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使用基于微珠的多重免疫测定法对抗因子VIII抗体进行全面的特定领域分析和免疫球蛋白G谱分析。

Comprehensive domain-specific analysis and immunoglobulin G profiling of anti-factor VIII antibodies using a bead-based multiplex immunoassay.

作者信息

Pezeshkpoor Behnaz, Berkemeier Ann-Cristin, Herbst Kerstin, Albert Thilo, Müller Jens, Oldenburg Johannes

机构信息

Institute of Experimental Hematology and Transfusion Medicine, University Hospital Bonn, Medical Faculty, University of Bonn, Bonn, Germany.

Institute of Experimental Hematology and Transfusion Medicine, University Hospital Bonn, Medical Faculty, University of Bonn, Bonn, Germany.

出版信息

J Thromb Haemost. 2024 Jun;22(6):1591-1604. doi: 10.1016/j.jtha.2024.02.016. Epub 2024 Mar 5.

Abstract

BACKGROUND

Antibodies against factor (F)VIII are a major complication in the treatment of patients with severe hemophilia A. The Nijmegen-Bethesda assay (NBA) is the gold standard for detection of neutralizing antibodies (inhibitors), whereas both inhibitors and nonneutralizing antibodies can be detected by immunoassays such as enzyme-linked immunosorbent assay (ELISA) and multiplex bead-based assays.

OBJECTIVES

Evaluation of an in-house Luminex bead-based assay (LumiTope) compared with a commercially available ELISA and NBA.

METHODS

The LumiTope method comprised full-length and B-domain-deleted FVIII as well as 9 purified FVIII single or multidomains. The respective proteins were coupled to magnetic beads to detect domain-specific immunoglobulin (IgG; IgG) anti-FVIII antibodies in a large cohort of patients with hemophilia A with and without inhibitors.

RESULTS

Overall, LumiTope assay had a high sensitivity (94.9%) and specificity (91.2%), particularly in patients with low-titer inhibitors compared with ELISA (sensitivity of 72.2% vs 27.7%). IgG was the most abundant IgG subclass in NBA-positive patients. NBA-positive and -negative patients showed different domain profiles. Patients with genetic variants in the heavy chain predominantly exhibited antibodies specific to this chain, while those with a light-chain variant showed a more diverse distribution of antibody specificities. Patients with an intron 22 inversion resembled those with a light-chain defect, with a majority of antibodies targeting the light chain.

CONCLUSION

LumiTope assay provides a sensitive and specific method for not only detection but also domain specification of anti-FVIII-antibodies. Implementation of bead-based assays could improve antibody detection, profiling, and comparability of results and complement NBA.

摘要

背景

抗凝血因子(F)VIII抗体是重度甲型血友病患者治疗中的主要并发症。奈梅亨-贝塞斯达检测法(NBA)是检测中和抗体(抑制剂)的金标准,而酶联免疫吸附测定(ELISA)和基于多重微珠的检测等免疫测定法可检测抑制剂和非中和抗体。

目的

将一种内部开发的基于Luminex微珠的检测法(LumiTope)与市售ELISA和NBA进行比较评估。

方法

LumiTope方法包含全长和B结构域缺失的FVIII以及9种纯化的FVIII单结构域或多结构域。将各自的蛋白质偶联到磁珠上,以检测一大群有或无抑制剂的甲型血友病患者中结构域特异性免疫球蛋白(IgG;IgG)抗FVIII抗体。

结果

总体而言,LumiTope检测法具有较高的灵敏度(94.9%)和特异性(91.2%),特别是与ELISA相比,在低滴度抑制剂患者中(灵敏度分别为72.2%和27.7%)。IgG是NBA阳性患者中最丰富的IgG亚类。NBA阳性和阴性患者表现出不同的结构域谱。重链存在基因变异的患者主要表现出针对该链特异性的抗体,而轻链变异的患者抗体特异性分布更为多样。内含子22倒位的患者与轻链缺陷患者相似,大多数抗体靶向轻链。

结论

LumiTope检测法不仅为抗FVIII抗体的检测提供了一种灵敏且特异的方法,还能对其结构域进行鉴定。基于微珠的检测法的应用可改善抗体检测、分析以及结果的可比性,并补充NBA检测法。

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