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The Journal of Neuroscience, July 1, 2000, 20(13):4904-4911
Immunoisolation of GABA-Specific Synaptic Vesicles Defines a Functionally Distinct Subset of Synaptic Vesicles
Shigeo Takamori, Dietmar Riedel, and Reinhard Jahn Department of Neurobiology, Max-Planck-Institute for Biophysical Chemistry, D-37077 Göttingen, Germany
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Synaptic vesicles from mammalian brain are among the best characterized trafficking organelles. However, so far it has not been possible to characterize vesicle subpopulations that are specific for a given neurotransmitter. Taking advantage of the recent molecular characterization of vesicular neurotransmitter transporters, we have used an antibody specific for the vesicular GABA transporter (VGAT) to isolate GABA-specific synaptic vesicles. The isolated vesicles are of exceptional purity as judged by electron microscopy. Immunoblotting revealed that isolated vesicles contain most of the major synaptic vesicle proteins in addition to VGAT and are devoid of vesicular monoamine and acetylcholine transporters. The vesicles are 10-fold enriched in GABA uptake activity when compared with the starting vesicle fraction. Furthermore, glutamate uptake activity and glutamate-induced but not chloride-induced acidification are selectively lost during immunoisolation. We conclude that the population of GABA-containing synaptic vesicles is separable and distinct from vesicle populations transporting other neurotransmitters.
Key words: GABA uptake; glutamate uptake; neurotransmitter phenotype; vesicular neurotransmitter uptake; synaptic vesicle proteins; vesicular GABA transporter
INTRODUCTION
Synaptic vesicles, the presynaptic storage compartment for neurotransmitters, are presently the best characterized trafficking organelles. More than a dozen membrane proteins that perform specific functions in membrane trafficking are known to be specific to synaptic vesicles (Südhof, 1995
). These include the synaptobrevins/vesicle-associated membrane proteins (VAMPs) that mediate membrane fusion, the synaptotagmins that are involved in transmitting the Ca2+ signal to the exocytotic apparatus, synaptophysin, synaptogyrin, and secretory carrier membrane proteins whose functions are not yet known, small GTPases of the rab family that are probably involved in vesicle attachment, and the vacuolar H+-ATPase, which is responsible for intravesicular acidification. Most of these proteins are represented by multiple isoforms that are differentially expressed within the CNS and peripheral nervous system. From numerous immunocytochemical and electron microscopic studies, it can be concluded that at least one member of each protein family is present on every synaptic vesicle within the nervous system (Südhof, 1995
Despite the similarities in their overall protein composition, synaptic vesicles are distinguished by their neurotransmitter content. The neurotransmitter phenotype is defined by at least three components: the biosynthetic enzyme(s) that generate high concentrations of the transmitter within the presynaptic cytosol, the vesicular carriers specific for the transmitter that are driven by a proton electrochemical potential, and the reuptake systems in the plasma membrane that use the energy provided primarily by the transmembrane sodium gradients (Maycox et al., 1990
In recent years, several of the vesicular neurotransmitter transporters have been characterized at the molecular level (Liu and Edwards, 1997
Presently, it is not known whether vesicles specific for a given neurotransmitter phenotype contain additional specific components. For instance, it has long been known that the shape of synaptic vesicles in inhibitory synapses is different from that of vesicles in excitatory synapses. This difference is evident under certain fixation conditions (Gray, 1959
In the present study, we report the immunoisolation of GABAergic synaptic vesicles from rat brain using an antibody specific for the vesicular GABA transporter. The resulting vesicle fraction is of exceptional purity, ~10-fold enriched in vesicular GABA transporter but virtually devoid of other vesicular transporters, and functionally active. Our findings document for the first time that GABAergic vesicles are indeed equipped only with the molecular machinery required for GABA uptake and thus are finally responsible for defining the GABAergic phenotype of a neuron.
