Deciphering the Autoantibody Response to the OJ Antigenic Complex

被引:5
作者
Fritzler, Marvin J. [1 ]
Bentow, Chelsea [2 ]
Satoh, Minoru [3 ,4 ]
McHugh, Neil [5 ]
Ghirardello, Anna [6 ]
Mahler, Michael [2 ]
机构
[1] Univ Calgary, Cumming Sch Med, Calgary, AB T2N 1N4, Canada
[2] Werfen Autoimmun, San Diego, CA 92131 USA
[3] Univ Occupat & Environm Hlth, Dept Human Informat & Sci, Kitakyushu 8078555, Japan
[4] Kitakyushu Yahata Higashi Hosp, Dept Med, Kitakyushu 8050071, Japan
[5] Univ Bath, Dept Pharm & Pharmacol, Bath BA2 7AY, England
[6] Univ Padua, Dept Med, Unit Rheumatol, I-35122 Padua, Italy
关键词
autoantibodies; OJ; myositis; antisynthetase syndrome; IDIOPATHIC INFLAMMATORY MYOPATHIES; RHEUMATOLOGY CLASSIFICATION CRITERIA; TRANSFER RNA-SYNTHETASES; 2017 EUROPEAN LEAGUE; RHEUMATISM/AMERICAN COLLEGE; DETECT AUTOANTIBODIES; ANTINUCLEAR ANTIBODY; LINE BLOT; MYOSITIS; IMMUNOASSAYS;
D O I
10.3390/diagnostics13010156
中图分类号
R5 [内科学];
学科分类号
1002 ; 100201 ;
摘要
(1) Background: Myositis specific antibodies (MSA) are important diagnostic biomarkers. Among the rarest and most challenging MSA are anti-OJ antibodies which are associated with anti-synthetase syndrome (ASS). In contrast to the other tRNA synthetases that are targets of ASS autoantibodies (e.g Jo-1, PL-7, PL-12, EJ, KS, Zo), OJ represents a macromolecular complex with several ribonucleoprotein subunits. Therefore, the choice of the antigen in autoantibody assays can be challenging. (2) Methods: We collected two independent cohorts with anti-OJ antibodies, one based on a commercial line immunoassay (LIA) (n = 39), the second based on protein immunoprecipitation (IP) (n = 15). Samples were tested using a particle-based multi-analyte technology (PMAT) system that allows for the simultaneous detection of antibodies to various autoantigens. For the detection of anti-OJ antibodies, two different antigens were deployed (KARS, IARS) on PMAT. The reactivity to the two antigens KARS and IARS was analyzed individually and combined in a score (sum of the median fluorescence intensities). (3) Results: In the cohort selection based on LIA, 3/39 (7.7%) samples were positive for anti-KARS and 7/39 (17.9%) for anti-IARS and 14/39 (35.9%) when the two antigens were combined. In contrast, in samples selected by IP the sensitivity of anti-KARS was higher: 6/15 (40.0%) samples were positive for anti-KARS, 4/15 (26.7%) for anti-IARS and 12/15 (80.0%) for the combination of the two antigens. 18/39 (46.2%) of the LIA samples generated a cytoplasmic IIF pattern (compatible with anti-synthetase antibodies), but there was no association with the antibody levels, neither with LIA nor with PMAT. (4) Conclusions: The combination of IARS and KARS might represent a promising approach for the detection of anti-OJ antibodies on a fully automated platform.
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