Functional and Biochemical Analysis of the C2 Domains of Synaptotagmin IV

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Vol. 10, Issue 7, 2285-2295, July 1999

Functional and Biochemical Analysis of the C2 Domains of Synaptotagmin IV

David M. Thomas,^* Gregory D. Ferguson,^§ Harvey R. Herschman,^§ and Lisa A. Elferink^*^¶

^*Department of Biological Sciences, Wayne State University, Detroit, Michigan 48202; and Molecular Biology Institute and Departments of ^§Biological Chemistry and Molecular and Medical Pharmacology, University of California, Los Angeles, California 90095-1570

Submitted December 2, 1998; Accepted May 3, 1999
Monitoring Editor: Ari Helenius

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Synaptotagmins (Syts) are a family of vesicle proteins that have been implicated in both regulated neurosecretion and generalmembrane trafficking. Calcium-dependent interactions mediatedthrough their C2 domains are proposed to contribute to the mechanismby which Syts trigger calcium-dependent neurotransmitter release.Syt IV is a novel member of the Syt family that is induced bycell depolarization and has a rapid rate of synthesis and a shorthalf-life. Moreover, the C2A domain of Syt IV does not bind calcium.We have examined the biochemical and functional properties ofthe C2 domains of Syt IV. Consistent with its non-calcium bindingproperties, the C2A domain of Syt IV binds syntaxin isoforms ina calcium-independent manner. In neuroendocrine pheochromocytoma(PC12) cells, Syt IV colocalizes with Syt I in the tips of theneurites. Microinjection of the C2A domain reveals that calcium-independentinteractions mediated through this domain of Syt IV inhibit calcium-mediatedneurotransmitter release from PC12 cells. Conversely, the C2Bdomain of Syt IV contains calcium binding properties, which permithomo-oligomerization as well as hetero-oligomerization with SytI. Our observation that different combinatorial interactions existbetween Syt and syntaxin isoforms, coupled with the calcium stimulatedhetero-oligomerization of Syt isoforms, suggests that the secretorymachinery contains a vast repertoire of biochemical propertiesfor sensing calcium and regulating neurotransmitter releaseaccordingly.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Synaptotagmins (Syts) are a large family of vesicle proteins implicated in neurotransmitter release from neural and neuroendocrinetissues. All Syt isoforms are characterized by an amino-terminalintravesicular domain, a single transmembrane domain, and a largecytoplasmic region containing two homologous repeats termed C2domains (C2A and C2B). A role for the C2 domains of Syt I in modulatingneurotransmitter release is well established (O'Connor et al.,1994; Südhof and Rizo, 1996). The first C2 (C2A) domain of SytI consists of an eight-stranded $beta$ -sandwich containing a C2 key(Sutton et al., 1995). Structural and mutational studies indicatethat calcium binds to the top of the domain via five clusteredaspartic acid residues. Calcium binding does not induce significantconformational changes in the Syt I C2A domain but rather increasesits affinity for effector molecules such as negatively chargedphospholipids and the plasma membrane protein syntaxin 1a (Stx1a) (Perin et al., 1990; Bennett et al., 1993a; Davletov and Südhof,1993; Chapman et al., 1995; Li et al., 1995; Shao et al., 1996,1997). Microinjected recombinant Syt I C2A fragments inhibit neurotransmitterrelease from squid giant presynaptic terminals, adrenal chromaffincells, and neuroendocrine PC12 cells (Elferink et al., 1993; Mikoshibaet al., 1995; Ohara-Imaizumi et al., 1997). Mutational studieswith recombinant Syt I C2A fragments reveal that the inhibitoryeffect of these fragments on neurotransmitter release from PC12cells involves calcium-independent events mediated through a polybasicmotif, which is highly conserved in the C2A domains of eight Sytisoforms (Thomas and Elferink, 1998). Therefore, the C2A domainof Syt I contains distinct calcium-dependent and -independentactivities, which may function in concert to trigger neurotransmitterrelease.

The second C2 domain (C2B) of Syt I mediates several calcium-dependent and -independent interactions. The Syt I C2B domainbinds clathrin AP-2, high inositol polyphosphates, brain-specificsoluble NSF attachment protein, N-type calcium channels, and Stx1a in a calcium-independent manner (Niinobe et al., 1994; Zhanget al., 1994; Li et al., 1995; Kee and Scheller, 1996; Sheng etal., 1997). Conversely, calcium promotes the oligomerization ofSyt I through its C2B domain (Chapman et al., 1996). Evidencesupporting a role for calcium-stimulated oligomerization in SytI function comes from genetic studies. In Drosophila, a subsetof mutations in the Syt I C2B domain reduces the calcium responsivenessof neurotransmitter release (Littleton et al., 1994). These studiessuggest that oligomer assembly is essential for Syt I functionin synaptictransmission.

The high degree of conservation between the C2 domains of neural-specific and ubiquitously expressed Syts suggests that theseproteins play a critical role in regulated neurosecretion as wellas general membrane trafficking events. Syt IV expression is restrictedto neural and neuroendocrine tissues (Vician et al., 1995). SytIV is an immediate-early gene, whose expression is induced afterkainic acid-induced seizures in rat brain and depolarization ofneuroendocrine PC12 cells (Vician et al., 1995). The C2A domainof Syt IV does not bind calcium because of the presence of a serineresidue at position 244 in the putative calcium coordination site.Substitution of this serine residue with an aspartic acid residueendows the Syt IV C2A domain with calcium binding properties (vonPoser et al., 1997).

