Interplay between Presynaptic and Postsynaptic Activities Is Required for Dendritic Plasticity and Synaptogenesis in the Supraoptic Nucleus

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The Journal of Neuroscience, January 1, 2002, 22(1):265-273

Interplay between Presynaptic and Postsynaptic Activities Is Required for Dendritic Plasticity and Synaptogenesis in the Supraoptic Nucleus
Vivien Chevaleyre, Françoise C. Moos, and Michel G. Desarménien
Centre National de la Recherche Scientifique Unité Mixte de Recherche 5101, Biologie des Neurones Endocrines, 34094 Montpellier Cedex 5, France

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Developing oxytocin and vasopressin (OT/AVP) supraoptic nucleus (SON) neurons positively autocontrol their electrical activityvia dendritic release of their respective peptide. The effectsof this autocontrol are maximum during the second postnatal week(PW2), when the dendritic arbor transiently increases and glutamatergicpostsynaptic potentials appear. Here, we studied the role andinteraction of dendritic OT/AVP release and glutamate releasein dendritic plasticity and synaptogenesis in SON. In vivo treatmentwith the peptides antagonists or with an NMDA antagonist suppressedthe transient increase in dendritic arbor of SON neurons at thebeginning of PW2. Incubation of acute slices with these compoundsdecreased the dendritic arbor on a short time scale (3-8 hr) inslices of postnatal day 7 (P7) to P9 rats. Conversely, applicationof OT/AVP or NMDA increased dendritic branches in slices of P3-P6rats. Their effects were inhibited by blockade of electrical activity,voltage-gated Ca²⁺ channels, or intracellular Ca²⁺ mobilization. They were also interdependent because both OT/AVPand NMDA (but not AMPA) receptor activation were required forincreasing the dendritic arbor. Part of this interdependence probablyresults from a retrograde action of the peptides facilitatingglutamate release. Finally, blocking OT/AVP receptors by in vivotreatment with the peptides antagonists during development decreasedspontaneous glutamatergic synaptic activity recorded in youngadults. These results show that an interplay between postsynapticdendritic peptide release and presynaptic glutamate release isinvolved in the transient increase in dendritic arbor of SON neuronsand indicate that OT/AVP are required for normal synaptogenesisof glutamatergic inputs inSON.

Key words: oxytocin; vasopressin; glutamate; NMDA receptor; development; electrical activity; retrograde messenger

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The structure of the dendritic arbor is a critical feature determining the number, diversity, and integration of inputs receivedby a neuron (Koester and O'Leary, 1994). For instance, alterationin the development of the neuronal morphology is likely to affectnormal brain function. Reduced dendrites have been related tomental retardation in children (Purpura, 1975), strongly suggestingthat neuronal structure and cognitive capacity are closely related.The formation of dendritic arbor and synaptic connections is ahighly dynamic process. Neurites bearing postsynaptic elements,such as filopodia, display a high motility during synaptogenesis,whereas synapses are repeatedly formed and eliminated before themature connection pattern is achieved. Recent in vivo studiesin zebra fish and rat have shown that dynamic interactions betweenfilopodia and growth cones occur (Jontes et al., 2000) and thatthe rate of filopodia motility depends on the level of input activity(Lendvai et al., 2000). Here, we studied the influence of interactionsbetween presynaptic and postsynaptic activities on the dendriticarbor plasticity during synaptogenesis in the supraoptic nucleus(SON).

Hypothalamic SON neurons project to the neurohypophysis in which they secrete oxytocin or vasopressin (OT/AVP) into the bloodcirculation. The peptides are also released at dendritic sitesand exert an autocontrol on their secreting neurons. During development,the peptides maintain spontaneous electrical activity via a depolarizationand a facilitation of their own dendritic release (Chevaleyreet al., 2000). This autocontrol loop is maximum during the secondpostnatal week (PW2) and is correlated with a transient increasein dendritic branching (Chevaleyre et al., 2001). Meanwhile, functionalmonoaminergic synapses are formed (Ugrumov, 1992; Nelson et al.,1998), NMDA receptor density transiently increases (Hussy et al.,1997), and glutamatergic postsynaptic potentials appear (Chevaleyreet al., 2001), indicating an intense period of synapse formation.In view of this concomitance of events, we studied the role ofdendritic peptide release and its interaction with glutamate releasedby incoming inputs [the major excitatory neurotransmitter in theSON (van den Pol et al., 1990)] on the morphological plasticityobserved in SON neurons. We used in vivo and in vitro experimentsto show that NMDA receptor and OT/AVP receptor activation areboth needed to increase the dendritic arbor, suggesting that aninterplay between presynaptic and postsynaptic activities is requiredfor this plasticity. In addition, the peptides are able to acton presynaptic endings and increase glutamatergic synaptic transmission.Moreover, injection of OT/AVP antagonists during the first twopostnatal weeks (PW2) decreased spontaneous synaptic activityin SON slices from young adult rats, suggesting that early activationof OT/AVP receptors indeed plays a determinant role for normalsynaptogenesis inSON.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In vivo drug treatment. Some littermates were assigned to receive daily subcutaneous injection of a solution containing either(+)-5-methyl-10,11-dihydro-5H-dibenzo [a,d] cyclohepten-5,10-iminemaleate (MK801) (1 mg/kg; 1 µl/gm) or a mixture of OT antagonistand V_1a and V₂ AVP antagonists (9, 0.5, and 0.6 µg/kg, respectively;0.7 µl/gm) from birth to postnatal day 7 (P7) or P8. Others pupsof the litter received saline (with 0.36% DMSO for controls ofOT/AVP-treated rats). Pups were killed 14-16 hr later, and themorphology of SON neurons was studied in acute slice (see below).For experiments on synaptic activity, rats were treated dailywith saline or OT/AVP antagonists mixture from P3 to P17, andglutamatergic activity was recorded during PW4 (seebelow).

