Karela Christina, Tsagarakis Nikolaos J, Oudatzis Georgios, Xanthopoulos Vasileios, Milaiou Maroula, Nikolaou Sofia, Zina Vassiliki, Vasileiou Paraskevi, Karianakis Georgios, Marinakis Theodoros, Griva Elpiniki, Paterakis Georgios
Department of Immunology, General Hospital of Athens "G. Gennimatas", Athens, Greece.
Hematology Laboratory, General Hospital of Athens "G. Gennimatas", Athens, Greece.
Int J Lab Hematol. 2025 Apr;47(2):228-235. doi: 10.1111/ijlh.14394. Epub 2024 Oct 30.
Fluorescently labeled aerolysin (FLAER) is widely used for the identification of paroxysmal nocturnal hemoglobinuria (PNH) clones in peripheral blood (PB) samples. However, there are only a few reports on the differential fluorescent intensity of FLAER in normal bone marrow (BM) cell subpopulations. The purpose of this study was to evaluate FLAER expression during normal and pathological hematopoiesis, to map the critical existence of non-PNH FLAER-dim cells.
A total of 54 BM aspirates were prospectively analyzed with FLAER-based flow cytometric (FC) protocols, during their routine work-up. These were obtained from patients with the following diagnoses: PNH (3), infections/reactive (5), myelodysplastic syndromes (MDS) (7), myelodysplastic/myeloproliferative neoplasms (MDS/MPN) (4), chronic myelogenous leukemia (CML) (3), acute myelogenous leukemia (AML) at diagnosis (20), AML in measurable residual disease (MRD) assessment (7), and B-cell acute lymphoblastic leukemia (B-ALL) in MRD assessment (5). The applied protocols consisted of FLAER, HLA-DR, CD14, CD33, CD34, CD66b, CD38, CD117, CD64, CD45, and FLAER, CD66c, CD14, CD33, CD34, CD66b, CD123, CD16, CD64, and CD45, respectively. FLAER expression was assessed in CD34++/CD38- and CD34+/CD38+ stem cells, CD34-/CD117+/HLA-DR+/CD33+ myeloid precursors, and CD64+/CD14-/HLA-DR+ monocyte precursors but also in mature myeloid cells.
All patients revealed an intermediate FLAER intensity in CD34++/CD38- stem cells, with a discrete FLAER-negative subpopulation observed only in maturing CD34+/CD38+ stem cells of patients with PNH. The lowest FLAER intensity was noticed in CD34-/CD117+/HLA-DR+/CD33+ myeloid precursors, not only in patients with PNH but also in PNH-negative BM aspirates. An ascending FLAER intensity was further observed during monocytic and granulocytic maturation, with a discrete FLAER-negative population in CD64+/CD14-/HLA-DR+ monocyte precursors and maturing neutrophils and monocytes of patients with PNH only. The maturation pattern of FLAER expression was further confirmed in a patient with acute promyelocytic leukemia treated with all-trans retinoic acid (ATRA), where FLAER was concurrently upregulated with CD66b in a consecutive series of PB samples tested over a 20-day-period after diagnosis.
The application of FLAER in PNH-positive and PNH-negative reactive or malignant BM aspirates identified normally expected non-PNH FLAER-dim CD34-/CD117+/HLA-DR+/CD33+ myeloid precursors in all samples. A specific FLAER-associated maturation pattern was observed, which is proposed for further study within MRD and diagnostic protocols.
荧光标记气单胞菌溶素(FLAER)广泛用于鉴定外周血(PB)样本中的阵发性睡眠性血红蛋白尿(PNH)克隆。然而,关于正常骨髓(BM)细胞亚群中FLAER荧光强度差异的报道较少。本研究旨在评估正常和病理造血过程中FLAER的表达情况,以明确非PNH FLAER低荧光细胞的关键存在情况。
在54例骨髓穿刺液的常规检查过程中,采用基于FLAER的流式细胞术(FC)方案进行前瞻性分析。这些样本来自以下诊断的患者:PNH(3例)、感染/反应性疾病(5例)、骨髓增生异常综合征(MDS)(7例)、骨髓增生异常/骨髓增殖性肿瘤(MDS/MPN)(4例)、慢性粒细胞白血病(CML)(3例)、初诊急性髓系白血病(AML)(20例)、可测量残留病(MRD)评估中的AML(7例)以及MRD评估中的B细胞急性淋巴细胞白血病(B-ALL)(5例)。所应用的方案分别包括FLAER、HLA-DR、CD14、CD33、CD34、CD66b、CD38、CD117、CD6,4、CD45,以及FLAER、CD66c、CD14、CD33、CD34、CD66b、CD123、CD16、CD64和CD45。在CD34++/CD38-和CD34+/CD38+干细胞、CD34-/CD117+/HLA-DR+/CD33+髓系前体细胞以及CD64+/CD14-/HLA-DR+单核细胞前体细胞中评估FLAER表达,同时也在成熟髓系细胞中进行评估。
所有患者的CD34++/CD38-干细胞均显示中等强度的FLAER荧光,仅在PNH患者成熟的CD34+/CD38+干细胞中观察到离散的FLAER阴性亚群。在CD34-/CD117+/HLA-DR+/CD33+髓系前体细胞中观察到最低的FLAER荧光强度,不仅在PNH患者中如此,在PNH阴性的骨髓穿刺液中也是如此。在单核细胞和粒细胞成熟过程中进一步观察到FLAER荧光强度逐渐升高,仅在PNH患者的CD64+/CD14-/HLA-DR+单核细胞前体细胞以及成熟的中性粒细胞和单核细胞中存在离散的FLAER阴性群体。在一名接受全反式维甲酸(ATRA)治疗的急性早幼粒细胞白血病患者中进一步证实了FLAER表达的成熟模式,在诊断后的20天内连续检测的一系列外周血样本中,FLAER与CD66b同时上调。
在PNH阳性和PNH阴性的反应性或恶性骨髓穿刺液中应用FLAER,在所有样本中均鉴定出正常预期的非PNH FLAER低荧光CD34-/CD117+/HLA-DR+/CD33+髓系前体细胞。观察到一种特定的与FLAER相关的成熟模式,建议在MRD和诊断方案中进一步研究。
