Interactions of synapsin I with phospholipids: possible role in synaptic vesicle clustering and in the maintenance of bilayer structures.

Synapsin I is a synaptic vesicle-specific phosphoprotein composed of a globular and hydrophobic head and of a proline-rich, elongated and basic tail. Synapsin I binds with high affinity to phospholipid and protein components of synaptic vesicles. The head region of the protein has a very high surface activity, strongly interacts with acidic phospholipids and penetrates the hydrophobic core of the vesicle membrane. In the present paper, we have investigated the possible functional effects of the interaction between synapsin I and vesicle phospholipids. Synapsin I enhances both the rate and the extent of Ca(2+)-dependent membrane fusion, although it has no detectable fusogenic activity per se. This effect, which appears to be independent of synapsin I phosphorylation and localized to the head region of the protein, is attributable to aggregation of adjacent vesicles. The facilitation of Ca(2+)-induced liposome fusion is maximal at 50-80% of vesicle saturation and then decreases steeply, whereas vesicle aggregation does not show this biphasic behavior. Association of synapsin I with phospholipid bilayers does not induce membrane destabilization. Rather, 31P-nuclear magnetic resonance spectroscopy demonstrated that synapsin I inhibits the transition of membrane phospholipids from the bilayer (L alpha) to the inverted hexagonal (HII) phase induced either by increases in temperature or by Ca2+. These properties might contribute to the remarkable selectivity of the fusion of synaptic vesicles with the presynaptic plasma membrane during exocytosis.

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Identification of synapsin I peptides that insert into lipid membranes

Biochemical Journal ◽

10.1042/bj3540057 ◽

2001 ◽

Vol 354 (1) ◽

pp. 57-66 ◽

Cited By ~ 24

Author(s):

James J. CHEETHAM ◽

Sabine HILFIKER ◽

Fabio BENFENATI ◽

Thomas WEBER ◽

Paul GREENGARD ◽

...

Keyword(s):

Synaptic Vesicle ◽

Synaptic Vesicles ◽

Molecular Mechanisms ◽

Phospholipid Bilayer ◽

Synapsin I ◽

Affinity Binding ◽

Hydrophobic Core ◽

Vesicle Membrane ◽

High Affinity Binding ◽

High Affinity

The synapsins constitute a family of synaptic vesicle-associated phosphoproteins essential for regulating neurotransmitter release and synaptogenesis. The molecular mechanisms underlying the selective targeting of synapsin I to synaptic vesicles are thought to involve specific protein–protein interactions, while the high-affinity binding to the synaptic vesicle membrane may involve both protein–protein and protein–lipid interactions. The highly hydrophobic N-terminal region of the protein has been shown to bind with high affinity to the acidic phospholipids phosphatidylserine and phosphatidylinositol and to penetrate the hydrophobic core of the lipid bilayer. To precisely identify the domains of synapsin I which mediate the interaction with lipids, synapsin I was bound to liposomes containing the membrane-directed carbene-generating reagent 3-(trifluoromethyl)-3-(m-[125I]iodophenyl)diazirine and subjected to photolysis. Isolation and N-terminal amino acid sequencing of 125I-labelled synapsin I peptides derived from CNBr cleavage indicated that three distinct regions in the highly conserved domain C of synapsin I insert into the hydrophobic core of the phospholipid bilayer. The boundaries of the regions encompass residues 166–192, 233–258 and 278–327 of bovine synapsin I. These regions are surface-exposed in the crystal structure of domain C of bovine synapsin I and are evolutionarily conserved among isoforms across species. The present data offer a molecular explanation for the high-affinity binding of synapsin I to phospholipid bilayers and synaptic vesicles.

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Interactions of synapsin I with small synaptic vesicles: distinct sites in synapsin I bind to vesicle phospholipids and vesicle proteins.

The Journal of Cell Biology ◽

10.1083/jcb.108.5.1863 ◽

1989 ◽

Vol 108 (5) ◽

pp. 1863-1872 ◽

Cited By ~ 122

Author(s):

F Benfenati ◽

M Bähler ◽

R Jahn ◽

P Greengard

Keyword(s):

