Petrij-Bosch A, Peelen T, van Vliet M, van Eijk R, Olmer R, Drüsedau M, Hogervorst F B, Hageman S, Arts P J, Ligtenberg M J, Meijers-Heijboer H, Klijn J G, Vasen H F, Cornelisse C J, van 't Veer L J, Bakker E, van Ommen G J, Devilee P
Department of Human Genetics, Leiden University Medical Centre, The Netherlands.
Nat Genet. 1997 Nov;17(3):341-5. doi: 10.1038/ng1197-341.
To date, more than 300 distinct small deletions, insertions and point mutations, mostly leading to premature termination of translation, have been reported in the breast/ovarian-cancer susceptibility gene BRCA1. The elevated frequencies of some mutations in certain ethnic subpopulations are caused by founder effects, rather than by mutation hotspots. Here we report that the currently available mutation spectrum of BRCA1 has been biased by PCR-based mutation-screening methods, such as SSCP, the protein truncation test (PTT) and direct sequencing, using genomic DNA as template. Three large genomic deletions that are not detected by these approaches comprise 36% of all BRCA1 mutations found in Dutch breast-cancer families to date. A 510-bp Alu-mediated deletion comprising exon 22 was found in 8 of 170 breast-cancer families recruited for research purposes and in 6 of 49 probands referred to the Amsterdam Family Cancer Clinic for genetic counselling. In addition, a 3,835-bp Alu-mediated deletion encompassing exon 13 was detected in 4 of 170 research families, while an deletion of approximately 14 kb was detected in a single family [corrected]. Haplotype analyses indicated that each recurrent deletion had a single common ancestor.
迄今为止,在乳腺癌/卵巢癌易感基因BRCA1中已报道了300多种不同的小缺失、插入和点突变,其中大多数导致翻译提前终止。某些种族亚群中一些突变的频率升高是由奠基者效应引起的,而非突变热点。我们在此报告,目前可用的BRCA1突变谱因基于PCR的突变筛查方法而存在偏差,这些方法如单链构象多态性分析(SSCP)、蛋白质截短试验(PTT)以及以基因组DNA为模板的直接测序。三种未被这些方法检测到的大片段基因组缺失占迄今在荷兰乳腺癌家族中发现的所有BRCA1突变的36%。在为研究目的招募的170个乳腺癌家族中的8个以及转介至阿姆斯特丹家族癌症诊所进行遗传咨询的49名先证者中的6名中,发现了一个包含第22外显子的510 bp Alu介导的缺失。此外,在170个研究家族中的4个中检测到一个包含第13外显子的3835 bp Alu介导的缺失,而在一个家族中检测到一个约14 kb的缺失[已修正]。单倍型分析表明,每个反复出现的缺失都有一个单一的共同祖先。
