Granule Neuron Regulation of Purkinje Cell Development: Striking a Balance Between Neurotrophin and Glutamate Signaling

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 (90)

Citing Articles via Google Scholar

Google Scholar

Articles by Morrison, M. E.

Articles by Mason, C. A.

Search for Related Content

PubMed

PubMed Citation

Articles by Morrison, M. E.

Articles by Mason, C. A.

Previous Article  |  Next Article

The Journal of Neuroscience, May 15, 1998, 18(10):3563-3573

Granule Neuron Regulation of Purkinje Cell Development: Striking a Balance Between Neurotrophin and Glutamate Signaling
Mary E. Morrison and Carol A. Mason
Departments of Pathology, and Anatomy and Cell Biology, Center for Neurobiology and Behavior, College of Physicians and Surgeons, Columbia University, New York, New York 10032

  ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Granule neurons, presynaptic afferents of Purkinje cells, are potent regulators of Purkinje cell development. Purified Purkinjecells survive and differentiate poorly, whereas coculture withgranule neurons enhances their survival and dendritic development.Here we investigate the role of neurotrophins in granule-Purkinjecell interactions. BDNF or NT-4 improves, but NT-3 or CNTF reduces,survival of isolated Purkinje cells. When granule neurons arepresent, however, BDNF or NT-4 treatment leads to Purkinje cellloss. This decrease is overcome by anti-BDNF or TrkB-IgG-blockingreagents or by CNQX, a non-NMDA glutamate receptor antagonist.Furthermore, BDNF increases the spine density on the survivingPurkinje cells. These results suggest that Purkinje cell survivaland differentiation are context-dependent and require a balancebetween neurotrophin- and activity-dependent signaling.

Key words: Purkinje cell; granule cell; cerebellum; neurotrophins; BDNF; CNQX; spines

  INTRODUCTION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Afferent regulation of CNS target cell development has been studied extensively (Kandel et al., 1995). In the cerebellum,experimental and genetic ablations have identified granule neuronafferents as being more influential than olivocerebellar climbingfiber afferents for Purkinje cell survival and development (Altmanand Anderson, 1972; Rakic, 1975; Privat and Drian, 1976; Soteloand Arsenio-Nunes, 1976; Mariani et al., 1977; Hatten and Heintz,1995). Previously, we directly tested granule neuron involvementin these processes using methods for purification of cerebellarPurkinje cells (Baptista et al., 1994) and granule neurons (Hatten,1985; Baird et al., 1992). These experiments demonstrated thatthe granule neuron is a potent regulator of Purkinje cell survivaland differentiation. Although purified Purkinje cells survivepoorly when cultured alone, developing axons but only rudimentarydendrites (Baptista et al., 1994) (see Fig. 1A), coculture ofpurified Purkinje and granule cells improves survival of the Purkinjecells and triggers their dendritic differentiation (Baptista etal., 1994) (see Fig. 1C).

What molecules underlie granule neuron regulation of Purkinje cell survival and differentiation? A variety of neurotrophinand Trk mRNAs and proteins have been localized in Purkinje cells(Yan and Johnson, 1988; Cohen-Cory et al., 1989; Lindholm et al.,1993; Rocamora et al., 1993; Gao et al., 1995; Torres et al.,1995) (see Discussion) or in granule cells (Yan and Johnson, 1988;Hofer et al., 1990; Ernfors et al., 1992; Wheeler and Bothwell,1992; Lindholm et al., 1993; Rocamora et al., 1993; Leingartneret al., 1994; Muller et al., 1994; Gao et al., 1995; Segal etal., 1995) (see Discussion), suggesting that neurotrophins maybe involved in granule-Purkinje cell interactions. Moreover, neurotrophinsand CNTF affect Purkinje cell development in vitro (NGF, Cohen-Coryet al., 1991; NT-3, Lindholm et al., 1993; BDNF, Mount et al.,1993; CNTF, Larkfors et al., 1994, 1996). All of these experiments,however, were performed in cultures of whole dissociated cerebellum,confounding the interpretation of which cells act or react inspecific signaling events. We therefore chose to examine the roleof neurotrophins in granule neuron-mediated Purkinje cell developmentusing cocultures of granule and Purkinje cells. In addition, westudied the interplay between neurotrophins and neurotransmittersin this reductionist system.

Neurotrophin signaling pathways interact with neurotransmitter systems during a number of developmental processes (for review,see Lo, 1995; Thoenen, 1995; Bonhoeffer, 1996; Henderson, 1996;Katz and Shatz, 1996; Snider and Lichtman, 1996; Schuman, 1997).These include cell survival (Cohen-Cory et al., 1991; Mount etal., 1993; Meyer-Franke et al., 1995; Riddle et al., 1995), axonarborization (Cabelli et al., 1995, 1996, 1997; Galuske et al.,1996; Prakash et al., 1996), dendritic differentiation (McAllisteret al., 1995, 1997), synaptic transmission (Lohof et al., 1993;Levine et al., 1995; Stoop and Poo, 1996), and plasticity (Kangand Schuman, 1995, 1996; Figurov et al., 1996; Patterson et al.,1996; Akaneya et al., 1997; Schuman, 1997). Despite these difficultand elegant analyses, the cell types that mediate the collaborationof neurotrophin- and activity-dependent processes are largelyunknown.

This study shows that neurotrophin action depends on the context in which a cell is growing. Survival of purified Purkinjecells cultured alone is increased by BDNF or NT-4, but surprisingly,survival of Purkinje cells cultured with granule neurons, theirnormal presynaptic afferents, is diminished by the same treatment.This neurotrophin-induced death is blocked by a non-NMDA receptorantagonist, revealing that a precise balance between the neurotrophinand neurotransmitter signaling systems is required for Purkinjecell survival.

  MATERIALS AND METHODS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Animals. Experiments were performed with C57BL/6J mice from a timed pregnancy breeding colony with the plug date consideredembryonic day 0 (E0). For mixed cerebellar cultures or for purifiedPurkinje cells, cerebella were taken from animals on the firstday after birth, designated postnatal day 0 (P0). For any singlePurkinje cell purification experiment, 30 P0 pups were used, butoccasionally it was necessary to use some P1 pups as well. Granuleneurons were purified from pups on postnatal day 4.

Culture media and substrates. The composition of the media differed somewhat from that published previously (Baptista et al.,1994). Serum-free medium was composed of Eagle's basal mediumwith Earle's salts (Life Technologies, Gaithersburg, MD) supplementedwith bovine serum albumin (10 mg/ml; A-9418, Sigma, St. Louis,MO), glutamine (2 mM; Life Technologies), glucose (32 mM), penicillin-streptomycin(29 U/ml each; Life Technologies), and Sigma I-1884 supplement(1:100 dilution, giving final concentrations of 5 µg/ml insulin,5 µg/ml transferrin, and 5 ng/ml sodium selenite). Serum-containingmedium was composed of Eagle's basal medium with Earle's salts,glutamine, glucose, penicillin-streptomycin, and 10% horse serum(Life Technologies).

Culture surfaces were pretreated overnight at 4°C with high molecular weight (>300,000 kDa) poly-D-lysine (500 µg/ml; Sigmaor Specialty Media) and washed three times with distilled waterbefore use.

