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1
Detection of minor clones with internal tandem duplication mutations of FLT3 gene in acute myeloid leukemia using delta-PCR.使用delta-PCR检测急性髓系白血病中具有FLT3基因内部串联重复突变的微小克隆。
Diagn Mol Pathol. 2013 Mar;22(1):1-9. doi: 10.1097/PDM.0b013e31825d81f4.
2
Δ-PCR, A Simple Method to Detect Translocations and Insertion/Deletion Mutations.Δ-PCR,一种用于检测易位和插入/缺失突变的简单方法。
J Mol Diagn. 2011 Jan;13(1):85-92. doi: 10.1016/j.jmoldx.2010.11.004. Epub 2010 Dec 23.
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A molecular fraction collecting tool for the ABI 310 automated sequencer.用于ABI 310自动测序仪的分子级分收集工具。
J Mol Diagn. 2007 Nov;9(5):598-603. doi: 10.2353/jmoldx.2007.070022. Epub 2007 Oct 4.
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Processes of de novo duplication of human alpha-globin genes.人类α-珠蛋白基因的从头复制过程。
Proc Natl Acad Sci U S A. 2007 Jun 26;104(26):10950-5. doi: 10.1073/pnas.0703856104. Epub 2007 Jun 15.
5
FLT3 length mutations as marker for follow-up studies in acute myeloid leukaemia.FLT3长度突变作为急性髓系白血病随访研究的标志物
Acta Haematol. 2004;112(1-2):68-78. doi: 10.1159/000077561.
6
Detection of FLT3 internal tandem duplication and D835 mutations by a multiplex polymerase chain reaction and capillary electrophoresis assay.通过多重聚合酶链反应和毛细管电泳分析法检测FLT3内部串联重复和D835突变。
J Mol Diagn. 2003 May;5(2):96-102. doi: 10.1016/S1525-1578(10)60458-8.
7
Internal tandem duplication of FLT3 in relapsed acute myeloid leukemia: a comparative analysis of bone marrow samples from 108 adult patients at diagnosis and relapse.复发急性髓系白血病中FLT3的内部串联重复:108例成年患者诊断和复发时骨髓样本的比较分析
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Analysis of FLT3 length mutations in 1003 patients with acute myeloid leukemia: correlation to cytogenetics, FAB subtype, and prognosis in the AMLCG study and usefulness as a marker for the detection of minimal residual disease.1003例急性髓系白血病患者FLT3长度突变分析:与细胞遗传学、FAB亚型的相关性及在AMLCG研究中的预后,以及作为检测微小残留病标志物的实用性。
Blood. 2002 Jul 1;100(1):59-66. doi: 10.1182/blood.v100.1.59.
9
Analysis of FLT3-activating mutations in 979 patients with acute myelogenous leukemia: association with FAB subtypes and identification of subgroups with poor prognosis.979例急性髓性白血病患者FLT3激活突变分析:与FAB亚型的关联及预后不良亚组的鉴定
Blood. 2002 Jun 15;99(12):4326-35. doi: 10.1182/blood.v99.12.4326.
10
Quantitative, real-time polymerase chain reactions for FLT3 internal tandem duplications are highly sensitive and specific.用于检测FLT3内部串联重复序列的定量实时聚合酶链反应具有高度的敏感性和特异性。
Leuk Res. 2001 Dec;25(12):1085-8. doi: 10.1016/s0145-2126(01)00087-x.

串联重复聚合酶链反应:一种用于检测FLT3基因内部串联重复的超灵敏检测方法。

Tandem duplication PCR: an ultrasensitive assay for the detection of internal tandem duplications of the FLT3 gene.

作者信息

Lin Ming-Tseh, Tseng Li-Hui, Beierl Katie, Hsieh Antony, Thiess Michele, Chase Nadine, Stafford Amanda, Levis Mark J, Eshleman James R, Gocke Christopher D

机构信息

Department of Pathology, Johns Hopkins University School of Medicine, Baltimore, MD 21287, USA.

出版信息

Diagn Mol Pathol. 2013 Sep;22(3):149-55. doi: 10.1097/PDM.0b013e31828308a1.

DOI:10.1097/PDM.0b013e31828308a1
PMID:23846441
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3744591/
Abstract

Internal tandem duplication (ITD) mutations of the FLT3 gene have been associated with a poor prognosis in acute myeloid leukemia. Detection of ITD-positive minor clones at the initial diagnosis and during the minimal residual disease stage may be essential. We previously designed a delta-PCR strategy to improve the sensitivity to 0.1% ITD-positive leukemia cells and showed that minor mutants with an allele burden of <1% can be clinically significant. In this study, we report on tandem duplication PCR (TD-PCR), a modified inverse PCR assay, and demonstrate a limit of detection of a few molecules of ITD mutants. The TD-PCR was initially designed to confirm ITD mutation of an amplicon, which was undetectable by capillary electrophoresis and was incidentally isolated by a molecular fraction collecting tool. Subsequently, TD-PCR detected ITD mutation in 2 of 77 patients previously reported as negative for ITD mutation by a standard PCR assay. TD-PCR can also potentially be applied to monitor minimal residual disease with high analytic sensitivity in a portion of ITD-positive acute myeloid leukemia patients. Further studies using TD-PCR to detect ITD mutants at diagnosis may clarify the clinical significance of those ITD mutants with extremely low allele burden.

摘要

FLT3基因的内部串联重复(ITD)突变与急性髓系白血病的不良预后相关。在初始诊断时以及微小残留病阶段检测ITD阳性微小克隆可能至关重要。我们之前设计了一种delta-PCR策略,将灵敏度提高到0.1%的ITD阳性白血病细胞,并表明等位基因负担<1%的微小突变体可能具有临床意义。在本研究中,我们报告了串联重复PCR(TD-PCR),一种改良的反向PCR检测方法,并证明了对少量ITD突变体分子的检测限。TD-PCR最初设计用于确认一个扩增子的ITD突变,该扩增子通过毛细管电泳无法检测到,并通过分子级分收集工具偶然分离得到。随后,TD-PCR在77例之前标准PCR检测报告为ITD突变阴性的患者中检测到2例ITD突变。TD-PCR还可能潜在地应用于监测一部分ITD阳性急性髓系白血病患者的微小残留病,具有高分析灵敏度。使用TD-PCR在诊断时检测ITD突变体的进一步研究可能会阐明那些等位基因负担极低的ITD突变体的临床意义。