Species Specificity of Anti-β2 Glycoprotein I Autoantibodies and Its Relevance to Anticardiolipin Antibody Quantitation

J Arvieux; L Darnige; E Hachulla; B Roussel; J C Bensa; M G Colomb

doi:10.1055/s-0038-1650356

Thrombosis and Haemostasis, Inhaltsverzeichnis

Thromb Haemost 1996; 75(05): 725-730
DOI: 10.1055/s-0038-1650356

Original Article

Schattauer GmbH Stuttgart

Species Specificity of Anti-β₂ Glycoprotein I Autoantibodies and Its Relevance to Anticardiolipin Antibody Quantitation

J Arvieux

¹The Laboratoire d’Imnnunologie, Centre de Transfusion Sanguine, Grenoble, France

,

L Darnige

²Département de Biologie Clinique, CH Compiègne, France

,

E Hachulla

³Service de Médecine Interne, CHU Lille, France

,

B Roussel

¹The Laboratoire d’Imnnunologie, Centre de Transfusion Sanguine, Grenoble, France

,

J C Bensa

¹The Laboratoire d’Imnnunologie, Centre de Transfusion Sanguine, Grenoble, France

,

M G Colomb

⁴CEA Laboratoire d’Immunochimie, INSERM U238, DBMS, CEN-G, Grenoble, France

› Institutsangaben

Abstract

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Summary

Some patients suspected of having antiphospholipid antibody syndrome (APS) were found to be positive for anti-β₂ glycoprotein I (β₂GPI) antibodies despite negative results for antibodies to cardiolipin (ACA). Since the major source of β₂GPI in the ACA assay is animal (usually bovine) serum, we studied the influence on ACA quantitation of the species specificity of anti-β₂GPI antibodies from patients with various autoimmune disorders, mostly systemic lupus erythematosus and primary APS. Ninety-seven sera were selected based on IgG (n = 76) or IgM (n = 64) positivity by ELISA using γ-irradiated plates coated with human or bovine purified β₂GPI. A higher proportion of IgM (43.7%) than IgG (7.9%) reacted to human, but not bovine, β₂GPI. Furthermore, from the samples reactive to both proteins, the ratio of antibody level against bovine to that against human β₂GPI was 1.08 ± 0.58 for IgG and 0.58 ± 0.3 for IgM (p <10⁻⁵). IgG and IgM ACA were detected in 78 and 40 sera, respectively; concordance between the two ELISAs for ACA and anti-β₂GPI antibodies was 94% for IgG and 75% for IgM. Out of 28 IgM showing recognition restricted to human β₂GPI, 21 were missed by the ACA assay, possibly because of lower concentrations of β₂GPI in those patients’ sera. The antibody reactivity pattern towards human and bovine β₂GPI of individual sera showed no variation with time and was related to the relative antibody avidity for each protein. A murine anti-human β₂GPI monoclonal antibody, 9G1, that cross-reacts with bovine β₂GPI, competed to a large extent with the patients’ anti-β₂GPI antibody binding sites whatever isotype involved or protein recognized. Therefore, anti-β₂GPI antibodies of IgM isotype display a marked preference for human compared to bovine β₂GPI responsible for frequent inconsistencies in the ACA assay.

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Referenzen

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