Angiogenesis, the sprouting of new capillary blood vessels from existing vasculature, is a complex biological process of critical importance to the treatment of numerous pathologies and the success of tissue engineering. Cell-based strategies to promote therapeutic vascularization have shown pre-clinical and clinical success, particularly for the treatment of critical limb ischemia, and typically involve the delivery of a single mesenchymal cell type to ischemic sites to stimulate angiogenesis. By contrast, strategies to vascularize engineered tissues typically involve two cell types, with endothelial cells (or their progenitors) combined with some sort of supporting stromal cell type and delivered via a hydrogel-based extracellular matrix (ECM). However, the choices of stromal cells and ECM have varied widely across studies. In the prior funding period, we used a combination of 3D cell culture models in vitro and subcutaneous implants in vivo to discover that the formation of nascent vasculature is regulated by both the biophysical properties of the ECM and the identity of the supporting stromal cells. Our data suggest that stromal cells of different origins differentially control ECM proteolysis during angiogenic sprouting, and that controlling the rate o ECM breakdown is critical to yield stable, functional vessels. In this competing renewal application, we propose to mechanistically investigate how these two critical instructive elements of the local microenvironment (i.e., the stromal cells and the ECM) influence the quantity, functional quality, and stability of new vasculature.
Aim 1 will quantify the impact of stromal cell identity on the rates of ECM proteolysis and capillary morphogenesis in a fibrin-based 3D co-culture model, using active microrheology to monitor local ECM mechanics as a function of time.
Aim 2 will use an engineered biomaterial platform with tunable degradative properties to determine the impact of ECM proteolytic susceptibility on the quantity and functional qualities of capillary networks.
Aim 3 will investigate how stromal cell identity and ECM proteolytic susceptibility affect the quantity and quality of neovasculature in a clinically relevant ischemic model. Successful completion of these studies will enhance current understanding of the role of the microenvironment in capillary morphogenesis, and ultimately guide the judicious selection of the ideal combination of cells and ECM for the treatment of ischemic conditions.

Public Health Relevance

Capillary morphogenesis is critical to many normal (e.g., wound healing) and pathologic (e.g., tumor progression) conditions, as well as emerging therapeutic approaches to treat ischemic conditions. In broad terms, this application will determine how two keys features of the microenvironment (e.g., the extracellular matrix and supporting stromal cells) regulate the quantity, functional quality, and stability of new capillary blood vessels. Results from the proposed studies will help bring cell-based strategies for revascularization therapies closer to a translational endpoint, and enhance ongoing efforts to vascularize engineered tissues.

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL085339-07
Application #
8909158
Study Section
Biomaterials and Biointerfaces Study Section (BMBI)
Program Officer
Lundberg, Martha
Project Start
2006-07-01
Project End
2018-04-30
Budget Start
2015-05-01
Budget End
2016-04-30
Support Year
7
Fiscal Year
2015
Total Cost
$371,721
Indirect Cost
$95,255
Name
University of Michigan Ann Arbor
Department
Biomedical Engineering
Type
Schools of Engineering
DUNS #
073133571
City
Ann Arbor
State
MI
Country
United States
Zip Code
48109
Kong, Yen P; Rioja, Ana Y; Xue, Xufeng et al. (2018) A systems mechanobiology model to predict cardiac reprogramming outcomes on different biomaterials. Biomaterials 181:280-292
Juliar, Benjamin A; Keating, Mark T; Kong, Yen P et al. (2018) Sprouting angiogenesis induces significant mechanical heterogeneities and ECM stiffening across length scales in fibrin hydrogels. Biomaterials 162:99-108
Bezenah, Jonathan R; Kong, Yen P; Putnam, Andrew J (2018) Evaluating the potential of endothelial cells derived from human induced pluripotent stem cells to form microvascular networks in 3D cultures. Sci Rep 8:2671
Beamish, Jeffrey A; Chen, Evan; Putnam, Andrew J (2017) Engineered extracellular matrices with controlled mechanics modulate renal proximal tubular cell epithelialization. PLoS One 12:e0181085
Keating, M; Kurup, A; Alvarez-Elizondo, M et al. (2017) Spatial distributions of pericellular stiffness in natural extracellular matrices are dependent on cell-mediated proteolysis and contractility. Acta Biomater 57:304-312
Romero-López, Mónica; Trinh, Andrew L; Sobrino, Agua et al. (2017) Recapitulating the human tumor microenvironment: Colon tumor-derived extracellular matrix promotes angiogenesis and tumor cell growth. Biomaterials 116:118-129
Janson, Isaac A; Putnam, Andrew J (2015) Extracellular matrix elasticity and topography: material-based cues that affect cell function via conserved mechanisms. J Biomed Mater Res A 103:1246-58
Rao, Rameshwar R; Vigen, Marina L; Peterson, Alexis W et al. (2015) Dual-phase osteogenic and vasculogenic engineered tissue for bone formation. Tissue Eng Part A 21:530-40
Carrion, Bita; Janson, Isaac A; Kong, Yen P et al. (2014) A safe and efficient method to retrieve mesenchymal stem cells from three-dimensional fibrin gels. Tissue Eng Part C Methods 20:252-63
Rao, Rameshwar R; Ceccarelli, Jacob; Vigen, Marina L et al. (2014) Effects of hydroxyapatite on endothelial network formation in collagen/fibrin composite hydrogels in vitro and in vivo. Acta Biomater 10:3091-7

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