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使用错配修复检测(MRD)快速鉴定结直肠癌和乳腺癌组织中的体细胞突变。

Rapid identification of somatic mutations in colorectal and breast cancer tissues using mismatch repair detection (MRD).

作者信息

Bentivegna Steven, Zheng Jianbiao, Namsaraev Eugeni, Carlton Victoria E H, Pavlicek Adam, Moorhead Martin, Siddiqui Farooq, Wang Zhiyong, Lee Liana, Ireland James S, Suyenaga Kent, Willis Thomas D, Faham Malek, Seymour Albert B

机构信息

Molecular Profiling-Pharmacogenomics, Pfizer Global Research and Development, Groton Laboratories, Groton, Connecticut, USA.

出版信息

Hum Mutat. 2008 Mar;29(3):441-50. doi: 10.1002/humu.20672.

Abstract

Mismatch repair detection (MRD) was used to screen 93 matched tumor-normal sample pairs and 22 cell lines for somatic mutations in 30 cancer relevant genes. Using a starting amount of only 150 ng of genomic DNA, we screened 102 kb of sequence for somatic mutations in colon and breast cancer. A total of 152 somatic mutations were discovered, encompassing previously reported mutations, such as BRAF V600E and KRAS G12S, G12V, and G13D, as well as novel mutations, including some in genes in which somatic mutations have not previously been reported, such as MAP2K1 and MAP2K2. The distribution of mutations ranged widely within and across tumor types. The functional significance of many of these mutations is not understood, with patterns of selection only evident in KRAS and BRAF in colon cancer. These results present a novel approach to high-throughput mutation screening using small amounts of starting material and reveal a mutation spectrum across 30 genes in a large cohort of breast and colorectal cancers.

摘要

错配修复检测(MRD)用于筛查93对匹配的肿瘤-正常样本对以及22种细胞系,以检测30个癌症相关基因中的体细胞突变。仅使用150 ng基因组DNA的起始量,我们就对结肠癌和乳腺癌中的102 kb序列进行了体细胞突变筛查。共发现152个体细胞突变,包括先前报道的突变,如BRAF V600E和KRAS G12S、G12V以及G13D,还有新的突变,包括一些此前未报道过体细胞突变的基因中的突变,如MAP2K1和MAP2K2。突变分布在肿瘤类型内部和之间差异很大。许多这些突变的功能意义尚不清楚,仅在结肠癌的KRAS和BRAF中存在明显的选择模式。这些结果提出了一种使用少量起始材料进行高通量突变筛查的新方法,并揭示了一大组乳腺癌和结直肠癌中30个基因的突变谱。

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