TrkB Receptor Ligands Promote Activity-Dependent Inhibitory Synaptogenesis

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The Journal of Neuroscience, July 15, 2000, 20(14):5367-5373

TrkB Receptor Ligands Promote Activity-Dependent Inhibitory Synaptogenesis
Fredrick J. Seil¹^,²^,³ and Rosemarie Drake-Baumann¹^,²
¹ Neurology Research, Veterans Affairs Medical Center and Departments of ² Neurology and ³ Cell and Developmental Biology, Oregon Health Sciences University, Portland, Oregon 97201

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Organotypic cerebellar cultures derived from newborn mice were simultaneously exposed to activity-blocking agents and neurotrophinsfor 2 weeks. Activity-blocked explants treated with the TrkB receptorligands BDNF and neurotrophin-4 (NT-4) developed a full complementof Purkinje cell inhibitory axosomatic synapses, as defined ultrastructurally,and displayed control spontaneous cortical discharge rates afterrecovery from activity blockade. Otherwise untreated activity-blockedcultures and activity-blocked cultures exposed to the TrkC receptorligand NT-3 had reduced inhibitory synapse development and persistentcortical hyperactivity after recovery. The added TrkB receptorligands did not induce axonal sprouting to account for increasedinhibitory synaptogenesis. Addition of neurotrophins to untreatedcerebellar cultures did not increase the complement of Purkinjecell axosomatic synapses. Exposure of cerebellar cultures to acombination of antibodies to BDNF and NT-4 resulted in reducedinhibitory synapse formation, similar to the effects of activityblockade, indicating the necessity for endogenous neurotrophinsfor development of the full complement of inhibitory synapsesin the presence of neuronal activity. Application of antibodiesto BDNF and NT-4 to cerebellar explants exposed to picrotoxinto increase neuronal activity prevented the hyperinnervation ofPurkinje cell somata by inhibitory terminals characteristic ofcultures exposed to picrotoxin alone. These results are consistentwith the concept that TrkB receptor ligands promote inhibitorysynaptogenesis. The ability of neurotrophins to substitute forneuronal activity in encouraging development of inhibitory synapsesmay have therapeuticimplications.

Key words: neurotrophins; neuronal activity; development; inhibitory synapses; cerebellar cultures; Purkinje cells

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Consistent with earlier studies of effects of activity blockade in cultured CNS tissue (Ramakers et al., 1990; Baker and Ruijter,1991; Furshpan, 1991; Ruijter et al., 1991; Corner and Ramakers,1992), we reported a sustained increase of cortical spike dischargesafter transfer of newborn mouse-derived organotypic cerebellarcultures maintained in medium with tetrodotoxin (TTX) and elevatedlevels of Mg²⁺ to a physiological recording medium (Seil and Drake-Baumann,1994). The increased activity correlated with ultrastructuralfindings of reduced numbers of inhibitory axosomatic and axodendriticsynapse profiles on Purkinje cells, whereas numbers of excitatoryparallel fiber-Purkinje cell dendritic spine synapse profilesremained at control levels. In contrast, cerebellar cultures continuouslyexposed to anti-GABA agents [picrotoxin (PTX) and bicuculline]that initially increased neuronal activity had a decreased rateof spontaneous cortical discharge after transfer to a physiologicalmedium 2 weeks later, and the ratio of inhibitory axosomatic synapseprofiles to Purkinje cell somatic profiles was twice that of controlcultures (Seil et al., 1994a). Excitability of the circuitry inthese cultures appeared to be regulated by activity-dependenteffects on inhibitory (GABAergic) neurons orsynapses.

In a study with postnatal rat dissociated visual cortex cultures containing GABAergic interneurons and target pyramidal cells(Rutherford et al., 1997), it was shown that activity blockadewith TTX reduced the percentage of GABA-immunopositive neuronswithout affecting neuronal survival, whereas correlative electrophysiologicalstudies indicated that GABA-mediated inhibition onto pyramidalneurons was decreased, with concomitant increases in pyramidalcell discharge rates. The effects of activity blockade were preventedby simultaneous exposure of the cultures to the TrkB receptorligand brain-derived neurotrophic factor (BDNF) but not to theTrkA and TrkC receptor ligands nerve growth factor (NGF) and neurotrophin-3(NT-3), suggesting to the authors that activity regulates corticalinhibition by regulation of BDNF. We subsequently reported ina brief communication (Seil, 1999) that application of BDNF andthe other TrkB receptor ligand neurotrophin-4 (NT-4) to cerebellarcultures during activity blockade promoted development of thefull complement of inhibitory axosomatic synapses on Purkinjecells, whereas application of NT-3 did not prevent the reducedformation of axosomatic synapses resulting from exposure to activity-blockingagents. Neither Purkinje cell survivability nor size were affectedby neurotrophin application in this study, and the results weresuggestive of BDNF and NT-4 having a role in the promotion ofactivity-dependent inhibitorysynaptogenesis.

