长距离聚合酶链反应检测甲型血友病患者F8C基因的倒位突变

Poláková H, Zmetáková I, Kádasi L'

Institute of Molecular Physiology and Genetics, Slovak Academy of Sciences, Bratislava, Slovakia.

Gen Physiol Biophys. 2003 Jun;22(2):243-53.

In the present paper, the experience with detection of intron 22 inversion of F8C gene in severe hemophilia A patients using a recently described long-distance PCR (LD-PCR) method was reported. To test the sensitivity and the specifity of the LD-PCR, analysis of 46 DNA samples of patients and their family members, previously tested by Southern hybridization, was performed. In addition, 16 DNA samples of severe hemophilia A patients in which causative mutation was unknown, were included in analysis. Four-primers, P, Q, A&B, which are able to differentiate between the affected males with or without the inversion, and in female carriers, were used in LD-PCR. Two primers, P&Q, are located within the F8C gene flanking int22h1. Two further primers, A&B, flank int22h2 and int22h3, extragene homologs of int22h1. Nine combinations of four primers were used to identify the optimal one. Four-primers (P, Q, A&B), three-primers (P,Q & B;P, A & B; A, B & Q;P, Q & A) and two-primers (A & B; P & Q; A & Q; P & B) PCR amplifications were performed in the hemophilia A patients as well as in obligate carriers DNA samples. Successful amplification required introduction of some modifications of the original protocol. The most reproducible and uniform results were obtained using two-primers PCR, performed in four single reactions. Thus, a total of 46 DNA samples, 22 were hemizygous for inversion, 6 without the inversion, 14 carriers and 4 non-carriers of inversion. Perfect correlation between genotypes determined using Southern hybridization and LD-PCR was achieved. The optimalized two-primers LD-PCR protocol was used for analysis of 16 DNA samples of severe hemophilia A patients with unknown mutation. Ten cases of inversions and six cases without them were detected. Thus in additional 10 severe hemophilic patients DNA diagnosis was completed. The most successful and reproducible results were obtained performing four single LD-PCR reactions with combinations of two-primers A & B; P & Q; A&Q, and P&B in each DNA sample and this approach is recommended for routine using in clinical practice.

本文报道了使用最近描述的长距离聚合酶链反应（LD-PCR）方法检测重度甲型血友病患者F8C基因内含子22倒位的经验。为了测试LD-PCR的敏感性和特异性，对46例患者及其家庭成员的DNA样本进行了分析，这些样本之前已通过Southern杂交进行检测。此外，还纳入了16例致病突变未知的重度甲型血友病患者的DNA样本进行分析。在LD-PCR中使用了四种引物，即P、Q、A和B，它们能够区分有或无倒位的患病男性以及女性携带者。两种引物P和Q位于F8C基因中int22h1侧翼。另外两种引物A和B位于int22h2和int22h3侧翼，int22h2和int22h3是int22h1的基因外同源物。使用四种引物的九种组合来确定最佳组合。在甲型血友病患者以及确定携带者的DNA样本中进行了四种引物（P、Q、A和B）、三种引物（P、Q和B；P、A和B；A、B和Q；P、Q和A）和两种引物（A和B；P和Q；A和Q；P和B）的PCR扩增。成功的扩增需要对原始方案进行一些修改。使用在四个单独反应中进行的两种引物PCR获得了最可重复和一致的结果。因此，总共46个DNA样本中，22个为倒位半合子，6个无倒位，14个为携带者，4个为非倒位携带者。使用Southern杂交和LD-PCR确定的基因型之间实现了完美的相关性。优化后的两种引物LD-PCR方案用于分析16例致病突变未知的重度甲型血友病患者的DNA样本。检测到10例倒位和6例无倒位的病例。因此，又完成了10例重度血友病患者的DNA诊断。在每个DNA样本中使用两种引物A和B、P和Q、A和Q以及P和B的组合进行四个单独的LD-PCR反应，获得了最成功和可重复的结果，这种方法推荐用于临床实践中的常规使用。