Slice preparation and drug treatment. Standard methods were used as described previously (Chevaleyre et al., 2000). Briefly,P3-P9 rats were killed by decapitation, and brains were rapidlyremoved and immersed in a cold oxygenated (95% O₂, 5% CO₂) sucrosesolution [in mM: 220 sucrose, 2.3 KCl, 26 NaHCO₃, 2.5 CaCl₂, 10glucose, 1.2 KH₂PO₄, and 1.2 MgSO₄, pH 7.4 (300 mOsm/l)]. A blockcontaining the hypothalamus was dissected out and mounted on avibratome (Campden Instruments, Loughborough, UK), and a horizontalslice (250-µm-thick) was cut. Each half containing one SON wasthen incubated in oxygenated (95% O₂, 5% CO₂) artificial CSF (ACSF)[in mM: 110 NaCl, 1.2 KCl, 26 NaHCO₃, 2 CaCl₂, 10 glucose, 1.2KH₂PO₄, and 2 MgCl₂, pH 7.4 (300 mOsm/l)] supplemented with variousagents during 3-8 hr at room temperature. A half slice was thentransferred into an immersion type recording chamber, under theobjective (40×) of a conventional microscope and perfused withoxygenated (95% O₂, 5% CO₂) ACSF (34°C) at a rate of 2 ml/min,and neurons were dyed with Lucifer yellow(LY).

Morphological analysis. Neurons were loaded with LY (Sigma, St. Quentin Fallavier, France) added into the intrapipette solution[in mM: 135 KMeSO₃, 5 KCl, 1 CaCl₂, 5 EGTA-Na, 4 ATP-Mg, 10 HEPES-Na,and 1 LY, pH 7.2 (290 mOsm/l)]. Neurons with large cell body andgenerally exhibiting an $alpha$ dendrite (Hatton, 1990), shown previouslyto synthesize either OT or AVP at all stages of postnatal development(Hussy et al., 1997), were selected in the SON. After establishmentof the whole-cell configuration, LY diffusion was facilitatedby application of repetitive voltage steps from $-$ 60 to $-$ 90 mVduring ~30 min. Neuronal shapes were then drawn either directlyor after acquisition of z series images with a PCO camera (Dipsi,Chatillon, France) and Axon Imaging Workbench software (Axon Instruments,Foster City, CA). The number and order of each dendritic branchwas measured. To avoid variability between rats, all comparisonswere made between the two SON of the same rat incubated duringthe same time (3-8 hr) in different solutions. Results were pooledonly if the experimental conditions for each of the two SONs ofeach rat were identical. Data are expressed as mean ± SEM, andsignificance was evaluated using ANOVAtest.

Electrophysiological recordings. Horizontal slices were prepared from P7-P9 or P21-P23 rats, and the neurons were visualizedunder infrared interference microscopy. Because the number ofsynapses can increase after slicing (Kirov et al., 1999), carewas taken to respect similar delay between slicing and recordingfor control and treated rats (between 2 and 8 hr). Slices wereperfused with ACSF (34°C) at a rate of 2 ml/min, and neurons wererecorded in the whole-cell configuration with 3-5 M $Omega$ patch pipettescontaining the intrapipette solution without LY (see above). EPSCswere recorded and digitized (6.6 kHz; Clampex software; Axon Instruments)and filtered at 5 kHz (eight-pole Bessel filter) for at least10 min from a holding potential of $-$ 60 mV; series resistance wascontrolled before and after this collection. EPSCs were analyzedoff-line using a home-made routine (Origin; Microcal SoftwareInc., Northampton, MA) for measurement of frequency and amplitude.Recordings were performed close to the reversal potential of GABA-evokedchloride currents and in the presence of a GABA_A receptor blocker(3 µM gabazin) in two-thirds of the neurons. No difference wasobserved in the mean amplitude and frequency between neurons recordedwith or without gabazin, indicating that only glutamatergic EPSCswererecorded.

Pharmacological compounds. OT/AVP antagonists consisted of a cocktail of an OT antagonist [100 nM dOVT or Manning compound:d(CH₂)₅[Tyr(Me)²,Thr⁴,Tyr-NH₂⁹; kindly provided by Dr C. Barberis, Montpellier, France], a V_1areceptor antagonist [10 nM SR49059: (2S)1[(2R,3S)-(5-chloro-3-(2-chlorophenyl)-1-(3,4-dimethoxybenzene-sulfonyl))-3-hydroxy-2,3-dihydro-1H-indole-2-carbonyl]-pyrrolidine-2-carboxamide],and a V₂ antagonist [10 nM SR121463A: 1-[4-(N-tert-butylcarbamoyl)-2-metoxybenzenesulfonyl]-5-ethoxy-3-spiro-[4-(2-morpholino ethoxy) cyclohexane]-indol-2-one,furamate; equatorial isomer] (both provided by Sanofi SynthelaboRecherche, Toulouse, France). OT and AVP were purchased from Calbiochem-Novabiochem(La Jolla, CA). CNQX and MK801 were purchased from Research Biochemicals(Sigma). Thapsigargin, $omega$ -conotoxin-GVIA, and $omega$ -agatoxin-IVA werepurchased from Alomone Labs (Jerusalem, Israel). CNQX, NMDA, TTX,nicardipin, and all salts were purchased fromSigma.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

SON neurons from hypothalamic slices were injected with Lucifer yellow through a patch-clamp pipette, drawn after 30 min diffusionof the dye, and the number of dendritic branches was counted.Previous study has shown that the number of branches increasesin SON neurons at the beginning of PW2 and then decreases duringPW2-PW3, leading to bipolar or tripolar neurons with a few branching(Chevaleyre et al., 2001). Here, the mechanisms involved in theincrease in dendritic arbor were studied in 414 neurons dyed afterdifferent experimental conditions during two developmental periods:between P3 and P6, the period preceding the normal increase indendritic branches, and between P7 and P9, the period of maximaldendritic arbor. The mean number of dendritic branches per neuronin control condition was 12.6 ± 0.6 at P3-P6 (n = 53) and 16.2± 0.7 at P7-p9 (n = 39; p < 0.01).