In this study, we examine the biochemical and functional properties of the C2 domains of Syt IV. Our studies demonstrate thatthe C2A domain of Syt IV contains distinct calcium-independentStx binding properties, which may modulate neurotransmitter release.Microinjection of a recombinant Syt IV C2A fragment perturbs depolarization-inducedsecretion from PC12 cells. Furthermore, the inhibitory effectof this fragment involves calcium-independent interactions. Conversely,the C2B domain of Syt IV possesses calcium binding properties,which promote both the homo-oligomerization of Syt IV and hetero-oligomerizationwith Syt I. Together, our results suggest that Syt IV may functionin calcium regulatedsecretion.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Materials

All chemicals and reagents were purchased from Sigma (St. Louis, MO) and Fisher Scientific (Houston, TX) unless stated otherwise.Recombinant Stxs 2-4 in pGEX-KG and anti-HPC-1 antibody were giftsfrom Mark Bennett (University of California, Berkeley, CA). Anti-dopamine- $beta$ -hydroxylase(D $beta$ H) antibody was a gift from Ruth Angeletti (Albert EinsteinCollege of Medicine, Bronx, NY). Plasmids encoding Syt I-VIII-GSTfusion proteins, encompassing the C2A and C2B domains, were agift from Dr. Tom Südhof (University of Texas Southwestern MedicalCenter, Dallas, TX), and a plasmid encoding a GST fusion proteinof the C2 domain of neuronal precursor cell-expressed developmentallydown-regulated 4 (Nedd4) was a gift from Dr. Daniela Rotin (TheHospital for Sick Children, Toronto, Ontario, Canada). $alpha$ -Latrotoxinwas purchased from Alomone Laboratories (Jerusalem, Israel). Theanti-hemagglutinin (HA) antibody 12CA5 was purchased from BoehringerMannheim (Indianapolis,IN).

Plasmid Construction and GST Fusion Proteins

For Stx binding and microinjection studies, plasmids encoding recombinant GST-Syt IV fusion proteins were constructed as follows:a cDNA fragment encoding the C2A domain of Syt IV (Syt IV C2A;amino acids 152-282) was generated by PCR using the followingprimers: 5'-GCG GAA TTC CGG AGA AGC TGG GCA CTC TC-3' and 5'-CCCAAG CTT TCA AGC ATT TCT CTT GAT G-3'. A mutant Syt IV C2A fragment(Syt IV C2A/AAAA) was generated using outside primers listed aboveand the following internal mutagenic primers: 5'-GAC AAT CTT ACCAGA GGC AGC AGC AGC AGT GAA AAC CAG AGT GCT GAG G-3' and 5'-CCTCAG CAC TCT GGT TTT CAC TGC TGC TGC TGC CTC TGG TAA GAT TGT C-3'.The PCR products were directionally cloned into the unique EcoRIand HindIII (New England Biolabs, Beverly, MA) sites of pGEX-KG(Guan and Dixon, 1991). The plasmid encoding a GST fusion proteinwith the C2A domain of Syt I (residues 140-267) has been describedelsewhere (Thomas and Elferink, 1998). Plasmids encoding epitope-taggedrat Stxs 2-4-GST fusion proteins were constructed in a derivativeof the expression vector pGEX-KG, in which oligonucleotides encodingthe HA epitope (MYPYDVPDYA) were directionally cloned into thepolylinker of pGEX-KG in frame with GST, generating pGEX-KG:HA.cDNAs encoding the cytoplasmic domains of Stxs 2-4 were insertedinto the EcoRI and HindIII sites of pGEX-KG:HA so that the HAepitope extended from the amino terminus of each Stx isoform.To create a GST fusion protein for Syt IV antibody affinity purification,a cDNA fragment encoding the C2A domain and adjacent spacer regionof Syt IV (amino acids 54-262) was generated by PCR from rat SytIV cDNA (Vician et al., 1995) using primers 5'-GCG GGA TCC GTGCAC GTG CTT AAA GGA G-3' and 5'-GCG GAA TTC CTC TTG ATG ATC TCTCTG G-3', and cloned into the EcoRI and HindIII sites of the expressionvector pGEX-2T (Pharmacia, Piscataway, NJ). For oligomerizationstudies, Syt I (amino acids 95-421) was amplified by reverse transcriptionPCR as previously described (Vician et al., 1995). Syt IV (aminoacids 54-425) was amplified by PCR from rat Syt IV cDNA (Vicianet al., 1995) using primers 5'-GCG GTC GAC GGT CAC GTG CTT AAAGGA G-3' and 5'-GCG GCG GCC GCC CAC AAG CTT ACA ATC GCG-3'. SytI and Syt IV PCR products were cloned into a modified versionof the in vitro translation vector pSP64 Poly(A). Plasmids encodinga GST-Syt I C2B fragment (amino acids 248-421) and a Nedd4 C2fragment (amino acids 78-218) have been previously described (Bennettet al., 1993b; Plant et al., 1997). Syt IV C2B (amino acids 258-425)domains were amplified by PCR from rat Syt IV cDNA using the primerpair 5'-GCG GTC GAC GCT CGT TCC TCT TTC AGG G-3' and 5'-GCG GCGGCC GCC CAC AAG CTT ACA ATC GCG-3'. These PCR products were clonedinto the expression vector pGEX-2T. After expression in Escherichiacoli DH5 $alpha$ or JM109, all fusion proteins were purified from bacteriallysates by glutathione-agarose chromatography (Guan and Dixon,1991).

Oligomerization of Syt I and IV

Syt I (amino acids 95-421) and Syt IV (amino acids 54-425) were in vitro translated using the TnT-coupled reticulocyte lysatesystem (Promega, Madison, WI) according to the manufacturer'sinstructions. Five microliters of in vitro-translated Syt I orSyt IV were incubated with 10 µg of GST-Syt IV C2A, GST-Syt IVC2B, GST-Syt I C2B, or GST alone in binding buffer (50 mM Tris-HCl,pH 8.0, 100 mM KCl, 1% nonfat dry-milk, and 0.05% Tween 20) supplementedwith 1 mM CaCl₂ or 2 mM EGTA for 1 h at 4°C. The samples werewashed three times in binding buffer, solubilized in 1% SDS, passedover a Chroma Spin-30 column (Clontech, Palo Alto, CA) previouslyequilibrated in PBS (137 mM NaCl, 2.68 mM KCl, 8.1 mM Na₂HPO₄,and 1.47 mM KH₂PO₄) to remove high concentrations of calcium,resuspended in SDS loading buffer, and fractionated by 12% SDS-PAGE.The gels were dried and exposed to autoradiographic filmovernight.

Antibody Preparation and Purification

A polyclonal antisera against a soluble recombinant Syt IV fragment encompassing residues 54-262 was generated as describedelsewhere (Ferguson et al., 1999). Anti-Syt IV antibodies wereaffinity purified using the soluble recombinant Syt IV fragmentcoupled to Affi-Gel 15 (Bio-Rad, Hercules, CA) according to themanufacturer's specifications. After elution from the Syt IV affinitycolumn, IgG fractions were pooled, supplemented with 150 mM NaCl,5 mg/ml BSA, and 25% glycerol, and anti-Syt IV antibody aliquotswere stored at $-$ 80°C.

