Abstract

We propose to study the cellular and molecular mechanisms controlling new blood vessel formation (angiogenesis) during embryonic development, using a concerted biochemical, pharmacological, and biological approach. Angiogenesis is a key step in the development of many normal and pathological tissues, and thus represents a potential control point for diseases such as cancer, rheumatoid arthritis, and retinopathies. Because adipocyte differentiation and angiogenesis are tightly coordinated during embryogenesis, the interaction between cultured 3T3-adipocytes and vascular endothelial cells provides an excellent model system. We have previously shown that as 3T3-preadipocytes differentiate, they begin to secrete factor(s) into the medium which stimulate angiogenesis in vivo, and three important components of the angiogenic response in vitro--protease activity, chemotaxis, and mitogenesis. Preliminary results suggest that prostaglandins or other arachidonic acid derivatives may be involved. We plan to identify the major influences modulating production of the angiogenic activities by adipocytes, using agents known to affect adipocyte metabolism--insulin, cyclic AMP agents, hypoxia, and arachidonate derivatives. We plan to examine factors which may modulate the response of blood vessels to various angiogenic stimuli, including arachidonate derivatives and heparin. We will fractionate adipocyte-conditioned medium using various chromatographic techniques (including high-pressure liquid chromatography) to determine if a single factor stimulates angiogenesis, or if several molecular signals are required. If factors stimulating growth, chemotaxis, protease activity, and angiogenesis are separable, the effects of combining individual factors will be studied. Subsequently, we will continue purification of the angiogenesis factor(s). A key aspect of this proposal is that we intend to follow angiogenesis in vivo as well as endothelial cell protease activity, chemotaxis, and proliferation in vitro after each of the biochemical or pharmacological manipulations. Techniques employed will include: the chick chorioallantoic membrane assay for angiogenesis; plasminogen activator and collagenase assays; modified Boyden chamber assays for chemotaxis; and growth curves of endothelial cell number to assay mitogenesis.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL030290-03
Application #
3341353
Study Section
Cognition and Perception Study Section (CP)
Project Start
1983-06-01
Project End
1986-05-31
Budget Start
1985-06-01
Budget End
1986-05-31
Support Year
3
Fiscal Year
1985
Total Cost
Indirect Cost

  Institution

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

  Publications

Sun, J; Marx, S O; Chen, H J et al. (2001) Role for p27(Kip1) in Vascular Smooth Muscle Cell Migration. Circulation 103:2967-72
Dobson, D E; Kambe, A; Block, E et al. (1990) 1-Butyryl-glycerol: a novel angiogenesis factor secreted by differentiating adipocytes. Cell 61:223-30
McGuire, P G; Castellot Jr, J J; Orkin, R W (1987) Size-dependent hyaluronate degradation by cultured cells. J Cell Physiol 133:267-76
Rogers, K A; Hoover, R L; Castellot Jr, J J et al. (1986) Dietary cholesterol-induced changes in macrophage characteristics. Relationship to atherosclerosis. Am J Pathol 125:284-91
Castellot Jr, J J; Kambe, A M; Dobson, D E et al. (1986) Heparin potentiation of 3T3-adipocyte stimulated angiogenesis: mechanisms of action on endothelial cells. J Cell Physiol 127:323-9