Induction of arthritis with monoclonal antibodies to collagen

mAb were developed from DBA/1 mice immunized with chick type II collagen. A total of 69 IgG antibodies was isolated and characterized. The majority (36%) reacted with a CNBr-derived peptide CB11 previously identified as containing a major immunogenic and arthritogenic epitope(s). Seven of the antibo...

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Bibliographic Details
Published inThe Journal of immunology (1950) Vol. 148; no. 7; pp. 2103 - 2108
Main Authors Terato, K, Hasty, KA, Reife, RA, Cremer, MA, Kang, AH, Stuart, JM
Format Journal Article
LanguageEnglish
Published Bethesda, MD Am Assoc Immnol 01.04.1992
American Association of Immunologists
Subjects
Animals
Antibodies, Monoclonal - immunology
Antibody Specificity
Arthritis - immunology
Arthritis - pathology
Biological and medical sciences
Collagen - immunology
Diseases of the osteoarticular system
Immunization
Inflammatory joint diseases
Male
Medical sciences
Mice
Mice, Inbred DBA
Animal model
Immunization
Induction
Pathogenesis
Rodentia
Diseases of the osteoarticular system
Inflammatory joint disease
Arthritis
Glycoproteins
Monoclonal antibody
Vertebrata
Specificity
Mammalia
Mouse
Collagen
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Summary:mAb were developed from DBA/1 mice immunized with chick type II collagen. A total of 69 IgG antibodies was isolated and characterized. The majority (36%) reacted with a CNBr-derived peptide CB11 previously identified as containing a major immunogenic and arthritogenic epitope(s). Seven of the antibodies reactive with CB11 crossreacted strongly with mouse type II collagen. These were administered to DBA/1 mice in an attempt to induce arthritis. Individual antibodies were able to induce mild lesions consisting of minimal synovial proliferation but not overt arthritis. However, a combination of antibodies induced severe arthritis with marked destruction of articular cartilage. The minimal effective combination consisted of three antibodies. Arthritis developed within 48 to 72 h after injection of the antibodies and persisted for the duration of the observation period of 3 wk. Antibody levels were measured at intervals and persisted for the 3 wk observation period although at diminishing levels. Competitive binding assays demonstrated that each of the effective antibodies bound independently suggesting that some spatial or quantitative relationship was important possibly related to their ability to activate complement.
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ISSN:0022-1767
1550-6606
DOI:10.4049/jimmunol.148.7.2103