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- Mechanisms Determining the Time Course of Secretion in Neuro...Mechanisms Determining the Time Course of Secretion in Neuroendocrine Cells
Neuron, Volume 16, Issue 2, 1 February 1996, Pages 369-376
Robert H Chow, Jürgen Klingauf, Christian Heinemann, Robert S Zucker and Erwin Neher
SummaryTransmitter release from chromaffin cells differs from that in synapses in that it persists for a longer time after Ca entry has stopped. This prolonged secretion is not due to a delay between vesicle fusion and transmitter release, nor to slow detection of released substance: step increases in capacitance due to single vesicle fusion precede the release detected by amperometry by only a few milliseconds. The persistence of secretion after a depolarization is reduced by addition of mobile calcium buffer. This suggests that most of the delay is due to diffusion of Ca between channels and release sites, implying that Ca channels and secretory vesicles are not colocalized in chromaffin cells, in contrast to presynaptic active zones.
Summary | Full Text | PDF (113 kb) - Monitoring secretion in real time: capacitance, amperometry ...Monitoring secretion in real time: capacitance, amperometry and fluorescence compared
Trends in Neurosciences, Volume 20, Issue 7, 1 July 1997, Pages 281-287
Joseph K Angleson and William J Betz
AbstractTechniques for measuring exocytosis, endocytosis and vesicle cycling in living cells in real time have resulted in a rapid expansion in the knowledge of these processes in neurons and other secretory cells. Several experimental approaches, developed during the past decade, have played key roles in this expansion. In this review we focus on three techniques: electrophysiological methods for monitoring membrane capacitance, electrochemical methods for detecting released secretory contents and optical methods for imaging membranes of endosomes and recycled vesicles that are stained with fluorescent dyes. Each technique has contributed unique and complementary information about the vesicle cycle, advancing our knowledge of the kinetics of membrane fusion and retrieval, the identity of the secretory contents and the spatial patterns and directional pathways involved in secretory membrane recycling. Naturally, each technique has inherent limitations; some of these shortcomings have recently been resolved by using more than one method simultaneously.
Abstract | Full Text | PDF (584 kb) - Release of small transmitters through kiss-and-run fusion po...Release of small transmitters through kiss-and-run fusion pores in rat pancreatic β cells
Cell Metabolism, Volume 4, Issue 4, 1 October 2006, Pages 283-290
Patrick E. MacDonald, Matthias Braun, Juris Galvanovskis and Patrik Rorsman
SummaryExocytosis of secretory vesicles begins with a fusion pore connecting the vesicle lumen to the extracellular space. This pore may then expand or it may close to recapture the vesicle intact. The contribution of the latter, termed kiss-and-run, to exocytosis of pancreatic β cell large dense-core vesicles (LDCVs) is controversial. Examination of single vesicle fusion pores demonstrated that rat β cell LDCVs can undergo exocytosis by rapid pore expansion, by the formation of stable pores, or via small transient kiss-and-run fusion pores. Elevation of cAMP shifted LDCV fusion pore openings to the transient mode. Under this condition, the small fusion pores were sufficient for release of ATP, stored within LDCVs together with insulin. Individual ATP release events occurred coincident with amperometric “stand alone feet” representing kiss-and-run. Therefore, the LDCV kiss-and-run fusion pores allow small transmitter release but likely retain the larger insulin peptide. This may represent a mechanism for selective intraislet signaling.
Summary | Full Text | PDF (442 kb) - …more
Copyright © 1996 The Biophysical Society. All rights reserved.
Biophysical Journal, Volume 71, Issue 2, 1131-1139, 1 August 1996
doi:10.1016/S0006-3495(96)79315-3
Research Article
Simultaneous capacitance and amperometric measurements of exocytosis: a comparison
A.F. Oberhauser, I.M. Robinson and J.M. Fernandez
Department of Physiology and Biophysics, Mayo Clinic, Rochester, Minnesota 55905, USA.
Abstract
We measured the exocytotic response induced by flash photolysis of caged compounds in isolated mast cells and chromaffin cells. Vesicle fusion was measured by monitoring the cell membrane capacitance. The release of vesicular contents was followed by amperometry. In response to a GTP gamma S stimulus we found that the time integral of the amperometric current could be superimposed on the capacitance trace. This shows that the integrated amperometric signal provides an alternative method of measuring the extent and kinetics of the secretory response. Very different results were obtained when photolysis of caged Ca2+ (DM-nitrophen) was used to stimulate secretion. In mast cells, there was an immediate, graded increase in membrane capacitance that was followed by step increases (indicative of granule fusion). During the initial phase of the capacitance increases, no release of oxidizable secretory products was detected. In chromaffin cells we also observed a considerable delay between increases in capacitance, triggered by uncaging Ca2+, and the release of oxidizable secretory products. Here we demonstrate that there can be large increases in the membrane capacitance of a secretory cell, triggered by flash photolysis of DM-nitrophen, which indicate events that are not due to the fusion of granules containing oxidizable substances. These results show that increases in capacitance that are not resolved as steps cannot be readily interpreted as secretory events unless they are confirmed independently.
