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Fast detection of MYCN copy number alterations in brain neuronal tumors by real‐time PCR

机译:实时荧光定量PCR快速检测脑神经元肿瘤中MYCN拷贝数变化

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摘要

Increased gene copy number is a characteristic property of neurogenic tumors. Fluorescence in situ hybridization (FISH) and array‐based comparative genomic hybridization (array‐CGH) are traditionally used to determine amplification for tumor stratification. A unique ability of real‐time quantitative polymerase chain reaction (qPCR) to determine gene copy number, even within a small percent of observed tumor cells, and can be more appropriate. genomic copy number from 44 human brain tumors (22 medulloblastomas and 22 neurocytomas) was determined by means of FISH, array‐CGH, and qPCR. By qPCR, with the original set of oligonucleotides, 17 out of 44 (38.6%) tumors were found to contain a 1.3‐ to 2.9‐fold increase of defined as low‐level gain. An absolute qPCR method was used to get high accuracy of results. Strong correlation was observed between the three methods: for medulloblastomas, r=1 ( <0.01) between FISH and array‐CGH and r=0.92 ( <0.01) between qPCR and FISH/array‐CGH. For neurocytomas, r=0.9 ( <0.01) between FISH and array‐CGH and r=0.34/0.43 ( <0.01) between qPCR and FISH/array‐CGH. Absolute qPCR assays possess high precision compared to other conventional methods and can be used for accurate and quickness detection of status (low‐level gene gain and amplification). J. Clin. Lab. Anal. 22:123–130, 2008. © 2008 Wiley‐Liss, Inc.
机译:基因拷贝数增加是神经源性肿瘤的特征。传统上使用荧光原位杂交(FISH)和基于阵列的比较基因组杂交(array-CGH)来确定肿瘤分层的扩增。实时定量聚合酶链反应(qPCR)能够确定基因拷贝数的独特能力,即使在观察到的肿瘤细胞的一小部分之内,也可能更合适。通过FISH,array-CGH和qPCR测定了44种人脑肿瘤(22个成神经细胞瘤和22个神经细胞瘤)的基因组拷贝数。通过qPCR,使用原始的寡核苷酸组,发现44个肿瘤中有17个(38.6%)的肿瘤增加了1.3到2.9倍,定义为低水平获得。绝对定量PCR方法用于获得高精度结果。三种方法之间存在强相关性:对于髓母细胞瘤,FISH和array-CGH之间的r = 1(<0.01),而qPCR和FISH / array-CGH之间的r = 0.92(<0.01)。对于神经细胞瘤,FISH和array-CGH之间的r = 0.9(<0.01),而qPCR和FISH / array-CGH之间的r = 0.34 / 0.43(<0.01)。与其他常规方法相比,绝对定量PCR分析具有很高的精确度,可用于状态的准确和快速检测(低水平基因扩增和扩增)。 J.临床实验室肛门22:123–130,2008.©2008 Wiley-Liss,Inc.

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