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Intracellular Electrochemical Nanomeasurements Reveal that Exocytosis of Molecules at Living Neurons is Subquantal and Complex

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TLDR
It is shown that the fraction of the vesicular octopamine content released from a living Drosophila neuromuscular neuron is very small, and combined with partial release controlled by fluctuations of the fusion pore, offers presynaptic plasticity that can be widely regulated.
Abstract
Since the early work of Bernard Katz, the process of cellular chemical communication via exocytosis, quantal release, has been considered to be all or none. Recent evidence has shown exocytosis to be partial or 'subquantal' at single-cell model systems, but there is a need to understand this at communicating nerve cells. Partial release allows nerve cells to control the signal at the site of release during individual events, where the smaller the fraction released, the greater the range of regulation. Here we show that the fraction of the vesicular octopamine content released from a living Drosophila larval neuromuscular neuron is very small. The percentage of released molecules was found to be only 4.5% for simple events and 10.7% for complex (i.e., oscillating or flickering) events. This large content, combined with partial release controlled by fluctuations of the fusion pore, offers presynaptic plasticity that can be widely regulated. Two works published in 2010 suggested that the Katz principle, [1] was incorrect for all-or-none release and that only part of the chemical load of vesicles was released during exocytosis, at least as measured as a full spike during amperometry. [2] The combination of electrochemical methods to measure both release and vesicle content in 2015 added a wealth of information to support the concept of partial release in exocytosis. [3] Additionally, this has recently been supported by work with TIRF microscopy showing 'subquantal' release from vesicles in adrenal chromaffin cells and using super-resolution STED microscopy. [4] It appears that the full event generally involves release of only part of the load of chemical messenger in single-cell model systems like adrenal chromaffin and PC12 cells. Is this also true at living neurons in a nervous system and to what extent? To answer this critical question, we quantified the number of octopamine molecules in the neuromuscular neurons of Drosophila larvae by adapting an amperometric technique developed in our

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Multimodal Imaging Mass Spectrometry: Next Generation Molecular Mapping in Biology and Medicine.

TL;DR: This review describes MALDI, SIMS, and DESI imaging mass spectrometric technologies and how these have been integrated with other analytical modalities such as microscopy, transcriptomics, spectroscopy, and electrochemistry in a field termed multimodal imaging.
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Electrochemically Probing Dynamics of Ascorbate during Cytotoxic Edema in Living Rat Brain.

TL;DR: An electrochemical system that pinpoints a critical neurochemical involved in cytotoxic edema is presented, and it is revealed that this release is associated with an increase in the amount of cytot toxic edema-inducing agent and that blockage of cytoskeletal edema abolishes ascorbate release, further supporting that asCorbate efflux is cytot Toxic Edema-dependent.
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A Robust Au-C≡C Functionalized Surface: Toward Real-Time Mapping and Accurate Quantification of Fe 2+ in the Brains of Live AD Mouse Models.

TL;DR: Using the powerful tool, it was first discovered that the uptake of extracellular Fe 2+ into cortex and striatum was largely mediated by cyclic adenosine monophosphate (cAMP) through CREB-related pathway in AD mouse brain.
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Chemical Analysis of Single Cells and Organelles.

TL;DR: This paper presents Electrochemical Analysis of Single Cells and Organelles, a large-scale study of single cells and organelles using SuperResolution Microscopy for imaging, and some of the techniques used in this study, as well as some new approaches to characterization.
Journal ArticleDOI

Quantitative Nano‑amperometric Measurement of Intravesicular Glutamate Content and its Sub‑Quantal Release by Living Neurons

TL;DR: In this article, a single SiC nanowire was used to measure real-time Glu fluxes released via exocytosis by large Glu vesicles ( ca. 125 nm diameter) present in single hippocampal axonal varicosities.
References
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Journal ArticleDOI

Quantal components of the end-plate potential

TL;DR: It was found that the size of the end-plate response approached that of the spontaneous potential and at the same time exhibited large random fluctuations, apparently involving steps of unit size.
Journal ArticleDOI

Spontaneous subthreshold activity at motor nerve endings

P. Fatt, +1 more
TL;DR: The present study arose from the chance observation that end-plates of resting muscle fibres are the seat of spontaneous electric discharges which have the character of miniature end-plate potentials.
Journal ArticleDOI

The exocytotic event in chromaffin cells revealed by patch amperometry

TL;DR: Exocytosis of individual chromaffin granules is investigated by using cell-attached capacitance measurements, combined with electrochemical detection of catecholamines, achieved by inserting a carbon-fibre electrode into the patch pipette and finding that the fusion-pore diameter stays at <3 nm for a variable period, which can last for several seconds, before it expands.
Journal ArticleDOI

Single synaptic vesicles fusing transiently and successively without loss of identity

TL;DR: The experimental evidence supports a predominance of kiss-and-run fusion events and rapid vesicular re-use in vesicle cycling, and an alternative hypothesis of independent fusion of partially stained vesicles arising from endosomal splitting could be excluded.
Journal ArticleDOI

Differential ultrastructure of synaptic terminals on ventral longitudinal abdominal muscles in Drosophila larvae

TL;DR: The innervation of ventral longitudinal abdominal muscles of third-instar Drosophila larvae was investigated with Nomarski, confocal, and electron microscopy to define the ultrastructural features of synapse-bearing terminals.
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