Neuronal Activity and Brain-Derived Neurotrophic Factor Regulate the Density of Inhibitory Synapses in Organotypic Slice Cultures of Postnatal Hippocampus

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (86)

Citing Articles via Google Scholar

Google Scholar

Articles by Marty, S.

Articles by Sotelo, C.

Search for Related Content

PubMed

PubMed Citation

Articles by Marty, S.

Articles by Sotelo, C.

Pubmed/NCBI databases
Compound via MeSH
Substance via MeSH

Previous Article  |  Next Article

The Journal of Neuroscience, November 1, 2000, 20(21):8087-8095

Neuronal Activity and Brain-Derived Neurotrophic Factor Regulate the Density of Inhibitory Synapses in Organotypic Slice Cultures of Postnatal Hippocampus
Serge Marty, Rosine Wehrlé, and Constantino Sotelo
Institut National de la Santé et de la Recherche Médicale U106, Hôpital de la Salpêtrière, Pavillon de l'Enfance et de l'Adolescence, 75651 Paris cedex 13, France

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Hippocampal interneurons inhibit pyramidal neurons through the release of the neurotransmitter GABA. Given the importanceof this inhibition for the proper functioning of the hippocampus,the development of inhibitory synapses must be tightly regulated.In this study, the possibility that neuronal activity and neurotrophinsregulate the density of GABAergic inhibitory synapses was investigatedin organotypic slice cultures taken from postnatal day 7rats.
In hippocampal slices cultured for 13 d in the presence of the GABA_A receptor antagonist bicuculline, the density of glutamicacid decarboxylase (GAD) 65-immunoreactive terminals was increasedin the CA1 area when compared with control slices. Treatment withthe glutamate receptor antagonist 6,7-dinitroquinoxaline-2,3-dionedecreased the density of GAD65-immunoreactive terminals in thestratum oriens of CA1. These treatments had parallel effects onthe density of GABA-immunoreactive processes. Electron microscopicanalysis after postembedding immunogold labeling with antibodiesagainst GABA indicated that bicuculline treatment increased thedensity of inhibitory but not excitatory synapses. Applicationof exogenous BDNF partly mimicked the stimulatory effect of bicucullineon GAD65-immunoreactive terminals. Finally, antibodies againstBDNF, but not antibodies against nerve growth factor, decreasethe density of GAD65-immunoreactive terminals in bicuculline-treatedslices.
Thus, neuronal activity regulates the density of inhibitory synapses made by postnatal hippocampal interneurons, and BDNFcould mediate part of this regulation. This regulation of thedensity of inhibitory synapses could represent a feedback mechanismaimed at maintaining an appropriate level of activity in the developinghippocampalnetworks.

Key words: rat; development; Ammon's horn; GABAergic neurons; interneurons; neurotrophins

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Hippocampal interneurons inhibit pyramidal cells through the release of the neurotransmitter GABA (Freund and Buzsáki, 1996).According to their axonal projection and neurochemical characteristics,the interneurons can be classified into several subgroups (Freundand Buzsáki, 1996). Interneurons innervating the cell body ofpyramidal neurons may exert the inhibitory effect by suppressingsodium-dependent action potentials, whereas interneurons innervatingthe dendrites of pyramidal neurons may suppress calcium-dependentdendritic spikes (Miles et al., 1996).

There is an important maturation of hippocampal excitatory transmission during the postnatal period. Non-NMDA glutamatergictransmission becomes prominent at the end of the first postnatalweek, simultaneous with the establishment of the hyperpolarizingeffects of GABA (Ben-Ari et al., 1989, 1997; Hosokawa et al.,1994; Durand et al., 1996; Petralia et al., 1999). The first postnatalmonth is also characterized by an increase in the number of excitatorysynapses (Steward and Falk, 1991). Thus, the number and/or efficiencyof inhibitory synapses may also increase during the postnatalperiod to adjust the strength of inhibition to counter the increasednumber of excitatorysynapses.

Neuronal activity is a good candidate to regulate the development of inhibitory synapses. After chronic blockade of neuronalactivity in cortical cell cultures, the transfer to control mediumresults in an increased activity likely attributable to, at leastin part, a decrease of GABA-mediated inhibition (Rutherford etal., 1997). The neurotrophin brain-derived neurotrophic factor(BDNF) might mediate this activity-dependent modulation of synapticinhibition. BDNF is synthesized and released by pyramidal neuronsin an activity-dependent manner (Thoenen, 1995). BDNF treatmentprevents the decrease of GABA-mediated inhibition during chronicblockade of neuronal activity (Rutherford et al., 1997). Furthermore,downregulation of BDNF in hippocampal cultures reduces the frequencyof miniature IPSCs (Murphy et al., 1998). However, these experimentsdo not discriminate between the effects of neuronal activity andBDNF on either the efficacy or the number of inhibitory synapses.The hypothesis of a presumptive control of the number of inhibitorysynapses by neuronal activity has been evaluated previously inultrastructural studies. For instance, in organotypic cerebellarcultures, neuronal activity exerts its effects on synaptic inhibitionby increasing the number of inhibitory synapses (Seil et al.,1994), and this regulation seems to be mediated by BDNF (Seil,1999). Control of the number of inhibitory synapses by neuronalactivity also occurs in the somatosensory cortex in vivo, becausesensory deprivation during development causes a specific decreasein the number of GABAergic synapses in the rat barrel field cortex(Micheva and Beaulieu, 1995).

The present study was undertaken to determine whether neuronal activity and BDNF can regulate the density of inhibitory synapsesmade by postnatal hippocampal interneurons. Organotypic slicecultures of the hippocampus were used, because both excitatorytransmission and BDNF expression mature in the slices with a similartime course to that seen in vivo (Buchs et al., 1993; Försteret al., 1993; Muller et al., 1993). Slices were taken from 7-d-oldrats, when GABAergic transmission becomes hyperpolarizing andnon-NMDA glutamatergic transmission is established (Ben-Ari etal., 1997). Endogenous neuronal activity was manipulated by chronicapplication of antagonists of either GABA_A or non-NMDA glutamatereceptors. The effects of these treatments on GABAergic synapseswere evaluated with light microscopy, using antibodies againstGABA or the GABA-synthesizing enzyme glutamic acid decarboxylase(GAD) 65 and ultrastructurally with the postembedding immunogoldlabeling with antibodies against GABA. The quantitative resultsindicate that neuronal activity regulates the density of inhibitorysynapses made by postnatal hippocampal interneurons and that BDNFcould mediate part of thisprocess.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Slice culture. Hippocampal slice cultures were prepared according to the method developed by Stoppini et al. (1991), exceptthat a defined medium was used. Seven-day-old Wistar rats (IffaCredo, L'arbresle, France) were decapitated, and their brainswere rapidly removed. Hippocampi were dissected in Gey's balancedsalt solution (catalog #24260-028; Life Technologies, Cergy Pontoise,France) with 5 mg/ml glucose under sterile conditions. Slices,350-µm-thick, were cut perpendicular to the septotemporal axisof the hippocampus using a McIllwain tissue chopper (Mickle Laboratory,Surrey, UK). Hippocampal slices were first transferred into theculture medium, separated, and ultimately transferred onto Millicell-CMmembranes (Millipore, St. Quentin Yvelines, France). Twelve adjacentslices were obtained per brain. Adjacent slices were transferredonto different Millicells to compare the effects of the treatmentswith adjacent controlmaterial.

