Author:
WINKLER BARRY S.,KAPOUSTA-BRUNEAU NATALIA,ARNOLD MATTHEW J.,GREEN DANIEL G.
Abstract
The purpose of the present experiments was to evaluate
the contribution of the glutamate-glutamine cycle in retinal
glial (Müller) cells to photoreceptor cell synaptic
transmission. Dark-adapted isolated rat retinas were superfused
with oxygenated bicarbonate-buffered media. Recordings
were made of the b-wave of the electroretinogram
as a measure of light-induced photoreceptor to ON-bipolar
neuron transmission. L-methionine sulfoximine (1–10
mM) was added to superfusion media to inhibit glutamine
synthetase, a Müller cell specific enzyme, by more
than 99% within 5–10 min, thereby disrupting the
conversion of glutamate to glutamine in the Müller
cells. Threo-hydroxyaspartic acid and D-aspartate were
used to block glutamate transporters. The amplitude of
the b-wave was well maintained for 1–2 h
provided 0.25 mM glutamate or 0.25 mM glutamine was included
in the media. Without exogenous glutamate or glutamine
the amplitude of the b-wave declined by about
70% within 1 h. Inhibition of glutamate transporters led
to a rapid (2–5 min) reversible loss of the b-wave
in the presence and absence of the amino acids. In contrast,
inhibition of glutamine synthetase did not alter significantly
either the amplitude of the b-wave in the presence
of glutamate or glutamine or the rate of decline of the
b-wave found in the absence of these amino acids.
Excellent recovery of the b-wave was found when
0.25 mM glutamate was resupplied to L-methionine sulfoximine–treated
retinas. The results suggest that in the isolated rat retina
uptake of released glutamate into photoreceptors plays
a more important role in transmitter recycling than does
uptake of glutamate into Müller cells and its subsequent
conversion to glutamine.
Publisher
Cambridge University Press (CUP)
Subject
Sensory Systems,Physiology
Cited by
49 articles.
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