Integrin-Mediated Regulation of Synaptic Morphology, Transmission, and Plasticity

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 (66)

Citing Articles via Google Scholar

Google Scholar

Articles by Rohrbough, J.

Articles by Broadie, K.

Search for Related Content

PubMed

PubMed Citation

Articles by Rohrbough, J.

Articles by Broadie, K.

Previous Article  |  Next Article

The Journal of Neuroscience, September 15, 2000, 20(18):6868-6878

Integrin-Mediated Regulation of Synaptic Morphology, Transmission, and Plasticity
Jeffrey Rohrbough¹, Michael S. Grotewiel², Ronald L. Davis³, and Kendal Broadie¹
¹ Department of Biology, University of Utah, Salt Lake City, Utah 84112, ² Department of Zoology, Michigan State University, East Lansing, Michigan 48824-1312, and ³ Department of Cell Biology and Department of Psychiatry and Behavioral Sciences, Baylor College of Medicine, Houston, Texas 77030

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Volado, the gene encoding the Drosophila $alpha$ PS3-integrin, is required for normal short-term memory formation (Grotewiel et al.,1998), supporting a role for integrins in synaptic modulationmechanisms. We show that the Volado protein (VOL) is localizedto central and peripheral larval Drosophila synapses. VOL is stronglyconcentrated in a subpopulation of synaptic boutons in the CNSneuropil and to a variable subset of synaptic boutons at neuromuscularjunctions (NMJs). Mutant morphological and functional synapticphenotypes were analyzed at the NMJ. Volado mutant synaptic arborsare structurally enlarged, suggesting VOL negatively regulatesdevelopmental synaptic sprouting and growth. Mutant NMJs exhibitabnormally large evoked synaptic currents and reduced Ca²⁺ dependence of transmission. Strikingly, multiple forms of Ca²⁺- and activity-dependent synaptic plasticity are reduced or absent.Conditional Volado expression in mutant larvae largely rescuesnormal transmission and plasticity. Pharmacologicially disruptingintegrin function at normal NMJs phenocopies features of mutanttransmission and plasticity within 30-60 min, demonstrating thatintegrins acutely regulate functional transmission. Our resultsprovide direct evidence that Volado regulates functional synapticplasticity processes and support recent findings implicating integrinsin rapid changes in synaptic efficacy and in memoryformation.

Key words: integrins; synaptic plasticity; synaptic signaling; adhesion; learning and memory; neuromuscular junction; Drosophila

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

A recent screen in Drosophila for new learning and memory mutants (Grotewiel et al., 1998) added a particularly intriguingnew gene, Volado, to the growing list of genes involved in variousphases of the learning-to-memory process (Boynton and Tully, 1992;Davis et al., 1995; Davis, 1996; Skoulakis and Davis, 1996; Dubnauand Tully, 1998). Volado, also known as $alpha$ PS3 (Stark et al., 1997),encodes two $alpha$ -integrin proteins differing only in their first63 amino acids (Stark et al., 1997; Grotewiel et al., 1998). TheVolado (VOL) proteins have enriched expression in the adult mushroombodies (Grotewiel et al., 1998), synapse-dense brain structuresthat serve as insect olfactory memory centers and have long beenimplicated in cAMP signaling-dependent forms of behavioral learningand memory (Davis et al., 1995; Davis, 1996; Dubnau and Tully,1998). Viable Volado mutants have a dominant effect on adult olfactorymemory, reducing short-term memory (STM) assessed 3-15 min aftertraining by ~50%. The mutant STM defect is reversibly rescuedby conditional VOL expression just 3 hr before training (Grotewielet al., 1998), suggesting a dynamic role for integrins in behaviormodulation. These results indicate an exciting new potential rolefor integrins in mediating persistent changes in synaptic efficacythought to accompany memoryformation.

Integrins function as $alpha$ $beta$ receptor heterodimers capable of interacting with a variety of extracellular matrix (ECM) and cytoskeletalproteins, mediating cell-cell and cell-ECM adhesion interactionsand bidirectional signaling across cell membranes (Hynes, 1992;Diamond and Springer, 1994; Clarke and Brugge, 1995; Jones, 1996).Cellular studies using peptide inhibitors of integrin-ECM ligandinteractions have recently implicated synaptic integrins in rapid(minutes) and reversible consolidation of long-term potentiation(LTP) in the mammalian hippocampus (Bahr et al., 1997; Staubliet al., 1998), providing evidence that integrins function in long-termphysiological plasticity related to learning. Dynamic changesin integrin-dependent adhesive interactions or intracellular signalingactivity could mediate alterations in synapse morphology or number,or modulate transmission strength at existing synapses. Synapticintegrins are thus strategically positioned to have roles in bothmorphological and functional synaptic plasticity mechanisms usedin memory formation andstabilization.

To test these models of integrin synaptic function, we have investigated the role of VOL at the Drosophila neuromuscular junction(NMJ), where previous studies have suggested a conserved mechanisticlink with plasticity properties of central synapses (Zhong andWu, 1991; Zhong et al., 1992; Wang et al., 1994; Broadie et al.,1997; Rohrbough et al., 1999). We examine an allelic series ofVolado mutants to assess the role of VOL in regulating synapticterminal morphology, functional transmission, and plasticity properties,and demonstrate that mutant defects can be conditionally rescuedby expression of a Volado transgene. We complement this geneticapproach by acutely inhibiting normal integrin function with apeptide containing the Arg-Gly-Asp consensus sequence common tomany integrin-binding ECM ligands (Chen and Grinnell, 1995, 1997;Bahr et al., 1997; Baneres et al., 1998; Graner et al., 1998;Staubli et al., 1998). Our results suggest that VOL may activelyregulate both synaptic architecture and functional transmissionproperties.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Drosophila mutant and transgenic stocks. Analysis of the Volado gene structure and transcripts, and construction and analysisof the viable P-element insertion allele (Vol¹; ry) and viable excision allele (Vol²; ry), were described previously (Grotewiel et al., 1998). Thesame $alpha$ -integrin subunit gene, designated $alpha$ PS3, and transcriptswere identified in an independent study (Stark et al., 1997);this study also indicated that $alpha$ PS3/ Volado is allelic to scab,previously identified as a dorsal closure mutant (Nusslein-Volhardet al., 1984). Two additional putative $alpha$ -integrins with homologyto $alpha$ PS3 (currently designated $alpha$ PS4 and $alpha$ PS5) have also recentlybeen identified in the Drosophila genome (FlyBase, 2000).

The Volado locus is organized into two transcription units, Vol-long (Vol-l) and Vol-short (Vol-s), encoding RNAs of 4.6 and4.4 kb, respectively (Stark et al., 1997; Grotewiel et al., 1998).The VOL $alpha$ -integrin proteins (VOL-l and VOL-s) encoded by thesetranscripts consist of identical 1115 amino acids sequences exceptfor their first 63 amino acids (Grotewiel et al., 1998). The Vol¹ P-element carrying the ry⁺ reporter gene is located in intron 1 of the Vol-l transcript.Vol² deletes 816 bp spanning exon 1 of the Vol-s transcript. The homozygousVol¹ and Vol² strains selectively eliminate expression of the VOL-l and VOL-sintegrin isoforms, respectively (Grotewiel et al., 1998).

Imprecise excision of the Vol¹ insertion element generated two additional alleles, Vol³ and Vol⁴, which are homozygous-lethal in larval stages. PCR and sequenceanalysis of the Volado gene in these two excision mutants revealsthat both delete portions of the open reading frame common toboth transcripts (exons 2-8). The Vol³ allele deletes 925 bp of the locus, including all of exon 3 andparts of exons 2 and 4; the deleted region includes the threeconsensus divalent cation-binding domains essential for integrinfunction. The Vol⁴ allele deletes 1640 bp, including the first 118 bp of exon 2and 1522 bp of the preceding intron. Molecular criteria predictthese two mutations to be nullalleles.