The Millicell membranes were kept above 750 µl of defined medium in six-well plates. The medium consisted of minimum essentialmedium (catalog #11012-010; Life Technologies), 1% D-glucose,5 mM Tris-HCl, 100 µg/ml bovine serum albumin (BSA), 100 µg/mltransferrin, 16 ng/ml putrescin, 40 ng/ml Na-selenium, 30 ng/mltri-iodothyronin, 5 µg/ml insulin, and 60 ng/ml progesterone.All chemicals were purchased from Sigma (St. Quentin Fallavier,France). Slices were incubated at 35°C in 5% CO₂. The medium wasexchanged every second or thirdday.

Pharmacological treatments. To manipulate neuronal activity in the slices, either 10 µM of the GABA_A receptor antagonist bicuculline(Sigma) or 20 µM of the non-NMDA glutamate receptor antagonist6,7-dinitroquinoxaline-2,3-dione (DNQX) (Sigma) were added tothe medium during the 13 d of the cultivationperiod.

One microliter of recombinant human BDNF (Chemicon, Temecula, CA) at a dilution of 100 ng/µl in PBS (catalog #14200-067; LifeTechnologies) containing 0.1% BSA (Sigma) was applied directlyon top of each slice as described previously (Marty et al., 1996).The neurotrophin was applied twice to the slices at 7 and 10 DIV,after exchange of the medium. Recombinant human neurotrophin-3(NT-3) (Upstate Biotechnology, Lake Placid, NY) at a dilutionof 100 ng/µl in PBS containing 0.1% BSA was applied as describedabove for BDNF. The neurotrophins were applied to untreated orDNQX-treated slices. In this last case, adjacent slices treatedwith DNQX only were used as controls. One microliter of PBS containing0.1% BSA was applied to control slices as described above fortheneurotrophins.

Antibodies against BDNF (50 µg/ml) (which is considered as specific by the provider; catalog #G1641; Promega, Madison, WI)or antibodies against nerve growth factor (NGF) [a gift of Dr.Yves-Alain Barde (Max-Planck-Institute, Martinsried, Germany)]were added to the medium during the 13 d in culture. The mediumcontaining the antibodies was exchanged every second or thirdday. The antibodies were added to bicuculline-treated slices,and adjacent slices treated with bicuculline alone were used ascontrols.

Immunohistochemistry for light microscopy. After 13 d in culture, control and adjacent treated slices were fixed for 1.5 hrin 4% paraformaldehyde in phosphate buffer (0.12 M PBS, pH 7.4)at 4°C, rinsed several times in PBS, and incubated for 1 hr in0.12 M phosphate buffer, pH 7.4, containing 0.9% NaCl, 0.25% TritonX-100, 0.1% gelatin, 0.1% sodium azide (PBSGTA), and lysine (0.1M). The slices were then incubated overnight with antibodies raisedagainst GAD65 [1:1000; GAD-6, this monoclonal antibody developedby D. I. Gottlieb (Washington University School of Medicine, St.Louis, MO) was obtained from the Developmental Studies HybridomaBank developed under the auspices of the National Institute ofChild Health and Human Development and maintained by the Universityof Iowa, Department of Biological Sciences (Iowa City, IA)] orGABA (1:2000; rabbit polyclonal antibodies A-2052; Sigma) dilutedin PBSGTA. After washes, the slices were incubated for 3 hr witha solution containing either goat anti-mouse or goat anti-rabbitCY3 (1:1000; Jackson ImmunoResearch, West Grove, PA). After washes,the slices were mounted in mowiol (Calbiochem, La Jolla, CA),examined, and photographed with a Zeiss (Oberkochen, Germany)Axiophot.

Quantification of the density of GAD65-immunoreactive puncta and GABA-immunoreactive processes in the CA1 area. Immunofluorescencewas observed with a Zeiss LSM 410 confocal microscope, using 543nm excitation wavelength and 570 nm emission wavelength. The explantswere observed with the 63×/1.4 numerical aperture lens (Plan-Apochromat;Zeiss). The pinhole was set at 20, and the resolution was 0.75µm on z-axis. Confocal sections of the labeling were obtainedevery 1 µm in the middle of the hippocampal slices in the CA1region. The labeling was present in 10-15 µm in the thicknessof the slices. For GAD65 immunoreactivity, three areas were sampled,in the stratum oriens, the stratum pyramidale, and the stratumradiatum. For GABA immunoreactivity, only the stratum oriens wassampled because of the poor quality of labeling in the other areasof the CA1 subfield. Three-dimensional reconstructions of theseconfocal sections were then obtained using LSM software (Zeiss)and printed at a magnification of 880×.

For quantification of the density of GAD65-immunoreactive puncta or of GABA-immunoreactive processes, a 36 cm² square with a lattice of puncta spaced by 0.5 cm was appliedover the prints of the three-dimensional reconstructions. Thenumber of points of the lattice hitting the elements of interestwas then counted to determine the density of these elements (Gundersenet al., 1988). For each treatment, counts were performed blindlyin slices taken from three to five animals. For each animal, twoor three slices were used as control, and two or three adjacentslices were treated. At least two independent experiments weredone for each experimental condition. The mean of the values wascalculated for each animal for either the control or the treatedslices. The mean value, SD, and SEM were then calculated fromthese mean values obtained with different animals. Because wewere interested in the effects of the treatments relative to controlsrather than in absolute values, these mean values are presentedas percentages of control values, together with the SEM. The numberof animals for each condition is indicated below each bar of thehistograms in the figures. Comparison between the mean valuesof control and treated slices was performed by statistical analysisusing the two-tailed unpaired Student's ttest.

