Ogino S, Cantor M, Kawasaki T, Brahmandam M, Kirkner G J, Weisenberger D J, Campan M, Laird P W, Loda M, Fuchs C S
Department of Pathology, Brigham and Women's Hospital, Harvard Medical School, 75 Francis St, Boston, MA 02115, USA.
Gut. 2006 Jul;55(7):1000-6. doi: 10.1136/gut.2005.082933. Epub 2006 Jan 11.
The concept of CpG island methylator phenotype (CIMP) is not universally accepted. Even if specific clinicopathological features have been associated with CIMP, investigators often failed to demonstrate a bimodal distribution of the number of methylated markers, which would suggest CIMP as a distinct subtype of colorectal cancer. Previous studies primarily used methylation specific polymerase chain reaction which might detect biologically insignificant low levels of methylation.
To demonstrate a distinct genetic profile of CIMP colorectal cancer using quantitative DNA methylation analysis that can distinguish high from low levels of DNA methylation.
We developed quantitative real time polymerase chain reaction (MethyLight) assays and measured DNA methylation (percentage of methylated reference) of five carefully selected loci (promoters of CACNA1G, CDKN2A (p16), CRABP1, MLH1, and NEUROG1) in 460 colorectal cancers from large prospective cohorts.
There was a clear bimodal distribution of 80 microsatellite instability-high (MSI-H) tumours according to the number of methylated promoters, with no tumours showing 3/5 methylated loci. Thus we defined CIMP as having >or=4/5 methylated loci, and 17% (78) of the 460 tumours were classified as CIMP. CIMP was significantly associated with female sex, MSI, BRAF mutations, and wild-type KRAS. Both CIMP MSI-H tumours and CIMP microsatellite stable (MSS) tumours showed much higher frequencies of BRAF mutations (63% and 54%) than non-CIMP counterparts (non-CIMP MSI-H (0%, p<10(-5)) and non-CIMP MSS tumours (6.6%, p<10(-4)), respectively).
CIMP is best characterised by quantitative DNA methylation analysis. CIMP is a distinct epigenotype of colorectal cancer and may be less frequent than previously reported.
CpG岛甲基化表型(CIMP)的概念尚未得到普遍认可。即使特定的临床病理特征与CIMP相关,但研究人员往往未能证明甲基化标记数量的双峰分布,而这将提示CIMP是结直肠癌的一种独特亚型。以往研究主要使用甲基化特异性聚合酶链反应,该方法可能会检测到生物学上无意义的低水平甲基化。
使用能够区分DNA甲基化高水平和低水平的定量DNA甲基化分析,来证明CIMP结直肠癌具有独特的基因特征。
我们开发了定量实时聚合酶链反应(MethyLight)检测方法,并测量了来自大型前瞻性队列的460例结直肠癌中五个精心挑选位点(CACNA1G、CDKN2A(p16)、CRABP1、MLH1和NEUROG1的启动子)的DNA甲基化(甲基化参考百分比)。
根据甲基化启动子的数量,80例微卫星高度不稳定(MSI-H)肿瘤存在明显的双峰分布,没有肿瘤显示3/5个甲基化位点。因此,我们将CIMP定义为具有≥4/5个甲基化位点,460例肿瘤中有17%(78例)被归类为CIMP。CIMP与女性、MSI、BRAF突变和野生型KRAS显著相关。CIMP MSI-H肿瘤和CIMP微卫星稳定(MSS)肿瘤的BRAF突变频率(分别为63%和54%)均远高于非CIMP对应肿瘤(非CIMP MSI-H为0%,p<10⁻⁵;非CIMP MSS肿瘤为6.6%,p<10⁻⁴)。
CIMP的最佳特征是通过定量DNA甲基化分析来体现。CIMP是结直肠癌的一种独特表观基因型,其发生率可能比先前报道的要低。
