Abstract

The HVEM has remarkable potential as an instrument which will allow a correlation of morphology with physiology and function. This potential has not been fully realized in the mammalian central nervous system, principally because the necessary techniques have not been systematically developed. This work will develop both specimen preparation and instrumentation needed to combine the power of both methods. Specimen preparation methods will be developed to localize sites on single mammalian CNS neurons at which neurologic, pharmacologic or toxic agents have been applied. These methods will identify a volume of tissue for detailed study by serial thick sections in the HVEM. The deposition of collodial gold or fluorescent markers by means of a microelectrode at the site under physiologic study will identify the volume of tissue during sectioning. Since 0.25 or 0.5 Mum sections will be used, the site under study will be encompassed within a limited number of serial sections. Nearby areas on the same or different neurons will be observed as controls. Instrumentation will be developed to provide elemental analysis and enhanced contrast imaging of unstained specimens. First, our X-ray detector will be used to analyze tissue in which high levels of Ca have been manipulated. Second, a simple electron energy loss spectrometer (EELS) will be used to improve detection. These methods if adequately developed, will allow a variety of types of investigation directed at critical questions related to morphology and function in the mammalian central nervous system, such as 1) Determination of sites of action of transmitter (i.e. soma vs dendrites) and induced local morphological changes on single central neurons. 2) Determination of site of generation of field on synaptic potentials on a single neuron, with correlation with synaptic inputs. 3) Determination of relation of postsynaptic interval membraneous specialization relative to synaptic inputs, and their ultrastructure. 4) Local effects induced by discrete actions of toxins. 5) The morphological characterization of areas of subcellular localization of elements, particularly metals such as Ca++, Zn++, and Al+++ in neuronal and pathological tissues.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Center for Research Resources (NCRR)
Type
Resource-Related Research Projects (R24)
Project #
1R24RR002984-01
Application #
3450724
Study Section
(SSS)
Project Start
1987-09-30
Project End
1990-09-29
Budget Start
1987-09-30
Budget End
1988-09-29
Support Year
1
Fiscal Year
1987
Total Cost
Indirect Cost

  Institution

Name
Wadsworth Center
Department
Type
DUNS #
110521739
City
Menands
State
NY
Country
United States
Zip Code
12204

  Publications

Stewart, Joanna D; Horvath, Rita; Baruffini, Enrico et al. (2010) Polymerase ? gene POLG determines the risk of sodium valproate-induced liver toxicity. Hepatology 52:1791-6
Turner, J N; Swann, J W; Szarowski, D H et al. (1996) Three-dimensional confocal light and electron microscopy of central nervous system tissue and neurons and glia in culture. Int Rev Exp Pathol 36:53-72
Smith, K L; Szarowski, D H; Turner, J N et al. (1995) Diverse neuronal populations mediate local circuit excitation in area CA3 of developing hippocampus. J Neurophysiol 74:650-72
Smith, K L; Turner, J N; Szarowski, D H et al. (1994) Localizing sites of intradendritic electrophysiological recordings by confocal light microscopy. Microsc Res Tech 29:310-8
Turner, J N; Swann, J W; Szarowski, D H et al. (1993) Three-dimensional confocal light microscopy of neurons: fluorescent and reflection stains. Methods Cell Biol 38:345-66
Shain, W; Bausback, D; Fiero, A et al. (1992) Regulation of receptor-mediated shape change in astroglial cells. Glia 5:223-38
Smith, K L; Turner, J N; Szarowski, D H et al. (1991) Three-dimensional imaging of neurophysiologically characterized hippocampal neurons by confocal scanning laser microscopy. Ann N Y Acad Sci 627:390-4
Turner, J N; Szarowski, D H; Smith, K L et al. (1991) Confocal microscopy and three-dimensional reconstruction of electrophysiologically identified neurons in thick brain slices. J Electron Microsc Tech 18:11-23
Deitch, J S; Smith, K L; Swann, J W et al. (1991) Ultrastructural investigation of neurons identified and localized using the confocal scanning laser microscope. J Electron Microsc Tech 18:82-90
Deitch, J S; Smith, K L; Swann, J W et al. (1990) Parameters affecting imaging of the horseradish-peroxidase-diaminobenzidine reaction product in the confocal scanning laser microscope. J Microsc 160:265-78

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