Postembedding immunohistochemistry. After 13 DIV, the culture medium of control and treated slices was exchanged for a solutioncontaining 3/4 vol of culture medium-1/4 vol of fixative (1% paraformaldehydeand 2.5% glutaraldehyde in PBS) for 5 min, followed by 1/2 vol ofculture medium-1/2 vol of fixative for 5 min, followed by 1/4 volof culture medium-3/4 vol of fixative for 5 min, followed by fixative.Then the fixative was added also over the slices for 2 hr at 4°C.The slices were then transferred into a solution containing 2%osmium tetroxide for 2 hr. After washes, the slices were staineden bloc with a solution containing 2% uranyl acetate for 45 min.After washes, the slices were dehydrated in graded ethanols andflat embedded in Araldite. For each slice, one block containingthe CA1 area was trimmed out from the middle of the slice. Theseblocks were sectioned with a Reichert-Jung ultramicrotome. Inpreliminary experiments, 1-µm-thick semithin sections were madein 26 control, 10 bicuculline-treated, and 12 DNQX-treated slices.One every 6th, 10th, or 15th section was stained with 0.5% toluidineblue (catalog #1.15930; Merck, Darmstadt, Germany) in 1% di-sodiumtetraborate (catalog #6306; Merck) in distilled water. These preliminaryexperiments indicated that areas of necrosis were not observedin our preparation, that the final thickness of the slices was~180 µm, and that there were no significant differences betweenthe thickness of control and bicuculline- or DNQX-treated slices.Ultrathin sections were collected onto 300 mesh nickel grids ata depth of 90 µm in the thickness of control or bicuculline-treatedslices.

The ultrathin sections were treated for 5 min with 1% periodic acid, washed with ultrapure water, treated with 1% sodium metaperiodate,washed, and incubated 45 min with 5% bovine serum albumin in Tris-bufferedsaline, pH 7.6. After washes, the sections were incubated overnightat 4°C with rabbit polyclonal antibodies against GABA (1:250;catalog #0602; Immunotech, Marseille, France). After washes, thesections were incubated with goat anti-rabbit immunogold conjugatewith 15 nm gold particles (1:10; EM-GAR15; British Bio Cell International,Cardiff, UK) for 1 hr. After rapid washes in ultrapure water,the sections were stained with uranyl acetate and lead citrateand examined with a PhilipsCM100.

Quantification of the density and morphological characteristics of GABA- and non-GABA-immunoreactive synapses in the stratumoriens. Counts of GABA-immunoreactive synapses were performedon sections taken from four animals, with two or three controland two or three adjacent bicuculline-treated slices analyzedper animal. For each slice, only one section was analyzed. Foreach section, two squares of the grid located in the stratum orienswere systematically screened, each square measuring 3969 µm², and the GABAergic synapses that had their synaptic junctionin the plane of the section were counted. Stereological methodswere not used for counting the synapses, because our quantificationwas not intended to obtain absolute values for which other countingmethods are more appropriate (Guillery and Herrup, 1997). Instead,our counts were determined solely to compare relative synapticdensities in treated and control slices. GABAergic presynapticterminals contained synaptic vesicles and gold particles and couldtherefore easily be identified. The synaptic junctions were identifiedby the slight widening of the synaptic cleft and the paralleldisposition of presynaptic and postsynaptic membranes undercoatedby cytoplasmic differentiations (Peters et al., 1991). In threecontrol and three adjacent treated sections, the counts were repeatedblindly. The GABAergic synapses were also photographed at a 27,500×magnification on sections taken from three of the animals usedfor quantification of synaptic number, with three control andthree adjacent bicuculline-treated slices per animal. The electronphotomicrographs were printed at a magnification of 60,000×. Usingthese photomicrographs, the area of the presynaptic terminalsand the length of the synaptic junctions were measured, and thenumber of gold particles was counted. The gold particles in mitochondriawere excluded. The area of presynaptic terminals was measuredby applying a lattice of puncta spaced by 1 cm over the photographs.The number of points overlying presynaptic terminals was countedto determine the area of these terminals (Gundersen et al., 1988).

Counts of non-GABA-immunoreactive synapses were performed on sections taken from three animals, with three control and threeadjacent bicuculline-treated slices analyzed per animal. The countsof non-GABA-immunoreactive synapses were performed blindly inthe squares in which GABAergic synapses were previously counted.Non-GABAergic synapses with a presynaptic terminal containingat least three synaptic vesicles were counted. These non-GABAergicsynapses exhibited a widened synaptic cleft and thicker postsynapticdifferentiations than the GABA-labeled synapses, and they mostprobably belong to excitatory synapses (Peters et al., 1991).An analysis of 84 presynaptic terminals from this type of synapsesindicated that they contained a very low number of gold particles,with a mean value of 0.1 particles/0.03 µm² in control slices and 0.07 particles/0.03 µm² in bicuculline-treatedslices.

Results were obtained in two independent experiments. The distribution of the values from slices of each animal, for eachof the parameters that were analyzed, i.e., area of GABAergicpresynaptic terminals, length of synaptic junctions of GABAergicsynapses, and density of gold particles in GABAergic presynapticterminals, exhibited one clear peak. Furthermore, the distributionof these values was similar in control and bicuculline-treatedslices. The mean of the values was calculated for each animalfor either control or treated sections. The mean value, SD, andSEM were then calculated from these mean values obtained withdifferent animals. Because we were interested in the effects ofthe treatments relative to control rather than in absolute values,these mean values were presented as percentages of control values,together with the SEM. The number of animals is indicated beloweach bar of the histograms in the figures. Comparisons betweenthe mean values of control and treated slices were performed bystatistical analysis using two-tailed, unpaired Student's ttest.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Flattening of hippocampal slices was apparent after 2 d in culture. This flattening increased progressively over time, particularlyat the edge of the slices. Nevertheless, the slices retained theirstructural organization over the incubation period. The pyramidaland dentate granule cell layers remained easily detectable, exceptfor the infra-pyramidal blade of the dentate gyrus, which is generatedat a later date and could not be recognized clearly as a celllayer. Treatment of the slices with bicuculline, DNQX, BDNF, orNT-3 did not induce conspicuous changes either in the size ofthe slices or their organotypic organization. We selected theCA1 area to examine the effects of modifications of neuronal activityor neurotrophin levels on GAD65 immunoreactivity, GABA immunoreactivity,or synapsedensity.

Effects on GAD65 immunoreactivity of treatments with GABA_A or non-NMDA glutamate receptor antagonists, BDNF or NT-3, or antibodies against BDNF or NGF

After 13 DIV, a dense, punctate GAD65 immunolabeling was observed throughout the CA1 area (Fig. 1A,C,E). This punctate immunostainingwas less dense in the stratum pyramidale than in the other layers(Fig. 1E). Scattered GAD65-immunoreactive soma were occasionallyobserved (Fig. 1C,E).

View larger version (177K):
[in this window]
[in a new window]
Figure 1. Effects of bicuculline treatment on GAD65 immunoreactivity. A, C, E, Control slice. B, D, F, Bicuculline-treated slice. A, B, Stratum oriens at the border of the slice. C, D, Middle of the stratum oriens. E, F, Stratum pyramidale (sp) with part of the stratum oriens (so) and part of the stratum radiatum (sr). Arrows point to neuronal cell bodies. Note the increased density of GAD65-immunoreactive puncta after bicuculline treatment, which is particularly evident in the stratum oriens. Scale bar, 40 µm.