Western Blot Analysis

For Western analysis, protein complexes were fractionated by SDS-PAGE and transferred to nitrocellulose, and the filters wereblocked overnight at 4°C in buffer A (150.4 mM NaCl, 10 mM Tris-Cl,pH 7.4, 0.1% Tween 20 [TBST], and 5% dry milk). After blocking,the filters were incubated in buffer A for 1 h at room temperaturewith primary antibodies: anti-Stx 1a mAb (HPC-1) diluted 1:10,000,anti-HA antibody (12CA5) diluted 1:3000, affinity-purified anti-SytIV antibody (1:1000), and anti-GST mAb (1:1000) (Zymed, San Francisco,CA). The blots were washed five times with TBST before incubationin buffer A with the appropriate HRP-conjugated 2° antibody diluted1:5000 for 1 h at room temperature. Blots were washed five timeswith TBST followed by a single wash in 0.1 M Tris-Cl, pH 8.6,for 10 min. Immunoreactivity was visualized by enhanced chemiluminescenceand autoradiography (Thomas and Elferink, 1998).

Stx Binding Studies

Binding studies using recombinant Syt and Stx isoforms were performed as described previously (Thomas and Elferink, 1998)with the following modifications. Briefly, 10 µg of GST-Syt Iand GST-Syt IV C2A fragments immobilized on glutathione agarosebeads were incubated with a 100 nM concentration of the indicatedStx isoform in the presence or absence of 3 mM CaCl₂. For studiesinvolving native Stx 1a, rat brain synaptosomes were preparedusing established conditions with the following changes (Chapmanet al., 1995). Rat brain detergent extracts were prepared by solubilizingsynaptosomes in buffer B (50 mM HEPES-HCl, pH 7.6, 100 mM NaCl,and 1% Triton X-100) at a detergent-to-protein ratio of 10:1,with 10 strokes in a tight fitting Teflon glass homogenizer, followedby mixing end-over-end for 2 h at 4°C. Eight hundred microgramsof the solubilized rat brain synaptosomes were incubated in thepresence or absence of 3 mM CaCl₂ with 15 µg of recombinant GST-SytI and IV C2A domains, GST only, or the Nedd4 C2 domain immobilizedon glutathione-agarose beads in buffer C (10 mM HEPES-NaOH, pH7.4, 0.15 M NaCl, 2 mM MgCl₂, 0.2% Triton X-100, and 0.5 mM EGTA).Protein complexes were recovered by brief centrifugation, washedfour times with buffer C, and fractionated by SDS-PAGE. Aftertransfer to nitrocellulose, blots were probed with HPC-1 as outlinedabove.

Cell Culture Conditions and Transfections

COS-7 cells were grown to 50% confluence in 60-mm tissue culture plates containing Dulbecco's modified Eagle's medium (DMEM)supplemented with 10% FBS. For LipofectAMINE transfections (LifeTechnologies, Grand Island, NY), full-length Syt IV was clonedinto the eukaryotic expression vector pcDNA3.1 zeo⁺ (Invitrogen, San Diego, CA) in both the forward and reverse orientations.After transfection, cells were harvested with 1% SDS in PBS andhomogenized in a Teflon glass homogenizer, and cell lysates wereanalyzed by Western analysis. For Western analysis of Syt IV expression,PC12 cells were first grown to 70% confluence in 60-mm tissueculture plates containing DMEM supplemented with 10% FBS and 5%heat-inactivated horse serum. To prepare differentiated cells,dishes were treated with 50 ng/ml nerve growth factor (NGF) inDMEM containing 2% FBS and 1% horse serum for 48 h. PC12 lysateswere prepared by homogenization, and 10 µg of each lysate werefractionated by SDS-PAGE and analyzed by Westernblotting.

PC12 Cell Microinjections and Confocal Microscopy

PC12 cell culture, microinjection, detection, and quantitation of D $beta$ H surface immunoreactivity were performed as previouslydescribed (Elferink et al., 1993; Thomas and Elferink, 1998).For microinjection studies, soluble recombinant C2A and C2 fragmentsfrom Syt IV and Nedd4, respectively, were expressed as GST fusionproteins, purified by affinity chromatography, isolated by thrombincleavage, and dialyzed in injection buffer as previously described(Thomas and Elferink, 1998). Before microinjection, soluble fragmentswere diluted to a working concentration of 0.75 µg/µl in microinjectionbuffer containing 3 mg/ml Texas Red-conjugated dextran 10,000. $alpha$ -Latrotoxin-evoked secretion was performed using a stimulationbuffer devoid of CaCl₂ and supplemented with 2.2 mM MgCl₂ and5 mM EGTA. Cells were stimulated at 37°C for 10 min with 9.6 µM $alpha$ -latrotoxin, fixed, and processed for D $beta$ H cell surface staining.For immunofluorescence confocal microscopy, NGF-differentiatedPC12 cells were depolarized in a stimulation buffer (10 mM HEPES,pH 7.4, 77 mM NaCl, 55 mM KCl, 2.2 mM CaCl₂, 0.33 M Na₂HPO₄, 0.44M KH₂PO₄, NaHCO₃, and 5.6 mM glucose) for 10 min to induce SytIV production, followed by a 2-h recovery in DMEM containing 2%NGF. Cells were then fixed and stained with affinity-purifiedanti-Syt IV (1:100) and anti-Syt I (1:100) antibodies, using previouslydescribed conditions (Elferink et al., 1993; Thomas and Elferink,1998). Immunofluorescence confocal microscopy was performed usinga Zeiss 310 laser scanning microscope (Wayne State University,School ofMedicine).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