MATERIALS AND METHODS
Plasmids and antibodies. The following peptides, all based on the predicted sequence of rat VGAT (McIntire et al., 1997
Antibodies specific for VMAT2 were generated using recombinant protein fragments as antigen and will be described in detail elsewhere (Hoeltje et al., 2000
For transfection experiments, first strand cDNA was generated from rat brain total RNA with SuperScript RT-PCR system and oligo-dT primer (Life Technologies, Gaithersburg, MD). The full-length of rat VGAT was amplified by PCR from the rat brain first strand cDNA using Pfu DNA polymerase and the primers 5'-CGGGATCCATAATGGCCACCCTGCTCCGCAG-3' and 5'-CGTCTAGAGTCCTCTGCGTTGGTTCGGT-3'. The amplified fragment was digested by BamHI and XbaI and was purified by gel electrophoresis. The fragment was subcloned into pcDNA3.1 (Invitrogen, San Diego, CA) at BamHI/XbaI sites, and the construct was then sequenced to confirm the identity with the published sequence (McIntire et al., 1997
Cell transfection. tsA201 cells, which are HEK293 cells that are transformed to express an SV40 T antigen, were kindly provided by Richard Horn (Thomas Jefferson University, Philadelphia, PA). They were cultured in high glucose DMEM, supplemented with 10% fetal bovine serum, 100 IU/ml penicillin, and 100 µg/ml streptomycin. Ten micrograms of either VGAT-pcDNA or pcDNA without insert were used for transfecting cells at 50% confluence on a 10 cm dish by means of the calcium-phosphate method. Twenty-four hours after transfection, the cells were washed twice with ice-cold PBS and then collected. The resulting cell pellet was solubilized in 1% Triton X-100 containing PBS, and insoluble material was pelleted by 10,000 × g for 15 min. The supernatant was used for immunoblot analysis.
Immunofluorescence. Adult female Sprague Dawley rats were anesthetized, perfused, and post-fixed as described by Mugnaini and Dahl (1983)
Electron microscopy. The procedure was adapted from De Camilli et al. (1983)
For immunogold labeling, purified synaptic vesicles were adsorbed to glow discharged grids and fixed with a mixture of 4% paraformaldehyde and 0.1% glutaraldehyde in 0.1% potassium-sodium phosphate buffer, pH 7.4. Thereafter, labeling with diluted respective antibodies and 6 nm of protein A gold conjugates diluted at 1:1000 in 1% BSA in phosphate buffer were performed. The samples were post-fixed for 10 min with 2% glutaraldehyde in phosphate buffer, washed with H2O, rinsed with three drops of 1% uranyl acetate, and immediately dried with filter paper.
Immunoisolation. Affinity-purified VGAT-antibodies (VGAT/1) were conjugated to Eupergit C1Z methacrylate microbeads (1 µm mean diameter; Röhm Pharmaceuticals, Darmstadt, Germany) as described previously (Burger et al., 1989
Vesicular GABA and glutamate uptake assay. Uptake assays for glutamate and GABA was performed as described previously (Hell et al., 1988
Acidification assay. Either starting material (LP2) or immunoisolates (synaptophysin beads, VGAT beads, and control beads) were resuspended in acidification assay buffer containing 320 mM sucrose, 2 mM MgSO4, 2 mM MgCl2, and 10 mM 3-[N-morpholino]propanesulfonic acid, adjusted to pH 7.4 with KOH. The acidification assay for each fraction was performed as described by Hell et al. (1990)
Immunoblot analysis. SDS-PAGE was performed according to Laemmli (1970)
RESULTS
VGAT-specific antibodies recognize a subset of synaptic vesicles
To characterize GABAergic synaptic vesicles, we generated a panel of serum antibodies specific for VGAT. Rabbits were immunized with peptides corresponding to regions in the C- and N-terminal cytoplasmic tails of the transporter, respectively. After affinity purification, three of the sera recognized a major double-band in purified synaptic vesicles with a molecular weight expected for VGAT (McIntire et al., 1997
We compared the enrichment of VGAT with that of other vesicular transporters during the purification of synaptic vesicles from rat brain. Synaptic vesicles were isolated from synaptosomes (P2 fraction) by differential and sucrose-gradient centrifugations, followed by chromatography on controlled-pore glass beads using established procedures (for details, see Huttner et al., 1983
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Figure 1. Characterization of antibodies specific for the VGAT. A, Antibodies specific for the N- (VGAT/1 and VGAT/3) or C-terminal (VGAT/4) domain recognize identical bands in synaptic vesicles and in cells expressing VGAT. tsA201 cells were transiently transfected with either a rVGAT plasmid (VGAT) or a plasmid without insert (pcDNA) and analyzed by immunoblotting. For comparison, purified synaptic vesicles (SV) were analyzed in parallel. All three antibodies recognized a doublet band (57 and 50 kDa) in both synaptic vesicles and transfected cells (filled arrowheads). Note that some degradation was observed in the heterologous expression system (open arrowheads). B, VGAT copurifies with other vesicular transporters and the vesicle protein synaptophysin during the isolation of synaptic vesicles. Synaptic vesicles were purified using established procedures, with the following fractions being analyzed: Homogenate; P1, crude nuclear pellet; P2, crude synaptosomes (10,000 × g pellet); S2, 10,000 × g supernatant; LP1, 25,000 × g pellet obtained after synaptosomal lysis; LP2, crude synaptic vesicles; Peak 1 and SV, large membrane and purified synaptic vesicles as separated by controlled-pore glass (CPG) bead chromatography, respectively (for details, see Huttner et al., 1983