In bicuculline-treated slices, an increase in the density of GAD65-immunoreactive puncta was evident in all layers (Fig. 1B,D,F),although it was more prominent in the stratum oriens. Quantificationof the density of GAD65-immunoreactive puncta indicated a 133%increase in the stratum oriens, a 42% increase in the stratumpyramidale, and a 32% increase in the stratum radiatum (Fig. 2A-C).

View larger version (31K):
[in this window]
[in a new window]
Figure 2. Histograms illustrating the effects of bicuculline and DNQX treatments on the density of GAD65-immunoreactive puncta. Results are presented as percentages of controls (white bars). n, Number of animals; Bic., bicuculline. *p < 0.05; **p < 0.01.

In DNQX-treated slices, a decrease in the density of GAD65-immunoreactive puncta was observed in the stratum oriens (Fig.3A-D). Quantification of this density revealed a 38% decreasein the stratum oriens, whereas no significant decreases were observedin the stratum pyramidale or in the stratum radiatum (Fig. 2A-C).

View larger version (105K):
[in this window]
[in a new window]
Figure 3. Effects of DNQX treatment on GAD65 immunoreactivity. A, C, Control slice. B, D, DNQX-treated slice. A, B, Stratum oriens at the border of the slice. C, D, Middle of the stratum oriens. so, Stratum oriens; sp, stratum pyramidale. Note the decreased density of GAD65-immunoreactive puncta in the stratum oriens after DNQX treatment. Scale bar, 40 µm.

In slices treated with BDNF during the last 6 DIV, the density of GAD65-immunoreactive puncta increased in the stratum oriens.Quantification of the density of these puncta indicated a 63%increase in the stratum oriens (Fig. 4A). BDNF has been shownto facilitate excitatory transmission (Berninger and Poo, 1996;Schuman, 1999). To exclude the possibility that the effects ofBDNF on the density of GAD65-immunoreactive puncta could arisefrom a direct increase in excitatory transmission, BDNF was appliedto DNQX-treated slices. Under these conditions, the density ofGAD65-immunoreactive puncta was also increased in the stratumoriens (43%) when compared with the stratum oriens of DNQX-treatedslices that received BSA only (Fig. 4B). However, stimulationwith NT-3 did not affect the density of GAD65-immunoreactive punctain the stratum oriens of DNQX-treated slices (Fig. 4C).

View larger version (23K):
[in this window]
[in a new window]
Figure 4. Quantification of the effects of treatments with BDNF or NT-3 and with antibodies against BDNF or NGF on the density of GAD65-immunoreactive puncta in the stratum oriens. A, Untreated slices. B, C, DNQX-treated slices. D, E, Bicuculline-treated slices. Results are presented as percentages of controls (white bars). n, Number of animals; Bic., bicuculline. *p < 0.05; **p < 0.01.

In bicuculline-treated slices that received in addition antibodies against BDNF, the density of GAD65-immunoreactive punctawas decreased in the stratum oriens when compared with adjacentslices treated only with bicuculline. Quantification of the densityof these puncta indicated a 38% decrease in the stratum oriens(Fig. 4D). On the other hand, addition of antibodies against NGFdid not affect the density of GAD65-immunoreactive puncta in thestratum oriens of bicuculline-treated slices (Fig. 4E).

Effects of treatments with GABA_A and non-NMDA glutamate receptor antagonists on GABA immunoreactivity

In cultures stained with anti-GABA antibodies, immunoreactivity was very dense and not restricted to punctated elements. Inaddition, despite the use of confocal microscopy, immunostainedstructures were sharply defined only in the thinnest regions,i.e., at the borders of the slices, containing the stratum oriens(Fig. 5). In thicker slice regions, containing the strata pyramidaleand radiatum, the immunolabeling was somewhat blurred and variable,probably because of the large amounts of GABA present in the thickpart of the slices and its presumed leakage during fixation. Assuch, quantitative analyses were therefore restricted to the stratumoriens.

View larger version (127K):
[in this window]
[in a new window]
Figure 5. Effects of bicuculline treatment on GABA immunoreactivity. A, C, Control slice. B, D, Bicuculline-treated slice. A, B, Stratum oriens at the border of the slice. Brackets delineate a bundle of thin processes. Arrowheads point to thick processes. C, D, Middle of the stratum oriens. Arrows point to cell bodies. Note the increased density of GABA-immunoreactive processes after bicuculline treatment. Scale bar, 20 µm.

In control slices after 13 DIV, a dense network of labeled processes was observed in the stratum oriens (Fig. 5A,C). At theperiphery of the slices, the network consisted of a bundle ofthin, varicose, parallel processes (Fig. 5A), whereas such thin,varicose processes ran in every direction in the middle of thestratum oriens (Fig. 5C). Other labeled processes were also distinguished,which were thicker and tapered along their course (Fig. 5A). Faintlystained cell bodies were also observed (Fig. 5A,C).

In bicuculline-treated slices, an overall increase in the density of GABAergic processes occurred in both the peripheral parallelbundle and the middle of the stratum oriens (Fig. 5B,D). Therewas no increase in the staining intensity of cell bodies (Fig.5C,D). Quantification of the density of GABA-immunoreactive processesindicated a 29% increase in the stratum oriens (Fig. 6A).

View larger version (14K):
[in this window]
[in a new window]
Figure 6. Quantification of the effects of bicuculline and DNQX treatments on the density of GABA-immunoreactive processes in the stratum oriens. Results are presented as percentages of controls (white bars). n, Number of animals; Bic., bicuculline. *p < 0.05; **p < 0.01.

In DNQX-treated slices, a decrease in the density of GABAergic processes was observed both at the border and in the middleof the stratum oriens (Fig. 7A-D). This decrease coexisted withan increase in the intensity of immunostaining of thick processesand cell bodies (Fig. 7B,D). Quantification of the density ofGABA-immunoreactive processes indicated a 31% decrease in thestratum oriens (Fig. 6B).

View larger version (159K):
[in this window]
[in a new window]
Figure 7. Effects of DNQX treatment on GABA immunoreactivity. A, C, Control slice. B, D, DNQX-treated slice. A, B, Stratum oriens at the border of the slice. C, D, Middle of the stratum oriens. Arrowheads point to thick processes; arrows point to cell bodies; brackets delineate a bundle of thin processes. Note the decreased density of GABA-immunoreactive processes and the increased intensity of labeling of thick processes and cell body after DNQX treatment. Scale bar, 20 µm.