Synaptic Vesicles ◽

High Ionic Strength ◽

Synapsin I ◽

Hydrophobic Core ◽

Tail Domain ◽

Vesicle Membrane ◽

High Affinity ◽

Cytoplasmic Surface ◽

Head Domain ◽

Protease Treatment

Synapsin I is a major neuron-specific phosphoprotein that is specifically localized to the cytoplasmic surface of small synaptic vesicles. In the present study, the binding of synapsin I to small synaptic vesicles was characterized in detail. The binding of synapsin I was preserved when synaptic vesicles were solubilized and reconstituted in phosphatidylcholine. After separation of the protein and lipid components of synaptic vesicles under nondenaturing conditions, synapsin I bound to both components. The use of hydrophobic labeling procedures allowed the assessment of interactions between phospholipids and synapsin I in intact synaptic vesicles. Hydrophobic photolabeling followed by cysteine-specific cleavage of synapsin I demonstrated that the head domain of synapsin I penetrates into the hydrophobic core of the bilayer. The purified NH2-terminal fragment, derived from the head domain by cysteine-specific cleavage, bound to synaptic vesicles with high affinity confirming the results obtained from hydrophobic photolabeling. Synapsin I binding to synaptic vesicles could be inhibited by the entire molecule or by the combined presence of the NH2-terminal and tail fragments, but not by an excess of either NH2-terminal or tail fragment alone. The purified tail fragment bound with relatively high affinity to synaptic vesicles, though it did not significantly interact with phospholipids. Binding of the tail fragment was competed by holosynapsin I; was greatly decreased by phosphorylation; and was abolished by high ionic strength conditions or protease treatment of synaptic vesicles. The data suggest the existence of two sites of interaction between synapsin I and small synaptic vesicles: binding of the head domain to vesicle phospholipids and of the tail domain to a protein component of the vesicle membrane. The latter interaction is apparently responsible for the salt and phosphorylation dependency of synapsin I binding to small synaptic vesicles.

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Redistribution of synaptophysin and synapsin I during alpha-latrotoxin-induced release of neurotransmitter at the neuromuscular junction.

The Journal of Cell Biology ◽

10.1083/jcb.110.2.449 ◽

1990 ◽

Vol 110 (2) ◽

pp. 449-459 ◽

Cited By ~ 87

Author(s):

F Torri-Tarelli ◽

A Villa ◽

F Valtorta ◽

P De Camilli ◽

P Greengard ◽

...

Keyword(s):

Synaptic Vesicle ◽

Synaptic Vesicles ◽

Low Dose ◽

Synapsin I ◽

Nerve Terminals ◽

Frozen Sections ◽

Vesicle Membrane ◽

Ultrathin Frozen Sections ◽

Nerve Muscle ◽

Molecular Components

The distribution of two synaptic vesicle-specific phosphoproteins, synaptophysin and synapsin I, during intense quantal secretion was studied by applying an immunogold labeling technique to ultrathin frozen sections. In nerve-muscle preparations treated for 1 h with a low dose of alpha-latrotoxin in the absence of extracellular Ca2+ (a condition under which nerve terminals are depleted of both quanta of neurotransmitter and synaptic vesicles), the immunolabeling for both proteins was distributed along the axolemma. These findings indicate that, in the presence of a block of endocytosis, exocytosis leads to the permanent incorporation of the synaptic vesicle membrane into the axolemma and suggest that, under this condition, at least some of the synapsin I molecules remain associated with the vesicle membrane after fusion. When the same dose of alpha-latrotoxin was applied in the presence of extracellular Ca2+, the immunoreactivity patterns resembled those obtained in resting preparations: immunogold particles were selectively associated with the membrane of synaptic vesicles, whereas the axolemma was virtually unlabeled. Under this condition an active recycling of both quanta of neurotransmitter and vesicles operates. These findings indicate that the retrieval of components of the synaptic vesicle membrane is an efficient process that does not involve extensive intermixing between molecular components of the vesicle and plasma membrane, and show that synaptic vesicles that are rapidly recycling still have the bulk of synapsin I associated with their membrane.

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Botulinum Neurotoxin a Blocks Synaptic Vesicle Exocytosis but Not Endocytosis at the Nerve Terminal

The Journal of Cell Biology ◽

10.1083/jcb.147.6.1249 ◽

1999 ◽

Vol 147 (6) ◽

pp. 1249-1260 ◽

Cited By ~ 59

Author(s):

Elaine A. Neale ◽

Linda M. Bowers ◽

Min Jia ◽

Karen E. Bateman ◽

Lura C. Williamson

Keyword(s):