The purpose of the present series of experiments was to extend the study of the results of exogenous application of neurotrophinsduring activity blockade in cerebellar cultures by examining effectson cortical discharge rates and axonal sprouting, to define therole of endogenous neurotrophins in inhibitory synaptogenesisby application of neurotrophins to cultures in the presence ofneuronal activity and by blocking their effect with anti-neurotrophinantibodies, and finally to determine whether increased inhibitorysynapse formation consequent to picrotoxin-induced increased activitywould be prevented by simultaneous exposure to anti-neurotrophinantibodies.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Culture procedures. Organotypic cerebellar cultures were prepared from newborn (within 24 hr after birth) Swiss-Webster mice(Harlan Sprague Dawley, Indianapolis, IN and Charles River Laboratories,Hollister, CA) by well established methods (Bornstein and Murray,1958; Seil, 1979, 1993). The mice were cold-anesthetized and killedby exsanguination after an incision through the heart. After isolationof the cerebella under aseptic conditions and trimming of theirlateral ends, each cerebellum was cross cut with scalpel bladesinto seven parasagittal sections 0.5-mm-thick. Each section wasplaced on a collagen-coated coverslip with a drop of nutrientmedium, incorporated into a Maximow assembly, and incubated at35.5-36°C in the lying-drop position. The nutrient medium wasinitially changed at 5 d in vitro (DIV) and twice weekly thereafter.Standard nutrient medium consisted of two parts 3 IU/ml low-zincinsulin (Squibb Institute for Medical Research, Princeton, NJ),one part 20% dextrose, eight parts Eagle's minimum essential mediumwith Hanks' base and added L-glutamine, seven parts Simms' X-7balanced salt solution (BSS) with sufficient incorporated HEPESbuffer to make its concentration 10² M in the fully constituted medium, and 12 parts fetal calf serum.For cultures chronically incubated with activity-blocking agents,MgCl₂ and TTX (Sigma, St. Louis MO) dissolved in BSS bufferedwith HEPES were incorporated into the nutrient medium to finalconcentrations of 11.1 mM Mg²⁺ and 10⁸ M TTX, concentrations that we had determined previously blockedall spontaneous cortical discharges (Seil and Drake-Baumann, 1994).A combination of TTX and high levels of Mg²⁺ was used to achieve complete blockade of Purkinje cell dischargebecause somatic electroresponsiveness is attributable to voltage-gatedsodium conductance, whereas dendritic spikes are calcium-dependent(Llinás and Sugimori, 1980a,b). Neurotrophins, including BDNF(courtesy of Genentech, South San Francisco, CA; purchased fromAlexis Corporation, San Diego, CA and Promega, Madison, WI), NT-3(courtesy of Genentech and purchased from Alexis) and NT-4 (courtesyof Genentech and Regeneron, Tarrytown, NY; purchased from Alexis),were incorporated into the nutrient medium at concentrations of25 ng/ml each, with or without the activity-blocking agents, andapplied at explantation and at each of the subsequent feedingsat 5, 9, and 12 DIV. Antibodies to BDNF and NT-4 (purchased fromPromega) were incorporated together into standard nutrient mediumat concentrations of 50 µg/ml each and applied to the culturesat explantation and during the subsequent feedings. PTX (Sigma)was incorporated into the nutrient medium at a 10⁴ M concentration and applied to the cultures at explantation andwith each of the subsequent feedings, whereas some PTX-treatedcultures were additionally and simultaneously exposed to antibodiesto BDNF and NT-4, as described above, and also to greater antibodyconcentrations of 100 µg/ml each to determine whether the effectof antibody exposure could be increased with higher antibody levelsin PTX-treatedcultures.

Stain and immunocytochemical methods. Axonal sprouting was evaluated in silver-stained preparations and in culture preparationsreacted with antibody to nonphosphorylated neurofilament protein(SMI 32; purchased from Sternberger Monoclonals, Baltimore, MD).In some cases, explants were processed for silver or neurofilamentprotein procedures after electrophysiological recording. Culturesfor silver staining were fixed after 13-16 DIV as whole-mountpreparations (total of 134) in 10% formalin in BSS and processedby a Holmes silver method modified for tissue culture (Wolf, 1964).For immunocytochemistry, explants were fixed as whole-mount preparations(total of 84) for 20 min at room temperature in 10% formalin inPBS, followed by 1 hr in fresh PBS containing 0.5% Triton X-100.After repeated washes with PBS, endogenous peroxide activity wasblocked with 3% H₂O₂ in methanol for 20 min. The cultures werethen incubated for 2-4 d at 10°C in a 1:2000 dilution of antibodyin PBS with 1% rabbit carrier serum. They were subsequently exposedovernight to a 1:40 dilution of rabbit anti-mouse IgG in PBS-carrierserum, followed by a 4 hr incubation in mouse peroxidase-antiperoxidasecomplex in PBS-carrier serum at room temperature (Sternbergeret al., 1970). The last step was a 15-30 min incubation in a freshdiaminobenzidine-peroxidasemixture.

