Your search keyword '"Wu, Ling-gang"' showing total 18 results

1. Light and electron microscopic imaging of synaptic vesicle endocytosis at mouse hippocampal cultures.

Author

Shi B, Wu XS, Cordero NP, Moreira SL, and Wu LG

Subjects

Animals, Endocytosis physiology, Hippocampus, Mice, Microscopy, Electron, Neurotransmitter Agents metabolism, Synaptophysin metabolism, Electrons, Synaptic Vesicles metabolism

Abstract

Following the release of neurotransmitters at synaptic vesicles via exocytosis, endocytosis is initiated to retrieve vesicles that have fused with the plasma membrane of nerve terminals and recycle them, thus sustaining synaptic transmission. Here, we describe imaging-based protocols for quantitative measurements of endocytosis at cultured synapses. These protocols include (1) primary culture of mouse hippocampal neurons, (2) studying endocytosis at neurons transfected with a pH-sensitive synaptophysin-pHluorin2× using fluorescent microscopy, and (3) imaging endocytosis at fixed neurons with electron microscopy. For complete details on the use and execution of this protocol, please refer to Wu et al. (2016) and Wu et al. (2021)., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2022 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2022

2. Phospholipase A 2 -based probes to study vesicle trafficking.

Author

Wang X, Sun M, Chan CY, and Wu LG

Subjects

Phospholipases A2 metabolism, Synaptic Transmission, Multimodal Imaging, Synaptic Vesicles metabolism, Endocytosis

Abstract

Vesicle exo- and endocytosis mediate important biological functions, including synaptic transmission. In this issue of Cell Reports Methods , Seong J. An et al. found that the fluorescently tagged C2 domain of phospholipase A 2 binds to membrane phosphatidylcholine and thus labels vesicle membrane, allowing for super-resolution and electron microscopic visualization of vesicle trafficking., Competing Interests: The authors declare no competing interests., (© 2022 The Author(s).)

Published

2022

3. Presynaptic Kv3 channels are required for fast and slow endocytosis of synaptic vesicles.

Author

Wu XS, Subramanian S, Zhang Y, Shi B, Xia J, Li T, Guo X, El-Hassar L, Szigeti-Buck K, Henao-Mejia J, Flavell RA, Horvath TL, Jonas EA, Kaczmarek LK, and Wu LG

Subjects

Actins metabolism, Animals, CHO Cells, Cricetulus, Mice, Mutation, Presynaptic Terminals metabolism, Shaw Potassium Channels genetics, Endocytosis physiology, Shaw Potassium Channels metabolism, Synaptic Transmission physiology, Synaptic Vesicles metabolism

Abstract

Since their discovery decades ago, the primary physiological and pathological effects of potassium channels have been attributed to their ion conductance, which sets membrane potential and repolarizes action potentials. For example, Kv3 family channels regulate neurotransmitter release by repolarizing action potentials. Here we report a surprising but crucial function independent of potassium conductance: by organizing the F-actin cytoskeleton in mouse nerve terminals, the Kv3.3 protein facilitates slow endocytosis, rapid endocytosis, vesicle mobilization to the readily releasable pool, and recovery of synaptic depression during repetitive firing. A channel mutation that causes spinocerebellar ataxia inhibits endocytosis, vesicle mobilization, and synaptic transmission during repetitive firing by disrupting the ability of the channel to nucleate F-actin. These results unmask novel functions of potassium channels in endocytosis and vesicle mobilization crucial for sustaining synaptic transmission during repetitive firing. Potassium channel mutations that impair these "non-conducting" functions may thus contribute to generation of diverse neurological disorders., Competing Interests: Declaration of interests The authors declare no competing interests., (Published by Elsevier Inc.)

Published

2021

4. Measuring Synaptic Vesicle Endocytosis in Cultured Hippocampal Neurons.

Author

Villarreal S, Lee SH, and Wu LG

Subjects

Animals, Cells, Cultured, Hippocampus cytology, Neurons cytology, Endocytosis physiology, Hippocampus metabolism, Neurons metabolism, Synaptic Transmission physiology, Synaptic Vesicles metabolism