Synaptic Vesicle ◽

Nerve Terminal ◽

Neurotransmitter Release ◽

Synaptic Vesicles ◽

Botulinum Neurotoxin ◽

Vesicle Membrane ◽

Botulinum Neurotoxin A ◽

Synaptic Vesicle Exocytosis ◽

Vesicle Exocytosis ◽

Botulinum Neurotoxins

The supply of synaptic vesicles in the nerve terminal is maintained by a temporally linked balance of exo- and endocytosis. Tetanus and botulinum neurotoxins block neurotransmitter release by the enzymatic cleavage of proteins identified as critical for synaptic vesicle exocytosis. We show here that botulinum neurotoxin A is unique in that the toxin-induced block in exocytosis does not arrest vesicle membrane endocytosis. In the murine spinal cord, cell cultures exposed to botulinum neurotoxin A, neither K+-evoked neurotransmitter release nor synaptic currents can be detected, twice the ordinary number of synaptic vesicles are docked at the synaptic active zone, and its protein substrate is cleaved, which is similar to observations with tetanus and other botulinal neurotoxins. In marked contrast, K+ depolarization, in the presence of Ca2+, triggers the endocytosis of the vesicle membrane in botulinum neurotoxin A–blocked cultures as evidenced by FM1-43 staining of synaptic terminals and uptake of HRP into synaptic vesicles. These experiments are the first demonstration that botulinum neurotoxin A uncouples vesicle exo- from endocytosis, and provide evidence that Ca2+ is required for synaptic vesicle membrane retrieval.

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Prerequisites for conversion of coated vesicles to synaptic vesicles. A biochemical examination of synaptic-vesicle membrane recycling hypothesis.

Proceedings of the Japan Academy Series B ◽

10.2183/pjab.60.277 ◽

1984 ◽

Vol 60 (7) ◽

pp. 277-280 ◽

Cited By ~ 1

Author(s):

Ken KADOTA ◽

Naoji TOYOTA ◽

Noriyuki MIYAZAKI ◽

Tomoko KADOTA

Keyword(s):

Synaptic Vesicle ◽

Synaptic Vesicles ◽

Coated Vesicles ◽

Membrane Recycling ◽

Vesicle Membrane ◽

Biochemical Examination

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Synaptic vesicle membrane proteins interact to form a multimeric complex.

The Journal of Cell Biology ◽

10.1083/jcb.116.3.761 ◽

1992 ◽

Vol 116 (3) ◽

pp. 761-775 ◽

Cited By ~ 156

Author(s):

M K Bennett ◽

N Calakos ◽

T Kreiner ◽

R H Scheller

Keyword(s):

Membrane Proteins ◽

Membrane Protein ◽

Synaptic Vesicle ◽

Protein Interactions ◽

Synaptic Vesicles ◽

Spatial Organization ◽

Gel Filtration ◽

Vesicle Membrane ◽

Multicomponent Complex ◽

Membrane Components

Potential interactions between membrane components of rat brain synaptic vesicles were analyzed by detergent solubilization followed by size fractionation or immunoprecipitation. The behavior of six synaptic vesicle membrane proteins as well as a plasma membrane protein was monitored by Western blotting. Solubilization of synaptic vesicle membranes in CHAPS resulted in the recovery of a large protein complex that included SV2, p65, p38, vesicle-associated membrane protein, and the vacuolar proton pump. Solubilization in octylglucoside resulted in the preservation of interactions between SV2, p38, and rab3A, while solubilization of synaptic vesicles with Triton X-100 resulted in two predominant interactions, one involving p65 and SV2, and the other involving p38 and vesicle-associated membrane protein. The multicomponent complex preserved with CHAPS solubilization was partially reconstituted following octylglucoside solubilization and subsequent dialysis against CHAPS. Reduction of the CHAPS concentration by gel filtration chromatography resulted in increased recovery of the multicomponent complex. Examination of the large complex isolated from CHAPS-solubilized vesicles by negative stain EM revealed structures with multiple globular domains, some of which were specifically labeled with gold-conjugated antibodies directed against p65 and SV2. The protein interactions defined in this report are likely to underlie aspects of neurotransmitter secretion, membrane traffic, and the spatial organization of vesicles within the nerve terminal.

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Retrieval and recycling of synaptic vesicle membrane in pinched-off nerve terminals (synaptosomes).

