Abstract

The hallmark of rheumatoid arthritis is the progressive destruction of the articular cartilage which ultimately results in loss of joint function and eventual debilitation. Over the years, much information has accumulated which would implicate metalloproteinases in the destruction of cartilage matrix. First, all of these enzymes are fully active at physiological conditions and avidly degrade the major cartilage matrix components including proteoglycans, chondronectin and collagen types II, IX, and XI. Second, these enzymes are increased in the rheumatoid lesion and are produced by inflammatory phagocytes, synovial cells,a nd native chondrocytes. Third, the synthesis of these enzymes is upregulated by inflammatory cytokines which are also present in increased amounts in these tissues. In the past 5 years, the primary structure of the major enzymes of this family has been characterized and striking homologies have been found. In this application, we propose to study certain aspects of the enzymatic function of three members of this family (neutrophil collagenase, 92 kDa gelatinase and stromelysin) and correlate them with the primary structure of the proteins. Our experimental approach will be to construct mutations within the cDNA of these enzymes and express the mutant proteins using eukaryotic and prokaryotic expression vectors. the mutant proteins will be purified by affinity chromatography and functional properties evaluated in specific assay systems. The functional properties will be focused on substrate specificity, divalent cation binding, interaction with the tissue inhibitor of metalloproteinases and identification of the critical carboxylic acid residues. The recombinant mutant enzymes will be assayed for their ability to degrade and/or bind to a panel of substrates known to be degraded by one or more of these enzymes. The mutant proteins will be evaluated for their ability to bind Zn2+ and Ca2+ and divalent cation binding will be correlated with enzymatic activity and substrate binding. In other studies, mutant proteins will be examined for binding to the tissue inhibitor of collagenase (TIMP) and for susceptibility to inhibition by this protein. Finally, our techniques of site-directed mutagenesis will be directed at the putative active site of these enzymes. It is hypothesized that an acidic residue (Glu or Asp) functions as the active base catalyst in these enzymes. Candidate acidic residues in this region will be mutated to identify the essential amino acid(s). These studies will advance our understanding of the action of metalloproteinases to a new level and may lead to therapeutic concepts which would focus on protection of articular tissues from the degradative machinery of the rheumatoid lesion.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Arthritis and Musculoskeletal and Skin Diseases (NIAMS)
Type
Specialized Center (P50)
Project #
5P50AR039166-09
Application #
3728073
Study Section
Project Start
Project End
Budget Start
Budget End
Support Year
9
Fiscal Year
1995
Total Cost
Indirect Cost

  Institution

Name
University of Tennessee Health Science Center
Department
Type
DUNS #
941884009
City
Memphis
State
TN
Country
United States
Zip Code
38163

  Publications

Qian, Zhaohui; Latham, Kary A; Whittington, Karen B et al. (2013) Engineered regulatory T cells coexpressing MHC class II:peptide complexes are efficient inhibitors of autoimmune T cell function and prevent the development of autoimmune arthritis. J Immunol 190:5382-91
Qian, Zhaohui; Latham, Kary A; Whittington, Karen B et al. (2010) An autoantigen-specific, highly restricted T cell repertoire infiltrates the arthritic joints of mice in an HLA-DR1 humanized mouse model of autoimmune arthritis. J Immunol 185:110-8
Tang, Bo; Zhou, Jing; Park, Jeoung-Eun et al. (2009) T cell receptor signaling induced by an analog peptide of type II collagen requires activation of Syk. Clin Immunol 133:145-53
Myers, Linda K; Tang, Bo; Rosioniec, Edward F et al. (2007) An altered peptide ligand of type II collagen suppresses autoimmune arthritis. Crit Rev Immunol 27:345-56
Ye, X J; Tang, B; Ma, Z et al. (2007) The effects of interleukin-18 on rat articular chondrocytes: a study of mRNA expression and protein synthesis of proinflammatory substances. Clin Exp Immunol 149:553-60
Rosloniec, Edward F; Brandstetter, Tilmann; Leyer, Sigmar et al. (2006) Second-generation peptidomimetic inhibitors of antigen presentation effectively treat autoimmune diseases in HLA-DR-transgenic mouse models. J Autoimmun 27:182-95
Ahn, Jae I; Erdin, Robert A; Smith, Richard et al. (2006) Chondrocyte injection in distraction epiphysiolysis (rabbit model). J Orthop Res 24:355-65
Rosloniec, Edward F; Ivey 3rd, Robert A; Whittington, Karen B et al. (2006) Crystallographic structure of a rheumatoid arthritis MHC susceptibility allele, HLA-DR1 (DRB1*0101), complexed with the immunodominant determinant of human type II collagen. J Immunol 177:3884-92
Sakurai, Yoshihiko; Tang, Bo; Rosloniec, Edward F et al. (2006) Molecular characterization of an arthritogenic collagen peptide interacting with I-Ar. Immunology 117:136-42
Sakurai, Yoshihiko; Brand, David D; Tang, Bo et al. (2006) Analog peptides of type II collagen can suppress arthritis in HLA-DR4 (DRB1*0401) transgenic mice. Arthritis Res Ther 8:R150

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