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. 2013 Jun;40(3):182-9.
doi: 10.1159/000351459. Epub 2013 May 8.

Luminex(®) and its applications for solid organ transplantation, hematopoietic stem cell transplantation, and transfusion

Affiliations

Luminex(®) and its applications for solid organ transplantation, hematopoietic stem cell transplantation, and transfusion

Nils Lachmann et al. Transfus Med Hemother. 2013 Jun.

Abstract

The detection of antibodies against the human leukocyte antigen (HLA) complex has become indispensable in every clinical practice. The development of solid-phase assays like the Luminex allows the standardized measurement of anti-HLA antibodies (HLAab) with high sensitivity, albeit the relevance for some clinical settings remains a matter of debate. In this review we aim to describe the principle of Luminex-based antibody detection, including two modifications that allow identifying solely complement-activating antibodies. We then describe three applications for Luminex: i) detection of HLAab preceding solid-organ transplantation and monitoring of donor-specific antibodies posttransplant as a risk factor for antibody-mediated rejection; ii) presence of HLAab in recipients as a risk for graft failure in hematopoietic stem cell transplantation, especially in haploidentical or mismatched transplantations; iii) role of HLAab in blood transfusion including refractory thrombocytopenia and selection of suitable platelet donors, transfusion-related lung injury after plasma transfusion, and immunization against HLA after red blood cell transfusion despite leukodepletion. Although the Luminex platform constitutes a potent technology for HLA antibody detection, some drawbacks require the well-educated analysis and interpretation of data in critical cases. In addition, Luminex has become an important tool to identify clinically relevant antibodies.

Keywords: HLA antibodies; Luminex; Transfusion.

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Figures

Fig. 1
Fig. 1
A Principle of the Luminex assay to detect HLA antibodies. Each specific bead impregnated with two fluorophores is coated with HLA from cell lines and platelets or recom-binant HLA. In case the test serum contains antibodies directed against the specific HLA it will bind to the appropriate bead. The binding is then detected by a PE-conjugated secondary antibody specific for human IgG. The combination of the fluorescence signals from each bead indicating the HLA specificity and the secondary reagent indicating bound HLA-specific antibodies is acquired by the Luminex system using appropriate lasers and detectors. B Comparison of the characteristics of the three distinct bead preparations commercially available.
Fig. 2
Fig. 2
Decreasing variability of the relative antigen density on HLA class I SAB of one vendor comparing an early and the most current lot. Relative antigen density was assessed by the monoclonal antibody clone W6/32 which binds a conformational epitope carried by all HLA-A, -B and -C native antigens. Variability of antigen density could be significantly reduced from an early (LAB-Screen lot#003) to a current lot (lot#007). HLA-C antigen density still reveals the highest variability.

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