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使用变性梯度凝胶电泳和直接测序法进行高分辨率HLA - DRB分型

High-resolution HLA-DRB typing using denaturing gradient gel electrophoresis and direct sequencing.

作者信息

Knapp L A, Lehmann E, Hennes L, Eberle M E, Watkins D I

机构信息

Wisconsin Regional Primate Research Center, University of Wisconsin, Madison, USA.

出版信息

Tissue Antigens. 1997 Aug;50(2):170-7. doi: 10.1111/j.1399-0039.1997.tb02856.x.

DOI:10.1111/j.1399-0039.1997.tb02856.x
PMID:9271827
Abstract

High-resolution HLA-DRB typing is required for bone marrow transplantation between unrelated donors and recipients and also for identification of novel HLA-DRB alleles. Here we describe a method for the unambiguous identification of HLA-DRB alleles using the polymerase chain reaction (PCR), denaturing gradient gel electrophoresis (DGGE) and direct sequencing. The highly variable second exon of all HLA-DRB1, -DRB3, -DRB4, -DRB5, -DRB6 and -DRB7 alleles was amplified using a single pair of generic DRB-specific primers and alleles were separated by DGGE. DNA was then reamplified from plugs removed from the gel and the sequences of these alleles were determined using fluorescent-based sequencing and allele-assignment software. The validity of this typing procedure was confirmed by identification of HLA-DRB alleles for 17 individuals previously characterized by PCR-SSP and/or cloning and sequencing techniques. We identified 34 different HLA-DRB alleles in these 17 unrelated individuals. Importantly, our analysis revealed HLA-DRB1 alleles which had not been identified using the PCR-SSP typing technique. Additionally, alleles from the HLA-DRB3, -DRB4 and -DRB5 loci were identified. Whereas traditional HLA-DRB typing methods provide limited information or require the use of multiple oligonucleotide primers or probes, our technique provides a reliable, specific and relatively rapid way of identifying all HLA-DRB alleles for high-resolution tissue typing.

摘要

在无关供体与受体之间进行骨髓移植以及鉴定新的HLA - DRB等位基因时,需要进行高分辨率的HLA - DRB分型。在此,我们描述一种使用聚合酶链反应(PCR)、变性梯度凝胶电泳(DGGE)和直接测序来明确鉴定HLA - DRB等位基因的方法。使用一对通用的DRB特异性引物扩增所有HLA - DRB1、- DRB3、- DRB4、- DRB5、- DRB6和 - DRB7等位基因的高变第二外显子,并通过DGGE分离等位基因。然后从凝胶中切下的胶块重新扩增DNA,并使用基于荧光的测序和等位基因指定软件确定这些等位基因的序列。通过对17名先前已用PCR - SSP和/或克隆及测序技术进行特征分析的个体进行HLA - DRB等位基因鉴定,证实了该分型程序的有效性。我们在这17名无关个体中鉴定出34种不同的HLA - DRB等位基因。重要的是,我们的分析揭示了使用PCR - SSP分型技术未鉴定出的HLA - DRB1等位基因。此外,还鉴定出了来自HLA - DRB3、- DRB4和 - DRB5位点的等位基因。传统的HLA - DRB分型方法提供的信息有限,或者需要使用多个寡核苷酸引物或探针,而我们的技术提供了一种可靠、特异且相对快速的方法,用于高分辨率组织分型中鉴定所有HLA - DRB等位基因。

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