TROPHIC INTERACTIONS DURING VISUAL SYSTEM DEVELOPMENT
Project Number5R01EY011912-02
Contact PI/Project LeaderCOHEN-CORY, SUSANA
Awardee OrganizationUNIVERSITY OF CALIFORNIA LOS ANGELES
Description
Abstract Text
DESCRIPTION: (Adapted From The Applicant's Abstract) The proposed
studies will examine the mechanisms by which retinal projection neurons
make precise and functional connections with their central targets. The
hypothesis that neuronal activity and neurotrophic factors interact
synergistically to modulate axon terminal arborization, as well as
synapse formation and stabilization will be tested in the live
developing brain. Specifically, the roles and interactions between
neurotrophins, and pre- and post-synaptic activity during the dynamic
elaboration of optic axon terminal arbors and formation of synaptic
contracts will be examined in live, anesthetized tadpoles. The Xenopus
laevis visual system is a uniquely accessible vertebrate model in which
the development of neuronal connections between retinal ganglion cells
and their tecta target neurons can be followed over time in the intact
embryo. The mechanisms controlling axon growth, arborization, and
complexity will be studied in connections with target neurons. Growth
and arborization patterns of individual, fluorescently labeled retinal
ganglion cell axons will be followed over time using low-light level
video microscopy and laser scanning confocal microscopy. The
interactions between neurotrophins and pre- and post-synaptic neuronal
activity in the dynamics of axon arborization (axon branch addition and
withdrawal) and the final complexity of axonal arbors will be examined
by perturbing endogenous neurotrophic factor levels and the activity
patterns of projection or target neurons. Neurotrophic factor levels
will be altered by direct microinjection of neurotrophins, function-
blocking antibodies, or control solutions into the tecta of live,
anesthetized tadpoles. The contributions of neuronal activity to the
dynamics of axon arborization and refinement will be tested by
selectively altering pre- or post-synaptic activity by direct
microinjection of pharmacological agents into the retina (sodium channel
blocks) or rectum (glutamate receptor agonists or antagonists) of the
anesthetized tadpole. A combination of in vivo microscopic imaging of
individual retinal ganglion cell axon arbors, and targeted expression
and in vivo imaging of chimeric, fluorescently labeled synaptic proteins
will be used to determine the correlates between axon morphology and
synaptic structure. This will provide simultaneous, single cell
observation of axon arborization dynamics and refinement, and synapse
formation and stabilization. The roles of activity and neurotrophic
signals during synapse formation and stabilization will be examined by
combining pharmacologic perturbations of neurotrophic factor levels and
activity signaling with simultaneous in vivo imaging of axonal arbors
and synaptic proteins. The results of these studies will provide
valuable insights into fundamental mechanisms of synaptogenesis in the
living brain, and will further our understanding of the mechanisms that
control the development of regeneration of the visual pathways, that are
critically important in the maintenance of normal visual function.
No Sub Projects information available for 5R01EY011912-02
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