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Standardization and quality control studies of ‘real-time’ quantitative reverse transcriptase polymerase chain reaction of fusion gene transcripts for residual disease detection in leukemia – A Europe Against Cancer Program

微小残留病 急性早幼粒细胞白血病 髓系白血病 白血病 医学 塔克曼 实时聚合酶链反应 生物 金标准(测试) 肿瘤科 基因 融合基因 免疫学 内科学 遗传学 维甲酸
作者
Jean Gabert,Emmanuel Beillard,Vincent H.J. van der Velden,W Bi,David Grimwade,Niels Pallisgaard,Gisela Barbany,Giovanni Cazzaniga,Jean‐Michel Cayuela,Hélène Cavé,Fabrizio Pane,Joeri L. Aerts,Daniela De Micheli,Xavier Thirion,Vincent Pradel,Marcos González,Susanne Viehmann,Maria Malec,Giuseppe Saglio,Jacques J. M. van Dongen
出处
期刊:Leukemia [Springer Nature]
卷期号:17 (12): 2318-2357 被引量:1438
标识
DOI:10.1038/sj.leu.2403135
摘要

Detection of minimal residual disease (MRD) has proven to provide independent prognostic information for treatment stratification in several types of leukemias such as childhood acute lymphoblastic leukemia (ALL), chronic myeloid leukemia (CML) and acute promyelocytc leukemia. This report focuses on the accurate quantitative measurement of fusion gene (FG) transcripts as can be applied in 35-45% of ALL and acute myeloid leukemia, and in more than 90% of CML. A total of 26 European university laboratories from 10 countries have collaborated to establish a standardized protocol for TaqMan-based real-time quantitative PCR (RQ-PCR) analysis of the main leukemia-associated FGs within the Europe Against Cancer EAC) program. Four phases were scheduled: (1) training, (2) optimization, (3) sensitivity testing and (4) patient sample testing. During our program, three quality control rounds on a large series of coded RNA samples were performed including a balanced randomized assay, which enabled final validation of the EAC primer and probe sets. The expression level of the nine major FG transcripts in a large series of stored diagnostic leukemia samples (n = 278) was evaluated. After normalization, no statistically significant difference in expression level was observed between bone marrow and peripheral blood on paired samples at diagnosis. However, RQ-PCR revealed marked differences in FG expression between transcripts in leukemic samples at diagnosis that could account for differential assay sensitivity. The development of standardized protocols for RQ-PCR analysis of FG transcripts provides a milestone for molecular determination of MRD levels. This is likely to prove invaluable to the management of patients entered into multicenter therapeutic trials.
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