Abstract

During endocytosis, fused synaptic vesicles are retrieved at nerve terminals, allowing for vesicle recycling and thus the maintenance of synaptic transmission during repetitive nerve firing. Impaired endocytosis in pathological conditions leads to decreases in synaptic strength and brain functions. Here, we describe methods used to measure synaptic vesicle endocytosis at the mammalian hippocampal synapse in neuronal culture. We monitored synaptic vesicle protein endocytosis by fusing a synaptic vesicular membrane protein, including synaptophysin and VAMP2/synaptobrevin, at the vesicular lumenal side, with pHluorin, a pH-sensitive green fluorescent protein that increases its fluorescence intensity as the pH increases. During exocytosis, vesicular lumen pH increases, whereas during endocytosis vesicular lumen pH is re-acidified. Thus, an increase of pHluorin fluorescence intensity indicates fusion, whereas a decrease indicates endocytosis of the labelled synaptic vesicle protein. In addition to using the pHluorin imaging method to record endocytosis, we monitored vesicular membrane endocytosis by electron microscopy (EM) measurements of Horseradish peroxidase (HRP) uptake by vesicles. Finally, we monitored the formation of nerve terminal membrane pits at various times after high potassium-induced depolarization. The time course of HRP uptake and membrane pit formation indicates the time course of endocytosis.

Published

2017

5. Calcineurin is universally involved in vesicle endocytosis at neuronal and nonneuronal secretory cells.

Author

Wu XS, Zhang Z, Zhao WD, Wang D, Luo F, and Wu LG

Subjects

Animals, Brain Stem cytology, Brain Stem metabolism, Chromaffin Cells cytology, Chromaffin Cells metabolism, Female, Male, Mice, Mice, Knockout, Calcineurin metabolism, Endocytosis physiology, Neurons metabolism, Synaptic Vesicles metabolism

Abstract

Calcium influx triggers and accelerates endocytosis in nerve terminals and nonneuronal secretory cells. Whether calcium/calmodulin-activated calcineurin, which dephosphorylates endocytic proteins, mediates this process is highly controversial for different cell types, developmental stages, and endocytic forms. Using three preparations that previously produced discrepant results (i.e., large calyx-type synapses, conventional cerebellar synapses, and neuroendocrine chromaffin cells containing large dense-core vesicles), we found that calcineurin gene knockout consistently slowed down endocytosis, regardless of cell type, developmental stage, or endocytic form (rapid or slow). In contrast, calcineurin and calmodulin blockers slowed down endocytosis at a relatively small calcium influx, but did not inhibit endocytosis at a large calcium influx, resulting in false-negative results. These results suggest that calcineurin is universally involved in endocytosis. They may also help explain the discrepancies among previous pharmacological studies. We therefore suggest that calcineurin should be included as a key player in mediating calcium-triggered and -accelerated vesicle endocytosis., (Copyright © 2014 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2014

6. The yin and yang of calcium effects on synaptic vesicle endocytosis.

Author

Wu XS and Wu LG

Subjects

Animals, Organ Culture Techniques, Patch-Clamp Techniques, Rats, Brain Stem metabolism, Calcium metabolism, Endocytosis physiology, Synaptic Vesicles metabolism

Abstract

A large number of studies suggest that calcium triggers and accelerates vesicle endocytosis at many synapses and non-neuronal secretory cells. However, many studies show that prolonging the duration of the stimulation train, which induces more calcium influx, slows down endocytosis; and several studies suggest that instead of triggering endocytosis, calcium actually inhibits endocytosis. Here we addressed this apparent conflict at a large nerve terminal, the calyx of Held in rat brainstem, in which recent studies suggest that transient calcium increase up to tens of micromolar concentration at the micro/nano domain triggers endocytosis. By dialyzing 0-1 μM calcium into the calyx via a whole-cell pipette, we found that slow endocytosis was inhibited by calcium dialysis in a concentration-dependent manner. Thus, prolonged, small, and global calcium increase inhibits endocytosis, whereas transient and large calcium increase at the micro/nano domain triggers endocytosis and facilitates endocytosis. This yin and yang effect of calcium may reconcile apparent conflicts regarding whether calcium accelerates or inhibits endocytosis. Whether endocytosis is fast or slow depends on the net outcome between the yin and yang effect of calcium.