Electron microscopy. Cultures for ultrastructural examination were fixed at 15 DIV in a mixture of glutaraldehyde (1.5%) andparaformaldehyde (1.5%) in cold cacodylate buffer (0.1 M) supplementedwith 0.05 M sucrose and 2.25 mM CaCl₂ (osmolarity between 650and 750 mOsm, pH adjusted to 7.4), as described previously (Blanket al., 1982; Seil and Drake-Baumann, 1994). They were post-fixedin cacodylate-buffered 2% osmium tetroxide, dehydrated in a seriesof cold-graded ethanol and polymerized in LR white resin (LondonResin Co., Reading Berkshire, UK). Thick sections were stainedwith toluidine blue and scanned by light microscopy. Thin sectionswere stained with uranyl acetate and lead citrate and examinedwith a Zeiss (Oberkochen, Germany) EM 10C electron microscope.Purkinje cell axosomatic synapse profiles, whose presynaptic elementsare either basket cell axon terminals or Purkinje cell recurrentaxon collateral terminals, both inhibitory (Palay and Chan-Palay,1974), were identified and counted in Purkinje cell sections thatincluded nucleus (only one section per cell was counted) at magnificationsfrom 6000 to 10,000×, and ratios of synapse profiles to soma profiles(not absolute synapse numbers) were determined. Synapse profileswere counted only if they included presynaptic and postsynapticmembrane thickenings and aggregates of synaptic vesicles. Datacollection was restricted to axosomatic synapses, because thesecould be expressed as a ratio to Purkinje cell somata rather thanin absolute numbers or in numbers per given cortical area. Wedid show previously, however, that activity blockade also reducesdevelopment of inhibitory axodendritic cortical synapses in cerebellarcultures but does not affect excitatory axospinous synapse development(Seil and Drake-Baumann, 1994), so that neurotrophin effects onaxosomatic inhibitory synapses might reasonably be expected tobe reflected on axodendritic inhibitory synapses as well. Becausethe more potent inhibitory synapses are those closest to the axonhillock in which Purkinje cell axonal spikes originate (Palayand Chan-Palay, 1974; Vincent and Marty, 1996), correlations offunctional properties, such as spontaneous cortical dischargerate, with the density of axosomatic synapses would be expectedto be close, as has been the case in previous studies (Seil andDrake-Baumann, 1994; Seil et al., 1994a). Synapse/soma profileratios from the various experimental conditions were processedby one-way ANOVA, followed by the Tukey highly significant difference(HSD) multiple comparisons test using Systat software (SPSS, ChicagoIL). p $<=$ 0.05 was considered statisticallysignificant.

Electrophysiology. Extracellular electrophysiological recording procedures were as described previously (Leiman and Seil,1973; Seil and Drake-Baumann, 1994; Seil et al., 1994a). Cultureswere transferred after 13-16 DIV from the Maximow assemblies toa tissue chamber mounted on the stage of an inverted Zeiss Axiovertmicroscope. The nutrient medium was replaced with BSS additionallybuffered with 1.5 × 10² M HEPES. Etched tungsten microelectrodes with tip diameters <1µm were placed in cortical regions of the explants, and electricalactivity was recorded at room temperature by means of a GrassInstruments (Quincy, MA) P15 preamplifier. Traces were monitoredon an oscilloscope screen (Tektronix, Beaverton, OR), digitized(PCM-2; Medical Systems, Greenvale, NY), and stored on videotape(VCR; Panasonic, Secaucus, NJ) for subsequent retrieval and examination.Recordings were analyzed with a 486-IBM type computer with a 1401-plusCED interface and Spike 2 software (Cambridge Electronic Design,Cambridge, UK). Single-unit discharge rates were derived usingthe spike recognition features of Spike 2 software. Only spikesexceeding a signal-to-noise ratio of 2 were counted. The firingrate after recovery from activity blockade of each group of explants,with or without neurotrophin treatment, was averaged and comparedwith that of sister control cultures. Statistical differencesbetween groups of data were determined using one-way ANOVA, followedby the Tukey HSD test for multiplecomparisons.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

BDNF and NT-4 promote inhibitory synaptogenesis in the absence of neuronal activity

Our expanded data on the results of exogenous application of neurotrophins to activity-blocked cerebellar cultures are presentedin Table 1, which incorporates the data reported previously ina brief communication (Seil, 1999). Approximately half of thecontrol numbers of Purkinje cell axosomatic synapse profiles werepresent in cerebellar cultures after 15 d of activity blockade,consistent with our previously reported results (Seil and Drake-Baumann,1994). Cultures exposed to BDNF or NT-4 during activity blockadehad axosomatic synapse profile to Purkinje cell somatic profileratios comparable with those of control cultures, whereas exposureof activity-blocked cultures to NT-3 did not alter the reduceddevelopment of axosomatic synapses that occurred in the absenceof neuronal activity. Representative Purkinje cells from control,activity-blocked, and NT-3- and NT-4-treated activity-blockedcultures are shown at low magnification in Figure 1. Presynapticelements of axosomatic synapse profiles were either basket cellaxon terminals or Purkinje cell recurrent axon collateral terminals,as identified by established ultrastructural criteria (Palay andChan-Palay, 1974; Seil and Drake-Baumann, 1994). There were noevident aberrant axon terminals in any of the culture groups andno differences in Purkinje cell somata among the various groups.Astrocytic ensheathment of Purkinje cells was also unaffected,by either activity blockade, as reported previously (Seil andDrake-Baumann, 1994), or addition of neurotrophins to activity-blockedexplants.


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Table 1. Ratio of axosomatic synapse profiles to Purkinje cell somatic profiles in control, activity-blocked, and neurotrophin-treated activity-blocked organotypic cerebellar cultures

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Figure 1. Electron micrographs of Purkinje cell soma profiles from control, activity-blocked, and neurotrophin-treated activity-blocked newborn mouse-derived organotypic cerebellar cultures at 15 DIV. All cells are shown at the same magnification (3150×). The arrows indicate axosomatic synapse profiles. Astrocytic sheaths are evident as relatively clear areas around the circumferences of the cells. A, Purkinje cell from a control culture maintained in standard nutrient medium. B, Purkinje cell from a cerebellar explant continuously exposed to activity-blocking agents, 10⁸ M TTX and 11.1 mM Mg²⁺, incorporated into the nutrient medium. C, Purkinje neuron from a cerebellar culture exposed since explantation to nutrient medium with incorporated activity-blocking agents and 25 ng/ml NT-3. D, Purkinje cell from a cerebellar explant continuously exposed to activity-blocking agents and 25 ng/ml NT-4. There are no significant differences in the morphology of the cells other than the ratios of axosomatic synapse to soma profiles, which are reduced in activity-blocked cultures and activity-blocked cultures treated with NT-3, and at control levels in activity-blocked explants treated with TrkB receptor ligands (Table 1).

