Anti-histone and anti-nucleosome rather than anti-dsDNA antibodies associate with IFN-induced biomarkers in Sudanese and Swedish SLE patients

Author:

Elbagir Sahwa1ORCID,Mohammed NasrEldeen A2,Oke Vilija34,Larsson Anders5,Nilsson Jan6ORCID,Elshafie Amir17,Elagib Elnour M8,Nur Musa A M9,Gunnarsson Iva3,Svenungsson Elisabet3ORCID,Rönnelid Johan1ORCID

Affiliation:

1. Department of Immunology, Genetics and Pathology, Uppsala University , Uppsala, Sweden

2. Faculty of Medical Laboratory Sciences, Al Neelain University , Khartoum, Sudan

3. Division of Rheumatology, Department of Medicine Solna, Karolinska Institute, Karolinska University Hospital , Stockholm, Sweden

4. Centre for Rheumatology, Academic Specialist Centre , Stockholm, Sweden

5. Department of Medical Sciences, Section of Clinical Chemistry, Uppsala University , Uppsala, Sweden

6. Department of Experimental Medical Science, Lund University , Lund, Sweden

7. Department of Clinical Immunology and Transfusion Medicine, Linköping University Hospital , Linköping, Sweden

8. Rheumatology Unit, Military Hospital , Omdurman, Sudan

9. Rheumatology Unit, Alribat University Hospital , Khartoum, Sudan

Abstract

Abstract Objectives In SLE, anti-dsDNA can co-occur with autoantibodies against other chromatin components, like histones and nucleosomes. These antibodies induce type-1 interferon production, a hallmark of SLE. We measured ANA sub-specificities and investigated their associations to inflammatory biomarkers including interferon-regulated chemokines. Methods We included 93 Sudanese and 480 Swedish SLE patients and matched controls (N = 104 + 192). Autoantibodies targeting ANA sub-specificities: dsDNA, Sm, Sm/U1RNPcomplex, U1RNP, SSA/Ro52, SSA/Ro60, SSB/La, ribosomal P, PCNA and histones were quantified in all subjects, anti-nucleosome only in the Swedish patients, with a bead-based multiplex immunoassay. Levels of 72 plasma biomarkers were determined with the Proximity Extension Assay technique or ELISA. Results Among Sudanese patients, the investigated antibodies were significantly associated with 9/72 biomarkers. Anti-histone antibodies showed the strongest positive correlations with MCP-3 and S100A12 as well as with interferon I-inducible factors MCP-1 and CXCL10. Anti-dsDNA antibodies were associated with CXCL10 and S100A12, but in multivariate analyses, unlike anti-histone, associations lost significance. Among Swedish patients, MCP-1, CXCL10, and SA100A12 also demonstrated stronger associations to anti-histone and anti-nucleosome antibodies, compared with anti-dsDNA and other ANA sub-specificities. In multiple regression models, anti-histone/nucleosome retained the strongest associations. When excluding anti-histone or anti-nucleosome positive patients, the associations between MCP-1/CXCL10 and anti-dsDNA were lost. In contrast, when excluding anti-dsDNA positive patients, associations with anti-histone and anti-nucleosome remained significant. Conclusion In two cohorts of different ethnical origins, autoantibodies targeting chromatin correlate stronger with IFN-induced inflammatory biomarkers than anti-dsDNA or other ANA sub-specificities. Our results suggest that anti-histone/nucleosome autoantibodies may be the main drivers of type-1 interferon activity in SLE.

Funder

Swedish Rheumatism Association

Agnes and Mac Rudberg Foundation

Signe and Reinhold Sund’s Foundation for Rheumatological Research

Swedish Society of Medicine

Ingegerd Johansson Donation

Swedish Research Council

Uppsala County Council

Stockholm County Council

Swedish Heart-Lung Foundation

Publisher

Oxford University Press (OUP)

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