Objective The CLASS (Classification Criteria of Anti-Synthetase Syndrome) project is a large international multicentre study that aims to create the first data-driven anti-synthetase syndrome (ASSD) classification criteria. Identifying anti-aminoacyl tRNA synthetase antibodies (anti-ARS) is crucial for diagnosis, and several commercial immunoassays are now available for this purpose. However, using these assays risks yielding false-positive or false-negative results, potentially leading to misdiagnosis. The established reference standard for detecting anti-ARS is immunoprecipitation (IP), typically employed in research rather than routine autoantibody testing. We gathered samples from participating centers and results from local anti-ARS testing. As an "ad-interim" study within the CLASS project, we aimed to assess how local immunoassays perform in real-world settings compared to our central definition of anti-ARS positivity. Methods We collected 787 serum samples from participating centres for the CLASS project and their local anti-ARS test results. These samples underwent initial central testing using RNA-IP. Following this, the specificity of ARS was reconfirmed centrally through ELISA, line-blot assay (LIA), and, in cases of conflicting results, protein-IP. The sensitivity, specificity, positive likelihood ratio and positive and negative predictive values were evaluated. We also calculated the inter-rater agreement between central and local results using a weighted ? co-efficient. Results Our analysis demonstrates that local, real-world detection of anti-Jo1 is reliable with high sensitivity and specificity with a very good level of agreement with our central definition of anti-Jo1 antibody positivity. However, the agreement between local immunoassay and central determination of anti-non-Jo1 antibodies varied, especially among results obtained using local LIA, ELISA and "other" methods. Conclusion Our study evaluates the performance of real-world identification of anti-synthetase antibodies in a large cohort of multi-national patients with ASSD and controls. Our analysis reinforces the reliability of real-world anti-Jo1 detection methods. In contrast, challenges persist for anti-non-Jo1 identification, particularly anti-PL7 and rarer antibodies such as anti-OJ/KS. Clinicians should exercise caution when interpreting anti-synthetase antibodies, especially when commercial immunoassays test positive for non-anti-Jo1 antibodies.
Agreement between local and central anti-synthetase antibodies detection: results from the Classification Criteria of Anti-Synthetase Syndrome project biobank / Aravinthan, Loganathan; Giovanni, Zanframundo; Akira, Yoshida; Sara, Faghihi-Kashani; Iazsmin, Bauer Ventura; Eduardo, Dourado; Francisca, Bozan; Gianluca, Sambataro; Yasuhiko, Yamano; Sharon Sangmee, Bae; Darosa, Lim; Angela, Ceribelli; Natasa, Isailovic; Carlo, Selmi; Noreen, Fertig; Elena, Bravi; Yuko, Kaneko; André Pinto, Saraiva; Vega, Jovani; Javier, Bachiller-Corral; Jose, Cifrian; Antonio, Mera-Varela; Siamak, Moghadam-Kia; Veronica, Wolff; Julien, Campagne; Alain, Meyer; Margherita, Giannini; Konstantinos, Triantafyllias; Johannes, Knitza; Latika, Gupta; Yair, Molad; Florenzo, Iannone; Ilaria, Cavazzana; Matteo, Piga; Giacomo, De Luca; Sarah, Tansley; Emanuele, Bozzalla-Cassione; Francesco, Bonella; Tamera J, Corte; Tracy J, Doyle; David, Fiorentino; Miguel Angel, Gonzalez-Gay; Marie, Hudson; Masataka, Kuwana; Ingrid E, Lundberg; Andrew L, Mammen; Neil John, Mchugh; Fredrick W, Miller; Carlomaurizio, Montecucco; Chester V, Oddis; Jorge, Rojas-Serrano; Jens, Schmidt; Carlo Alberto, Scirè; Albert, Selva-O'Callaghan; Victoria P, Werth; Claudia, Alpini; Sara, Bozzini; Lorenzo, Cavagna; Rohit, Aggarwal; Agarwal, Class Project: