Abstract

Angiogenesis, the growth of new blood vessels from extant capillaries, is a continuous process throughout most of the embryonic and mature lifespan of vertebrates. It is also necessary for remodeling and tumor growth. The angiogenic process is thought to proceed in discrete stages that include migration, proliferation, and remodeling of the extracellular matrix (ECM) by endothelial cells, although the regulation of these events is poorly understood. We have recently defined a group of secreted macromolecules that modulate interactions between cells and ECM. Several of these components are major products of endothelial cells undergoing angiogenesis in vitro and in vivo. In this proposal we focus on SPARC (secreted protein, acidic and rich in cysteine), a Cu+2 and Ca+2-binding protein which modulates the shape, adhesion, cell-cycle progression, ECM production, and migration of cultured endothelial cells. The expression of SPARC in tissues exhibiting morphogenesis and remodeling, as well as the interaction of SPARC with angiogenesis factors such as platelet-derived growth factor (PDGF) and basic fibroblast growth factor (bFGF), indicate potential functions for SPARC as an endothelial morphogen. We have advanced the hypothesis that SPARC alters the relationship among endothelial cells, mitogens, and ECM and thereby predisposes endothelium toward an activated state of remodeling and neovascularization. In 7 Aims we address the function of SPARC at specific stages of angiogenesis in vivo and in vitro. Sequences of SPARC protein with growth-modulatory activity will be mutated, and recombinant proteins will be used to identify signaling pathways in endothelial cells that are responsive to native SPARC. The ability of SPARC to modulate endothelial cell proliferation and migration, through high-affinity binding to PDGF or indirectly through a serum factor that alters responses of cells to bFGF, will be characterized by identifying a) a binding site(s) on SPARC for PDGF, and b) the factor in serum or plasma responsible for the subversion of bFGF activity. A Cu+2-binding sequence in SPARC will be tested for angiogenic activity in vivo and in vitro, and its proteolytic release from SPARC will be characterized; mutations in this region will target critical residues. A potential role for SPARC in the modulation of matrix integrity will be examined during vasculogenesis and angiogenesis in embryonic mice that lack type I collagen, a protein expressed at high levels during capillary formation. Related experiments will test the effect of SPARC on the contraction of collagen gels by angiogenic endothelial cells that form cords and tubes in vitro. Finally, we will attempt to ascertain how the SPARC gene is regulated in angiogenic cells by performing transient transfections with regions of the SPARC promoter and first intron. Since 2 genes related to SPARC have been isolated from embryonic brain, we will attempt to clone similar genes from tissues rich in capillaries with probes corresponding to bioactive regions of SPARC. Through these aims we hope to elucidate how blood vessels grow int he context of signals mediated by SPARC, a dynamic participant in the extracellular regulation of cell behavior.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
2R01GM040711-06
Application #
3298534
Study Section
Pathology A Study Section (PTHA)
Project Start
1989-07-01
Project End
1997-06-30
Budget Start
1993-07-01
Budget End
1994-06-30
Support Year
6
Fiscal Year
1993
Total Cost
Indirect Cost

  Institution

Name
University of Washington
Department
Type
Schools of Medicine
DUNS #
135646524
City
Seattle
State
WA
Country
United States
Zip Code
98195

  Publications

Cheng, Lamei; Sage, E Helene; Yan, Qi (2013) SPARC fusion protein induces cellular adhesive signaling. PLoS One 8:e53202
Millecamps, Magali; Tajerian, Maral; Naso, Lina et al. (2012) Lumbar intervertebral disc degeneration associated with axial and radiating low back pain in ageing SPARC-null mice. Pain 153:1167-79
Kucukdereli, Hakan; Allen, Nicola J; Lee, Anthony T et al. (2011) Control of excitatory CNS synaptogenesis by astrocyte-secreted proteins Hevin and SPARC. Proc Natl Acad Sci U S A 108:E440-9
Nie, Jing; Bradshaw, Amy D; Delany, Anne M et al. (2011) Inactivation of SPARC enhances high-fat diet-induced obesity in mice. Connect Tissue Res 52:99-108
Workman, Gail; Sage, E Helene (2011) Identification of a sequence in the matricellular protein SPARC that interacts with the scavenger receptor stabilin-1. J Cell Biochem 112:1003-8
Millecamps, Magali; Tajerian, Maral; Sage, E Helene et al. (2011) Behavioral signs of chronic back pain in the SPARC-null mouse. Spine (Phila Pa 1976) 36:95-102
Weaver, Matt; Workman, Gail; Schultz, Chad R et al. (2011) Proteolysis of the matricellular protein hevin by matrix metalloproteinase-3 produces a SPARC-like fragment (SLF) associated with neovasculature in a murine glioma model. J Cell Biochem 112:3093-102
Weaver, Matt S; Workman, Gail; Cardo-Vila, Marina et al. (2010) Processing of the matricellular protein hevin in mouse brain is dependent on ADAMTS4. J Biol Chem 285:5868-77
Arnold, Shanna A; Rivera, Lee B; Miller, Andrew F et al. (2010) Lack of host SPARC enhances vascular function and tumor spread in an orthotopic murine model of pancreatic carcinoma. Dis Model Mech 3:57-72
Nie, Jing; Sage, E Helene (2009) SPARC inhibits adipogenesis by its enhancement of beta-catenin signaling. J Biol Chem 284:1279-90

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