Effects of treatment with the GABA_A receptor antagonist bicuculline on GABAergic and non-GABAergic synapses in the stratum oriens

The ultrastructural study allowed us to ascertain that neurons in the slices were healthy and that there were no signs ofdegeneration in synaptic terminals. In control slices after 13DIV, the GABAergic axon terminals in the stratum oriens were readilyidentified on the basis of containing both synaptic vesicles andgold particles, together with the symmetric appearance of theirsynaptic complexes (Fig. 8A). The lower values found in the 104GABAergic synapses analyzed were five vesicles and seven goldparticles (mean value, 42 gold particles per terminal; the goldparticles in mitochondria were not counted). The shape of theseaxon terminals was most often irregular, varying from roundedto elongated. Sometimes, en passant terminals were observed. Inbicuculline-treated slices, GABAergic synapses were also clearlyidentifiable in the stratum oriens (Fig. 8B). The lower valuesfound in the 170 GABAergic synapses analyzed were seven vesiclesand five gold particles (the gold particles in mitochondria werenot counted). The density of GABAergic synapses in bicuculline-treatedslices was increased by 79% when compared with adjacent, controlslices (mean ± SEM; 14 ± 1 GABAergic synapses per 7938 µm² in control slices, and 25 ± 3 GABAergic synapses per 7938 µm² in bicuculline-treated slices) (Fig. 9A).

View larger version (115K):
[in this window]
[in a new window]
Figure 8. Electron photomicrographs of GABAergic synapses in control (A) and bicuculline-treated (B) slices. The asterisks mark labeled presynaptic terminals of GABAergic synapses, which contain pleomorphic synaptic vesicles, and establish type II synaptic complexes. Note the difference in the densities at the cytoplasmic faces of the postsynaptic differentiations (arrowheads) in GABAergic and non-GABAergic (stars) synapses. The latter correspond to type I synaptic complexes. Scale bars, 300 nm.

View larger version (23K):
[in this window]
[in a new window]
Figure 9. Quantification of the effects of bicuculline treatment on GABAergic and non-GABAergic synapses in the stratum oriens. Results are presented as percentages of controls (white bars). Bicuculline increased the density of GABAergic synapses (A) but did not affect the density of non-GABAergic synapses (B), the area of GABAergic presynaptic terminals (C), the length of synaptic junctions of GABAergic synapses (D), or the density of gold particles in GABAergic presynaptic terminals (E). n, Number of animals; Bic., bicuculline. *p < 0.05.

Non-GABAergic synapses were distinguished from GABAergic synapses by their almost complete lack of gold particles (Fig. 8A,B).Furthermore, the postsynaptic differentiations of non-GABAergicsynapses were thicker and more electron-dense than those of GABAergicsynapses (Fig. 8A,B). Non-GABAergic synapses were more frequentlyencountered than GABAergic synapses (mean ± SEM; 135 ± 8 non-GABAergicsynapses per 7938 µm²). However, bicuculline treatment did not significantly changethe density of non-GABAergic synapses (mean ± SEM; 114 ± 18 non-GABAergicsynapses per 7938 µm²) (Fig. 9B).

In control slices, the mean area of GABAergic axon terminals was 0.5 ± 0.03 µm², whereas the mean length of their synaptic complexes was 334± 5 nm, and the mean density of gold particles was 2.4 particles/0.03µm². The increase in the density of GABAergic synapses after bicucullinetreatment occurred without detectable changes in the area of GABAergicterminals, the length of their synaptic complexes, or in the numberof gold particles per unit area of terminal axoplasm (Fig. 9C-E).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The results of this study indicate that neuronal activity regulates the density (number per surface area) of GAD65-immunoreactiveinhibitory terminals in organotypic slice cultures from rat postnatalhippocampus. When endogenous neuronal activity was increased byblocking GABA_A receptors, the density of GAD65-immunoreactiveterminals increased. An opposite effect was observed when neuronalactivity was reduced by blockade of non-NMDA glutamate receptors.The density of GABA-immunoreactive processes was regulated inthe same manner. Electron microscopic analysis indicated thatneuronal activity exerted at least part of its effects by increasingthe density of GABAergic synapses. BDNF application mimicked partlythe effect of neuronal activity on GAD65-immunoreactive terminals.Finally, antibodies against BDNF but not against NGF decreasedthe density of GAD65-immunoreactive terminals in bicuculline-treatedslices. These results indicate that neuronal activity regulatesthe density of inhibitory synapses in organotypic slice culturesof postnatal hippocampus and that this process is partly mediatedbyBDNF.

Activity-dependent regulation of the density of inhibitory synapses

Subcellular fractionation and immunohistochemistry have revealed that GAD65 is enriched in presynaptic terminals (Erlanderet al., 1991; Esclapez et al., 1994). Because 90% of hippocampalinterneurons expressing GAD67 also express GAD65 (Stone et al.,1999), the latter is an optimal, light microscopic marker of presynapticinhibitory terminals. In the present study, the density of GAD65-immunoreactivepuncta was increased in response to an increased neuronal activityinduced by bicuculline treatment, and, in the stratum oriens only,decreased in response to a decrease of neuronal activity afterDNQX treatment. Changes in the density of GAD65-immunoreactivepuncta did not result from differential shrinkage of the tissue,because the thickness of the slices remained constant after bicucullineor DNQX treatments (see Materials and Methods). These modificationswere probably also independent from changes in the survival ofinhibitory neurons, because spontaneous pyramidal cell death inhippocampal organotypic cultures can be blocked by glutamate receptorantagonists (Pozzo Miller et al., 1994). Thus, increasing neuronalactivity should be expected to promote excitotoxic cell deathrather than increasing the density of GAD65-immunoreactive puncta.Therefore, if the survival of interneurons is regulated by activityin the same manner as the survival of pyramidal neurons, the modulationof the density of GAD65-immunoreactive terminals most likely resultsfrom a modulation of the number of axon terminals perinterneuron.

Different types of interneurons innervate the different layers of the hippocampal slices (Freund and Buzsáki, 1996). Afterbicuculline treatment, GAD65-immunoreactive terminals increasedtheir overall density, suggesting that neuronal activity controlsthe density of GAD65-immunoreactive terminals of various typesof interneurons. In contrast, DNQX treatment decreased the densityof GAD65-immunoreactive terminals only in the stratum oriens.Interneurons that exclusively innervate the stratum oriens (Parraet al., 1998) could be particularly sensitive to activity deprivation.Alternately, the effects of modifications of neuronal activitymay be more important for axon terminals in the stratum oriens,even for interneurons that also have axon terminals in other layers.This more valid hypothesis is supported by our observation that,after bicuculline treatment, despite the general numerical increaseof GAD65-labeled terminal in different layers of the CA1 area,the increase in the stratum oriens was the most prominent. Whateverthe reason for this different response in specific regions, theregulation of the density of GAD65-immunoreactive terminals isless profound after DNQX than after bicuculline treatment, suggestingthat this regulation is more sensitive to an increase than toa decrease in neuronalactivity.

