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Author

O H Viveros

Bio: O H Viveros is an academic researcher from University of North Carolina at Chapel Hill. The author has contributed to research in topics: Exocytosis & Adrenal medulla. The author has an hindex of 1, co-authored 1 publications receiving 224 citations.

Papers
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Journal ArticleDOI
TL;DR: Nicotinic receptor-mediated secretion of catecholamines from individual cultured bovine adrenal medullary chromaffin cells was measured and characterized with a voltametric microelectrode placed adjacent to the cells, consistent with direct chemical measurement of single exocytotic events.

231 citations


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Journal ArticleDOI
TL;DR: The wide range of cell types in which regulated secretory granule exocytosis occurs is described and the evidence for the expression of the conserved fusion machinery in these cells is assessed.
Abstract: Regulated exocytosis of secretory granules or dense-core granules has been examined in many well-characterized cell types including neurons, neuroendocrine, endocrine, exocrine, and hemopoietic cells and also in other less well-studied cell types. Secretory granule exocytosis occurs through mechanisms with many aspects in common with synaptic vesicle exocytosis and most likely uses the same basic protein components. Despite the widespread expression and conservation of a core exocytotic machinery, many variations occur in the control of secretory granule exocytosis that are related to the specialized physiological role of particular cell types. In this review we describe the wide range of cell types in which regulated secretory granule exocytosis occurs and assess the evidence for the expression of the conserved fusion machinery in these cells. The signals that trigger and regulate exocytosis are reviewed. Aspects of the control of exocytosis that are specific for secretory granules compared with synaptic vesicles or for particular cell types are described and compared to define the range of accessory control mechanisms that exert their effects on the core exocytotic machinery.

900 citations

Journal ArticleDOI
05 Mar 1992-Nature
TL;DR: In this article, the authors show that under voltage-clamp conditions, stochastically occurring signals can be recorded from adrenal chromaffin cells using a carbon-fibre electrode as an electrochemical detector.
Abstract: In synapses, a rise in presynaptic intracellular calcium leads to secretory vesicle fusion in less than a millisecond, as indicated by the short delay from excitation to postsynaptic signal. In nonsynaptic secretory cells, studies at high time resolution have been limited by the lack of a detector as fast and sensitive as the postsynaptic membrane. Electrochemical methods may be sensitive enough to detect catecholamines released from single vesicles. Here, we show that under voltage-clamp conditions, stochastically occurring signals can be recorded from adrenal chromaffin cells using a carbon-fibre electrode as an electrochemical detector. These signals obey statistics characteristic for quantal release; however, in contrast to neuronal transmitter release, secretion occurs with a significant delay after short step depolarizations. Furthermore, we identify a pedestal or 'foot' at the onset of unitary events which may represent the slow leak of catecholamine molecules out of a narrow 'fusion pore' before the pore dilates for complete exocytosis.

805 citations

Journal ArticleDOI
TL;DR: It is more than likely that in the following decade PC12 cells will continue to serve as a model to study exocytosis, which has some advantages over other models for neurosecretion, including chromaffin cells.
Abstract: This review attempts to touch on the history and application of amperometry at PC12 cells for fundamental investigation into the exocytosis process. PC12 cells have been widely used as a model for neural differentiation and as such they have been used to examine the effects of differentiation on exocytotic release and specifically release at varicosities. In addition, dexamethasone-differentiated cells have been shown to have an increased number of releasable vesicles with increased quantal size, thereby allowing for an even broader range of applications including neuropharmacological and neurotoxicological studies. PC12 cells exhibiting large numbers of events have two distinct pools of vesicles, one about twice the quantal size of the other and each about half the total releasable vesicles. As will be outlined in this review, these cells have served as an extremely useful model of exocytosis in the study of the latency of stimulation-release coupling, the role of exocytotic proteins in regulation of release, effect of drugs on quantal size, autoreceptors, fusion pore biophysics, environmental factors, health and disease. As PC12 cells have some advantages over other models for neurosecretion, including chromaffin cells, it is more than likely that in the following decade PC12 cells will continue to serve as a model to study exocytosis.

351 citations

Journal ArticleDOI
TL;DR: Communication between cellular organisms occurs, among other mechanisms, through the release of specific biochemical or chemicalmessengers by an emitting cell, generally coupled to a specific detection of these messengers by a receiving cell.
Abstract: Communication between cellular organisms occurs, among other mechanisms, through the release of specific biochemical or chemical messengers by an emitting cell, generally coupled to a specific detection of these messengers by a receiving cell. According to the target or the scope of the information exchanged, these messengers are released into biological fluids (for instance, into the blood flow), a restricted volume (i.e., a * To whom correspondence should be addressed. Tel: 33-1-4432-3388. Fax: 33-1-4432-3863. E-mail: Christian.Amatore@ens.fr. Chem. Rev. 2008, 108, 2585–2621 2585

333 citations

Journal ArticleDOI
TL;DR: The purpose of this review is to provide practical guidelines for performing amperometric recordings of exocytotic activity and interpreting the results based on shape characteristics of individual release events.
Abstract: Amperometry is widely used to study exocytosis of neurotransmitters and hormones in various cell types. Analysis of the shape of the amperometric spikes that originate from the oxidation of monoamine molecules released during the fusion of individual secretory vesicles provides information about molecular steps involved in stimulation-dependent transmitter release. Here we present an overview of the methodology of amperometric signal processing, including (i) amperometric signal acquisition and filtering, (ii) detection of exocytotic events and determining spike shape characteristics, and (iii) data manipulation and statistical analysis. The purpose of this review is to provide practical guidelines for performing amperometric recordings of exocytotic activity and interpreting the results based on shape characteristics of individual release events.

308 citations