Abstract

When artificial surfaces are exposed to blood, a single or relatively few molecular signals from non-specific attachment of protein molecules to the surface can cause a fast and precipitous response, such as in the surface activation of the coagulation and complement systems. Blood proteins reach surfaces before the cellular blood components; cellular blood components collide with the surface already covered with a (multi)layer of proteins. This hierarchy of events causes the effects of nonspecific interactions between proteins and the surface to be propagated to a higher, cellular level by mediating the specific attachment of cells to the protein layer. The reason for this is that the attachment of cells to surfaces is controlled by the spatial pattern of proteins which expose their specific amino acid sequence for specific cell membrane receptors. This is equally true for the attachment of platelets to the surfaces of subendothelial matrix and to artificial materials. Direct observation of proteins binding to surfaces by scanning force microscopy (SFM) is now possible. It is also possible to deliberately manipulate surface-bound proteins in ordered arrays using the same scanning probe technique. Our preliminary experiments indicate that the attachment and spreading of platelets can be directly observed in situ with high resolution (10 nm). In this competing continuation application we propose to continue development of SFM as an in situ, high resolution research tool for direct observation of cell interactions with protein-coated biomaterials and model surfaces. In particular, we propose to apply the scanning force microscopy technique to the following studies: 1. The in situ mechanism of platelet adhesion and spreading onto patterned, protein-coated surfaces and onto the surfaces of microphase-separated biomaterials. 2. Characterization of microphase-separated biomaterial surfaces in aqueous environment using SFM adhesion and elasticity maps. 3. Characterization of the homogeneity of biomaterial coatings on the submicron scale using SFM probes with specific ligands attached.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL044538-05
Application #
2221554
Study Section
Surgery and Bioengineering Study Section (SB)
Project Start
1990-04-01
Project End
1996-03-31
Budget Start
1994-04-01
Budget End
1995-03-31
Support Year
5
Fiscal Year
1994
Total Cost
Indirect Cost

  Institution

Name
University of Utah
Department
Biomedical Engineering
Type
Schools of Engineering
DUNS #
City
Salt Lake City
State
UT
Country
United States
Zip Code
84112

  Publications

Hlady, Vladimir; Jogikalmath, Gangadhar (2007) Albumin binding and insertion into PS-b-PEO monolayers at air-water interface. Colloids Surf B Biointerfaces 54:179-87
Hodgkinson, Gerald N; Tresco, Patrick A; Hlady, Vladimir (2007) The differential influence of colocalized and segregated dual protein signals on neurite outgrowth on surfaces. Biomaterials 28:2590-602
Turner, Nicholas W; Jeans, Christopher W; Brain, Keith R et al. (2006) From 3D to 2D: a review of the molecular imprinting of proteins. Biotechnol Prog 22:1474-89
Hlady, V; Buijs, J; Jennissen, H P (1999) Methods for studying protein adsorption. Methods Enzymol 309:402-29
Stuart, J K; Hlady, V (1999) Reflection interference contrast microscopy combined with scanning force microscopy verifies the nature of protein-ligand interaction force measurements. Biophys J 76:500-8
Dupont-Gillain, CC; Nysten, B; Hlady V, V et al. (1999) Atomic Force Microscopy and Wettability Study of Oxidized Patterns at the Surface of Polystyrene. J Colloid Interface Sci 220:163-169
Webb, K; Hlady, V; Tresco, P A (1998) Relative importance of surface wettability and charged functional groups on NIH 3T3 fibroblast attachment, spreading, and cytoskeletal organization. J Biomed Mater Res 41:422-30