基于DNA测序和多特异性单克隆抗体(Msmab-1)的免疫组化检测急性髓系白血病IDH1/2突变的比较

Akanksha Agarwal, Mili Jain, R. Kushwaha, S. Tewari, S. Nayak, Nishant Verma, A. Tripathi, Ashutosh Kumar
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摘要

背景:IDH1/2突变是参与AML发病的重要表观遗传修饰因子。它与AML患者的不同预后有关。缺乏适当的分子诊断基础设施和高成本限制了PCR与测序作为常规诊断方法的常规使用。本研究的目的是利用PCR测序和免疫组织化学方法发现AML病例中IDH突变的患病率。方法:我们对60例在勒克瑙KGMU登记的AML患者进行诊断和治疗。进行PCR和测序。使用骨活检或血块切片对所有病例(在儿童AML病例中)进行IDH1/2突变的免疫组化染色。结果:60例AML患者中有4例(6.7%)患者有IDH1R312突变,5例(8.3%)患者有IDH2R172突变。所有样本均未检测到IDH2 R140突变。免疫组化分析10例患者抗IDH1/2突变体(R132/R172)抗体阳性,克隆MsMab-1,敏感性77.8%,特异性94.1%。结论:免疫组化可作为直接Sanger测序检测AML患者IDH1/2突变的替代方法。然而,研究中使用的抗体对IDH1和IDH2突变的个体评估并不有效。关键词:免疫组织化学,Sanger测序,IDH1/2突变,急性髓系白血病
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Comparison of DNA Sequencing and Multispecific Monoclonal Antibody (Msmab-1) based Immunohistochemical Detection of IDH1/2 Mutation in Acute Myeloid Leukemia Cases.
Background: The IDH1/2 mutation is an important epigenetic modifier involved in the pathogenesis of AML. It is associated with variable prognosis in AML cases. Lack of proper molecular diagnostic infrastructure and high cost limits the routine use of PCR with sequencing as routine diagnostic methodology. The aim of this study was to find the prevalence of IDH mutation in AML cases using both PCR with sequencing and Immunohistochemistry method. Methods: We evaluated 60 patients registered at KGMU, Lucknow for diagnosis and treatment of AML. PCR followed by sequencing was done. IHC staining of the IDH1/2 mutation was performed on all cases using bone biopsy or clot section (in cases of pediatric AML cases). Results: Out of the total 60 patients of AML 4(6.7%) patients had IDH1R312 mutation and 5(8.3%) Patients had IDH2R172 mutation. IDH2 R140 mutation was not detected in any sample. On immunohistochemistry analysis 10 cases showed positive staining against anti IDH1/2 mutant (R132/R172) antibody, clone MsMab-1 with a sensitivity of 77.8% and specificity of 94.1%. Conclusion: IHC could be an alternative method to direct Sanger sequencing for IDH1/2 mutation detection in AML cases. However, the antibody used in the study is not effective for individual assessment of IDH1 and IDH2 mutation. Keywords: Immunohistochemistry, Sanger sequencing, IDH1/2 Mutation, Acute Myeloid Leukemia
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