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Differentiation of acute myeloid leukemia from B- and T-lineage acute lymphoid leukemias by real-time quantitative reverse transcription-PCR of lineage marker mRNAs.

机译:通过沿袭谱系标记物mRNA的实时定量逆转录PCR,从B和T系急性淋巴细胞白血病中区分出急性髓细胞性白血病。

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摘要

BACKGROUND: Flow cytometry of lineage markers is useful in the classification of leukemias. Our aim was to assess whether the study of lineage genes at the RNA level would enable differentiation of acute myeloid leukemias (AMLs) from B-and T-lineage acute lymphoid leukemias (ALLs). METHODS: We measured mRNA of four lineage markers [CD19, CD79a, CD3e, and myeloperoxidase (MPO)] by reverse transcription followed by real-time quantitative (RTQ)-PCR. We investigated 72 acute leukemias (40 AMLs with 23-93% blast cells plus 27 B-lineage ALLs and 5 T-lineage ALLs) defined by morphologic criteria at diagnosis. RTQ-PCR analysis was performed on bone marrow without cell sorting. The expression of each gene was calculated as the difference in the threshold cycle [DeltaCT; CT value of target gene minus CT value of housekeeping gene (Abelson)]. RESULTS: Three patterns of expression were detected. In the first, CD19, CD79a, and MPO mRNAs were less abundant than CD3e. In the second pattern, MPO mRNA was more abundant than the other three mRNAs. In the third, CD19 or CD79a was more highly expressed than CD3e and MPO. The three patterns corresponded to T-ALL, AML, and B-ALL, respectively. The use of cutoffs to establish qualitatively the pattern of coexpression of the four lineage markers provided the same information as the comparison among the four DeltaCT values. Prospective use of the scoring system correctly classified each of 13 additional cases (8 AML, 4 B-lineage ALL, and 1 T-lineage ALL). CONCLUSION: Study of lineage markers at diagnosis by RTQ-PCR allows differentiation of AML from B-ALL or T-ALL without cell sorting, even when the bone marrow contains few blast cells.
机译:背景:沿袭标记的流式细胞仪可用于白血病的分类。我们的目的是评估在RNA水平上对谱系基因的研究是否能够使急性髓系白血病(AML)与B和T谱系急性淋巴白血病(ALL)区分。方法:我们通过逆转录然后实时定量(RTQ)-PCR测量了四个谱系标记[CD19,CD79a,CD3e和髓过氧化物酶(MPO)]的mRNA。我们在诊断时调查了由形态学标准定义的72例急性白血病(40例AML,其中23-93%的原始细胞加上27例B谱系ALL和5例T谱系ALL)。在不进行细胞分选的情况下,对骨髓进行了RTQ-PCR分析。计算每个基因的表达,作为阈值循环中的差异[DeltaCT;靶基因的CT值减去管家基因的CT值(Abelson)]。结果:检测到三种表达模式。首先,CD19,CD79a和MPO mRNA不如CD3e丰富。在第二种模式中,MPO mRNA比其他三种mRNA更丰富。在第三种中,CD19或CD79a比CD3e和MPO高表达。这三种模式分别对应于T-ALL,AML和B-ALL。使用截断定性建立四个谱系标记的共表达模式提供了与四个DeltaCT值之间的比较相同的信息。计分系统的预期使用正确地对13种其他情况(8种AML,4种B谱系ALL和1种T谱系ALL)进行了正确分类。结论:通过RTQ-PCR在诊断时研究谱系标记,可以将AML与B-ALL或T-ALL进行区分,而无需进行细胞分选,即使骨髓中的胚细胞很少。

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