Role of OT/AVP in shaping the dendritic arbor

Rat pups were injected daily with OT/AVP antagonists from birth to P6 or P7. The morphology of the dendrites was studied 14-16hr later. A decrease in the dendritic arbor was observed in OT/AVPantagonist-treated rats compared with saline-treated rats (Fig.1a). The number of primary dendrites was not affected (Fig. 1b),but the total number of dendritic branches was reduced by 36%(Fig. 1c). To analyze the underlying mechanisms, experiments withacute hypothalamic slices were performed. For each slice, one-halfcontaining one SON was incubated 3-8 hr with OT/AVP antagonists,and the dendritic arbor was compared with that of neurons of theother SON incubated in control condition. Incubation with OT/AVPantagonists (100 and 10 nM for OT and AVP antagonists, respectively)significantly decreased the large dendritic arbor of P7-P9 rats(37% decrease) (Fig. 1d,e), whereas it had only a slight effectbefore the normal increase in P3-P6 rats (12% decrease) (Fig.1f,g). Conversely, incubation with OT/AVP (each at 100 nM) increasedthe number of branches (Fig. 2a). The effects of OT/AVP were smalland nonsignificant at P7-P9 (15% increase) (Fig. 2d,e) but significantat P3-P6 (53% increase) (Fig. 2f,g). Again, the number of primarydendrites was not changed by the various treatments, with onlyhigher-order dendrites being affected. These results show thatthe peptide receptors and growth mechanisms are already functionalat P3-P6 and that endogenous peptides are involved in the increaseand maintenance of the dendritic arbor at P7-P9.

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Figure 1. Endogenous OT/AVP are required for dendritic arbor maintenance. a, Example of representative SON neurons dyed at P7 from a control and an OT/AVP antagonist-treated rat. b, Mean number of dendrites versus dendrite order for neurons dyed from P7-P8 control (C; open circles) or OT/AVP antagonist (OT/VP Antago)-treated rats (filled squares), indicating that mostly third- and higher-order dendrites were affected. c, Neurons of OT/AVP antagonist-treated rats displayed an important decrease in their total number of dendrites compared with control ones. d-g, In vitro incubation of the slices in OT/AVP antagonists led at P7-P9 to a similar decrease in the dendritic arbor compared with the in vivo treatment (d, e) but had almost no effect at P3-P6 (f, g). Note that, at P7-P9, antagonists reduced the number of dendritic branches to values similar to that of P3-P6 controls. The number of neurons is indicated in each bar (*p < 0.05; ANOVA).

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Figure 2. OT/AVP increase the number of dendritic branches. a, Example of representative SON neurons dyed at P4-P5 in control condition or after in vitro incubation in OT/AVP showing an increase in the number of branches. b, Mean number of dendrites versus the dendrite order at P3-P6 showing no effect of OT/AVP (OT/VP; filled squares) on primary dendrites and a significant increase in fourth- and fifth-order dendritic branches compared with control neurons (C; open circles). This resulted in an important increase in the total number of dendritic branches (c). At P3-P6, however, OT/AVP application only slightly increased fourth-order dendrites (d) and had no significant effect on the total number of dendrites (e). The number of neurons is indicated in each bar (**p < 0.01; ANOVA).

Role of NMDA receptor activation in shaping the dendritic arbor

Because glutamatergic EPSPs appear and somatic NMDA receptors transiently increase during PW2 in SON neurons, we tested therole of NMDA in dendritic plasticity. In vivo daily injectionof the NMDA antagonist MK801 from P0 to P6 resulted in a significantreduction (27%) in the number of dendritic branches observed atP7 (Fig. 3a-c). Incubation of a slice with MK801 (1 µM) did notchange the number of primary dendrites but decreased the dendriticbranches in a manner similar to OT/AVP antagonists. The decreasewas important at P7-P9 (34% decrease) (Fig. 3d,e) and small atP3-P6 (6% decrease) (Fig. 3f,g). Conversely, incubation with NMDA(1 µM) increased the dendritic arbor (Fig. 4a). As for OT/AVP,the NMDA effect was marked at P3-P6 (32% increase) (Fig. 4b,c)and smaller at P7-P9 (12% increase) (Fig. 4d,e). These resultsshow that NMDA receptor activation by endogenous glutamate isnecessary for the increase and maintenance of the dendritic arbor.

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Figure 3. Natural activation of NMDA receptor is necessary for dendritic arbor maintenance. a, Example of representative SON neurons at P7, showing a decrease in the number of branches after incubation in MK801. b, Mean number of dendritic branches versus the dendrite order for neurons dyed from control (C; open circles) or MK801-treated rats (MK801; filled squares) showing a decrease in third- and fourth-order dendrites. c, The total number of dendritic branches was significantly decreased in MK801-treated rats. d-g, In vitro experiments showing an important decrease in branching by MK801 in slices of P7-P9 rats (d, e) but not in slices of P3-P6 rats (f, g). The number of neurons is indicated in each bar (*p < 0.05; ANOVA).

