on cell surfaceson the side exposed to endo N was confirmed with electron microscopy.

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Figure 4. Effect of endo N treatment on PSA expression in the adult SON in vivo. Twelve days after one single microinjection of the enzyme in the vicinity of one SON, in this example from a lactating rat, PSA immunoreactivity disappeared from the neuropile in a large area (dotted lines) around and within the nucleus (SON₁). Degenerated cells in this area illustrate the point of the cannula used to deliver the enzyme. Note that some astrocytic fibers within and outside the nucleus display reaction, indicating ongoing PSA-NCAM synthesis. On the uninjected side (SON_2, and at higher magnification in the inset on the right), PSA immunoreaction appears normal in the SON and fills the neuropile around immunonegative magnocellular somata. Immunoperoxidase reaction, bright-field optics.

The neuronal-glial and synaptic changes expected to occur in response to HNS stimulation were not apparent in any part ofthe endo N-treated SON (Figs. 5, 6). Comparative quantitativeanalysis of sections that were obtained from the whole anteroposteriorand dorsoventral aspects of the SON showed that the proportionof directly juxtaposed and synaptically coupled neuronal profilesin nuclei exposed to endo N remained low, as in the unstimulated,virgin group (Fig. 6). In contrast, neurons and glia in the SONopposite to that treated with endo N in the stimulated animalsdisplayed morphological changes, to an extent similar to thatreported in earlier analyses (Tweedle and Hatton, 1976; Theodosiset al., 1981; Theodosis and Poulain, 1984); close to 40% of allsoma or dendritic profiles were directly juxtaposed to anotherneuronal profile, and ~6% were coupled by the same axonal terminal(Fig. 6). It is noteworthy that injection of endo N into the SONof control virgin rats did not induce any morphological changes;the incidence of directly juxtaposed and synaptically coupledprofiles in the SON of the endo N-injected side were as low asthat in the contralateral, uninjected side and similar to thosereported previously (Tweedle and Hatton, 1976; Theodosis et al.,1981; Theodosis and Poulain, 1984).

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Figure 5. Effect of endo N in the adult SON in vivo. In the SON of stimulated rats not exposed to endo N (A), there are many neuronal somata whose surfaces are directly juxtaposed, without glia interposition (between arrows); they are also coupled by the same synapse (asterisk). On the other hand, in the same animals, in the contralateral SON that had been exposed to endo N (B), astrocytic processes containing many glial filaments (open arrows) separate the neuronal profiles.

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Figure 6. Effect of endo N on activity-dependent neuronal-glial and synaptic plasticity in the adult SON. Comparative ultrastructural analysis showed that lactation (Lact) and salt loading (Deh) induced a significant increase in the proportion of directly juxtaposed and synaptically coupled neuronal profiles (see Fig. 5A) in the SON not exposed to endo N. On the other hand, in the contralateral SON of the same animals in which endo N had been effective in removing surface PSA, the proportion of juxtaposed and synaptically coupled profiles is low and similar to those in unstimulated virgin rats that had or had not received endo N treatment. Note that, in the SON of salt-loaded rats that had received one microinjection of vehicle (Deh-CSF), plasticity occurred as expected, and the proportion of directly juxtaposed and synaptically coupled neuronal profiles is high and similar to that recorded in the SON of stimulated rats not exposed to the enzyme. $chi$ ² analysis on raw data.

Light and electron microscopy showed that endo N removed PSA from cell surfaces but did not visibly disturb cell metabolism.Moreover, it did not appear to impair PSA-NCAM synthesis becausePSA immunoreactivity was detected in the cytoplasm of some astrocyticprocesses (Fig. 4). As expected (Eng, 1988), the mere introductionof the cannula to inject endo N or vehicle induced a gliosis throughoutthe side of the brain ipsilateral to the injection. This gliosiswas similar to that described after various kinds of injury tothe adult brain and was associated with the appearance of numerousactivated astrocytes that displayed PSA immunoreactivity (Fig.4). Ultrastructurally, such glia in the SON were characterizedby large, thick processes filled with intermediate filaments (Fig.5B). It was not the presence of these astrocytes that inhibitedmorphological remodeling in the magnocellular nuclei. In the groupof salt-loaded rats exposed to vehicle alone, the SON and surroundingareas showed the same signs of reactive gliosis and damage asthat seen in the endo N group yet continued to display the PSAimmunoreaction in the neuropile and did undergo the expected morphologicalchanges (Fig. 6).

