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使用体外集落测定法对急性淋巴细胞白血病中克隆形成细胞进行免疫表型分析。

Immunophenotypic analysis of clonogenic cells in acute lymphoblastic leukemia using an in vitro colony assay.

作者信息

Hudson A M, Makrynikola V, Kabral A, Bradstock K F

机构信息

Haematology Department, Westmead Hospital, Australia.

出版信息

Blood. 1989 Nov 1;74(6):2112-20.

PMID:2804349
Abstract

A culture system was used to analyze the expression of membrane differentiation antigens on the proliferative or clonogenic fraction of cells from cases of common (precursor B) acute lymphoblastic leukemia (c-ALL). Colonies of leukemic cells were obtained in 18 of 20 cases after 1 week in culture in a liquid layer containing recombinant interleukin-2 (IL-2), phytohemagglutinin (PHA), and B-cell growth factor over an agar feeder layer containing irradiated peripheral blood mononuclear cells plus fetal calf serum (FCS) and horse serum. Cultured cells expressed HLA-DR, CD-9, CD-10, CD-20, and CD-34 antigens, indicating conservation of precursor B phenotype. Differentiation antigen expression on the clonogenic subpopulation giving rise to leukemic colonies was assessed by treating cells prior to culture with selected cytotoxic monoclonal antibodies (MoAbs) and complement or by fluorescence-activated cell sorting. Lytic treatment with HLA-DR, CD-10, CD-9, and CD-20 antibodies produced median reductions in colony formation of 93%, 81%, 73%, and 58% respectively. Combined treatment with CD-9 and CD-10 antibodies produced complete inhibition in 11 of 13 cases. Cell-sorting experiments after CD-10 staining indicated a good correlation with complement lysis studies and also demonstrated that the CD-19 antigen is expressed on a high proportion of clonogenic cells. Colony formation was also significantly reduced in 13 of 17 cases by lytic treatment of cells with the CD-33 antibody MY-9, suggesting expression of this "myeloid" lineage antigen on ALL clonogenic cells. The substantial case-to-case variation in expression of individual differentiation antigens indicates that leukemic cellular heterogeneity is a major consideration in ex vivo bone marrow purging using MoAbs and emphasizes the need for more critical evaluation of purging techniques.

摘要

采用一种培养系统来分析普通(前体B)急性淋巴细胞白血病(c-ALL)病例中细胞增殖或克隆形成部分的膜分化抗原表达。在含有重组白细胞介素-2(IL-2)、植物血凝素(PHA)和B细胞生长因子的液体层中,于含有经照射的外周血单核细胞加胎牛血清(FCS)和马血清的琼脂饲养层上培养1周后,20例中有18例获得了白血病细胞集落。培养的细胞表达HLA-DR、CD-9、CD-10、CD-20和CD-34抗原,表明前体B表型得以保留。通过在培养前用选定的细胞毒性单克隆抗体(MoAbs)和补体处理细胞或通过荧光激活细胞分选来评估产生白血病集落的克隆形成亚群上的分化抗原表达。用HLA-DR、CD-10、CD-9和CD-20抗体进行裂解处理分别使集落形成的中位数减少了93%、81%、73%和58%。用CD-9和CD-10抗体联合处理在13例中有11例产生了完全抑制。CD-10染色后的细胞分选实验表明与补体裂解研究有良好的相关性,并且还证明CD-19抗原在高比例的克隆形成细胞上表达。用CD-33抗体MY-9对细胞进行裂解处理在17例中有13例集落形成也显著减少,表明该“髓系”谱系抗原在ALL克隆形成细胞上表达。个体分化抗原表达在病例之间存在很大差异,这表明白血病细胞的异质性是使用MoAbs进行体外骨髓净化时的一个主要考虑因素,并强调需要对净化技术进行更严格的评估。

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