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Figure 4. NMDA increases the number of dendritic branches. a, Example of representative neurons dyed at P4 indicating an increase in small branches after incubation in NMDA. b, The mean number of dendrites by order revealed that, at P3-P6, NMDA (filled squares) had no effect on first- and second-order dendrites but increased significantly fifth-order dendrites compared with controls (C; open circles). This resulted in a significant increase in the total number of dendritic branches at P3-P6 (c). Conversely, at P7-P9, NMDA had only slight effects on third- and fourth-order dendrites (d) and did not change significantly the total number of dendrites (e). The number of neurons is indicated in each bar (*p < 0.05; ANOVA).

Role of electrical activity in shaping the dendritic arbor

Because electrical activity is increased by OT/AVP and NMDA, its role in dendritic plasticity was investigated using TTX (0.3µM). At P7-P9, a decrease in the number of branches was observedwhen TTX (0.3 µM) was applied in the presence of OT/AVP and NMDAto compensate for a putative decrease in endogenous peptides andglutamate release (Fig. 5a). Conversely, application of OT/AVPand NMDA did not increase the dendritic arbor at P3-P6 in thepresence of TTX, even when the voltage-dependent block of NMDAreceptors was relieved by omitting Mg²⁺ from the medium (Fig. 5b). Electrical activity seems, therefore,to be involved in the increase in dendritic branches. However,activity could act indirectly, via an increase in endogenous peptidesrelease. This would imply that the amount of exogenous peptideswas not sufficient to increase branching and that additional endogenouspeptides release was needed. This seems unlikely because increasingthe peptides concentration by a factor 10 or 100 did not counteractthe effect of TTX at P3-P6 (106 and 97% of TTX alone with 1 and10 µM OT/AVP, respectively; n = 7 and 8; data not shown). However,electrical activity is not sufficient to increase the dendriticarbor because a high K⁺ solution, able to increase the number of dendritic branches atP3-P6, had no effect when OT/AVP and NMDA receptors were blocked(Fig. 5c). Altogether, these results suggest an hypothesis inwhich electrical activity is involved in the increase in the dendriticarbor independently of increasing endogenous peptides releasebut is not a unique downstream consequence in OT/AVP and NMDAaction on dendrites.

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Figure 5. Electrical activity, voltage-gated Ca²⁺ channels, and intracellular Ca²⁺ stores are involved in the effect of OT/AVP and NMDA. a, Suppression of electrical activity by TTX at P7-P9 decreased the number of dendritic branches, even when OT/AVP and NMDA were added to compensate for the decrease in endogenous release induced by TTX. All other experiments were performed at P3-P6. b, In the presence of TTX, OT/AVP and NMDA were unable to increase the number of dendritic branches, even when Mg²⁺ was removed to increase NMDA receptor activation. c, Application of 12.5 mM K⁺ increased the total number of dendritic branches. However, when applied in the presence of OT/AVP antagonists (OT/AVP Antago.) and MK801, the high-K⁺ solution had no effect on the dendritic arbor, indicating that electrical activity alone was not effective. d, The blockade of L-, N-, and P/Q-type voltage-gated Ca²⁺ channels by a cocktail of toxins (VGCC toxins) disrupted the effects of OT/AVP and NMDA, even when high K⁺ was added. The increase in the dendritic arbor also depends on mobilization of intracellular Ca²⁺ stores because OT/AVP and NMDA were ineffective in the presence of thapsigargin (Thapsig.). The number of neurons is indicated in each bar (*p < 0.05; ANOVA).

Role of Ca²⁺ in shaping the dendritic arbor

Whatever its precise implication in the process of increasing the dendritic arbor, electrical activity could act by triggeringCa²⁺ influx via voltage-gated Ca²⁺ channels (VGCCs). At P3-P6, in the presence of toxins for L,N, and P/Q channels (3 µM nicardipin, 500 nM $omega$ -conotoxin-GVIA,and 200 nM $omega$ -agatoxin-IVA, respectively), OT/AVP, NMDA, and highK⁺ had no effect on the dendritic arbor (Fig. 5c). Because OT/AVPare known to mobilize intracellular Ca²⁺ in adults, stores were depleted with thapsigargin (0.2 µM), ablocker of the reticulum Ca²⁺-ATPase. In the presence of thapsigargin, which did not changethe number of dendritic branches compared with control (n = 5and 4, respectively; data not shown), OT/AVP and NMDA were unableto increase the dendritic arbor at P3-P6 (Fig. 5d). These resultssuggest that both Ca²⁺ influx via VGCC and Ca²⁺ release from intracellular stores are involved in the increasein the dendriticarbor.

Interdependence of OT/AVP and NMDA effects

To study whether OT/AVP and NMDA act on separated pathways, OT/AVP were applied at P3-P6 in the presence of MK801. Under thiscondition, OT/AVP were unable to increase the number of dendriticbranches (Fig. 6a). However, because electrical activity appearsto be involved in dendritic plasticity and could have been reducedby MK801, the same experiment was performed in the presence ofhigh K⁺. Under this condition, OT/AVP were still unable to increase thedendritic arbor (Fig. 6a). This effect was specific for NMDA receptoractivation because OT/AVP increased the number of dendritic branchesin the presence of CNQX (50 µM), a blocker of AMPA/KA receptors(Fig. 6a), and CNQX alone did not decrease the number of dendriticbranches when compared with controls at P7-P9 (n = 4 and 4; datanot shown). Conversely, when applied with OT/AVP antagonists,NMDA had no effect on the dendritic branches, even in a high-K⁺ medium (Fig. 6b). These results show that activation of bothNMDA receptors and OT/AVP receptors are needed for increasingthe dendritic arbor.