Axonal sprouting is not a factor in neurotrophin-promoted synaptogenesis

Because neurotrophins have been reported to induce axonal sprouting that could result in formation of increased numbers ofsynapses (Mansour-Robaey et al., 1994; Cohen-Cory and Fraser,1995; Rashid et al., 1995), overall neurite density was evaluatedin silver stains, and Purkinje cell axonal sprouting was estimatedin cultures reacted with antibody to nonphosphorylated neurofilamentprotein. We had demonstrated previously the sensitivity of theHolmes stain to neurite density in cerebellar cultures exposedto cytosine arabinoside after explantation in which increasedneurite density attributable to axonal sprouting was dramaticallyevident upon qualitative evaluation of silver-stained whole-mountculture preparations (Seil et al., 1980). No increase in neuritedensity was apparent qualitatively in any of the Holmes-stainedpreparations in the present study. Purkinje cell recurrent axoncollaterals are the source of half of the presynaptic elementsof Purkinje cell axosomatic synapses in cerebellar cultures (Seiland Drake-Baumann, 1994; Seil et al., 1994a), and Purkinje cells,their axons, and their target deep nucleus neurons are specificallystained in the reaction with nonphosphorylated neurofilament protein(Seil et al., 1994b). No recurrent axon collateral sprouting attributableto neurotrophin stimulation was evident in neurofilament-stainedpreparations, as shown by the representative Purkinje cells inFigure 2. Purkinje cells and portions of their axons and axoncollaterals from an activity-blocked culture are illustrated inFigure 2A, whereas the activity-blocked Purkinje cells in Figure2B had been continuously exposed to BDNF. No differences wereevident qualitatively in the axonal or axon collateral trees inthe two conditions, nor were axons of activity-blocked Purkinjecells distinguishable from axons of Purkinje cells in untreatedcontrol cultures.

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Figure 2. Whole-mount preparations of cerebellar cultures reacted at 15 DIV with antibody to nonphosphorylated neurofilament protein and processed by the peroxidase-antiperoxidase method (375× magnification). Purkinje cell recurrent axon collaterals are indicated by arrows. A, Purkinje cells from a culture continuously exposed to activity-blocking agents. B, Purkinje cells from an activity-blocked culture treated since explantation with BDNF, 25 ng/ml nutrient medium. Axonal sprouting was not evident in neurotrophin-treated activity-blocked cultures.

Activity-blocked cultures exposed to BDNF and NT-4 have cortical discharge rates equivalent to control cultures

The results of extracellular recordings of spontaneous cortical activity in cerebellar cultures are presented in Table 2.Although control cultures were immediately active after transferto the buffered BSS recording medium, all activity-blocked cultures,whether simultaneously treated with neurotrophins or not, wereelectrically silent for at least 10 min after transfer. As reportedpreviously (Seil and Drake-Baumann, 1994), untreated activity-blockedcultures began to discharge slowly after 10 min, with a subsequentincrease in discharge rates until they attained a state of continuoushyperactivity, often with spike bursts, ~30 min after transferto a medium without blocking agents. The spontaneous corticaldischarge pattern of a control explant is illustrated in Figure3A, and the hyperactive pattern of an otherwise untreated culturerecovered from activity blockade is shown in Figure 3B. Activity-blockedcerebellar cultures continuously exposed to BDNF and NT-4 hadcortical discharge rates comparable with control cultures (Table2; Fig. 3C, which shows the cortical discharge pattern of a BDNF-treatedculture after recovery from activity blockade), whereas activity-blockedcultures treated with NT-3 developed persistently hyperactivecortical discharge rates after recovery from activity blockade(Table 2). The cortical discharge patterns, which primarily representPurkinje cell spikes (Seil and Drake-Baumann, 1994), correlatedwith the complement of Purkinje cell inhibitory axosomatic synapses,because control discharge rates were present in cultures withthe full complement of inhibitory synapses, whereas cortical hyperactivitywas evident in cultures with reduced inhibition. The electrophysiologicalresults were thus consistent with the morphological findings.


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Table 2. Spontaneous cortical discharge rates in control, activity-blocked, and neurotrophin-treated activity-blocked organotypic cerebellar cultures

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Figure 3. Extracellular records of spontaneous cortical activity in cerebellar cultures after 2 weeks in vitro. A, Untreated control explant recorded at 14 DIV. B, Increased activity with spike bursts in a cerebellar explant 40 min after recovery from activity blockade induced by continuous exposure to 10⁸ M TTX and 11.1 mM Mg²⁺. The culture had been silent during the first 10 min after transfer to a medium without activity-blocking agents, in contrast to control cultures, which were immediately active after transfer to a physiological recording medium. Recorded at 15 DIV. C, Cortical spikes recorded 45 min after transfer to a recording medium. The culture had been exposed to a combination of activity-blocking agents and BDNF (25 ng/ml medium) for 15 DIV before recording. The spontaneous cortical activity pattern is similar to that of untreated control cultures. Time bar at the bottom, 5 sec.