The Specificity of Syt-Stx Interactions Differs for Syt I and Syt IV

Syt I has been postulated to function in exocytosis through a mechanism involving interactions with the plasma membrane proteinStx 1a through the C2A domain (Südhof and Rizo, 1996). To determinewhether Syt IV is also capable of interacting with native Stx1a, recombinant Syt IV C2A was immobilized on glutathione-agaroseand incubated with detergent-solubilized rat brain synaptosomesin the absence and presence of calcium. Recombinant protein-synaptosomecomplexes were detected by Western blot analysis using the anti-Stx1a antibody HPC-1. As shown in Figure 1A, the Syt IV C2A domainbinds Stx 1a in the absence and presence of calcium. In contrast,the Syt I C2A domain bound Stx 1a in a calcium-dependent manner,consistent with previous studies (Chapman et al., 1995; Li etal., 1995). As expected, GST alone fails to bind Stx 1a. To confirmthe specificity of the Syt IV-Stx 1a interactions, we examinedthe Stx binding properties of the C2 domain from Nedd4. Nedd4is a ubiquitin protein ligase, which interacts directly with Na⁺ channels in apical membranes of epithelial cells. The C2 domainof Nedd4 binds phospholipids and membranes in a calcium-dependentmanner and is involved in localizing the protein to the apicalmembranes in epithelial cells (Staub et al., 1996; Plant et al.,1997). Given the calcium binding properties of the Nedd4 C2 domain,we examined its Stx 1a binding properties. No Stx 1a binding wasobserved with the Nedd4 C2 domain in the presence or absence ofcalcium (Figure 1A) using a wide concentration range of nativeStx 1a (our unpublished results). Together, these data indicatethat the C2A domain of Syt IV interacts specifically with Stx1a, and that this interaction is not enhanced by calcium.

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Figure 1. Distinct Syt-Stx interactions exist for Syt I and Syt IV isoforms. (A) The indicated recombinant GST fusion proteins were immobilized on glutathione-agarose and incubated with 800 µg of rat brain synaptosomes in the absence ( $-$ ) or presence (+) of 3 mM calcium. Protein complexes were isolated, fractionated by SDS-PAGE, and examined by Western analysis. Stx 1a binding was detected with HPC-1, followed by enhanced chemiluminescence. One hundred nanograms of soluble Stx 1a (Con) were used as a Western control. (B) Ten micrograms of immobilized recombinant Syt I and IV C2A domains were incubated with 100 nM soluble recombinant Stx 1a (amino acids 4-266) or HA-tagged Stxs 2 (amino acids 4-264), 3 (amino acids 4-264), or 4 (amino acids 1-268), and the protein complexes were examined by Western analysis. Stx 1a binding was detected with the anti-Stx 1a antibody HPC-1. Binding of HA-tagged Stxs 2-4 was detected with the anti-HA antibody 12CA5. No binding was detected with GST alone (Con).

The identification of multiple Syt and Stx isoforms in mammals suggests that isoform-specific Syt-Stx interactions may conferspecificity to regulated secretion. To examine the specificityof Syt-Stx interactions, we compared the binding of recombinantStxs 1a, 2, 3, and 4 with the C2A domains of Syts I and IV. TheC2A domains of Syts I and IV were expressed as GST fusion proteins,immobilized on glutathione-agarose, and incubated with solublerecombinant Stxs. For detection purposes, Stxs 2-4 were HA taggedon their amino termini (Bennett et al., 1993a). Binding was detectedby Western blot analysis using anti-HPC-1 (Stx 1a) or anti-HAepitope (Stxs 2-4) (Figure 1B). In the presence of calcium, strongbinding to the C2A domain of Syt I is observed with Stx 1a andStx 4. In contrast, lower levels of calcium-dependent bindingare observed with Stx 2 and Stx 3. The C2A domain of Syt IV bindsto each of the four Stxs tested; however, the strongest bindingis observed with Stx 1a and Stx 2. In contrast to the calcium-dependentinteractions of the Syt I C2A domain with the recombinant Stxproteins, Syt IV-Stx interactions are calcium independent, consistentwith the non-calcium binding nature of the Syt IV C2A domain.No binding was observed with GST alone (Con) or with the recombinantNedd4 C2 fragment (our unpublished results). These data indicatethat both the specificity and calcium dependency of Syt-Stx interactionsdiffer significantly between the C2A domains of Syt I and SytIV.

The C2B Domain of Syt IV Mediates Homo- and Hetero-Oligomerization

Biochemical and genetic studies suggest that Syt I acts as a multimeric complex to regulate neurotransmitter release (Littletonet al., 1994; Chapman et al., 1996). In detergent-solubilizedrat brain extracts, native Syt I exists as an oligomeric structure,the basic unit of which is a homodimer (Geppert et al., 1994;Chapman et al., 1996). Dimerization of Syt I occurs through theC2B domain and is enhanced by calcium (Chapman et al., 1996).In Drosophila, mutations in the C2B domain of Syt I lower thecalcium responsiveness of the dimeric complex, suggesting thatSyt I functions as a homo-oligomer during synaptic transmission(Littleton et al., 1994). Comparison of the rat Syt I and SytIV amino acid sequences suggests that, akin to the Syt I C2 domains,the C2B domain of Syt IV may also form a C2 key, which is capableof binding calcium. To examine the calcium binding propertiesof the Syt IV C2B domain, we compared the oligomerization propertiesof Syt IV with Syt I. Immobilized recombinant C2A and C2B SytIV fragments were incubated with soluble, in vitro-translated,radiolabeled Syt I or Syt IV. Binding was detected by autoradiography(Figure 2). GST alone or the C2A domain of Syt IV shows essentiallyno binding (Figure 2A). In contrast, strong Syt I and Syt IV bindingis observed with the C2B domain of Syt IV. These results indicatethat the C2B domain of Syt IV is capable of both homo- and hetero-oligomerizationwith Syt I. To determine the calcium dependence of these interactions,these studies were performed in the presence or absence of calcium(Figure 2B). In the presence of calcium, both immobilized recombinantSyt I and Syt IV C2B domains interact with in vitro-translatedSyt I and Syt IV; both Syt I C2B and Syt IV C2B form homo- andhetero-oligomers. Furthermore, calcium-dependent homo- and hetero-oligomerinteractions were detected with an in vitro-translated, radiolabeledSyt IV C2B fragment and not a Syt IV C2A fragment (our unpublishedresults). Together, these data indicate that the C2B domain ofSyt IV exhibits calcium binding properties, which promote boththe formation of Syt IV homo-oligomers as well as the formationof hetero-oligomers with the C2B domain of Syt I.

