Agrin Controls Synaptic Differentiation in Hippocampal Neurons

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The Journal of Neuroscience, December 15, 2000, 20(24):9086-9095

Agrin Controls Synaptic Differentiation in Hippocampal Neurons
Christian M. Böse¹, Dike Qiu¹, Andrea Bergamaschi³, Biagio Gravante³, Mario Bossi², Antonello Villa², Fabio Rupp¹, and Antonio Malgaroli³
¹ Department of Neuroscience, The Johns Hopkins University, School of Medicine, Baltimore, Maryland 21205, ² Microscopy and Image Analysis, University of Milan School of Medicine, and ³ Department of Biological and Technological Research, Scientific Institute San Raffaele, 20123 Milano, Italy

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Agrin controls the formation of the neuromuscular junction. Whether it regulates the differentiation of other types of synapsesremains unclear. Therefore, we have studied the role of agrinin cultured hippocampal neurons. Synaptogenesis was severely compromisedwhen agrin expression or function was suppressed by antisenseoligonucleotides and specific antibodies. The effects of antisenseoligonucleotides were found to be highly specific because theywere reversed by adding recombinant agrin and could not be detectedin cultures from agrin-deficient animals. Interestingly, the fewsynapses formed in reduced agrin conditions displayed diminishedvesicular turnover, despite a normal appearance at the EM level.Thus, our results demonstrate the necessity of agrin for synaptogenesisin hippocampalneurons.

Key words: agrin; synaptogenesis; synapses; primary hippocampal neurons; agrin antibodies; antisense oligonucleotides

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The fidelity of neural transmission depends on interactions of a large number of presynaptic and postsynaptic molecules. Despitethe importance of these processes for neural communication, themechanisms controlling the assembly and the targeting of moleculesto synapses remain primarily unknown (Sanes et al., 1998). Onehypothesis of synapse formation proposes that growth cones secretefactors that bind to specific receptors located on the plasmamembrane of the target cell (McMahan, 1990). Signaling cascadesactivated via these receptors lead to the recruitment and/or thetargeted insertion of postsynaptic molecules at contact sites.The discovery of the synaptic differentiation factor agrin supportsthis model (Nitkin et al., 1987). Agrin is an extracellular matrixproteoglycan necessary for the aggregation of the ACh receptor(AChR) at developing neuromuscular junctions (NMJs), which istranscribed from a single gene but exists in different isoformsthat are produced by alternative splicing (Rupp et al., 1991,1992; Ruegg et al., 1992; Smith et al., 1992; Tsim et al., 1992).Alternative splicing at a specific site, referred to as the z-sitein rodents, affects the AChR-clustering activity of agrin (Fernset al., 1992, 1993; Ruegg et al., 1992). Recently, mice that eitherexpress extremely low levels of agrin transcripts or do not expresshighly active (z+) isoforms have been produced. The phenotypeof these mutations is very similar; homozygous mutant embryosdie late during gestation, and a dramatic reduction in number,size, and density of AChR clusters is observed at NMJs (Gautamet al., 1996; Burgess et al., 1999). These results, together withexperiments using anti-agrin antibodies to block agrin functionin vitro (Cohen and Godfrey, 1992; Reist et al., 1992; Campagnaet al., 1997), demonstrate that agrin is necessary for the differentiationofNMJs.

Despite the evidence supporting the role of agrin in the formation of NMJ, it is still unknown whether synaptogenesis in theCNS is regulated similarly. A series of observations suggeststhat agrin may have a more widespread role and may also controlthe formation of synapses in the CNS. Agrin mRNA and immunoreactivitycan be detected in CNS neurons, where the temporal pattern ofexpression of agrin parallels synaptogenesis (Hoch et al., 1993;O'Connor et al., 1994; Stone and Nikolics, 1995; N. A. Cohen etal., 1997). Agrin is targeted to axons in spinal cord neurons,and it is secreted from hippocampal neurons (Dutton et al., 1995;Escher et al., 1996). Electrical activity regulates agrin expressionin hippocampal neurons (O'Connor et al., 1995; N. A. Cohen etal., 1997). Agrin z(+), but not z( $-$ ), isoforms are able to inducethe phosphorylation of the transcription factor cAMP responseelement-binding protein (CREB) in primary hippocampal neurons(Ji et al., 1998). In addition, a recent study suggests that diminishedagrin expression leads to morphological and synaptic alterationsin primary hippocampal neurons (Ferreira, 1999). However, synaptogenesisoccurs normally in primary hippocampal and cortical neurons derivedfrom agrin-deficient mice (Li et al., 1999; Serpinskaya et al.,1999). A caveat in assessing results obtained from null-mutantmice produced by homologous recombination is the possibility offunctional redundancy and/or activation of compensatory mechanismsduring development. To avoid these complications, we tested thepossibility that agrin functions as a synaptic differentiationfactor in primary hippocampal neurons. This type of neuronal cultureis particularly suited for studies of synaptogenesis because themolecular events associated with the culture and the kineticsof synaptic differentiation have been well characterized and becausethese neurons form functional synapses (Fletcher et al., 1991;Malgaroli et al., 1995; Rao et al., 1998). Our results show thatsynaptic differentiation was inhibited when agrin expression orfunction was suppressed by either agrin-antisense oligonucleotidesor anti-agrin antibodies, thus demonstrating the requirement ofagrin for synaptogenesis in hippocampalneurons.

  MATERIALS AND METHODS

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MATERIALS AND METHODS
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Antibodies. Monoclonal antibodies specific for synaptophysin, microtubule-associated protein 2 (MAP-2), actin, and GABA_A werepurchased from Boehringer Mannheim (Indianapolis, IN); those foragrin (m247 and m33) were from StressGen Biotechnologies (Victoria,British Columbia, Canada). Antibodies specific for neuron-specificenolase, synapsin-I, glutamic acid decarboxylase, postsynapticdensity 95 (PSD-95), and CREB were purchased from Polysciences(Warrington, PA), Molecular Probes (Eugene, OR), Chemicon (Temecula,CA), Affinity Bioreagents (Golden, CO), and New England Biolabs(Beverly, MA), respectively. Antibodies against NR1 were a kindgift from Dr. R. Huganir (Johns Hopkins University, Baltimore,MD). A polyclonal serum specific for GluR1 was raised as described(Molnar et al., 1994). Secondary antibodies conjugated with indocarbocyanine,FITC, and Texas Red were purchased from Jackson ImmunoResearch(West Grove,PA).

Oligonucleotides. Oligonucleotides were synthesized by Oligos Etc. (Wilsonville, OR). All oligonucleotides used in this studywere chimeric phosphorothioates (first and last three residues).The antisense oligonucleotides AS and AS2 are overlapping sequencestargeted to regions of the rat agrin cDNA spanning the presumptivestart codon, and the antisense oligonucleotide ASY is targetedto the Y insertion site (Rupp et al., 1991). The sense oligonucleotideS was synthesized as the reverse complement of the antisense oligonucleotideAS. The scrambled oligonucleotide SC has the same base compositionas the antisense oligonucleotide AS but in a random order. Nucleotidesequences are as follows: AS, 5'-GGAGGCATGATACATACAGCTCGAGC-3';AS2, 5'-TTCCAGTGGCAGAGGAGGCATGATAC-3'; ASY, 5'-GGAACCTTGCGGGATTTCGGAGATTC3';SC,5'-TGCGGTACGGAAGACACTCCATAAGG-3'; and S, 5'-GCTCGAGCTGTATGTATCATGCCTCC-3'.None of the sequences shows significant homology to known genesin the GenBank database. The oligonucleotides were added at theonset of the cultures and subsequently every 3 d at the concentrationsindicated. The quality of the oligonucleotides is crucial becausebatches from other suppliers were cytotoxic at much lowerconcentrations.

Synaptosome preparations. Synaptosomes were prepared as described (Whittaker, 1984) from hippocampi of 21-d-oldrats.

Hippocampal cell cultures. Primary hippocampal cell cultures from 3- to 5-d-old [postnatal day 3 (P3)-P5] Sprague Dawley ratswere prepared as described previously (Malgaroli et al., 1995;Ji et al., 1998). Briefly, hippocampi were rapidly dissected,dissociated by trypsinization and gentle trituration, and platedonto precoated (poly-D-lysine or poly-D-ornithine; 10 µg/ml) glasscoverslips or Permanox chamber slides (Nalge Nunc, Naperville,IL). Cell cultures from embryonic day 17 (E17) agrin-deficientmice were prepared as described above with the exception thathippocampal cells from each embryo were processed and culturedindividually.

Purified recombinant agrin isoforms (50 pM) (Campanelli et al., 1996) were added as described for the oligonucleotides. Agrin(m247) and control antibodies (mouse $alpha$ rat IgG; Jackson ImmunoResearch)were applied at 150 µg/ml once at the onset of thecultures.