Mixed cerebellar cultures. Mixed cerebellar cultures were prepared as previously published (Baptista et al., 1994). Briefly,animals were killed by decapitation. Cerebella were dissectedinto calcium- and magnesium-free PBS (CMF-PBS), and meninges wereremoved. Cerebella were digested with trypsin (1% in CMF-PBS;Worthington, Freehold, NJ) for 3 min at room temperature. Trypsinwas replaced with DNase (0.05% in BME; Worthington), and cerebellawere triturated with fire-polished Pasteur pipettes of three sequentiallydecreasing bore sizes. Cells were centrifuged and resuspendedin CMF-PBS with DNase, and the cell slurry was passed througha 33 µM nylon mesh filter. Cells were resuspended in horse serummedium, counted, diluted with serum-free medium, and plated ata density of 11 × 10⁵ cells/cm² in Nunc Lab-Tek (Naperville, IL) 7 mm diameter wells (300,000cells per well in 0.2 ml). This plating density produced a uniformmonolayer.

Purkinje cell purification. Purkinje cells were purified essentially as previously described (Baptista et al., 1994) withsome details changed. Briefly, cerebella were cut into three piecesand digested with papain (10 U/ml; Worthington) in a solutioncontaining Earle's balanced salts (1×; Life Technologies), NaHCO₃(26 mM), glucose (0.5%), L-cysteine, and EDTA (0.5 mM) at 35.5°Cfor 45-60 min. The papain solution was replaced with ovomucoid-(0.2%;Boehringer Mannheim, Indianapolis, IN) or horse serum-containingmedium, and tissue chunks were triturated sequentially with fire-polishedPasteur pipettes of three decreasing sizes to give a single-cellsuspension. Cells were centrifuged and resuspended in ice-coldCMF-PBS containing DNase and then loaded onto cushions of 35%Percoll in CMF-PBS with EDTA. The cells accumulating at the 0-35%interface were removed and washed with CMF-PBS.

This cell fraction was resuspended in BME with 0.6% glucose and transferred onto anti-GD3 dishes prepared as follows. Four6 cm Petri dishes (Falcon 1007) were coated the night before thepurification at 4°C with goat anti-mouse IgG (Cappell-Worthington,Durham, NC; 20 µg/ml in 50 mM Tris Cl, pH 9.5), washed with PBSthe morning of the preparation, double-coated with anti-GD3 supernatant(HB8445, from the R24 hybridoma; American Type Culture Collection,Rockville, MD) at room temperature, washed again with PBS, andpreblocked with bovine serum albumin (2 mg/ml; Sigma A-9418) inBME at 35.5°C for 1 hr. Glial cells were allowed to attach tothe anti-GD3 dishes for 45 min at 35.5°C, and nonadherent cellswere transferred onto anti-Thy 1.2 dishes prepared as follows.Four 6 cm Petri dishes were coated the night before the purificationat 4°C with anti-Thy 1.2 (Boeringer Mannheim 1199 005; 2.7 µg/mlin 50 mM Tris Cl, pH 9.5), washed with PBS, and preblocked withBME containing BSA at 35.5°C during the anti-GD3 panning step.Cells were allowed to attach to the anti-Thy 1.2 dishes for 45min at 35.5°C, and then nonadherent cells and debris were removedby seven to nine washes with warmed CMF-PBS. Adherent, highlyenriched Purkinje cells were removed from the final panning plateswith trypsin-EDTA (0.05%, 0.53 mM; Life Technologies 25300-013)at 35.5°C for 10 min. The trypsin was inactivated by adding horseserum-containing medium, and the cells were centrifuged and resuspendedin serum-free medium, counted, and plated at a density of 30,000cells per Lab-Tek well (Nunc; this corresponds to 1 × 10⁵ cells/cm²). Cultures prepared in this way consisted of 85-95% calbindin-D_28k-positivePurkinje cells, with <5% GFAP-positive cells. When Purkinje cellsand granule cells were cocultured, the granule cells were platedfirst in serum-free medium, and Purkinje cells were plated ontop of the granule cells on the next day.

Granule cell purification. Cerebellar granule neurons were purified as previously described (Hatten, 1985; Baird et al., 1992).Briefly, cerebella were collected and digested as for the mixedcerebellar cultures (above), resuspended in CMF-PBS with DNase,and put through a two-step Percoll gradient. The dense cell fractionat the interface between the 35 and 60% Percoll phases was collected,and non-neuronal cells were removed by two sequential platingson Petri dishes precoated overnight with poly-D-lysine (100 µg/ml;Sigma) and washed as for the Lab-Tek wells. Nonadherent neuronalcells were collected, centrifuged at 1100 rpm for 5 min, counted,and plated into poly-D-lysine-coated Lab-Tek wells at 300,000cells per well (this corresponds to 11 × 10⁵ cells/cm²). Cultures purified in this way consisted of ~95% granule cellsand typically contained <5% GFAP-positive cells.

Growth factors, blocking antibodies, and glutamate receptor antagonists. Growth factors and TrkB-IgG were generously providedby Dr. G. Yancopoulos (Regeneron Pharmaceuticals, Tarrytown, NY).For each cerebellar cell combination, dose-response curves weregenerated for each growth factor. Subsequent experiments weredesigned to include concentrations of each growth factor thatgave maximal Purkinje cell survival at 6 and 14 days in vitro(div). Optimal growth factor concentrations were as follows: NT-3,50 ng/ml; NT-4, 50 ng/ml; BDNF, 10 ng/ml; and CNTF, 10 ng/ml.TrkB-IgG was used at a final concentration of 25 µg/ml.

Turkey polyclonal anti-BDNF antiserum (Ghosh et al., 1994) was obtained from Dr. J. Carnahan (Amgen, Thousand Oaks, CA) andused at a final dilution of 1:100.

The NMDA receptor antagonist D-APV and the non-NMDA receptor antagonist CNQX were purchased from Tocris Cookson and used at50 µM.

Immunocytochemistry. Purkinje cells were visualized as previously published (Baptista et al., 1994) by immunostaining witha rabbit polyclonal antibody against calbindin-D_28k (Swant, Bellinzona,Switzerland). This marker has been shown to label Purkinje cellsspecifically within the cerebellum (Wassef et al., 1985; Christakoset al., 1987). In some experiments, glial cells were identifiedby immunostaining with a rabbit polyclonal antibody against glialfibrillary acidic protein generously supplied by Dr. R. Liem (ColumbiaUniversity).

Cell cultures were fixed in 4% paraformaldehyde in 0.1 M Sorensen's phosphate buffer, pH 7.4, for 30 min at room temperatureand washed three times with PBS. Cultures were blocked with 10%normal goat serum in PBS containing 0.05% Triton X-100 for 30min. Cultures were incubated overnight at 4°C with primary antibodydiluted 1:1000 in PBS containing 1% normal goat serum and 0.05%Triton X-100 and then washed three times with PBS. Cultures wereincubated with goat anti-rabbit peroxidase- or rhodamine isothiocyanate-conjugatedsecondary antibody (Boehringer) diluted 1:100 in PBS containing1% goat serum and 0.05% Triton X-100 for 30 min at room temperatureand washed three times with PBS. When Hoechst staining was desired,cultures were incubated for 10 min at room temperature in PBScontaining 5 µg/ml Hoechst 33258 (Boehringer Mannheim) betweenthe second and third washes. The peroxidase reaction was developedwith 0.5 mg/ml diaminobenzidine (Wako Chemicals, Richmond, VA)and 0.006% H₂O₂ in PBS. Cultures stained with peroxidase-conjugatedsecondary antibody were dehydrated through an ethanol series andmounted in Permount. Cultures stained with rhodamine-conjugatedsecondary antibody and Hoechst 33258 were mounted in GelMount(BioMeda) and photographed on a Zeiss AxioPhot.