All fly stocks were maintained at 25°C on standard cornmeal medium supplemented with dry yeast. Balanced stocks carrying theVol³ or Vol⁴ chromosomes were crossed to yw; Sco/CyO y⁺ flies to generate new balanced Volado mutant strains (yw; Vol^-/CyO y⁺). Wild-type (Oregon R), yw and ry control, and Volado mutantflies were transferred daily to fresh tubes for a laying periodof <24 hr. Wild-type (Oregon-R) and lethal Vol mutant animalsused for developmental studies of VOL protein expression and synapticmorphology analyses were selected from midembryonic stages [10hr after egg laying (AEL)], to mature (wandering) third instarstages (~6 d after hatching). Mature third instar larvae wereused for all other experiments. Homozygous Vol³ and Vol⁴ larvae were selected at ~3 d AEL by the y marker and transferred to new tubes for the remainder of development.At late third instar stages, the surviving Vol mutant larvae (10-20%)rarely exhibit normal wandering behavior, and most are undersizedand weak compared to control and viable mutant larvae. We selectedthe most robust and normal-appearing Vol survivors to avoid includingdata from animals near lethality; selected animals (6-7 d AEL)were comparable or slightly smaller in size compared to controllarvae.

For conditional rescue experiments, we used the Volado transgene (VS-T3) containing the Volado-short genomic sequence drivenby the heat-shock promoter hsp70 (Grotewiel et al., 1998). ThisT3 transgene was crossed onto the Vol³ and Vol⁴ mutant second chromosomes by standard crosses and confirmed byPCR (our unpublished results), and the resulting Vol³-T3 and Vol⁴-T3 constructs were balanced over CyO GFP. Homozygous Vol³-T3 and Vol⁴-T3 larvae were selected at 3 d AEL and transferred to agar platessupplemented with wet yeast or food tubes. Animals were heat-shockedby immersing sealed tubes or plates in a water bath (30 min at37°C) once per day on days 3-6 AEL, or alternatively, three timesover a 36 hr period on days 6-7 AEL. Vol³-T3 and Vol⁴-T3 larvae receiving HS display markedly improved growth, robustmovement, and improved viability compared to homozygous Vol³ and Vol⁴ larvae; the majority of heat-shocked Vol³-T3 and Vol⁴-T3 animals survive to midpupal stages, and a minority are rescuedto adult viability. All physiological recordings were made fromheat-shocked Vol⁴-T3 larvae. Again, we observed no significant differences in averagetransmission amplitude or short-term facilitation properties betweenlarvae receiving either HS treatment, and these results are pooledin Figure 7, A and B; all results in Figure 7C were obtained fromanimals given four HS treatments over days 3-6AEL.

Synaptogmin-GFP and Synaptobrevin-GFP flies were constructed and kindly supplied by Dr. Yong Zhang. Enhanced GFP (catalog#6084-1; Clontech, Palo Alto, CA) was fused to the C-terminalof synaptotagmin (GenBank accession number M55048) and n-synaptobrevin(GenBank accession number S66686). The fusion constructs werethen introduced into Drosophila transformation vector pP{UAST}(FlyBase, 2000) under the control of UAS. Transformants were crossedto elav-GFP or 4G-GFP flies to drive expression pan-neuronallyor in a subset of central neurons, respectively. Neurally expressedneuronal Synaptobrevin-GFP (n-Syb GFP) has recently been reportedto be normally transported and specifically localized to synapticvesicle membranes at Drosophila NMJs (Estes et al., 2000).

Immunohistology. Preparations were fixed and immunohistologically stained as reported previously (Broadie and Bate, 1993;Broadie et al., 1995; Rohrbough et al., 1999). The rabbit polyclonalVolado antibody was raised against the protein C terminus andrecognizes both adult VOL isoforms (Grotewiel et al., 1998). Larvaewere dissected along the dorsal midline and secured flat withpins or histoacryl glue in Ca²⁺-free saline, fixed for 45-75 min with 4% paraformaldehyde inPBS, then washed in PBS-TX (0.1% Triton X-100 in PBS) containing5 mg/ml BSA. Preparations were then stained overnight at 4°C withrabbit polyclonal anti-Volado (1:50), rat monoclonal anti-Disks-large(DLG; 1:500), or mouse monoclonal anti-cysteine string protein(CSP; 1:100) antibodies, followed by incubation with a biotinylated(Volado, CSP) secondary antibody (1:300 to 1:500) for 2 hr atroom temperature. All antibody dilutions were in PBS-TX. Voladoand CSP immunostaining was visualized using a Vectastain ABC Elitekit (Vector Laboratories, Burlingame, CA) with DAB reaction andNiCl₂ enhancement, as reported previously (Broadie and Bate, 1993;Broadie et al., 1995; Rohrbough et al., 1999). Preparations weredehydrated with an ethanol series, cleared in Histoclear, mountedin araldite, and visualized with Nomarski optics at 1000× on aZeiss Axioskop microscope. In fluorescent antibody-labeling experimentsfor confocal analysis, immunostaining was visualized with fluorescence-conjugatedstreptavidin (1:500) bound to biotinylated secondary antibody(Volado), or with directly conjugated fluorescent secondary antibodies(DLG, CSP). As controls for the specificity of the Volado antibody,we stained embryos homozygous for a Volado deficiency; additionally,we treated wild-type larvae with rabbit preimmune serum or withanti-rabbit secondary antibody only. No specific staining wasobserved in thesecases.

Optical sections of the CNS and NMJs were collected for analysis on a Bio-Rad (Hercules, CA) MRC 600 confocal microscope.Color images and microscopy figures were constructed and manipulatedusing Adobe Photoshopsoftware.

NMJ morphological analysis. Anti-CSP-stained NMJs in wild-type, yw control, and lethal Vol mutant (Vol³ and Vol⁴) larvae were viewed at 1000× on a Zeiss Axioskop microscope.The number of type I terminal branch segments (muscle 4) and synapticboutons (muscles 4 and 6/7) were counted in both hemisegmentsof abdominal segment A3 and averaged for each larva. Branchesoriginating directly from the nerve entry point were classifiedas primary branches, and each subsequent branch fork with at leasttwo boutons defined progressively higher-order (i.e., secondary,tertiary) segments (Rohrbough et al., 1999). Average bouton andbranch numbers were determined from 12 control larvae and 8 larvaefrom each mutant strain. Only the principle NMJ formed near theinternal center of the muscle and containing type Ib boutons,was analyzed. We observed no significant morphological differencesbetween wild-type OR and yw control animals. Digital images ofrepresentative terminals were collected at 400× using a SPOT digitalcamera and image acquisition software (Zeiss).

Electrophysiology. All recordings were made at 18°C from muscle 6 in abdominal segments A3-A4 of freshly dissected third instarlarvae, as described previously (Rohrbough et al., 1999). Twoelectrode voltage-clamp recordings were made at a holding potentialof $-$ 60 mV with an Axoclamp 2B amplifier (Axon Instruments, Burlingame,CA). Dissections and recordings were made in modified standardDrosophila saline (Jan and Jan, 1976) containing additional sucrose,composed of (in mM): 128 NaCl, 2 KCl, 4 MgCl₂, 5 trehalose, 70sucrose, 5 HEPES, and 0.15-1.5 CaCl₂; pH-adjusted to 7.1 withNaOH. Gly-Arg-Gly-Asp-Ser-Pro (GRGDSP) inhibitory and Gly-Arg-Ala-Asp-Ser-Pro(GRADSP) control peptides (Calbiochem-Novabiochem, San Diego,CA) were initially solubilized at 2 mM in 0.2 mM Ca²⁺ saline containing 0.02% acetic acid and frozen in ~1 ml aliquots.Aliquots were diluted to a final peptide concentration of 0.2mM in 0.2 mM Ca²⁺ saline (pH 7.1 ± 0.1) on the day of use. Intracellular electrodeswere filled with a 3:1 mixture of 3 M K⁺acetate:KCl and had resistances of 8-15 M $Omega$ . Segmental nerves weresevered near the CNS to eliminate junctional responses originatingfrom CNS activity, and excitatory junctional currents (EJCs) wereevoked by stimulating (0.4-1 msec) the severed nerve at 0.2-20Hz frequencies with a suction electrode filled with external saline.Miniature excitatory junctional currents (mEJCs) were recordedat $-$ 60 mV in 0.2 mM Ca²⁺ saline containing 0.1 µg/ml TTX. Currents were filtered (500-1000Hz), digitized to disk (5 kHz), and analyzed using pClamp6 acquisitionand analysis hardware and software (Axon Instruments). For continuousrecordings of mEJCs, and EJCs in post-tetanic potentiation (PTP)experiments, synaptic currents were detected, and amplitudes weremeasured as described previously (Rohrbough et al., 1999), usingevent-detection and analysis software (ACSPLOUF) written and providedby Dr. P. Vincent. Exemplar EJC traces were averaged from 5-10consecutive individual responses, except for the individual eventsshown in Figures 4B and 5A. Event averaging and amplitude analysiswas performed using pClamp6 and commercial spreadsheetsoftware.

