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Allelic discrimination of genetic human prion diseases by real-time PCR genotyping

机译:实时PCR基因分型对遗传性人类病毒疾病的等位基因鉴别

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摘要

The complete molecular characterization of human genetic prion diseases from different backgrounds is important for clinical diagnosis and epidemiological classification. The characterization of the PRNP gene should always include the description of the pathogenic mutation, as well as the status at each allele of the polymorphic codon 129 (M129V), a well-established susceptibility marker and phenotypic variability factor for different types of human prion diseases. Indeed, the phenotypical expression of two of the most common mutations in the human PRNP gene associated with genetic prion diseases, D178N and E200K, is clearly modulated by the codon 129 polymorphism. Here, we describe two simple, fast, cost-effective and suited for high-throughput protocols to resolve cis-trans ambiguities between these mutations respect the M129V polymorphism. This methodology is based on differential amplification by allele-specific primers using Real-time PCR monitored by SYBR® Green dye. The main advantages of these protocols are their relative simplicity and the reduced cost compared to other methods such as cloning protocols, and that it may be readily applicable to the characterization of other mutations with codon 129-dependent expression, e.g., P102L.
机译:来自不同背景的人类遗传性pr病毒疾病的完整分子表征对于临床诊断和流行病学分类非常重要。 PRNP基因的特征应始终包括病原性突变的描述以及多态性密码子129(M129V)的每个等位基因的状态,针对各种类型的人类病毒疾病的公认的易感性标记物和表型变异因子。确实,与遗传ion病毒疾病有关的人类PRNP基因中两个最常见的突变D178N和E200K的表型表达明显受到129位密码子多态性的调节。在这里,我们描述了两种简单,快速,具有成本效益的方法,适用于解决这些突变之间尊重M129V多态性的顺反歧义的高通量方案。该方法基于等位基因特异性引物的差异扩增,该引物使用了SYBR ® Green染料监控的实时PCR。这些方案的主要优点是,与其他方法(如克隆方案)相比,它们相对简单,并且成本降低,并且可以很容易地应用于表征具有密码子129依赖性表达的其他突变,例如P102L。

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