Analysis of cultures. Purkinje cell survival was determined by counting all of the calbindin-positive cells in each Lab-Tekwell using a Nikon Optiphot microscope with a 20× objective. Thepercentage of control cell survival for each treated well wasdetermined by dividing the calbindin-positive cell count fromthat well by the cell count from its matched, untreated controlwell. All Purkinje cell survival estimates were made from at leasttwo wells from each of at least three independent experiments,giving a total well number of at least six for each estimate.Calbindin-positive Purkinje cells were photographed using the20× or 63× objectives on a Zeiss Axiophot with Nomarski optics.

Granule cell survival in Purkinje-granule cell cocultures was estimated by counting calbindin-D_28k-negative granule cellswith phase optics in eight randomly selected field positions usinga Leitz Orthoplan microscope with a 63× objective and a cameralucida to mark the counted cells. This sample area contained 2000-3000granule cells, representing ~1.4% of the total Lab-Tek well surface.The percentage of control granule cell survival was calculatedas described for Purkinje cell survival above. Granule cell survivaldata for glutamate antagonist and TrkB-IgG experiments were collectedfrom at least two wells from each of at least three independentexperiments, giving a total well number of at least six for eachestimate. Granule cell survival data for anti-BDNF experimentsrepresent five wells from a total of three independent experimentsand four wells from two independent experiments, respectively.

Statistical analysis. Statistical comparisons were performed using the SAS software package or using Microsoft Excel pairedt tests. ANOVA was conducted using the SAS General Linear Models(GLM) procedure, which performs calculations similar to thoseof the ANOVA procedure but is preferable for data sets containingunequal sample sizes. For Figure 2, raw numbers of surviving Purkinjecells were compared with untreated, matched controls using GLMwith Dunnett's t tests. For Figure 3, Purkinje cell survival ingrowth factor-treated cultures was normalized to a percentageof survival in cultures with serum-free medium, and the differencesin survival between serum-containing and serum-free conditionswere compared within each growth factor treatment using pairedt tests. For Figures 4 and 5, raw numbers were converted to apercentage of untreated control cell survival and then comparedwith survival in BDNF-treated cultures using GLM with Dunnett'st tests.

  RESULTS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Effects of neurotrophins on Purkinje cell survival

As a first approach to exploring the involvement of neurotrophins in Purkinje cell survival and development, we decided tostudy cerebellar cells in culture. This approach permits analysisof growth factor activities in a defined, serum-free medium, avoidingthe confounding effects of additional growth factors present inserum. It also facilitates study of specific cell-cell interactionsby allowing subsets of cells to be purified and selectively recombined.These advantages can help distinguish the direct effects of growthfactors from those that are mediated indirectly, through othercell types, thus complementing in vivo approaches.

To determine the effects of neurotrophins on Purkinje cells in cultures containing defined cell populations, three cell combinationswere studied: purified Purkinje cells cultured alone, purifiedPurkinje cells cocultured with purified granule cells, and mixedcultures from whole cerebella. Cerebellar granule neurons werepurified and plated onto Nunc Lab-Tek wells at a density of 300,000cells per well (~11 × 10⁵ cells/cm²). Purkinje cells were purified and plated at 30,000 cells perwell. Mixed cultures were prepared by dissociating whole cerebellaand plating 300,000 cells per well. All cultures were grown inserum-free medium unless otherwise indicated. Plated cells wereallowed to attach to the culture substrate for 60-90 min, andthen the medium was changed to medium including growth factors,neurotrophin-blocking reagents, or glutamate receptor antagonists.After the day of plating, the medium was changed every 3-4 d,and each medium change included fresh growth factors or blockingreagents.

Purkinje cell development in cultures of dissociated whole cerebellum or in cocultures of purified Purkinje and granule neuronsmimics development in vivo. At E17-P2 in vivo or 7 div, Purkinjecells have numerous short perisomatic processes. By postnatalday 7 in vivo or 14 div, apical dendrites emerge, bearing spinesthat receive synapses from granule cell parallel fibers (Fig.1C,E). By P10-adult in vivo or 21 div, higher-order dendrite branchingand high-density spines with synapses are well established (Weberand Schachner, 1984; Hockberger et al., 1989; Armengol and Sotelo,1991; Schilling et al., 1991; Baptista et al., 1994). We choseto examine Purkinje cell survival and development at 6 div, duringinitial dendrite development, and 14 div, a time when Purkinjecell dendrites are maturing and receiving granule cell synapses.Cultures were fixed with 4% paraformaldehyde at 6 or 14 div andimmunostained with an antibody against calbindin-D_28k, a markerfound throughout the brain but specific within the cerebellumfor Purkinje cells (Wassef et al., 1985; Christakos et al., 1987).

View larger version (106K):
[in this window]
[in a new window]
Figure 1. Purkinje cell development with and without granule cell afferents and BDNF. A, B, Purkinje cells cultured alone; C-F, Purkinje cells cocultured with granule cells; A, C, E, no BDNF added; B, D, F, with BDNF. All cultures were fixed at 14 div and immunostained with anti-calbindin_D2Bk peroxidase. Scale bars: A-D, 50 µm; E, F, 10 µm.

Purkinje cell survival is profoundly affected by cell context. Purkinje cells cultured alone, with no growth factor treatment,yield relatively fewer surviving cells than Purkinje cells coculturedwith granule cells or in mixed cerebellar cultures (Baptista etal., 1994) (Table 1). To facilitate comparison of growth factoreffects among different cell combinations, normalization to survivalin control cultures is necessary. Purkinje cell survival in treatedcultures is therefore expressed as a percentage of survival inmatched, untreated control cultures having the same cell combinationat the same time point.


View this table:
[in this window]
[in a new window]
Table 1. Cell context affects Purkinje cell survival

Trophic factor modulation of Purkinje cell survival was examined using three different cell combinations: Purkinje cells alone,Purkinje cells cocultured with granule neurons, and mixed cerebellarcells. Cultures were treated with each of four growth factors:NT-3, NT-4, BDNF, and CNTF. The concentration of growth factorsused was determined by generating dose-response curves for eachcell combination with each growth factor at concentrations rangingfrom 0.1 to 1000 ng/ml (data not shown). For Purkinje cells culturedalone, 50 ng/ml NT-4 or 10 ng/ml BDNF gave optimal increases insurvival relative to those in untreated control cultures at 14div (Fig. 2A). In contrast, 50 ng/ml NT-3 or 10 ng/ml CNTF decreasedPurkinje cell survival at 6 or 14 div (Fig. 2A). No higher orlower growth factor concentrations from the dose-response experimentsgave greater Purkinje cell survival for any of the three cellcombinations. All subsequent experiments were therefore conductedusing these concentrations of growth factors.

