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B型血友病中缺失携带者的鉴定:定量实时聚合酶链反应或多重连接探针扩增。

Identification of deletion carriers in hemophilia B: quantitative real-time polymerase chain reaction or multiple ligation probe amplification.

作者信息

Casaña Pilar, Haya Saturnino, Cid Ana R, Oltra Silvestre, Martínez Francisco, Cabrera Noelia, Aznar José A

出版信息

Transl Res. 2009 Mar;153(3):114-7. doi: 10.1016/j.trsl.2008.12.006. Epub 2009 Jan 27.

Abstract

Gross deletions in the F9 gene are easily detected by routinely sequencing hemophilia B-affected men. Nevertheless, a carrier diagnosis proves difficult as the presence of a normal allele does not recognize the partial or complete loss of the F9 gene and may be challenging if no DNA sample from affected men is available. This work aimed to identify hemophilia carriers in 2 families in which gross deletions of the F9 gene could be expected. The indirect genetic study was not conclusive, and sequencing did not show genetic defects in family 1. A real-time polymerase chain reaction (RT-PCR) assay using SYBR Green revealed the deletion of a copy of exon 8 in 3 women, whereas the multiple ligation-dependent probe amplification (MLPA) assay showed the deletion of a copy of exons 7 and 8 in these 3 women. These studies enabled us not only to rule out a pregnant woman as a carrier but also to confirm a complete deletion of the gene in the patient from family 2 and the heterozygous state of his mother. The advantages that the MLPA method offers are the identification of a multiple exon deletion in the same assay and commonly used technology. The RT-PCR technology used involves standardizing and analyzing each exon independently.

摘要

通过对患B型血友病男性进行常规测序,很容易检测到F9基因的大片段缺失。然而,由于存在正常等位基因无法识别F9基因的部分或完全缺失,携带者诊断颇具困难;如果没有来自患病人群的DNA样本,诊断可能更具挑战性。这项研究旨在确定两个可能存在F9基因大片段缺失的家族中的血友病携带者。间接基因研究尚无定论,测序未显示家族1存在基因缺陷。使用SYBR Green的实时聚合酶链反应(RT-PCR)分析显示,3名女性缺失了一个外显子8拷贝,而多重连接依赖探针扩增(MLPA)分析显示这3名女性缺失了外显子7和8的各一个拷贝。这些研究不仅使我们能够排除一名孕妇为携带者,还能确认家族2中患者的基因完全缺失以及其母亲的杂合状态。MLPA方法的优势在于能在同一次检测中识别多个外显子缺失,且是常用技术。所使用的RT-PCR技术需要对每个外显子进行独立标准化和分析。

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