Addition of neurotrophins to cultures in the presence of neuronal activity does not increase inhibitory synaptogenesis

As shown in Table 3, exogenous application of neurotrophins in the presence of neuronal activity, by continuous exposureof otherwise untreated cerebellar cultures to the same concentrationsof neurotrophins (25 ng/ml medium) as in the experiments withactivity-blocking agents, did not induce an increase in inhibitorysynaptogenesis. The ratio of Purkinje cell axosomatic synapseprofiles to somatic profiles after exposure to any of the neurotrophinstested was not significantly different from that of untreatedcontrol explants. Addition of higher levels of neurotrophins tootherwise untreated explants remains to be tested. The controlvalues for the mean ratios of synapse to cell profiles in thisand the subsequent experiment with antibodies to neurotrophins(Table 3) are higher than in Table 1, possibly because of seasonalvariations in donor mice, and for this reason specific controlsare always set up with each individual experiment in studies withcultures.


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Table 3. Ratio of axosomatic synapse profiles to Purkinje cell somatic profiles in organotypic cerebellar cultures treated with neurotrophins, with a combination of antibodies to BDNF and NT-4 ( $alpha$ BDNF/ $alpha$ NT-4), or with PTX with or without antibodies to BDNF and NT-4

Blocking neurotrophins with antibodies reduces inhibitory synaptogenesis

In initial experimental trials with antibody to BDNF, Purkinje cells in cultures exposed to 50 µg/ml BDNF/nutrient mediumhad a ratio of 1.85 ± 0.31 (SEM) axosomatic synapse to soma profiles(n = 27) after 15 DIV compared with a ratio of 2.61 ± 0.31 forPurkinje cells in untreated control cultures (n = 31). In subsequentexperiments, a combination of antibodies to BDNF and NT-4 (50µg/ml each) were applied to the cultures, with resultant reductionof the development of Purkinje cell axosomatic synapses to approximatelyhalf of the control value (Table 3), similar to the effect ofactivity blockade. The greater reduction of inhibitory synapseformation on Purkinje cell somata with the combination of antibodiesto BDNF and NT-4 suggested that both TrkB receptor ligands contributedto the development of Purkinje cell inhibitory axosomatic synapsesin cultures with neuronalactivity.

Antibodies to BDNF and NT-4 prevent increased inhibitory synapse formation in cultures exposed to PTX to increase neuronal activity

Anti-BDNF plus anti-NT-4 antibody (50 µg/ml medium each) treatment of organotypic cerebellar cultures simultaneously exposedto the anti-GABA agent PTX to increase neuronal activity preventedthe increase in Purkinje cell axosomatic synapse development characteristicof cultured Purkinje cells chronically exposed to PTX (Seil etal., 1994a) (Table 3). However, the number of axosomatic synapseprofiles was not reduced to the same degree as in cultures withbackground levels of neuronal activity (not exposed to PTX) (Table3). To determine whether this was possibly because the quantityof antibody was not sufficient to bind all of the BDNF and NT-4released as a result of PTX exposure, the antibody concentrationswere doubled, with resultant reduction of the ratio of axosomaticsynapse to Purkinje cell soma profiles to a value comparable withthat of otherwise untreated cultures exposed to the lower antibodyconcentrations (Table 3). The prevention by anti-BDNF and anti-NT-4antibodies of increased inhibitory synaptogenesis in responseto exposure to an agent that induces accelerated Purkinje celldischarge, as well as the further reduction in synapse formationwith increased concentrations of antibody, suggests that the increasedinhibitory synaptogenesis is attributable at least in part toelevated levels of these neurotrophins in the presence of increasedneuronalactivity.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Evidence that neuronal activity is necessary for the full development and maintenance of inhibitory circuitry has been derivednot only from investigations with tissue culture systems (Ramakerset al., 1990; Baker and Ruijter, 1991; Furshpan, 1991; Ruijteret al., 1991; Corner and Ramakers, 1992; Seil and Drake-Baumann,1994; Seil et al., 1994a; Rutherford et al., 1997) but also fromstudies in vivo. Hendry and Jones (1986) reported markedly reducedGABA immunoreactivity in adult monkey visual cortex ocular dominancecolumns that had been deprived of input by enucleation of oneeye. Monocular injection of TTX to prohibit retinal ganglion celldischarge achieved the same effect (Hendry and Jones, 1988). Morerecently, Benevento et al. (1995) recorded an increase in spontaneousactivity in the visual cortex of dark-reared rats, correlatingwith a decrease in the number of GABA-reactive neurons. Michevaand Beaulieu (1995) described a significant reduction of GABA-immunopositivesynapses in layer IV of the barrel field cortex of rats in whichsensory deprivation was achieved by removal of whiskers soon afterbirth. This finding was consistent with an earlier report of increasedspontaneous activity in the barrel field cortex of neonatallysensory-deprived animals (Simons and Land, 1987).

Neurotrophins have been reported to be synthesized and released in an activity-dependent manner (Zafra et al., 1991; Lindholmet al., 1994; Blöchl and Thoenen, 1995; Thoenen, 1995). Theseneurotrophic factors have also been reported to have functionaleffects at synapses (for review, see Schuman, 1999). BDNF enhancedsynaptic currents in hippocampal cultures, an enhancement thatwas partially prevented by the "universal" Trk receptor inhibitorK252a (Kang and Schuman, 1995). BDNF and NT-3, but not NGF, enhancedsynaptic strength at Schaffer collateral-CA1 synapses in hippocampalslices from adult rats, an effect that was blocked by K252a (Levineet al., 1995). Hippocampal long-term potentiation (LTP) was reducedin CA1 of mutant mice that lacked BDNF (Korte et al., 1995), andtreatment of hippocampal slices from BDNF knock-out mice withBDNF completely reversed deficits in LTP (Patterson et al., 1996).