The Journal of Cell Biology ◽

10.1083/jcb.78.3.685 ◽

1978 ◽

Vol 78 (3) ◽

pp. 685-700 ◽

Cited By ~ 72

Author(s):

R C Fried ◽

M P Blaustein

Keyword(s):

Synaptic Vesicle ◽

Synaptic Vesicles ◽

Plasma Membranes ◽

Large Diameter ◽

Small Diameter ◽

Physiological Saline ◽

Nerve Terminals ◽

Vesicle Membrane ◽

Thorium Dioxide ◽

Vesicular Exocytosis

The morphological features of pinched-off presynaptic nerve terminals (synaptosomes) from rat brain were examined with electron microscope techniques; in many experiments, an extracellular marked (horseradish peroxidase or colloidal thorium dioxide) was included in the incubation media. When incubated in physiological saline, most terminals appeared approximately spherical, and were filled with small (approximately 400-A diameter) "synaptic vesicles"; mitochondria were also present in many of the terminals. In a number of instances the region of synaptic contact, with adhering portions of the postsynaptic cell membrane and postsynaptic density, could be readily discerned. Approximately 20--30% of the terminals in our preparations exhibited clear evidence of damage, as indicated by diffuse distribution of extracellular markers in the cytoplasm; the markers appeared to be excluded from the intraterminal vesicles under these circumstances. The markers were excluded from the cytoplasm in approximately 70--80% of the terminals, which may imply that these terminals have intact plasma membranes. When the terminals were treated with depolarizing agents (veratridine or K-rich media), in the presence of Ca, many new, large (600--900-A diameter) vesicles and some coated vesicles and new vacuoles appeared. When the media contained an extracellular marker, the newly formed structures frequently were labeled with the marker. If the veratridine-depolarized terminals were subsequently treated with tetrodotoxin (to repolarize the terminals) and allowed to "recover" for 60--90 min, most of the large marker-containing vesicles disappeared, and numerous small (approximately 400-A diameter) marker-containing vesicles appeared. These observations are consistent with the idea that pinched-off presynaptic terminals contain all of the machinery necessary for vesicular exocytosis and for the retrieval and recycling of synaptic vesicle membrane. The vesicle membrane appears to be retrieval primarily in the form of large diameter vesicles which are subsequently reprocessed to form new "typical" small-diameter synaptic vesicles.

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Cross-linking mass spectrometry uncovers protein interactions and functional assemblies in synaptic vesicle membranes

Nature Communications ◽

10.1038/s41467-021-21102-w ◽

2021 ◽

Vol 12 (1) ◽

Author(s):

Sabine Wittig ◽

Marcelo Ganzella ◽

Marie Barth ◽

Susann Kostmann ◽

Dietmar Riedel ◽

...

Keyword(s):

Mass Spectrometry ◽

Synaptic Vesicle ◽

Protein Interactions ◽

Synaptic Vesicles ◽

Large Scale ◽

Cross Linking ◽

Synaptic Membrane ◽

Biophysical Parameters ◽

Vesicle Membrane ◽

Pass Through

AbstractSynaptic vesicles are storage organelles for neurotransmitters. They pass through a trafficking cycle and fuse with the pre-synaptic membrane when an action potential arrives at the nerve terminal. While molecular components and biophysical parameters of synaptic vesicles have been determined, our knowledge on the protein interactions in their membranes is limited. Here, we apply cross-linking mass spectrometry to study interactions of synaptic vesicle proteins in an unbiased approach without the need for specific antibodies or detergent-solubilisation. Our large-scale analysis delivers a protein network of vesicle sub-populations and functional assemblies including an active and an inactive conformation of the vesicular ATPase complex as well as non-conventional arrangements of the luminal loops of SV2A, Synaptophysin and structurally related proteins. Based on this network, we specifically target Synaptobrevin-2, which connects with many proteins, in different approaches. Our results allow distinction of interactions caused by ‘crowding’ in the vesicle membrane from stable interaction modules.

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EVIDENCE FOR RECYCLING OF SYNAPTIC VESICLE MEMBRANE DURING TRANSMITTER RELEASE AT THE FROG NEUROMUSCULAR JUNCTION

The Journal of Cell Biology ◽

10.1083/jcb.57.2.315 ◽

1973 ◽

Vol 57 (2) ◽

pp. 315-344 ◽

Cited By ~ 1429

Author(s):

J. E. Heuser ◽

T. S. Reese

Keyword(s):

