The objective is to develop methodologies for the detection and observation of protein association in a single living cell using a time-resolved microluminescence spectrophotometer (= time-resolved microfluorescence and microphosphorescence spectrophotometer), and at the same time to establish time resolved microluminometry as a useful tool for biomedical research and medical diagnosis. The key idea is combination of the spotting capability of the microscope optics and time-resolved (real time) fluorescence or phosphorescence spectrophotometric measurements on the spot, i.e., we select a structure of our interest under the fluorescence microscope and obtain molecular information on that structure using spectroscopic means. We emphasize the time-resolved techniques because of the wealth of information and because the characteristic time (e.g. excited-state lifetime) is often the only quantitative parameter whose absolute value can be measured under the microscope. We already have almost all necessary equipment and we will concentrate our effort on methodological development for detection of membrane protein association in a single cell during the proposed project period. Our strategies for development and systematic evaluation of time-resolved microluminometric methods include [A] use of rhodopsin in reconstituted membranes and rod outer segment membranes as model samples, [B] comparison of results obtained by microspectroscopic methods with those obtained by usual (macroscopic) spectroscopic methods, [C] measurement of time-dependent depolarization of phosphorescence and delayed fluorescence for observation of rotational diffusion, which is very sensitive to the size of the diffusing unit (oligomers), [D] use of the time-resolved fluorescence energy transfer method for evaluation of (average) inter-protein distances, and [E] development of """"""""antibody probes"""""""" specifically tailored to rotational diffusion and fluorescence energy transfer measurements to observe association of a specific protein in a cell. The developed methods will be applied to our desmosome project: Desmosomal protein association in plasma membranes is observed at initial stages of calcium-induced synchronous formation of desmosomes in mouse epidermal cells in culture. We will detect formation of oligomeric complexes and colocalize at the molecular level two or more kinds of proteins in a cellular structure.

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
1R01GM035947-01
Application #
3289433
Study Section
Biophysics and Biophysical Chemistry A Study Section (BBCA)
Project Start
1986-01-01
Project End
1988-12-31
Budget Start
1986-01-01
Budget End
1986-12-31
Support Year
1
Fiscal Year
1986
Total Cost
Indirect Cost
Name
Medical College of Wisconsin
Department
Type
Schools of Medicine
DUNS #
073134603
City
Milwaukee
State
WI
Country
United States
Zip Code
53226