Statistical analysis was performed using Instat Graphpad software. All data are presented as mean ± SEM unless otherwiseindicated.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Volado protein expression at central and peripheral synaptic connections

A role for Volado in memory mechanisms predicts that the VOL protein is expressed at synaptic connections. To investigateneuronal and synaptic VOL expression during development, we stainedwild-type embryonic and larval preparations with a polyclonalantibody that recognizes both VOL isoforms (Grotewiel et al.,1998; see Materials and Methods). VOL immunostaining is not detectedin the nervous system before early second instar (~24 hr afterhatching; data not shown), but thereafter VOL protein is detectableboth in the CNS and at the NMJ. In the CNS, conventional and confocalmicroscopy reveals VOL to be consistently and distinctly localizedto numerous 0.2- to 2-µm-diameter puncta in the ventral nervecord neuropil (Fig. 1A). These puncta, which appear to be synapticboutons, are distributed primarily throughout a path of 10-20µm width running the length of the ventral nerve cord (VNC), althoughthe number and specific pattern of distinguishable VOL-positiveboutons is variable among individual preparations. In addition,VOL appears to be less distinctly concentrated in the VNC midline(Fig. 1A, center panels, B, center left) and occasionally in afew laterally situated neuronal soma (Fig. 1B). We compared VOLexpression pattern in the VNC with that of synaptic vesicle GFP-fusionproteins, Synaptotagmin- (Syt) and Synaptobrevin- (Syb) GFP, transgenicallyexpressed pan-neuronally [using a gal4 (elav) driver] or in aneuronal subset [using a gal4 (4G) driver] (Fig. 1B). In double-labeledCNS preparations, VOL puncta are always contained within the highlyconcentrated and broader area of Syt- or Syb-GFP expression inthe neuropil (Fig. 1B, left and middle), indicating that VOL expressionis limited to a small subset of the central neurons and boutonslabeled by these two proteins. When expressed in a neuronal subset,both Syt- and Syb-GFP are also observed in densely concentratedpuncta and larger aggregate patches, which presumably are individualsynapses or synaptic clusters (Fig. 1B, right). These synapticstructures are present in the same neuropil regions as VOL andstrongly resemble VOL puncta in their size and distribution, furthersuggesting that VOL is localized to subsets of synaptic boutons.VOL immunoreactivity is completely absent or only weakly detectedin the CNS of third instar Vol³ and Vol⁴ mutants (see below) (Fig. 1A, right). Strong VOL immunostainingis also present in the salivary glands, midgut, and dorsal vesselof wild-type embryos; this staining is absent in embryos homozygousfor a Volado deficiency (data not shown). Both of these controlsindicate specificity of the antibody for the VOL protein.

View larger version (84K):
[in this window]
[in a new window]
Figure 1. Volado (VOL) protein is localized to synaptic connections in the central neuropil. A, VOL expression in the CNS neuropil of third instar wild-type larvae. Left, VOL is localized to 0.2- to 2-µm- diameter puncta resembling synaptic boutons (arrows) within the central neuropil (np, neuropil; vm, ventral midline). Center left and right, Confocal images of localized VOL expression (in green) at synaptic boutons in the central neuropil; magnification is increased twofold in center right panel. Images are Z-series projections of five 1 µm sections (left) and eight 1 µm sections (right). VOL synaptic bouton staining is absent in the central neuropil of a third instar Vol⁴ mutant larva (Z-series projection of six 1 µm sections (rightmost panel). Scale bar: Left, center left, 20 µm; center right, right, 10 µm. B, Comparison of VOL CNS expression with presynaptic Syt and Syb proteins. Left, Z-series (8 µm depth) image of pan-neuronally driven Syt [gal4 (elav): Syt-GFP] concentrated throughout the entire central neuropil; line indicates neuropil margins. Compare with left panels in A. The bottom panel shows a higher magnification image in the neuropil of another CNS; Syt-GFP synaptic puncta (arrows) are visible within a background of Syt expression. Center left, Syb-GFP (green) expressed in a subset of central neurons [gal4 (4G): Syb-GFP] to better visualize synaptic puncta and aggregates. VOL punctate expression (red) is completely contained within the Syb-GFP expression domain in the synaptic neuropil. VOL occasionally also labels a few laterally situated cell bodies. Image is a Z-series of 11 µm depth. Center right, A second Z-series image (4 µm depth) from the boxed region at higher magnification; arrows indicate examples of discrete synaptic puncta labeled by both markers. Right panels, Magnified examples of VOL, Syb-GFP, and Syt-GFP synaptic puncta, showing similarity of the localized synaptic expression of all three proteins. Syb- and Syt-GFP are expressed in a subset of neurons using the gal4 (4G) driver. Scale bars: top left, center left, 20 µm; all other panels, 10 µm.

The VOL protein is also localized to the NMJ throughout late larval development (Fig. 2). At the majority of NMJs in wild-typelarvae, VOL immunostaining in the synaptic terminal is presentonly at low levels near the limit of detection (Fig. 2A). Thisexpression is distinctive compared to that of the other knownDrosophila synaptic integrins ( $alpha$ PS1, $alpha$ PS2, $beta$ PS), which are stronglyconcentrated at all large (type Ib and Is) synaptic boutons atthe NMJ (Beumer et al., 1999). However, strong bouton-specificVOL expression is clearly present in a subset of synaptic boutonsat NMJs in nearly all third instar larvae (44 of 47 examined;Table 1). Localized VOL expression is found in as few as 1-3boutons, to as many as one or two dozen, of the several dozensto hundreds of synaptic boutons composing the synaptic terminal.VOL is clearly localized to both large type I boutons as wellas smaller type II and III boutons at multiple classes of NMJs(Fig. 2B,C, Table 1). The highest frequency of strong synapticbouton expression (23%) occurs at the muscle 12/13 NMJ, a complexterminal that receives all three types of innervation (Fig. 2C);however, comparable localized expression was observed at all otherclasses of NMJs examined (Table 1). At NMJs double-stained againstVOL and the presynaptically localized cysteine string protein(CSP), VOL and CSP appear to be colocalized at multiple typesof boutons (Fig. 1C), suggesting that VOL has a primarily presynapticlocalization. Thus, as in the CNS, localized VOL expression atthe NMJ appears to be restricted to a small and variable subsetof synaptic boutons in individual animals at a given time.