Reverse transcription-PCR analysis. Total RNA was prepared from hippocampal cell cultures by the use of TRIZOL (Life Technologies,Gaithersburg, MD) according to the manufacturer's protocol. cDNAsynthesis was performed in 15 µl of 1× Superscript II reversetranscription (RT) buffer, 200 µM deoxynucleotide triphosphates(dNTPs), 5 µCi of [ $alpha$ -³²P]dCTP (NEN, Boston, MA), 10 mM DTT with 200 U of SuperscriptII (Life Technologies), and 0.5 µg/ml oligo-dT (Pharmacia Biotech,Piscataway, NJ) for 90 min at 37°C and terminated by heating at65°C for 20 min. PCR amplifications with agrin-specific primers(0.2 µM) and 1 µl of cDNA were performed in 50 µl containing 1×PCR reaction buffer, 1.5 mM MgCl₂, 0.5 mM dNTPs, and 1 U of Taqpolymerase (Display Systems Biotechnology, Vista, CA). Cycle parameterswere 1 min at 95°C, 1 min at 60°C, and 2 min at 72°C for 25 cycles.At these parameters the amplification reactions were in the exponentialphase. Ten microliters of the reaction products were separatedon 8% polyacrylamide gels. Signals for the individual isoformswere visualized and quantified by the use of a PhosphorImagerand ImageQuant 3.3 software (Molecular Dynamics, Sunnyvale, CA).Control PCR amplifications were performed in a similar mannerusing glyceraldehyde-3-phosphate dehydrogenase (GAPDH)-specificprimers. Primer sequences are as follows: rat agrin forward andreverse primers, 5'-CACTGGCCTTTGATGGGCGG-3' and 5'-GTCATAGCT-CAGTTGCAGGT-3',respectively; and rat GAPDH forward and reverse primers, 5'-ACCACAGTCCATGCCATCAC-3'and 5'-TCCACCACCC-TGTTGCTGTA-3', respectively. Data were analyzedby the use of the Student's t test, and the criterion for statisticalsignificance was p < 0.01.

Western blot analysis. Cells from hippocampal cultures were scraped into cold lysis buffer containing 1% Triton X-100, 10%glycerol, 20 mM Tris-HCl, pH 8.0, 150 mM NaCl, 0.5 mM EDTA, 0.5mM EGTA, 1 mM sodium vanadate, and protease inhibitors. Afterincubation on ice for 30 min, the insoluble material was removedby centrifugation at 16,000 × g for 3 min at 4°C. The proteincontent of the samples was assessed via the ABC method with akit from Pierce (Rockford, IL). Equal amounts of protein wereseparated on 3-8% Tris-acetate SDS-PAGE gels (Novex, San Diego,CA) and transferred onto polyvinylidene difluoride membranes.After incubation in blocking buffer (PBS containing 3% casein)for 1 hr at room temperature, blots were probed with the monoclonalantibody m33 overnight at 4°C. Membranes were exposed to a horseradishperoxidase-conjugated anti-mouse IgG secondary antibody (Amersham,Arlington Heights, IL), and the signal was visualized via enhancedchemiluminescence (ECL Plus; Amersham) onto x-ray film. The blotswere stripped and reprobed with differentantibodies.

Immunocytochemistry. Hippocampal cell cultures on glass coverslips or Permanox chamber slides were fixed with 4% paraformaldehydeand 4% sucrose in PBS and permeabilized with blocking solution(0.4% BSA and 0.4% saponin in PBS). Incubation with primary antibodieswas performed in blocking solution overnight at 4°C. After washing,cells were incubated at room temperature with species-specificfluorochrome-conjugated secondary antibodies. Fluorescence-containingimages were captured with a CCD camera (Dage-MTI, Michigan City,IN) mounted on a Nikon TE 3000 using IP Lab 1.3 software (Scanalytics,Fairfax, VA). Quantification of the number of synapses and/orimmunoreactive clusters per neurite area was performed by countingfluorescent puncta on neurites longer than 100 µm. Only punctaof threefold or greater intensity above the background fluorescenceof the process were considered. No distinction between dendritesand axons was made, and values were normalized for length andthickness of theprocesses.

Electron microscopy. Standard electron microscopy was performed as described previously (Forti et al., 1997). Briefly, cellmonolayers were washed with control Tyrode solution, fixed with2% glutaraldehyde and 4% paraformaldehyde in 0.1 M cacodylatebuffer (45 min; 24°C), and post-fixed with 2% OsO₄. After dehydrationin ethanol and overnight infiltration (75% Epon 812 and 25% ethanol),samples were embedded in Epon. Ultrathin serial sections (~60nm) were doubly stained with uranyl acetate and lead citrate andexamined with a Hitachi H-7000microscope.

Electrophysiological recordings. Hippocampal neurons were continuously perfused with a Tyrode solution containing 119 mM NaCl,5 mM KCl, 2 mM CaCl₂, 2 mM MgCl₂, 25 mM HEPES, 30 mM glucose,100 µM picrotoxin (Sigma, St. Louis, MO), and 25-100 µM APV (TocrisCookson, St. Louis, MO), adjusted to 305 mOsm and pH 7.4. Patchelectrodes (2-5 M $Omega$ ) contained 110 mM Cs-gluconate, 5 mM MgCl₂,10 mM NaCl, 0.6-10 mM EGTA or BAPTA, 2 mM ATP, 0.2 mM GTP, and49 mM HEPES, adjusted to pH 7.2 and 290 mOsm. Minis were recordedin 0.5 µM tetrodotoxin (TTX; Latoxan, Rosans, France). Other reagentswere obtained from Sigma except as noted. Synaptic currents wererecorded using an Axopatch 1D amplifier (Axon Instruments, FosterCity, CA). Recordings were obtained at the soma of neurons usingthe standard whole-cell configuration. Each cell was held at amembrane potential (V_hold) of $-$ 50 or $-$ 70 mV, and the series resistance(5-20 M $Omega$ ) was monitored by applying 1-5 mV depolarizing pulses.Presynaptic neurons were stimulated in the vicinity of the cellsoma using brief (100 µsec) constant-current injections deliveredthrough small glass electrodes filled with physiological saline.Current traces were filtered at 2-5 kHz and stored using a digitaltape recorder. Data were digitized off-line from the tape at 10-70kHz after low-pass filtering at 3-5 kHz. The detection of miniatureevents was semiautomatically performed, as described previously(Forti et al., 1997). Briefly, miniature excitatory synaptic currents(minis) were detected using two threshold-crossing criteria onthe current signal and on its first derivative (thresholds, threetimes background SD). Computer simulations estimated the undetectedevents to be <3% for signal-to-noise ratios (S/N) >4 and <20%for S/N between 3 and4.

Antibody uptake experiments. Hippocampal cultures were grown on glass coverslips for $>=$ 15 d. Cultures were incubated for 1hr at 37°C in serum-free medium containing antibodies (affinity-purifiedrabbit polyclonal serum) specific for the intravesicular N-terminalportion of synaptotagmin-I (Malgaroli et al., 1995) and 1 µM TTX.Cells were washed with Tyrode solution (37°C) and with PBS at4°C, fixed in 4% paraformaldehyde, and permeabilized for 1-2 hrat room temperature with 1% BSA and 0.4% saponin in PBS. Synapsesand dendrites were then retrospectively stained using antibodiesspecific for synaptotagmin-I (goat) and MAP-2 (mouse). Species-specific,fluorochrome (DTAF-, Cy5-, or Texas Red)-conjugated secondaryantibodies were used at 1:100 dilutions (Chemicon and JacksonImmunoResearch). Coverslips were washed with PBS and mounted onglass slides in Slowfade (Molecular Probes). Microscopy and confocalimaging were performed using an upright Zeiss Axiophot microscope(60× oil-immersion objective) equipped with a 1024 Bio-Rad confocalsystem with an argon-krypton laser (Bio-Rad). For data analysis,synapses (synaptotagmin-I, goat antibody, and immunoreactive puncta)were identified on the basis of intensity and shape parametersby the use of a computer program written in-house. Fluorescenceintensity from the internalized antibody (rabbit) was then measuredon a different excitation/emission channel. Values of intensitywere determined near the middle of individual boutons and usedfor analysis if they exceeded three times the SD of backgroundfluorescence.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Antisense oligonucleotide treatment reduces agrin expression specifically

Three agrin-specific antisense oligonucleotides (referred to as AS, AS2, and ASY; see Materials and Methods for details) wereused to assess agrin's function in the development of primarypostnatal rat hippocampal neurons. The hypothesis that agrin participatesin synapse formation in these neurons was reinforced by resultsindicating that agrin immunoreactivity was highly enriched insynaptosome preparations from rat hippocampus (Fig. 1E). Oligonucleotideswere applied at the onset of the cultures, which were maintainedfor 10-15 d. To control for specificity, measurements of agrinmRNA and protein levels in relation to several housekeeping andneuronal proteins were performed in cells treated with antisense,sense, and scrambled oligonucleotides. The effect of the antisenseoligonucleotide treatment on the expression of agrin mRNA wasevaluated by relative reverse transcription-PCR (RT-PCR). Figure1, A and B, shows a comparison between the levels of agrin mRNAexpression in control and in sense (S)- and antisense (AS)-treatedprimary hippocampal neurons over a period of 10 d. Agrin mRNAexpression was normalized to the expression of the ubiquitouslyexpressed gene GAPDH (Biragyn et al., 1994). Agrin expressionis presented as a percentage of the agrin/GAPDH ratio in controluntreated cultures. A moderate but significant reduction (28 ±8%, mean ± SEM; p < 0.01; n = 9) of agrin mRNA expression wasdetected at as early as 2 d in AS-treated neurons. A much largereffect was measured at 5 and 10 d (70 ± 4%, mean ± SEM; p < 0.01;n = 9; and 84 ± 1%, mean ± SEM; p < 0.01; n = 9, respectively)(Fig. 1B).

