FLAER as a standalone reagent for paroxysmal nocturnal hemoglobinuria: Do we need to reconsider the guidelines for testing?

被引:0
|
作者
Sharma, Praveen [1 ]
Bose, Parveen [1 ]
Mallik, Nabhajit [1 ]
Gupta, Dikshat Gopal [2 ]
Rachagiri, Suneel [1 ]
Kumar, Arun [1 ]
Kaur, Jasbir [1 ]
Malhotra, Pankaj [3 ]
Varma, Neelam [1 ]
Sachdeva, Man Updesh Singh [1 ]
机构
[1] Post Grad Inst Med Educ & Res, Dept Hematol, Chandigarh 160012, India
[2] Northwestern Univ, Feinberg Sch Med, Robert H Lurie Comprehens Canc Ctr, Dept Urol, Chicago, IL USA
[3] Post Grad Inst Med Educ & Res, Dept Clin Hematol & Med Oncol, Chandigarh, India
关键词
CD55; CD59; FLAER; flow cytometry; PNH; ICCS/ESCCA CONSENSUS GUIDELINES; GPI-DEFICIENT CELLS; HIGH-SENSITIVITY DETECTION; COMPLEMENT REGULATORY PROTEIN; DECAY-ACCELERATING FACTOR; ANTIBODY CLONE SY11B5; PIG-A GENE; FLOW-CYTOMETRY; SOMATIC MUTATIONS; PERIPHERAL-BLOOD;
D O I
10.1111/ijlh.14213
中图分类号
R5 [内科学];
学科分类号
1002 ; 100201 ;
摘要
Introduction: Flow cytometry-based paroxysmal nocturnal hemoglobinuria (PNH) testing involves utilization of monoclonal antibodies against GPI-linked proteins and FLAER. The ability of FLAER to bind to a wide variety of GPI-linked structures and to be utilized across different leukocyte subsets is remarkable. We hypothesize that FLAER as a standalone reagent may be equally effective for detecting PNH clones. The present study intends to compare the results of a FLAER alone-based strategy to the recommended FLAER+GPI-linked protein-based approach for applicability in clinical settings.Methods: EDTA-anticoagulated blood samples from patients for PNH workup were tested for PNH by multiparametric flow cytometry. A conventional panel comprising gating markers (CD45 for WBC, CD15 for granulocytes, and CD64 for monocytes) and a combination of FLAER and GPI-linked markers, such as CD24 and CD14, henceforth referred to as the "routine panel," was employed. Second, a "FLAER-only panel" comprising the gating markers and FLAER alone (excluding the GPI-linked markers CD24 and CD14) was set up. The samples were processed using the lyse-wash-stain-wash technique, and events were acquired on BC Navios Ex flow cytometer (Beckman Coulter, Inc., USA) and analyzed on Kaluza Software 2.1. The presence of a PNH clone was reported at a value of >= 0.01%.Results: A total of 209 patients were tested. Both panels found a PNH clone in 20.1% of patients (n = 42/209) with a 100% concordance rate. The PNH clone range for granulocytes was 0.01%-89.68%, and for monocyte was 0.04%-96.09% in the routine panel. The range in the FLAER-only panel for granulocytes was 0.01%-89.61%, and for monocytes, it was 0.01%-96.05%. Pearson correlation statistics revealed a significant correlation between the size of the PNH clone of granulocytes and monocytes among the two panels tested (granulocytes r = 0.9999, p < 0.0001, 95% CI = 0.9999 to 1.000; monocytes r = 0.9974, p < 0.0001, 95% CI = 0.9966-0.9980).Conclusion: Based on our results, FLAER as a standalone marker is specific and sensitive for identifying PNH clones in granulocytes and monocytes, even for high-sensitivity PNH assay. The proposed "FLAER-only panel" panel is efficient and cost-effective for highly sensitive PNH testing in two different cell lineages, especially in resource-limited clinical settings.
引用
收藏
页码:383 / 389
页数:7
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