View larger version (49K):
[in this window]
[in a new window]
Figure 2. VOL is localized to synaptic boutons at the NMJ in wild-type third instar larvae. A, Confocal images at a type I NMJ (muscle 4) double-stained with antibodies against VOL (top, green) and the primarily postsynaptic Disks-large (DLG) protein (center, red), which is localized to all type I boutons. VOL immunostaining is weakly observed in nerve branches (n), presynaptic axons (a), and the synaptic terminal arbor. Arrows indicate two individual type I boutons. Bottom panel shows the green and red images merged. Scale bar, 10 µm. B, Confocal images at a muscle 12 NMJ, which receives multiple (type I, II, and III) innervation, double-stained against VOL (top, green) and the presynaptic CSP protein (center, red). VOL immunostaining is strongly localized to multiple subtypes of synaptic boutons (arrows); insets show several VOL-positive boutons at threefold greater magnification. VOL staining colocalizes with CSP staining, suggesting VOL localization is primarily presynaptic. Bottom panel shows the green and red images merged. Scale bar, 10 µm. C, Conventional (top and center) and confocal images (bottom) of variable VOL immunostaining at NMJs. Strong VOL localization is observed in a small subset of boutons at each terminal. Scale bars, 10 µm in each panel.


View this table:
[in this window]
[in a new window]
Table 1. Summary of Volado immunoreactivity in Drosophila larvae

These synaptic protein expression characteristics are unique to VOL among the other PS integrins and other known Drosophilasynaptic proteins described to date. However, VOL is clearly ahighly, if variably, expressed synaptic protein, and a functionalrole for VOL at synaptic connections is supported by the strong,broad-ranging synaptic phenotypes observed in Volado mutants,describedbelow.

Morphological synaptic overgrowth at Volado mutant NMJs

The Volado gene encodes two mRNA transcripts (Stark et al., 1997; Grotewiel et al., 1998), previously designated Vol-long(Vol-l) and Vol-short (Vol-s) (Grotewiel et al., 1998). Both transcriptsare expressed throughout the majority of embryonic and larvaldevelopment, as well as in adults (Stark et al., 1997; Grotewielet al., 1998). The viable Vol¹ and Vol² mutant alleles selectively eliminate Vol-l and Vol-s expression,respectively (Grotewiel et al., 1998). The Vol³ and Vol⁴ alleles were generated by imprecise precision of the P-elementinserted into the Volado gene and contain deletions in the Voladocoding region predicted to eliminate both VOL protein isoforms(see Materials and Methods). These alleles are thus consideredto be either strong hypomorphs or nulls. Homozygous Vol³ and Vol⁴ mutant embryos hatch normally but exhibit increasingly impairedlocomotion in larval stages. Most mutant larvae die during secondand third instars. Although 10-20% survive to mature third instarstage (5-6 d after hatching), few pupate and none survive throughmetamorphosis to adultstages.

Vol³ and Vol⁴ mutant embryos show no obvious defects in neuronal pathfinding or synaptogenesis at the NMJ. Likewise, CNS morphology,peripheral nerve branching, neuromuscular patterning, and numberand distribution of NMJs all appear normal in the mutant larvaeat hatching (data not shown). However, beginning in the mid-secondinstar (~30 hr after hatching), Vol³ and Vol⁴ NMJs exhibit morphological overgrowth in several respects comparedto normal. At two NMJs (6/7 and 4) analyzed in third instar larvae,mutant terminals are significantly enlarged and overgrown, exhibiting60-100% more synaptic terminal branches and 30-40% more synapticboutons than NMJs in control larvae (Fig. 3). These results suggestthat VOL has a role in limiting morphological synaptic terminalgrowth at most, if not all NMJs despite its limited localizationin most terminals at a given time.

View larger version (109K):
[in this window]
[in a new window]
Figure 3. NMJs of lethal Volado mutants exhibit morphological overgrowth. A, Synaptic terminal morphology visualized with CSP immunostaining in yw control (left panels) and Vol⁴ mutant third instar larvae (right panels) at the NMJs of muscle 6/7 (top) and muscle 4 (bottom). Arrows indicate individual type I synaptic boutons; the nerve branch (n) and presynaptic axon (a) at muscle 4 are indicated in bottom panels. Vol³ and Vol⁴ mutant NMJs have larger terminal arbors, increased terminal branching, and increased numbers of synaptic boutons compared to control NMJs. Scale bar, 20 µm. B, Quantification of terminal branching and synaptic bouton number in lethal Volado mutants. The Vol⁴ allele has significantly greater numbers of higher-order (2-3^o) terminal branches at the muscle 4 NMJ; both Vol³ and Vol⁴ NMJs have significantly greater total number of branches than control NMJs (left). Synaptic bouton number is increased in both mutant alleles at both muscle 4 and muscle 6/7 NMJs (right); dots indicate significance at $bullet$ p < 0.05 and $bullet$ $bullet$ p < 0.01; ANOVA and Dunnett's multiple comparisons test. Legend indicates number of larvae analyzed in both plots.

Altered amplitude and Ca²⁺ dependence of transmission at Volado mutant synapses

Functional synaptic transmission properties were recorded at the NMJ in third instar larvae both for the viable Vol¹ and Vol² hypomorphs that display adult STM defects and for the lethalVol³ and Vol⁴ alleles. At a physiological level of external Ca²⁺ (1.5 mM), mutant NMJs display essentially normal transmission.EJCs evoked at basal stimulation frequencies (0.2-0.5 Hz) havecomparable peak amplitudes and variability in both viable andlethal Vol mutants as in yw control larvae (241 ± 19 nA, yw; 278± 18 nA, Vol¹; 225 ± 32 nA, Vol²; 265 ± 13 nA, Vol³; 212 ± 17 nA, Vol⁴; n $>=$ 6 for each genotype) (Fig. 4A,C), as well as normal responsesto higher frequency stimulation (10-20 Hz; data not shown). However,as external Ca²⁺ concentration is progressively reduced (<0.5 mM), EJC amplitudesdisplay greater variability among mutant larvae and larger overallmean amplitudes (Fig. 4A-C). In 0.2 mM Ca²⁺, the elevated transmission is least pronounced for Vol² animals, but highly significant for the Vol¹, Vol³, and Vol⁴ alleles (p < 0.01, ANOVA and Dunn's multiple comparisons test),which each have threefold to fourfold larger EJC amplitudes onaverage than control larvae (Fig. 4B). The indistinguishable transmissionphenotypes for these latter three alleles indicate that the alteredsynaptic function is attributable to a deficiency in VOL and notto the lethality associated with Vol³ and Vol⁴ mutants. Over the 0.15-0.25 mM concentration range, Vol² transmission displays normal dependence on external Ca²⁺, exhibiting a slope of 3.6 for the logarithmic relationship betweenEJC amplitude and Ca²⁺ concentration, compared to a control slope of 3.7. By contrast,the other three Vol mutant alleles each display reduced slopes,ranging from 2.6 to 2.9, indicating similarly reduced Ca²⁺ dependence of transmission (Fig. 4C).