To see whether removal of PSA from neuronal and glial surfaces in the SON is of any consequence to HNS function, we performedbilateral injections of endo N in the region of each of the twoSON in a group of gestating female rats. PSA immunocytochemistrywas used to control that the enzyme had diffused properly throughoutthe nuclei and that it had succeeded to remove PSA from cell surfaces.Parturition in these rats (n = 4) appeared to take place normally.Lactation also proceeded as expected, as judged by the mean dailyweight gain of the litters. Thus, after 4 d of lactation (and11 d after endo N injection), the litters of the endo N-treatedfemales showed a mean weight gain (17.3 ± 4.1 gm) that was notsignificantly different from that of litters (19.2 ± 2.0) thathad been nursed by normal, uninjected dams (n =4).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present study confirms our earlier observations describing high levels of PSA-NCAM in the adult HNS and shows that PSA-NCAMis particularly conspicuous in HNS astrocytes. Neuronal expressionof PSA-NCAM is well documented (Rougon, 1993), but less attentionhas been given to its presence in glia. Activated astrocytes thatappear in response to different kinds of lesions express PSA-NCAM(Daniloff et al., 1986; Le Gal La Salle et al., 1992; Bonfantiet al., 1996), but there have been comparatively few reports ofsuch expression in normal adult glia (Bonfanti et al., 1992; Foxet al., 1995). As shown here, strong PSA immunoreactivity wasassociated with HNS astrocytes, and in particular, their processes,even under normal conditions. Cell transport block with colchicinerendered such a localization more telling because it resultedin the accumulation of the glycoprotein throughout the cytoplasmof their processes and cellbodies.

HNS neurons also make PSA-NCAM, but PSA immunoreactivity was usually visible only on their axonal surfaces in the neurohypophysisand on the surface of some rare axonal and dendritic surfacesin the magnocellular nuclei. Colchicine treatment was necessaryto detect PSA immunolabel in the cytoplasm of their somata, areaction that was lighter and more variable than that seen inastrocytes. This indicates that PSA-NCAM expression is polarizedin HNS neurons and that the glycoprotein is quickly transportedto cell surfaces after synthesis, a contention supported by earlierin vitro studies (Alcaraz and Goridis, 1991). Under normal conditions,most of the glycoprotein probably occurs on cell surfaces becausein vivo endo N treatment dramatically reduced the intense neuropileimmunoreaction associated with PSA immunolabeling of the magnocellularnuclei.

That PSA-NCAM is associated with the surface of astrocytic and neuronal processes, which are considered major actors of morphologicalplasticity (Theodosis and Poulain, 1993; Hatton, 1997), offersstrong correlative evidence that this cell adhesion molecule isimportant to their capacity for remodeling. Our experiments usingspecific enzymatic removal of PSA from NCAM in the SON providedirect evidence for this. Enzymatic manipulation of PSA-NCAM expression,especially in vivo, is considered today a most direct test forpresumed PSA functions. In contrast to genetic manipulation ofNCAM (Tomasiewicz et al., 1993; Cremer et al., 1994), which canreflect dysfunction because of the polypeptide itself or leadto adaptive reactions, endo N specifically cleaves the $alpha$ -2,8-linkedsialic acid residues (Rutishauser et al., 1985) without alteringthe NCAM backbone (Ono et al., 1994). Such a procedure has beenapplied successfully in vivo in several neuronal systems to demonstrateintervention of PSA-NCAM in dynamic cellular processes as differentas neurite outgrowth (Landmesser et al., 1990), cell migration(Ono et al., 1994; Yoshida et al., 1999), and control of circadianrhythm (Shen et al., 1997).

In the present study, such in vivo enzymatic manipulation of PSA-NCAM showed, for the first time, that PSA on NCAM is necessaryfor activity-dependent morphological synaptic plasticity and neuronal-glialremodeling. The existence of two bilateral SON in the hypothalamusoffered the unique opportunity to have a built-in control forthis kind of experimentation. As seen with light and electronmicroscopy, injection of endo N succeeded to remove PSA from arelatively large area within and around one SON, whereas the correspondingnucleus on the uninjected side continued to display the expectedreaction. Moreover, as also noted by others (Landmesser et al.,1990; Shen et al., 1997; Yoshida et al., 1999), the action ofthe enzyme was long-lasting, being effective over 2 weeks afterinjection. Coupled with comparative ultrastructural analysis,this approach allowed us to show unambiguously that PSA-NCAM isessential to morphological neuronal and glial remodeling. In theendo N-treated SON, therefore, astrocytic processes continuedto separate neuronal profiles, and there was no increase in synapticinputs, despite sustained, strong stimuli that normally induceglial retraction and synapse proliferation. In contrast, thesemodifications occurred in the expected proportions in the contralateralnuclei not exposed to endoN.