Published

2014

7. Most vesicles in a central nerve terminal participate in recycling.

Author

Xue L, Sheng J, Wu XS, Wu W, Luo F, Shin W, Chiang HC, and Wu LG

Subjects

Animals, Animals, Newborn, Biophysics, Brain Stem cytology, Electric Stimulation, Endocytosis drug effects, Enzyme Inhibitors, Excitatory Amino Acid Agents pharmacology, Excitatory Postsynaptic Potentials drug effects, Excitatory Postsynaptic Potentials physiology, Exocytosis drug effects, Exocytosis physiology, Female, Glutamic Acid metabolism, Glycine analogs & derivatives, Glycine pharmacology, In Vitro Techniques, Kynurenic Acid pharmacology, Macrolides pharmacology, Male, Patch-Clamp Techniques, Presynaptic Terminals drug effects, Rats, Rats, Wistar, Synaptic Vesicles drug effects, Endocytosis physiology, Presynaptic Terminals physiology, Synaptic Transmission physiology, Synaptic Vesicles physiology

Abstract

Studies over the last decade using FM dyes to label vesicles at many terminals, including the calyx-type nerve terminal, led to a well accepted "principle" that only a small fraction of vesicles (∼5-20%) participate in recycling under physiological conditions. This principle imposes a large challenge in maintaining synaptic transmission during repetitive firing, because the small recycling pool may limit the number of available vesicles for release and nerve terminals would have to distinguish the recycling pool from the reserve pool and keep reserve pool vesicles from being used. By recording the presynaptic capacitance changes and the postsynaptic EPSC at rat calyx of Held synapses in the absence or presence of transmitter glutamate in nerve terminals, we developed a new method to count functional recycling vesicles. We found that essentially all vesicles in calyces participated in recycling, challenging the small-recycling-pool principle established by FM dye labeling. Nerve terminals may use all available vesicles to maximize their ability in maintaining synaptic transmission during repetitive firing.

Published

2013

8. Voltage-dependent calcium channels at the plasma membrane, but not vesicular channels, couple exocytosis to endocytosis.

Author

Xue L, Zhang Z, McNeil BD, Luo F, Wu XS, Sheng J, Shin W, and Wu LG

Subjects

Amino Acid Sequence, Animals, Botulinum Toxins pharmacology, Calcium Channels chemistry, Calcium Signaling drug effects, Cell Membrane drug effects, Egtazic Acid analogs & derivatives, Egtazic Acid pharmacology, HEK293 Cells, Humans, Ion Channel Gating drug effects, Membrane Fusion drug effects, Molecular Sequence Data, Nerve Endings drug effects, Nerve Endings metabolism, Protein Transport drug effects, Rats, Rats, Wistar, Synaptic Vesicles drug effects, Calcium Channels metabolism, Cell Membrane metabolism, Endocytosis drug effects, Exocytosis drug effects, Synaptic Vesicles metabolism

Abstract

Although calcium influx triggers endocytosis at many synapses and non-neuronal secretory cells, the identity of the calcium channel is unclear. The plasma membrane voltage-dependent calcium channel (VDCC) is a candidate, and it was recently proposed that exocytosis transiently inserts vesicular calcium channels at the plasma membrane, thus triggering endocytosis and coupling it to exocytosis, a mechanism suggested to be conserved from sea urchin to human. Here, we report that the vesicular membrane, when inserted into the plasma membrane upon exocytosis, does not generate a calcium current or calcium increase at a mammalian nerve terminal. Instead, VDCCs at the plasma membrane, including the P/Q-type, provide the calcium influx to trigger rapid and slow endocytosis and, thus, couple endocytosis to exocytosis. These findings call for reconsideration of the vesicular calcium channel hypothesis. They are likely to apply to many synapses and non-neuronal cells in which VDCCs control exocytosis, and exocytosis is coupled to endocytosis., (Copyright © 2012 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2012

9. Calcium-channel number critically influences synaptic strength and plasticity at the active zone.

Author

Sheng J, He L, Zheng H, Xue L, Luo F, Shin W, Sun T, Kuner T, Yue DT, and Wu LG

Subjects

Animals, Animals, Newborn, Calcium Channels ultrastructure, Organ Culture Techniques, Random Allocation, Rats, Rats, Wistar, Synapses ultrastructure, Synaptic Vesicles ultrastructure, Action Potentials physiology, Calcium Channels physiology, Neuronal Plasticity physiology, Synapses physiology, Synaptic Vesicles physiology