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Figure 1. Specific effects of the antisense oligonucleotides on agrin expression in rat hippocampal neurons. A, RT-PCR analysis of agrin mRNA expression of control primary hippocampal neurons (C) and after 10 d of treatment with sense (S) and antisense (AS) oligonucleotides is shown. Alternative splicing events at the z position were analyzed; amplified products corresponding to the isoforms Ag0, Ag8, Ag11, and Ag19 are shown. Relative glyceraldehyde-3-phosphate dehydrogenase (GAPDH) amplification products are shown at the bottom. B, Quantification of agrin mRNA expression in control (C) and in sense (S) and antisense (AS) oligonucleotide (7.5 µM)-treated cells at 2, 5, and 10 d in culture is shown. Agrin expression was normalized to the levels of GAPDH mRNA. Bars represent the mean ± SEM (3 independent experiments; samples in triplicates). C, Antisense (AS), but not sense (S), oligonucleotides reduced agrin protein expression (3 d; 7.5 µM treatment). The arrowhead indicates agrin immunoreactivity of an apparent molecular weight of ~350 kDa; the asterisk indicates a nonspecific cross-reactive band. Analysis of protein extracts from postnatal (P2-P5) hippocampi revealed the same pattern of agrin immunoreactivity. The same amount of protein was loaded in each lane. D, The expression level of the following proteins in control (C) and AS-treated (AS) neurons is shown: agrin, actin, cAMP response element-binding protein (CREB), neuronal-specific enolase (NSE), microtubule-associated protein 2 (MAP-2), the NMDA receptor subunit NR1, the $beta$ -chain of the GABA_A receptor, synapsin-I (syn), synaptophysin (syp), and glutamic acid decarboxylase (GAD). Hippocampal neurons were treated for 10 d with 7.5 µM AS oligonucleotide. The treatment substantially affected agrin expression but not the expression of the other proteins tested. E, Agrin immunoreactivity is enriched in synaptosomes. Ten micrograms per lane of rat hippocampus homogenate (tot) and the synaptosome preparation from rat hippocampus (sy) were immunoblotted with antibodies specific for agrin (m247), the AMPA receptor subunit GluR1, synaptotagmin (syt), and tubulin. An enrichment of >10 of agrin immunoreactivity was observed in synaptosomes (n = 5 independent experiments).

The overall pattern of protein expression, as detected by silver staining, was not affected by the oligonucleotide treatments.No significant changes, including changes in the amount, number,and type of proteins, were noted in extracts from control andagrin sense or antisense oligonucleotide-treated neurons (datanot shown). The level of agrin protein was tested at 3 and 10d of treatment by the use of Western blot analysis. Results indicatethat the level of agrin expression was greatly reduced in 3-d-oldcultures treated with the AS oligonucleotide but was unaffectedin control and S oligonucleotide-treated neurons (Fig. 1C). After10 d of AS treatment, agrin expression was below the level ofdetection (Fig. 1D). The levels of expression of a transcriptionfactor and cytoskeletal, neuronal, and synapse-specific proteinswere also tested. Figure 1D shows that 10 d of treatment withthe AS oligonucleotide did not significantly affect the levelof expression of any of the proteinstested.

Reduced agrin expression induces changes in neuronal morphology and synaptic density

The effects of reduced agrin expression in primary hippocampal cultures were followed over time. By 3 d, cultures treatedwith antisense oligonucleotides contained multicellular aggregateswith fascicles of neurites (Fig. 2A,B). Aggregates were definedas clusters of more than five cells and were detected exclusivelyin antisense-treated neurons (n $>=$ 50 independent experiments).Between 3 and 14 d, the number of cells in the clusters and thethickness of the fascicles increased. Little or no arborizationof the neurites was noticed in AS-treated neurons (Fig. 2A). Similareffects were observed when cultures were exposed to either oftwo other antisense oligonucleotides (AS2 and ASY) (Fig. 2D; datanot shown). In contrast, neurons grown in the presence of eithersense (Fig. 2A) or scrambled oligonucleotides displayed morphologiesindistinguishable from those of control cultures. The rate ofneurite elongation did not significantly differ between controluntreated and any of the oligonucleotide-treated cells (data notshown).

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Figure 2. Agrin antisense oligonucleotides induced a change in phenotype in rat hippocampal neurons. A, Morphology of cultured neurons at 3 d (3d), 7 d (7d), and 14 d (14d) in culture. Only neurons treated with the agrin antisense oligonucleotide AS appeared clustered in multicellular aggregates with extended neurites in fascicles. All three antisense oligonucleotides tested produced the same phenotype. The concentration of S (S) and AS (AS) oligonucleotides was 7.5 µM. Scale bar, 100 µm. B, Concentration dependence of the AS oligonucleotides. The severity of the phenotype described in A increases with increasing concentration of AS oligonucleotides. Decreased cell numbers were observed in cultures treated with all three AS oligonucleotides tested at concentrations $>=$ 25 µM. Scale bar, 60 µm. C, Determination of the concentration-response curve of the AS oligonucleotide for synaptic differentiation. Synapsin-I-immunoreactive puncta per neurite area were measured in hippocampal neurons treated for 10 d with the AS oligonucleotide (AS oligo). Mean ± SEM values (synapses on n = 20 neurites in 5 randomly chosen fields) of a representative experiment (n = 3 independent experiments) are shown. D, Quantification of the number of synapsin-I-immunoreactive puncta per neurite area in cultured hippocampal neurons treated for 10 d with 5 µM agrin sense (S), scrambled (SC), and three agrin antisense oligonucleotides (AS, AS2, and ASY). Mean ± SEM values of a representative experiment (n = 3 independent experiments) are shown (n = 20 neurites in 5 randomly chosen fields of view/treatment; p < 0.05). Control cultures (C).

The degree of cell clustering and of process fasciculation depended on the concentration of antisense oligonucleotides used.Concentrations of AS oligonucleotides <2.5 µM did not produceany noticeable change. Appearance and exacerbation of the phenotypewere observed at concentrations between 5 and 10 µM (Fig. 2B).Decreased cell numbers could be observed in cultures treated withall of the oligonucleotides (sense, scrambled, AS, AS2, and ASY)at the highest concentrations tested (25-30 µM) (data notshown).

To investigate whether treatment with agrin antisense oligonucleotides affected synapse formation in primary hippocampal neurons,we examined the appearance of punctate immunoreactivity stainingof presynaptic markers, such as the synaptic vesicle proteinssynaptotagmin-I, synaptophysin, and synapsin-I. This phenomenonis one of the earliest detectable events of synaptogenesis invitro (Fletcher et al., 1991; Rao et al., 1998). To standardizethe measurements among experiments, the number of synapses perneurite area was determined. Antisense oligonucleotide treatmentshad dramatic effects on synapse formation. The number of synapsesformed depends on the amount of antisense oligonucleotide used.Concentrations between 0 and 2.5 µM had small effects; 50% reductionwas observed at 5 µM, whereas maximal effects ( $>=$ 90% reduction)were seen at concentrations $>=$ 10 µM (Fig. 2C). All three antisenseoligonucleotides tested produced similar effects (Fig. 2D). Allexperiments described hereafter were performed, if not otherwisestated, at 7.5 µM AS oligonucleotide. At this concentration, an~75-80% reduction in the number of synapses was consistently observedwithout any detectable decrease in cell number (Fig. 2).

