Novel anti-citrullinated peptide autoantibodies identified by proteomics with. citrullinated proteins in patients with rheumatoid arthritis

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Original ArticleProteomic surveillance of ACPAs in RA 121 Original Article Novel anti-citrullinated peptide autoantibodies identified by proteomics with citrullinated proteins in patients with rheumatoid arthritis Hiroyuki Mitsui 1, 2), Mitsumi Arito 1), Toshiyuki Sato 1), Michiyo K. Yokoyama 1), Naoya Suematsu 1), Kazuki Okamoto 1), Manae S. Kurokawa 1), Kazuo Yudo 3), Hiroshi Nakamura 4), Moroe Beppu 2) and Tomohiro Kato 1,) 1) Clinical Proteomics and Molecular Medicine, St. Marianna University Graduate School of Medicine, Kawasaki, Japan 2) Department of Orthopedic Surgery and 3) Institute of Medical Science, St. Marianna University School of Medicine, Kawasaki, Japan 4) Department of Rheumatology, Nippon Medical School, Tokyo, Japan Rheumatoid arthritis (RA) is immunologically characterized by generation of anti-citrullinated peptide antibodies (ACPAs). To promote understanding of ACPAs, we here identified novel ACPA antigens by proteomics using citrullination and investigated effects of citrullination on one of the ACPA antigens. Specifically, we citrullinated protein extracts from Jurkat cells and separated the citrullinated protein extracts as well as non-treated ones by 2-dimensional electrophoresis (2DE). By western blotting, we detected protein spots that reacted to RA serum samples only when they were citrullinated and identified them by mass spectrometry. On two of the identified proteins, adenosine deaminase (ADA) 1 and proliferation associated protein 2G4 (PA2G4), we confirmed the citrulline-dependent recognition by ACPAs using enzyme-linked immunosorbent assay (ELISA). Finally, we compared the activity of citrullinated ADA1 and nontreated one. As a result, we detected 8 candidate antigens for ACPAs, and identified 7 of them. In ELISA, 6 (24%) out of the tested 25 RA serum samples reacted to citrullinated ADA1, but none (0%) to non-treated ADA1 ( = 0.022). Similarly, 9 (36.0%) out of the same RA samples reacted to citrullinated PA2G4, but only 1 (4.0%) to non-treated PA2G4 ( = 0.01). In addition, we found that citrullination enhanced activity of ADA. In conclusion, we demonstrated novel autoantigens for ACPAs including ADA1 and PA2G4 and enhancement of the ADA activity by citrullination. The enhanced ADA activity may decrease anti-inflammatory adenosine and thus may hamper the pharmaceutical increase of adenosine by methotrexate in RA. Rec.10/18/2012, Acc.12/12/2012, pp121-130 Correspondence should be addressed to: Tomohiro Kato, MD, PhD, Clinical Proteomics and Molecular Medicine, St. Marianna University Graduate School of Medicine, 2-16-1, Sugao, Miyamae, Kawasaki, Kanagawa, 216-8511, Japan. Phone: +81-44-977-8111, Fax: +81-44-976-7553, E-mail: t3kato@marianna-u.ac.jp Key words rds rds

Original ArticleProteomic surveillance of ACPAs in RA 122 Introduction Materials and Methods 1)Clinical samples 2) citrullination, 2-dimensional electrophoresis (2DE), and western blotting (WB)

Original ArticleProteomic surveillance of ACPAs in RA 123 3)Protein identification 4)Preparation of proteins 5)Enzyme-linked immunosorbent assay (ELISA) Measurement of ADA activity 1)Statistical analysis Results 1)Surveillance of citrullinated autoantigens by 2DE-WB

Original ArticleProteomic surveillance of ACPAs in RA 124 Fig.1 Protein citrullination and 2DE-WB screening of citrullinedependent autoantigens (a)protein extracts from Jurkat cells, -citrullinated or non-treated, were separated by SDS-PAGE. Then the separated protein extracts were transferred onto nitrocellulose membranes and were reacted with anti- MC antibodies (left) and serum samples from patients with RA (right). A representative result is shown. (b)citrulline-dependent autoantigens were detected by 2DE-WB. The protein extracts from Jurkat cells, -citrullinated or non-treated, were separated by 2DE. Then the separated protein extracts were transferred onto nitrocellulose membranes and were reacted with serum samples from 5 patients with RA. A representative result from P1 is shown. The arrowheads indicate protein spots that reacted to two or more of the 5 serum samples in the 2DE-WB using the cutrullinated protein extracts but did not react to the samples in the 2DE-WB using non-treated protein extracts. Cit: citrullination, p: isoelectric point Fig.2 The positions of the identified 7 protein spots are indicated on a 2DE gel stained with SYPRO Ruby. The information on the identified proteins are summarized in Table 1. 2)Identification of the candidate autoantigens of ACPAs 3)Antibody titers to the identified citrullinated autoantigens by ELISA

Original ArticleProteomic surveillance of ACPAs in RA 125 Table 1 A list of candidate citrullinated autoantigens Fig.3 Preparation of citrullinated recombinant human ADA1 and PA2G4 proteins (a)recombinant human (rh) ADA1 prepared as a GST fusion protein was citrullinated, as positively detected by the anti- MC antibody by WB (left). The citrullinated rhada1-gst and similarly citrullinated GST were incubated with the anti-citrullinated ADA1-positive serum samples in the 2DE-WB screening. The samples reacted to the citrullinated rhada1 but not to the citrullinated GST. Results from P2 and P8 are shown (right). (b)rhpa2g4 prepared as a GST fusion protein was citrullinated in vitro, as positively detected by the anti-mc antibody by WB (left). The citrullinated rhpa2g4-gst and citrullinated GST were incubated with the anti-citrullinated PA2G4-positive serum samples in the 2DE-WB screening. The samples reacted to the citrullinated rhpa2g4 but not to the citrullinated GST. Results from P1 and P8 are shown (right).

Original ArticleProteomic surveillance of ACPAs in RA 126 Table 2 Relations between the presence of antibodies to citrullinated ADA1 and that of antibodies to citrullinated PA2G4 Table 3 Relations between the presence of antibodies to citrullinated ADA1 and that of anti-ccp antibodies Fig.4 Reactivity of the citrullinated ADA1 and PA2G4 measured by ELISA Autoantibodies to the citrullinated and non-treated rhada1 (a) and rhpa2g4 (b) were measured by ELISA using serum samples from 25 patients with RA and 25 healthy donors. The binding units of 100 were defined as the cut-off point, as described in the materials and methods section. The percentages of serum samples with positive titers are described in the parentheses. Cit-: citrullinated, NS: not significant. Table 4 Relations between the presence of antibodies to citrullinated PA2G4 and that of anti-ccp antibodies

Original ArticleProteomic surveillance of ACPAs in RA 127 Fig.5 Effects of citrullination on the ADA activity Bovine intestine-derived ADA, citrullinated or incubated in the same solution without PAD as a negative control, was subjected to the ADA activity assay (a). Human erythrocyte-derived ADA1, similarly citrullinated or incubated without PAD as a negative control, were refolded by dialysis and then were subjected to the ADA activity assay (b). 4)Effects of citrullination on the ADA activity Discussion

Original ArticleProteomic surveillance of ACPAs in RA 128 Acknowledgements and Source of funding Disclosure

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