Previous studies have shown that the major synaptic vesicle proteins are present on virtually all vesicles in a purified synaptic vesicle fraction (for review, see Südhof, 1995
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Figure 2. VGAT is present on a subset of synaptic vesicles. Immunogold labeling of synaptic vesicles purified through controlled-pore glass chromatography using anti-synaptophysin antibody (poly-clonal) (A), anti-VGAT antibody (B), and preimmune serum (C). D shows an overview of VGAT labeling at a lower magnification. Counting of labeled vesicles from several independent experiments revealed that ~16% of all small vesicular profiles were labeled with anti-VGAT antibody, whereas synaptophysin labeling was observed on virtually all synaptic vesicles. Scale bars: A, D, 100 nm. Comparison of the staining patterns for VGAT (E, H) with those of synapto-brevin 2 (F) and GAD (I) in sections of rat cerebellum. The staining patterns of VGAT and GAD are identical. In contrast, synaptobrevin 2 antibody stains many more nerve terminals than VGAT; this is particularly obvious in the molecular cell layer (MO). High-magnification overlays of VGAT (red) and GAD (green) (J), and VGAT (red) and synaptobrevin 2 (green) (G) showing Purkinje cell bodies. GC, Granular cell layer; PC, Purkinje cell layer; MO, molecular cell layer. Scale bars: E, F, H, I, 50 µm; G, J, 10 µm.
To confirm that the antigen recognized by our VGAT antibody is indeed specific for GABAergic nerve terminals, we compared its distribution with that of the GABA-synthesizing enzyme GAD by light microscope immunocytochemistry. In sections of the rat cerebellum, VGAT staining was prominent around the cell body of the Purkinje cells, particularly in the basket cell synapse at the axon hillock, which is known to be GABAergic (Oertel et al., 1981
Immunoisolation of GABAergic vesicles defines a functionally distinct subpopulation of synaptic vesicles
To isolate VGAT-specific synaptic vesicles from rat brain, affinity-purified VGAT/1 antibody was coupled to methacrylate beads (referred as VGAT beads). Methacrylate beads are nonporous and exhibit virtually no nonspecific binding of proteins or membranes (Burger et al., 1989
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Figure 3. VGAT immunobeads bind a highly homogenous organelle population with the size and shape of synaptic vesicles. A, VGAT beads; B, synaptophysin beads; C, control beads. D shows a representative field of the enriched vesicle fraction (LP2; arrows indicate small profiles of the size of synaptic vesicles) used as starting material for immunoisolation. See Materials and Methods for details. Scale bars, 500 nm.
Next, we analyzed the protein composition of the bead-bound membranes by immunoblotting using a panel of antibodies specific for synaptic vesicle proteins. For comparison, the same relative amount of starting material, bead-bound, and unbound material were analyzed by SDS-PAGE and immunoblotting. The results are shown in Figure 4. First, VGAT was almost quantitatively bound to the VGAT beads. Commassie blue staining showed that the VGAT bead fraction contained only a small percentage of starting material with most protein remaining in the supernatant solution. Second, the immunoisolates were completely devoid of VMAT2 and VAChT, demonstrating that no overlap exists between GABAergic and monoaminergic or cholinergic vesicles. Third, VGAT immunoisolates contained all the major synaptic vesicle proteins tested (Fig. 4). As evident from the figure and further confirmed by quantitative immunoblotting (data not shown), the relative proportions of these proteins were similar to the starting material (Fig. 4) and to synaptophysin immunoisolates (data not shown). Although it has been inferred previously from immunocytochemical studies that GABAergic nerve terminals contain most of these proteins (Südhof, 1995
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Figure 4. Vesicles isolated on beads containing VGAT antibodies (VGAT Beads) are devoid of VAChT and VMAT2 but contain other synaptic vesicle proteins. The resuspended vesicle fraction (LP2) used as starting material (Input) was compared with the bead-bound material (Beads) and the material remaining in the supernatant after bead incubation (Sup). To allow for direct comparison, equal relative amounts of each fraction were separated in parallel.