Plasma Membrane ◽

Synaptic Vesicle ◽

Synaptic Vesicles ◽

Motor Nerve ◽

Coated Vesicles ◽

Synaptic Membrane ◽

Nerve Terminals ◽

Frog Neuromuscular Junction ◽

Vesicle Membrane ◽

Intracellular Compartments

When the nerves of isolated frog sartorius muscles were stimulated at 10 Hz, synaptic vesicles in the motor nerve terminals became transiently depleted. This depletion apparently resulted from a redistribution rather than disappearance of synaptic vesicle membrane, since the total amount of membrane comprising these nerve terminals remained constant during stimulation. At 1 min of stimulation, the 30% depletion in synaptic vesicle membrane was nearly balanced by an increase in plasma membrane, suggesting that vesicle membrane rapidly moved to the surface as it might if vesicles released their content of transmitter by exocytosis. After 15 min of stimulation, the 60% depletion of synaptic vesicle membrane was largely balanced by the appearance of numerous irregular membrane-walled cisternae inside the terminals, suggesting that vesicle membrane was retrieved from the surface as cisternae. When muscles were rested after 15 min of stimulation, cisternae disappeared and synaptic vesicles reappeared, suggesting that cisternae divided to form new synaptic vesicles so that the original vesicle membrane was now recycled into new synaptic vesicles. When muscles were soaked in horseradish peroxidase (HRP), this tracerfirst entered the cisternae which formed during stimulation and then entered a large proportion of the synaptic vesicles which reappeared during rest, strengthening the idea that synaptic vesicle membrane added to the surface was retrieved as cisternae which subsequently divided to form new vesicles. When muscles containing HRP in synaptic vesicles were washed to remove extracellular HRP and restimulated, HRP disappeared from vesicles without appearing in the new cisternae formed during the second stimulation, confirming that a one-way recycling of synaptic membrane, from the surface through cisternae to new vesicles, was occurring. Coated vesicles apparently represented the actual mechanism for retrieval of synaptic vesicle membrane from the plasma membrane, because during nerve stimulation they proliferated at regions of the nerve terminals covered by Schwann processes, took up peroxidase, and appeared in various stages of coalescence with cisternae. In contrast, synaptic vesicles did not appear to return directly from the surface to form cisternae, and cisternae themselves never appeared directly connected to the surface. Thus, during stimulation the intracellular compartments of this synapse change shape and take up extracellular protein in a manner which indicates that synaptic vesicle membrane added to the surface during exocytosis is retrieved by coated vesicles and recycled into new synaptic vesicles by way of intermediate cisternae.

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Characterization of synapsin I fragments produced by cysteine-specific cleavage: a study of their interactions with F-actin.

The Journal of Cell Biology ◽

10.1083/jcb.108.5.1841 ◽

1989 ◽

Vol 108 (5) ◽

pp. 1841-1849 ◽

Cited By ~ 75

Author(s):

M Bähler ◽

F Benfenati ◽

F Valtorta ◽

A J Czernik ◽

P Greengard

Keyword(s):

Synaptic Vesicles ◽

Function Analysis ◽

Actin Binding ◽

Structural Basis ◽

Synapsin I ◽

Dependent Manner ◽

Tail Region ◽

Head Region ◽

Parent Molecule

Synapsin I is a neuron-specific phosphoprotein that is concentrated in the presynaptic nerve terminal in association with the cytoplasmic surface of synaptic vesicles. It has been demonstrated to bundle F-actin in a phosphorylation-dependent manner in vitro, a property consistent with its proposed role in linking synaptic vesicles to the cytoskeleton and its involvement in the regulation of neurotransmitter release. Synapsin I is composed of two distinct domains, a COOH terminal, collagenase-sensitive, hydrophilic, and strongly basic tail region, and an NH2 terminal, collagenase-resistant head region relatively rich in hydrophobic amino acids. To elucidate the structural basis for the interactions between synapsin I and F-actin and how it relates to other characteristics of synapsin I, we have performed a structure-function analysis of fragments of synapsin I produced by cysteine-specific cleavage with 2-nitro-5-thiocyanobenzoic acid. The fragments were identified and aligned with the parent molecule using the deduced primary structure of synapsin I and the known phosphorylation sites as markers. We have purified these fragments and examined their interactions with F-actin. Two distinct fragments, a 29-kD NH2-terminal fragment and a 15-kD middle fragment, were shown to contain F-actin binding sites. A 51/54-kD middle/tail fragment retained the F-actin binding and bundling activity of synapsin I, but the isolated tail fragment did not retain either activity. In contrast to phosphorylation of sites two and three in intact synapsin I, which abolishes F-actin bundling activity, phosphorylation of these sites in the middle/tail fragment failed to abolish this activity. In conclusion, three domains of synapsin I appear to be involved in F-actin binding and bundling.

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