View larger version (26K):
[in this window]
[in a new window]
Figure 2. Cell context alters trophic factor modulation of Purkinje cell survival. A, Purkinje cells cultured alone; B, Purkinje cells cocultured with granule cells; C, mixed cultures of whole cerebellum. Purkinje cell survival is represented as a percentage of the Purkinje cell number in untreated, matched control cultures at each time point. Error bars indicate SE. div, Days in vitro. Line, 100% of control cell survival. Asterisks, Statistically significant differences from untreated control cell survival; *p < 0.05; **p < 0.01.

BDNF or NT-4 increased survival of Purkinje cells cultured alone (Fig. 2A). When Purkinje cells were cocultured with granuleneurons, their normal presynaptic afferents (Fig. 2B), or whenPurkinje cells were cultured in the presence of mixed cerebellarcells (Fig. 2C), the survival-enhancing effects of NT-4 or BDNFapparent in Purkinje cells cultured alone were counteracted. AlthoughNT-4 in cultures of Purkinje cells alone at 14 div gave 148% ofuntreated control cell survival, NT-4 in Purkinje-granule coculturesgave only 13% of control cell survival, and NT-4 in mixed culturesgave 29% of control cell survival (Fig. 2). Although BDNF in culturesof Purkinje cells alone at 14 div produced 147% of control cellsurvival, addition of BDNF when granule cells were present reducedPurkinje cell survival to 24% of control levels, and BDNF treatmentof mixed cultures reduced Purkinje cell survival to 33% of controllevels. NT-3 or CNTF treatment decreased Purkinje cell survivalin all cell combinations tested (Fig. 2). All combinations ofthese four growth factors were also tested, but no combinationincreased Purkinje cell survival above that in the singly treatedcultures (data not shown).

In summary, although BDNF or NT-4 increased the survival of purified Purkinje cells cultured alone, addition of exogenousneurotrophins when Purkinje and granule cells were both presentresulted in Purkinje cell death.

BDNF and Purkinje cell dendritic differentiation

Purified Purkinje cells cultured alone extend axons but develop only rudimentary, unbranched dendrites resembling the "perisomaticprocess" stage of Purkinje cells in vivo (Baptista et al., 1994)(Fig. 1A). Purified Purkinje cells cultured with granule neuronselaborate axons and mature, highly branched dendrites bearingspines (Baptista et al., 1994) (Fig. 1C). Despite the increasein purified Purkinje cell survival with BDNF or NT-4 treatment(Fig. 2A), none of the growth factors tested triggered developmentof mature dendrites in cultures containing only purified Purkinjecells (Fig. 1B) (data not shown). In neurotrophin-treated coculturescontaining Purkinje and granule cells, Purkinje cell survivalwas reduced relative to untreated controls, but the Purkinje cellsthat did survive developed dendrites with branch orders similarto those in untreated control cultures (Fig. 1C-F). BDNF treatmentof cocultures seemed to increase spine density (Fig. 1E,F). Theseresults will be detailed in a separate report. Combined with recentdata on Purkinje cell development in BDNF^/ mice (Schwartz et al., 1997), these effects on spine densityimply that BDNF may be required for at least two stages of Purkinjecell dendrite development (see Discussion).

Serum alters responses to growth factor treatment in mixed cultures

BDNF or NT-4 increases survival of purified Purkinje cells cultured alone, and NT-3 or CNTF decreases survival of purifiedPurkinje cells whether they are cultured alone or with granulecells. These results are in marked contrast to previous studiesthat showed that BDNF decreases (Mount et al., 1993), CNTF increases(Larkfors et al., 1994, 1996), and NT-3 either boosts (Mount etal., 1994) or has no effect on (Lindholm et al., 1993) Purkinjecell survival. Several factors could account for the differencesbetween the experiments presented here and those from other laboratories.The first difference is that all of the latter studies used culturesof mixed cerebellar neurons and glia, rather than purified cells.The second difference is that others frequently used serum-containingmedium, rather than the serum-free medium used here. The thirddifference is that others used animals of ages different fromthose used here. To determine the source of the differences betweenour results and those published previously, we compared the effectsof neurotrophins on matched mixed cerebellar cultures, from animalsof different ages, using serum-containing or serum-free media.

Under control conditions with no growth factor treatment in mixed cultures from P0 cerebella, more Purkinje cells survivein serum-free medium than in horse serum-containing medium (Fig.3; p < 0.05). This trend is reversed when serum and neurotrophinsare present together; a higher percentage of Purkinje cells surviverelative to controls in neurotrophin-treated cultures with serum-containingmedium than with serum-free medium (Fig. 3). Only CNTF treatmentgave better Purkinje cell survival with serum-free medium thanwith serum. It therefore seems likely that serum affects neurotrophineffects on Purkinje cell survival, explaining part of the differencebetween our results and previous reports.

View larger version (41K):
[in this window]
[in a new window]
Figure 3. Serum alters responses to growth factor treatment in mixed cultures. Purkinje cell survival is represented as a percentage of Purkinje cell number in untreated cultures with serum-free medium. Fewer untreated Purkinje cells survive in horse serum than in serum-free medium, but this trend is reversed when serum and neurotrophins are present together. Mixed cerebellar cells from perinatal mice were cultured in serum-free medium or in medium containing 10% horse serum for 14 div. Error bars indicate SE. Asterisks, Significant differences between serum-free and serum-containing conditions; *p < 0.05; **p < 0.01.

Another difference between our experiments and those from other laboratories is the age of the animals used to prepare cultures.The present experiments studied Purkinje cells purified from perinatalmice, whereas other laboratories have used mixed cultures of cerebellarcells from E16 rats. Experiments comparing neurotrophin effectson purified cells from animals of different ages were not possiblein the present study, because the Purkinje cell purification protocolin its present form requires perinatal animals. Surface levelsof GD3 and Thy 1.2, the cell surface markers used for the immunopanningsteps in the purification procedure, are optimal at perinatalages. Comparison of mixed cerebellar cultures from P0 and E14mice, however, revealed no age-related differences in the deleteriouseffects of NT-3, NT-4, or BDNF on Purkinje cell survival underserum-free conditions (data not shown). More Purkinje cells inCNTF-treated mixed cultures survived when the cultures were preparedfrom E14 rather than P0 mice, although we did not observe an increasein Purkinje cell survival over 100% of untreated control levelswith CNTF treatment, as had been previously reported.

Taken together, these results implicate serum in altering the response of Purkinje cells to neurotrophin treatment. Althoughinclusion of serum does not explain all of the previously mentionedquantitative differences in Purkinje cell survival, other uncontrolledfactors, such as different degrees of glial contamination in previousreports, may also account for some differences between our resultsand those of others.

BDNF-blocking reagents counteract BDNF-induced toxicity of Purkinje cells cocultured with granule cells

The expression patterns of neurotrophins and their receptors within the cerebellum suggest a mechanism for neurotrophin-inducedPurkinje cell loss when Purkinje cells are cocultured with theirgranule cell afferents. Granule cells express BDNF RNA (Hoferet al., 1990; Lindholm et al., 1993; Rocamora et al., 1993) andTrkB receptors (Gao et al., 1995; Segal et al., 1995). Purkinjecells, the postsynaptic target of granule cells, do not expressRNA encoding BDNF (Hofer et al., 1990; Rocamora et al., 1993)but do contain BDNF protein (Dugich-Djordjevic et al., 1995) andTrkB receptors (Gao et al., 1995). Granule cells may thereforenormally produce BDNF that is transferred to Purkinje cells, enhancingPurkinje cell survival. Our finding that BDNF increases survivalof Purkinje cells cultured alone to 147% of the control level(Fig. 2A), combined with previous findings that granule cellsincrease survival of Purkinje cells (Baptista et al., 1994), supportsthis hypothesis. Under this model, the BDNF-induced decrease inPurkinje cell survival (toxicity) in Purkinje cell-granule neuroncocultures could be attributable to excess, exogenous BDNF beyondthe levels of BDNF normally supplied to Purkinje cells by thegranule neurons.

