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鉴定 Xq28 上的第三种重排,导致严重血友病 A,原因是反转重复之间的同源重组。

Identification of a third rearrangement at Xq28 that causes severe hemophilia A as a result of homologous recombination between inverted repeats.

机构信息

Institute of Experimental Hematology and Transfusion Medicine, University of Bonn, Bonn, Germany.

出版信息

J Thromb Haemost. 2012 Aug;10(8):1600-8. doi: 10.1111/j.1538-7836.2012.04809.x.

Abstract

BACKGROUND

Intrachromosomal homologous recombination between inverted repeats on the X chromosome account for about half of severe hemophilia A cases. Repeats in F8 intron 1 and intron 22 can recombine with homologous inverted repeats located about 200 kb upstream and 500 kb downstream of F8, respectively, resulting in partial sequence inversion of the F8 open reading frame and, subsequently, no functional protein production.

OBJECTIVES

In the present study, we characterize a third novel homologous recombination at Xq28 consistent with absence of F8 transcription that we previously reported for the affected chromosome of the index patient as well as his mother and sister.

RESULTS

The rearrangement occurs between a repeat in F8 intron 1 (Int1R-1) and an inverted identical repeat (Int1R-2d) in intron 2 of a duplicated copy of IKBKG located about 386 kb upstream of F8. The rearrangement was confirmed by Southern blot and inverse PCR and results in failure of PCR amplification across Int1R-1.

CONCLUSION

We developed a PCR-based diagnostic method that can be used to screen for this genetic rearrangement in cases of severe hemophilia A for which mutations cannot be identified.

摘要

背景

X 染色体上倒位重复序列之间的染色体内同源重组约占严重甲型血友病病例的一半。F8 内含子 1 和内含子 22 中的重复序列可分别与位于 F8 上游约 200kb 和下游 500kb 处的同源倒置重复序列重组,导致 F8 开放阅读框的部分序列倒位,随后无功能性蛋白产生。

目的

本研究我们对 Xq28 处的第三个新的同源重组进行了特征描述,该重组与我们之前报道的索引患者及其母亲和妹妹受影响染色体上的 F8 转录缺失一致。

结果

该重排发生在 F8 内含子 1 中的重复序列(Int1R-1)和位于 IKBKG 重复拷贝内含子 2 中的倒置相同重复序列(Int1R-2d)之间,该重复拷贝位于 F8 上游约 386kb 处。通过 Southern blot 和反向 PCR 证实了重排的存在,导致 Int1R-1 之间的 PCR 扩增失败。

结论

我们开发了一种基于 PCR 的诊断方法,可用于筛查无法识别突变的严重甲型血友病病例中的这种遗传重排。

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