Abstract

The major aim of this research is to elucidate cellular and molecular interactions governing the formation of precise sets of connections during mammalian visual system development. Research is centered on how connections between the lateral geniculate nucleus (LGN) and primary visual cortex are established during fetal development and during the postnatal critical period for t he effects of visual experience. Three interrelated specific aims address the central hypothesis that precise adult connections arise as a consequence of circuit readjustment in primary visual cortex driven by dynamic interactions between neural activity and gene expression. 1. To determine the sign of synaptic input from subplate to layer 4. The hypothesis that subplate neurons, along with LGN axons, regulate cortical activity and during the critical period will be addressed. Ablation of subplate neurons prevents formation of ocular dominance columns (ODCs) and alters the expression of genes considered to be key regulators of synaptic plasticity. Experiments will identify and characterize subplate inputs to cortex using electrophysiological, anatomical and calcium imaging approaches. 2. To determine the functional contribution of subplate neurons to formation to formation and maturation of thalamocortical connections. Experiments will acutely or chronically eliminate subplate neurons prematurely, or alter their excitability, to examine the consequences for ensuing development of ODCs and cortical circuits. These manipulations exploit the fact that subplate neurons have distinct physiological and molecular phenotypes that permit their selective inactivation, activation, or removal. 3. To identify sets of genes expressed by cortical neurons and regulated by retinal activity. These experiments address the hypothesis that there is a dynamic and reciprocal relationship between neural activity and the expression of genes required for synaptic readjustments leading to the final patterning of connections. Candidate genes will be identified via unbiased differential screens for activity-regulated genes expressed in visual cortex during the critical period. Preliminary results using cDNA microarrays have identified a set of 50 candidates-both known and novel. Experiments to extend findings, and to test candidate gene function are proposed. Collectively, these experiments should contribute to a framework for constructing a molecular understanding of the critical period in visual system development. Results should also add to knowledge of mechanisms of normal development and learning in children, and to an understanding of causes of developmental and neurological disorders such as Dyslexia, Cerebral Palsy and Autism.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Research Project (R01)
Project #
3R01EY002858-25S1
Application #
6588968
Study Section
Visual Sciences B Study Section (VISB)
Program Officer
Oberdorfer, Michael
Project Start
1979-01-01
Project End
2006-12-31
Budget Start
2002-01-01
Budget End
2002-12-31
Support Year
25
Fiscal Year
2002
Total Cost
$400,000
Indirect Cost

  Institution

Name
Harvard University
Department
Biology
Type
Schools of Medicine
DUNS #
082359691
City
Boston
State
MA
Country
United States
Zip Code
02115

  Publications

Nguyen-Vu, Td Barbara; Zhao, Grace Q; Lahiri, Subhaneil et al. (2017) A saturation hypothesis to explain both enhanced and impaired learning with enhanced plasticity. Elife 6:
Vidal, George S; Djurisic, Maja; Brown, Kiana et al. (2016) Cell-Autonomous Regulation of Dendritic Spine Density by PirB. eNeuro 3:
Adelson, Jaimie D; Sapp, Richard W; Brott, Barbara K et al. (2016) Developmental Sculpting of Intracortical Circuits by MHC Class I H2-Db and H2-Kb. Cereb Cortex 26:1453-1463
Bochner, David N; Sapp, Richard W; Adelson, Jaimie D et al. (2014) Blocking PirB up-regulates spines and functional synapses to unlock visual cortical plasticity and facilitate recovery from amblyopia. Sci Transl Med 6:258ra140
Lee, Hanmi; Brott, Barbara K; Kirkby, Lowry A et al. (2014) Synapse elimination and learning rules co-regulated by MHC class I H2-Db. Nature 509:195-200
Djurisic, Maja; Vidal, George S; Mann, Miriam et al. (2013) PirB regulates a structural substrate for cortical plasticity. Proc Natl Acad Sci U S A 110:20771-6
Kim, Taeho; Vidal, George S; Djurisic, Maja et al. (2013) Human LilrB2 is a ?-amyloid receptor and its murine homolog PirB regulates synaptic plasticity in an Alzheimer's model. Science 341:1399-404
Adelson, Jaimie D; Barreto, George E; Xu, Lijun et al. (2012) Neuroprotection from stroke in the absence of MHCI or PirB. Neuron 73:1100-7
William, Christopher M; Andermann, Mark L; Goldey, Glenn J et al. (2012) Synaptic plasticity defect following visual deprivation in Alzheimer's disease model transgenic mice. J Neurosci 32:8004-11
Datwani, Akash; McConnell, Michael J; Kanold, Patrick O et al. (2009) Classical MHCI molecules regulate retinogeniculate refinement and limit ocular dominance plasticity. Neuron 64:463-70

Showing the most recent 10 out of 73 publications