To test the hypothesis that BDNF in excess of that provided by granule cells becomes toxic to Purkinje cells in granule-Purkinjecell cocultures, either TrkB-IgG fusion protein or anti-BDNF antiserumpreviously shown to block BDNF signaling (Ghosh et al., 1994)was added to the culture medium. As in the experiments shown inFigure 2, BDNF treatment decreased the survival of coculturedPurkinje cells relative to that of untreated controls (Fig. 4).TrkB-IgG fusion protein was more efficient than anti-BDNF at rescuingPurkinje cells from BDNF-induced death (Fig. 4). At 6 div, TrkB-IgGincreased Purkinje cell survival in BDNF-treated cocultures from31 to 89% of control survival (p < 0.01). At 14 div, TrkB-IgGincreased Purkinje cell survival from 17 (BDNF-only) to 98% (BDNFplus TrkB-IgG) of control survival (p < 0.01). TrkB-IgG alonehad little or no effect on Purkinje cell survival (Fig. 4A). Possibleexplanations for this result are explored in Discussion.

View larger version (34K):
[in this window]
[in a new window]
Figure 4. Reagents that block BDNF signaling block BDNF-induced toxicity of Purkinje cells cocultured with granule cells. A, TrkB-IgG fusion protein experiments; B, anti-BDNF antiserum experiments. Purified Purkinje and granule cells were cultured in serum-free medium for 6 or 14 div, with or without 10 ng/ml BDNF, TrkB-IgG fusion protein (final concentration, 25 µg/ml), or turkey anti-BDNF antiserum (final dilution, 1:100). Purkinje cell survival is represented as a percentage of the Purkinje cell number in matched control cultures at each time point. Error bars indicate SE. div, Days in vitro; Ab, anti-BDNF. Asterisks, Statistically significant differences from BDNF-treated cultures; *p < 0.05; **p < 0.01.

Inclusion of anti-BDNF in the medium of cultures treated with BDNF produced a partial rescue from BDNF-induced Purkinje celldeath. This rescue was specific, because treatment of Purkinje-granulecocultures (or of Purkinje cells cultured alone) with anti-BDNFalone did not alter Purkinje cell survival relative to that inuntreated control cultures (Fig. 4B) (data not shown). At 6 div,treatment with BDNF gave 56% of control cell survival, whereastreatment with BDNF and antibody gave 80% of control cell survival(Fig. 4B). At 14 div, BDNF treatment gave 25% of control cellsurvival, whereas addition of BDNF and antibody gave 54% of controlcell survival, double that in cultures treated with BDNF alone(Fig. 4B).

These results are consistent with the hypothesis that BDNF in excess of that normally supplied by the granule cells is toxicto Purkinje cells.

CNQX, but not APV, rescues cocultured Purkinje cells from BDNF toxicity

BDNF (or other neurotrophins) increases synaptic transmission in hippocampal slices and in the neuromuscular junction (Kangand Schuman, 1995; Stoop and Poo, 1996). We therefore hypothesizedthat if the glutamatergic granule cells release glutamate in responseto BDNF treatment, decreased survival of Purkinje cells coculturedwith granule cells and treated with BDNF might be caused by glutamate-inducedexcitotoxicity. In support of this idea, dose-response curvesrevealed that glutamate added to cultures of purified Purkinjecells decreased their survival, even at concentrations as lowas 3 µM (data not shown). Glutamate receptor antagonists wereused in an attempt to block BDNF-induced toxicity in granule cell-Purkinjecell cocultures treated with BDNF. The non-NMDA receptor-specificantagonist CNQX partially rescued Purkinje cell survival in BDNF-treatedcocultures with granule cells (Fig. 5A; p < 0.01 at 6 or 14 div),whereas the NMDA receptor-specific antagonist APV failed to rescuecocultured Purkinje cells treated with BDNF (Fig. 5B). Neitherantagonist alone changed the percentage of Purkinje cell survivalin cocultures without BDNF (Fig. 5A,B). These results supportthe growing literature describing non-NMDA receptor-mediated formsof excitotoxicity (Tokita et al., 1996; Pozas et al., 1997), implicatingnon-NMDA receptor-mediated glutamate excitotoxicity as a mechanismof BDNF-induced cell death in cocultures of Purkinje and granulecells.

View larger version (34K):
[in this window]
[in a new window]
Figure 5. CNQX, but not APV, rescues Purkinje cells from BDNF toxicity. A, Experiments with CNQX; B, experiments with APV. Purified Purkinje and granule cells were cocultured in serum-free medium for 6 or 14 div, with or without 10 ng/ml BDNF, 50 µM APV (an NMDA receptor antagonist), or 50 µM CNQX (a non-NMDA receptor antagonist). Purkinje cell survival is represented as a percentage of the Purkinje cell number in untreated control cultures at each time point. Error bars indicate SE. div, Days in vitro. Asterisks, Statistically significant differences from BDNF-treated cultures; **p, < 0.01.

BDNF-induced Purkinje cell loss is not explained by decreased granule cell number

Granule cell number can influence Purkinje cell survival in cocultures (Baptista et al., 1994). To test whether the Purkinjecell loss in BDNF-treated cocultures was secondary to decreasesin granule cell number, we counted granule cells in coculturesused for the anti-BDNF, TrkB-IgG, or CNQX experiments presentedin Figures 4 and 5 (Table 2). At 14 div, BDNF treatment reducedgranule cell survival to 66 ± 3% of control levels, compared withPurkinje cell survival at 26 ± 4% of control levels (Table 2).At 6 div, BDNF treatment decreased the number of granule cellsto 74 ± 10% of control granule cell survival levels, comparedwith Purkinje cell survival at 51 ± 8% of control levels (datanot shown). Previous work from this laboratory established thatreducing granule cell number to 72% of control granule cell levelsproduced Purkinje cell survival at 93% of control Purkinje celllevels (Baptista et al., 1994). Thus, the granule cell numberspresent in our BDNF-treated cultures are sufficient to supportfull Purkinje cell survival. Moreover, Purkinje cell survivalmay be increased independent of granule cell numbers. TrkB-IgGtreatment restores Purkinje cell survival in BDNF-treated coculturesand increases granule cell number, but CNQX treatment improvesPurkinje cell survival without significant changes in granulecell number. Anti-BDNF treatment increases Purkinje cell survivalin BDNF-treated cocultures despite decreasing the number of granulecells (Table 2). We therefore conclude that the large reductionsin Purkinje cell survival seen in BDNF-treated cocultures arenot explained by granule cell loss.


