A general method for the detection of large CAG repeat expansions by fluorescent PCR

被引:214
作者
Warner, JP
Barron, LH
Goudie, D
Kelly, K
Dow, D
Fitzpatrick, DR
Brock, DJH
机构
[1] UNIV ABERDEEN, SCH MED, MED GENET LAB, ABERDEEN AB9 2ZD, SCOTLAND
[2] ADDENBROOKES HOSP, E ANGLIAN REG GENET SERV, CAMBRIDGE CB2 2QQ, ENGLAND
[3] UNIV DUNDEE, NINEWELLS HOSP & MED SCH, DEPT PATHOL, DUNDEE DD1 9SY, SCOTLAND
关键词
fluorescent PCR; CAG repeat; myotonic dystrophy; TP PCR;
D O I
10.1136/jmg.33.12.1022
中图分类号
Q3 [遗传学];
学科分类号
071007 ; 090102 ;
摘要
The expansion of a tandemly repeated trinucleotide sequence, CAG, is the mutational mechanism for several human genetic diseases. We present a generally applicable PCR amplification method using a fluorescently labelled locus specific primer flanking the CAG repeat together with paired primers amplifying from multiple priming sites within the CAG repeat. Triplet repeat primed PCR (TP PCR) gives a characteristic ladder on the fluorescence trace enabling the rapid identification of large pathogenetic CAG repeats that cannot be amplified using flanking primers. We used our method to test a cohort of 183 people from myotonic dystrophy families inducting unaffected subjects and spouses. Eighty five clinically affected subjects with expanded alleles on Southern blot analysis were all correctly identified by TP PCR. This method is applicable for any human diseases involving CAG repeat expansions.
引用
收藏
页码:1022 / 1026
页数:5
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