Abstract

BackgroundAlloantibodies against human platelet antigens (HPAs) and human leukocyte antigen (HLA) are implicated in several immune-mediated platelet disorders. Detection of these antibodies is crucial in the diagnosis and management of these disorders. The aim of this study was to establish a novel method to simultaneously detect HPA-1, HPA-2, HPA-3, HPA-5 and HLA antibodies with Luminex microbeads technology.MethodsMonoclonal antibodies specific for platelet glycoproteins and HLA class I molecules were separately coupled to the Luminex microbeads. We validated specificity of the Luminex platform using the following antibodies: anti-HPA-1a, anti-HPA-2b, anti-HPA-3a, anti-HPA-5a, and anti-HLA positive samples. Sensitivity was evaluated by a serial dilution (from neat to 1/1024) using the following antibodies: anti-HPA-1a, anti-HPA-3a standard sera, and anti-HPA-5a positive serum. Serum samples were collected from 36 neonatal alloimmune thrombocytopenia (NAIT) patients suspected of having HPA or HLA antibodies and 8 samples from ISBT platelet workshop were tested using the Luminex assay.ResultsThe Luminex assay detected all antibodies tested from the known samples. The sensitivities of the Luminex assay detecting anti-HPA-1a, anti-HPA-3a, and anti-HPA-5a were 1:512, 1:64, and 1:128, respectively. The sensitivity of Luminex assay was higher than monoclonal antibody immobilization of platelet antigen method (MAIPA). No cross-reactivity was observed in the samples containing multi-platelet antibodies or mixture antibodies against HPA and HLA. The results of 44 samples with platelet disorders were consistent with those of the same samples processed with the MAIPA assay.ConclusionLuminex microbeads coupled with monoclonal antibodies could be successfully used to detect HPA and HLA antibodies simultaneously, especially with high sensitivity in detecting HPA antibodies.

Highlights

  • Alloantibodies against human platelet antigens (HPAs) and human leukocyte antigen (HLA) are implicated in several immune-mediated platelet disorders

  • Serum samples Forty-four serum samples including 8 samples from ISBT platelet workshop and 36 samples previously collected from patients suspected of having HPA or HLA antibodies were tested in this study

  • The MFI values of coupled bead reacted with goat anti-mouse are 2661 ± 327 for antiGPIa, 7871 ± 585 for GPIba, 4573 ± 399 for GPIIb/IIIa, 4471 ± 283 for CD109, 3741 ± 89 for HLA, 4831 ± 27 for human IgG, and 20 ± 1 to 40 ± 7 for empty beads

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Summary

Introduction

Alloantibodies against human platelet antigens (HPAs) and human leukocyte antigen (HLA) are implicated in several immune-mediated platelet disorders. Detection of these antibodies is crucial in the diagnosis and management of these disorders. Alloantibodies against human leukocyte antigen (HLA)I class and human platelet antigen (HPA) are involved in several immune-mediated platelet disorders including neonatal alloimmune thrombocytopenia (NAIT), post-transfusion purpura (PTP), and platelet transfusion refractoriness (PTR) [1–4]. There are several methods to detect HPA antibodies, including solid phase red cell adherence (SPRCA), monoclonal antibody specific immobilization of platelet antigen (MAIPA) technology, immuno-complex capture fluorescence analysis (ICFA), gel antigen-specific assay (GASA), and HP cell-based monoclonal antibodyindependent Immobilization of Platelet Antigen [6–8]. It is necessary to update these methods to effectively identify HPA antibody, which is important for the clinical diagnosis of HPA antibody and the improvement of platelet transfusion efficiency

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