Berenstein Rimma, Blau Igor Wolfgang, Kar Asiye, Cay Ruhiye, Sindram Annette, Seide Claudia, Blau Olga
Department of Hematology, Oncology and Tumourimmunology, Charité Universitätsmedizin Berlin, Hindenburgdamm 30, 12200 Berlin, Germany.
J Exp Clin Cancer Res. 2014 May 21;33(1):44. doi: 10.1186/1756-9966-33-44.
Mutations in epigenetic modifiers were reported in patients with acute myeloid leukaemia (AML) including mutations in DNA methyltransferase 3A gene (DNMT3A) in 20%-30% patients and mutations in isocitrate dehydrogenase 1/2 gene (IDH1/2) in 5%-15% patients. Novel studies have shown that mutations in DNMT3A and IDH1/2 influence prognosis, indicating an increasing need to detect these mutations during routine laboratory analysis. DNA sequencing for the identification of these mutations is time-consuming and cost-intensive. This study aimed to establish rapid screening tests to identify mutations in DNMT3A and IDH1/2 that could be applied in routine laboratory procedures and that could influence initial patient management.
In this study we developed an endonuclease restriction method to identify the most common DNMT3A mutation (R882H) and an amplification-refractory mutation system (ARMS) to analyse IDH2 R140Q mutations. Furthermore, we compared these methods with HRM analysis and evaluated the latter for the detection of IDH1 mutations.
Of 230 samples from patients with AML 30 (13%) samples had DNMT3A mutations, 16 (7%) samples had IDH2 R140Q mutations and 36 (16%) samples had IDH1 mutations. Sensitivity assays performed using serial dilutions of mutated DNA showed that ARMS analysis had a sensitivity of 4.5%, endonuclease restriction had a sensitivity of 0.05% and HRM analysis had a sensitivity of 5.9%-7.8% for detecting different mutations. HRM analysis was the best screening method to determine the heterogeneity of IDH1 mutations. Furthermore, for the identification of mutations in IDH2 and DNMT3A, endonuclease restriction and ARMS methods showed a perfect concordance (100%) with Sanger sequencing while HRM analysis showed a near-perfect concordance (approximately 98%).
Our study suggested that all the developed methods were rapid, specific and easy to use and interpret. HRM analysis is the most timesaving and cost-efficient method to rapidly screen all the 3 genes at diagnosis in samples obtained from patients with AML. Endonuclease restriction and ARMS assays can be used separately or in combination with HRM analysis to obtain more reliable results. We propose that early screening of mutations in patients with AML having normal karyotype could facilitate risk stratification and improve treatment options.
急性髓系白血病(AML)患者中报道了表观遗传修饰因子的突变,包括20%-30%的患者存在DNA甲基转移酶3A基因(DNMT3A)突变,5%-15%的患者存在异柠檬酸脱氢酶1/2基因(IDH1/2)突变。新的研究表明,DNMT3A和IDH1/2突变会影响预后,这表明在常规实验室分析中检测这些突变的需求日益增加。通过DNA测序来鉴定这些突变既耗时又成本高昂。本研究旨在建立快速筛查试验,以鉴定DNMT3A和IDH1/2中的突变,这些突变可应用于常规实验室程序,并可能影响患者的初始管理。
在本研究中,我们开发了一种内切酶限制方法来鉴定最常见的DNMT3A突变(R882H),并开发了一种扩增阻滞突变系统(ARMS)来分析IDH2 R140Q突变。此外,我们将这些方法与高分辨率熔解曲线分析(HRM)进行了比较,并评估了HRM分析用于检测IDH1突变的效果。
在230例AML患者的样本中,30例(13%)样本存在DNMT3A突变,16例(7%)样本存在IDH2 R140Q突变,36例(16%)样本存在IDH1突变。使用突变DNA的系列稀释液进行的敏感性分析表明,ARMS分析检测不同突变的敏感性为4.5%,内切酶限制法的敏感性为0.05%,HRM分析的敏感性为5.9%-7.8%。HRM分析是确定IDH1突变异质性的最佳筛查方法。此外,对于IDH2和DNMT3A突变的鉴定,内切酶限制法和ARMS方法与桑格测序法显示出完全一致(100%),而HRM分析显示出近乎完全一致(约98%)。
我们的研究表明,所有开发的方法都快速、特异且易于使用和解读。HRM分析是在AML患者样本诊断时快速筛查所有这3个基因最省时且最具成本效益的方法。内切酶限制法和ARMS检测可单独使用或与HRM分析联合使用以获得更可靠的结果。我们建议对核型正常的AML患者进行突变的早期筛查有助于风险分层并改善治疗选择。
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