V.; Fornaro, M.; Alberti, M. L.; Needham, M.; Houssiau, F.; Shinjo, S.; Basharat, P.; Wang, Q.; Quintana, G.; Gallay, L.; Ebstein, E.; Fiehn, C.; Feist, E.; Schneider, M.; Drott, U.; Voll, R. E.; Danko, K.; Shobha, V.; Rajasekhar, L.; Danieli, M. G.; Limonta, M.; Matucci-Cerinic, M.; Emmi, G.; Parronchi, P.; Bargagli, E.; Maggi, L.; Sebastiani, M.; Luppi, F.; Sainaghi, P. P.; Bartoloni, E.; Barsotti, S.; Nakashima, R.; Pipitone, N.; Riccieri, V.; Sebastiani, G.; Scarpato, S.; Cantarini, L.; Berti, A.; Colombelli, P. L.; Tomietto, P.; Lomater, C.; Quartuccio, L.; Orsolini, G.; Kondo, Y.; Kimura, N.; Vazquez-Del mercado, M.; Andersson, H.; Cabral De Fonseca, J. E.; Prieto-González, S.; Greco Merino, M. G.; Castaneda, S.; Barrio, J. M.; Nuno, L.; Pintó, I. R.; Alén55, J. C.; Sáez-Comet, L.; Cagnotto, G.; Alpsoy, E.; Chinoy, H.; Schiopu, E.; Gandiga, P.; Dimachkie, M. M.; Charles-Schoeman, C.; Wilfong, E.; Marder, G.; Gunawardena, H.; Ghetie, D.. - In: CLINICAL AND EXPERIMENTAL RHEUMATOLOGY. - ISSN 0392-856X. - STAMPA. - 42:2(2024), pp. 277-287. [10.55563/clinexprheumatol/s14zq8]
Agreement between local and central anti-synthetase antibodies detection: results from the Classification Criteria of Anti-Synthetase Syndrome project biobank
M. L. AlbertiMembro del Collaboration Group
;M. G. DanieliMembro del Collaboration Group
;L. CantariniMembro del Collaboration Group
;
2024-01-01
Abstract
Objective The CLASS (Classification Criteria of Anti-Synthetase Syndrome) project is a large international multicentre study that aims to create the first data-driven anti-synthetase syndrome (ASSD) classification criteria. Identifying anti-aminoacyl tRNA synthetase antibodies (anti-ARS) is crucial for diagnosis, and several commercial immunoassays are now available for this purpose. However, using these assays risks yielding false-positive or false-negative results, potentially leading to misdiagnosis. The established reference standard for detecting anti-ARS is immunoprecipitation (IP), typically employed in research rather than routine autoantibody testing. We gathered samples from participating centers and results from local anti-ARS testing. As an "ad-interim" study within the CLASS project, we aimed to assess how local immunoassays perform in real-world settings compared to our central definition of anti-ARS positivity. Methods We collected 787 serum samples from participating centres for the CLASS project and their local anti-ARS test results. These samples underwent initial central testing using RNA-IP. Following this, the specificity of ARS was reconfirmed centrally through ELISA, line-blot assay (LIA), and, in cases of conflicting results, protein-IP. The sensitivity, specificity, positive likelihood ratio and positive and negative predictive values were evaluated. We also calculated the inter-rater agreement between central and local results using a weighted ? co-efficient. Results Our analysis demonstrates that local, real-world detection of anti-Jo1 is reliable with high sensitivity and specificity with a very good level of agreement with our central definition of anti-Jo1 antibody positivity. However, the agreement between local immunoassay and central determination of anti-non-Jo1 antibodies varied, especially among results obtained using local LIA, ELISA and "other" methods. Conclusion Our study evaluates the performance of real-world identification of anti-synthetase antibodies in a large cohort of multi-national patients with ASSD and controls. Our analysis reinforces the reliability of real-world anti-Jo1 detection methods. In contrast, challenges persist for anti-non-Jo1 identification, particularly anti-PL7 and rarer antibodies such as anti-OJ/KS. Clinicians should exercise caution when interpreting anti-synthetase antibodies, especially when commercial immunoassays test positive for non-anti-Jo1 antibodies.| File | Dimensione | Formato | |
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