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Figure 2. Calcium-dependent, C2B domain-mediated homo- and hetero-oligomerization of Syt I and Syt IV. (A) Five microliters of in vitro-translated, [³⁵S]methionine-labeled cytoplasmic domain of Syt I and Syt IV were incubated with 10 µg of immobilized GST-Syt IV C2A, GST-Syt IV C2B, or GST alone in the presence of calcium. Protein complexes were isolated and analyzed by SDS-PAGE. Gels were dried and exposed to autoradiographic film overnight. In vitro-translated, [³⁵S]methionine-labeled Syt I and Syt IV products are shown in the left two lanes (Input). (B) Five microliters of in vitro-translated, [³⁵S]methionine-labeled cytoplasmic domain of Syt I and Syt IV were incubated with 10 µg of immobilized GST-Syt I C2B or GST-Syt IV C2B in the absence ( $-$ ) or presence (+) of calcium. Protein complexes were analyzed as described above.

Syt IV and Syt I Colocalize in the Tips of Neurites in NGF-differentiated PC12 Cells

We have recently used biochemical approaches to demonstrate that Syt IV colocalizes with Syt I to the large dense core vesicles(LDCVs) and synaptic-like microvesicles (SLMVs) of neuroendocrinePC12 cells (Ferguson et al., 1999). To examine the subcellularlocalization of these Syt isoforms in vivo, we prepared affinity-purifiedanti-Syt IV antibodies. Before staining PC12 cells, we examinedthe specificity of the affinity-purified antibody for Syt IV byWestern blot analysis against recombinant Syt I-VIII isoformsexpressed as GST fusion proteins. As shown in Figure 3A (top panel),the anti-Syt IV antibody reacts only with recombinant Syt IV andnot with the other Syt isoforms tested. Additionally, Syt IV immunoreactivityis blocked by preincubating the antibody with soluble Syt IV protein(Figure 3A, middle panel). Probing a second filter with anti-GSTantibody confirms the presence of all GST-Syt proteins (Figure3A, bottom panel). To further confirm the specificity of the affinity-purifiedantibody, we transiently expressed the Syt IV cDNA in COS-7 cells.Western analysis of COS-7 cell lysates detects an immunoreactive46-kDa product present in cells transfected with Syt IV (consistentwith its predicted molecular mass) but not in cells transfectedwith a plasmid containing the Syt IV cDNA in the reverse orientation(Figure 3B, top panel) or parental vector only (our unpublishedresults). Furthermore, preincubating the antibody with recombinantSyt IV C2A domain abolishes Syt IV immunoreactivity (Figure 3B,bottom panel). We next examined the ability of our affinity-purifiedantisera to detect Syt IV in NGF-differentiated and undifferentiatedPC12 cells (Figure 3C, top panel). Although Syt IV immunoreactivityis not detected in undifferentiated PC12 cells, low levels aredetected in cells differentiated with NGF for 48 h. In a recentstudy, we demonstrated that Syt IV is a relatively labile proteinin PC12 cells, with a half-life of 2 h (Ferguson et al., 1999).However, expression of Syt IV in PC12 cells can be induced bychemical depolarization. Therefore, we examined the effect ofchemical depolarization on expression of the Syt IV protein inNGF-differentiated PC12 cells. As shown in Figure 3C, chemicaldepolarization of NGF-differentiated PC12 cells with 55 mM KClfor 10 min induces significant expression of Syt IV protein; SytIV immunoreactivity is blocked by preincubating the antibody withsoluble recombinant Syt IV protein.

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Figure 3. Affinity-purified anti-Syt IV antibody does not react with other Syt isoforms. (A) Five hundred nanograms of each soluble Syt I-VIII-GST fusion protein were subjected to SDS-PAGE and analyzed by Western blotting. Filters were probed with the affinity-purified Syt IV antibody in the absence (A, top panel) or presence (A, middle panel) of 500 µg of soluble Syt IV. The presence of GST-Syt fusion proteins was confirmed by probing a filter with an anti-GST mAb (A, bottom panel). (B) Cell lysates from COS-7 cells transiently transfected with full-length Syt IV cDNA cloned into the eukaryotic expression vector pcDNA3.1 zeo⁺, in the forward (+) and reverse ( $-$ ) orientations, were examined for expression of Syt IV by Western analysis. Filters were probed in the absence (B, top panel) or presence (B, bottom panel) of 500 µg of soluble Syt IV. (C) PC12 cells treated as indicated were examined for Syt IV expression by Western analysis. Filters were probed with anti-Syt IV antibody in the absence (C, top panel) or presence (C, bottom panel) of 500 µg of soluble Syt IV.

To compare the subcellular localization of Syt IV with Syt I in vivo, we performed double immunofluorescent labeling and confocalmicroscopy on NGF-differentiated PC12 cells. Although Syt IV isexpressed at low levels in PC12 cells (Ferguson et al., 1999),native Syt IV is not readily detected in the tips of these cellsby immunofluorescent microscopy (our unpublished results). Chemicaldepolarization induces the rapid synthesis of Syt IV in the cellbody, reaching maximal levels in the tips within 1-2 h after depolarization(our unpublished results). Therefore, we performed our subcellularlocalization studies on depolarized PC12 cells. As shown in Figure4, Syt I and Syt IV immunoreactivities concentrate in the tipsof the neurites (compare A-C). Furthermore, Syt IV immunoreactivityin the tips of extending neurites overlaps with Syt I (Figure4D), consistent with the distribution of LDCVs and SLMVs in PC12cells. Coupled with our recent studies demonstrating that SytI and Syt IV coprecipitate from a PC12 cell fraction enrichedin LDCVs and SLMVs (Ferguson et al., 1999), these data indicatethe vesicular colocalization of these Syt isoforms.

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Figure 4. Syt I and Syt IV colocalize to the tips of neurites in PC12 cells in vivo. NGF-differentiated PC12 cells were K⁺ depolarized and 2 h after depolarization analyzed by double immunofluorescence confocal microscopy. A phase-contrast image of representative cells is shown in A. Cells were costained for endogenous Syt I (B) and Syt IV (C) and detected using secondary antibodies coupled to RITC and FITC, respectively. Representative areas of overlap between Syt I and Syt IV in these panels and the merged image (D) are indicated by the arrows in the tips of PC12 cells. Bar, 20 µm.

