林奇综合征结直肠癌中体细胞错配修复同源蛋白1启动子高甲基化的患病率
Prevalence of somatic mutl homolog 1 promoter hypermethylation in Lynch syndrome colorectal cancer.
作者信息
Moreira Leticia, Muñoz Jenifer, Cuatrecasas Míriam, Quintanilla Isabel, Leoz Maria Liz, Carballal Sabela, Ocaña Teresa, López-Cerón María, Pellise Maria, Castellví-Bel Sergi, Jover Rodrigo, Andreu Montserrat, Carracedo Angel, Xicola Rosa Maria, Llor Xavier, Boland Clement Richard, Goel Ajay, Castells Antoni, Balaguer Francesc
机构信息
Department of Gastroenterology, Barcelona Hospital Clinic, Networked Biomedical Research Center on Hepatic and Digestive Diseases (CIBERehd), August Pi i Sunyer Biomedical Research Institute (IDIBAPS), University of Barcelona, Barcelona, Catalonia, Spain.
出版信息
Cancer. 2015 May 1;121(9):1395-404. doi: 10.1002/cncr.29190. Epub 2014 Dec 29.
BACKGROUND
Colorectal cancers (CRCs) that have microsatellite instability (MSI) and mutL homolog 1 (MLH1) immunoloss are observed in 3 clinical scenarios: Lynch syndrome (LS), sporadic MSI CRC, and Lynch-like syndrome (LLS). v-Raf murine sarcoma viral oncogene homolog B1 (BRAF) mutational analysis is used to differentiate LS from sporadic MSI CRC. The role of MLH1 promoter methylation status for the differential diagnosis of these clinical forms is not well established. The objectives of this study were: 1) to analyze MLH1 promoter methylation in MLH1-deficient CRCs by pyrosequencing, and 2) to assess its role in the differential diagnosis of MLH1-deficient CRCs.
METHODS
In total, 165 CRCs were analyzed, including LS (n = 19), MSI BRAF-mutated CRC (n = 37), MSI BRAF wild-type CRC (n = 60), and a control group of CRCs without MSI (microsatellite stable [MSS] CRC; n = 49). MLH1 promoter methylation status was analyzed by pyrosequencing, and the ability of different strategies to identify LS was assessed.
RESULTS
The average ± standard deviation methylation in LS (9% ± 7%) was significantly lower than that in MSI BRAF-mutated CRC (42% ± 17%; P < .001) and in MSI BRAF wild-type CRC (25% ± 19%; P = .002). Somatic MLH1 hypermethylation was detected in 3 patients (15.8%) with LS, in 34 patients (91.9%) with MSI BRAF-mutated CRC, and in 37 patients (61.7%) with MSI BRAF wild-type tumors. Patients with MSI BRAF wild-type, unmethylated tumors (ie, LLS) had a stronger family history of CRC than those who had tumors with MLH1 methylation (P < .05). The sensitivity for ruling out LS was 100% for BRAF analysis, 84.2% for MLH1 methylation analysis, and 84.2% for the combination of both analyses.
CONCLUSIONS
Somatic MLH1 promoter methylation occurs in up to 15% of LS CRCs. Somatic BRAF analysis is the most sensitive strategy for ruling out LS. Patients who have CRCs with loss of MLH1 protein expression and neither BRAF mutation nor MLH1 methylation resemble patients with LS.
背景
在三种临床情况下可观察到具有微卫星不稳定性(MSI)和错配修复蛋白同源物1(MLH1)免疫缺失的结直肠癌(CRC):林奇综合征(LS)、散发性MSI CRC和类林奇综合征(LLS)。v-Raf鼠肉瘤病毒癌基因同源物B1(BRAF)突变分析用于区分LS与散发性MSI CRC。MLH1启动子甲基化状态在这些临床类型鉴别诊断中的作用尚未明确。本研究的目的是:1)通过焦磷酸测序分析MLH1缺陷型CRC中MLH1启动子甲基化情况,2)评估其在MLH1缺陷型CRC鉴别诊断中的作用。
方法
共分析了165例CRC,包括LS(n = 19)、MSI BRAF突变型CRC(n = 37)、MSI BRAF野生型CRC(n = 60)以及一组无MSI的CRC对照组(微卫星稳定[MSS] CRC;n = 49)。通过焦磷酸测序分析MLH1启动子甲基化状态,并评估不同策略鉴别LS的能力。
结果
LS组的平均±标准差甲基化水平(9%±7%)显著低于MSI BRAF突变型CRC(42%±17%;P <.001)和MSI BRAF野生型CRC(25%±19%;P =.002)。在3例(15.8%)LS患者、34例(91.9%)MSI BRAF突变型CRC患者和37例(61.7%)MSI BRAF野生型肿瘤患者中检测到体细胞MLH1高甲基化。MSI BRAF野生型、未甲基化肿瘤(即LLS)患者的CRC家族史比MLH1甲基化肿瘤患者更强(P <.05)。BRAF分析排除LS的敏感性为100%,MLH1甲基化分析为84.2%,两者联合分析为84.2%。
结论
高达15%的LS CRC中存在体细胞MLH1启动子甲基化。体细胞BRAF分析是排除LS最敏感的策略。MLH1蛋白表达缺失、无BRAF突变且无MLH1甲基化的CRC患者与LS患者相似。
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