The dendritic cell is a recently recognized new cell type having important immunological functions. It provides accessory activity required for responses of T lymphocytes, acts as a potent stimulator of a mixed leukocyte reaction and, owing to its richness in Ia antigens, serves as a critical """"""""passenger cell"""""""" that elicits rejection of transplanted tissues. Dendritic cells arise from precursors in bone marrow by a process that is the major focus of this research proposal. Virtually all precursors are recovered in a low density fraction (LD-BMC) that provides a 20-fold enrichment of these cells. Studies in vitro with LD-BMC indicate that, unlike the dendritic cell, the precursor is a dividing cell and is deficient or devoid of Ia. In cultures of LD-BMC, precursors develop over a five day period into dendritic cells that are functionally and morphologically indistinguishable from dendritic cells isolated from tissues. A soluble factor(s) produced by mitogen-treated lymphoid cells markedly augments the production of dendritic cells. Proposed studies aim at defining the role played by various cell types in the development of dendritic cells from precursors in a liquid culture system. Specific immunoadsorption and rosetting procedures will be applied. Autoradiography, immunofluorescence, and functional tests will be used to determine the kinetics of formation of Ia+ dendritic cells capable of accessory and stimulatory activity. The factor(s) responsible for augmenting dendritic cell production will be purified for the purposes of characterization and determining whether it acts directly on the precursor or on some other regulatory cell. The factor will also be used in an agar system for studies on the frequency, composition, and renewal of colonies of dendritic cells. An attempt will also be made to propagate dendritic cells. With bone marrow replacement increasingly used as a therapeutic tool, a greater knowledge of dendritic cell dynamics may contribute to making it a more efficacious procedure. No studies have been performed on the development in vitro of dendritic cells, and our research will provide new information about this process.

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
5R01AI017887-06
Application #
3127490
Study Section
Allergy and Immunology Study Section (ALY)
Project Start
1981-07-01
Project End
1989-05-31
Budget Start
1987-06-01
Budget End
1989-05-31
Support Year
6
Fiscal Year
1987
Total Cost
Indirect Cost
Name
Mary Imogene Bassett Hospital
Department
Type
DUNS #
City
Cooperstown
State
NY
Country
United States
Zip Code
13326
Bowers, W E; Ruhoff, M S; Goodell, E M (1990) Conditioned medium from activated rat macrophages and the recombinant factors, IL-1 beta and GM-CSF, enhance the accessory activity of dendritic cells. Immunobiology 180:362-84
Rochester, C L; Goodell, E M; Stoltenborg, J K et al. (1988) Dendritic cells from rat lung are potent accessory cells. Am Rev Respir Dis 138:121-8
Bowers, W E; Ruhoff, M S; Goodell, E M et al. (1988) The effect of silica treatment on accessory cell-dependent rat T lymphocyte proliferation. Immunobiology 176:179-94
Goodell, E M; Stoltenborg, J K; Bowers, W E (1987) Accessory cell dependent T lymphocyte proliferation: potent activity of dendritic cells. Immunobiology 174:30-42
Bowers, W E; Berkowitz, M R (1986) Differentiation of dendritic cells in cultures of rat bone marrow cells. J Exp Med 163:872-83
Bowers, W E; Berkowitz, M R (1985) Development of dendritic cells from rat bone marrow. Adv Exp Med Biol 186:377-81
Goodell, E M; Blumenstock, D A; Bowers, W E (1985) Canine dendritic cells from peripheral blood and lymph nodes. Vet Immunol Immunopathol 8:301-10