View this table:
[in this window]
[in a new window]
Table 2. Purkinje cell survival is independent of granule cell number

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

A plethora of protein and mRNA localization studies have suggested that neurotrophins function during cerebellar cell maturation,providing the impetus for testing the role of growth factors incerebellar cultures (Lindholm et al., 1993; Mount et al., 1993;Larkfors et al., 1994, 1996). We have extended these early experiments,examining neurotrophin influences on Purkinje cell survival anddendrite development using purified Purkinje cells and purifiedgranule cell afferents.

Neurotrophin effects on Purkinje cell survival vary depending on cell-cell interactions

Cerebellar granule cells contain BDNF RNA (Hofer et al., 1990; Lindholm et al., 1993; Rocamora et al., 1993). Purkinje cellsdo not express RNAs encoding BDNF or NT3 (Hofer et al., 1990;Lindholm et al., 1993; Rocamora et al., 1993) but do contain BDNFand NT3 proteins in vivo (Zhou and Rush, 1994; Dugich-Djordjevicet al., 1995). Both granule and Purkinje cells display TrkB proteinon their surfaces (Gao et al., 1995; Segal et al., 1995; Lindholmet al., 1997).

Based on these expression data and on the fact that granule cells are presynaptic to Purkinje cells, we predicted that BDNFsignaling would occur in granule-Purkinje cell cocultures andthat exogenous BDNF would affect Purkinje cell survival and/ordifferentiation. Consistent with these predictions, BDNF increasedthe survival of Purkinje cells cultured alone (Fig. 2A). In contrast,BDNF added to granule cell-Purkinje cell cocultures decreasedPurkinje cell survival (Fig. 2B) beyond levels that might be explainedby concomitant loss of granule cells (Table 2), implicating thecellular environment (absence or presence of granule cells) andcorresponding levels of BDNF and TrkB expression in determiningwhether BDNF treatment promotes survival or death of Purkinjecells.

The results presented here differ significantly from those already in the literature. Specifically, CNTF was reported to increasePurkinje cell survival above untreated controls in mixed culturesfrom E16 rats (Larkfors et al., 1994, 1996) but decreased Purkinjecell survival under our culture conditions (Fig. 2). BDNF, previouslyshown to decrease Purkinje cell survival (Mount et al., 1993),actually increased survival of purified Purkinje cells culturedalone (Fig. 2A). Comparison of our methods with those used previouslyrevealed several differences that may account for our novel results.Principal among these is use of serum-containing medium, whichalters the effects of all the growth factors tested here on Purkinjecells (Fig. 3). Our study included purified cell populations inaddition to a mixture of cerebellar cells, and our results highlightthe importance of using defined cell populations in unravelingwhich factors directly contribute to Purkinje cell survival anddifferentiation.

Neurotrophins can mediate cell death

A new view of neurotrophin action is emerging, including the concept that in addition to their growth- and differentiation-enhancingeffects, neurotrophins can induce neuronal death if introducedat improper levels or times, either through their Trk receptorsor p75, and associated neurotransmitter receptors (NGF, von Bartheldet al., 1994; Cassaccia-Bonnefil et al., 1996; Frade et al., 1996;BDNF or NT-3, Fernandez-Sanchez and Novelli, 1993, 1995; Koh etal., 1995). Such analyses led Koh et al. (1995) to propose thatalthough neurotrophins function to protect neurons from apoptosis,they also may potentiate neuronal death by necrosis (Koh et al.,1995). Results from Hoechst 33258 staining of granule-Purkinjecell cocultures support this idea. All Purkinje cells in cocultureswith granule cells at 6 or 14 div contain nuclei diffusely labeledby Hoechst staining, suggesting that any Purkinje cell death occurringat these times is necrotic (data not shown). These data indicatethat a precise balance between BDNF signaling and glutamate stimulationis vital for Purkinje cell survival, with excess BDNF triggeringPurkinje cell death.

The finding that cellular environment and/or contacts can alter Purkinje cell responses to growth factors has implicationsfor experiments involving growth factor administration to theintact nervous system (Cabelli et al., 1995; Riddle et al., 1995).In such experiments, the reagents may exert their effects indirectly,by damaging bystander cells, as well as directly, by stimulatingtarget cells. These results suggest that general application ofneurotrophins in vivo may upset critical balances and lead tounintended neuronal loss.

A model for Purkinje cell-granule neuron interactions

A model for Purkinje and granule cell interactions that hinges on a balance between glutamate stimulation and neurotrophinsignaling illuminates the effects of neurotrophins and glutamatereceptor antagonists on Purkinje cell survival. Purkinje cellscultured alone survive poorly, developing axons but not dendrites(Fig. 1A). Addition of BDNF increases survival of isolated Purkinjecells but does not drive dendritic differentiation (Fig. 1B).Granule cells cultured with Purkinje cells enhance Purkinje cellsurvival and induce dendrite formation, most likely through acombination of glutamate stimulation and BDNF production by theglutamatergic granule cells (Fig. 1C). Adding exogenous BDNF tosuch Purkinje-granule cocultures may stimulate the granule cellsto produce even more glutamate, which in turn becomes excitotoxicto the Purkinje cells. In support of this hypothesis, glutamateadded continuously to Purkinje cells cultured alone was toxicat concentrations as low as 3 µM (data not shown). Decreasingthe BDNF overload with anti-BDNF antibodies or with TrkB-IgG bringsthe system back toward the proper balance of BDNF and glutamateaction, restoring Purkinje cell survival (Fig. 4). Purkinje cellsin cocultures with granule cells also can be protected from BDNF-induceddeath by CNQX, a specific non-NMDA glutamate receptor antagonist(Fig. 5), supporting the hypothesis that Purkinje cell loss inBDNF-treated cocultures is attributable in part to glutamate excitotoxicity.This hypothesis provides one possible explanation for the lackof effects of anti-BDNF or TrkB-IgG alone on Purkinje cell survivalin cocultures (Fig. 4). Anti-BDNF or TrkB-IgG may reduce the activityof the granule cells, reducing ill effects on Purkinje cells fromoverstimulation by granule cells, thus boosting survival and counteractingthe expected reduction in Purkinje cell survival predicted fromsimple BDNF deprivation.

Alternatively, if excitation of granule cell-Purkinje cell synapses causes an increase in Purkinje cell TrkB levels, the BDNF-inducedPurkinje cell death in cocultures may be attributable to increasedsensitivity of the Purkinje cells to BDNF itself and not to glutamateexcitotoxicity. In this case, CNQX may rescue Purkinje cells inBDNF-treated cocultures by blocking the glutamate signaling thatwould normally increase TrkB expression in Purkinje cells, ratherthan by blocking direct glutamate excitotoxicity. This alternatemodel would require that the Purkinje cell distinguish betweentwo signaling conditions, responding to changes in BDNF signalingcaused by increased exogenous BDNF with increased survival versusresponding to changes in BDNF signaling caused by increased TrkBreceptor levels with decreased survival. Electrophysiologicalrecordings and measurements of levels of TrkB in cultures withand without BDNF and CNQX treatment would clarify which of thesetwo models is correct.