The data presented so far suggest that immunoisolation of VGAT-containing vesicles resulted in a pure GABAergic vesicle fraction with only negligible contamination by vesicles specific for other neurotransmitters. To confirm that the immunoisolates represent a functionally separate subpopulation of synaptic vesicles, we assayed for proton gradient-dependent GABA uptake using a standard transport assay (Hell et al., 1990
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Figure 5. VGAT immunoisolates are enriched for GABA uptake activity and impoverished for glutamate uptake activity. FCCP-sensitive GABA (A) and glutamate (B) uptake activities in LP2 (Input), unbound material (Sup), and bound material on VGAT beads (Beads) were measured using radiolabeled substrates and a standard filtration assay as described in Materials and Methods. All values were normalized to the relative amount of vesicle marker synaptophysin. The figures shows mean ± SD values of at least two independent experiments (in each experiment, n = 4).
Finally, we also monitored vesicular acidification in response to glutamate and chloride using the pH-sensitive dye acridine orange. Previous work showed that glutamate uptake is associated with vesicular acidification, suggesting that it serves as a counterion in addition to chloride for the vacuolar ATPase (Maycox et al., 1988
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Figure 6. Comparison of ATP-induced acidification using glutamate and chloride as counterion in VGAT and synaptophysin immunoisolates. Acidification was monitored by double-wavelength spectroscopy using acridine orange as indicator dye. The reaction was started by adding ATP. At the end of the reaction, 20 mM (NH4)2SO4 was added to equalize the intravesicular pH with that of the medium (Hell et al., 1990
DISCUSSION
In the present study, we have shown that antibodies specific for vesicular neurotransmitter transporters can be used to quantitatively immunoisolate synaptic vesicles that are specific for the transmitter, with virtually no contamination by vesicles specific for other neurotransmitters.
The vesicle subpopulation isolated with our VGAT antibodies is highly enriched for GABA uptake activity. This finding strongly supports the inference that VGAT is functioning as the GABA transporter in mammalian brain synaptic vesicles. Our data complement previous reports showing that expression of the transporter in a heterologous expression system (PC12 cells) leads to proton gradient-dependent GABA uptake in isolated membrane fractions (McIntire et al., 1997
The availability of purified fractions of transmitter-specific vesicles for biochemical studies permits us to investigate differences in the transport mechanisms of individual transmitters. As outlined in the introductory remarks, vesicular uptake of glutamate, GABA, and catecholamines is dependent on different components of the electrochemical proton gradient created by the vacuolar H+-ATPase. Unlike any of the other transmitters, glutamate was shown to be cotransported with protons (Maycox et al., 1988
Our analysis has revealed that all the major synaptic vesicle proteins for which we have tested are present on GABAergic synaptic vesicle membranes. Moreover, a comparison of general protein staining patterns on electropherograms has revealed no obvious differences in banding. This sort of uniformity of vesicle membranes was inferred previously from immunocytochemistry but has never been systematically investigated. Of course, we cannot yet exclude the possibility that GABAergic vesicles contain other idiotypic proteins that are not resolved by one-dimensional electrophoresis. However, at present, our findings are consistent with the notion that synaptic vesicles are biochemically homogeneous with respect to most of their constituents and thus that the mechanisms of exocytosis and vesicle recycling are the same for all neurotransmitter vesicles. Neurotransmitter vesicles become unique by virtue of the inclusion of selective transporters in their membranes.
FOOTNOTES Received Jan. 20, 2000; revised March 27, 2000; accepted April 7, 2000.
We thank Drs. P. De Camilli (New Haven, CT) and K. Buckley (Boston, MA) for providing antibodies. We are grateful to M. Rudnick (New Haven, CT) for her help in raising the VAChT-antibody, W. Jahn and S. Lausmann for their skillful assistance with the light and electron microscopy immunocytochemistry, and Dr. S. Arch for helpful comments and critical reading of this manuscript.
Correspondence should be addressed to Dr. Reinhard Jahn, Department of Neurobiology, Max-Planck-Institute for Biophysical Chemistry, Am Fassberg D-37077 Göttingen, Germany. E-mail: rjahn{at}gwdg.de.
