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Immunoglobulin kappa deleting element rearrangements in precursor-B acute lymphoblastic leukemia are stable targets for detection of minimal residual disease by real-time quantitative PCR

机译：预防 - B急性淋巴细胞白血病中的免疫球蛋白Kappa缺失元素重排是通过实时定量PCR检测最小残留疾病的稳定靶标

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Immunoglobulin gene rearrangements are used as PCR targets for detection of minimal residual disease (MRD) in acute lymphoblastic leukemia (ALL). We Investigated the occurrence of monoclonal immunoglobulin kappa-deleting element (IGK-Kde) rearrangements by Southern blotting and PCR/heteroduplex analysis at diagnosis, their stability at relapse, and their applicability in real-time quantitative PCR (RQ-PCR) analysis. In 77 selected children with precursor-B-ALL, Southern blotting detected 122 IGK-Kde rearrangements, 12 of which were derived from subclones in six patients (8%). PCR/heteroduplex analysis with BIOMED-1 Concerted Action primers identified 100 of the 110 major IGK-Kde rearrangements (91%). Comparison between diagnosis and relapse samples from 21 patients with PCR-detectable IGK-Kde rearrangements (using Southern blotting, PCR/heteroduplex analysis, and sequencing) demonstrated that 27 of the 32 rearrangements remained stable at relapse. When patients with oligoclonal IGK-Kde rearrangements were excluded, 25 of the 27 rearrangements remained stable at relapse and at least one stable rearrangement was present In 17 of the 18 patients. Subsequently, RQ-PCR analysis with allele-specific forward primers, a germline Kde Taq-Man-probe, and a germline Kde reverse primer was evaluated for 18 IGK-Kde rearrangements. In 16 of the 18 targets (89%) a sensitivity of less than or equal to10(-4) was reached. Analysis of MRD during follow-up of eight patients with IGK-Kde rearrangements showed comparable results between RQ-PCR data and classical dot-blot data. We conclude that the frequently occurring IGK-Kde rearrangements are generally detectable by PCR (similar to90%) and are highly stable MRD-PCR targets, particularly where monoclonal rearrangements at diagnosis similar to(95%) are concerned. Furthermore, most IGK-Kde rearrangements (similar to90%) can be used for sensitive detection of MRD (less than or equal to10(-4)) by RQ-PCR analysis

机译：免疫球蛋白基因重排用作PCR靶标检测急性淋巴细胞白血病（全部）中的最小残留疾病（MRD）。我们调查了在诊断，其复发稳定性的Southern印迹和PCR / Heteroputople分析的单克隆免疫球蛋白Kappa-Deleting元素（Igk-KDE）重排的发生，以及它们在实时定量PCR（RQ-PCR）分析中的适用性。在77名选定的儿童中，具有前体 - B-全部，检测到122个Igk-KDE重排，其中12例遍布六名患者中的亚克隆（8％）。 PCR / Heteroduplex分析与生物密合 - 1齐齐齐子作用引物鉴定为110个主要IGK-KDE重排（91％）。从21例PCR可检测IGK-KDE重排患者（使用Southern印迹，PCR / Heteroputople分析和测序）之间的诊断和复发样本的比较证明了32个重排部中的27个在复发时保持稳定。除了少胶质Igk-KDE重排患者的情况下，25例重排仍然保持稳定，在18例患者中有17例中存在至少一个稳定的重排。随后，用等位基因特异性前引物，种系KDE Taq-man-探针和种系KDE反向引物进行RQ-PCR分析，对18只IgK-KDE重排进行评价。在18个靶标中的16个（89％）中，达到了小于或等于10（-4）的敏感性。 IGK-KDE重排患者随访期间MRD分析显示RQ-PCR数据和经典点刻度数据之间的相当结果。我们得出结论，经常发生的IgK-KDE重排通过PCR（类似于90％）可检测到的，并且是高度稳定的MRD-PCR靶标，特别是在诊断中涉及（95％）的单克隆重排。此外，大多数IGK-KDE重排（类似于90％）可用于通过RQ-PCR分析用于MRD的敏感检测（小于或等于10（-4））

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VHJ van der Velden; MJ Willemse; CE van der Schoot; K Hählen; ER van Wering; JJM van Dongen;
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年度 2002
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1. Minimal residual disease-directed risk stratification using real-time quantitative PCR analysis of immunoglobulin and T-cell receptor gene rearrangements in the international multicenter trial AIEOP-BFM ALL 2000 for childhood acute lymphoblastic leukemia [J] . T Flohr, A Schrauder, G Cazzaniga, Leukemia . 2008,第4期

机译：在国际多中心试验AIEOP-BFM ALL 2000中对儿童急性淋巴细胞白血病的免疫球蛋白和T细胞受体基因重排进行实时定量PCR分析，从而最小化了以疾病为导向的最小风险分层
2. Immunoglobulin and T-cell receptor gene rearrangements as PCR-based targets are stable markers for monitoring minimal residual disease in acute lymphoblastic leukemia after stem cell transplantation [J] . H Kreyenberg, C Eckert, Y Yarkin, Leukemia . 2009,第7期

机译：免疫球蛋白和T细胞受体基因重排作为基于PCR的靶标是监测干细胞移植后急性淋巴细胞白血病最小残留病的稳定标志物
3. Kappa deleting element as an alternative molecular target for minimal residual disease assessment by real-time quantitative PCR in patients with multiple myeloma [J] . PuigN., SarasqueteM.E., AlcocebaM., European Journal of Haematology . 2012,第4期

机译：κ缺失元素作为实时定量定量PCR对多发性骨髓瘤患者最小残留疾病评估的替代分子靶标
4. Discrimination of minimal residual disease in acute lymphoblastic leukemia by using single-beam acoustic tweezer [C] . Hsiao-Cliuan Liu, Hye Na Kim, Enzi Jiang, IEEE International Ultrasonics Symposium . 2017

机译：用单束声镊鉴别急性淋巴细胞白血病的最小残留病
5. Targeted Capture and Sequencing of Immunoglobulin Rearrangements in Multiple Myeloma to Enable Detection of Minimal Residual Disease [D] . Chow, Signy. 2017

机译：在多发性骨髓瘤中针对性捕获和免疫球蛋白重排测序，以检测出最小的残留疾病
6. Time point-dependent concordance of flow cytometry and real-time quantitative polymerase chain reaction for minimal residual disease detection in childhood acute lymphoblastic leukemia [O] . Giuseppe Gaipa, Giovanni Cazzaniga, Maria Grazia Valsecchi, 2012

机译：流式细胞仪和实时定量聚合酶链反应的时间点依赖性可用于儿童急性淋巴细胞白血病最小残留疾病的检测
7. T cell receptor gamma gene rearrangements as targets for detection of minimal residual disease in acute lymphoblastic leukemia by real-time quantitative PCR analysis [O] . VHJ van der Velden, JM Wijkhuijs, DCH Jacobs, 2002

机译：T细胞受体γ基因重排作为检测急性淋巴细胞白血病最小残留疾病的靶标通过实时定量PCR分析

Immunoglobulin kappa deleting element rearrangements in precursor-B acute lymphoblastic leukemia are stable targets for detection of minimal residual disease by real-time quantitative PCR

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