The modulation of the density of GAD65-immunoreactive puncta by neuronal activity suggests an effect of the activity on thereal number of inhibitory synapses, providing some indirect evidenceon the role of neuronal activity in the establishment of hippocampalcircuitry. However, the observed changes could be also explainedby an activity-dependent regulation of GAD65 mRNA transcripts,thereby increasing GAD65 protein levels in already existing inhibitoryterminals; more enzymatic protein would produce more biosynthesisof GABA. Such an hypothetical increase of both antigens contentscould increase the density of axon terminals that contain GAD65and GABA at levels above the threshold for immunohistochemicaldetection. Neither of these two mechanisms explains, however,the difference between the 133% increase in GAD65-positive terminalsand the much lesser (29%) increase in GABA-labeled processes observedin bicuculline-treated slices. This apparent discrepancy couldbe explained considering that GABA immunohistochemistry likelylabels both dendrites and axons of interneurons. However, thatan activity-dependent modulation of the dendrites of the interneuronscould contribute to the modifications of GABA immunoreactivityremains to bedetermined.

Our electron microscopy study does provide the required evidence in favor of an activity-dependent mechanism regulating thedensity of inhibitory synapses. The increase in numerical densityfound in the stratum oriens of cultures treated with bicuculline,occurred without the following: (1) changes in the surface areaoccupied by the terminals; (2) changes in the length of synapticcomplexes; and (3) changes in the density of gold particles. Thus,it is likely that the observed numerical increase is neither theresult of an enlargement of the terminals nor an increase of theGABA content. It can only be explained by a real augmentationin number of inhibitory synapses. The increase in the densityof GABA-immunoreactive synapses after bicuculline treatment (79%)was less important than the increase in the density of GAD65-immunoreactivepuncta (133%). This numerical mismatch suggests that, in additionto regulating the density of GABAergic synapses, neuronal activityregulates also GAD65 levels, as reported in other systems (Hendryand Jones, 1988; Aamodt et al., 2000). The activity-dependentmodulation of the density of inhibitory synapses during postnataldevelopment could be a general process, because such a densityis also regulated by neuronal activity in organotypic cerebellarcultures (Seil and Drake-Baumann, 1994; Seil et al., 1994) andin the rat barrel field neocortex in vivo (Micheva and Beaulieu,1995). Finally, this modulation of the density of inhibitory synapsesby neuronal activity could explain the decrease of GABA-mediatedinhibition that follows activity blockade in neocortical cultures(Rutherford et al., 1997).

Possible involvement of BDNF in the activity-dependent regulation of the density of inhibitory synapses

Neuronal activity regulates BDNF mRNA levels and BDNF release (Zafra et al., 1991, 1992; Goodman et al., 1996; Heymach etal., 1996; Canossa et al., 1997; Shieh et al., 1998; Tao et al.,1998; Mowla et al., 1999). BDNF treatment mimicked the effectsof a raise in neuronal activity on the density of GAD65-immunoreactiveterminals. The effect of BDNF was specific, because NT-3 did notaffect GAD65 immunoreactivity despite the fact that its receptor,TrkC, is expressed in the hippocampus (Barbacid, 1994). Furthermore,treatment with antibodies against BDNF decreased the density ofGAD65-immunoreactive terminals in bicuculline-treated slices.This effect appeared specific, because antibodies against NGFdid not affect GAD65 immunoreactivity, although NGF is synthesizedand released by hippocampal neurons in an activity-dependent manner(Thoenen, 1995). These results are in agreement with previouslypublished data showing that BDNF increases the number of axonalbranches and the total length of GABA-immunoreactive axons indissociated cultures from embryonic hippocampus (Vicario-Abejónet al., 1998). The effects of BDNF on inhibitory terminals arenot limited to hippocampal neurons and has been also reportedin organotypic cerebellar slices (Seil, 1999). Furthermore, BDNFis also implicated in the activity-dependent regulation of thedevelopment of ocular dominance in primary visual cortex in whichit plays a key role in the modulation of intracortical inhibitoryinterneurons (Berardi and Maffei, 1999; Huang et al., 1999). However,treatment with antibodies against BDNF (the present study) didnot fully antagonize the effect of bicuculline on the numericalincrease of GAD65-immunoreactive terminals. This partial effectcould arise from insufficient blockade of available BDNF. Nevertheless,our observation that BDNF treatment reproduces only 47% of thebicuculline effect strongly suggests that this neurotrophin mediatesonly part of the effects of increased activity on inhibitory synapsedensity.

The mechanism of action of BDNF on inhibitory terminals remains to be elucidated. In this study, BDNF exerted its effect onGAD65-immunoreactive terminals in DNQX-treated slices. This resultindicates that the increased density of GAD65-immunoreactive terminalsafter BDNF treatment was not attributable to an enhancement ofexcitatory synaptic transmission by the neurotrophin (Berningerand Poo, 1996; Schuman, 1999). However, in addition to the activationof intracellular signaling pathways, BDNF may also depolarizeneurons through the activation of a sodium ion conductance (Kafitzet al., 1999). Whether such depolarizing effects of BDNF contributeto the effects of this neurotrophin on inhibitory terminals remainsto betested.

From a functional point of view, the effect of BDNF on the density of inhibitory synapses may underlie the capability of chronictreatment with this neurotrophin to increase the frequency ofinhibitory currents in dissociated cultures from neocortex orhippocampus (Rutherford et al., 1997; Murphy et al., 1998). Finally,such a regulation of inhibitory function by BDNF may occur invivo, because BDNF overexpression accelerates the maturation ofGABAergic inhibition in mouse visual cortex, in parallel withan acceleration of the maturation of GABAergic innervation (Huanget al., 1999).

Possible functional consequences of the activity-dependent regulation of the density of inhibitory synapses

The modifications of the density of inhibitory synapses occurred without concomitant changes of the density of excitatorysynapses. This observation is in agreement with the finding thatlong-term treatment with a GABA_A receptor blocker does not affectthe number of dendritic spines in cultured hippocampal slices(Collin et al., 1997). The same specificity was also found inorganotypic cerebellar cultures and in the rat barrel field cortexin vivo (Seil and Drake-Baumann, 1994; Micheva and Beaulieu, 1995).Such a regulation of the density of inhibitory synapses withoutchanging the density of excitatory synapses may explain the imbalanceof neuronal activity when cultures are returned to control mediumafter long-term blockade of excitatory or inhibitory activities.Cultures in which neuronal activity was blocked exhibit an increasedactivity (Furshpan and Potter, 1989; Segal and Furshpan, 1990;Corner and Ramakers, 1992; Seil and Drake-Baumann, 1994). In contrast,cultures in which neuronal activity was increased exhibit a decreasedactivity (Corner and Ramakers, 1992; Seil et al., 1994; Turrigianoet al., 1998). Such regulations may also take place in vivo. Increasedspontaneous activity in the rat barrel field cortex after sensorydeprivation during development may be related to a specific decreasein the number of GABAergic synapses (Micheva and Beaulieu, 1995).The specific modulation of the density of inhibitory synapsesin response to changes in neuronal activity could therefore representa feedback mechanism aimed at maintaining an appropriate levelof activity in developing corticalnetworks.

