首页> 外文期刊>Thrombosis and Haemostasis: Journal of the International Society on Thrombosis and Haemostasis >Rapid identification of female haemophilia A carriers with deletions in the factor VIII gene by quantitative real-time PCR analysis.
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Rapid identification of female haemophilia A carriers with deletions in the factor VIII gene by quantitative real-time PCR analysis.

机译:通过定量实时PCR分析快速鉴定具有因子VIII基因缺失的女性A型血友病携带者。

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摘要

Large deletions of the factorVIII gene account for approximately 5% of severe haemophilia A patients. Although deletions are readily detectable in males, the identification of heterozygosity in possible carriers of these families still constitutes a challenge. In order to identify a deleted allele over the background of the normal allele in these carriers, we developed a rapid real-time quantitative PCR approach by means of LightCycler technology and SYBR green I for monitoring product formation. The method was applied to families with independent deletions (one in exon 14 and the other in exons 23-24) of the Factor VIII gene, thereby allowing a reliable determination of carrier or non-carrier status.The method is extremely versatile and can be adapted to other deletions within the factorVIII gene as well as to other diseases whose molecular pathology consists of deletions or duplications.
机译:严重的A型血友病患者中factorVIII基因的大量缺失约占5%。尽管在男性中容易检测到缺失,但是在这些家族的可能携带者中鉴定杂合性仍然构成挑战。为了在这些携带者的正常等位基因的背景下识别缺失的等位基因,我们开发了一种快速实时定量PCR方法,该方法通过LightCycler技术和SYBR green I来监测产物的形成。该方法适用于因子VIII基因具有独立缺失(第14外显子一个,第23-24外显子另一个)的家族,因此可以可靠地确定携带者或非携带者的状态。适用于factorVIII基因内的其他缺失以及分子病理由缺失或重复组成的其他疾病。

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