REFERENCES
- Alfonso A, Grundahl K, Duerr JS, Han HP, Rand JB (1993) The Caenorhabditis elegans unc-17 gene: a putative vesicular acetylcholine transporter. Science 261:617-619
[Abstract/Free Full Text] .- Angel I, Fleissner AS (1983) Synaptic vesicles from hog brain: their isolation and the coupling between synthesis and uptake of gamma-aminobutyrate by glutamate decarboxylase. Neurochem Int 5:697-712.
- Bajjalieh SM, Frantz GD, Weimann JM, McConnell SK, Scheller RH (1994) Differential expression of synaptic vesicle protein 2 (SV2) isoforms. J Neurosci 14:5223-5235[Abstract].
- Brose N, Petrenko AG, Südhof TC, Jahn R (1992) Synaptotagmin: a Ca2+ sensor on the synaptic vesicle surface. Science 256:1021-1025
[Abstract/Free Full Text] .- Burger PM, Mehl E, Cameron PL, Maycox PR, Baumert M, Lottspeich F, De Camilli P, Jahn R (1989) Synaptic vesicles immunoisolated from rat cerebral cortex contain high levels of glutamate. Neuron 3:715-720[ISI][Medline].
- Burger PM, Hell JW, Mehl E, Krasel C, Lottspeich F, Jahn R (1991) GABA and glycine in synaptic vesicles: storage and transport characteristics. Neuron 7:287-293[ISI][Medline].
- Chapman ER, Hanson PI, An S, Jahn R (1995) Ca2+ regulates the interaction between synaptotagmin and syntaxin. J Biol Chem 270:23667-23671
[Abstract/Free Full Text] .- Chaudhry FA, Reimer RJ, Bellocio E, Danbolt NC, Osen KK, Edwards RH, Storm-Mathisen J (1998) The vesicular GABA transporter, VGAT, localizes to synaptic vesicles in sets of glycinergic as well as GABAergic neurons. J Neurosci 18:9733-9750
[Abstract/Free Full Text] .- Christensen H, Fykse EM, Fonnum F (1991) Inhibition of gamma-aminobutyrate and glycine uptake into synaptic vesicles. Eur J Pharmacol 207:73-79[ISI][Medline].
- De Camilli P, Harris SM, Huttner WB, Greengard P (1983) Synapsin I (Protein I), a nerve-terminal-specific phosphoprotein. II. Its specific association with synaptic vesicles demonstrated by immunocytochemistry in agarose-embedded synaptosomes. J Cell Biol 96:1355-1373
[Abstract/Free Full Text] .- Edelmann L, Hanson PI, Chapman ER, Jahn R (1995) Synaptophysin-binding to synaptobrevin: a potential mechanism for controlling the exocytotic fusion machine. EMBO J 14:224-231[ISI][Medline].
- Erickson JD, Eiden LE, Hoffman B (1992) Expression cloning of a reserpine-sensitive vesicular monoamine transporter. Proc Natl Acad Sci USA 89:10993-10997
[Abstract/Free Full Text] .- Fykse EM, Takei K, Walch-Solimena C, Geppert M, Jahn R, De Camilli P, Südhof TC (1993) Relative properties and localizations of synaptic vesicle protein isoforms: the case of the synaptophysins. J Neurosci 13:4997-5007[Abstract].
- Gray EG (1959) Axosomatic and axodendritic synapses of the cerebral cortex: an electron microscope study. J Anat 93:420-433[ISI][Medline].
- Hell JW, Jahn R (1994) Preparation of synaptic vesicles from mammalian brain. In: Cell biology: a laboratory handbook, Ed 1 (Celis JE, ed), pp 567-574. New York: Academic.
- Hell JW, Maycox PR, Stadler H, Jahn R (1988) Uptake of GABA by rat brain synaptic vesicles isolated by a new procedure. EMBO J 7:3023-3029[ISI][Medline].
- Hell JW, Maycox PR, Jahn R (1990) Energy dependence and functional reconstitution of the GABA carrier from synaptic vesicles. J Biol Chem 265:2111-2117
[Abstract/Free Full Text] .- Holtje M, von Jagow B, Pahner I, Lautenschlager M, Hortnagl H, Nurnberg B, Jahn R, Ahnert-Hilger G (2000) The neuronal monoamine transporter VMAT2 is regulated by the trimeric GTPase Go(2). J Neurosci 20:2131-2141
[Abstract/Free Full Text] .- Huttner WB, Schiebler W, Greengard P, De Camilli P (1983) Synapsin I (Protein I), a nerve terminal-specific phosphoprotein. III. Its association with synaptic vesicles studied in a highly purified synaptic vesicle preparation. J Cell Biol 96:1374-1388
[Abstract/Free Full Text] .- Jahn R, Schiebler W, Greengard P (1984) A quantitative dot-immunobinding assay for proteins using nitrocellulose membrane filters. Proc Natl Acad Sci USA 81:1684-1687
[Abstract/Free Full Text] .- Jahn R, Schiebler W, Ouimet C, Greengard P (1985) A 38,000 dalton membrane protein (p38) present in synaptic vesicles. Proc Natl Acad Sci USA 82:4137-4141
[Abstract/Free Full Text] .- Laemmli UK (1970) Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227:680-685[Medline].