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Figure 6. OT/AVP and NMDA effects are interdependent. a, Application of OT/AVP had no effect on the number of dendritic branches when NMDA receptors were blocked by MK801, even in the presence of high K⁺. Conversely, AMPA receptor blockade by CNQX did not suppress the increase in the number of dendritic branches induced by OT/AVP. b, Activation of NMDA receptors did not increase the dendritic arbor in the presence of OT/AVP antagonists (OT/AVP Antago.), even in the presence of 12.5 mM K⁺. The number of neurons is indicated in each bar (**p < 0.01; ANOVA).

Acute effect of OT/AVP on synaptic activity

Because a presynaptic action of OT on glutamatergic endings has been described in adults, we tested whether part of the interdependencemay result from a facilitatory effect of the peptides on glutamaterelease. The spontaneous glutamatergic synaptic activity was recordedin slices of P7-P9 rats, a period just after the appearance ofthe first EPSPs. Experiments were initially performed with thepeptides at 1 µM because no presynaptic effects were observedin adults below this concentration (Kombian et al., 1997). In10 of 14 neurons, OT/AVP induced a marked increase in EPSC frequency(Fig. 7a-c). Among the four insensitive neurons, three displayedthe highest mean EPSC frequency, which was decreased (Fig. 7d)by OT/AVP antagonists. This shows that, in some neurons, endogenousOT/AVP exert a maximal increase in synaptic activity, which cannotbe further enhanced by exogenous peptides. The peptides are alsoefficient at 0.1 µM but with smaller effects (42% of the effectof 1 µM on EPSP frequency; n = 3). In four neurons in which OT/AVPinduced the strongest increase in frequency, a 30-100% increasein EPSC amplitude was also observed during OT/AVP application(Fig. 7e). These results suggest a presynaptic action of the peptidesin neurons in which EPSC amplitude was not affected. In the otherneurons, a postsynaptic increase in EPSC amplitude may also beresponsible for the increase in frequency. To test this possibility,and because the NMDA receptor antagonist MK801 (1 µM) did notaffect spontaneous or OT/AVP-evoked EPSCs (n = 3; data not shown),the current evoked by application of kainate (25 µM, 30 sec) wasstudied in control condition and under OT/AVP exposure. In neuronsin which EPSC amplitude was increased by the peptides, the presenceof OT/AVP affected neither the amplitude nor the kinetics of kainate-evokedcurrent (n = 3) (Fig. 7f). This indicates that, even in cellsin which EPSC amplitude was increased, OT/AVP increased synaptictransmission by acting at presynaptic sites. To exclude the possibilitythat OT/AVP acted on the cell body of afferent neurons to increaseelectrical activity and synaptic transmission, the peptides wereapplied in the presence of TTX. TTX (0.3 µM) alone had no effecton spontaneous EPSC frequency and did not affect the increasein frequency induced by OT/AVP (n = 4) (Fig. 7g). Together, theseresults show that, during synaptogenesis, dendritically releasedOT/AVP are able to act on presynaptic endings and increase glutamatergictransmission.

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Figure 7. OT/AVP act presynaptically to increase glutamatergic transmission. a, Spontaneous EPSCs recorded at $-$ 60 mV, in the presence of the GABA_A receptor antagonist GABAzine (3 µM), in a neuron of a P8 rat in control condition and during OT/AVP application. b, Graph of the mean cumulative probability showing an increase in EPSCs frequency during OT/AVP application (Kolmogorov-Smirnov test; p < 0.0001). c, Mean effects of OT/AVP on EPSC frequency for the 10 neurons in which the frequency was increased by the peptides. d, Effect of OT/AVP antagonists in three neurons not affected by OT/AVP, demonstrating the implication of endogenous peptides on EPSCs frequency. e, In four neurons in which OT/AVP induced the strongest increase in EPSCs frequency, an increase in EPSC amplitude was also observed. In these neurons, the effect on EPSC amplitude appears to be presynaptic because OT/AVP did not affect kainate (KA; 25 µM)-evoked current (f). g, OT/AVP did not act by increasing electrical activity of presynaptic neurons because their effect on EPSC frequency was not affected by TTX (0.3 µM).

Putative role of OT/AVP on synaptogenesis

The role of OT/AVP in increasing the dendritic arbor and glutamate release suggests an important function of these peptidesin glutamatergic synapse establishment. To test this hypothesis,OT/AVP receptors were blocked by daily injection of OT/AVP antagonistsduring a period expected to overlap the one of glutamatergic synapseestablishment (P3-P17). The spontaneous glutamatergic synapticactivity was then recorded at P21-P23 in acute horizontal slicesof saline- or antagonists-treated rats (Fig. 8a). This treatmenthad no effect on the amplitude of glutamatergic EPSCs (Fig. 8b,c)but significantly reduced their frequency (Fig. 8d,e). The moststraightforward explanation is that the number of synapses orthe neurotransmitter release probability was decreased. This resultsupports the idea that OT/AVP receptors indeed play an importantrole in synaptogenesis of glutamatergic inputs.