NMDA receptor clustering precedes synapse formation in primary hippocampal neurons (Rao and Craig, 1997; Rao et al., 1998).Microclusters of NMDA receptors are present on dendrites, proximalto the perikarya, as early as day 2 in vitro but become localizedat synapses, even at considerable distance from the cell bodies,after 10 d. To test whether this specific arrangement of NMDAreceptors depends on the expression of agrin, we determined thepattern of immunoreactivity in AS-treated hippocampal neuronsof the NMDA receptor subunit NR1. All subtypes of NMDA receptorscontain this particular subunit. Neither the number nor the localizationof the NR1-immunoreactive puncta in relation to the cell somachanged in neurons treated for 10 d with AS oligonucleotides (Fig.3c,c'), suggesting that agrin is not necessary for the initialclustering of NMDA receptors.

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Figure 3. Effects of the antisense oligonucleotide treatment on wild-type and agrin-deficient neurons. Immunocytochemical analysis of synaptic differentiation in 10-d-old, antisense oligonucleotide-treated hippocampal neurons. a-c', Rat (P3-P5) hippocampal neurons were treated with 7.5 µM AS oligonucleotides. Patterns of immunoreactivity are shown for synapsin-I (a, a'), synGAP (b, b'), and the NMDA receptor subunit NR1 (c, c'). The treatment with the AS oligonucleotides affected the synapsin-I and synGAP staining but not the NR1 immunoreactivity. d-e', E18 mouse hippocampal neurons were treated for 10 d with 7.5 µM AS oligonucleotides. Synapsin-I immunoreactivity is shown in untreated (d, e) and treated (d', e') neurons. Synapsin-I-immunoreactive puncta disappeared in AS-treated wild-type (d') but not in AS-treated agrin-deficient (e') neurons. f-g', synGAP staining in wild-type (f, f') and agrin-deficient (g, g') E18 hippocampal neurons is shown. Cultures were maintained for 13 d (f, g) and 24 d (f', g'). Although synGAP puncta disappeared in mutant neurons between 13 and 24 d, they were still observed in wild-type neurons. The pattern of synapsin-I immunoreactivity did not change during this time period (data not shown). Scale bar, 20 µm.

The differentiation of mature synapses is accompanied by the specific association of cytosolic and cytoskeletal moleculesto postsynaptic proteins. The postsynaptic molecule synGAP isa component of a multimeric complex that includes NMDA receptors(Chen et al., 1998; Kim et al., 1998). We tested whether the synapticlocalization of synGAP is affected by the agrin antisense oligonucleotidetreatment. In contrast to NMDA receptors, treatment with AS oligonucleotidesfor 10 d completely abolished the punctate pattern of synGAP immunoreactivity(Fig. 3b,b'). This suggests that synGAP associates with the NMDAreceptors only after synapses have formed, which is consistentwith the developmental pattern of expression of these two proteins(Chen et al., 1998; Kim et al., 1998).

Agrin antisense oligonucleotide treatment does not alter the morphology and the synaptic density of agrin-deficient neurons

Our data indicate that reduction of agrin expression strongly affects synaptic differentiation in vitro. However, this isin contrast to results obtained from hippocampal and corticalneurons from agrin-deficient mice in which the morphological andfunctional development of synapses appeared normal (Li et al.,1999; Serpinskaya et al., 1999). We reasoned that if the agrinantisense oligonucleotides affected wild-type neurons in a specificmanner (i.e., by reducing agrin expression), they should not elicitthe same phenotype in neurons from agrin-deficient mice. Therefore,embryonic day 17 hippocampal neurons obtained from wild-type,agrin-heterozygous, and agrin-deficient mice were treated forvarious times with the AS oligonucleotide. The treatment equallyaffected wild-type and agrin-heterozygous murine and postnatalrat neurons (Fig. 3a,a',d,d') but did not affect agrin-deficientneurons; untreated or AS-treated agrin-deficient neurons showedthe same morphology and synaptic density (determined with antibodiesfor the presynaptic markers synaptophysin, synapsin-I, and synaptotagmin-I)(Fig. 3e,e'; data not shown). These results indicate that theantisense oligonucleotide treatments affected neurons specificallyby reducing agrin expression and did not have generalized cytopathiceffects.

Surprisingly, when the pattern of immunoreactivity for synGAP was studied in neurons obtained from agrin-deficient mice, astriking difference was detected between 13- and 24-d-old untreatedcultures. At 13 d, distinct immunoreactive puncta were visibleboth in wild-type and agrin-deficient neurons (Fig. 3f,g). However,punctate synGAP immunoreactivity was no longer detectable in 24-d-oldagrin-deficient neurons (89 ± 2% reduction compared with controlwild-type neurons, mean ± SEM; p < 0.01; n = 10) (Fig. 3f',g').

Incubation of neurons with an agrin-specific antibody produces synaptic alterations similar to those produced by agrin antisense oligonucleotides

It was shown previously that anti-agrin antibodies prevent the formation of neuromuscular junctions in vitro (Cohen and Godfrey,1992; Reist et al., 1992). Therefore, we tested whether agrin-specificantibodies inhibit synaptic differentiation in hippocampal neurons.We used an agrin-specific monoclonal antibody (m247) that recognizesan epitope close to the z-site and that greatly reduces the AChR-aggregatingactivity of agrin (Hoch et al., 1994). The number of synapsin-I-immunoreactivepuncta was dramatically reduced (83 ± 2%, mean ± SEM; p < 0.05;n = 15 fields of view, 3 independent experiments) in 10-d-oldneurons treated from the onset of the culture with the m247 antibody(Fig. 4A,B). Incubation with control antibodies did not affectsynaptic differentiation. Interestingly, the treatment with theagrin-specific antibody was effective in preventing synaptic differentiationbut did not produce the aggregation of cell bodies and the fasciculationof processes that were seen with the agrin antisense oligonucleotides.To investigate further the relationship between the synaptic differentiatingactivity of agrin and the adhesive properties of the substrate,we treated neurons plated on laminin-coated coverslips with theantisense oligonucleotides. Surprisingly, the AS oligonucleotide(7.5 µM) produced the same effects as did the anti-agrin antibodytreatment: synaptic differentiation was inhibited without changesin cell or process morphology (data not shown).

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Figure 4. Treatment with an agrin-specific antibody prevented synaptic differentiation; recombinant agrin countered the effects of the antisense oligonucleotides in hippocampal neurons. A, Rat P3-P5 hippocampal neurons were plated in the presence of the m247 antibody. Cultures were kept for 10 d. Immunofluorescence staining for synapsin-I was performed on untreated (Untr; a cluster of 3 neurons is shown) and m247-treated ( $alpha$ AgAb) cultures. The number of synapsin-I-immunoreactive puncta was greatly reduced in the treated neurons. Treatment with an unrelated antibody did not produce any phenotype (data not shown). Scale bar, 50 µm. B, Quantification of the effects of the m247 antibody on synaptic differentiation is shown. The number of synapsin-I-immunoreactive puncta per neurite area was greatly reduced ( $>=$ 80%) in treated cells ( $alpha$ AgAb) compared with untreated (Untr) and mock antibody-treated (C) cells. Values are from a representative experiment (n = 3); mean ± SEM values were calculated from 20 fields of view (p < 0.01). C, Neurons were incubated with antisense oligonucleotides and purified recombinant agrin isoforms. P3-P5 rat hippocampal neurons were treated for 10 d with the AS oligonucleotide (10 µM) with either the Ag4,0 or Ag4,8 isoforms (50 pM). Immunofluorescence staining with synapsin-I-specific antibodies is shown for untreated (Untr), AS-treated (AS), AS and Ag4,0-treated (AS/Ag0), and AS and Ag4,8-treated (AS/Ag8) neurons. Only the cultures treated with the Ag4,8 isoforms appeared similar to control untreated cells. D, Quantification of the effects of the antisense oligonucleotide and agrin isoform treatment is shown. The number of synapses per neurite area was determined for 10-d-untreated (Untr), AS-treated (AS), AS and Ag4,0-treated (AS/Ag0), and AS and Ag4,8-treated (AS/Ag8) neurons. Mean ± SEM values (n = 20 neurites in 5 randomly chosen fields of view per treatment; p < 0.05) are shown from a representative experiment (n = 4 independent experiments). Scale bar, 40 µm.

Recombinant agrin rescues the changes induced by antisense oligonucleotides

Using soluble recombinant agrin, we then tested whether specific isoforms differentially reversed the effects of the agrinantisense oligonucleotide treatment. The Ag4,0 and Ag4,8 have100- to 1000-fold differences in their AChR-aggregating activityand also have different abilities to induce pCREB in hippocampalneurons (Bowen et al., 1996; Ji et al., 1998). Therefore, hippocampalneurons were treated for 10 d with 7.5 µM AS oligonucleotidesand with ~50 pM purified Ag4,0 or Ag4,8 isoforms. AS oligonucleotide-treatedneurons incubated with the Ag4,8, but not the Ag4,0, isoform hada much larger (>90%) number of synapsin-I-immunoreactive punctacompared with AS-treated neurons (Fig. 4C,D). Interestingly, theincubation with the Ag4,8 isoform also reversed the morphologicalchanges (clustering of cell bodies and fasciculation of processes)induced by the AS treatment. These results indicate that the Ag4,8isoform is able to induce synaptic differentiation in AS-treatedhippocampal neurons, thus confirming that the effects of the agrinantisense oligonucleotide treatments were caused by a reductionin agrinexpression.

