Transcranial Direct Current Stimulation (TDCS) Improved Cognitive Outcomes in a Cancer Survivor With Chemotherapy-induced Cognitive Difficulties

Performing cyclic voltammetry at scan rates into the megavolt per second range allows the exploration of the nanosecond time scale as well as the creation of nanometric diffusion layers adjacent to the electrode surface. This latter property is used here to adjust precisely the diffusion layer width within the outer shell of a fourth-generation dendrimer molecule decorated by 64 [Ru(II)(tpy)2] redox centers (tpy = terpyridine). Thus the shape of the dendrimer molecule adsorbed onto the ultramicroelectrode surface can be explored voltammetrically in a way reminiscent of an analysis with a nanometric microtome. The quantitative analysis developed here applied to the experimental voltammograms demonstrates that in agreement with previous scanning tunneling microscopy (STM) studies the adsorbed dendrimer molecules are no more spherical as they are in solution but resemble more closely hemispheres resting onto the electrode surface on their diametrical planes. The same quantitative analysis gives access to the apparent diffusion coefficient featuring electron hopping between the [Ru(II)/ Ru(III)(tpy)2] redox centers distributed on the dendrimer surface. Based on the electron hopping rate constant thus measured and on a Smoluchowski-type model developed here to take into account viscosity effects during the displacement of the [Ru(II)/Ru(III)(tpy)2] redox centers around their equilibrium positions, it is shown that the [Ru(II)/Ru(III)(tpy)2] redox centers are extremely labile in their potential wells so that they may cross-talk considerably more easily than they would do in solution at an equivalent concentration.

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Correlation between Vesicle Quantal Size and Fusion Pore Release in Chromaffin Cell Exocytosis

Amatore

Arbault

Bonifas

et al. 2005

Biophysical Journal

107

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A significant number of exocytosis events recorded with amperometry demonstrate a prespike feature termed a "foot" and this foot has been correlated with messengers released via a transitory fusion pore before full exocytosis. We have compared amperometric spikes with a foot with spikes without a foot at chromaffin cells and found that the probability of detecting a distinct foot event is correlated to the amount of catecholamine released. The mean charge of the spikes with a foot was found to be twice that of the spikes without a foot, and the frequency of spikes displaying a foot was zero for small spikes increasing to approximately 50% for large spikes. It is hypothesized that in chromaffin cells, where the dense core is believed to nearly fill the vesicle, the expanding core is a controlling factor in opening the fusion pore, that prefusion of two smaller vesicles leads to excess membrane, and that this slows pore expansion leading to an increased observation of events with a foot. Clearly, the physicochemical properties of vesicles are key factors in the control of the dynamics of release through the fusion pore and the high and variable frequency of this release makes it highly significant.

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Ultrafast Voltammetry of Adsorbed Redox Active Dendrimers with Nanometric Resolution: An Electrochemical Microtome

et al. 2001

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Time-Resolved Dynamics of the Vesicle Membrane During Individual Exocytotic Secretion Events, as Extracted from Amperometric Monitoring of Adrenaline Exocytosis from Chromaffin Cells

1999

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In chromaffin cells, adrenaline is known to be released through docking and then fusion of a secretory vesicle to the cytoplasmic membrane of the cell. Here we propose a method for the calculation of the dynamics of the vesicle membrane during the fusion from amperometric currents observed during individual exocytotic secretion events. The method is based on recognition of the fact that the overall current spike shape results from the convolution of the membrane dynamics with the rate of diffusion and exchange of the catecholamine cation inside the matrix core of the vesicle. This convolution can be treated analytically thanks to a reasonable approximation on the relative time scales of the opening function and diffusion; this leads to a convolution integral with which one deconvolutes the experimental amperometric data. An alternative numerical treatment through Brownian motion simulations dispenses with the need for this simplifying approximation. Combination of both approaches yields the membrane dynamics with a precision and a time resolution never achieved before. The peculiar dynamics of the vesicle membrane hint that exocytotic events are regulated by the swelling of the matrix polyelectrolyte core of the vesicle (although this important component is transparent in the analysis proposed here); this points to the important role of matrix swelling in exocytotic behavior. In particular, the effect may be elaborated to offer a new energetic interpretation of the transition between pore release and fusion release: secretory vesicles which involve pores and matrices similar to those of the adrenal cells investigated here can be separated into two classes according to their radius and catecholamine content. Small vesicles (`ca. 25 nm radius, and containing ca. 20 000 molecules) should always release their contents through pore docking; larger vesicles should always fuse, unless another mechanism closes the pore before ca. 20 000 molecules of catecholamine have been released.

