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与HLA - DRw52相关的DRB1等位基因:利用聚合酶链反应扩增DNA、序列特异性寡核苷酸探针及化学发光检测系统进行鉴定

HLA-DRw52-associated DRB1 alleles: identification using polymerase chain reaction-amplified DNA, sequence-specific oligonucleotide probes, and a chemiluminescent detection system.

作者信息

Shaffer A L, Falk-Wade J A, Tortorelli V, Cigan A, Carter C, Hassan K, Hurley C K

机构信息

Naval Medical Research Institute, Bethesda, MD.

出版信息

Tissue Antigens. 1992 Feb;39(2):84-90. doi: 10.1111/j.1399-0039.1992.tb01912.x.

Abstract

Polymerase chain reaction (PCR) primers were designed to specifically amplify exon 2 of the DRw52-associated DRB1 alleles for subsequent typing by sequence-specific oligonucleotide probe (SSOP) hybridization and chemiluminescent detection. The DRw52 DRB1 group, encoding 22 of the 44 W.H.O. designated DRB1 allelic products, was divided by differential PCR with two polymorphism-directed forward primers. Based on a polymorphism at codon 13, these forward primers separate the DRw52-associated alleles into subsets; one comprised of the alleles of DR3/DRw11/DRw6 and the other of DRw8/DRw12/DRB1*1404. The DRB1 alleles in the latter subset were then defined by SSOP hybridization to the amplified DNA. The preferential amplification also resulted in SSOP definition of 15 alleles in the DR3/DRw11/DRw6 subset but some DRw11/DRw13 heterozygous allelic combinations were still unresolved. Two reverse PCR primers specific for the polymorphism at codon 86 were used to obtain amplified material to which SSOP reactivity provided definitive identification of the ambiguous heterozygotes.

摘要

设计聚合酶链反应(PCR)引物以特异性扩增与DRw52相关的DRB1等位基因的外显子2,随后通过序列特异性寡核苷酸探针(SSOP)杂交和化学发光检测进行分型。编码世界卫生组织指定的44种DRB1等位基因产物中的22种的DRw52 DRB1组,通过使用两种多态性导向的正向引物进行差异PCR来划分。基于密码子13处的多态性,这些正向引物将与DRw52相关的等位基因分成子集;一个子集由DR3/DRw11/DRw6的等位基因组成,另一个由DRw8/DRw12/DRB1*1404的等位基因组成。然后通过与扩增的DNA进行SSOP杂交来定义后一个子集中的DRB1等位基因。优先扩增还导致通过SSOP在DR3/DRw11/DRw6子集中定义了15个等位基因,但一些DRw11/DRw13杂合等位基因组合仍未解决。使用两种针对密码子86处多态性的反向PCR引物来获得扩增材料,SSOP反应性可对模糊的杂合子进行明确鉴定。

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