趋化因子受体CCR5 Δ32使用多种标本类型和NucliSens基本试剂盒的遗传分析

S. Tetali, Eun Mi Lee, M. Kaplan, Joseph P. Romano, C. Ginocchio
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引用次数: 6

摘要

HIV-1感染抵抗和疾病进展延迟与编码CCR5趋化因子受体的基因32 bp缺失(Δ32)有关。在本研究中,我们使用一种新的靶向特异性三明治寡核苷酸检测方法,对基于核酸序列扩增(NASBA)的CCR5基因分型检测方法进行了修改,用于NucliSens基本试剂盒(Organon Teknika, Durham, N.C.)格式。新方法允许使用NucliSens Basic Kit中提供的通用电化学发光探针,而原始的NASBA方法需要昂贵的靶向特异性钌检测探针。Basic Kit CCR5 Δ32基因型分析与原始NASBA测定和DNA PCR结果100%一致。本研究还评估了多种标本类型的使用,包括外周血单个核细胞(PBMC)、全血、干血斑、口腔刮痕和血浆,用于CCR5基因型分析。当PBMC或全血为标本来源时,这三种检测方法的敏感性可比较。相比之下,当使用干血斑、口腔刮痕或血浆作为样品源时,DNA PCR的灵敏度分别为80.95、42.8和0%,而原始NASBA和Basic Kit NASBA检测方法的灵敏度为100%。我们的研究表明,NucliSens Basic Kit NASBA检测对CCR5 Δ32多种样品类型的基因分型非常敏感和特异性。
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Chemokine Receptor CCR5 Δ32 Genetic Analysis Using Multiple Specimen Types and the NucliSens Basic Kit
ABSTRACT Resistance to HIV-1 infection and delayed disease progression have been associated with a 32-bp deletion (Δ32) in the gene encoding the CCR5 chemokine receptor. In the present study we describe the modification of a nucleic acid sequence-based amplification (NASBA)-based CCR5 genotyping assay for a NucliSens Basic Kit (Organon Teknika, Durham, N.C.) format using a new target-specific sandwich oligonucleotide detection methodology. The new method permitted the use of generic electrochemiluminescent probes supplied in the NucliSens Basic Kit, whereas the original NASBA method required expensive target-specific ruthenium detection probes. The Basic Kit CCR5 Δ32 genotypic analysis was in 100% concordance with both the original NASBA assay and DNA PCR results. This study also evaluated the use of multiple specimen types, including peripheral blood mononuclear cells (PBMC), whole blood, dried blood spots, buccal scrapings, and plasma, for CCR5 genotype analysis. The sensitivities of the three assays were comparable when PBMC or whole blood was the specimen source. In contrast, when dried blood spots, buccal scrapings, or plasma was used as the sample source, the sensitivity of DNA PCR was 80.95, 42.8, or 0%, respectively, compared to 100% sensitivity obtained with the original NASBA and Basic Kit NASBA assays. Our study indicates that the NucliSens Basic Kit NASBA assay is very sensitive and specific for CCR5 Δ32 genotyping using multiple sample types.
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