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使用聚合酶链反应(PCR)和序列特异性寡核苷酸对三个非洲裔人群的达菲血型基因型进行测定。

Determination of Duffy genotypes in three populations of African descent using PCR and sequence-specific oligonucleotides.

作者信息

Nickel R G, Willadsen S A, Freidhoff L R, Huang S K, Caraballo L, Naidu R P, Levett P, Blumenthal M, Banks-Schlegel S, Bleecker E, Beaty T, Ober C, Barnes K C

机构信息

Department of Medicine, Johns Hopkins University, Baltimore, Maryland, USA.

出版信息

Hum Immunol. 1999 Aug;60(8):738-42. doi: 10.1016/s0198-8859(99)00039-7.

DOI:10.1016/s0198-8859(99)00039-7
PMID:10439320
Abstract

The expression of the Duffy Antigen/Receptor for Chemokines (DARC) on red blood cells (RBC) has been commonly determined using hemagglutination tests. Because the vast majority of African individuals are Duffy-negative, screening for DARC expression on RBC is a valuable tool to assess Caucasian admixture in populations of African descent. Furthermore, blood group antigens have been frequently tested as potential risk factors for complex diseases. We established a dot-blotting protocol using sequence-specific oligonucleotides (SSOs) for the DARC-46T ("Duffy-positive") and -46C ("Duffy-negative") alleles. With this method, but not with serological methods, Duffy-positive individuals can be further characterized as homozygous or heterozygous for the dominant Duffy-positive allele, allowing more precise estimation of allele frequencies and admixture in heterogeneous populations. In unrelated African American (n = 235), Afro-Caribbean (n = 90) and Colombian (n = 93) subjects, the frequency of the -46T allele was 21.7%, 12.2% and 74.7%, respectively. The percentage of Duffy-positive individuals (homozygous or heterozygous for the -46T allele) in each population was in accordance with published frequencies. As expected, the -46C allele was not detected in 20 Caucasian subjects. This sensitive and specific method allows for the rapid and inexpensive screening of large samples for Duffy genotypes using small quantities of genomic DNA.

摘要

红细胞(RBC)上趋化因子的达菲抗原/受体(DARC)的表达通常采用血凝试验来测定。由于绝大多数非洲人是达菲阴性,因此筛查红细胞上DARC的表达是评估非洲裔人群中高加索人混合比例的一项重要工具。此外,血型抗原经常作为复杂疾病的潜在风险因素进行检测。我们建立了一种斑点杂交方案,使用针对DARC - 46T(“达菲阳性”)和 - 46C(“达菲阴性”)等位基因的序列特异性寡核苷酸(SSO)。通过这种方法,而非血清学方法,可以将达菲阳性个体进一步区分为显性达菲阳性等位基因的纯合子或杂合子,从而更精确地估计异质人群中的等位基因频率和混合比例。在不相关的非裔美国人(n = 235)、非裔加勒比人(n = 90)和哥伦比亚人(n = 93)受试者中, - 46T等位基因的频率分别为21.7%、12.2%和74.7%。每个群体中达菲阳性个体( - 46T等位基因的纯合子或杂合子)的百分比与已发表的频率一致。正如预期的那样,在20名高加索受试者中未检测到 - 46C等位基因。这种灵敏且特异的方法能够使用少量基因组DNA对大量样本进行快速且低成本的达菲基因型筛查。

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