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利用聚合酶链反应诊断乙型血友病

Diagnosis of haemophilia B using the polymerase chain reaction.

作者信息

Reiss J, Neufeldt U, Wieland K, Zoll B

机构信息

Institut für Humangenetik, Göttingen, Federal Republic of Germany.

出版信息

Blut. 1990 Jan;60(1):31-6. doi: 10.1007/BF01720200.

Abstract

The polymerase chain reaction (PCR) was used to amplify specific DNA sequences within the factor IX gene of haemophilia B patients and their relatives. Three of the amplified fragments contain polymorphic sites, which can be used as markers in segregation analyses. These restriction fragment length polymorphisms (RFLPs) were until recently detected by Southern blotting after digestion with the restriction enzymes Taq I, Dde I and Xmn I. All three RFLP's are located in introns of the factor IX gene and together are informative in approximately 70% of all cases. Each of the polymorphisms was successfully used in carrier detection studies after amplification of the relevant fragments. This method is also suitable for rapid antenatal diagnosis. Additionally we were able to amplify all eight exons of the factor IX gene including the splice junctions and a part of the 5'-region. Large deletions or insertions can be detected without further analysis. Several possibilities for the rapid detection of point mutations after DNA amplification have been described recently. The complete amplification of all functional parts of the Factor IX gene in combination with these new techniques should enable us to detect the majority of mutations leading to haemophilia B.

摘要

采用聚合酶链反应(PCR)扩增B型血友病患者及其亲属凝血因子IX基因内的特定DNA序列。扩增出的三个片段含有多态性位点,可作为连锁分析的标记。这些限制性片段长度多态性(RFLP)直到最近才在使用限制性内切酶Taq I、Dde I和Xmn I消化后通过Southern印迹法检测到。所有这三种RFLP均位于凝血因子IX基因的内含子中,合起来在大约70%的病例中具有信息性。在扩增相关片段后,每种多态性均成功用于携带者检测研究。该方法也适用于快速产前诊断。此外,我们能够扩增凝血因子IX基因的所有八个外显子,包括剪接位点和部分5'区域。无需进一步分析即可检测到大的缺失或插入。最近已经描述了几种DNA扩增后快速检测点突变的方法。凝血因子IX基因所有功能部分的完全扩增与这些新技术相结合,应该能够使我们检测到导致B型血友病的大多数突变。

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