Cawkwell L, Lewis F A, Quirke P
Centre for Cancer Studies, Research School of Medicine, University of Leeds, UK.
Br J Cancer. 1994 Nov;70(5):813-8. doi: 10.1038/bjc.1994.404.
We report here the use of multiplex fluorescent polymerase chain reaction (PCR) for quantitative allele loss detection using microsatellites with 2-5 base pair repeat motifs. Allele loss of APC, DCC, p53 and RB1 in colorectal tumours has been reported previously using a variety of methods. However, not all workers used intragenic markers. We have used microsatellite polymorphisms which map within, or are closely linked to, these tumour-suppressor gene loci in order to determine whether these loci are indeed the targets for alteration in colorectal cancer. In addition, we have assayed two other tumour-suppressor genes, WT1 and NF1, to see whether they play a role in colorectal carcinogenesis. The putative metastasis-suppressor gene, NM23, was also investigated since there have been conflicting reports about its involvement in colorectal carcinogenesis. Allele loss was detected at the DCC (29%), p53 (66%), RB1 (50%) and NF1 (14%) loci and in the APC/MCC region (50%), but not at the WT1 or NM23 loci. These rapid, and mostly gene-specific, fluorescent multiplex PCR assays for allele loss detection could be modified to devise a single molecular diagnostic test for the important lesions in colorectal cancer.
我们在此报告使用多重荧光聚合酶链反应(PCR),通过具有2 - 5个碱基对重复基序的微卫星进行定量等位基因缺失检测。先前已使用多种方法报道了结直肠癌中APC、DCC、p53和RB1的等位基因缺失情况。然而,并非所有研究人员都使用基因内标记。我们使用了位于这些肿瘤抑制基因位点内或与之紧密连锁的微卫星多态性,以确定这些位点是否确实是结直肠癌中改变的靶点。此外,我们检测了另外两个肿瘤抑制基因WT1和NF1,以观察它们在结直肠癌发生过程中是否发挥作用。由于关于其在结直肠癌发生中的作用存在相互矛盾的报道,还对假定的转移抑制基因NM23进行了研究。在DCC(29%)、p53(66%)、RB1(50%)和NF1(14%)位点以及APC/MCC区域(50%)检测到等位基因缺失,但在WT1或NM23位点未检测到。这些用于等位基因缺失检测的快速且大多具有基因特异性的荧光多重PCR检测方法可进行修改,以设计出一种针对结直肠癌重要病变的单一分子诊断测试。
