B型急性淋巴细胞白血病中白血病相关表型标记物的免疫表型表征。

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS
Emilia Boris, Alexandre Theron, Valentin Montagnon, Nicolas Rouquier, Marion Almeras, Jérôme Moreaux, Caroline Bret
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引用次数: 0

摘要

背景:多参数流式细胞术(MFC)是B型急性淋巴细胞白血病(B ALL)的重要诊断工具,用于确定母细胞群体的B系关系并确定其完整的免疫表型谱。常规实验室中使用的大多数MFC策略包括白血病相关表型(LAP)标记,其表达谱难以解释。我们的研究目的是为了更好地了解7种LAP标记物在B ALL中的作用:CD9、CD21、CD66c、CD58、CD81、CD123和NG2。方法:采用10色MFC方法,我们评估了7种LAP标志物CD9、CD21、CD66c、CD58、CD81、CD123和NG2在正常外周血白细胞(n = 10个健康供者)、正常前体B再生细胞(n = 40个未受损伤骨髓样本)和淋巴母细胞(n = 100个诊断时B ALL患者外周血或骨髓样本)表面的表达水平。根据复发性细胞遗传异常的存在与否分析B淋巴细胞的表达谱。采用Maxstat R算法检测7种LAP标记物的预后价值。结果:为了帮助解释常规实验室的MFC数据,我们首先确定了正常白细胞中7种评估的LAP标记物的内部阳性和阴性群体。其次,将它们在正常B细胞分化中的表达谱与B淋巴母细胞的表达谱进行比较,以建立它们在正常造血中的表达概况。然后,我们评估了这些LAP标记物在B淋巴细胞表面的表达频率,以诊断B淋巴细胞白血病。CD9在60%的病例中表达,CD21在3%的病例中表达,CD58在96%的病例中表达,CD66c在45%的病例中表达,CD81在97%的病例中表达,CD123在72%的病例中表达,而NG2仅在2%的病例中表达。我们证实了CD81/CD58 MFI表达比作为区分造血细胞和淋巴细胞的一种方法的兴趣。我们观察到,与没有复发性细胞遗传学改变的B淋巴母细胞(p = 0.0317和p = 0.0011)以及具有其他细胞遗传学复发异常的B淋巴母细胞(p = 0.0032和p)相比,具有t(9;22)(BCR-ABL)的B淋巴母细胞表面CD9和CD81的表达显著降低(p = 0.0317和p = 0.0011)。结论:淋巴母细胞在B ALL诊断时的表型特征的复杂性可以通过LAP抗原表达的变异性来说明。了解这些标志物在正常白细胞和正常B细胞分化过程中的表达水平对于最佳解释诊断细胞术结果至关重要,并可作为B ALL生物学随访的基础。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Immunophenotypic portrait of leukemia-associated-phenotype markers in B acute lymphoblastic leukemia

Immunophenotypic portrait of leukemia-associated-phenotype markers in B acute lymphoblastic leukemia

Background

Multiparametric flow cytometry (MFC) is an essential diagnostic tool in B acute lymphoblastic leukemia (B ALL) to determine the B-lineage affiliation of the blast population and to define their complete immunophenotypic profile. Most MFC strategies used in routine laboratories include leukemia-associated phenotype (LAP) markers, whose expression profiles can be difficult to interpret. The aim of our study was to reach a better understanding of 7 LAP markers' landscape in B ALL: CD9, CD21, CD66c, CD58, CD81, CD123, and NG2.

Methods

Using a 10-color MFC approach, we evaluated the level of expression of 7 LAP markers including CD9, CD21, CD66c, CD58, CD81, CD123, and NG2, at the surface of normal peripheral blood leukocytes (n = 10 healthy donors), of normal precursor B regenerative cells (n = 40 uninvolved bone marrow samples) and of lymphoblasts (n = 100 peripheral blood samples or bone marrow samples from B ALL patients at diagnosis). The expression profile of B lymphoblasts was analyzed according the presence or absence of recurrent cytogenetic aberrations. The prognostic value of the 7 LAP markers was examined using Maxstat R algorithm.

Results

In order to help the interpretation of the MFC data in routine laboratories, we first determined internal positive and negative populations among normal leukocytes for each of the seven evaluated LAP markers. Second, their profile of expression was evaluated in normal B cell differentiation in comparison with B lymphoblasts to establish a synopsis of their expression in normal hematogones. We then evaluated the frequency of expression of these LAP markers at the surface of B lymphoblasts at diagnosis of B ALL. CD9 was expressed in 60% of the cases, CD21 in only 3% of the cases, CD58 in 96% of the cases, CD66c in 45% of the cases, CD81 in 97% of the cases, CD123 in 72% of the cases, and NG2 in only 2% of the cases. We confirmed the interest of the CD81/CD58 MFI expression ratio as a way to discriminate hematogones from lymphoblasts. We observed a significant lower expression of CD9 and of CD81 at the surface of B lymphoblasts with a t(9;22)(BCR-ABL) in comparison with B lymphoblasts without any recurrent cytogenetic alteration (p = 0.0317 and p = 0.0011, respectively) and with B lymphoblasts harboring other cytogenetic recurrent abnormalities (p = 0.0032 and p < 0.0001, respectively). B lymphoblasts with t(1;19) at diagnosis significantly overexpressed CD81 when compared with B lymphoblasts with other recurrent cytogenetic abnormalities or without any recurrent alteration (p = 0.0001). An overexpression of CD58 was also observed in the cases harboring this abnormal cytogenetic event, when compared with B lymphoblasts with other recurrent cytogenetic abnormalities (p = 0.030), or without any recurrent alteration (p = 0.0002). In addition, a high expression of CD123, of CD58 and of CD81 was associated with a favorable prognosis in our cohort of pediatric and young adult B ALL patients. We finally built a risk score based on the expression of these 3 LAP markers, this scoring approach being able to split these patients into a high-risk group (17%) and a better outcome group (83%, p < 0.0001).

Conclusion

The complexity of the phenotypic signature of lymphoblasts at diagnosis of B ALL is illustrated by the variability in the expression of LAP antigens. Knowledge of the expression levels of these markers in normal leukocytes and during normal B differentiation is crucial for an optimal interpretation of diagnostic cytometry results and serves as a basis for the biological follow-up of B ALL.

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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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