View larger version (30K):
[in this window]
[in a new window]
Figure 4. Increased synaptic transmission amplitude and decreased Ca²⁺ dependence of evoked transmitter release at Vol mutant NMJs. A, EJCs recorded from yw control and lethal Vol mutant (Vol³, Vol⁴) larvae in 0.2 mM (top), 0.4 mM (middle), and 1.5 mM external Ca²⁺ (bottom). Each trace shows the average of 10 consecutive EJCs evoked at basal stimulation frequency (0.2-0.5 Hz). Mutant EJC amplitudes deviate significantly from those in control animals in 0.4 mM or lower external Ca²⁺. All recordings were made from muscle 6 in abdominal segments A3-A4 of third instar larvae at 18°C. B, Mean EJC amplitudes in 0.2 mM Ca²⁺ for yw and ry control larvae (solid and hatched bars, respectively), viable Vol mutants (Vol¹, Vol²; shaded bars), and lethal Vol mutants (Vol³, Vol⁴; open bars). EJC amplitudes among Vol mutant larvae exhibit significantly greater variability than in control larvae (p < 0.0001; one-way ANOVA). Mean EJC amplitude for Vol² larvae is elevated but not significantly different from control. Mean EJC amplitudes for Vol¹, Vol³, and Vol⁴ mutants are significantly greater than for control larvae ( $bullet$ $bullet$ p < 0.01, Vol³; $bullet$ $bullet$ $bullet$ p < 0.001, Vol¹ and Vol⁴; nonparametric ANOVA and Dunn's multiple comparisons test). Number of larvae is indicated within bars for each genotype. C, Logarithmic plot of mean EJC amplitudes versus external Ca²⁺ concentration for yw control (solid circles), viable Vol mutants (shaded symbols), and lethal Vol mutants (open symbols). Mutant EJC amplitudes are comparable to control values at physiological Ca²⁺ levels (1.5 mM) but become progressively increased relative to control EJC amplitudes at more reduced Ca²⁺ concentrations. Each point represents the mean value for at least five larvae from each genotype. Inset shows the data plotted for 0.15-0.25 mM Ca²⁺ concentrations and fit to power relationships (straight lines). The Vol² allele exhibits normal dependence of transmission amplitude on external Ca²⁺ (slope of 3.6 vs 3.7 for control). The Vol¹, Vol³, and Vol⁴ alleles exhibit strongly elevated EJCs and reduced Ca²⁺ dependence of transmission (slopes of 2.6, Vol¹; 2.8, Vol³; and 2.9, Vol⁴). D, mEJC amplitude and frequency at yw control (solid bars) and Vol³ and Vol⁴ mutant NMJs (open bars). mEJCs were recorded at $-$ 60 mV in 0.2 mM Ca²⁺ containing 0.1 µg/ml TTX (n = 8 larvae for each genotype). Neither mutant allele has altered mEJC variability (0.24 ± 0.01 nA, yw; 0.28 ± 0.02 nA, Vol³; 0.23 ± 0.01 nA, Vol⁴) or mean amplitude (top plot) compared to control. mEJC frequency in Vol⁴ larvae is increased by 63% relative to control ( $bullet$ p < 0.05), but no difference is observed for Vol³ larvae (bottom plot; ANOVA and Dunnett multiple comparison test).

To determine whether increased mutant EJC amplitudes result from greater number of postsynaptic glutamate receptors or fromincreased probability of quantal transmitter release, we recordedspontaneous mEJCs in control, Vol³, and Vol⁴ larvae in 0.2 mM Ca²⁺. Control and mutant NMJs have indistinguishable mEJC variabilityand mean amplitudes, indicating mutant postsynaptic glutamatereceptor density is not significantly altered (Fig. 4D). A modestbut significant increase in mEJC frequency is observed in Vol⁴ mutants (63% over control; p < 0.05 vs control; ANOVA and multiplecomparisons test; Fig. 4D). This increase could be attributedto the increased number of synaptic boutons at mutant NMJs; however,mEJC frequency is not altered in Vol³ mutants, although they display the same increase in bouton number.Despite this slight allelic difference, mutant NMJs exhibit nochanges in mEJC amplitude or frequency sufficient to account forthe threefold to fourfold increase in evoked EJC amplitude underthe same recording condition. We therefore conclude that VOL specificallyregulates Ca²⁺-dependent, evoked neurotransmitter releaseprocesses.

Loss of functional plasticity at Volado mutant synapses

To assess the role of VOL in synaptic modulation processes, we next examined several forms of Ca²⁺- and activity-dependent plasticity previously shown to be alteredin other Drosophila learning/memory mutants (Zhong and Wu, 1991;Wang et al., 1994; Broadie et al., 1997; Rohrbough et al., 1999).Volado mutant NMJs display significant defects in two forms ofshort-term facilitation, paired-pulse facilitation (PPF) and frequency-dependentshort-term facilitation (STF), measured in 0.2 mM Ca²⁺ (Fig. 5). At control NMJs, EJC amplitude is facilitated (PPF)by paired stimuli at 20-100 msec intervals, with approximatelytwofold PPF at 20 msec intervals (Fig. 5A). For the Vol² allele, which has basal transmission properties most similarto control, PPF is essentially normal. Among the other three mutantstrains, which all exhibit strongly elevated, or "prefacilitated"EJC amplitudes in 0.2 mM Ca²⁺, PPF in Vol¹ animals is reduced by ~35% at the briefest interval (20 msec),and more severely reduced (by 50-60%) for the Vol³ and Vol⁴ alleles at 20-30 msec intervals (Fig. 5A). Paired-pulse depression,which was never observed in controls, also occurred in severalVol³ and Vol⁴ animals (data not shown).

View larger version (39K):
[in this window]
[in a new window]
Figure 5. Short-term forms of synaptic facilitation are greatly impaired at lethal Vol mutant NMJs. Short-term facilitation was evoked in 0.2 mM Ca²⁺ with paired stimuli (20-100 msec intervals) and short trains (20 stimuli) at 2-20 Hz. A, PPF. Right, Traces show averages of 5-10 responses to paired stimuli delivered at 20 msec intervals. Examples are shown for two larvae each for control (yw, top) and lethal Vol mutant alleles (Vol³, middle; Vol⁴, bottom). Left, Mean PPF ratio (I₂/I₁) is plotted for each stimulus interval. For each stimulus interval, 5-10 responses (separated by 5 sec rest) were averaged. I₂/I₁ is defined as the ratio: mean amplitude of response 2/mean amplitude of response 1. I₂ peak amplitudes were determined relative to a baseline value immediately preceding the second EJC. Of the viable mutant alleles, Vol ² PPF (shaded squares) is indistinguishable from control, whereas Vol¹ (shaded triangles) exhibits reduced PPF at the briefest interval (20 msec). Both Vol³ and Vol⁴ lethal alleles (open symbols) exhibit strongly impaired PPF at 20-30 msec intervals, at which facilitation is normally greatest. Number of larvae for each genotype is indicated in legends. B, STF. Right, Representative responses to 20 Hz stimulation trains. The first 10 consecutive EJCs are shown (response number indicated above traces), with the average of the last 10 of 20 responses in the train shown in the rightmost traces (average, 11-20). STF at each frequency was defined as the average amplitude of responses 11-20, normalized to mean EJC amplitude at the basal stimulation frequency (0.5 Hz). Stimulus trains were separated by 10-20 sec rest. EJC amplitude rapidly facilitates by several-fold at control yw or ry NMJs (yw, top). Vol³ and Vol⁴ mutant NMJs (middle and bottom traces) have greater initial EJC amplitudes and weaker facilitation in response 20 Hz stimuli; in some cases facilitation is absent or replaced with depression (Vol⁴, bottom traces). Left, Mean STF at 2-20 Hz stimulation is plotted for each genotype. Vol² NMJs (shaded squares) have nearly normal STF, whereas Vol¹ (shaded triangles), Vol³ (open triangles), and Vol⁴ (open diamonds) genotypes, respectively, exhibit progressively weaker STF. In particular, Vol⁴ has on average no STF at 2-5 Hz stimulation, and STF reduced to ~20% of control levels at 20 Hz.

Control EJC amplitudes undergo rapid and reversible frequency-dependent STF by as much as threefold to fourfold over initialbasal amplitude, in response to short stimulus trains at 2-20Hz (Fig. 5B). Mutant STF is nearly normal in Vol² larvae, but is significantly (40-50%) reduced at all stimulationfrequencies in Vol¹ larvae. The lethal Vol alleles exhibit severely (>65%) reducedSTF relative to control levels. STF defects are particularly severein many Vol⁴ larvae. In 9 of 17 Vol⁴ animals, facilitation was either absent, or strikingly, gaveway to depression during 10-20 Hz stimulus trains (Fig. 5B, bottomtraces). Basal transmission amplitudes, PPF, and STF were alsoindistinguishable from yw animals in ry control larvae (Figs.3B, 4), ruling out any functional abnormality associated withthe ry chromosome present in Vol¹ and Vol² mutants (Grotewiel et al., 1998; see Materials and Methods).These results indicate that VOL is required for normal short-term,Ca²⁺-dependent synaptic facilitationprocesses.

