一种用于功能性HIV-1 env基因拯救与分析的有效方法：tat/rev剪接位点附近重组的证据

An efficient method for the rescue and analysis of functional HIV-1 env genes: evidence for recombination in the vicinity of the tat/rev splice site.

作者信息

Douglas N W, Knight A I, Hayhurst A, Barrett W Y, Kevany M J, Daniels R S

机构信息

Virology Division, National Institute of Medical Research, Mill Hill, London, UK.

出版信息

AIDS. 1996 Jan;10(1):39-46. doi: 10.1097/00002030-199601000-00006.

DOI:10.1097/00002030-199601000-00006

PMID:8924250

Abstract

OBJECTIVE

To establish a robust procedure for the isolation and characterization of full-length expression-competent HIV-1 env genes directly from patient samples.

DESIGN

HIV exists as a quasispecies which can be disturbed by in vitro culture, in which numerous members of the population are likely to be defective due to the high error rate of the viral reverse transcriptase. Defective viruses are unlikely to play a dominant role in disease progression. Since env gene translation products play major roles in the initiation and spread of infection we need to study genes with open reading frames.

METHODS

A nested polymerase chain reaction (PCR) approach has been used to rescue intact (2.6 kb) env genes, which are cloned into a T7-promoter-containing vector. Expression of gp160 in CV-1 cells is detected by Western blot. Expression-competent clones are sequenced and resulting sequences used for phylogenetic studies. Translation products are analysed in relation to the known immunogenic structure of gp160.

RESULTS

From random patient samples collected in London clinics, only HIV-1 subtype B was found. Two of the samples contained viruses with an additional pair of cysteine residues in their V1 regions. For samples collected in Uganda, HIV-1 subtypes A, D and an A/D recombinant were recovered.

CONCLUSION

An effective procedure is described for the isolation of HIV-1 env genes directly from patient samples, which has worked for A, B and D subtypes to date. The PCR primers can be utilized with other subtypes with the possible exception of subtype O viruses. Phylogenetic analyses revealed the potential importance of a G/C-rich region near the tat/rev splice site as a site of recombination. The sequences and translation products generated may be more relevant to disease progression in vivo and vaccine formulations than those obtained from viruses selected in long-term culture.

摘要

目的

建立一种直接从患者样本中分离和鉴定全长具有表达能力的HIV-1 env基因的可靠方法。

设计

HIV以准种形式存在，体外培养可能会干扰其状态，由于病毒逆转录酶的高错误率，群体中的许多成员可能存在缺陷。缺陷病毒在疾病进展中不太可能起主导作用。由于env基因翻译产物在感染的起始和传播中起主要作用，我们需要研究具有开放阅读框的基因。

方法

采用巢式聚合酶链反应（PCR）方法拯救完整的（2.6 kb）env基因，将其克隆到含T7启动子的载体中。通过蛋白质免疫印迹法检测CV-1细胞中gp160的表达。对具有表达能力的克隆进行测序，并将所得序列用于系统发育研究。根据已知的gp160免疫原性结构分析翻译产物。

结果

在伦敦诊所收集的随机患者样本中，仅发现HIV-1 B亚型。其中两个样本中的病毒在其V1区域有一对额外的半胱氨酸残基。在乌干达收集的样本中，回收了HIV-1 A、D亚型以及一种A/D重组体。

结论

描述了一种直接从患者样本中分离HIV-1 env基因有效的方法，该方法目前已适用于A、B和D亚型。除O亚型病毒外，PCR引物可用于其他亚型。系统发育分析揭示了tat/rev剪接位点附近富含G/C的区域作为重组位点的潜在重要性。与从长期培养中选择的病毒获得的序列和翻译产物相比，所产生的序列和翻译产物可能与体内疾病进展和疫苗配方更相关。