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Molecular Dynamics Simulations of the Lipid Bilayer Edge

Jiang

Bouret²,

Kindt³

2004

Biophysical Journal

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Phospholipid bilayers have been intensively studied by molecular dynamics (MD) simulation in recent years. The properties of bilayer edges are important in determining the structure and stability of pores formed in vesicles and biomembranes. In this work, we use molecular dynamics simulation to investigate the structure, dynamics, and line tension of the edges of bilayer ribbons composed of pure dimyristoylphosphatidylcholine (DMPC) or palmitoyl-oleoylphosphatidylethanolamine (POPE). As expected, we observe a significant reorganization of lipids at and near the edges. The treatment of electrostatic effects is shown to have a qualitative impact on the structure and stability of the edge, and significant differences are observed in the dynamics and structure of edges formed by DMPC and palmitoyl-oleoylphosphatidylethanolamine. From the pressure anisotropy in the simulation box, we calculate a line tension of approximately 10-30 pN for the DMPC edge, in qualitative agreement with experimental estimates for similar lipids.

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Na + /H + antiporter (NHE1) and lactate/H + symporters (MCTs) in pH homeostasis and cancer metabolism

Counillon

Bouret

Marchiq

et al. 2016

Biochimica et Biophysica Acta (BBA) - Molecular Cell Research

100

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The Na(+)/H(+)-exchanger NHE1 and the monocarboxylate transporters MCT1 and MCT4 are crucial for intracellular pH regulation, particularly under active metabolism. NHE1, a reversible antiporter, uses the energy provided by the Na(+) gradient to expel H(+) ions generated in the cytosol. The reversible H(+)/lactate(-) symporters MCT1 and 4 cotransport lactate and proton, leading to the net extrusion of lactic acid in glycolytic tumors. In the first two sections of this article we review important features and remaining questions on the structure, biochemical function and cellular roles of these transporters. We then use a fully-coupled mathematical model to simulate their relative contribution to pH regulation in response to lactate production, as it occurs in highly hypoxic and glycolytic tumor cells. This article is part of a Special Issue entitled: Mitochondrial Channels edited by Pierre Sonveaux, Pierre Maechler and Jean-Claude Martinou.

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Regulation of Exocytosis in Chromaffin Cells by Trans‐Insertion of Lysophosphatidylcholine and Arachidonic Acid into the Outer Leaflet of the Cell Membrane

et al. 2006

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Vesicular exocytosis is an important complex process in the communication between cells in organisms. It controls the release of chemical and biochemical messengers stored in an emitting cell. In this report, exocytosis is studied amperometrically (at carbon fiber ultramicroelectrodes) at adrenal chromaffin cells, which release catecholamines after appropriate stimulation, while testing the effects due to trans-insertion of two exogenous compounds (lysophosphatidylcholine (LPC) and arachidonic acid (AA)) on the kinetics of exocytotic events. Amperometric analyses showed that, under the present conditions (short incubation times and micromolar LPC or AA solutions), LPC favors catecholamine release (rate, event frequency, charge released) while AA disfavors the exocytotic processes. The observed kinetic features are rationalized quantitatively by considering a stalk model, for the fusion pore formation, and the physical constraints applied to the cell membrane by the presence of small fractions of LPC and AA diluted in its external leaflet (trans-insertion). We also observed that the detected amount of neurotransmitters in the presence of LPC was larger than under control conditions, while the opposite trend is observed with AA.

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Yann Bouret

Interplay between membrane dynamics, diffusion and swelling pressure governs individual vesicular exocytotic events during release of adrenaline by chromaffin cells

Precise Adjustment of Nanometric-Scale Diffusion Layers within a Redox Dendrimer Molecule by Ultrafast Cyclic Voltammetry: An Electrochemical Nanometric Microtome

Correlation between Vesicle Quantal Size and Fusion Pore Release in Chromaffin Cell Exocytosis

Ultrafast Voltammetry of Adsorbed Redox Active Dendrimers with Nanometric Resolution: An Electrochemical Microtome

Time-Resolved Dynamics of the Vesicle Membrane During Individual Exocytotic Secretion Events, as Extracted from Amperometric Monitoring of Adrenaline Exocytosis from Chromaffin Cells

Molecular Dynamics Simulations of the Lipid Bilayer Edge

Na + /H + antiporter (NHE1) and lactate/H + symporters (MCTs) in pH homeostasis and cancer metabolism

Regulation of Exocytosis in Chromaffin Cells by Trans‐Insertion of Lysophosphatidylcholine and Arachidonic Acid into the Outer Leaflet of the Cell Membrane

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