Abstract

How synaptic-vesicle release is controlled at the basic release structure, the active zone, is poorly understood. By performing cell-attached current and capacitance recordings predominantly at single active zones in rat calyces, we found that single active zones contained 5-218 (mean, 42) calcium channels and 1-10 (mean, 5) readily releasable vesicles (RRVs) and released 0-5 vesicles during a 2-ms depolarization. Large variation in the number of calcium channels caused wide variation in release strength (measured during a 2-ms depolarization) by regulating the RRV release probability (P(RRV)) and the RRV number. Consequently, an action potential opened ∼1-35 (mean, ∼7) channels, resulting in different release probabilities at different active zones. As the number of calcium-channels determined P(RRV), it critically influenced whether subsequent release would be facilitated or depressed. Regulating calcium channel density at active zones may thus be a major mechanism to yield synapses with different release properties and plasticity. These findings may explain large differences reported at synapses regarding release strength (release of 0, 1 or multiple vesicles), P(RRV), short-term plasticity, calcium transients and the requisite calcium-channel number for triggering release.

Published

2012

10. Cysteine string protein α: a new role in vesicle recycling.

Author

Sheng J and Wu LG

Subjects

Animals, Humans, Alzheimer Disease metabolism, Dynamin I metabolism, Exocytosis physiology, HSP40 Heat-Shock Proteins metabolism, Membrane Proteins metabolism, Motor Neurons metabolism, Synapses metabolism, Synaptic Transmission physiology, Synaptic Vesicles metabolism, Synaptosomal-Associated Protein 25 metabolism

Abstract

Zhang et al. (2012) and Rozas et al. (2012) in this issue of Neuron find that cysteine string protein α, a protein involved in neurodegeneration, regulates vesicle endocytosis via interaction with dynamin 1, which may participate in regulating synaptic transmission and possibly in maintaining synapses., (Copyright © 2012 Elsevier Inc. All rights reserved.)

Published

2012

11. A membrane pool retrieved via endocytosis overshoot at nerve terminals: a study of its retrieval mechanism and role.

Author

Xue L, McNeil BD, Wu XS, Luo F, He L, and Wu LG

Subjects

Animals, Female, Male, Rats, Rats, Wistar, Cell Membrane physiology, Endocytosis physiology, Presynaptic Terminals physiology, Synaptic Vesicles physiology

Abstract

Endocytosis overshoot, which retrieves more membrane than vesicles just being exocytosed, occurs at nerve terminals and non-neuronal secretory cells. The mechanism that retrieves the overshoot membrane pool and the role of this pool remain largely unknown. We addressed this issue at the rat calyx of Held nerve terminal with capacitance measurements. We found that every calyx contained an overshoot pool ∼1.8 times the readily releasable pool. Retrieval of this pool required large calcium influx, and was inhibited by blockers of calcium/calmodulin-activated calcineurin and dynamin, suggesting the involvement of calcineurin and dynamin in endocytosis overshoot. Depletion of the overshoot pool slowed down compensatory endocytosis, whereas recovery of the overshoot pool via exocytosis that deposited stranded vesicles to the plasma membrane led to recovery of compensatory endocytosis, suggesting that the overshoot pool enhances endocytosis efficiency. These results suggest that the overshoot pool exists at every nerve terminal, is of limited size arising from vesicles stranded at the plasma membrane, is retrieved via calcium/calmodulin/calcineurin and dynamin signaling pathway, and can enhance endocytosis efficiency. Potential mechanisms for how the endocytosis overshoot pool enhances endocytosis efficiency are discussed.

Published

2012

12. Rapid endocytosis does not recycle vesicles within the readily releasable pool.

Author

Wu XS and Wu LG

Subjects

Animals, Exocytosis physiology, Presynaptic Terminals metabolism, Rats, Rats, Wistar, Synaptic Potentials physiology, Time Factors, Endocytosis physiology, Synaptic Vesicles metabolism

Abstract

Endocytosis is essential in maintaining exocytosis at secretory cells. Rapid endocytosis with a time course less than a few seconds is widely observed at nerve terminals and non-neuronal secretory cells. It is generally assumed that rapid endocytosis recycles vesicles within the readily releasable pool (RRP) via a kiss-and-run mechanism that involves rapid opening and closure of a fusion pore at the release site. The present work suggests that both rapid (tau less than approximately 2 s) and slow (tau = approximately 10-20 s) endocytosis do not recycle vesicles to the RRP but to a recycling pool at least a few times larger than the RRP at a nerve terminal, the calyx of Held in rat brainstem. Challenging the long-held view that rapid endocytosis offers a rapid, local vesicle recycling within the RRP, our finding calls for reconsideration of the function and the underlying mechanism of rapid endocytosis. We suggest that rapid endocytosis provides the nerve terminal the ability to recycle vesicles rapidly via the recycling pool and to maintain the normal morphology of the nerve terminal, including the release site, by rapidly clearing the fused vesicle membrane from the release site during intense firing.

