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一种通过聚合酶链反应和等位基因特异性引物来确定达菲(FY)血型位点上三个主要等位基因的临床适用方法。

A clinically applicable method for determining the three major alleles at the Duffy (FY) blood group locus using polymerase chain reaction with allele-specific primers.

作者信息

Olsson M L, Hansson C, Avent N D, Akesson I E, Green C A, Daniels G L

机构信息

Blood Center, University Hospital, Lund, Sweden.

出版信息

Transfusion. 1998 Feb;38(2):168-73. doi: 10.1046/j.1537-2995.1998.38298193099.x.

DOI:10.1046/j.1537-2995.1998.38298193099.x
PMID:9531948
Abstract

BACKGROUND

The clinically significant antigens of the Duffy (Fy [FY]) blood group system are expressed on the red cell form of the FY glycoprotein, a promiscuous chemokine receptor and also a receptor for malarial parasites. After the cloning of cDNA coding for FY glycoprotein, the molecular basis of the three major alleles (Fya/Fyb/Fy) has been established. Because of the mistyping of the silent Fy allele as Fyb, the error rate of current genotyping methods is high in black populations.

STUDY DESIGN AND METHODS

Two hundred blood donors (European whites and African Blacks) and some amniotic DNA samples were investigated by a new allele-specific primer polymerase chain reaction technique. Sense primers corresponding to normal and GATA-1-mutated FY gene promoter region sequences were combined with antisense primers discriminating the Fya/Fyb polymorphism.

RESULTS

Complete correlation between FY phenotypes and genotypes was obtained in all samples studied, although, in two whites and one black, serology showed weak Fyb expression while polymerase chain reaction indicated a Fyb allele. Gene frequencies were calculated.

CONCLUSION

This simple and rapid polymerase chain reaction method was shown to detect the three common alleles at the FY locus in two representative ethnic populations. Its future use as an independent technique in red cell FY investigations and for fetal genotyping in hemolytic disease of the newborn is predicted.

摘要

背景

达菲(Fy [FY])血型系统中具有临床意义的抗原在FY糖蛋白的红细胞形式上表达,FY糖蛋白是一种多特异性趋化因子受体,也是疟原虫的受体。在编码FY糖蛋白的cDNA克隆后,已确定了三个主要等位基因(Fya/Fyb/Fy)的分子基础。由于沉默的Fy等位基因被误定型为Fyb,目前的基因分型方法在黑人人群中的错误率很高。

研究设计和方法

采用一种新的等位基因特异性引物聚合酶链反应技术,对200名献血者(欧洲白人和非洲黑人)及一些羊水DNA样本进行了研究。将与正常和GATA-1突变的FY基因启动子区域序列相对应的正义引物与区分Fya/Fyb多态性的反义引物相结合。

结果

在所有研究样本中,FY表型和基因型之间完全相关,不过,在两名白人和一名黑人中,血清学显示Fyb表达较弱,而聚合酶链反应表明存在Fyb等位基因。计算了基因频率。

结论

这种简单快速的聚合酶链反应方法能够在两个代表性种族群体中检测FY位点的三个常见等位基因。预计该方法未来可作为红细胞FY研究中的一项独立技术,用于新生儿溶血病的胎儿基因分型。

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