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Figure 8. OT/AVP antagonists treatment during development decreases spontaneous glutamatergic synaptic activity in young adults. a, Spontaneous EPSCs recorded at $-$ 60 mV in the presence of gabazin in neurons of a P23 control rat and a P23 OT/AVP antagonists-treated rat. b, Graph of the mean cumulative probability for the amplitude of the EPSCs showing that the curves in control and treated rats are superposed. c, The absence of effect was confirmed by the mean amplitude for all EPSCs that was not affected in treated rats (T) compared with control (C). Conversely, the cumulative probability curves for the instantaneous frequency were significantly different between control and treated rats (d) [Kolmogorov-Smirnov test (K.S.); p < 0.0098], as well as the mean frequency of all EPSC (e) (n = 11 in both conditions; *p < 0.05; ANOVA).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study shows that the transient increase in the dendritic arbor of developing SON neurons is supported by a coordinatedaction of OT/AVP released by the dendrites themselves and glutamateprobably released by incoming afferents. However, some glial cellsare known to release glutamate (Parpura and Haydon, 2000), andthis possibility cannot be excluded. The action of these transmittersprobably requires electrical activity, influx of calcium throughvoltage-activated channels, and mobilization of intracellularstores. The peptides are also able to act on presynaptic endingsand increase glutamate release, and they are probably requiredfor normal synaptogenesis, because chronic OT/AVP receptor blockageduring development decreases the frequency of spontaneous synapticEPSCs in youngadults.

Events involved in the increase in the dendritic arbor

The transient increase in dendritic arbor of SON neurons appears to be a complex phenomenon (Fig. 9). The peptides OT/AVP,released at dendritic sites, play a determinant role in this plasticity.Application of exogenous peptides had maximal effects at P3-P6,whereas endogenous peptides are mostly involved at P7-P9, suggestingthat endogenous OT/AVP release is low at P3-P6, whereas receptorsand mechanisms involved in dendritic growth are already present.Although the roles of OT and AVP were not studied separately,it is probable that they act in a similar manner on their respectiveneurons. Both peptides act specifically on their secreting neuronswith similar depolarizing actions and facilitatory effects ontheir own release during development (Chevaleyre et al., 2000),and both lead to mobilization of intracellular Ca²⁺ in adult neurons (Dayanithi et al., 2000). These results supportthe hypothesis that OT and AVP may be directly involved in thedendritic morphology changes (Stern and Armstrong, 1998) and ultrastructuralreorganization (Theodosis et al., 1986) observed in mature SONduring lactation.

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Figure 9. Hypothetical model of the OT/AVP and NMDA action on dendritic arbor. OT/AVP (black triangles) are released at a dendritic level and increase electrical activity and their own dendritic release, mostly during the second postnatal week. This autocontrol loop is involved in the transient increase in dendritic arbor, possibly by increasing intracellular Ca²⁺ stores mobilization. NMDA receptor activation is also involved in the increase in dendritic arbor, probably by promoting Ca²⁺ influx. Electrical activity seems also to be involved in increasing the dendritic arbor, independently of increasing endogenous peptides release, and may act by triggering Ca²⁺ influx via voltage-gated Ca²⁺ channels. All of these events appear to be implicated in the increase in the number of dendritic branches, showing that presynaptic glutamate release and postsynaptic OT/AVP release are needed to increase the dendritic arbor. The peptides are also able to act on presynaptic endings and increase glutamate release. When OT/AVP receptors are blocked during development, the spontaneous glutamatergic synaptic activity is reduced in young adults, indicating a decrease in the number of synapses or in the probability of spontaneous glutamate release. Another hypothesis is that both OT/AVP and NMDA receptor activation are needed for increasing vesicle exocytosis that releases other molecules than OT/AVP involved in the increase in dendritic branches. Glu, Glutamate; NMDAR, NMDA receptors; Ret, reticulum.

Another major component involved in the control of dendritic arbor is NMDA receptor activation by glutamate release. NMDAreceptors regulate dendritic growth during development of neuronsin Xenopus (Rajan and Cline, 1998; Li et al., 2000), chick (Wonget al., 2000), mouse (Inglis et al., 1998), rat (Kalb, 1994),and cat (Bodnarenko and Chalupa, 1993) and may do so by activatingmembers of the Rho family GTPases (Li et al., 2000; Wong et al.,2000). In the SON, NMDA and MK801 had similar effects as OT/AVPand their antagonists, respectively. NMDA was mostly effectiveat P3-P6, whereas MK801 had a significant effect only at P7-P9.Glutamate action is probably mediated by the Ca²⁺ influx evoked by NMDA receptor activation because blockade ofAMPA/KA receptors, generally non-Ca²⁺ permeable, did not prevent the increase in the number of dendriticbranches.

Electrical activity also appears to be involved in dendritic plasticity. TTX prevented OT/AVP and NMDA actions on the dendriticarbor at P3-P6 and decreased the number of branches at P7-P9.TTX effects are probably not a consequence of a decrease in glutamaterelease because spontaneous and OT/AVP-evoked EPSCs were not affectedby TTX. TTX may have decreased endogenous peptides release, butincreasing exogenous peptides concentration by a factor up to100 did not restore the increase in dendritic branches. Althoughwe cannot be sure that even high concentration of exogenous peptidesefficiently counteract a putative decrease in endogenous release,this suggests that electrical activity is involved in increasingthe dendritic arbor, independently of increasing endogenous peptidesrelease. However, electrical activity alone is not sufficientbecause the high-K⁺-induced increase in dendritic branches was prevented when OT/AVPand NMDA receptors were blocked. One putative role for activitycould be to increase Ca²⁺ influx viaVGCCs.

Because activation of both OT/AVP and NMDA receptors is required for increasing dendritic arbor, our results indicate thatan interplay between glutamate release and dendritic peptide releaseis involved in this plasticity. It is not known whether the retrogradeaction of the peptides is required in this process, but it couldexplain part of the interdependence between OT/AVP and NMDA actions.However, because dendrites display a rapid rate of branch additionand retraction during development, an important issue that remainsto be elucidated is whether OT/AVP and NMDA acted by increasingdendritic extension or by decreasing dendriticretraction.