Published

2009

13. Location matters: synaptotagmin helps place vesicles near calcium channels.

Author

McNeil BD and Wu LG

Subjects

Animals, Calcium Channels chemistry, Calcium Channels physiology, Cell Communication genetics, Humans, Multigene Family physiology, Presynaptic Terminals chemistry, Presynaptic Terminals metabolism, Presynaptic Terminals physiology, Synaptic Vesicles chemistry, Synaptic Vesicles physiology, Calcium Channels metabolism, Cell Communication physiology, Synaptic Transmission physiology, Synaptic Vesicles metabolism, Synaptotagmins physiology

Abstract

Positioning releasable vesicles near voltage-gated calcium channels may ensure transmitter release upon calcium influx. Disruption of vesicle positioning may underlie short-term synaptic depression. However, how this positioning is achieved is unclear. In this issue of Neuron, Young and Neher find that synaptotagmin 2 helps to align readily releasable vesicles near calcium channels at nerve terminals.

Published

2009

14. Compound vesicle fusion increases quantal size and potentiates synaptic transmission.

Author

He L, Xue L, Xu J, McNeil BD, Bai L, Melicoff E, Adachi R, and Wu LG

Subjects

Animals, Calcium metabolism, Excitatory Postsynaptic Potentials, Exocytosis physiology, Mice, Rats, Rats, Wistar, Synaptic Vesicles metabolism, Synaptotagmin II genetics, Synaptotagmin II metabolism, Synaptic Transmission physiology, Synaptic Vesicles physiology

Abstract

Exocytosis at synapses involves fusion between vesicles and the plasma membrane. Although compound fusion between vesicles was proposed to occur at ribbon-type synapses, whether it exists, how it is mediated, and what role it plays at conventional synapses remain unclear. Here we report the existence of compound fusion, its underlying mechanism, and its role at a nerve terminal containing conventional active zones in rats and mice. We found that high potassium application and high frequency firing induced giant capacitance up-steps, reflecting exocytosis of vesicles larger than regular ones, followed by giant down-steps, reflecting bulk endocytosis. These intense stimuli also induced giant vesicle-like structures, as observed with electron microscopy, and giant miniature excitatory postsynaptic currents (mEPSCs), reflecting more transmitter release. Calcium and its sensor for vesicle fusion, synaptotagmin, were required for these giant events. After high frequency firing, calcium/synaptotagmin-dependent mEPSC size increase was paralleled by calcium/synaptotagmin-dependent post-tetanic potentiation. These results suggest a new route of exocytosis and endocytosis composed of three steps. First, calcium/synaptotagmin mediates compound fusion between vesicles. Second, exocytosis of compound vesicles increases quantal size, which increases synaptic strength and contributes to the generation of post-tetanic potentiation. Third, exocytosed compound vesicles are retrieved via bulk endocytosis. We suggest that this vesicle cycling route be included in models of synapses in which only vesicle fusion with the plasma membrane is considered.

Published

2009

15. Modes of vesicle retrieval at ribbon synapses, calyx-type synapses, and small central synapses.

Author

Wu LG, Ryan TA, and Lagnado L

Subjects

Animals, Endocytosis physiology, Presynaptic Terminals physiology, Synapses ultrastructure, Models, Biological, Synapses classification, Synapses physiology, Synaptic Vesicles ultrastructure

Published

2007

16. The debate on the kiss-and-run fusion at synapses.

Author

He L and Wu LG

Subjects

Animals, Endocrine Glands physiology, Endocytosis physiology, Goldfish, Hippocampus physiopathology, Humans, Synapses physiology, Synaptic Vesicles physiology

Abstract

It has long been proposed that following vesicle fusion, a small pore might open and close rapidly without full dilation. Such 'kiss-and-run' vesicle fusion can in principle result in rapid vesicle recycling and influence the size and the kinetics of the resulting synaptic current. However, the existence of kiss-and-run remains highly controversial, as revealed by recent imaging and electrophysiological studies at several synapses, including hippocampal synapses, neuromuscular junctions and retinal bipolar synapses. Only a minor fraction of fusion events has been shown to be kiss-and-run, as determined using cell-attached capacitance recordings in endocrine cells, pituitary nerve terminals and calyx-type synapses. Further work is needed to determine whether kiss-and-run is a major mode of fusion and has a major role in controlling synaptic strength at synapses.