Ultrastructural analysis of synapses formed in primary hippocampal neurons expressing low levels of agrin

To study the ultrastructural morphology of synapses when agrin expression was strongly reduced, we analyzed and compared serialsections from untreated and from agrin sense and antisense oligonucleotide-treatedneurons by electron microscopy. After 15 d in culture, synapsespresent in untreated neurons displayed a fully mature ultrastructuralphenotype, as reported previously (Forti et al., 1997). Synapsesformed in the presence of either sense (S; n = 243) or antisense(AS; n = 285) oligonucleotides were morphologically indistinguishablefrom terminals in untreated cultures (n = 310). However, the numberof synapses was dramatically reduced in AS-treated cultures. Asfor untreated neurons, most synapses analyzed in sense and antisenseoligonucleotide-treated neurons were localized on spiny extroflexionsfrom dendrites (Papa et al., 1995). Dendritic shafts could beeasily identified by the presence of numerous mitochondria andmicrotubules. Synapses on the dendritic shaft could also be found(Fig. 5). Presynaptic terminals displayed a large pool of availablevesicles (n_vesicles = 57 ± 25 per section, mean ± SD). Approximately15% of these vesicles appeared to be docked at the active zones(Fig. 5). Most presynaptic varicosities (85%) were found juxtaposedto membranes containing electron-dense PSDs (Fig. 5, top row;type I synapses). This type of synapse invariably contained asingle PSD, which could be observed across a series of sections.The remaining synapses (~15%), without detectable PSDs (Fig. 5,bottom row; type II synapses), were presumably inhibitory. Theseresults confirm that puncta seen by immunofluorescence stainingwith synaptic markers represent differentiated synapses.

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Figure 5. Ultrastructural morphology of synapses formed at low levels of agrin expression. The two major types of morphologically distinct synapses present in the P3-P5 rat hippocampal cultures are shown in untreated (C) and in sense (S)- and antisense (AS)-treated neurons. Top row, Type I synapses with distinct postsynaptic densities. Bottom row, Type II synapses (presumably inhibitory) without postsynaptic densities. No noticeable changes in morphology were observed between untreated and treated neurons. The frequency of type I and II synapses was similar in all experimental conditions (~85 and 15%, respectively).

Low levels of agrin expression inhibit spontaneous and evoked synaptic transmission

To characterize further the phenotype of synapses established by hippocampal neurons expressing low levels of agrin, synapticfunction was analyzed. Evoked and spontaneous transmission wasmonitored in individual neurons by patch-clamp recording in thewhole-cell configuration. Evoked responses were elicited with0.2 Hz stimulation using a glass electrode filled with physiologicalsaline placed on the cell soma of nearby neurons. The probabilityof detecting a pair of synaptically connected neurons in bothuntreated and agrin sense oligonucleotide-treated cultures wascomparable (~40%). In these cultures, the average evoked currentsexceeded 200 pA (I = 224 ± 30 pA, mean ± SEM; n = 12), and transmissionfailures were very low (Fig. 6). In cultures treated with agrinantisense oligonucleotides (AS), the stimulation of neighboringneurons produced detectable current in only 3% of the postsynapticneurons tested. In these instances, transmission failures werehigh (83% transmission failure; n = 6 successful recordings),and the amplitude of the response was small (I = 52 ± 14 pA, mean± SEM) as shown in Figure 6, A and C.

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Figure 6. Low levels of agrin expression affect minis and evoked responses in hippocampal neurons. A, Representative examples of excitatory currents evoked by action potentials in neurons treated with agrin sense (control) (left) or antisense (right) oligonucleotides (Vm = $-$ 60 mV). B, Miniature events recorded from control (left) and antisense oligonucleotide-treated (right) neurons in the presence of TTX. Sweep numbers are shown on the right of the corresponding traces. In the antisense traces, only two minis were detected between sweeps 354 and 378. C, Quantification of the effects of the oligonucleotide treatments on the frequency of minis [left; data from n = 12, 7, and 10 experiments for control (C), sense (S), and antisense (AS) conditions, respectively] and the amplitude of the evoked EPSCs (right; data from n = 12, 8, and 6 experiments for control, sense, and antisense conditions, respectively) (mean ± SEM).

Analyses of minis provide important information on the synaptic physiology of evoked responses. Therefore, minis were recordedfrom neurons treated with AS oligonucleotides in the presenceof TTX (1 µM). Distinct minis were detected in AS oligonucleotide-treatedneurons although their frequency was dramatically reduced comparedwith that of untreated neurons (91% reduction; n = 12 controland 10 AS-treated recordings; p < 0.05) (Fig. 6B,C). The amplitudeof the minis seemed unaffected (I_control = 22.8 ± 5.1 pA; I_AS=26.3 ± 7.4 pA, mean ± SEM) although the small number of eventsdid not allow a more careful evaluation of thisparameter.

The reduced number of synapses in the AS-treated cultures could account for the conservation of the quantal size, the decreasedfrequency of minis, and the reduced amplitude of evoked responsesin pairs of electrically connected neurons. However, the magnitudeof the observed decrease in these responses (91 and 83%, respectively)appears to be larger than the decrease in the number of synapsesinduced by the AS treatment (~75% at 7.5 µM). This discrepancycould be explained by either a relative increase of silent synapses(Feldman and Knudsen, 1998) or a reduced probability of releaseat presynaptic terminals. Electrophysiological analysis cannoteasily differentiate between presynaptic and postsynaptic phenomena,and the number of synapses contributing to the response on a particularneuron is difficult toestimate.

Reduced agrin expression inhibits exo-endocytosis of synaptic vesicles

The results presented above suggest that low levels of agrin expression affect the function of presynaptic terminals. Therefore,we have measured the rate of spontaneous exocytosis at hippocampalsynapses using antibodies as described previously (Matteoli etal., 1992; Malgaroli et al., 1995). This method allows us to quantifydifferences in synaptic vesicle turnover independently from postsynapticresponses. Briefly, living neurons were incubated with antibodiesspecific for the intralumenal domain of synaptotagmin-I for 1hr in the presence of TTX (1 µM). The cells were then fixed andincubated with a second antibody specific for the cytosolic portionof synaptotagmin-I, which was raised in a species different fromthat used for the first antibody. Species-specific secondary antibodies,coupled with different fluorochromes, were used to determine theextent of exo-endocytosis at individual synapses (revealed bythe internalized antibody) versus the total number of synapses(detected by the second synaptotagmin-I antibody). The data wereanalyzed by confocal fluorescence microscopy and expressed asarbitrary units of intensity. Most synapses in untreated or agrinsense oligonucleotide-treated neurons showed uptake of anti-synaptotagmin-Iantibody (n = 15 experiments; p < 0.05), with individual synapsesrevealing variable levels of uptake. However, no significant differencein the mean uptake was detected between the two experimental groups(Fig. 7). In agrin antisense oligonucleotide-treated neurons,the number of synapses was drastically reduced (76% reduction;5-10 fields/condition analyzed in n = 10 experiments; p < 0.05).Furthermore, the remaining synapses displayed a marked reductionin the number of cycles of exo-endocytosis (Fig. 7). Thus, thereduction in the number of synapses combined with their diminishedcapability to release quanta could explain the decrease in synapticresponses detected in neurons treated with AS oligonucleotides.

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Figure 7. Reduction of synaptic vesicle turnover in hippocampal neurons expressing low levels of agrin. A, Triple confocal immunofluorescence staining was performed using different excitation/emission channels as described in Materials and Methods. Dendrites are depicted in green (corresponding to MAP-2 immunoreactivity). Left, Synapses in control and AS-treated neurons are shown in red (Cy5-coupled secondary antibody; 680 nm emission). Right, Spontaneous vesicular turnover at individual synapses also is depicted in red (Texas Red-coupled antibodies; 568 nm emission). The AS oligonucleotide treatment not only reduced the number of synapses but also the exo-endocytic cycling of vesicles occurring at individual synapses. B, Distributions of probability for the antibody internalization (in arbitrary units of fluorescence) at individual synapses from a representative experiment are shown. Note the similar degree of exo-endocytosis in control (n = 850 boutons) and sense-treated cultures (n = 659 boutons) versus that in antisense-treated cultures (n = 389 boutons). C, Percentage of synapses (left) and percentage synaptic uptake (right) from control (C) and agrin sense (S)- or antisense (AS)-treated cultures (mean ± SEM; n = 15 experiments) are shown. All incubations with living hippocampal neurons were performed in the presence of TTX (1 µM) and APV (25 µM). Values are indicated as a percentage of control levels.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Evidence is presented here in support of the hypothesis that agrin is necessary for synaptogenesis in hippocampal neurons.Reducing agrin expression with antisense oligonucleotides or blockingagrin function with antibodies greatly reduced synapse formationin these neurons. A specific synaptic change occurs over timein neurons obtained from agrin-deficientmice.