Retrograde action of OT/AVP and roles in synaptogenesis

Just after the appearance of the first EPSPs at the end of PW1 (Chevaleyre et al., 2001), EPSC frequency was increased byOT/AVP or decreased by their antagonists in almost all neuronstested. Because EPSC amplitude was affected in only some of theseneurons and kainate-induced currents were not affected by OT/AVP,the peptides probably acted at a presynaptic site. The increasein amplitude sometime accompanying frequency enhancement may resultfrom intraterminal Ca²⁺ store mobilization after OT/AVP application, leading to concomitantexocytosis of several vesicles within a release site or betweenseveral release sites of the same terminal. Such shared synapseshave been described in adult SON and increase in number duringphysiological plasticity (Theodosis et al., 1995, 1998; Hatton,1997). A modulatory action of OT and AVP on glutamatergic transmissionhas been described previously in adult SON (Kombian et al., 1997,2000). However, both peptides acted by decreasing synaptic transmissionin adults, revealing that the effect of OT/AVP on glutamatergicsynaptic activity undergoes a developmental switch, from facilitatoryto inhibitory. By increasing the dendritic arbor and glutamaterelease, the peptides may act at different steps of synaptogenesis.If OT/AVP receptors are already expressed before contact betweenpresynaptic and postsynaptic elements, the peptides may eitherexert an attractive effect or act as a stop signal on growth cones.An indirect action by allowing a transient increase in the dendriticarbor is also expected. Dendritic extensions display a high mobilityduring synaptogenesis and play an important role in this process(Cline, 2001). Whether or not synapses are formed on the transientdendritic branches remains to be determined. However, transientdendrites may favor interactions with incoming axons, allowingthem to form synapses on stable dendrites. Finally, the peptides,by increasing synaptic strength, may favor the maintenance ofsynaptic contact. Neurotrophins or membrane-permeant molecules,such as arachidonic acid or nitric oxide, have been shown to actas retrograde messengers during synaptic plasticity and synaptogenesis(Fitzsimonds and Poo, 1998). Our results indicate that dendriticneuropeptide release also has a retrograde effect on glutamatergicendings during synaptogenesis. Whatever the exact mode of actionof OT/AVP, the fact that chronic blockade of OT/AVP receptorsduring this period decreased the frequency of spontaneous EPSCsin slices of young adults further argue in favor of a role ofthe peptides in glutamatergic synapse establishment. The decreasein frequency may result from either a change in presynaptic propertiesor most probably a decrease in the number of activesynapses.

In conclusion, our results show that glutamate release, probably by incoming afferents, and dendritic neuropeptide releaseare both required for the transient increase in the dendriticarbor during development of SON neurons. A developmental rolefor OT and AVP has been suggested previously (Carter et al., 1993)because several brain areas display a transient increase in OT/AVPreceptors during development (Tribollet et al., 1991a,b) and AVPincreases neurite outgrowth in Xenopus (Brinton and Gruener, 1987)and rat hippocampal and cortical cultured neurons (Brinton etal., 1994; Chen et al., 2000; Tarumi et al., 2000). However, directevidence for a neurotrophic role of endogenous peptides was lacking.Here we show that, during development, OT/AVP are involved indendritic plasticity of their secreting neurons and probably playan important role in synaptogenesis, particularly by acting retrogradelyon glutamatergicendings.

  FOOTNOTES

Received Feb. 26, 2001; revised Sept. 19, 2001; accepted Oct. 19, 2001.

