Abstract

. This is a competitive renewal of an ROI research project grant.
The aim of the proposed research is to apply state-of-the-art rheological methods, fluorescent optical sectioning microscopy and cell and molecular biology techniques to the study of atherosclerosis and thrombosis.
Four specific aims are outlined: 1) To understand the observed differences in gene expression patterns in endothelial cells (Ecs) and smooth muscle cells (SMCs) produced by physiological levels of fluid shear stress and cyclical mechanical strain. 2) To interpret the effect of shear preconditioning on gene expression profiles in response to subsequent change in mechanical environment or cytokine stimulation. 3) To understand the potential differences between various endothelial cell types in their response to mechanical forces. 4) To interpret early signal transduction of flow induced shear stress to the cellular nucleus via either cytoskeletal connections and/or diffusible second messengers. The PI hypothesizes that both stress and strain have quite different effects on gene expression and regulation of cell phenotype. Proteins important in thrombosis and atherosclerosis (thrombin receptor 1 [protease activated receptor - 1 or PAR - 1], VEGF, PGH Synthases, ICAM, VCAM, GP1b [a platelet receptor that can be expressed on endothelial cells] and von Willebrand factor) have been targeted for study. The PI has shown previously dramatic effects of arterial shear stress on TPA and endothelin syntheses and secretion. In addition, new DNA micro array technology will be used to greatly increase the amount of information obtained per experiment. This approach could lead to an understanding of groups of genes that are regulated in a coordinated manner by mechanical forces and thus result in important new hypotheses in vascular biology. A major question is how are mechanical signals transduced to produce intracellular changes. Optical sectioning fluorescence microscopy and digital image processing will be used to study stress effects on calcium fluxes and intracellular pH. The equipment is able to obtain both multicellular averages and single cell changes in fluorescence. The ability has also been developed to examine the three-dimensional distribution of ions in a single-cell using optical sectioning and image analysis and reconstruction. Changes in nuclear geometry in response to cell mechanical loading will also be examined using this technology. A final question to be examined is the relative role of stress (or strain) magnitude versus the rate of change of stress (or strain). Since arterial blood flow is inherently pulsatile, in vivo application of the PI's in vitro results will require this knowledge.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL018672-24
Application #
6388812
Study Section
Special Emphasis Panel (ZRG1-SSS-W (28))
Program Officer
Ganguly, Pankaj
Project Start
1976-06-30
Project End
2005-06-30
Budget Start
2001-09-10
Budget End
2002-06-30
Support Year
24
Fiscal Year
2001
Total Cost
$306,971
Indirect Cost

  Institution

Name
Rice University
Department
Biomedical Engineering
Type
Schools of Engineering
DUNS #
050299031
City
Houston
State
TX
Country
United States
Zip Code
77005

  Publications

Sung, Derek C; Bowen, Caitlin J; Vaidya, Kiran A et al. (2016) Cadherin-11 Overexpression Induces Extracellular Matrix Remodeling and Calcification in Mature Aortic Valves. Arterioscler Thromb Vasc Biol 36:1627-37
Lee, Cho-Yin; Lou, Jizhong; Wen, Kuo-Kuang et al. (2016) Regulation of actin catch-slip bonds with a RhoA-formin module. Sci Rep 6:35058
Bowen, Caitlin J; Zhou, Jingjing; Sung, Derek C et al. (2015) Cadherin-11 coordinates cellular migration and extracellular matrix remodeling during aortic valve maturation. Dev Biol 407:145-57
Lee, Cho-yin; Lou, Jizhong; Wen, Kuo-kuang et al. (2013) Actin depolymerization under force is governed by lysine 113:glutamic acid 195-mediated catch-slip bonds. Proc Natl Acad Sci U S A 110:5022-7
Lee, Sungmun; Eskin, Suzanne G; Shah, Ankit K et al. (2012) Effect of zinc and nitric oxide on monocyte adhesion to endothelial cells under shear stress. Ann Biomed Eng 40:697-706
Coburn, L A; Damaraju, V S; Dozic, S et al. (2011) GPIbýý-vWF rolling under shear stress shows differences between type 2B and 2M von Willebrand disease. Biophys J 100:304-12
Conway, Daniel E; Lee, Sungmun; Eskin, Suzanne G et al. (2010) Endothelial metallothionein expression and intracellular free zinc levels are regulated by shear stress. Am J Physiol Cell Physiol 299:C1461-7
Conway, Daniel E; Williams, Marcie R; Eskin, Suzanne G et al. (2010) Endothelial cell responses to atheroprone flow are driven by two separate flow components: low time-average shear stress and fluid flow reversal. Am J Physiol Heart Circ Physiol 298:H367-74
Conway, Daniel E; Sakurai, Yumiko; Weiss, Daiana et al. (2009) Expression of CYP1A1 and CYP1B1 in human endothelial cells: regulation by fluid shear stress. Cardiovasc Res 81:669-77
Williams, Marcie R; Sakurai, Yumiko; Zughaier, Susu M et al. (2009) Transmigration across activated endothelium induces transcriptional changes, inhibits apoptosis, and decreases antimicrobial protein expression in human monocytes. J Leukoc Biol 86:1331-43

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