The role of BDNF in cerebellar development

A growth factor such as BDNF with survival effects on Purkinje cells might be expected to induce their dendritic differentiation.A precedent for single-factor induction of de novo dendrite formationis OP-1, a member of the BMP/TGF $beta$ family that has striking effectson dendrite outgrowth of sympathetic neurons (Lein et al., 1995).Indeed, NT-3 was previously reported to increase neurite outgrowthof Purkinje cells in mixed cerebellar cultures (Lindholm et al.,1993). Although BDNF and NT4 increased the survival of Purkinjecells cultured alone (Fig. 2A), none of the neurotrophins testedhere was able to induce Purkinje dendrite formation de novo, inthe absence of granule cells. These results are consistent withthe idea that CNS neurons in general may require a menu of signalsfor their survival and dendritogenesis (Meyer-Franke et al., 1995).

Our results provide an interesting counterpoint to those of Segal et al. (1995), who recently reported increased granule celldeath and stunting of Purkinje cell dendrites in BDNF^/ mice (Schwartz et al., 1997). All of the cells in these micedeveloped from their genesis in an environment lacking BDNF. Schwartzet al. (1997) concluded that BDNF acts to influence dendriticmorphology but is not required for granule cell-Purkinje cellsynapse formation. In our experimental paradigm, granule and Purkinjecells are generated and begin to develop in the presence of normalBDNF levels but are deprived of BDNF by antibody or TrkB-IgG treatmentlater on, during a 2 week culture period. Preliminary evidenceindicates that this late deprivation of BDNF does not alter dendriticbranch structure, whereas late addition of BDNF increases spinedensity (Fig. 1). Combined with the results of Schwartz et al.(1997), these observations suggest that normal Purkinje cell developmentrequires BDNF or TrkB activity during at least two distinct phases:prenatally, for effects on future branch structure, and postnatally,for effects on spine density.

BDNF effects on spine density would support the idea that neurotrophins may act on later stages of dendrite development, includinghigher-order branching and spine formation (McAllister et al.,1995, 1996, 1997), as well as on axonal outgrowth (Ghosh et al.,1994; Cohen-Cory and Fraser, 1995; Cohen-Cory et al., 1996; Sawaiet al., 1996). This is consistent with the synaptotrophic hypothesisthat neurotrophins exert their effect on neuronal growth, differentiation,and plasticity by mediating synaptic competition (Snider and Lichtman,1996). One of the predictions of this hypothesis is that neurotrophinsare released in a restricted manner, possibly at synaptic contacts.Such a mechanism is implicated by recent findings revealing arole for BDNF in synaptic plasticity (Kang and Schuman, 1995,1996; Patterson et al., 1996; Akaneya et al., 1997; Kang et al.,1997) as well as during refinement of synaptic connections (Cabelliet al., 1995, 1997; Riddle et al., 1995).

In conclusion, these experiments represent a new, reductionist approach to growth factor assays in cultures of CNS neurons,comparing the effects of specific factors on defined cell populationscultured alone with effects on the same cells in culture withtheir presynaptic partners. BDNF and NT-4 were each found to increasesurvival of Purkinje cells cultured alone. When Purkinje cellswere cocultured with their presynaptic afferent granule cells,however, the same factors triggered non-NMDA receptor-mediateddeath. These observations support the idea that the neurotrophinand neurotransmitter systems are intimately linked and must bein proper balance for neuronal survival and normal development.Further experiments will explore the effects of neurotrophinson the later stages of differentiation, including spine developmentand synaptogenesis.

  FOOTNOTES

Received Nov. 7, 1997; revised Jan. 28, 1998; accepted March 5, 1998.

