Platelet antibody detection assays: a single-laboratory comparison of MAIPA, PIFT, and microsphere-based multiplex assays Pak-Lx.

Thiago Henrique Costa, Carolina Bonet-Bub, José Mauro Kutner
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Abstract

Background and objectives: The identification of platelet antibodies is essential for diagnosing and managing conditions such as fetal and neonatal alloimmune thrombocytopenic purpura, post-transfusion purpura, and immune platelet refractoriness. Monoclonal antibody immobilization of platelet antigens (MAIPA) is the standard method for detecting anti-human platelet antigen (HPA) antibodies, while the detection of anti-HLA antibodies once relied on the complement-dependent cytotoxicity method, however advanced technologies such as enzyme-linked immunosorbent assay and Luminex have significantly improved sensitivity and accuracy in identifying these antibodies. Flow cytometry-based techniques (platelet immunofluorescence test - PIFT) and Luminex platform-driven microsphere-based multiplex assays (Pak-Lx) are widely employed in platelet immunology laboratories owing to their remarkable flexibility and versatility. The present study compared the sensitivity, specificity, and concordance of these different serological techniques used in platelet antibody identification.

Material and methods: One hundred serum samples from patients suspected of immune-mediated platelet disorders were examined. Initially, the samples underwent testing using the MAIPA method. Subsequently, the results were compared with three alternative methods: PIFT and microsphere-based multiplex assays for both HLA and HPA antibodies.

Results: Pak-Lx demonstrated a 94 % agreement with MAIPA, while PIFT had 88 % agreement for HPA antibodies. For HLA antibody detection, Pak-Lx versus DLX had 75 % concordance, MAIPA versus DLX showed 77 %, and PIFT versus DLX displayed an 81 % concordance rate. Remarkably, there were no significant differences in concordance levels between Pak-Lx and PIFT compared to MAIPA and DLX for anti-HPA and HLA antibodies, respectively.

Conclusion: This study found no significant differences in concordance among the tested assays for detecting anti-HPA and anti-HLA antibodies. These data suggest that no single method can detect all clinically important antibodies. Therefore, it is advisable that each laboratory develops customized protocols based on their expertise and employs complementary methods for comprehensive patient assessments.

血小板抗体检测测定:MAIPA、PIFT 和基于微球的多重测定 Pak-Lx 的单实验室比较。
背景和目的:血小板抗体的鉴定对于诊断和处理诸如胎儿和新生儿同种免疫性血小板减少性紫癜、输血后紫癜和免疫性血小板耐药等疾病至关重要。血小板抗原单克隆抗体固定化法(MAIPA)是检测抗人血小板抗原(HPA)抗体的标准方法,而抗 HLA 抗体的检测曾经依赖于补体依赖性细胞毒性法,但酶联免疫吸附试验和 Luminex 等先进技术大大提高了鉴定这些抗体的灵敏度和准确性。基于流式细胞仪的技术(血小板免疫荧光检测--PIFT)和基于微球的Luminex平台驱动的多重检测(Pak-Lx)因其出色的灵活性和多功能性而被血小板免疫学实验室广泛采用。本研究比较了这些用于血小板抗体鉴定的不同血清学技术的灵敏度、特异性和一致性:材料和方法:研究人员检测了 100 份疑似免疫介导血小板疾病患者的血清样本。这些样本首先使用 MAIPA 方法进行检测。随后,将结果与三种替代方法进行比较:结果:结果:Pak-Lx 与 MAIPA 的一致性为 94%,而 PIFT 与 HPA 抗体的一致性为 88%。在 HLA 抗体检测方面,Pak-Lx 与 DLX 的一致性为 75%,MAIPA 与 DLX 的一致性为 77%,PIFT 与 DLX 的一致性为 81%。值得注意的是,与 MAIPA 和 DLX 相比,Pak-Lx 和 PIFT 在抗 HPA 和 HLA 抗体方面的一致性水平没有明显差异:结论:本研究发现,在检测抗 HPA 和抗 HLA 抗体时,所测试的检测方法在一致性方面没有明显差异。这些数据表明,没有一种方法能检测出所有临床上重要的抗体。因此,建议各实验室根据自己的专长制定个性化方案,并采用互补方法对患者进行全面评估。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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