During more prolonged stimulation at intermediate frequencies (5-10 Hz), the Drosophila NMJ displays sustained augmentationof transmission amplitude and PTP after tetanic stimuli. ControlNMJs display greater than twofold augmentation after 60 sec stimulationat 5 Hz and sustained PTP of 60-65% over initial EJC amplitudefor >5 min (0.2 mM Ca²⁺; Fig. 6). The Volado mutant alleles display impaired augmentationand PTP paralleling the severity of STF defects described above.The Vol¹ allele, which has an intermediate severity of impaired STF, displaysreduced augmentation to ~75% over initial amplitudes and PTP reducedto 70-75% of control strength (Fig. 6B). The Vol² allele, which has essentially normal STF, also displays strongaverage augmentation that peaks near control levels. However,Vol² transmission amplitude decreases dramatically immediately afterthe tetanus, exhibiting only ~40% initial and ~30% sustained PTP,respectively; levels even more severely reduced than for Vol¹ animals (Fig. 6B). The Vol³ and Vol⁴ alleles display severely reduced relative augmentation and PTPcompared to control larvae. Vol³ NMJs on average display only weak augmentation, which increasesgradually to ~25% over initial amplitude; initial and sustainedcomponents of PTP are reduced to 25 and 18% over initial amplitude,respectively. At Vol⁴ NMJs, tetanic stimulation typically produces an initial depressionthat gradually recovers to weak (~15%) augmentation, followedby strongly reduced (~15% over initial amplitudes) average levelsof PTP (Fig. 6A,B).

View larger version (42K):
[in this window]
[in a new window]
Figure 6. Synaptic augmentation and PTP are greatly impaired at lethal Vol mutant NMJs. A, Representative recordings from yw control (top), Vol³ (middle), and Vol⁴ mutant (bottom) NMJs in 0.2 mM Ca²⁺. Synaptic augmentation was induced by a prolonged (60 sec) tetanic stimulation at 5 Hz (hatched bar). PTP was assayed for 4-5 min after termination of the tetanus, at the initial basal stimulation frequency of 0.5 Hz. Traces at left show portions of continuous recordings. EJCs shown at right in expanded time scale are taken from the corresponding continuous records during the initial control period (1), near the end of the tetanus (2), and ~100 sec after tetanus (3) (arrows). Calibration: 10 nA, 30 sec (continuous traces), and 85 msec (EJCs). B, Synaptic augmentation and PTP, normalized to mean initial EJC amplitude for each larva, are summarized for yw control (solid circles), viable Vol (shaded symbols), and lethal Vol mutant genotypes (open symbols). Each point plots the mean normalized amplitude for 20 consecutive EJCs during the tetanus period (hatched bar) and for 10 consecutive EJCs after tetanus. Control NMJs exhibit rapid initial facilitation, followed by a gradual augmentation of EJC amplitude throughout the 1 min tetanus. In control larvae, potentiation of 66% over pretetanus amplitude is observed during the initial minute after tetanus (0-1') and is sustained throughout the 5 min post-tetanus period (61%, 0-5'; see legend to right of plot). PTP for Vol¹ and Vol² alleles is reduced to 50-70% of control levels. Both Vol³ and Vol⁴ alleles exhibit strongly reduced augmentation and PTP, particularly the Vol⁴ allele, which sometimes undergoes depression during tetanic stimulation (note bottom trace in A) and exhibits overall PTP of only 14%. Rapid facilitation and augmentation is dramatically increased in Vol⁴ larvae by further reduction of external Ca²⁺ to 0.15 mM (hatched diamonds), and initial PTP is restored to the level exhibited by control larvae in 0.2 mM Ca²⁺; however, the late component of Vol⁴ PTP (3-5 min) remains decreased relative to control levels. n $>=$ 9 larvae for each genotype.

Because Vol mutant plasticity defects are observed in conjunction with abnormally elevated basal EJC amplitudes, we repeatedPTP recordings from Vol⁴ larvae in 0.15 mM external Ca²⁺, at which Vol⁴ basal EJC amplitude (8.5 ± 5.7 nA, mean ± SD; n = 15) does notdiffer significantly from the control amplitude in 0.2 mM Ca²⁺ (p > 0.10; Mann-Whitney U test). Vol⁴ augmentation under this condition (Fig. 6B, hatched diamonds)is dramatically and unexpectedly increased by nearly 10-fold,surpassing by ~50% yw control augmentation in 0.2 mM Ca²⁺. Despite decreasing sharply from end-tetanus levels, initial(1 min) Vol⁴ PTP is indistinguishable from that of control larvae in 0.2 mMCa²⁺. However, mutant PTP declines within 2-3 min from this initiallevel, and at late time points (4-5 min) is decreased to the rangeobserved for Vol², Vol³, and Vol⁴ mutants in 0.2 mM Ca²⁺. Thus, sustained PTP under these conditions remains impairedat the mutantNMJ.

Expression of Volado transgene in lethal Vol mutant larvae rescues transmission defects

To provide direct evidence that VOL has a specific role in synaptic transmission and plasticity mechanisms, we attempted torescue mutant transmission and plasticity defects by driving conditionalexpression of the Vol-s transcript with a heat-shock promoter(hsp70) (Grotewiel et al., 1998) in homozygous Vol⁴ mutant larvae (Vol⁴-T3/Vol⁴-T3). Vol⁴-T3 larvae receiving multiple heat-shock treatments (see Materialsand Methods) display noticeably improved growth and larger size,robust movement, and improved viability compared to Vol⁴ animals, with a subset of animals rescued to adult viability.Basal EJC amplitude in 0.2 mM Ca²⁺ (Vol⁴-T3 +HS; 11.4 ± 1.2 nA; n = 15) is significantly reduced (p <0.002) from the Vol⁴ mutant level and not different from heat-shocked controls (yw+HS; 9.4 ± 1.0 nA; n = 6) (Fig. 7A). Frequency-dependent STF inheat-shocked Vol⁴-T3 larvae is dramatically improved and rescued essentially tountreated control levels (Fig. 7B). Likewise, in heat-shockedVol⁴-T3 larvae both augmentation to prolonged 5 Hz stimulation andPTP are dramatically strengthened compared to Vol⁴ mutants and rescued to levels comparable to those observed inheat-shocked controls. These results demonstrate that all of thefunctional transmission defects observed in lethal Vol mutants,including synaptic plasticity defects, can be strongly rescuedthrough transgenic expression of the normal VOL protein.

View larger version (22K):
[in this window]
[in a new window]
Figure 7. Conditional Volado expression in Vol⁴ mutant larvae rescues overtransmission phenotype and synaptic plasticity defects. Volado expression in Vol⁴ mutant larvae (Vol⁴-T3/Vol⁴-T3) was heat-shock (HS)-induced (30 min, 37°C), using multiple HS spaced over either 4 d development or over 36 hr before recording (see Materials and Methods). A, HS significantly reduces elevated EJC amplitude at Vol⁴ NMJs (Vol⁴-T3 +HS, right bar vs Vol⁴ ( $-$ HS); p < 0.005) to the level of heat-shocked control larvae (yw +HS; no significant difference vs Vol⁴-T3 +HS). EJC amplitude for yw +HS is increased by 80% over untreated yw larvae. EJC data for yw and Vol⁴ are the same as in Figure 4B. B, HS restores Vol⁴ short-term facilitation (Vol⁴-T3 +HS; shaded diamonds) to untreated control levels (yw ( $-$ HS)). HS also slightly improves STF at intermediate stimulation frequencies in yw larvae (yw +HS; shaded circles). Data for yw and Vol⁴ is the same as in Figure 5B. C, HS largely restores Vol⁴ synaptic augmentation and PTP to levels of heat-shocked controls. Data for yw and Vol⁴ is the same as in Figure 6B.

Replication of Volado mutant transmission phenotype with an RGD integrin inhibitory peptide

Integrin-ligand interactions formed over a comparatively brief period of ~20 min have been implicated in long-term changesin synaptic efficacy (Staubli et al., 1998). Because the alteredsynaptic transmission amplitudes and impaired plasticity in Voladomutants are manifested after constitutively reducing or eliminatingdevelopmental VOL expression, we asked whether acutely inhibitingintegrin function at the Drosophila NMJ results in altered transmissionresembling the Volado mutant transmissionphenotypes.

