Brune Kieran, Hong Seung-Mo, Li Ang, Yachida Shinichi, Abe Tadayoshi, Griffith Margaret, Yang Dawei, Omura Noriyuki, Eshleman James, Canto Marcia, Schulick Rich, Klein Alison P, Hruban Ralph H, Iacobuzio-Donohue Christine, Goggins Michael
Department of Pathology, Medicine, Oncology, Johns Hopkins Medical Institutions, The Sol Goldman Pancreatic Cancer Research Center, 1550 Orleans Street, CRB2, Room 342, Baltimore, MD 21231, USA.
Cancer Epidemiol Biomarkers Prev. 2008 Dec;17(12):3536-42. doi: 10.1158/1055-9965.EPI-08-0630.
Little is known about the genetic and epigenetic changes that contribute to familial pancreatic cancers. The aim of this study was to compare the prevalence of common genetic and epigenetic alterations in sporadic and familial pancreatic ductal adenocarcinomas.
DNA was isolated from the microdissected cancers of 39 patients with familial and 36 patients with sporadic pancreatic adenocarcinoma. KRAS2 mutations were detected by BstN1 digestion and/or cycle sequencing. TP53 and SMAD4 status were determined by immunohistochemistry on tissue microarrays of 23 archival familial pancreatic adenocarcinomas and in selected cases by cycle sequencing to identify TP53 gene mutations. Methylation-specific PCR analysis of seven genes (FoxE1, NPTX2, CLDN5, P16, TFPI-2, SPARC, ppENK) was done on a subset of fresh-frozen familial pancreatic adenocarcinomas.
KRAS2 mutations were identified in 31 of 39 (80%) of the familial versus 28 of 36 (78%) of the sporadic pancreatic cancers. Positive immunolabeling for p53 was observed in 57% of the familial pancreatic cancers and loss of SMAD4 labeling was observed in 61% of the familial pancreatic cancers, rates similar to those observed in sporadic pancreatic cancers. The mean prevalence of aberrant methylation in the familial pancreatic cancers was 68.4%, which was not significantly different from that observed in sporadic pancreatic cancers.
The prevalence of mutant KRAS2, inactivation of TP53 and SMAD4, and aberrant DNA methylation of a seven-gene panel is similar in familial pancreatic adenocarcinomas as in sporadic pancreatic adenocarcinomas. These findings support the use of markers of sporadic pancreatic adenocarcinomas to detect familial pancreatic adenocarcinomas.
对于导致家族性胰腺癌的基因和表观遗传变化了解甚少。本研究的目的是比较散发性和家族性胰腺导管腺癌中常见基因和表观遗传改变的发生率。
从39例家族性胰腺癌患者和36例散发性胰腺癌患者的显微切割癌组织中提取DNA。通过BstN1酶切和/或循环测序检测KRAS2基因突变。通过免疫组织化学方法在23例存档的家族性胰腺癌组织芯片上检测TP53和SMAD4状态,并在部分病例中通过循环测序鉴定TP53基因突变。对一部分新鲜冷冻的家族性胰腺癌组织进行七个基因(FoxE1、NPTX2、CLDN5、P16、TFPI-2、SPARC、ppENK)的甲基化特异性PCR分析。
39例家族性胰腺癌中有31例(80%)检测到KRAS2基因突变,36例散发性胰腺癌中有28例(78%)检测到该突变。57%的家族性胰腺癌中观察到p53免疫阳性标记,61%的家族性胰腺癌中观察到SMAD4标记缺失,这些发生率与散发性胰腺癌中观察到的相似。家族性胰腺癌中异常甲基化的平均发生率为68.4%,与散发性胰腺癌中观察到的无显著差异。
家族性胰腺腺癌中KRAS2基因突变、TP53和SMAD4失活以及七基因panel的异常DNA甲基化发生率与散发性胰腺腺癌相似。这些发现支持使用散发性胰腺腺癌的标志物来检测家族性胰腺腺癌。