The C2A Domain of Syt IV Inhibits Calcium-regulated Secretion from Microinjected PC12 Cells

Although genetic and microinjection studies support a role for Syt I in calcium-regulated secretion, the contribution of otherSyt isoforms to this process remains to be determined. We previouslydemonstrated that a microinjected recombinant Syt I fragment encompassingthe C2A domain inhibits calcium-regulated secretion from PC12cells (Elferink et al., 1993). Interestingly, the inhibitory effecton secretion by recombinant Syt I C2A fragments occurs independentlyof calcium-mediated interactions with Stx 1a and is conferredby a novel polybasic motif unique to the C2A domains of severalSyt isoforms (Thomas and Elferink, 1998). Given the enriched expressionof Syt IV in PC12 cells after depolarization, Syt IV's vesicularcolocalization with Syt I, and the presence of a C2A polybasicmotif in Syt IV, the Syt IV C2A domain may inhibit neurotransmitterrelease when injected into PC12 cells. Additionally, we preparedand assayed a new recombinant Syt IV C2A fragment in which thepolybasic motif KKHK at residues 202-205 was replaced with alanines(Syt IV C2A/AAAA). We examined the functional consequences ofthese mutations on 1) Stx 1a interactions and 2) calcium-regulatedsecretion when microinjected into PC12 cells. For Stx 1a bindingstudies, immobilized GST-Syt IV C2A wild-type and mutant fragmentswere incubated with detergent-solubilized rat brain synaptosomesin the presence or absence of calcium. Binding of native Stx 1afrom the synaptosome extract was determined by Western blot analysis(Figure 5A). Recombinant wild-type and mutant Syt IV C2A fragmentsboth bind native Stx 1a; however, binding is calcium independent,consistent with the non-calcium binding properties of the SytIV C2A domain. As expected, calcium stimulates the binding ofnative Stx 1a to the recombinant Syt I C2A fragment, whereas nobinding is observed with GST only (Figure 5A) or Nedd4 (our unpublishedresults), demonstrating the specificity of these Syt IV-Stx 1ainteractions. These data suggest that like the wild-type recombinantSyt IV C2A fragment, the mutant Syt IV C2A domain is a well-foldedprotein.

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Figure 5. The polybasic motif in the C2A domain of Syt IV functions in calcium-regulated secretion. (A) The indicated recombinant GST fusion proteins were immobilized on glutathione-agarose and incubated with 800 µg of rat brain synaptosomes in the presence (+) or absence ( $-$ ) of 3 mM calcium. Protein complexes were isolated, fractionated by SDS-PAGE, and examined by Western analysis. Stx 1a binding was detected with HPC-1, followed by enhanced chemiluminescence. One hundred nanograms of soluble Stx 1a (Con) were used as a Western control. (B) NGF-differentiated PC12 cells were coinjected with Texas Red-conjugated dextran and the indicated soluble recombinant Syt IV or Nedd4 fragments. Control cells were injected with Texas Red-conjugated dextran only (Texas Red) or coinjected with a control GST extract (GST). One hour after microinjection, the cells were K⁺ depolarized in the presence of calcium, and D $beta$ H surface immunoreactivity was detected with a fluorescein-labeled secondary antibody. The numbers of individual fluorescent particles were counted, regardless of their size, and are presented as a percent of the total number of cells injected. Data are shown as the mean of two independent experiments ± SD with the total number of injected cells (n). Significant differences (p $<=$ 0.01, $chi$ ² analysis) between experimental and control treatments are indicated with an asterisk.

We previously demonstrated that depolarization of PC12 cells promotes the fusion of LDCVs with the plasma membrane, exposingan intravesicular form of the enzyme D $beta$ H on the cell surface thatcan be quantitated by immunofluorescent microscopy (Bennett etal., 1993a; Elferink et al., 1993; Thomas and Elferink, 1998).Using this in vivo secretion assay, we compared the effects ofmicroinjecting wild-type and mutant Syt IV C2A fragments on calcium-regulatedsecretion from NGF-differentiated PC12 cells (Figure 5B). Afterdepolarization, high levels of D $beta$ H surface staining ( $>=$ 41 fluorescentparticles) is observed on 60-65% of control cells injected withTexas Red-conjugated dextran only or coinjected with a controlGST extract or the soluble C2 domain of Nedd4. In contrast, microinjectionof the wild-type Syt IV C2A domain produces a 50% reduction inmaximal calcium-regulated secretion from PC12 cells ( $>=$ 41 fluorescentparticles). Microinjection of the soluble recombinant Syt IV C2Afragment containing mutations in the polybasic motif (Syt IV C2A/AAAA)results in a 20% reduction in maximal calcium-regulated secretion.The differences between the relative blocking effects of the wild-typeand mutant Syt IV C2A domains are statistically significant (p< 0.0001, $chi$ ² analysis), suggesting that the polybasic motif is important forthe inhibitory effect of the microinjected Syt IV C2A domains.Therefore, these data indicate that, akin to studies with SytI, the C2A domain of Syt IV blocks secretion when microinjectedinto PC12 cells. Furthermore, the blocking effect of the Syt IVC2A domain on calcium-regulated secretion is mediated, at leastpartially, through the polybasicmotif.

To ensure that the injected recombinant Syt IV C2A fragment interferes with the normal calcium-mediated cellular secretorymachinery, we performed a series of microinjection experimentsusing $alpha$ -latrotoxin. $alpha$ -Latrotoxin is a potent neurotoxin from blackwidow spider venom, which is proposed to bypass the calcium requirementfor vesicle fusion and trigger neurotransmitter release from neuraland neuroendocrine cells (Rosenthal et al., 1990). We hypothesizedthat, if the recombinant Syt IV C2A fragment impaired the functionalsecretory machinery, then $alpha$ -latrotoxin would overcome the inhibitoryeffect of this fragment in our in vivo secretion assay. In theabsence of calcium and $alpha$ -latrotoxin, minimal D $beta$ H cell surfacestaining is observed on 90% of control cells (0-20 fluorescentparticles) injected with control GST extracts (our unpublishedresults), Texas Red alone, or the wild-type Syt IV C2A fragment(Syt IV C2A) (Figure 6). $alpha$ -Latrotoxin treatment of cells injectedwith either Texas Red alone or Syt IV C2A triggers calcium-independentsecretion, as indicated by an increase to 70% of cells with maximalD $beta$ H cell surface staining ( $>=$ 41 fluorescent particles). Together,these data indicate that microinjection of a recombinant Syt IVC2A fragment specifically impairs neurotransmitter release fromneuroendocrine PC12 cells by interfering with the endogenous regulatedsecretory machinery.