  FOOTNOTES

Received March 2, 2000; revised Aug. 8, 2000; accepted Aug. 14, 2000.

This work was supported by Institut National de la Santé et de la Recherche Médicale Grant U106. C.S. and S.M. are CentreNational de la Recherche Scientifique investigators. We thankDenis Le Cren for photographic assistance. We are grateful toDr. Yves-Alain Barde for providing antibodies against NGF andto Dr. Kristy Ilinsky for providing antibodies against GAD65.We thank Dr. Fredrick Seil for advice regarding the experimentswith blocking antibodies. We also thank Dr. Benedikt Berninger,Dr. Jonathan Cooper, Dr. Isabelle Dusart, and Dr. Patricia Gasparfor critical reading of thismanuscript.
Correspondence should be addressed to S. Marty, Institut National de la Santé et de la Recherche Médicale U106, Hôpitalde la Salpêtrière, Pavillon de l'Enfance et de l'Adolescence,47 Boulevard de l'Hôpital, 75651 Paris cedex 13, France. E-mail:marty{at}chups.jussieu.fr.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aamodt SM, Shi J, Colonnese MT, Veras W, Constantine-Paton M (2000) Chronic NMDA exposure accelerates development of GABAergic inhibition in the superior colliculus. J Neurophysiol 83:1580-1591[Abstract/Free Full Text].
Barbacid M (1994) The Trk family of neurotrophin receptors. J Neurobiol 25:1386-1403[ISI][Medline].
Ben-Ari Y, Cherubini E, Corradetti R, Gaiarsa J-L (1989) Giant synaptic potentials in immature rat CA3 hippocampal neurones. J Physiol (Lond) 416:303-325[Abstract/Free Full Text].
Ben-Ari Y, Khazipov R, Leinekugel X, Caillard O, Gaiarsa J-L (1997) GABA_A, NMDA and AMPA receptors: a developmentally regulated "ménage à trois." Trends Neurosci 20:523-529[ISI][Medline].
Berardi N, Maffei L (1999) From visual experience to visual function: roles of neurotrophins. J Neurobiol 41:119-126[ISI][Medline].
Berninger B, Poo M-M (1996) Fast actions of neurotrophic factors. Curr Opin Neurobiol 6:324-330[ISI][Medline].
Buchs P-A, Stoppini L, Muller D (1993) Structural modifications associated with synaptic development in area CA1 of rat hippocampal organotypic cultures. Dev Brain Res 71:81-91[Medline].
Canossa M, Griesbeck O, Berninger B, Campana G, Kolbeck R, Thoenen H (1997) Neurotrophin release by neurotrophins: implications for activity-dependent neuronal plasticity. Proc Natl Acad Sci USA 94:13279-13286[Abstract/Free Full Text].
Collin C, Miyaguchi K, Segal M (1997) Dendritic spine density and LTP induction in cultured hippocampal slices. J Neurophysiol 77:1614-1623[Abstract/Free Full Text].
Corner MA, Ramakers GJA (1992) Spontaneous firing as an epigenetic factor in brain development: physiological consequences of chronic tetrodotoxin and picrotoxin exposure on cultured rat neocortex neurons. Dev Brain Res 65:57-64[Medline].
Durand GM, Kovalchuk Y, Konnerth A (1996) Long-term potentiation and functional synapse induction in developing hippocampus. Nature 381:71-75[Medline].
Erlander MG, Tillakaratne NJK, Feldblum S, Patel N, Tobin AJ (1991) Two genes encode distinct glutamate decarboxylases. Neuron 7:91-100[ISI][Medline].
Esclapez M, Tillakaratne NJK, Kaufman DL, Tobin AJ, Houser CR (1994) Comparative localization of two forms of glutamic acid decarboxylase and their mRNAs in rat brain supports the concept of functional differences between the forms. J Neurosci 14:1834-1855[Abstract].
Förster E, Otten U, Frotscher M (1993) Developmental neurotrophin expression in slice cultures of rat hippocampus. Neurosci Lett 155:216-219[ISI][Medline].
Freund TF, Buzsáki G (1996) Interneurons of the hippocampus. Hippocampus 6:345-470.
Furshpan EJ, Potter DD (1989) Seizure-like activity and cellular damage in rat hippocampal neurons in cell culture. Neuron 3:199-207[ISI][Medline].
Goodman LJ, Valverde J, Lim F, Geschwind MD, Federoff HJ, Geller AI, Hefti F (1996) Regulated release and polarized localization of brain-derived neurotrophic factor in hippocampal neurons. Mol Cell Neurosci 7:222-238[ISI][Medline].
Guillery RW, Herrup K (1997) Quantification without pontification: choosing a method for counting objects in sectioned tissues. J Comp Neurol 386:2-7[ISI][Medline].
Gundersen HJ, Bendtsen TF, Korbo L, Marcussen N, Moller A, Nielsen K, Nyengaard JR, Pakkenberg B, Sorensen FB, Vesterby A, West MJ (1988) Some new, simple and efficient stereological methods and their use in pathological research and diagnosis. APMIS 96:379-394[ISI][Medline].
Hendry SHC, Jones EG (1988) Activity-dependent regulation of GABA expression in the visual cortex of adult monkeys. Neuron 1:701-712[ISI][Medline].
Heymach J, Krüttgen A, Suter U, Shooter EM (1996) The regulated secretion and vectorial targeting of neurotrophins in neuroendocrine and epithelial cells. J Biol Chem 271:25430-25437[Abstract/Free Full Text].
Hosokawa Y, Sciancalepore M, Stratta F, Martina M, Cherubini E (1994) Developmental changes in spontaneous GABA-A mediated synaptic events in rat hippocampal CA3 neurons. Eur J Neurosci 6:805-813[ISI][Medline].
Huang ZJ, Kirkwood A, Pizzorusso T, Porciatti V, Morales B, Bear MF, Maffei L, Tonegawa S (1999) BDNF regulates the maturation of inhibition and the critical period of plasticity in mouse visual cortex. Cell 98:739-755[ISI][Medline].
Kafitz KW, Rose CR, Thoenen H, Konnerth A (1999) Neurotrophin-evoked rapid excitation through TrkB receptors. Nature 401:918-921[Medline].
Marty S, Carroll P, Cellerino A, Castren E, Staiger V, Thoenen H, Lindholm D (1996) Brain-derived neurotrophic factor promotes the differentiation of various hippocampal non-pyramidal neurons, including Cajal-Retzius cells, in organotypic slice cultures. J Neurosci 16:675-687[Abstract/Free Full Text].
Micheva KD, Beaulieu C (1995) An anatomical substrate for experience-dependent plasticity of the rat barrel field cortex. Proc Natl Acad Sci USA 92:11834-11838[Abstract/Free Full Text].
Miles R, Toth K, Gulyás AI, Hajos N, Freund TF (1996) Differences between somatic and dendritic inhibition in the hippocampus. Neuron 16:815-823[ISI][Medline].
Mowla SJ, Pareek S, Farhadi HF, Petrecca K, Fawcett JP, Seidah NG, Morris SJ, Sossin WS, Murphy RA (1999) Differential sorting of nerve growth factor and brain-derived neurotrophic factor in hippocampal neurons. J Neurosci 19:2069-2080[Abstract/Free Full Text].
Muller D, Buchs P-A, Stoppini L (1993) Time course of synaptic development in hippocampal organotypic cultures. Dev Brain Res 71:93-100[Medline].
Murphy DD, Cole NB, Segal M (1998) Brain-derived neurotrophic factor mediates estradiol-induced dendritic spine formation in hippocampal neurons. Proc Natl Acad Sci USA 95:11412-11417[Abstract/Free Full Text].
Parra P, Gulyás AI, Miles R (1998) How many subtypes of inhibitory cells in the hippocampus? Neuron 20:983-993[ISI][Medline].
Peters A, Palay SL, Webster HdeF (1991) In: The fine structure of the nervous system. New York: Oxford UP.
Petralia RS, Esteban JA, Wang Y-X, Partridge JG, Zhao H-M, Wenthold RJ, Malinow R (1999) Selective acquisition of AMPA receptors over postnatal development suggests a molecular basis for silent synapses. Nat Neurosci 2:31-36[ISI][Medline].
Pozzo Miller LD, Mahanty NK, Connor JA, Landis DMD (1994) Spontaneous pyramidal cell death in organotypic slice cultures from rat hippocampus is prevented by glutamate receptor antagonists. Neuroscience 63:471-487[ISI][Medline].
Rutherford LC, DaWan A, Lauer HM, Turrigiano GG (1997) Brain-derived neurotrophic factor mediates the activity-dependent regulation of inhibition in neocortical cultures. J Neurosci 17:4527-4535[Abstract/Free Full Text].
Schuman E (1999) Neurotrophin regulation of synaptic transmission. Curr Opin Neurobiol 9:105-109[ISI][Medline].
Segal MM, Furshpan EJ (1990) Epileptiform activity in microcultures containing small numbers of hippocampal neurons. J Neurophysiol 64:1390-1399[Abstract/Free Full Text].
Seil FJ (1999) BDNF and NT-4, but not NT-3, promote development of inhibitory synapses in the absence of neuronal activity. Brain Res 818:561-564[ISI][Medline].
Seil FJ, Drake-Baumann R (1994) Reduced cortical inhibitory synaptogenesis in organotypic cerebellar cultures developing in the absence of neuronal activity. J Comp Neurol 342:366-377[ISI][Medline].
Seil FJ, Drake-Baumann R, Leiman AL, Herndon RM, Tiekotter KL (1994) Morphological correlates of altered neuronal activity in organotypic cerebellar cultures chronically exposed to anti-GABA agents. Dev Brain Res 77:123-132[Medline].
Shieh PB, Hu S-C, Bobb K, Timmusk, Ghosh A (1998) Identification of a signaling pathway involved in calcium regulation of BDNF expression. Neuron 20:727-740[ISI][Medline].
Steward O, Falk PM (1991) Selective localization of polyribosomes beneath developing synapses: a quantitative analysis of the relationships between polyribosomes and developing synapses in the hippocampus and dentate gyrus. J Comp Neurol 314:545-557[ISI][Medline].
Stone DJ, Walsh J, Benes FM (1999) Localization of cells preferentially expressing GAD67 with negligible GAD65 transcripts in the rat hippocampus. A double in situ hybridization study. Mol Brain Res 71:201-209[Medline].
Stoppini L, Buchs P-A, Muller D (1991) A simple method for organotypic cultures of nervous tissue. J Neurosci Methods 37:173-182[ISI][Medline].
Tao X, Finkbeiner S, Arnold DB, Shaywitz AJ, Greenberg ME (1998) Ca²⁺ influx regulates BDNF transcription by a CREB family transcription factor-dependent mechanism. Neuron 20:709-726[ISI][Medline].
Thoenen H (1995) Neurotrophins and neuronal plasticity. Science 270:593-598[Abstract/Free Full Text].
Turrigiano GG, Leslie KR, Desai NS, Rutherford LC, Nelson SB (1998) Activity-dependent scaling of quantal amplitude in neocortical neurons. Nature 391:892-896[Medline].
Vicario-Abejón C, Collin C, McKay RDG, Segal M (1998) Neurotrophins induce formation of functional excitatory and inhibitory synapses between cultured hippocampal neurons. J Neurosci 18:7256-7271[Abstract/Free Full Text].
Zafra F, Castrén E, Thoenen H, Lindholm D (1991) Interplay between glutamate and gamma-aminobutyric acid transmitter systems in the physiological regulation of brain-derived neurotrophic factor and nerve growth factor synthesis in hippocampal neurons. Proc Natl Acad Sci USA 88:10037-10041[Abstract/Free Full Text].
Zafra F, Lindholm D, Castrén E, Hartikka J, Thoenen H (1992) Regulation of brain-derived neurotrophic factor and nerve growth factor mRNA in primary cultures of hippocampal neurons and astrocytes. J Neurosci 12:4793-4799[Abstract].