- Liu Y, Edwards RH (1997) The role of vesicular transport proteins in synaptic transmission and neural degeneration. Annu Rev Neurosci 20:125-156[ISI][Medline].
- Liu Y, Peter D, Roghani A, Schuldiner S, Prive GG, Eisenberg D, Brecha N, Edwards RH (1992) A cDNA that suppresses MPP+ toxicity encodes a vesicular amine transporter. Cell 70:539-551[ISI][Medline].
- Masson J, Sagne C, Hamon M, El Mestikawy S (1999) Neurotransmitter transporters in the central nervous system. Pharmacol Rev 51:439-464
[Abstract/Free Full Text] .- Maycox PR, Deckwerth T, Hell JW, Jahn R (1988) Glutamate uptake by brain synaptic vesicles: energy dependence of transport and functional reconstitution in proteoliposomes. J Biol Chem 263:15423-15428
[Abstract/Free Full Text] .- Maycox PR, Hell JW, Jahn R (1990) Amino acid neurotransmission: Spotlight on synaptic vesicles. Trends Neurosci 13:83-87[ISI][Medline].
- McIntire SL, Reimer RJ, Schuske K, Edwards RH, Jorgensen EM (1997) Identification and characterization of the vesicular GABA transporter. Nature 389:870-876[Medline].
- Mugnaini E, Dahl AL (1983) Zinc-aldehyde fication for light-microscopic immunocytochemistry of nervous tissues. J Histochem Cytochem 31:1435-1438[Abstract].
- Oertel WH, Schmechel DE, Mugnaini E, Tappaz ML, Kopin IJ (1981) Immunocytochemical localization of glutamate decarboxylase in rat cerebellum with a new antiserum. Neuroscience 6:2715-2735[ISI][Medline].
- Reetz A, Solimena M, Matteoli M, Folli F, Takei K, De Camilli P (1991) GABA and pancreatic
-cells: colocalization of glutamic acid decarboxylase (GAD) and GABA with synaptic-like microvesicles suggests their role in GABA storage and secretion. EMBO J 10:1275-1284[ISI][Medline].
- Renick SE, Kleven DT, Chan J, Stenius K, Milner TA, Pickel VM, Fremeau Jr RT (1999) The mammalian brain high-affinity L-proline transporter is enriched preferentially in synaptic vesicles in a subpopulation of excitatory nerve terminals in rat forebrain. J Neurosci 19:21-33
[Abstract/Free Full Text] .- Sagne C, El Mestikawy S, Isambert M-F, Hamon M, Henry J-P, Giros B, Gasnier B (1997) Cloning of a functional vesicular GABA and glycine transporter by screening of genome databases. FEBS Lett 417:177-183[ISI][Medline].
- Schneider WJ, Slaughter C, Goldstein JL, Anderson RGW, Capra JD, Brown MS (1983) Use of antipeptide antibodies to demonstrate external orientation of the NH2 terminus of the low density lipoprotein receptor in the plasma membrane of fibroblasts. J Cell Biol 97:1635-1640
[Abstract/Free Full Text] .- Stenius K, Janz R, Südhof TC, Jahn R (1995) Structure of synaptogyrin (p29) defines novel synaptic vesicle protein. J Cell Biol 131:1801-1809
[Abstract/Free Full Text] .- Südhof TC (1995) The synaptic vesicle cycle: a cascade of protein-protein interactions. Nature 375:645-653[Medline].
- Towbin H, Staehelin H, Gordon J (1979) Electrophoretic transfer of proteins from polyacrylamide gels to nitrocellulose sheets: procedure and some applications. Proc Natl Acad Sci USA 76:4350-4354
[Abstract/Free Full Text] .- Whittaker VP (1984) The structure and function of cholinergic synaptic vesicles. Biochem Soc Trans 12:561-576[ISI][Medline].
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