Control yw larval preparations were incubated for 20 min in 0.2 mM Ca²⁺ saline containing the GRGDSP peptide (RGD; 0.2 mM), which interfereswith integrin binding to ECM ligands containing the RGD consensussequence, or a noninhibitory GRADSP control peptide (RAD; 0.2mM) (Chen and Grinnell, 1995, 1997; Bahr et al., 1997; Stark etal., 1997; Staubli et al., 1998; Graner et al., 1998; Banereset al., 1998). We subsequently recorded EJCs in 0.2 mM Ca²⁺ in the continued presence of either RGD or RAD peptide, at exposuretimes ranging from 20 to 90 min (Fig. 7). RAD-treated controlsshow no effect and have stable EJC amplitudes (7.7 ± 2.4 nA overall,mean ± SD; n = 15) for >1 hr. In contrast, RGD-treated larvaehave elevated EJC amplitudes at initial recording time points(13.1 ± 8.8 nA, 20-25 min; n = 7), and exhibit a further time-dependentincrease in EJC amplitude by more than twofold (Fig. 7A,B). AlthoughNMJs were continuously stimulated at low basal frequencies (0.2-0.5Hz), there appeared to be a synergistic effect of combined activityand RGD exposure on transmission. EJC amplitudes after 20-30 minrecording in RGD were typically greater than those recorded initiallyin experiments begun at later exposure times (Fig. 7B). Transmissionamplitudes after 30-60 min RGD exposure are comparable (20-40nA) to those recorded in untreated Vol³ and Vol⁴ mutant larvae, and are twofold to threefold larger than for RADcontrols at exposure times $>=$ 30 min (p < 0.05; Fig. 7C). In addition,after prolonged RGD exposure relative STF in response to 10-20Hz (Fig. 7A, bottom traces) or paired pulse stimuli (data notshown) is significantly reduced compared to RAD-treated controls,an effect resembling Volado mutant short-term plasticitydefects.

Vol⁴ mutants exposed to 0.2 mM RGD have initial EJC amplitudes after 20-25 min exposure (17.6 ± 4.0 nA, mean ± SD; n = 4) comparableto those recorded from untreated Vol⁴ larvae (20.7 ± 10.8 nA; n = 28) in 0.2 mM Ca²⁺ (Fig. 8B,C; compare to Fig. 4B). Vol⁴ EJC amplitude also increases significantly over the course of>1 hr total RGD exposure (30.8 ± 11.1 nA, >60 min, n = 4 vs amplitudeat 20-25 min, p < 0.02, Mann-Whitney U test); however, the relativetransmission increase (75%) is less than observed for RGD-treatedyw larvae over a similar time period. The RGD-dependent transmissionchanges at normal NMJs strongly support a role for synaptic integrins,including VOL, in the modulation of transmission efficacy.

View larger version (39K):
[in this window]
[in a new window]
Figure 8. Inhibition of functional integrin interactions at the NMJ phenocopies Volado mutant synaptic transmission. A, EJCs (averages of 10 consecutive responses evoked at 0.2-0.5 Hz) recorded in yw larvae in 0.2 mM Ca²⁺ saline containing the integrin RGD inhibitory peptide (0.2 mM; left) or the noninhibitory control RAD peptide (0.2 mM; right). Dissected preparations were incubated with RGD- or RAD-containing saline for 20 min before beginning recording; total peptide exposure time (in minutes) is indicated above traces. Each row of traces was recorded from one NMJ. Left, EJCs recorded from RGD-treated NMJs. In bottom example, initial EJC amplitude (25 min RGD) is significantly elevated, and both RGD-treated NMJs exhibit a progressive increase in EJC amplitude over the 20-30 min recording period. After prolonged (>1 hr) RGD exposure, EJC amplitude can usually be further facilitated by 10-20 Hz stimulation (bottom right trace, 57 min, 10 Hz stimulation; last 10 of 20 responses are averaged as in Fig. 4B), but relative STF is significantly weaker than in RAD-treated controls (n = 4). Right, EJC amplitudes in RAD-treated NMJs (right) are comparable to those of untreated yw larvae, remain stable throughout continuous 25-30 min recordings, and exhibit robust facilitation to 10-20 Hz stimulation after >1 hr RAD exposure (bottom right trace, 62 min, 10 Hz stimulation). B, C, Time course of RGD-dependent alteration of transmission. B, EJC amplitudes recorded in RGD-treated yw control (open circles; n = 18) and Vol⁴ mutant larvae (shaded diamonds; n = 17) are plotted versus peptide exposure time. Control recordings from RAD-treated yw larvae are plotted in solid circles (n = 15). Symbols connected by lines represent continuous recordings from individual larvae. Mean EJC amplitudes (0.2-0.5 Hz stimulation) are plotted at 5 min intervals, except for several points recorded at intermediate (2.5 min) intervals. Most RGD-treated NMJs in yw larvae have elevated initial EJC amplitudes (20-30 min exposure) relative to RAD-treated controls and exhibit further increased EJC amplitude with increased exposure time and activity. EJC amplitudes in RGD-treated Vol⁴ mutant larvae at initial time points (20-25 min) are similar to those recorded in untreated Vol⁴ animals (compare with Fig. 3B) and also increase with RGD exposure time and stimulation. C, Mean EJC amplitudes for the experiments shown in B are averaged and binned at 20-25, 30-35, 40-45, 50-55, 60-65, 70-75, and 80-95 min exposure intervals. The number of recordings pooled in each time bin is indicated in parentheses; error bars indicate SEM for n $>=$ 3. In RAD-treated control larvae (solid circles), mean EJC amplitudes are stable for >1 hr. EJC amplitude is elevated approximately twofold after 20 min RGD exposure (open circles) compared to RAD-treated controls (solid circles). Prolonged (>1 hr) RGD exposure increases EJC amplitude by an additional 2- to 2.5-fold, producing a transmission phenotype comparable to that observed in Vol¹, Vol³, and Vol⁴ mutants (Fig. 3A,B). RGD-treated Vol⁴ larvae have elevated initial EJC amplitudes similar to those of untreated Vol⁴ larvae. Transmission is further increased by ~75% with exposure time and activity, suggesting multiple synaptic integrins are disrupted by RGD.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Integrins have only recently been shown to be localized to adult learning centers, including the mammalian hippocampus andDrosophila mushroom bodies (Einheber et al., 1996; Grotewiel etal., 1998; Pinkstaff et al., 1999). In the hippocampus, inhibitingintegrin binding to ligands containing the consensus Arg-Gly-Aspsequence within ~20 min of LTP induction blocks the subsequentconsolidation of LTP (Staubli et al., 1998). This time period(~20 min) is similar to that during which both LTP and early memoriesare easily disrupted (Staubli et al., 1998) and to the early componentof memory (3-15 min) specifically affected in Volado mutants (Grotewielet al., 1998), suggesting that integrin activation and signalingact over a course of a few minutes to stabilize these processes.The rescue of mutant STM defects by transgenic Volado expression3 hr before training demonstrates that the presence of VOL duringan interval including the learning period is sufficient for normalmemory formation (Grotewiel et al., 1998). The memory requirementof Volado prompted us to examine its synaptic role, particularlyin functional modulation processes related to those thought tounderlie learning and memory. Our results complement these recentcellular and behavioral studies and demonstrate a role for theVOL $alpha$ -integrin in regulating synaptic morphology, functional transmission,and activity-dependentplasticity.

