Abstract

Spiny neurons throughout the nervous system have thornlike protuberances arising from their dendrites. These dendritic spines are a site of asymmetric excitatory inputs to the neurons. Spine shape is thought to affect the efficacy of the synaptic input. The focus of this proposal will be to study the ultrastructure of dendritic spines on three different types of spiny neurons. The major emphasis will be on the pyramidal cells of area CA1 in the rat hippocampus. Comparison measurements will be made on granule cells of area dentata of the same hippocampus, and on cerebellar Purkinje cells of the same brain. I will use computer-assisted methods to reconstruct dendritic spines from serial electron micrographs. Then measurements of spine length, neck diameter, surface area and volume will be made. Synaptic surface area, the volume of spine cisternae and the diameter of the parent dendrite will also be measured. Then these measures will be used in computer programs that model how relationships among these structural features might affect synaptic efficacy. Ultrastructural studies of dendritic spines suggest that their necks shorten and widen following high frequency afferent activation. This structural change should increase the efficacy of synapses terminating on the spine by decreasing the resistance to synaptic current flow through the spine neck to the dendrite. In the hippocampus, high frequency stimulation of afferent input results in a long-lasting incrase in the physiological response of the postsynaptic cell. This change in response is referred to as long-term potentiation (LTP) and represents a candidate mechanism for information storage. In area CA1 of the rat hippocampus, the magnitude of LTP produced is about three times greater at postnatal day 15 than in the adult (Harris and Teyler, In Press). Spines will be studied to determine whether changes in there ultrastructure during development would account for this age related difference in LTP magnitude. In addition, LTP will be induced in the apical dendritic field of area CA1 in hippocampal slices at days 15 and 60. Spines in the vicinity of stimulation will be reconstructed and measured. Comparison measurements will be made on spines in the basillar dendritic field of the same slice, and on apical spines of non-potentiated slices. In order to unambiguously identify spines that contact stimulated axons, these axons will be filled with horse-radish peroxidase following the induction of LTP.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Unknown (R23)
Project #
5R23NS021184-02
Application #
3449744
Study Section
Neurology B Subcommittee 1 (NEUB)
Project Start
1984-07-01
Project End
1987-08-31
Budget Start
1985-09-01
Budget End
1986-08-31
Support Year
2
Fiscal Year
1985
Total Cost
Indirect Cost

  Institution

Name
Children's Hospital Boston
Department
Type
DUNS #
076593722
City
Boston
State
MA
Country
United States
Zip Code

  Publications

Harris, Kristen M; Spacek, Josef; Bell, Maria Elizabeth et al. (2015) A resource from 3D electron microscopy of hippocampal neuropil for user training and tool development. Sci Data 2:150046
Bartol, Thomas M; Bromer, Cailey; Kinney, Justin et al. (2015) Nanoconnectomic upper bound on the variability of synaptic plasticity. Elife 4:e10778
Cao, Guan; Harris, Kristen M (2014) Augmenting saturated LTP by broadly spaced episodes of theta-burst stimulation in hippocampal area CA1 of adult rats and mice. J Neurophysiol 112:1916-24
Bell, Maria Elizabeth; Bourne, Jennifer N; Chirillo, Michael A et al. (2014) Dynamics of nascent and active zone ultrastructure as synapses enlarge during long-term potentiation in mature hippocampus. J Comp Neurol 522:3861-84
Edwards, John; Daniel, Eric; Kinney, Justin et al. (2014) VolRoverN: enhancing surface and volumetric reconstruction for realistic dynamical simulation of cellular and subcellular function. Neuroinformatics 12:277-89
Kuwajima, Masaaki; Mendenhall, John M; Harris, Kristen M (2013) Large-volume reconstruction of brain tissue from high-resolution serial section images acquired by SEM-based scanning transmission electron microscopy. Methods Mol Biol 950:253-73
Kinney, Justin P; Spacek, Josef; Bartol, Thomas M et al. (2013) Extracellular sheets and tunnels modulate glutamate diffusion in hippocampal neuropil. J Comp Neurol 521:448-64
Bourne, Jennifer N; Chirillo, Michael A; Harris, Kristen M (2013) Presynaptic ultrastructural plasticity along CA3?CA1 axons during long-term potentiation in mature hippocampus. J Comp Neurol 521:3898-912
Kuwajima, M; Spacek, J; Harris, K M (2013) Beyond counts and shapes: studying pathology of dendritic spines in the context of the surrounding neuropil through serial section electron microscopy. Neuroscience 251:75-89
Kuwajima, Masaaki; Mendenhall, John M; Lindsey, Laurence F et al. (2013) Automated transmission-mode scanning electron microscopy (tSEM) for large volume analysis at nanoscale resolution. PLoS One 8:e59573

Showing the most recent 10 out of 19 publications