Copyright © 2000 Society for Neuroscience 0270-6474/00/20218087-09$05.00/0

This article has been cited by other articles:

N. Kuczewski, C. Porcher, N. Ferrand, H. Fiorentino, C. Pellegrino, R. Kolarow, V. Lessmann, I. Medina, and J.-L. Gaiarsa
Backpropagating Action Potentials Trigger Dendritic Release of BDNF during Spontaneous Network Activity
J. Neurosci., July 2, 2008; 28(27): 7013 - 7023.
[Abstract] [Full Text] [PDF]

L. Medrihan, E. Tantalaki, G. Aramuni, V. Sargsyan, I. Dudanova, M. Missler, and W. Zhang
Early Defects of GABAergic Synapses in the Brain Stem of a MeCP2 Mouse Model of Rett Syndrome
J Neurophysiol, January 1, 2008; 99(1): 112 - 121.
[Abstract] [Full Text] [PDF]

Y. Ben-Ari, J.-L. Gaiarsa, R. Tyzio, and R. Khazipov
GABA: A Pioneer Transmitter That Excites Immature Neurons and Generates Primitive Oscillations
Physiol Rev, October 1, 2007; 87(4): 1215 - 1284.
[Abstract] [Full Text] [PDF]

K. Kohara, H. Yasuda, Y. Huang, N. Adachi, K. Sohya, and T. Tsumoto
A Local Reduction in Cortical GABAergic Synapses after a Loss of Endogenous Brain-Derived Neurotrophic Factor, as Revealed by Single-Cell Gene Knock-Out Method
J. Neurosci., July 4, 2007; 27(27): 7234 - 7244.
[Abstract] [Full Text] [PDF]