Given an association between neuronal activity and the development and maintenance of inhibitory circuitry, activity-dependenteffects and neurotrophins, and neurotrophins and regulation ofsynaptic function, it seemed reasonable to consider the possibilitythat neurotrophins had a role in the development of inhibitorysynapses. That this might, indeed, be the case was supported bythe results of our study indicating that BDNF and NT-4 promotedthe development of inhibitory Purkinje cell axosomatic synapsesin cerebellar cultures in the absence of neuronal activity (Seil,1999).

Support for this concept was strengthened by the results of the present study. Although it was evident from the previous report(Seil, 1999) that Purkinje cell survival and size were not significantlyaffected by either activity blockade or addition of neurotrophinsto activity-blocked cultures, it was shown in the current workthat neurotrophin-induced axonal sprouting was also not a significantcontributory factor to the BDNF- and NT-4-promoted increase inPurkinje cell axosomatic synapses during activity blockade. Evenif axonal sprouting had occurred, the axosomatic synapse regulatoryfunction of the Purkinje cell astrocytic sheath would have hadto have been overcome for hyperinnervation of Purkinje cell somatato develop (Seil et al., 1992; Seil, 1996). The only example ofhyperinnervation of Purkinje cell somata by inhibitory axon terminalsin the presence of intact astrocytic sheaths known to us occurredwith continuous exposure of cerebellar cultures to agents thatincreased neuronal activity (Seil et al., 1994a).

Functional studies indicated a correlation with the morphological results. Activity-blocked Purkinje cells had reduced inhibitoryaxosomatic synapses and demonstrated persistent cortical hyperactivityafter recovery from activity blockade. Purkinje cells treatedwith the TrkB receptor ligands BDNF or NT-4 during activity blockadedeveloped the full complement of inhibitory axosomatic synapsesand displayed cortical activity patterns in the control rangeafter release from blockade. Spontaneous cortical discharge ratesappeared to be inversely proportional to the complement of Purkinjecell axosomatic synapses, and activity blockade-induced reductionof Purkinje cell axosomatic synapse development was preventedby exogenous addition of TrkB receptor ligands, thus maintainingthe functional integrity of the cortex. These studies also demonstratedthe effectiveness of the activity blockade, with or without thepresence of neurotrophins, for all cultures exposed to activity-blockingagents were electrically silent for at least 10 min after transferto a physiological recording medium, even at maximum intervalsafter the last feeding, which was 4d.

Collectively, the results of this study indicate that TrkB receptor ligands have a role in the regulation of numbers of synapses,at least with regard to inhibitory synapses. Njå and Purves (1978)had reported previously that NGF increased the number of synapseson superior cervical ganglion neurons. More recently, Vicario-Abejonet al. (1998) described enhancement of the number of functionalexcitatory glutamatergic synapses by treatment of developing hippocampalcultures with BDNF and NT-3, although BDNF also promoted the formationof inhibitory synaptic connections. Our study was focused on inhibitorysynapses because of our earlier finding of development of thefull complement of excitatory axospinous cortical synapses inactivity-blocked cerebellar cultures, although numbers of inhibitorysynapses were markedly reduced (Seil and Drake-Baumann, 1994).Thus, inhibitory cortical synapses were obvious targets for studiesof neurotrophin effects on activity-dependent synaptogenesis,but that is not to say that neurotrophins affect only inhibitorysynapse development, as it appears otherwise from theliterature.

The necessity for endogenous neurotrophins for development of the full complement of inhibitory synapses in the presence ofneuronal activity was shown by the reduced formation of Purkinjecell axosomatic synapses when the TrkB receptor ligands were functionallyblocked with antibodies. The reduction in inhibitory synapse developmentwas similar to that consequent to activity blockade, which presumablyreduces neurotrophin release (Blöchl and Thoenen, 1995; Thoenen,1995) or reduces the responsiveness of neurons to neurotrophins(McAllister et al., 1999). The latter possibility is less likelybecause added exogenous neurotrophins can promote developmentof the full complement of inhibitory axosomatic synapses in theabsence of neuronal activity (Seil, 1999). There may be a delicatebalance, however, between levels of neuronal activity and responsivenessto or release of neurotrophins, because Purkinje cells dischargingunder control conditions failed to respond with increased axosomaticsynapse development upon exogenous addition of the same levelsof BDNF and NT-4 that promoted inhibitory synaptogenesis in activity-blockedcultures, an effect that could also be accounted for by a feedbackmechanism that inhibited endogenous release in the presence ofexogenously supplied neurotrophins. On the other hand, an increasein neuronal activity induced by PTX exposure resulted in hyperinnervationof Purkinje cell somata by inhibitory terminals, an effect thatwas mitigated by application of antibodies to the TrkB receptorligands, which is consistent with the concept of accelerated neuronalactivity inducing an increased release of neurotrophins, resultingin an increased development of inhibitory synapses. The activitystate of the neuron may not only direct the release of neurotrophinsbut may also define the neurotrophin effect. Quantitative studieswith varying concentrations of neurotrophins and levels of neuronalactivity may provide some further insight into the nature of thecomplex interplay between neuronal activity and neurotrophinactions.

The fact that neurotrophins may substitute for neuronal activity in the promotion of synapse development does not necessarilymean that the effects of neuronal activity are mediated by neurotrophins.Regulation of the numbers of synapses may be only one of manyaspects of neuronal activity-neurotrophin interaction during synapsedevelopment. Recently Cohen-Cory (1999) argued that BDNF modulates,but does not mediate, activity-dependent optic axon arborizationbecause of a difference in mechanisms by which neurotrophins andneuronal activity regulate axonal arborization, with BDNF promotingaxonal growth, whereas neuronal activity is involved with stabilizationof axonal branching. Opportunities for such differences in mechanismsare probably greatly magnified in the complicated sequence ofsynaptogenesis, especially when the requirement for a balancebetween inhibition and excitation for proper circuit functionisconsidered.