Volado synaptic expression and localization

VOL protein is present at low levels throughout most larval synaptic terminals in fixed preparations. In contrast, stainingis strongly localized to a limited and variable subpopulationof central and peripheral synapses. Localized punctate VOL expressionis present extensively in the CNS neuropil, contained within thebroader expression domains of the constitutive presynaptic proteinsSynaptotagmin (Syt) and Synaptobrevin (Syb). When transgenicallyexpressed in a neuronal subset [using the gal4 (4G) driver], Syt-GFPand Syb-GFP are observed to be concentrated in extensive punctaand varicosities resembling VOL-localized expression, stronglysupporting the conclusion that VOL is indeed concentrated at centralsynaptic boutons. Likewise, at the NMJ localized VOL expressionis observed at all classes of terminals and at all morphologicalclasses of synaptic boutons. Thus, VOL is clearly expressed ina variable population of central and peripheral synapticboutons.

There are several alternative ways to interpret the intriguing and unusual pattern of synaptic VOL expression. First, VOLmay be present only transiently, may be restricted to an extremelylimited population of synapses, or both. However, the significantmorphological and functional phenotypes exhibited at mutant NMJsare inconsistent with VOL functioning only at a limited subsetof boutons or synapses. A second hypothesis that is consistentwith the morphological and physiological data is that VOL is expressedat most or all NMJs, but it is concentrated at detectable levelsat a subset of terminals and in a variable number of boutons ata given time. One possibility is that VOL is transiently concentratedto distinct boutons in response to an inducing signal. Althoughwe currently have no direct evidence for such dynamic relocalization,it is consistent with previous integrin studies and all of thedata presented in this study. A third possibility, which we cannotpresently exclude, is that an unknown mechanism that causes epitopemodification or masking of the antibody recognition site createsvariability in the level of VOL immunostaining. The more extensivelocalization of the protein to the central neuropil likely reflectsthe high density of synaptic connections in this region or differencesin the dynamic regulation of localized expression by activityor other mechanisms. However, the observation of VOL expressionin variable subsets of synaptic boutons is consistent in bothcentral and peripheral synapticterminals.

Volado regulates morphological growth, functional transmission, and activity-dependent plasticity at the NMJ

Vol mutant NMJs exhibit moderate but significant overgrowth at multiple terminal types, suggesting VOL has a broad developmentalrole in limiting morphological synaptic growth. The altered evokedtransmission amplitudes and defective plasticity properties inVol mutants, however, indicate that VOL has an additional functionalrole regulating synaptic transmission and activity-dependent synapticmodulation. The severity of transmission phenotypes among bothviable and lethal mutant (Vol¹, Vol³, Vol⁴) animals again strongly suggests that VOL directly regulatesfunction throughout the synapse, or alternatively, is able toindirectly influence the function of a broader area via some signaltransductionpathway.

Both viable (Vol¹) and lethal Vol mutant alleles (Vol³, Vol⁴) display abnormally elevated evoked transmission amplitudes, alteredCa²⁺ dependence of transmission, and severe defects in short-termplasticity at the NMJ. In the viable Vol² memory mutant, basal transmission amplitude and short-term plasticityare essentially normal. However, all alleles, including Vol², display significantly reduced PTP, indicating that mutant plasticitydefects do not result simply from elevated basal transmissionlevels. It should be stated clearly that these forms of synapticplasticity at the NMJ, although highly conserved at central synapses,cannot be directly correlated to particular phases of behaviorallearning or memory. The Vol mutant defects are consistent, however,with an inability to rapidly modulate transmission in responseto increased presynaptic activity and to maintain changes in transmissionstrength in the absence of maintained input, plasticity propertiesthat are likely to be relevant for memoryformation.

Conditional expression of the Vol-s isoform in the lethal Vol⁴ allele dramatically rescues transmission amplitude, STF, augmentation,and PTP to levels near or equal to those at control NMJs. Similarresults were obtained by driving VOL expression over most of larvaldevelopment, or over ~36 hr in late larval stages. The subtledifferences in the completeness of rescue of individual transmissionproperties may indicate different sensitivities to the timingand level of VOL expression relative to normal, or different functionsfor the Vol-l and Vol-s isoforms. These results strongly supporta direct role for VOL in synaptic transmission and plasticitymechanisms. Whereas the pharmacological perturbation with theRGD integrin inhibitory peptide lacks the specificity of the Voladogenetic knock-out and transgenic rescue approach, it offers theonly available means of assessing the consequence of acutely disruptingnormal synaptic integrin function. At wild-type NMJs, exposureto RGD rapidly (within 30-60 min) leads to increased transmissionamplitude and loss of presynaptic short-term facilitation. Thesimilarity of the RGD-dependent modulation of transmission tothe Vol mutant phenotype suggests VOL may mediate this rapid modulation.Consistent with this possibility, the $alpha$ VOL sequence includes threeconsensus extracellular Ca²⁺-binding domains (Grotewiel et al., 1998) conserved in integrinRGD receptors (Baneres et al., 1998). However, the ligand interactionsof VOL are not yet characterized. Our results also indicate thatthe RGD-dependent modulation may be mediated in part by othersynaptic integrins. The most likely such candidate is $alpha$ PS2/ $beta$ PS,which is abundantly localized to type I boutons at the NMJ (Beumeret al., 1999) and has been shown to mediate RGD-dependent celladhesion in vitro (Graner et al., 1998). These results primarilydemonstrate that acutely altering synaptic integrin function inDrosophila, as in vertebrates (Chen and Grinnell, 1995, 1997;Staubli et al., 1998), can rapidly and dramatically modulate transmissionefficacy.

Potential mechanisms for integrin-mediated modulation of synaptic function and memory

Our results show that integrin interactions at the synapse stabilize basal transmission, mediate rapid (minutes) changes intransmission strength, and are required for normal Ca²⁺- and activity-dependent forms of plasticity. The cellular mechanismsby which VOL regulates synaptic transmission and memory formationand the significance of its variable pattern of synaptic localizationremain to be determined. The richness of known integrin interactions(Hynes, 1992; Clarke and Brugge, 1995; Jones, 1996) suggests multiplepotential roles for VOL in synaptic mechanisms (Grotewiel et al.,1998). One possibility is that $alpha$ VOL, with its $beta$ PS integrin partner(Stark et al., 1997), is linked to or positioned to interact withthe synaptic vesicle fusion machinery. Integrins have recentlybeen reported to be localized to active zones of neuromuscularsynapses (Cohen et al., 2000). Such a close relationship withpresynaptic Ca²⁺ channels and the Ca²⁺-sensitive vesicle fusion machinery could position integrins todirectly modulate the probability of transmitter release in responseto Ca²⁺ influx, thereby regulating both evoked release and rapid modulatoryprocesses. Disrupting this relationship in Volado mutants mightaccount for increased EJC amplitudes, reduced Ca²⁺ dependence of transmission, loss of short-term forms of Ca²⁺-dependent plasticity, and the rapid phenocopying of similar synapticdefects by the RGDpeptide.

For synaptic integrins to contribute to long-term changes in synaptic efficacy, however, interactions with additional cellularsignaling pathways would appear necessary. Memory and long-termexperimental forms of synaptic plasticity are known to requireCa²⁺- and cAMP-dependent signaling (Hawkins et al., 1993; Bailey etal., 1996), and both appear to be accompanied by prolonged functionalmodulation of transmission properties, and/or the physical stabilizationor addition of synaptic connections (Bailey, 1999; Engert andBonhoeffer, 1999; Maletic-Savatic et al., 1999; Murase and Schuman,1999). Dynamic changes in the structure and function of synapticconnections could potentially be regulated by altered integrinadhesion and signaling function, triggered by increased synapticactivity. Localized integrin expression is detected in hippocampaldendritic spines and postsynaptic densities (Einheber et al.,1996), and appearance of new dendritic spines has been documentedwithin minutes after LTP induction (Engert and Bonhoeffer, 1999;Maletic-Savatic et al., 1999), suggesting integrins could be usedin formation or stabilization of new synapses or structural changesto existing contacts. Transient changes in cytosolic Ca²⁺ levels are known to regulate subcellular integrin redistributionand cell morphology (Lawson and Maxfield, 1995; Bixby and Bookman,1996). It was recently reported that intense synaptic activationstimulates the cellular relocalization and molecular stabilizationof another class of cell adhes