An obvious question is whether the ultrastructural changes are of functional consequence to the HNS. It would be surprisingif the synapse proliferation associated with HNS activation isof no consequence to the activity of HNS neurons (discussed furtherin Theodosis and Poulain, 1993, 1996). As for astrocytic remodeling,it might serve to either allow the synaptic changes or it mayhave other, more direct consequences, yet to be determined (Theodosisand MacVicar, 1996). In an attempt to address this question, wehere performed bilateral injections of endo N into the two SONin gestating animals. As expected from our unilateral endo N injectionexperiments, PSA immunoreactivity was no longer visible in theneuropile of the two nuclei, yet lactation and water intake proceededin an apparently normal manner. This could be taken as evidencethat the morphological changes are of no consequence to HNS function.It must be kept in mind, however, that the HNS is a very robustsecretory system. Because of its anatomical disposition (thereare four magnocellular nuclei and approximately one-third of allmagnocellular neurons are interspersed anywhere in the hypothalamus),it has not been possible to totally destroy the system withoutkilling the animals (for review, see Wakerley et al., 1994). However,extensive lesions of two nuclei leave HNS function grossly undisturbed(Wakerley et al., 1994), as we noted here after bilateral injectionof endo N into two SON. This indicates that strong compensatorymechanisms must occur rapidly, and they could mask any subtlealterations at the electrophysiological level, for instance. Furtherexperiments on hypothalamic slices, for example, are necessaryto pursue this question in moredetail.

What also remains to be elucidated is the cell mechanism by which PSA intervenes to permit morphological neuronal-glial andsynaptic changes. Our observations are in agreement with a mechanismwhereby large quantities of PSA on the extracellular domain ofNCAM would attenuate adhesion via physical impedance or chargerepulsion, thus allowing dynamic structural modifications (Rutishauserand Landmesser, 1996). Cells could then detach from their neighborsor from the extracellular matrix and be able to undergo changesin theirconformation.

Whatever the molecular mechanism, PSA-NCAM cannot be considered an inductive factor for this kind of plasticity because itis continuously expressed, whatever the physiological condition,in cells that can undergo such changes. On the other hand, ourobservations clearly show that it is a necessary determinant forthis plasticity. PSA-NCAM can be considered, therefore, as a permissivefactor to allow cells to undergo remodeling whenever the properstimulus intervenes. In the hypothalamic magnocellular nuclei,one such stimulus is oxytocin itself because its intracerebroventricularapplication in normal animals induced morphological changes similarto those observed under physiological stimulation (Theodosis etal., 1986). In other neuronal systems capable of similar morphologicalremodeling (for review, see Theodosis and Poulain, 1993) and whichalso express PSA-NCAM (Bonfanti et al., 1992), other inductivefactors mustintervene.

  FOOTNOTES

Received Aug. 5, 1999; accepted Sept. 15, 1999.