Three possible interpretations are compatible with our observations. First, it has been proposed that agrin functions as anadhesion molecule (Campagna et al., 1995; Chang et al., 1997)and that cell adhesion molecules regulate synapse formation andplasticity (Davis and Goodman, 1998; Hoffman, 1998). Consistentwith this model is the appearance of multicellular aggregatesand fasciculated processes in hippocampal cultures when agrinexpression is reduced, suggesting that agrin affects cell-substrateadhesion. However, blocking agrin function with agrin-specificantibodies, or reducing agrin expression with antisense oligonucleotidesin neurons plated onto laminin, inhibited synaptic differentiationwithout the induction of morphological changes. This suggeststhat diminished cell-substrate adhesion of neurons expressinglow levels of agrin is not the reason underlying their inabilityto form synapses. In the case of the antibody experiments, however,it is possible that agrin molecules involved in cell-substrateadhesion are less accessible to the antibodies than are thosemediating synapse formation (localized at cell-cell adhesion sites).Alternatively, the antibody treatment may be only partially effectivein blocking agrin function, implying that agrin-mediated synapseformation and adhesion require different thresholds of agrinexpression.

Second, agrin may affect synaptogenesis by controlling neural differentiation. One possibility is that agrin regulates genetranscription. In agreement with this hypothesis are results indicatingthat agrin regulates gene expression in muscles (I. Cohen et al.,1997; Jones et al., 1997; Meier et al., 1997; Gramolini et al.,1998) and cortical neurons (Hilgenberg et al., 1999) and thatspecific agrin isoforms activate the transcription factor CREBin hippocampal neurons (Ji et al., 1998). Another possibility,because agrin is an heparan sulfate proteoglycan, is that it bindsdifferentiation factors (Tsen et al., 1995; Halfter et al., 1997).Agrin binds basic fibroblast growth factors (bFGFs) and pleiotrophinand heparin-binding, growth-associated molecule (Daggett et al.,1996; Cotman et al., 1999). In some cases, such as bFGF, bindingto proteoglycans is necessary for the activation of specific receptors(Klagsbrun and Baird, 1991). Also, the N-terminal region of agrincontains domains homologous to Kazal-type serine protease inhibitors,which are also found in follistatin and osteonectin/SPARC/BM-40(Rupp et al., 1992; Patthy and Nikolics, 1993). Follistatin andosteonectin bind the differentiation factor activin and platelet-derivedgrowth factor, respectively (Patthy and Nikolics, 1993). In thecase of follistatin, this binding prevents the interaction ofactivin with its receptor (Hemmati-Brivanlou et al., 1994). Therefore,agrin may control neuronal differentiation either by facilitatingor by impeding the function of differentiationfactors.

Third, agrin may activate specific signaling events that lead to clustering and targeting of synaptic molecules. In fact,the activation of receptor tyrosine kinases is required for theagrin-mediated clustering of AChR at NMJs (Wallace, 1984; DeChiaraet al., 1996; Ferns et al., 1996) and for CREB phosphorylationin hippocampal neurons (Ji et al., 1998). Because only the Ag4,8isoform is able to restore synaptogenesis in antisense-treatedneurons and to induce CREB phosphorylation, these two functionsmay be related. Although our results demonstrate the importanceof specific agrin isoforms for synapse formation in hippocampalneurons, they do not resolve the mechanism of agrinfunction.

A surprising observation is that addition of recombinant soluble agrin isoforms to hippocampal neurons expressing normal levelsof agrin does not affect presynaptic or postsynaptic differentiation(Serpinskaya et al., 1999) (C. M. Böse, unpublished observations).Moreover, hippocampal neurons are not competent to function aspostsynaptic targets for 3-4 d in vitro (Fletcher et al., 1994).One possible explanation is that agrin cannot induce synapticdifferentiation in "young" neurons because they do not yet expressmolecules needed for the recruitment, stabilization, or targetingof synaptic molecules. After synapses have been established, however,the majority of the molecules required to form synaptic specializationsmay have accumulated at or been preferentially targeted to thosesynapses. Thus, despite the activation of the correct receptor-mediatedsignaling cascade by recombinant agrin, the concentration of synapticmolecules localized at extrasynaptic sites may be too low to formimmunocytochemically detectable structures. Alternatively, theaddition of agrin to mature neurons may increase the density ofpresynaptic and postsynaptic molecules at preexisting synapses.This process could also be technically difficult to evaluate.Lastly, it may be that contact between presynaptic and postsynapticterminals is necessary for the stabilization of synaptic moleculeaggregates in hippocampalneurons.

The shape of the concentration-response curve of the antisense oligonucleotide treatment suggests that a threshold of agrinexpression exists above which synapse formation may proceed. However,synapses established at intermediate or low levels of agrin expressionmay either belong to a specific type, whose formation does notdepend on agrin, or be established by a specific class of neurons.Both interpretations are unlikely because these synapses are morphologicallyheterogeneous and appeared evenly distributed throughout the cultures.These synapses appear indistinguishable, at the ultrastructurallevel, from control untreated synapses, even though their spontaneousand evoked release probabilities are diminished. Therefore, weconclude that reaching the critical threshold of agrin expressionmay not be sufficient to complete synaptic differentiation. Itwill be interesting to determine whether the formation of specifictypes of synapses requires different levels of agrin expressionor whether the synaptic localization of ion channels or subtypesof neurotransmitter receptors occurs at different thresholds ofagrinexpression.

The initial phase of synapse formation in agrin $-$ / $-$ neurons seems to occur normally in vitro (Li et al., 1999; Serpinskayaet al., 1999). This argues for the existence of functional redundancyfor agrin, which is further supported by our data showing thatthe treatment of agrin $-$ / $-$ neurons with agrin antisense oligonucleotidedoes not prevent synapse formation. How can the data presentedhere be reconciled with the idea of functional redundancy? Itis possible that when agrin expression is absent from the onsetof neurogenesis, neurons may be able to induce the expressionof compensatory alternatives. If their cellular and molecularenvironment mediates this regulation, then this will probablynot occur in vitro. Our data are consistent with this model: wild-typeneurons are unable to express compensatory mechanisms when agrinexpression is reduced in vitro, and agrin-deficient neurons culturedfor >24 d show a specific synaptic change, suggesting that theygradually loose their ability to compensate for agrin. Among possiblecompensatory molecules are adhesion molecules and synaptic differentiationfactors. Laminin is a likely candidate. Approximately 25% of theagrin polypeptide is homologous to regions in laminin subunits,and laminin can induce the aggregation of AChR on myotubes, althoughat high concentrations and via different mechanisms than seenwith agrin (M. W. Cohen et al., 1997; Sugiyama et al., 1997; Montanaroet al., 1998). Moreover, laminin and agrin bind $alpha$ -dystroglycan,and a specific pattern of laminin immunoreactivity can be detectedat NMJs and synaptic spines in hippocampal neurons (Sanes et al.,1990; Tian et al., 1997). In addition, agrin functions in partvia the activation of integrins (Martin and Sanes, 1997; Burkinet al., 1998). However, laminin is not able to compensate foragrin when functioning as a cell-substrate adhesion molecule.It will be interesting to determine whether this is also truefor other laminin isoforms. Recent results indicate that the secretedlectin neuronal activity-regulated pentraxin (Narp) satisfiesmany conditions of a synaptic differentiation factor (Tsui etal., 1996; O'Brien et al., 1999). Although Narp seems to regulatethe synaptic localization of a specific subset of glutamate receptors,it has not yet been determined whether it is indeed required forthe clustering of glutamate receptors and/or for synapse formation(O'Brien et al., 1999). Lastly, if the role of agrin is to bindand/or present synaptic differentiation factors to specific receptors,than the expression of other proteoglycans may also compensateforagrin.

The results of a recent study suggest, in contrast to our observations, that reduced agrin expression in hippocampal neuronscultured with monolayers of astroglial cells affected primarilyGABAergic synapses (Ferreira, 1999). This raises the interestingpossibility that astroglia also secrete factors able to compensatefor agrinactivity.

The localization of the postsynaptic molecule synGAP is affected in antisense oligonucleotide-treated and agrin $-$ / $-$ neurons.The role of synGAP is still undetermined. Because synGAP punctaappear at later stages of synaptogenesis (Kim et al., 1998), itwill be interesting to test aspects of synaptic transmission,including plasticity, in neurons displaying aberrant synGAPlocalization.

