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The Journal of Neurophysiology Vol. 84 No. 3 September 2000, pp. 1247-1255
Copyright ©2000 by the American Physiological Society
Department of Biology, McGill University, Montreal, Quebec H3A 1B1, Canada
Faulkes, Zen and
Gerald S. Pollack.
Effects of Inhibitory Timing on Contrast Enhancement in Auditory
Circuits in Crickets (Teleogryllus oceanicus). J. Neurophysiol. 84: 1247-1255, 2000. In
crickets (Teleogryllus oceanicus), the paired auditory
interneuron Omega Neuron 1 (ON1) responds to sounds with frequencies in
the range from 3 to 40 kHz. The neuron is tuned to frequencies similar to that of conspecific songs (4.5 kHz), but its latency is
longest for these same frequencies by a margin of 5-10 ms. Each ON1 is
strongly excited by input from the ipsilateral ear and inhibits
contralateral auditory neurons that are excited by the contralateral
ear, including the interneurons ascending neurons 1 and 2 (AN1 and
AN2). We investigated the functional consequences of ON1's long
latency to cricket-like sound and the resulting delay in inhibition of
AN1 and AN2. Using dichotic stimuli, we controlled the timing of
contralateral inhibition of the ANs relative to their excitation by
ipsilateral stimuli. Advancing the stimulus to the ear driving ON1
relative to that driving the ANs "subtracted" ON1's additional
latency to 4.5 kHz. This had little effect on the spike counts of AN1
and AN2. The response latencies of these neurons, however, increased
markedly. This is because in the absence of a delay in ON1's response,
inhibition arrived at AN1 and AN2 early enough to abolish the first
spikes in their responses. This also increased the variability of AN1
latency. This suggests that one possible function of the delay in
ON1's response may be to protect the precise timing of the onset of
response in the contralateral AN1, thus preserving interaural
difference in response latency as a reliable potential cue for sound
localization. Hyperpolarizing ON1 removed all detectable contralateral
inhibition of AN1 and AN2, suggesting that ON1 is the main, if not the
only, source of contralateral inhibition.
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