通过聚合酶链反应（PCR）改进对双重血清反应阳性个体中HIV-2前病毒DNA的检测。

Improved detection of HIV-2 proviral DNA in dually seroreactive individuals by PCR.

作者信息

Ishikawa K, Fransen K, Ariyoshi K, Nkengasong J N, Janssens W, Heyndrickx L, Whittle H, Diallo M O, Ghys P D, Coulibaly I M, Greenberg A E, Piedade J, Canas-Ferreira W, van der Groen G

机构信息

Institute of Tropical Medicine, Antwerp, Belgium.

出版信息

AIDS. 1998 Aug 20;12(12):1419-25. doi: 10.1097/00002030-199812000-00003.

DOI:10.1097/00002030-199812000-00003

PMID:9727562

Abstract

OBJECTIVE

To improve the detection rate of HIV-2 proviral DNA in primary uncultured peripheral blood mononuclear cells (PBMC) of HIV-2-seroreactive and HIV-1-HIV-2 dually seroreactive individuals.

MATERIALS AND METHODS

Two newly designed HIV-2 PCR primer pairs in the long terminal repeat (LTR) gag and gag-pol regions and a previously described env and LTR HIV-2 PCR primer pairs were tested on samples from 66 confirmed HIV-2-seropositive individuals (The Gambia, 40; Côte d'Ivoire, 17; Guinea-Bissau, nine), 209 dually seroreactive individuals (The Gambia, 82; Côte d'Ivoire, 127), 24 genetically characterized isolated HIV-1 strains (group M subtypes A-H and group O), one simian immunodeficiency virus (SIV) strain cpz, 10 HIV-2 isolates (subtype A, B and unidentified), two SIVsm isolates, and 10 seronegative samples.

RESULTS

All HIV-2 primers evaluated showed 100% specificity since there was no amplification observed with 24 HIV-1, one SIVcpz and 10 seronegative samples. One single copy of the HIV-2 genome could be detected with all outer primer pairs as well as all inner primer pairs on one PCR round used. Sensitivity of primers (at least one of the four primer pairs was positive) to HIV-2-seropositive samples was 100% (all nine) in Guinea-Bissau, 71% (12/17) in Côte d'Ivoire, 100% (all 20) in Gambian AIDS patients, and 85% (17/20) in Gambian pregnant women. Doubling the PBMC of dually seroreactive individuals from 7.5 x 10(4) to 1.5 x 10(5) in the PCR revealed the presence of both HIV-1 and 2 proviral DNA in 72% (92/127) in Côte d'Ivoire and 72% (59/82) in The Gambia. By doubling the number of PBMC, HIV-2 detection in dually seroreactive individuals by PCR was increased from 65 to 77% in Côte d'Ivoire and from 67 to 83% in The Gambia.

CONCLUSIONS

The use of 1.5 x 10(5) primary uncultured PBMC and the newly designed HIV-2 primer pairs allowed us to document the highest percentage (72%) ever reported of HIV-1-HIV-2 dual infections amongst HIV-1-HIV-2 dually seroreactive individuals in Côte d'Ivoire and The Gambia. Improved detection of HIV-2 proviral DNA, rather than exposure to both viruses, infection with only one virus, or infection with a unique third virus containing epitopes common to both HIV-1 and HIV-2, contributes to a more accurate monitoring of the prevalence of HIV-1-HIV-2 dual infections.

摘要

目的

提高在HIV-2血清反应阳性个体以及HIV-1-HIV-2双重血清反应阳性个体未经培养的外周血单个核细胞（PBMC）中HIV-2前病毒DNA的检测率。

材料与方法

在66例确诊的HIV-2血清阳性个体（冈比亚40例；科特迪瓦17例；几内亚比绍9例）、209例双重血清反应阳性个体（冈比亚82例；科特迪瓦127例）、24株经基因特征鉴定的分离HIV-1毒株（M组A - H亚型及O组）、1株猿猴免疫缺陷病毒（SIV）cpz毒株、10株HIV-2分离株（A、B亚型及未分型）、2株SIVsm分离株以及10份血清阴性样本中，对新设计的位于长末端重复序列（LTR）gag和gag - pol区域的两对HIV-2 PCR引物以及先前描述的env和LTR区域的HIV-2 PCR引物进行检测。

结果

所有评估的HIV-2引物均显示出100%的特异性，因为在24份HIV-1样本、1份SIVcpz样本以及10份血清阴性样本中均未观察到扩增现象。在一轮PCR反应中，所有外部引物对以及所有内部引物对均能检测到单拷贝的HIV-2基因组。引物对HIV-2血清阳性样本的敏感性（四个引物对中至少一个呈阳性）在几内亚比绍为100%（9例全部阳性），在科特迪瓦为71%（12/17），在冈比亚艾滋病患者中为100%（20例全部阳性），在冈比亚孕妇中为85%（17/20）。在PCR反应中将双重血清反应阳性个体的PBMC数量从7.5×10⁴增加到1.5×10⁵，结果显示在科特迪瓦72%（92/127）以及在冈比亚72%（59/82）的个体中同时存在HIV-1和2前病毒DNA。通过将PBMC数量翻倍，在科特迪瓦双重血清反应阳性个体中通过PCR检测HIV-2的比例从65%提高到77%，在冈比亚从67%提高到83%。

结论

使用1.5×10⁵未经培养的原代PBMC以及新设计的HIV-2引物对，使我们能够记录到在科特迪瓦和冈比亚的HIV-1-HIV-2双重血清反应阳性个体中，HIV-1-HIV-2双重感染率达到了有史以来最高的72%。对HIV-2前病毒DNA检测的改进，而非同时暴露于两种病毒、仅感染一种病毒或感染一种含有HIV-1和HIV-2共同表位的独特第三种病毒，有助于更准确地监测HIV-1-HIV-2双重感染的流行情况。