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The Journal of Neurophysiology Vol. 81 No. 2 February 1999, pp. 895-907
Copyright ©1999 by the American Physiological Society
Cold Spring Harbor Laboratory, Cold Spring Harbor, New York 11724
Light-induced calcium influx into retinal axons is regulated by
presynaptic nicotinic acetylcholine receptor activity in vivo. Visual activity is thought to be a critical factor in controlling the
development of central retinal projections. Neuronal activity increases
cytosolic calcium, which was hypothesized to regulate process outgrowth
in neurons. We performed an in vivo imaging study in the retinotectal
system of albino Xenopus laevis tadpoles with the
fluorescent calcium indicator calcium green 1 dextran (CaGD) to test
the role of calcium in regulating axon arbor development. We find that
visual stimulus to the retina increased CaGD fluorescence intensity in
retinal ganglion cell (RGC) axon arbors within the optic tectum and
that branch additions to retinotectal axon arbors correlated with a
local rise in calcium in the parent branch. We find three types of
responses to visual stimulus, which roughly correlate with the
ON, OFF, and SUSTAINED response types of RGC reported by physiological criteria. Imaging in bandscan mode indicated that patterns of calcium transients were nonuniform throughout the
axons. We tested whether the increase in calcium in the retinotectal axons required synaptic activity in the retina; intraocular application of tetrodotoxin (10 µM) or nifedipine (1 and 10 µM) blocked the stimulus-induced increase in RGC axonal fluorescence. A second series
of pharmacological investigations was designed to determine the
mechanism of the calcium elevation in the axon terminals within the
optic tectum. Injection of
bis-(o-aminophenoxy)-N,N,N',N'-tetraacetic acid-AM (BAPTA-AM) (20 mM) into the tectal ventricle reduced axonal calcium levels, supporting the idea that visual stimulation increases axonal calcium. Injection of BAPTA (20 mM) into the tectal ventricle to
chelate extracellular calcium also attenuated the calcium response to
visual stimulation, indicating that calcium enters the axon from the
extracellular medium. Caffeine (10 mM) caused a large increase in
axonal calcium, indicating that intracellular stores contribute to the
calcium signal. Presynaptic nicotinic acetylcholine receptors (nAChRs)
may play a role in axon arbor development and the formation of the
topographic retinotectal projection. Injection of nicotine (10 µM)
into the tectal ventricle significantly elevated RGC axonal calcium
levels, whereas application of the nAChR antagonist
BTX (100 nM)
reduced the stimulus-evoked rise in RGC calcium fluorescence. These
data suggest that light stimulus to the retina increases calcium in the
axon terminal arbors through a mechanism that includes influx through
nAChRs and amplification by calcium-induced calcium release from
intracellular calcium stores. Such a mechanism may contribute to
developmental plasticity of the retinotectal system by influencing both
axon arbor elaboration and the strength of synaptic
transmission.
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