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Development of a nucleic acid sequence-based amplification assay that uses gag-based molecular beacons to distinguish between human immunodeficiency virus type 1 subtype C and C ' infections in Ethiopia

机译:开发基于核酸序列的扩增检测方法,该方法使用基于gag的分子信标区分埃塞俄比亚的人类免疫缺陷病毒1型C亚型和C'感染

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摘要

A gag-based molecular beacon assay utilizing real-time nucleic acid sequence-based amplification technology has been developed to differentiate between the two genetic subclusters of human immunodeficiency virus type I (HIV-1) subtype C (C and C') circulating in Ethiopia. Of 41 samples, 36 could be classified as C or C' by sequencing of the gag gene. All 36 isolates were correctly identified by the gag beacon test. Three isolates with genomes that were recombinant in gag were unambiguously typed as belonging to the C' subcluster. Further analysis revealed that these contained the most sequence homology with a reference subcluster C' sequence in the target region of the beacon and hence were correct for the analyzed region. For one sample, sequencing and gag molecular beacon results did not match, while another isolate could not be detected at all by the beacon assay. Overall, high levels of sensitivity and specificity were achieved for both beacons (90.5% sensitivity and 100% specificity for the C beacon and 100% sensitivity and 95.2% specificity for the C' beacon). The availability of a diagnostic test which can quickly and reliably discriminate between C and C' HIV-1 infections in Ethiopia is an important first step toward studying their respective biological characteristics. As the assay is specific to the Ethiopian HIV-1 subtype C epidemic, it will contribute to characterizing the circulating viruses in this population, thereby generating the information necessary for the development of a potential efficacious HIV-1 vaccine appropriate for the Ethiopian context
机译:已经开发了一种基于gag的分子信标测定法,利用基于实时核酸序列的扩增技术来区分在埃塞俄比亚传播的人类免疫缺陷病毒I型(HIV-1)C型(C和C')的两个遗传亚群。在41个样本中,通过对gag基因进行测序可以将36个样本分类为C或C'。通过gag beacon测试可以正确识别所有36个分离株。带有gag重组基因组的三个分离株被明确地确定为属于C'亚簇。进一步的分析表明,它们与信标靶区域中的参考亚簇C'序列具有最高的序列同源性,因此对于分析区域而言是正确的。对于一个样品,测序和gag分子信标结果不匹配,而通过信标测定根本无法检测到另一种分离物。总体而言,两个信标都达到了很高的灵敏度和特异性水平(C信标的灵敏度为90.5%和100%,C'信标的灵敏度为100%和95.2%)。可以快速可靠地区分埃塞俄比亚C和C'HIV-1感染的诊断测试方法是研究其各自生物学特征的重要第一步。由于该测定法是针对埃塞俄比亚HIV-1 C亚型流行病的特异性,因此它将有助于表征该人群中正在传播的病毒,从而为开发适合埃塞俄比亚环境的潜在有效HIV-1疫苗提供必要的信息

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