This work was supported in part by Hoechst-Marrion-Roussel Grant 751285/00. We thank N. C. Spitzer for careful reading andcorrection of this manuscript. This work benefited from fruitfuldiscussions with N. Hussy, G. Alonso, and A. Rabié and theirsuggestions concerning thismanuscript.
Correspondence should be addressed to Michel G. Desarménien, Centre National de la Recherche Scientifique Unité Mixte deRecherche 5101, Biologie des Neurones Endocrines, 141 rue de laCardonille, 34094 Montpellier Cedex 5, France. E-mail: mgdesa{at}ccipe.montp.inserm.fr.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Bodnarenko SR, Chalupa LM (1993) Stratification of ON and OFF ganglion cell dendrites depends on glutamate-mediated afferent activity in the developing retina. Nature 364:144-146[Medline].
Brinton RD, Monreal AW, Fernandez JG (1994) Vasopressin-induced neurotrophism in cultured hippocampal neurons via V1 receptor activation. J Neurobiol 25:380-394[Web of Science][Medline].
Brinton RE, Gruener R (1987) Vasopressin promotes neurite growth in cultured embryonic neurons. Synapse 1:329-334[Web of Science][Medline]. [Erratum (1988) 2:107]
Carter DA, Fai CK, Murphy D (1993) Neurohypophyseal peptides as regulators of growth and development. A review. J Mol Neurosci 4:11-19[Web of Science][Medline].
Chen Q, Patel R, Sales A, Oji G, Kim J, Monreal AW, Brinton RD (2000) Vasopressin-induced neurotrophism in cultured neurons of the cerebral cortex: dependency on calcium signaling and protein kinase C activity. Neuroscience 101:19-26[Web of Science][Medline].
Chevaleyre V, Dayanithi G, Moos FC, Desarménien MG (2000) Developmental regulation of a local positive autocontrol of supraoptic neurons. J Neurosci 20:5813-5819[Abstract/Free Full Text].
Chevaleyre V, Moos FC, Desarménien MG (2001) Correlation between electrophysiological and morphological characteristics during maturation of rat supraoptic neurones. Eur J Neurosci 13:1136-1146[Web of Science][Medline].
Cline HT (2001) Dendritic arbor development and synaptogenesis. Curr Opin Neurobiol 11:118-126[Web of Science][Medline].
Dayanithi G, Sabatier N, Widmer H (2000) Intracellular calcium signalling in magnocellular neurones of the rat supraoptic nucleus: understanding the autoregulatory mechanisms. Exp Physiol 85:75S-84S[Abstract].
Fitzsimonds RM, Poo MM (1998) Retrograde signaling in the development and modification of synapses. Physiol Rev 78:143-170[Abstract/Free Full Text].
Hatton GI (1990) Emerging concepts of structure-function dynamics in adult brain: the hypothalamo-neurohypophysial system. Prog Neurobiol 34:437-504[Web of Science][Medline].
Hatton GI (1997) Function-related plasticity in hypothalamus. Annu Rev Neurosci 20:375-397[Web of Science][Medline].
Hussy N, Boissin-Agasse L, Richard P, Desarménien MG (1997) NMDA receptor properties in rat supraoptic magnocellular neurons: characterization and postnatal development. Eur J Neurosci 9:1439-1449[Web of Science][Medline].
Inglis FM, Furia F, Zuckerman KE, Strittmatter SM, Kalb RG (1998) The role of nitric oxide and NMDA receptors in the development of motor neuron dendrites. J Neurosci 18:10493-10501[Abstract/Free Full Text].
Jontes JD, Buchanan J, Smith SJ (2000) Growth cone and dendrite dynamics in zebrafish embryos: early events in synaptogenesis imaged in vivo. Nat Neurosci 3:231-237[Web of Science][Medline].
Kalb RG (1994) Regulation of motor neuron dendrite growth by NMDA receptor activation. Development 120:3063-3071[Abstract].
Kirov SA, Sorra KE, Harris KM (1999) Slices have more synapses than perfusion-fixed hippocampus from both young and mature rats. J Neurosci 19:2876-2886[Abstract/Free Full Text].
Koester SE, O'Leary DD (1994) Development of projection neurons of the mammalian cerebral cortex. Prog Brain Res 102:207-215[Medline].
Kombian SB, Mouginot D, Pittman QJ (1997) Dendritically released peptides act as retrograde modulators of afferent excitation in the supraoptic nucleus in vitro. Neuron 19:903-912[Web of Science][Medline].
Kombian SB, Mouginot D, Hirasawa M, Pittman QJ (2000) Vasopressin preferentially depresses excitatory over inhibitory synaptic transmission in the rat supraoptic nucleus in vitro. J Neuroendocrinol 12:361-367[Web of Science][Medline].
Lendvai B, Stern EA, Chen B, Svoboda K (2000) Experience-dependent plasticity of dendritic spines in the developing rat barrel cortex in vivo. Nature 404:876-881[Medline].
Li Z, Van Aelst L, Cline HT (2000) Rho GTPases regulate distinct aspects of dendritic arbor growth in Xenopus central neurons in vivo. Nat Neurosci 3:217-225[Web of Science][Medline].
Nelson EE, Alberts JR, Tian Y, Verbalis JG (1998) Oxytocin is elevated in plasma of 10-day-old rats following gastric distension. Brain Res Dev Brain Res 111:301-303[Medline].
Parpura V, Haydon PG (2000) From the cover: physiological astrocytic calcium levels stimulate glutamate release to modulate adjacent neurons. Proc Natl Acad Sci USA 97:8629-8634[Abstract/Free Full Text].
Purpura DP (1975) Dendritic differentiation in human cerebral cortex: normal and aberrant developmental patterns. Adv Neurol 12:91-134[Web of Science][Medline].
Rajan I, Cline HT (1998) Glutamate receptor activity is required for normal development of tectal cell dendrites in vivo. J Neurosci 18:7836-7846[Abstract/Free Full Text].
Stern JE, Armstrong WE (1998) Reorganization of the dendritic trees of oxytocin and vasopressin neurons of the rat supraoptic nucleus during lactation. J Neurosci 18:841-853[Abstract/Free Full Text].
Tarumi T, Sugimoto Y, Chen Z, Zhao Q, Kamei C (2000) Effects of metabolic fragments of [Arg(8)]-vasopressin on nerve growth in cultured hippocampal neurons. Brain Res Bull 51:407-411[Web of Science][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, el Majdoubi M, Gies U, Poulain DA (1995) Physiologically-linked structural plasticity of inhibitory and excitatory synaptic inputs to oxytocin neurons. Adv Exp Med Biol 395:155-171[Medline].
Theodosis DT, El Majdoubi M, Pierre K, Poulain DA (1998) Factors governing activity-dependent structural plasticity of the hypothalamoneurohypophysial system. Cell Mol Neurobiol 18:285-298[Web of Science][Medline].
Tribollet E, Goumaz M, Raggenbass M, Dreifuss JJ (1991a) Appearance and transient expression of vasopressin and oxytocin receptors in the rat brain. J Recept Res 11:333-346[Medline].
Tribollet E, Goumaz M, Raggenbass M, Dubois-Dauphin M, Dreifuss JJ (1991b) Early appearance and transient expression of vasopressin receptors in the brain of rat fetus and infant. An autoradiographical and electrophysiological study. Brain Res Dev Brain Res 58:13-24[Medline].
Ugrumov MV (1992) Development of the hypothalamic monoaminergic system in ontogenesis. Morpho-functional aspects. Zool Sci Tokyo 9:37-45.
van den Pol AN, Wuarin JP, Dudek FE (1990) Glutamate, the dominant excitatory transmitter in neuroendocrine regulation. Science 250:1276-1278[Abstract/Free Full Text].
Wong WT, Faulkner-Jones BE, Sanes JR, Wong RO (2000) Rapid dendritic remodeling in the developing retina: dependence on neurotransmission and reciprocal regulation by Rac and Rho. J Neurosci 20:5024-5036[Abstract/Free Full Text].

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