We are grateful to Dr. C. Henderson for his critical reading of an earlier version of this manuscript. We also thank I. Svahn(Service Commun de Microscopie Université Victor Segalen BordeauxII) for her expert photographicwork.
Correspondence should be addressed to D. T. Theodosis at the above address. E-mail: dionysia.theodosis{at}bordeaux.inserm.fr.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Alcaraz G, Goridis C (1991) Biosynthesis and processing of polysialylated NCAM by AtT-20 cells. Eur J Cell Biol 55:165-173[ISI][Medline].
Alonso G (1988) Effects of colchicine on the intraneuronal transport of secretory material prior to the axon: a morphofunctional study in hypothalamic neurosecretory neurons of the rat. Brain Res 453:191-203[ISI][Medline].
Bonfanti L, Theodosis DT (1994) Expression of polysialylated neural cell adhesion molecule by proliferating cells in the subependymal layer of the adult rat, in its rostral extension and in the olfactory bulb. Neuroscience 62:291-305[ISI][Medline].
Bonfanti L, Olive S, Poulain DA, Theodosis DT (1992) Mapping of the distribution of polysialylated neural cell adhesion molecule throughout the central nervous system of the adult rat: an immunohistochemical study. Neuroscience 49:419-436[ISI][Medline].
Bonfanti L, Merighi A, Theodosis DT (1996) Dorsal rhizotomy induces transient expression of the highly sialylated isoform of the neural cell adhesion molecule in neurons and astrocytes of the adult rat spinal cord. Neuroscience 74:619-623[ISI][Medline].
Cremer H, Lange R, Christoph A, Plomann M, Vopper G, Roes J, Brown R, Baldwin S, Kraemer P, Scheff S, Barthels D, Rajewsky K, Wille W (1994) Inactivation of the N-CAM gene in mice results in size reduction of the olfactory bulb and deficits in spatial learning. Nature 367:455-459[Medline].
Cremer H, Chazal G, Carleton A, Goridis C, Vincent JD, Lledo PM (1998) Long-term but not short-term plasticity at mossy fiber synapses is impaired in neural cell adhesion molecule-deficient mice. Proc Natl Acad Sci USA 95:13242-13247[Abstract/Free Full Text].
Daniloff JK, Levi G, Grumet M, Rieger F, Edelman GM (1986) Altered expression of neuronal cell adhesion molecules induced by nerve injury and repair. J Cell Biol 103:929-945[Abstract/Free Full Text].
El Majdoubi M, Metz-Boutigue M-H, Garcia-Sablonne P, Theodosis DT, Aunis D (1996) Immunocytochemical localization of chromogranin A in the hypothalamo-neurohypophysial system of the rat. J Neurocytol 25:405-416[ISI][Medline].
Eng LF (1988) Regulation of glial intermediate filaments in astrogliosis. In: The biochemical pathology of astrocytes (Norenberg MD, Hertz L, Schousboe A, eds), pp 79-90. New York: Liss.
Finne J, Mäkelä PH (1985) Cleavage of the polysialosyl units of brain glycoproteins by a bacteriophage endosialidase. J Biol Chem 260:1265-1270[Abstract/Free Full Text].
Fox GB, Kennedy N, Regan CM (1995) Polysialylated neural cell adhesion molecule expression by neurons and astroglial processes in the rat dentate gyrus declines dramatically with increasing age. Int J Dev Neurosci 13:663-672[ISI][Medline].
Fryer HJL, Hockfield S (1996) The role of polysialic acid and other carbohydrate polymers in neural structural plasticity. Curr Opin Neurobiol 6:113-118[ISI][Medline].
Hatton GI (1997) Function-related plasticity in the hypothalamus. Annu Rev Neurosci 20:375-397[ISI][Medline].
Kiss JZ, Wang C, Rougon G (1993) Nerve-dependent expression of high polysialic acid neural cell adhesion molecule in neurohypophysial astrocytes of adult rats. Neuroscience 53:213-222[ISI][Medline].
Landmesser L, Dahm L, Tang J, Rutishauser U (1990) Polysialic acid as a regulator of intramuscular nerve branching during embryonic development. Neuron 4:655-667[ISI][Medline].
Le Gal La Salle G, Rougon G, Valin A (1992) The embryonic form of neural cell surface molecule (E-NCAM) in rat hippocampus and its reexpression on glial cells following kainic acid-induced status epilepticus. J Neurosci 12:872-882[Abstract].
Malaisse WJ, Orci L (1979) The role of the cytoskeleton in pancreatic B-cell function. Methods Achiev Exp Biol 9:112-136.
Muller D, Wang C, Skibo G, Toni N, Cremer H, Calaora V, Rougon G, Kiss JZ (1996) PSA-NCAM is required for activity-induced synaptic plasticity. Neuron 17:413-422[ISI][Medline].
Nothias F, Vernier P, Von Boxberg Y, Mirman S, Vincent JD (1997) Modulation of NCAM polysialylation is associated with morphofunctional modification in the hypothalamo-neurohypophysial system during lactation. Eur J Neurosci 9:1553-1565[ISI][Medline].
Olive S, Rougon G, Pierre K, Theodosis DT (1995) Expression of a glycosyl phosphatidylinositol-anchored adhesion molecule, the glycoprotein F3, in the adult rat hypothalamo-neurohypophysial system. Brain Res 689:271-280[ISI][Medline].