In conclusion, our results show that agrin is necessary for the induction of synaptic differentiation in primary hippocampalneurons. Further investigations will be needed to study the roleof all agrin isoforms in the development of the CNS, to determinewhen and for how long cultured neurons become competent to respondto agrin, and to study the kinetics of the agrin-mediated responses.This information will be useful for designing approaches to isolatethe neuronal agrin receptor(s). Moreover, the elucidation of themolecular mechanisms underlying agrin's function and/or the identificationof the compensatory mechanisms for agrin may reveal other factorsrequired for synapseformation.

  FOOTNOTES

Received May 22, 2000; revised Sept. 18, 2000; accepted Sept. 21, 2000.

This work was supported by grants from the National Institutes of Health (R29MB 51158), the Esther A. and Joseph KlingensteinFund, and the Muscular Dystrophy Association to F.R. and by grantsfrom the telethon, Human Frontiers, and Ministero dell'Universitàe della Ricerca Scientifica e Tecnologica to A.M. C.M.B. was supportedby a fellowship of the Swiss Federal Institute of Technology.We thank D. Ginty, A. Kolodkin, R. Huganir, C. Hopf, and D. Lindenfor helpful discussions. We also thank M. Diana for some preliminaryelectrophysiologicalrecordings.
Correspondence should be addressed to Dr. Fabio Rupp, HySeq, Inc., 670 Almanor Avenue, Sunnyvale, CA 94085. E-mail: frupp{at}sbh.com.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Biragyn A, Arkins S, Kelley KW (1994) Riboprobe expression cassettes for measuring IGF-I, beta-actin and glyceraldehyde 3-phosphate dehydrogenase transcripts. J Immunol Methods 168:235-244[Web of Science][Medline].
Bowen DC, Sugiyama J, Ferns M, Hall ZW (1996) Neural agrin activates a high-affinity receptor in C2 muscle cells that is unresponsive to muscle agrin. J Neurosci 16:3791-3797[Abstract/Free Full Text].
Burgess RW, Nguyen QT, Son YJ, Lichtman JW, Sanes JR (1999) Alternatively spliced isoforms of nerve- and muscle-derived agrin: their roles at the neuromuscular junction. Neuron 23:33-44[Web of Science][Medline].
Burkin DJ, Gu M, Hodges BL, Campanelli JT, Kaufman SJ (1998) A functional role for specific spliced variants of the alpha7beta1 integrin in acetylcholine receptor clustering. J Cell Biol 143:1067-1075[Abstract/Free Full Text].
Campagna JA, Ruegg MA, Bixby JL (1995) Agrin is a differentiation-inducing "stop-signal" for motoneurons in vitro. Neuron 15:1365-1374[Web of Science][Medline].
Campagna JA, Ruegg MA, Bixby JL (1997) Evidence that agrin directly influences presynaptic differentiation at neuromuscular junctions in vitro. Eur J Neurosci 9:2269-2283[Web of Science][Medline].
Campanelli JT, Gayer GG, Scheller RH (1996) Alternative RNA splicing that determines agrin activity regulates binding to heparin and alpha-dystroglycan. Development 122:1663-1672[Abstract].
Chang D, Woo JS, Campanelli J, Scheller RH, Ignatius MJ (1997) Agrin inhibits neurite outgrowth but promotes attachment of embryonic motor and sensory neurons. Dev Biol 181:21-35[Web of Science][Medline].
Chen HJ, Rojas-Soto M, Oguni A, Kennedy MB (1998) A synaptic Ras-GTPase activating protein (p135 SynGAP) inhibited by CaM kinase II. Neuron 20:895-904[Web of Science][Medline].
Cohen I, Rimer M, Lomo T, McMahan UJ (1997) Agrin-induced postsynaptic-like apparatus in skeletal muscle fibers in vivo. Mol Cell Neurosci 9:237-253[Web of Science][Medline].
Cohen MW, Godfrey EW (1992) Early appearance of and neuronal contribution to agrin-like molecules at embryonic frog nerve-muscle synapses formed in culture. J Neurosci 12:2982-2992[Abstract].
Cohen MW, Jacobson C, Yurchenco PD, Morris GE, Carbonetto S (1997) Laminin-induced clustering of dystroglycan on embryonic muscle cells: comparison with agrin-induced clustering. J Cell Biol 136:1047-1058[Abstract/Free Full Text].
Cohen NA, Kaufmann WE, Worley PF, Rupp F (1997) Expression of agrin in the developing and adult rat brain. Neuroscience 76:581-596[Web of Science][Medline].
Cotman SL, Halfter W, Cole GJ (1999) Identification of extracellular matrix ligands for the heparan sulfate proteoglycan agrin. Exp Cell Res 249:54-64[Web of Science][Medline].
Daggett DF, Cohen MW, Stone D, Nikolics K, Rauvala H, Peng HB (1996) The role of an agrin-growth factor interaction in ACh receptor clustering. Mol Cell Neurosci 8:272-285[Web of Science][Medline].
Davis GW, Goodman CS (1998) Genetic analysis of synaptic development and plasticity: homeostatic regulation of synaptic efficacy. Curr Opin Neurobiol 8:149-156[Web of Science][Medline].
DeChiara TM, Bowen DC, Valenzuela DM, Simmons MV, Poueymirou WT, Thomas S, Kinetz E, Compton DL, Rojas E, Park JS, Smith C, DiStefano PS, Glass DJ, Burden SJ, Yancopoulos GD (1996) The receptor tyrosine kinase MuSK is required for neuromuscular junction formation in vivo. Cell 85:501-512[Web of Science][Medline].
Dutton EK, Uhm CS, Samuelsson SJ, Schaffner AE, Fitzgerald SC, Daniels MP (1995) Acetylcholine receptor aggregation at nerve-muscle contacts in mammalian cultures: induction by ventral spinal cord neurons is specific to axons. J Neurosci 15:7401-7416[Abstract].
Escher G, Bechade C, Levi S, Triller A (1996) Axonal targeting of agrin in cultured rat dorsal horn neurons. J Cell Sci 109:2959-2966[Abstract].
Feldman DE, Knudsen EI (1998) Experience-dependent plasticity and the maturation of glutamatergic synapses. Neuron 20:1067-1071[Web of Science][Medline].
Ferns M, Hoch W, Campanelli JT, Rupp F, Hall ZW, Scheller RH (1992) RNA splicing regulates agrin-mediated acetylcholine receptor clustering activity on cultured myotubes. Neuron 8:1079-1086[Web of Science][Medline].
Ferns M, Deiner M, Hall Z (1996) Agrin-induced acetylcholine receptor clustering in mammalian muscle requires tyrosine phosphorylation. J Cell Biol 132:937-944[Abstract/Free Full Text].
Ferns MJ, Campanelli JT, Hoch W, Scheller RH, Hall Z (1993) The ability of agrin to cluster AChRs depends on alternative splicing and on cell surface proteoglycans. Neuron 11:491-502[Web of Science][Medline].
Ferreira A (1999) Abnormal synapse formation in agrin-depleted hippocampal neurons. J Cell Sci 112:4729-4738[Abstract].
Fletcher TL, Cameron P, De Camilli P, Banker G (1991) The distribution of synapsin I and synaptophysin in hippocampal neurons developing in culture. J Neurosci 11:1617-1626[Abstract].
Fletcher TL, De Camilli P, Banker G (1994) Synaptogenesis in hippocampal cultures: evidence indicating that axons and dendrites become competent to form synapses at different stages of neuronal development. J Neurosci 14:6695-6706[Abstract].
Forti L, Bossi M, Bergamaschi A, Villa A, Malgaroli A (1997) Loose-patch recordings of single quanta at individual hippocampal synapses. Nature 388:874-878[Medline].
Gautam M, Noakes PG, Moscoso L, Rupp F, Scheller RH, Merlie JP, Sanes JR (1996) Defective neuromuscular synaptogenesis in agrin-deficient mutant mice. Cell 85:525-535[Web of Science][Medline].
Gramolini AO, Burton EA, Tinsley JM, Ferns MJ, Cartaud A, Cartaud J, Davies KE, Lunde JA, Jasmin BJ (1998) Muscle and neural isoforms of agrin increase utrophin expression in cultured myotubes via a transcriptional regulatory mechanism. J Biol Chem 273:736-743[Abstract/Free Full Text].
Halfter W, Schurer B, Yip J, Yip L, Tsen G, Lee JA, Cole GJ (1997) Distribution and substrate properties of agrin, a heparan sulfate proteoglycan of developing axonal pathways. J Comp Neurol 383:1-17[Web of Science][Medline].
Hemmati-Brivanlou A, Kelly OG, Melton DA (1994) Follistatin, an antagonist of activin, is expressed in the Spemann organizer and displays direct neuralizing activity. Cell 77:283-295[Web of Science][Medline].
