Serre J L, Taillandier A, Mornet E, Simon-Bouy B, Boué J, Boué A
Laboratoire de Génétique Epidémiologique, INSERM U.155, Paris, France.
Genomics. 1991 Dec;11(4):1149-51. doi: 10.1016/0888-7543(91)90043-e.
A technique allowing the simultaneous screening of the four main CF mutations in the French population (delta F508, delta I507, G542X, S549N) has been developed by means of allele sequence-specific oligonucleotide (ASO) reverse dot blot. Using a strategy proposed by R. K. Saïki et al. (1989, Proc. Natl. Acad. Sci. USA 86: 6230-6234) for HLA-DQA, the seven ASOs for normal and mutant CF alleles were given a homopolymer T tail with terminal deoxyribonucleotidyltransferase and then immobilized on a nylon membrane. T-tail homopolymers were preferentially bound to the nylon, leaving the specific ASO sequences free to hybridize with amplified and radiolabeled exons 10 and 11 of a patient. These exons were simultaneously coamplified by a multiplex PCR and radiolabeled by random priming. ASO reverse dot blot currently appears to be the most efficient, rapid, and economic means of screening the population for CF mutations. This screening can detect nearly 80% of carriers and 64% of couples at risk and could prevent the birth of CF-affected infants in these families.
通过等位基因序列特异性寡核苷酸(ASO)反向斑点杂交技术,开发出了一种可同时筛查法国人群中四种主要囊性纤维化(CF)突变(ΔF508、ΔI507、G542X、S549N)的方法。利用R.K. 萨伊基等人(1989年,《美国国家科学院院刊》86: 6230 - 6234)针对HLA - DQA提出的策略,用末端脱氧核糖核苷酸转移酶给正常和突变CF等位基因的七条ASO加上一个同聚物T尾,然后固定在尼龙膜上。T尾同聚物优先与尼龙结合,使特定的ASO序列能够自由地与患者经扩增和放射性标记的第10和11外显子杂交。这些外显子通过多重PCR同时进行共扩增,并通过随机引物进行放射性标记。目前,ASO反向斑点杂交似乎是筛查人群中CF突变最有效、快速且经济的方法。这种筛查能够检测出近80%的携带者以及64%有风险的夫妇,并可防止这些家庭中患有CF的婴儿出生。