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Figure 6. $alpha$ -Latrotoxin reverses the inhibitory effect of the Syt IV C2A domain on calcium-regulated secretion from PC12 cells. NGF-differentiated PC12 cells were injected with Texas Red-conjugated dextran alone (Texas Red) or a soluble recombinant fragment encompassing the C2A domain of Syt IV (Syt IV C2A). One hour after injection, cells were K⁺ depolarized in a calcium-free buffer supplemented with 2.2 mM MgCl₂, 5 mM EGTA, and $alpha$ -latrotoxin at a final concentration of 9.6 µM. D $beta$ H surface immunoreactivity was quantified and is presented as described in the legend to Figure 5. Data are shown as the mean of two independent experiments ± SD with the total number of injected cells (n). Significant differences (p $<=$ 0.01, $chi$ ² analysis) between experimental and control treatments are indicated with an asterisk.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Syts are a family of vesicle proteins that are proposed to function as regulators of exocytosis (O'Connor et al., 1994; Südhofand Rizo, 1996). The high level of conservation between the C2domains of 11 isoforms characterized to date suggests an importantrole for these domains in Syt function. Syt IV is the productof an immediate early gene whose expression is up-regulated inrat brain during seizure induction and in response to depolarizationin PC12 cells (Vician et al., 1995). We recently demonstratedthat Syt IV coprecipitates with Syt I in fractions enriched inSLMVs and LDCVs of neuroendocrine PC12 cells (Ferguson et al.,1999). Furthermore, Syt IV is a labile protein with a half-lifeof ~2 h in PC12 cells. Therefore, Syt IV may have a unique rolein regulating neurotransmitter release from neurons and neuroendocrinecells. In this paper, we extend these findings by examining thebiochemical and functional properties of the C2 domains of SytIV. Although the C2A domain of Syt IV binds Stxs 1a, 2, 3, and4, binding is calcium independent, consistent with the inabilityof the Syt IV C2A domain to bind calcium (Li et al., 1995). Inneuroendocrine PC12 cells, Syt IV colocalizes with Syt I in thetips of the neurites. Furthermore, calcium-independent interactionsmediated through the C2A domain of Syt IV are functionally importantfor neurotransmitter release from PC12cells.

Unlike the C2A domain, the C2B domain of Syt IV contains calcium binding properties that enable the assembly of both Syt IVhomo- and hetero-oligomers with Syt I, consistent with the vesicularcolocalization of these Syt isoforms. Consistent with our studies,we have observed calcium-dependent binding of recombinant GST-SytIV C2B domain with native Syt I overexpressed in COS-7 cells (Thomasand Elferink, unpublished observation). While this report wasunder review, a separate study demonstrated calcium-dependenthetero-oligomerization between recombinant Syt IV and native SytI derived from detergent-solubilized brain extracts (Chapman etal., 1998), confirming our observations. Together these studiesdemonstrate that the C2B domain of Syt IV is capable of calcium-dependentoligomerization.

During synaptic transmission, calcium influx into the nerve terminal promotes the fusion of docked vesicles with the presynapticplasma membrane (DeBello et al., 1993; Südhof and Rizo, 1996).Biochemical and genetic studies reveal that the C2 domains ofSyt I contain distinct calcium binding properties, which may functionto sense calcium influx and trigger vesicle fusion with the plasmamembrane (Davletov and Südhof, 1993; Broadie et al., 1994; Geppertet al., 1994; Littleton et al., 1994; Li et al., 1995; Damer andCreutz, 1996; Sugita et al., 1996). The dimerization of Syt Ivia its C2B domain occurs at low calcium concentrations (3-10µM), whereas calcium concentrations comparable with those triggeringexocytosis (20-200 µM) promote the binding of Syt I dimers toStx 1a (Chapman et al., 1996). The ability of increasing calciumlevels to sequentially trigger Syt I dimerization followed byStx 1a binding may enable Syt I to both sense calcium and triggerneurotransmitter release at sites of calcium influx (Heidelbergeret al., 1994; Chapman et al., 1996). Consistent with this model,discrete mutations in the Drosophila Syt I C2B domain abolishthe formation of Syt I dimers, thereby decreasing the calciumresponsiveness of the secretory machinery (Littleton et al., 1994).Furthermore, half-maximal binding of Stx 1a to the C2A domainof Syt I occurs at $>=$ 200 µM calcium, consistent with the levelsrequired for vesicle fusion at synaptic sites (Heidelberger etal., 1994; Li et al., 1995). Therefore, our observations thatdifferent combinatorial interactions exist between Syt and Stxisoforms, coupled with calcium-stimulated hetero-oligomerizationof Syt isoforms, suggest that the secretory machinery containsa vast repertoire of biochemical properties for sensing calciumand regulating neurotransmitter releaseaccordingly.

The tight coupling between a rise in intracellular calcium and the subsequent fusion event is a unique feature of neurotransmitterrelease. The calcium-dependent properties of the Syt I C2A domainare consistent with Syt I's proposed role as a low-affinity calciumsensor for fast calcium-dependent exocytosis (Brose et al., 1992;Davletov and Südhof, 1993). The C2A domain of Syt IV containsa serine at residue 244, which prevents calcium binding to theC2A metal coordination site. Our functional studies on the SytIV C2A domain suggest that this non-calcium binding domain mightalso function in calcium-regulated secretion from PC12 cells.In light of its non-calcium binding properties, how can Syt IVmodulate neurotransmitter release in response to calcium? It istempting to speculate that Syt IV may alter the fusogenic propertiesof synaptic and secretory vesicles by interacting directly withbona fide components of the calcium-sensing machinery. Therefore,the calcium-stimulated hetero-oligomerization of Syt I and SytIV may provide the regulated secretory machinery with a mechanismto temporally regulate Syt I-mediated vesicle fusion. The inducibilityand short half-life of Syt IV may offer an additional level ofcontrol on the secretory machinery. The formation of Syt IV-SytI hetero-oligomers is contingent on Syt IV levels, which are mediatedby depolarization-induced changes in Syt IV gene expression. Therefore,neurotransmitter release may be modulated directly by rapid signalingevents involving calcium and indirectly by calcium- and cAMP-mediatedregulation of Syt IV availability for incorporation into the cellularsecretorymachinery.