Ono K, Tomasiewicz H, Magnuson T, Rutishauser U (1994) N-CAM mutation inhibits tangential neuronal migration and is phenocopied by enzymatic removal of polysialic acid. Neuron 13:595-609[ISI][Medline].
Pierre K, Rougon G, Allard M, Bonhomme R, Gennarini G, Poulain DA, Theodosis DT (1998) Regulated expression of the cell adhesion glycoprotein F3 in adult hypothalamic magnocellular neurons. J Neurosci 18:5333-5343[Abstract/Free Full Text].
Rougon G (1993) Structure, metabolism and cell biology of polysialic acids. Eur J Cell Biol 61:197-207[ISI][Medline].
Rougon G, Dubois C, Buckley N, Magnani JL, Zollinger W (1986) A monoclonal antibody against meningococcus group B polysaccharides distinguishes embryonic from adult N-CAM. J Cell Biol 103:2429-2437[Abstract/Free Full Text].
Rousselot P, Lois C, Alvarez-Buylla A (1995) Embryonic (PSA) N-CAM reveals chains of migrating neuroblasts between the lateral ventricle and the olfactory bulb of adult mice. J Comp Neurol 351:51-61[ISI][Medline].
Rutishauser U, Landmesser L (1996) Polysialic acid in the vertebrate nervous system: a promoter of plasticity in cell-cell interactions. Trends Neurosci 19:422-427[ISI][Medline].
Rutishauser U, Watanabe M, Silver J, Troy FA, Vimr ER (1985) Specific alteration of NCAM-mediated cell adhesion by an endoneuraminidase. J Cell Biol 101:1842-1849[Abstract/Free Full Text].
Shen H, Watanabe M, Tomasiewicz H, Rutishauser U, Magnuson T, Glass JD (1997) Role of neural cell adhesion molecule and polysialic acid in mouse circadian clock function. J Neurosci 17:5221-5229[Abstract/Free Full Text].
Shu S, Ju G, Fan L (1988) The glucose oxidase-DAB-nickel method in peroxidase histochemistry of the nervous system. Neurosci Lett 85:169-171[ISI][Medline].
Theodosis DT, MacVicar BA (1996) Neuron-glia interactions in the hypothalamus and pituitary. Trends Neurosci 19:363-367[ISI][Medline].
Theodosis DT, Poulain DA (1984) Evidence for structural plasticity in the supraoptic nucleus of the rat hypothalamus in relation to gestation and lactation. Neuroscience 11:183-193[ISI][Medline].
Theodosis DT, Poulain DA (1993) Activity-dependent neuronal-glial and synaptic plasticity in the adult mammalian hypothalamus. Neuroscience 57:501-535[ISI][Medline].
Theodosis DT, Poulain DA (1996) Pulsatile neuronal activity and structural synaptic plasticity of the adult oxytocinergic system. Curr Opin Endocrinol Diab 3:164-170.
Theodosis DT, Poulain DA, Vincent JD (1981) Possible morphological bases for synchronisation of neuronal firing in the rat supraoptic nucleus during lactation. Neuroscience 6:919-929[ISI][Medline].
Theodosis DT, Montagnese C, Rodriguez F, Vincent JD, Poulain DA (1986) Oxytocin induces morphological plasticity in the adult hypothalamo-neurohypophysial system. Nature 322:738-740[Medline].
Theodosis DT, Rougon G, Poulain DA (1991) Retention of embryonic features by an adult neuronal system capable of plasticity: Polysialylated N-CAM in the hypothalamo-neurohypophysial system. Proc Natl Acad Sci USA 88:5494-5498[Abstract/Free Full Text].
Theodosis DT, Pierre K, Cadoret MA, Allard M, Faissner A, Poulain DA (1997) Expression of high levels of the extracellular matrix glycoprotein, tenascin-C, in the normal adult hypothalamo-neurohypophysial system. J Comp Neurol 379:386-398[ISI][Medline].
Theodosis DT, El Majdoubi M, Pierre K, Poulain DA (1998) Factors governing activity-dependent structural plasticity of the hypothalamo-neurohypophysial system. Cell Mol Neurobiol 18:285-298[ISI][Medline].
Tomasiewicz H, Ono K, Yee D, Thompson C, Goridis C, Rutishauser U, Magnuson T (1993) Genetic deletion of a neural cell adhesion molecule variant (N-CAM-180) produces distinct defects in the central nervous system. Neuron 11:1163-1174[ISI][Medline].
Tweedle CD, Hatton GL (1976) Ultrastructural comparisons of neurons of supraoptic and circularis nuclei in normal and dehydrated rats. Brain Res Bull 1:103-121[ISI][Medline].
Wakerley JB, Clarke G, Summerlee AJS (1994) Milk ejection and its control. In: The physiology of reproduction, Ed 2 (Knobil E, Neill JD, eds), pp 2283-2322. New York: Raven.
Wang C, Rougon G, Kiss JZ (1994) Requirement of polysialic acid for the migration of the O-2A glial progenitor cell from neurohypophysial explants. J Neurosci 14:4446-4457[Abstract].
Yoshida K, Rutishauser U, Crandall JE, Schwarting GA (1999) Polysialic acid facilitates migration of luteinizing migration of luteinizing hormone-releasing hormone neurons on vomeronasal axons. J Neurosci 19:794-801[Abstract/Free Full Text].

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