One of the most remarkable features of the nervous system is its capacity to undergo experience- dependent rewiring. Synaptic plasticity, the change in the number and efficacy of synaptic connections with experience, provides the basis for memory formation and storage in the brain. Long-lasting plasticity, such as that underlying long-term memory, requires new gene expression. Investigating how synaptically generated signals are transported from stimulated synapses to the nucleus to regulate transcription, the Martin lab previously uncovered a role for the synapse to nuclear transport of the transcriptional regulator CRTC1 (Ch'ng et al. 2012), a co-activator and regulator of CREB-dependent transcription. CRTC1 activity is regulated by desphosphorylation, with phosphorylated CRTC1 being cytoplasmically localized and dephosphorylated CRTC1 localizing to the nucleus. Thus, CRTC1 is anchored at synapses in unstimulated neurons, but undergoes rapid translocation to the nucleus in response to glutamatergic stimulation. In the nucleus, CRTC1 regulates the expression of CREB target genes. A striking finding that emerged from our studies was that CRTC1 underwent dramatic and complex changes in phosphorylation following neuronal stimulation. Initial mass spectrometric analyses revealed 50 amino acid residues in CRTC1 that are phosphorylated in the neuroblastoma N2a cell line. My fellowship research project aims to map the residues that undergo regulated dephosphorylation during long-term plasticity in mouse hippocampal neurons. As models of plasticity, I will study long-term potentiation (LTP) and long-term depression (LTD) of acute mouse hippocampal slices. My experiments test the hypothesis that distinct patterns of activity trigger distinct changes in the pattern of CRTC1 phosphorylation and that the differentially phosphorylated forms of CRTC1 regulate distinct programs of gene expression. In this way, the post-translational modification of CRTC1 can encode patterns of stimulation to produce appropriate changes in gene expression. To test this hypothesis, I propose two aims. In the first, I determine how LTP and LTD inducing stimuli alter the phosphorylation of CRTC1. In the second, I determine how these stimuli regulate the interaction of CRTC1 with specific transcription factors and how these complexes regulate downstream gene expression.

Public Health Relevance

Long-term memory requires new gene expression in neurons. This proposal focuses on the molecule CRTC1, which has been shown to travel from stimulated synapses to the nucleus to regulate gene expression during memory formation, and tests the hypothesis that activity-dependent modifications of CRTC1 control the specificity of gene expression. The results of the studies will elucidate the biology underlying many neuropsychiatric disorders.

Agency
National Institute of Health (NIH)
Institute
National Institute of Mental Health (NIMH)
Type
Predoctoral Individual National Research Service Award (F31)
Project #
1F31MH107210-01
Application #
8910152
Study Section
Special Emphasis Panel (ZRG1)
Program Officer
Driscoll, Jamie
Project Start
2015-04-01
Project End
2018-03-31
Budget Start
2015-04-01
Budget End
2016-03-31
Support Year
1
Fiscal Year
2015
Total Cost
Indirect Cost
Name
University of California Los Angeles
Department
Biochemistry
Type
Schools of Medicine
DUNS #
092530369
City
Los Angeles
State
CA
Country
United States
Zip Code
90095
Octeau, J Christopher; Chai, Hua; Jiang, Ruotian et al. (2018) An Optical Neuron-Astrocyte Proximity Assay at Synaptic Distance Scales. Neuron 98:49-66.e9