Hilgenberg LG, Hoover CL, Smith MA (1999) Evidence of an agrin receptor in cortical neurons. J Neurosci 19:7384-7393[Abstract/Free Full Text].
Hoch W, Ferns M, Campanelli JT, Hall ZW, Scheller RH (1993) Developmental regulation of highly active alternatively spliced forms of agrin. Neuron 11:479-490[Web of Science][Medline].
Hoch W, Campanelli JT, Harrison S, Scheller RH (1994) Structural domains of agrin required for clustering of nicotinic acetylcholine receptors. EMBO J 13:2814-2821[Web of Science][Medline].
Hoffman KB (1998) The relationship between adhesion molecules and neuronal plasticity. Cell Mol Neurobiol 18:461-475[Web of Science][Medline].
Ji RR, Bose CM, Lesuisse C, Qiu D, Huang JC, Zhang Q, Rupp F (1998) Specific agrin isoforms induce cAMP response element binding protein phosphorylation in hippocampal neurons. J Neurosci 18:9695-9702[Abstract/Free Full Text].
Jones G, Meier T, Lichtsteiner M, Witzemann V, Sakmann B, Brenner HR (1997) Induction by agrin of ectopic and functional postsynaptic-like membrane in innervated muscle. Proc Natl Acad Sci USA 94:2654-2659[Abstract/Free Full Text].
Kim JH, Liao D, Lau LF, Huganir RL (1998) synGAP: a synaptic RasGAP that associates with the PSD-95/SAP90 protein family. Neuron 20:683-691[Web of Science][Medline].
Klagsbrun M, Baird A (1991) A dual receptor system is required for basic fibroblast growth factor activity. Cell 67:229-231[Web of Science][Medline].
Li Z, Hilgenberg LG, O'Dowd DK, Smith MA (1999) Formation of functional synaptic connections between cultured cortical neurons from agrin-deficient mice. J Neurobiol 39:547-557[Web of Science][Medline].
Malgaroli A, Ting AE, Wendland B, Bergamaschi A, Villa A, Tsien RW, Scheller RH (1995) Presynaptic component of long-term potentiation visualized at individual hippocampal synapses. Science 268:1624-1628[Abstract/Free Full Text].
Martin PT, Sanes JR (1997) Integrins mediate adhesion to agrin and modulate agrin signaling. Development 124:3909-3917[Abstract].
Matteoli M, Takei K, Perin MS, Sudhof TC, De Camilli P (1992) Exo-endocytotic recycling of synaptic vesicles in developing processes of cultured hippocampal neurons. J Cell Biol 117:849-861[Abstract/Free Full Text].
McMahan UJ (1990) The agrin hypothesis. Cold Spring Harb Symp Quant Biol 55:407-418[Abstract/Free Full Text].
Meier T, Hauser DM, Chiquet M, Landmann L, Ruegg MA, Brenner HR (1997) Neural agrin induces ectopic postsynaptic specializations in innervated muscle fibers. J Neurosci 17:6534-6544[Abstract/Free Full Text].
Molnar E, McIlhinney RA, Baude A, Nusser Z, Somogyi P (1994) Membrane topology of the GluR1 glutamate receptor subunit: epitope mapping by site-directed antipeptide antibodies. J Neurochem 63:683-693[Web of Science][Medline].
Montanaro F, Gee SH, Jacobson C, Lindenbaum MH, Froehner SC, Carbonetto S (1998) Laminin and $alpha$ -dystroglycan mediate acetylcholine receptor aggregation via a MuSK-independent pathway. J Neurosci 18:1250-1260[Abstract/Free Full Text].
Nitkin RM, Smith MA, Magill C, Fallon JR, Yao YM, Wallace BG, McMahan UJ (1987) Identification of agrin, a synaptic organizing protein from Torpedo electric organ. J Cell Biol 105:2471-2478[Abstract/Free Full Text].
O'Brien RJ, Xu D, Petralia RS, Steward O, Huganir RL, Worley P (1999) Synaptic clustering of AMPA receptors by the extracellular immediate-early gene product Narp. Neuron 23:309-323[Web of Science][Medline].
O'Connor LT, Lauterborn JC, Gall CM, Smith MA (1994) Localization and alternative splicing of agrin mRNA in adult rat brain: transcripts encoding isoforms that aggregate acetylcholine receptors are not restricted to cholinergic regions. J Neurosci 14:1141-1152[Abstract].
O'Connor LT, Lauterborn JC, Smith MA, Gall CM (1995) Expression of agrin mRNA is altered following seizures in adult rat brain. Brain Res Mol Brain Res 33:277-287[Medline].
Papa M, Bundman MC, Greenberger V, Segal M (1995) Morphological analysis of dendritic spine development in primary cultures of hippocampal neurons. J Neurosci 15:1-11[Abstract].
Patthy L, Nikolics K (1993) Functions of agrin and agrin-related proteins. Trends Neurosci 16:76-81[Web of Science][Medline].
Rao A, Craig AM (1997) Activity regulates the synaptic localization of the NMDA receptor in hippocampal neurons. Neuron 19:801-812[Web of Science][Medline].
Rao A, Kim E, Sheng M, Craig AM (1998) Heterogeneity in the molecular composition of excitatory postsynaptic sites during development of hippocampal neurons in culture. J Neurosci 18:1217-1229[Abstract/Free Full Text].
Reist NE, Werle MJ, McMahan UJ (1992) Agrin released by motor neurons induces the aggregation of acetylcholine receptors at neuromuscular junctions. Neuron 8:865-868[Web of Science][Medline].
Ruegg MA, Tsim KW, Horton SE, Kroger S, Escher G, Gensch EM, McMahan UJ (1992) The agrin gene codes for a family of basal lamina proteins that differ in function and distribution. Neuron 8:691-699[Web of Science][Medline].
Rupp F, Payan DG, Magill-Solc C, Cowan DM, Scheller RH (1991) Structure and expression of a rat agrin. Neuron 6:811-823[Web of Science][Medline].
Rupp F, Ozcelik T, Linial M, Peterson K, Francke U, Scheller R (1992) Structure and chromosomal localization of the mammalian agrin gene. J Neurosci 12:3535-3544[Abstract].
Sanes JR, Engvall E, Butkowski R, Hunter DD (1990) Molecular heterogeneity of basal laminae: isoforms of laminin and collagen IV at the neuromuscular junction and elsewhere. J Cell Biol 111:1685-1699[Abstract/Free Full Text].
Sanes JR, Apel ED, Burgess RW, Emerson RB, Feng G, Gautam M, Glass D, Grady RM, Krejci E, Lichtman JW, Lu JT, Massoulie J, Miner JH, Moscoso LM, Nguyen Q, Nichol M, Noakes PG, Patton BL, Son YJ, Yancopoulos GD, Zhou H (1998) Development of the neuromuscular junction: genetic analysis in mice. J Physiol (Paris) 92:167-172[Web of Science][Medline].
Serpinskaya AS, Feng G, Sanes JR, Craig AM (1999) Synapse formation by hippocampal neurons from agrin-deficient mice. Dev Biol 205:65-78[Web of Science][Medline].
Smith MA, Magill-Solc C, Rupp F, Yao YM, Schilling JW, Snow P, McMahan UJ (1992) Isolation and characterization of a cDNA that encodes an agrin like protein in the marine ray. Mol Cell Neurosci 3:406-415.
Stone DM, Nikolics K (1995) Tissue- and age-specific expression patterns of alternatively spliced agrin mRNA transcripts in embryonic rat suggest novel developmental roles. J Neurosci 15:6767-6778[Abstract/Free Full Text].
Sugiyama JE, Glass DJ, Yancopoulos GD, Hall ZW (1997) Laminin-induced acetylcholine receptor clustering: an alternative pathway. J Cell Biol 139:181-191[Abstract/Free Full Text].
Tian M, Hagg T, Denisova N, Knusel B, Engvall E, Jucker M (1997) Laminin-alpha2 chain-like antigens in CNS dendritic spines. Brain Res 764:28-38[Web of Science][Medline].
Tsen G, Halfter W, Kroger S, Cole GJ (1995) Agrin is a heparan sulfate proteoglycan. J Biol Chem 270:3392-3399[Abstract/Free Full Text].
Tsim KW, Ruegg MA, Escher G, Kroger S, McMahan UJ (1992) cDNA that encodes active agrin. Neuron 8:677-689[Web of Science][Medline].
Tsui CC, Copeland NG, Gilbert DJ, Jenkins NA, Barnes C, Worley PF (1996) Narp, a novel member of the pentraxin family, promotes neurite outgrowth and is dynamically regulated by neuronal activity. J Neurosci 16:2463-2478[Abstract/Free Full Text].
Wallace BG (1984) Staurosporine inhibits agrin-induced acetylcholine receptor phosphorylation and aggregation. J Cell Biol 125:661-668[Abstract/Free Full Text].
Whittaker VP (1984) The synaptosomes. In: Handbook of neurochemistry, Vol 7 (Lathia A, ed), pp 1-39. New York: Plenum.

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