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焦磷酸测序法检测胶质母细胞瘤中MGMT启动子甲基化

Detection of MGMT promoter methylation in glioblastoma using pyrosequencing.

作者信息

Xie Hao, Tubbs Raymond, Yang Bin

机构信息

Robert J. Tomsick Pathology & Laboratory Medicine Institute, Cleveland Clinic Cleveland, OH.

出版信息

Int J Clin Exp Pathol. 2015 Jan 1;8(1):636-42. eCollection 2015.

Abstract

Recent clinical trials on patients with glioblastoma revealed that O(6)-Methylguanine-DNA methyltransferase (MGMT) methylation status significantly predicts patient's response to alkylating agents. In this study, we sought to develop and validate a quantitative MGMT methylation assay using pyrosequencing on glioblastoma. We quantified promoter methylation of MGMT using pyrosequencing on paraffin-embedded fine needle aspiration biopsy tissues from 43 glioblastoma. Using a 10% cutoff, MGMT methylation was identified in 37% cases of glioblastoma and 0% of the non-neoplastic epileptic tissue. Methylation of any individual CpG island in MGMT promoter ranged between 33% and 95%, with a mean of 65%. By a serial dilution of genomic DNA of a homogenously methylated cancer cell line with an unmethylated cell line, the analytical sensitivity is at 5% for pyrosequencing to detect MGMT methylation. The minimal amount of genomic DNA required is 100 ng (approximately 3,000 cells) in small fine needle biopsy specimens. Compared with methylation-specific PCR, pyrosequencing is comparably sensitive, relatively specific, and also provides quantitative information for each CpG methylation.

摘要

近期针对胶质母细胞瘤患者的临床试验表明,O(6)-甲基鸟嘌呤-DNA甲基转移酶(MGMT)的甲基化状态可显著预测患者对烷化剂的反应。在本研究中,我们试图开发并验证一种利用焦磷酸测序技术检测胶质母细胞瘤中MGMT甲基化的定量检测方法。我们采用焦磷酸测序技术对43例胶质母细胞瘤石蜡包埋细针穿刺活检组织中的MGMT启动子甲基化进行了定量分析。以10%为临界值,在37%的胶质母细胞瘤病例中检测到MGMT甲基化,而在非肿瘤性癫痫组织中未检测到。MGMT启动子中任何一个单独的CpG岛甲基化范围在33%至95%之间,平均为65%。通过将均匀甲基化的癌细胞系基因组DNA与未甲基化细胞系进行系列稀释,焦磷酸测序检测MGMT甲基化的分析灵敏度为5%。在小型细针活检标本中,所需的基因组DNA最小量为100 ng(约3000个细胞)。与甲基化特异性PCR相比,焦磷酸测序具有相当的灵敏度、相对较高的特异性,并且还能为每个CpG甲基化提供定量信息。

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