| Literature DB >> 15236752 |
Bernhard A Herzog1, Patrick A Ott, Marcus T Dittrich, Stefan Quast, Alexey Y Karulin, Hubert Kalbacher, Wolfram Karges, Magdalena Tary-Lehmann, Paul V Lehmann, Bernhard O Boehm, Ivana Durinovic-Belló.
Abstract
Active T cell recognition of islet antigens has been postulated as the pathogenic mechanism in human type 1 diabetes, but evidence is scarce. If T cells are engaged, they are expected to display increased clonal size and exhibit a T helper (Th)1/Th2 differentiation state. We used a peptide library that covers tyrosine phosphatase IA-2, a target antigen expressed in pancreatic beta cells, to probe 8 diabetic patients and 5 HLA-matched controls. When tested in a high resolution IFNgamma/IL-4 double color ELISPOT assay directly ex vivo, the number of IA-2-reactive IFNgamma producing cells was 17-fold higher in patients than in controls and IL-4 producing cells were not present. An average of 9 peptides was recognized in the patients vs. one in the controls. Determinant recognition primarily involved CD4+ cells and showed high variability among the patients. Furthermore, anti-CD28 antibody signal enhances quantitative assessment of effector T cells in T1D patients. In vitro expansion with peptides and IL-2 results in detection of responding cells in the controls and loss of disease specificity of the T cell response. Together these data provide strong evidence for the active targeting of IA-2 by Th1 memory effector cells in human type 1 diabetes. Copyright 2004 Elsevier Ltd.Entities:
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Year: 2004 PMID: 15236752 DOI: 10.1016/j.jaut.2004.03.009
Source DB: PubMed Journal: J Autoimmun ISSN: 0896-8411 Impact factor: 7.094