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The Journal of Neurophysiology Vol. 83 No. 1 January 2000, pp. 552-562
Copyright ©2000 by the American Physiological Society
Department of Biology, Boston University, Boston, Massachusetts 02215
Vyshedskiy, Andrey and
Jen-Wei Lin.
Presynaptic Ca2+ Influx at the Inhibitor of the
Crayfish Neuromuscular Junction: A Photometric Study at a High Time
Resolution. J. Neurophysiol. 83: 552-562, 2000. Presynaptic calcium influx at the inhibitor
of the crayfish neuromuscular junction was investigated by measuring
fluorescence transients generated by calcium-sensitive dyes. This
approach allowed us to correlate presynaptic calcium influx with
transmitter release at a high time resolution. Systematic testing of
the calcium indicators showed that only low-affinity dyes, with
affinities in the range of micromolar, should be used to avoid
saturation of dye binding and interference with transmitter release.
Presynaptic calcium influx was regulated by slowly increasing the
duration of the action potential through progressive block of potassium channels. The amplitude of the calcium transient, measured from a
cluster of varicosities, was linearly related to the duration of the
action potential with a slope of 1.2. Gradual changes in potassium
channel block allowed us to estimate the calcium cooperativity of
transmitter release over a 10-fold range in presynaptic calcium influx.
Calcium cooperativity measured here exhibited one component with an
average value of 3.1. Inspection of simultaneously recorded presynaptic
calcium transients and inhibitory postsynaptic currents (IPSCs) showed
that prolonged action potentials were associated with a slow rising
phase of presynaptic calcium transients, which were matched by a slow
rate of rise of IPSCs. The close correlation suggests that fluorescence
transients provide information on the rate of calcium influx. Because
there is an anatomic mismatch between the presynaptic calcium
transient, measured from a cluster of varicosities, and IPSC, measured
with two-electrode voltage clamp, macropatch recording was used to
monitor inhibitory postsynaptic responses from the same cluster of
varicosities from which the calcium transient was measured. Inhibitory
postsynaptic responses recorded with the macropatch method exhibited a
faster rising phase than that recorded with two-electrode voltage
clamp. This difference could be attributed to slight asynchrony of
transmitter release due to action potential conduction along fine
branches. In conclusion, this report shows that fluorescence transients generated by calcium-sensitive dyes can provide insights to the properties of presynaptic calcium influx, and its correlation with
transmitter release, at a high time resolution.
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