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Fluorescent multiplex linkage analysis and carrier detection for Duchenne/Becker muscular dystrophy.

机译:荧光多重连锁分析和杜兴氏/贝克尔肌营养不良症的载体检测。

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摘要

We have developed a fast and accurate PCR-based linkage and carrier detection protocol for families of Duchenne muscular dystrophy (DMD)/Becker muscular dystrophy (BMD) patients with or without detectable deletions of the dystrophin gene, using fluorescent PCR products analyzed on an automated sequencer. When a deletion is found in the affected male DMD/BMD patient by standard multiplex PCR, fluorescently labeled primers specific for the deleted and nondeleted exon(s) are used to amplify the DNA of at-risk female relatives by using multiplex PCR at low cycle number (20 cycles). The products are then quantitatively analyzed on an automatic sequencer to determine whether they are heterozygous for the deletion and thus are carriers. As a confirmation of the deletion data, and in cases in which a deletion is not found in the proband, fluorescent multiplex PCR linkage is done by using four previously described polymorphic dinucleotide sequences. The four (CA)n repeats are located throughout the dystrophin gene, making the analysis highly informative and accurate. We present the successful application of this protocol in families who proved refractory to more traditional analyses.
机译:我们使用自动分析的荧光PCR产物,开发了一种快速,准确的基于PCR的连锁和载体检测方案,适用于患有或不存在肌营养不良蛋白基因可检测缺失的Duchenne肌营养不良症(DMD)/ Becker肌营养不良症(BMD)患者的家庭定序器。通过标准的多重PCR在患病的男性DMD / BMD患者中发现缺失时,通过缺失PCR的低周期多重PCR,使用针对缺失和未缺失外显子的荧光标记引物来扩增高危女性亲属的DNA。数字(20个周期)。然后在自动测序仪上对产物进行定量分析,以确定它们对于缺失是否是杂合的,因此是否是载体。作为缺失数据的确认,并且在先证者中未发现缺失的情况下,通过使用四个先前描述的多态性二核苷酸序列进行荧光多重PCR连接。四个(CA)n重复序列位于整个肌营养不良蛋白基因中,从而使分析具有很高的准确性和准确性。我们介绍了在对传统分析难以证明的家庭中该协议的成功应用。

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