A unique antiphospholipid assay recognizing phospholipid mixture compared with criteria antiphospholipid immunoassays in lupus patients

Author:

Zuo Y1,Willis R2,Papalardo E2,Petri M3,Harris E N4,Schleh A2,DeCeulaer K4,Smikle M4,Vilá L M5,Reveille J D6,Alarcón G S7,Gonzalez E B2

Affiliation:

1. University of Texas Southwestern Medical Center, Texas, USA

2. University of Texas Medical Branch, Galveston, Texas, USA

3. John Hopkins University School of Medicine, Baltimore, Maryland, USA

4. University of the West Indies, Mona Campus, Kingston, Jamaica

5. Division of Rheumatology, University of Puerto Rico Medical Sciences Campus, San Juan, Puerto Rico

6. University of Texas School of Medicine at Houston, Texas, USA

7. University of Alabama at Birmingham, Alabama, USA

Abstract

Background While essential for the classification of antiphospholipid syndrome (APS), anticardiolipin (aCL) assays lack specificity and anti-β2glycoproteinI (anti-β2GPI) assays lack sensitivity in this regard. Our aim was to perform a comparative analysis of the APhL ELISA assay (IgG/IgM) and criteria antiphospholipid (aPL) immunoassays in identifying APS-related clinical manifestations in a large group of patients with systemic lupus erythematosus (SLE). Methods Serum samples from 1178 patients from the Hopkins ( n = 543), LUMINA ( n = 588) and Jamaican SLE cohorts ( n = 47) were examined for IgG/IgM positivity in aCL (in-house), anti-β2GPI (two commercial kits) and APhL (Louisville APL) ELISA assays. Correlation of assay positivity with clinical manifestations and sensitivity, specificity, positive and negative predictive values and likelihood ratios were evaluated. A case series analysis was also performed in patients for whom there was isolated positivity in the specific aPL assays. Results The prevalence of aCL positivity was 34.9%, anti-β2GPI kit A was 22.6%, APhL was 11.5% and anti-β2GPI kit B was 7.6% in the study population. Anti-β2GPI kit B, aCL and APhL assays were correlated with venous thrombosis, while only APhL was significantly correlated with arterial thrombosis and consistently correlated with pregnancy-related morbidity. No significant correlations were noted for anti-β2GPI kit A. Sensitivity was greatest for aCL assays followed by anti-β2GPI kit A, APhL and anti-β2GPI kit B, while specificity was greatest and equal for anti-β2GPI kit B and APhL assays. Conclusions Overall, APhL antibodies, especially IgG, represent a promising biomarker for the classification of APS patients in the context of autoimmunity and in risk assessment with regards to pregnancy morbidity and thrombotic manifestations.

Publisher

SAGE Publications

Subject

Rheumatology

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