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The Journal of Neurophysiology Vol. 87 No. 1 January 2002, pp. 15-29
Copyright ©2002 by the American Physiological Society
1Department of Neuroscience and Center for the Neural Basis of Cognition, University of Pittsburgh, Pittsburgh, Pennsylvania 15260; and 2Program in Neuroscience and Department of Biology, Boston University, Boston, Massachusetts 02215
Henze, Darrell A.,
David B. T. McMahon,
Kristen M. Harris, and
German Barrionuevo.
Giant Miniature EPSCs at the Hippocampal Mossy Fiber to CA3
Pyramidal Cell Synapse Are Monoquantal. J. Neurophysiol. 87: 15-29, 2002. The mechanisms generating giant
miniature excitatory postsynaptic currents (mEPSCs) were investigated
at the hippocampal mossy fiber (MF) to CA3 pyramidal cell synapse in
vitro. These giant mEPSCs have peak amplitudes as large as 1,700 pA
(13.6 nS) with a mean maximal mEPSC amplitude of 366 ± 20 pA
(mean ± SD; 5 nS; n = 25 cells). This is
compared with maximal mEPSC amplitudes of <100 pA typically observed
at other cortical synapses. We tested the hypothesis that giant mEPSCs
are due to synchronized release of multiple vesicles across the release
sites of single MF boutons by directly inducing vesicular release using
secretagogues. If giant mEPSCs result from simultaneous multivesicular
release, then secretagogues should increase the frequency of small
mEPSCs selectively. We found that hypertonic sucrose and spermine
increased the frequency of both small and giant mEPSCs. The peptide
toxin secretagogues alpha-latrotoxin and pardaxin failed to increase the frequency of giant mEPSCs, but the possible lack of tissue penetration of the toxins make these results equivocal. Because a
multiquantal release mechanism is likely to be mediated by a spontaneous increase in presynaptic calcium concentration, a
monoquantal mechanism is further supported by results that giant mEPSCs
were not affected by manipulations of extracellular or intracellular calcium concentrations. In addition, reducing the temperature of the
bath to 15°C failed to desynchronize the rising phases of giant
mEPSCs. Together these data suggest that the giant mEPSCs are generated
via a monovesicular mechanism. Three-dimensional analysis through
serial electron microscopy of the MF boutons revealed large clear
vesicles (50 to 160 nm diam) docked presynaptically at the MF synapse
in sufficient numbers to account for the amplitude and frequency of
giant mEPSCs recorded electrophysiologically. It is concluded that
release of the contents of a single large clear vesicle generates giant
mEPSCs at the MF to CA3 pyramidal cell synapse.
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