The formation of specific chemical synapses during development involves a multistep process that includes a) neurogenesis of the specific presynaptic and postsynaptic populations, b) axonogenesis and guidance of axons towards the appropriate target region, c) target recognition and formation of synapses with appropriate cells within the target region, and d) fine tuning the number and distribution of synapses by activity- dependent stabilization/elimination of specific connections. Local inductive interactions via diffusible factors and/or the selective expression of cell surface or extracellular matrix molecules facilitate each step in this process. One member of the immunoglobulin-like family of cell adhesion molecules, NCAM, appears to play important roles at several stages in development. The major objective of this proposal is to study the role of different isoforms of a recently characterized member of the NCAM-like family of cell adhesion molecules in the formation and stabilization of specific chemical synapses using an in vitro model system consisting of identified neurons isolated from the ganglia of the marine mollusk Aplysia californica. Individual Aplysia neurons in cell culture reliably form stable chemical connections. Some cells appear to form connections only with their appropriate targets while others are more permissive and form connections indiscriminately. Manipulating the level of expression of these NCAM-like molecules, called apCAM, on the surface of the cells can significantly influence the pattern of outgrowth and synapse formation. The proposed studies will combine electrophysiological methods for detecting the presence and modulation of chemical connections and for intracellular injection of pharmacological agents, with a variety of light microscope techniques to monitor live growth cone behavior and to detect by immunofluorescent methods the distribution or level of expression of different isoforms of apCAM, synapse-specific antigens, cytoskeletal elements and kinase activities, and with electron microscope techniques for characterizing newly formed transmitter release sites.
The specific aims of the proposal are to test the hypotheses: 1) Synapse formation is initiated when a presynaptic growth cone slows upon contact of apCAM 'hot spot' on the surface of the postsynaptic cell and is mediated by the activation of presynaptic protein kinase C. 2) Synapse stabilization involves asymmetric distribution of apCAM isoforms such that transmembrane forms are concentrated on the postsynaptic surface and GPI- linked forms are concentrated on the presynaptic surface. 3) Local modulation of apCAM isoforms on presynaptic or postsynaptic membrane is critical for local cell- and site-specific changes in the number of synaptic contacts. 4) Branch-specific target contact influences cellular changes at other branches of the same cell via signals first triggered by apCAM-apCAM interaction. These studies will begin to identify the critical cellular and molecular events during the formation of synapses that permit neurons to establish mature neural circuits that control normal behavior.

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
5R01NS027541-10
Application #
2714480
Study Section
Neurology B Subcommittee 2 (NEUB)
Program Officer
Chiu, Arlene Y
Project Start
1989-08-01
Project End
1999-05-31
Budget Start
1998-06-01
Budget End
1999-05-31
Support Year
10
Fiscal Year
1998
Total Cost
Indirect Cost
Name
New York State Psychiatric Institute
Department
Type
DUNS #
167204994
City
New York
State
NY
Country
United States
Zip Code
10032
Conrad, P; Wu, F; Schacher, S (1999) Changes in functional glutamate receptors on a postsynaptic neuron accompany formation and maturation of an identified synapse. J Neurobiol 39:237-48
Schacher, S; Wu, F; Panyko, J D et al. (1999) Expression and branch-specific export of mRNA are regulated by synapse formation and interaction with specific postsynaptic targets. J Neurosci 19:6338-47
Hatada, Y; Wu, F; Silverman, R et al. (1999) En passant synaptic varicosities form directly from growth cones by transient cessation of growth cone advance but not of actin-based motility. J Neurobiol 41:242-51
Zhu, H; Wu, F; Schacher, S (1997) Site-specific and sensory neuron-dependent increases in postsynaptic glutamate sensitivity accompany serotonin-induced long-term facilitation at Aplysia sensorimotor synapses. J Neurosci 17:4976-86
Sun, Z Y; Kauderer, B; Schacher, S (1996) Differential distribution of functional receptors for neuromodulators evoking short-term heterosynaptic plasticity in Aplysia sensory neurons. J Neurosci 16:7540-9
Sun, Z Y; Schacher, S (1996) Tetanic stimulation and cyclic adenosine monophosphate regulate segregation of presynaptic inputs on a common postsynaptic target neuron in vitro. J Neurobiol 29:183-201
Sun, Z Y; Schacher, S (1996) Development of short-term heterosynaptic facilitation at aplysia sensorimotor synapses in vitro is accompanied by changes in the functional expression of presynaptic serotonin receptors. J Neurophysiol 76:2250-61
Zhu, H; Wu, F; Schacher, S (1995) Changes in expression and distribution of Aplysia cell adhesion molecules can influence synapse formation and elimination in vitro. J Neurosci 15:4173-83
Wu, F; Friedman, L; Schacher, S (1995) Transient versus persistent functional and structural changes associated with facilitation of Aplysia sensorimotor synapses are second messenger dependent. J Neurosci 15:7517-27
Peter, N; Aronoff, B; Wu, F et al. (1994) Decrease in growth cone-neurite fasciculation by sensory or motor cells in vitro accompanies downregulation of Aplysia cell adhesion molecules by neurotransmitters. J Neurosci 14:1413-21

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