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使用甲基化敏感限制性指纹技术鉴定人乳腺癌的DNA甲基化标记物。

Identification of DNA methylation markers for human breast carcinomas using the methylation-sensitive restriction fingerprinting technique.

作者信息

Huang T H, Laux D E, Hamlin B C, Tran P, Tran H, Lubahn D B

机构信息

Department of Pathology and Anatomical Sciences, Ellis Fischel Cancer Center, University of Missouri, Columbia 65203, USA.

出版信息

Cancer Res. 1997 Mar 15;57(6):1030-4.

PMID:9067264
Abstract

We have developed a PCR-based method, called methylation-sensitive restriction fingerprinting (MSRF), to screen changes in DNA methylation in breast carcinomas. Two hypermethylation-containing fragments, HBC-1 (for "hypermethylation in breast cancer") and HBC-2, were identified in the amplified breast tumor DNA relative to the amplified normal breast DNA of a patient. Nucleotide sequence analysis revealed no significant matches between the sequence of HBC-1 and the known sequences in the GenBank database, whereas the sequence of HBC-2 matched the upstream region of an antisense WT1 (Wilms' tumor suppressor gene) promoter. The methylation status in the breast tumor DNA from this patient was confirmed by Southern hybridization using HBC-1 and HBC-2 as probes, respectively. Further analysis showed that HBC-1 was methylated aberrantly in 90% (17 of 19 patients) of the primary breast carcinomas examined. This study demonstrates that MSRF provides a useful means for screening aberrant changes in DNA methylation during tumorigenesis. The commonly methylated fragments identified by MSRF could potentially supplement pathological markers currently used for cancers and additionally lead to the discovery of novel methylated tumor suppressor genes.

摘要

我们开发了一种基于聚合酶链反应(PCR)的方法,称为甲基化敏感限制性指纹图谱法(MSRF),用于筛查乳腺癌中DNA甲基化的变化。相对于一名患者的扩增正常乳腺DNA,在扩增的乳腺肿瘤DNA中鉴定出两个含有高甲基化的片段,即HBC-1(代表“乳腺癌中的高甲基化”)和HBC-2。核苷酸序列分析显示,HBC-1的序列与GenBank数据库中的已知序列无明显匹配,而HBC-2的序列与反义WT1(威尔姆斯肿瘤抑制基因)启动子的上游区域匹配。分别使用HBC-1和HBC-2作为探针,通过Southern杂交证实了该患者乳腺肿瘤DNA中的甲基化状态。进一步分析表明,在所检测的原发性乳腺癌中,90%(19例患者中的17例)的HBC-1存在异常甲基化。这项研究表明,MSRF为筛查肿瘤发生过程中DNA甲基化的异常变化提供了一种有用的方法。通过MSRF鉴定出的常见甲基化片段可能会补充目前用于癌症的病理标志物,并额外导致发现新的甲基化肿瘤抑制基因。

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