The ability of neurotrophins to achieve similar outcomes as neuronal activity may in some circumstances have therapeutic implications.Activity is known to promote functional recovery after CNS insultssuch as trauma or stroke, both in experimental and clinical situations(Jenkins and Merzenich, 1987; Chollet et al., 1991; Cohen et al.,1991; Elbert et al., 1994; Nudo et al., 1996; Johansson, 2000).Because activity appears to be necessary for the development (andprobably restoration) of inhibitory circuitry, thus achievingan appropriate balance between excitation and inhibition and avoidingsuch negative consequences as seizures, it is conceivable thatneurotrophin treatment might serve as an adjunct to such measuresas physical therapy and perhaps as a substitute when use of activity-inducingmeasures is not possible. Such clinical considerations await developmentof more efficient methods of delivery of neurotrophins to appropriateCNSsites.

  FOOTNOTES

Received Jan. 13, 2000; revised April 19, 2000; accepted May 1, 2000.

This work was supported by the United States Department of Veterans Affairs. The technical assistance of Jennifer Jefferson,Marilyn Johnson, and Juany Rehling is gratefullyacknowledged.
Correspondence should be addressed to Dr. Fredrick J. Seil, Neurology Research (P3-R&D-35), Veterans Affairs Medical Center,Portland, OR 97201. E-mail: seilf{at}ohsu.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Baker RE, Ruijter JM (1991) Chronic blockade of bioelectric activity in neonatal rat neocortex in vitro: physiological effects. Int J Dev Neurosci 9:321-329[ISI][Medline].
Benevento LA, Bakkum BW, Cohen RS (1995) Gamma-aminobutyric acid and somatostatin immunoreactivity in the visual cortex of normal and dark- reared rats. Brain Res 689:172-182[ISI][Medline].
Blank NK, Seil FJ, Herndon RM (1982) An ultrastructural study of cortical remodeling in cytosine arabinoside induced granuloprival cerebellum in tissue culture. Neuroscience 7:1509-1531[ISI][Medline].
Blöchl A, Thoenen H (1995) Characterization of nerve growth factor (NGF) release from hippocampal neurons: evidence for a constitutive and an unconventional sodium-dependent regulated pathway. Eur J Neurosci 7:1220-1228[ISI][Medline].
Bornstein MB, Murray MR (1958) Serial observations on patterns of growth, myelin formation, maintenance and degeneration in cultures of new-born rat and kitten cerebellum. J Biochem Biophys Cytol 4:499-504.
Chollet F, DiPiero V, Wise RJS, Brocks DJ, Dolan RJ, Frackowiak RSJ (1991) The functional anatomy of motor recovery after stroke in humans: a study with positron emission tomography. Ann Neurol 29:63-71[ISI][Medline].
Cohen LG, Bandinelli S, Findley TW, Hallett M (1991) Motor reorganization after upper limb amputation in man. Brain 114:615-627[Abstract/Free Full Text].
Cohen-Cory S (1999) BDNF modulates, but does not mediate, activity-dependent branching and remodeling of optic axon arbors in vivo. J Neurosci 19:9996-10003[Abstract/Free Full Text].
Cohen-Cory S, Fraser S (1995) Effects of brain-derived neurotrophic factor on axon branching and remodeling in vivo. Nature 378:192-196[Medline].
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].
Elbert T, Flor H, Birbaumer N, Knecht S, Hampson S, Larbig W, Taub E (1994) Extensive reorganization of the somatosensory cortex in adult humans after nervous system injury. NeuroReport 5:2593-2597[ISI][Medline].
Furshpan EJ (1991) Seizure-like activity in cell culture. Epilepsy Res 10:24-32[ISI][Medline].
Hendry SAC, Jones EG (1986) Reduction in number of immunostained GABAergic neurones in deprived-eye dominance columns of monkey area 17. Nature 320:750-753[Medline].
Hendry SAC, Jones EG (1988) Activity-dependent regulation of GABA expression in the visual cortex of adult monkeys. Neuron 1:701-712[ISI][Medline].
Jenkins WM, Merzenich MM (1987) Reorganization of neocortical representation after brain injury: a neurophysiological model of the bases of recovery from stroke. In: Neural regeneration, Progress in brain research, Vol 71 (Seil FJ, Herbert E, Carlson BM, eds), pp 249-266. Amsterdam: Elsevier.
Johansson BB (2000) Brain plasticity and stroke rehabilitation. Stroke 31:223-230[Abstract/Free Full Text].
Kang H, Schuman EM (1995) Long-lasting neurotrophin-induced enhancement of synaptic transmission in the adult hippocampus. Science 267:1658-1662[Abstract/Free Full Text].
Korte M, Carroll P, Wolf E, Brem G, Thoenen H, Bonhoeffer T (1995) Hippocampal long-term potentiation is impaired in mice lacking brain-derived neurotrophic factor. Proc Natl Acad Sci USA 92:8856-8860[Abstract/Free Full Text].
Leiman AL, Seil FJ (1973) Spontaneous and evoked bioelectric activity in organized cerebellar tissue cultures. Exp Neurol 40:748-759[ISI][Medline].
Levine ES, Dreyfus CF, Black IR, Plummer MR (1995) Brain-derived neurotrophic factor rapidly enhances synaptic transmission in hippocampal neurons via postsynaptic tyrosine kinase receptors. Proc Natl Acad Sci USA 92:8074-8077[Abstract/Free Full Text].