Published

2007

17. The origin of quantal size variation: vesicular glutamate concentration plays a significant role.

Author

Wu XS, Xue L, Mohan R, Paradiso K, Gillis KD, and Wu LG

Subjects

Animals, Excitatory Postsynaptic Potentials physiology, Rats, Rats, Wistar, Synapses metabolism, Vesicular Glutamate Transport Proteins metabolism, Glutamic Acid metabolism, Synaptic Vesicles metabolism

Abstract

Fusion of a single vesicle induces a quantal response, which is critical in determining synaptic strength. Quantal size varies at most synapses. Its underlying mechanisms are not well understood. Here, we examined five sources of variation: vesicular glutamate concentration ([Glu]v), vesicle volume, ultrafast fusion pore closure, the postsynaptic receptor, and the location between release and the postsynaptic receptor cluster at glutamatergic, calyx of Held synapses. By averaging 2.66 million fusion events from 459 synapses, we resolved the capacitance jump evoked by single vesicle fusion. This capacitance jump, an indicator of vesicle volume, was independent of the amplitude of the miniature EPSC (mEPSC) recorded simultaneously at the same synapses. Thus, vesicle volume is not the main source of mEPSC variation. The capacitance jump was not followed by submillisecond endocytosis, excluding ultrafast endocytosis as a source of variation. Larger mEPSCs were increased to a lesser extent by presynaptic glutamate dialysis, and reduced to a lesser extent by gamma-DGG (gamma-D-glutamylglycine), a competitive AMPA receptor blocker, suggesting that a higher glutamate concentration in the synaptic cleft contributes to the large size of mEPSCs. Larger mEPSCs were not accompanied by briefer rise times, inconsistent with the prediction by, and thus arguing against, the scenario that larger mEPSCs are caused by a shorter distance between the release site and the postsynaptic receptor cluster. In summary, the different amplitudes of mEPSCs were mainly attributable to release of vesicles having similar volumes, but different glutamate amounts, suggesting that [Glu]v is a main source of quantal size variation.

Published

2007

18. Calcium/synaptotagmin-evoked compound fusion increases quantal size and synaptic strength

Author

He, Liming, Xue, Lei, Xu, Jianhua, McNeil, Benjamin D., Bai, Li, Melicoff, Ernestina, Adachi, Roberto, and Wu, Ling-Gang

Subjects

Mice, Synaptotagmin II, Animals, Excitatory Postsynaptic Potentials, Calcium, Synaptic Vesicles, Rats, Wistar, Synaptic Transmission, Article, Exocytosis, Rats

Abstract

Exocytosis at synapses involves fusion between vesicles and the plasma membrane. Although compound fusion between vesicles was proposed to occur at ribbon-type synapses, whether it exists, how it is mediated, and what role it plays at conventional synapses remain unclear. Here we report the existence of compound fusion, its underlying mechanism, and its role at a nerve terminal containing conventional active zones in rats and mice. We found that high potassium application and high frequency firing induced giant capacitance up-steps, reflecting exocytosis of vesicles larger than regular ones, followed by giant down-steps, reflecting bulk endocytosis. These intense stimuli also induced giant vesicle-like structures, as observed with electron microscopy, and giant miniature excitatory postsynaptic currents (mEPSCs), reflecting more transmitter release. Calcium and its sensor for vesicle fusion, synaptotagmin, were required for these giant events. After high frequency firing, calcium/synaptotagmin-dependent mEPSC size increase was paralleled by calcium/synaptotagmin-dependent post-tetanic potentiation. These results suggest a new route of exocytosis and endocytosis composed of three steps. First, calcium/synaptotagmin mediates compound fusion between vesicles. Second, exocytosis of compound vesicles increases quantal size, which increases synaptic strength and contributes to the generation of post-tetanic potentiation. Third, exocytosed compound vesicles are retrieved via bulk endocytosis. We suggest that this vesicle cycling route be included in models of synapses in which only vesicle fusion with the plasma membrane is considered.

Published

2009