This work was supported by National Institutes of Health Grant NS16951 (C.A.M.) and National Research Service Award NS09864(M.E.M.). We thank Drs. Amy MacDermott, Wilma Friedman, LloydGreene, Alcmene Chalazonitis, Domenique Toran-Allerand, Riva Marcus,Anna Dunaevsky, George Yancopoulos, and Ron Lindsay for ongoingdiscussions and advice during the course of this work. We alsothank Dr. Roger Vaughan of the Department of Public Health ofColumbia University for advice on statistical analyses and RichardBlazeski for expert assistance with the photographs. Growth factorsand TrkB-IgG were provided by Dr. G. Yancopoulos (Regeneron).Anti-neurotrophin antibodies were supplied by Dr. J. Carnahan(Amgen, Thousand Oaks, CA).
Correspondence should be addressed to Dr. Carol A. Mason, Department of Pathology, College of Physicians and Surgeons, ColumbiaUniversity, 630 West 168th Street, New York, NY 10032.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Akaneya Y, Tsumoto T, Kinoshita S, Hatanaka H (1997) Brain-derived neurotrophic factor enhances long-term potentiation in rat visual cortex. J Neurosci 17:6707-6716[Abstract/Free Full Text].
Altman J, Anderson WJ (1972) Experimental reorganization of the cerebellar cortex. I. Morphological effects of eliminating all microneurons with prolonged X-irradiation started at birth. J Comp Neurol 146:355-406[ISI][Medline].
Armengol JA, Sotelo C (1991) Early dendritic development of Purkinje cells in the rat cerebellum. A light and electron microscopic study using axonal tracing in in vitro slices. Brain Res 64:95-114.
Baird DH, Hatten ME, Mason CA (1992) Cerebellar target neurons provide a stop signal for afferent neurite extension in vitro. J Neurosci 12:619-634[Abstract].
Baptista CA, Hatten ME, Blazeski R, Mason CA (1994) Cell-cell interactions influence survival and differentiation of purified Purkinje cells in vitro. Neuron 12:243-260[ISI][Medline].
Bonhoeffer T (1996) Neurotrophins and activity-dependent development of the neocortex. Curr Opin Neurobiol 6:119-126[ISI][Medline].
Cabelli RJ, Hohn A, Shatz CJ (1995) Inhibition of ocular dominance column formation by infusion of NT-4/5 or BDNF. Science 267:1662-1666[Abstract/Free Full Text].
Cabelli RJ, Allendoerfer KL, Radeke MJ, Welcher AA, Feinstein SC, Shatz CJ (1996) Changing patterns of expression and subcellular localization of TrkB in the developing visual system. J Neurosci 16:7965-7980[Abstract/Free Full Text].
Cabelli RJ, Shelton DL, Segal RA, Shatz CJ (1997) Blockade of endogenous ligands of TrkB inhibits formation of ocular dominance columns. Neuron 19:63-76[ISI][Medline].
Cassaccia-Bonnefil P, Carter BD, Dobrowsky RT, Chao MV (1996) Death of oligodendrocytes mediated by the interaction of nerve growth factor with its receptor p75. Nature 383:716-719[Medline].
Christakos S, Rhoten WB, Feldman SC (1987) Rat calbindin D28k: purification, quantitation, immunocytochemical localization, and comparative aspects. Methods Enzymol 139:534-551[ISI][Medline].
Cohen-Cory S, Fraser SE (1995) Effects of brain-derived neurotrophic factor on optic axon branching and remodelling in vitro. Nature 378:192-196[Medline].
Cohen-Cory S, Dreyfus CF, Black IB (1989) Expression of high- and low-affinity nerve growth factor receptors by Purkinje cells in the developing rat cerebellum. Exp Neurol 105:104-109[ISI][Medline].
Cohen-Cory S, Dreyfus CF, Black IB (1991) NGF and excitatory neurotransmitters regulate survival and morphogenesis of cultured cerebellar Purkinje cells. J Neurosci 11:462-471[Abstract].
Cohen-Cory S, Escandon E, Fraser SE (1996) The cellular patterns of BDNF and trkB expression suggest multiple role for BDNF during Xenopus visual system development. Dev Biol 179:102-115[ISI][Medline].
Dugich-Djordjevic MM, Peterson C, Isono F, Ohsawa F, Widmer HR, Denton TL, Bennett GL, Hefti F (1995) Immunohistochemical visualization of brain-derived neurotrophic factor in the rat brain. Eur J Neurosci 7:1831-1839[ISI][Medline].
Ernfors P, Merlio J-P, Persson H (1992) Cells expressing mRNA for neurotrophins and their receptors during embryonic rat development. Eur J Neurosci 4:1140-1158[ISI][Medline].
Fernandez-Sanchez MT, Novelli A (1993) Basic fibroblast growth factor protects cerebellar neurons in primary culture from NMDA and non-NMDA receptor mediated neurotoxicity. FEBS Lett 335:124-131[ISI][Medline].
Fernandez-Sanchez MT, Novelli A (1995) Neurotrophins and excitotoxicity. Science 270:2019[Abstract].
Figurov A, Pozzo-Miller LD, Olafsson P, Wang T, Lu B (1996) Regulation of synaptic responses to high-frequency stimulation and LTP by neurotrophins in the hippocampus. Nature 381:706-709[Medline].
Frade JM, Rodriguez-Tebar A, Barde Y-A (1996) Induction of cell death by endogenous nerve growth factor through its p75 receptor. Nature 383:166-168[Medline].
Galuske RAW, Kim D-S, Castren E, Thoenen H, Singer W (1996) Brain-derived neurotrophic factor reverses experience-dependent synaptic modifications in kitten visual cortex. Eur J Neurosci 8:1554-1559[ISI][Medline].
Gao W-Q, Zheng JL, Karihaloo M (1995) Neurotrophin-4/5 (NT-4/5) and brain-derived neurotrophic factor (BDNF) act at later stages of cerebellar granule cell differentiation. J Neurosci 15:2656-2667[Abstract].
Ghosh A, Carnahan J, Greenberg ME (1994) Requirement for BDNF in activity-dependent survival of cortical neurons. Science 263:1618-1622[Abstract/Free Full Text].
Hatten ME (1985) Neuronal regulation of astroglial morphology and proliferation in vitro. J Cell Biol 100:384-396[Abstract/Free Full Text].
Hatten ME, Heintz N (1995) Mechanisms of neural patterning and specification in the developing cerebellum. Annu Rev Neurosci 18:385-408[ISI][Medline].
Henderson CE (1996) Role of neurotrophic factors in neuronal development. Curr Opin Neurobiol 6:64-70[ISI][Medline].
Hockberger PE, Tseng H-Y, Connor JA (1989) Development of rat cerebellar Purkinje cells: electrophysiological properties following acute isolation and in long-term culture. J Neurosci 9:2258-2271[Abstract].
Hofer M, Pagliusi SR, Hohn A, Leibrock J, Barde Y-A (1990) Regional distribution of brain-derived neurotrophic factor mRNA in the adult mouse brain. EMBO J 9:2459-2464[ISI][Medline].
Kandel ER, Schwartz JH, Jessell TM (1995) In: Essentials of neural science and behavior. Norwalk, CT: Appleton & Lange.
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].
Kang H, Schuman EM (1996) A requirement for local protein synthesis in neurotrophin-induced hippocampal synaptic plasticity. Science 273:1402-1406[Abstract].
Kang H, Welcher AA, Shelton D, Schuman EM (1997) Neurotrophins and time: different roles for TrkB signaling in hippocampal long-term potentiation. Neuron 19:653-664[ISI][Medline].
Katz LC, Shatz CJ (1996) Synaptic activity and the construction of cortical circuits. Science 274:1133-1138[Abstract/Free Full Text].
Koh J-Y, Gwag BJ, Lobner D, Choi DW (1995) Potentiated necrosis of cultured cortical neurons by neurotrophins. Science 268:573-575[Abstract/Free Full Text].
Larkfors L, Lindsay RM, Alderson RF (1994) Ciliary neurotrophic factor enhances the survival of Purkinje cells in vitro. Eur J Neurosci 6:1015-1025[ISI][Medline].
Larkfors L, Lindsay RM, Alderson RF (1996) Ciliary neurotrophic factor enhances the survival of Purkinje cells in vitro. Eur J Neurosci 6:1015-1025.
Lein P, Johnson M, Guo X, Rueger D, Higgins D (1995) Osteogenic protein-1 induces dendritic growth in rat sympathetic neurons. Neuron 15:597-605[ISI][Medline].
Leingartner A, Heisenberg C-P, Kolbeck R, Thoenen H, Lindholm D (1994) Brain-derived neurotrophic factor increases neurotrophin-3 expression in cerebellar granule neurons. J Biol Chem 269:828-830[Abstract/Free Full Text].
Levine E, Dreyfus C, Black I, Plummer M (1995) Brain-derived neurotrophic factor rapidly enhances synaptic transmission in hippocampal neurons via postsynaptic tyrosine kinase receptors. Proc Natl Acad Sci USA 15:8074-8077.
Lindholm D, Castren E, Tsoulfas P, Kolbeck R, Berzaghi MP, Leingartner A, Heisenberg C-P, Tesarollo L, Parada LF, Thoenen H (1993) Neurotrophin-3 induced by tri-iodothyronine in cerebellar granule cells promotes Purkinje cell differentiation. J Cell Biol 122:443-450[Abstract/Free Full Text].
Lindholm D, Dechant G, Heisenberg C-P, Thoenen H (1993) Brain-derived neurotrophic factor is a survival factor for cultured rat cerebellar granule neurons and protects them against glutamate-induced neurotoxicity. Eur J Neurosci 5:1455-1464[ISI][Medline].
Lindholm D, Hamner S, Zirrgiebel U (1997) Neurotrophins and cerebellar development. Perspect Dev Neurobiol 5:83-94[ISI][Medline].
Lo DC (1995) Neurotrophic factors and synaptic plasticity. Neuron 15:979-981[ISI][Medline].
Lohof AM, Ip NY, Poo M-m (1993) Potentiation of developing neuromuscular synapses by the neurotrophins NT-3 and BDNF. Nature 363:305-353[Medline].
Mariani J, Crepel F, Mikoshiba K, Changeux JP, Sotelo C (1977) Anatomical, physiological and biochemical studies of the cerebellum from reeler mutant mouse. Philos Trans R Soc Lond B Biol Sci 281:1-28[ISI][Medline].
McAllister AK, Lo DC, Katz LC (1995) Neurotrophins regulate dendritic growth in developing visual cortex. Neuron 15:791-803[ISI][Medline].
McAllister AK, Katz LC, Lo DC (1996) Neurotrophin regulation of cortical dendritic growth requires activity. Neuron 17:1057-1064[ISI][Medline].
McAllister AK, Katz LC, Lo DC (1997) Opposing roles for endogenous BDNF and NT-3 in regulating cortical dendritic growth. Neuron 18:767-78[ISI][Medline].
Meyer-Franke A, Kaplan MR, Pfrieger FW, Barres BA (1995) Characterization of the signalling interactions that promote the survival and growth of developing retinal ganglion cells in culture. Neuron 15:805-819[ISI][Medline].