Lindholm D, Castrén E, Berzaghi M, Blöchl A, Thoenen H (1994) Activity-dependent and hormonal regulation of neurotrophin mRNA levels in the brain: implications for neuronal plasticity. J Neurobiol 25:1362-1372[ISI][Medline].
Llinás R, Sugimori M (1980a) Electrophysiological properties of in vitro Purkinje cell somata in mammalian cerebellar slices. J Physiol (Lond) 305:171-195[Abstract/Free Full Text].
Llinás R, Sugimori M (1980b) Electrophysiological properties of in vitro Purkinje cell dendrites in mammalian cerebellar slices. J Physiol (Lond) 305:197-213[Abstract/Free Full Text].
Mansour-Robaey S, Clarke DB, Wang Y-C, Bray GM, Aguayo AJ (1994) Effects of ocular injury and administration of brain-derived neurotrophic factor on survival and regrowth of axotomized retinal ganglion cells. Proc Natl Acad Sci USA 91:1632-1636[Abstract/Free Full Text].
McAllister AC, Katz LC, Lo DC (1999) Neurotrophins and synaptic plasticity. Annu Rev Neurosci 22:295-318[ISI][Medline].
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].
Njå A, Purves D (1978) The effects of nerve growth factor and its antiserum on synapses in the superior cervical ganglion of the guinea pig. J Physiol (Lond) 277:53-75[ISI][Medline].
Nudo RJ, Wise BM, SiFuentes F, Miliken GW (1996) Neural substrates for the effects of rehabilitative training on motor recovery after ischemic infarct. Science 272:1791-1794[Abstract].
Palay S, Chan-Palay V (1974) In: Cerebellar cortex. Cytology and organization, pp 11-62, 180-215. New York: Springer.
Patterson SL, Abel T, Duel TAS, Martin KC, Rose JC, Kandel ER (1996) Recombinant BDNF rescues deficits in basal synaptic transmission and hippocampal LTP in BDNF knockout mice. Neuron 16:1137-1145[ISI][Medline].
Ramakers GJA, Corner MA, Habets AMMC (1990) Development in the absence of spontaneous bioelectric activity results in increased stereotype burst firing in cultures of dissociated cerebral cortex. Exp Brain Res 79:157-166[ISI][Medline].
Rashid K, Van der Zee CEEM, Ross GM, Chapman CA, Stanisz J, Riopelle RJ, Racine RJ, Fahnestock M (1995) A nerve growth factor peptide retards seizure development and inhibits neuronal sprouting in a rat model of epilepsy. Proc Natl Acad Sci USA 92:9495-9499[Abstract/Free Full Text].
Ruijter JM, Baker RE, DeJong BM, Romijn HJ (1991) Chronic blockade of bioelectric activity in neonatal rat cortex grown in vitro: morphological effects. Int J Dev Neurosci 9:331-338[ISI][Medline].
Rutherford LC, DeWan 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 activity. Curr Opin Neurobiol 9:105-109[ISI][Medline].
Seil FJ (1979) Cerebellum in tissue culture. In: Reviews of neuroscience, Vol 4 (Schneider DM, ed), pp 105-177. New York: Raven.
Seil FJ (1993) Organotypic neural cultures. In: In vitro biological systems: preparation and maintenance. Methods in toxicology, Vol 1 (Tyson CA, Frazier JM, eds), pp 7-26. Orlando, FL: Academic.
Seil FJ (1996) Neural plasticity in cerebellar cultures. Prog Neurobiol 50:533-556[ISI][Medline].
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 cultures developing in the absence of neuronal activity. J Comp Neurol 342:366-377[ISI][Medline].
Seil FJ, Leiman AL, Woodward WR (1980) Cytosine arabinoside effects on developing cerebellum in tissue culture. Brain Res 186:393-408[ISI][Medline].
Seil FJ, Drake-Baumann R, Herndon RM, Leiman AL (1992) Cytosine arabinoside effects in mouse cerebellar cultures in the presence of astrocytes. Neuroscience 51:149-158[ISI][Medline].
Seil FJ, Drake-Baumann R, Leiman AL, Herndon RM, Tiekotter KL (1994a) Morphological correlates of altered neuronal activity in organotypic cultures chronically exposed to anti-GABA agents. Dev Brain Res 77:123-132[Medline].
Seil FJ, Drake-Baumann R, Johnson ML (1994b) Dystrophic dendrites induced in cultured Purkinje cells by exposure to vinblastine. Brain Res 636:87-97[ISI][Medline].
Simons DJ, Land PW (1987) Early experience of tactile stimulation influences organization of somatic sensory cortex. Nature 326:694-697[Medline].
Sternberger LA, Hardy PH, Cuculis JJ, Meyer HG (1970) The unlabeled antibody enzyme method of immunohistochemistry. J Histochem Cytochem 18:315-333[Abstract].
Thoenen H (1995) Neurotrophins and neuronal plasticity. Science 270:593-598[Abstract/Free Full Text].
Vicario-Abejon 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].
Vincent P, Marty A (1996) Fluctuations of inhibitory postsynaptic currents in Purkinje cells from rat cerebellar slices. J Physiol (Lond) 494:183-199[ISI][Medline].
Wolf MK (1964) Differentiation of neuronal types and synapses in myelinating cultures of mouse cerebellum. J Cell Biol 22:259-279[Abstract/Free Full Text].
Zafra F, Castrén H, 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].

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