Microinjection of non-calcium binding recombinant Syt IV C2A fragments inhibits calcium-regulated secretion from PC12 cells.The ability of $alpha$ -latrotoxin to reverse the inhibitory effect ofinjected Syt IV C2A fragments suggests that these fragments functionto specifically perturb the regulated cellular secretory machinery.Mutational analysis of the Syt IV C2A domain reveals that thepolybasic motif KKHK confers an inhibitory effect of these fragmentson Syt function in vivo. The presence of a polybasic motif inthe C2A domains of eight Syt isoforms supports the hypothesisthat calcium-independent events mediated through this motif areimportant for neurotransmitter release in general (Thomas andElferink, 1998). Nedd4 fragments, fully capable of binding phospholipidsin a calcium-dependent manner, lack the polybasic motif and failto inhibit calcium-regulated secretion from PC12 cells. Theseresults suggest that the inhibitory effect observed with Syt Iand Syt IV C2A fragments is not due to nonspecific interactionsbut rather an interaction with a common effector molecule. Insupport of our hypothesis, microinjection of a 15-residue peptidecontaining the Syt I polybasic motif reversibly inhibits neurotransmitterrelease from giant squid presynaptic terminals (Bommert et al.,1993). Similarly, mutation of the C2A polybasic motif in recombinantSyt I C2A fragments reverses their inhibitory effect on neurotransmitterrelease from microinjected PC12 cells (Thomas and Elferink, 1998),independent of the calcium binding properties of the Syt I C2Afragments. Whether these calcium-independent events function directlyto modulate vesicle fusion or regulate specific sequential stepsleading to neurotransmitter release remains to be determined.Thus, given the unusual binding properties of its C2 domains andits inducibility after neuronal excitation, Syt IV may play aunique role in modulating neurotransmitterrelease.

	ACKNOWLEDGMENTS

We thank Dina M. Francescutti-Verbeem for technical assistance and members of the Elferink and Herschman laboratories forhelpful discussion. This work was supported by grants GM-53189(to L.A.E.) and NS-28660 (to H.R.H.) and training grant NS-07107(to G.D.F) from the National Institutes ofHealth.

	FOOTNOTES

These authors contributed equally to thiswork.

^¶ Corresponding author. E-mail address: laelferi{at}sun.science.wayne.edu.

ABBREVIATIONS

Abbreviations used: D $beta$ H, dopamine- $beta$ -hydroxylase; DMEM, Dulbecco's modified Eagle's medium; HA, hemagglutinin; LDCV, large dense core vesicle; Nedd4, neuronal precursor cell-expressed developmentally down-regulated 4; NGF, nerve growth factor; SLMV, synaptic-like microvesicle; Stx, syntaxin; Syt, synaptotagmin.

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				R. D. Burgoyne and A. Morgan Secretory Granule Exocytosis Physiol Rev, April 1, 2003; 83(2): 581 - 632. [Abstract] [Full Text] [PDF]

				R. Cohen, L. A. Elferink, and D. Atlas The C2A Domain of Synaptotagmin Alters the Kinetics of Voltage-gated Ca2+ Channels Cav1.2 (Lc-type) and Cav2.3 (R-type) J. Biol. Chem., March 7, 2003; 278(11): 9258 - 9266. [Abstract] [Full Text] [PDF]

				M. Fukuda, E. Kanno, Y. Ogata, C. Saegusa, T. Kim, Y. P. Loh, and A. Yamamoto Nerve Growth Factor-dependent Sorting of Synaptotagmin IV Protein to Mature Dense-core Vesicles That Undergo Calcium-dependent Exocytosis in PC12 Cells J. Biol. Chem., January 24, 2003; 278(5): 3220 - 3226. [Abstract] [Full Text] [PDF]

				C. Saegusa, M. Fukuda, and K. Mikoshiba Synaptotagmin V Is Targeted to Dense-core Vesicles That Undergo Calcium-dependent Exocytosis in PC12 Cells J. Biol. Chem., June 28, 2002; 277(27): 24499 - 24505. [Abstract] [Full Text] [PDF]

				T. C. Sudhof Synaptotagmins: Why So Many? J. Biol. Chem., March 1, 2002; 277(10): 7629 - 7632. [Full Text] [PDF]

				A Gut, C. Kiraly, M Fukuda, K Mikoshiba, C. Wollheim, and J Lang Expression and localisation of synaptotagmin isoforms in endocrine (&bgr;)-cells: their function in insulin exocytosis J. Cell Sci., January 5, 2001; 114(9): 1709 - 1716. [Abstract] [PDF]

				B. A. Eaton, M. Haugwitz, D. Lau, and H.-P. H. Moore Biogenesis of Regulated Exocytotic Carriers in Neuroendocrine Cells J. Neurosci., October 1, 2000; 20(19): 7334 - 7344. [Abstract] [Full Text] [PDF]

				I. Martinez, S. Chakrabarti, T. Hellevik, J. Morehead, K. Fowler, and N. W. Andrews Synaptotagmin VII Regulates Ca2+-dependent Exocytosis of Lysosomes in Fibroblasts J. Cell Biol., March 20, 2000; 148(6): 1141 - 1150. [Abstract] [Full Text] [PDF]

				G. D. Ferguson, X.-N. Chen, J. R. Korenberg, and H. R. Herschman The Human Synaptotagmin IV Gene Defines an Evolutionary Break Point between Syntenic Mouse and Human Chromosome Regions but Retains Ligand Inducibility and Tissue Specificity J. Biol. Chem., November 17, 2000; 275(47): 36920 - 36926. [Abstract] [Full Text] [PDF]

				G. D. Ferguson, S. G. Anagnostaras, A. J. Silva, and H. R. Herschman Deficits in memory and motor performance in synaptotagmin IV mutant mice PNAS, May 9, 2000; 97(10): 5598 - 5603. [Abstract] [Full Text] [PDF]