Abstract

Hypertrophic scarring and keloid formation are serious derangements in healing defined largely on the basis of an abnormal accumulation and arrangement of extracellular matrix. This project asks a simple question: Do fibroblasts from normal scar tissue and from hypertrophic (or keloid) scar tissue differ in the way they process (degrade) extracellular matrix? It will address the dynamics of extracellular matrix metabolism in reparative tissues and will establish if (and how) fibroblastic degradation of glycosaminoglycan (primarily hyaluronate) differs between normal skin, normal mature scar, and hypertrophic/keloid scar tissue.
The specific aims will be to: 1. Introduce radiolabeled glycosaminoglycan substrate to fibroblasts derived from normal mature scars and hypertrophic scars (as well as from other reparative tissues) and observe how the labeled matrix substrate is internalized by cells. 2. Determine if the affinity or capacity for internalizing substrate differs between normal and hypertrophic scar fibroblasts (since such a difference could explain the formation of excess matrix seen in abnormal scarring). 3. Establish how and where the internalized substrate is degraded within cells. 4. Learn whether depolymerized substrate (in the form of labeled monosaccharides, disaccharides or oligosaccharides) are salvaged and reused in synthesizing new glycosaminoglycan or other N-acetylhexosamine-containing substances. Previous work in our laboratory has shown that hyaluronidase resides within wound fibroblasts and functions entirely intracellularly; this project will compare the stated cell types in terms of the way they accomplish matrix internalization, degradation, and re-synthesis/secretion since such processes are likely to be key differences in the behavior of normal scar and hypertrophic scar cells. Explant-derived fibroblasts from both human and animal (rabbit) tissues will be cultured. In the case of human tissues, cells will be obtained from samples of normal skin, of normal (mature) scar and of hypertrophic/keloid scar. Analytical procedures will include determining binding of [3H]-hyaluronate to fibroblasts, measuring [3H]-hyaluronate internalization, accumulation and degradation within fibroblasts, identifying (by cellular disruption/density gradient centrifugation) the subcellular location(s) of labeled hyaluronate-derived digestion products and then correlating these sites with the hyaluronidase activities of corresponding subcellular fractions.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Dental & Craniofacial Research (NIDCR)
Type
Research Project (R01)
Project #
5R01DE009178-03
Application #
3223008
Study Section
Oral Biology and Medicine Subcommittee 1 (OBM)
Project Start
1989-02-01
Project End
1992-03-31
Budget Start
1991-02-01
Budget End
1992-03-31
Support Year
3
Fiscal Year
1991
Total Cost
Indirect Cost

  Institution

Name
University of California Los Angeles
Department
Type
Schools of Dentistry
DUNS #
119132785
City
Los Angeles
State
CA
Country
United States
Zip Code
90095

  Publications

Bertolami, C N; Messadi, D V (1994) The role of proteoglycans in hard and soft tissue repair. Crit Rev Oral Biol Med 5:311-37
Messadi, D V; Bertolami, C N (1993) CD44 and hyaluronan expression in human cutaneous scar fibroblasts. Am J Pathol 142:1041-9
Bertolami, C N; Berg, S; Messadi, D V (1992) Binding and internalization of hyaluronate by human cutaneous fibroblasts. Matrix 12:11-21
Bertolami, C N; Shetty, V; Milavec, J E et al. (1991) Preparation and evaluation of a nonproprietary bilayer skin substitute. Plast Reconstr Surg 87:1089-98
Bertolami, C N; Bronson, R E (1990) Expression of different glycosaminoglycan synthetic phenotypes by lapine dermal and dermal wound fibroblasts. Matrix 10:1-9