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| 广西HIV-1重组毒株env区快速基因分型方法的建立 | |
| 引用本文: | 梁浩,罗皓,邵一鸣,刘伟,张志勇,邢辉,卢灿健,沈菁,麦志丹.广西HIV-1重组毒株env区快速基因分型方法的建立[J].中华实验和临床病毒学杂志,2006,20(3):282-284. |
| 作者姓名: | 梁浩 罗皓 邵一鸣 刘伟 张志勇 邢辉 卢灿健 沈菁 麦志丹 |
| 作者单位: | 1. 530021,南宁,广西医科大学 2. 中国疾病预防控制中心性病艾滋病预防与控制中心 3. 广西区疾病预防控制中心 4. 横县卫生防疫站 |
| 基金项目: | 广西科学基金项目(桂科自0447049) |
| 摘 要: | 目的建立一种快速简便的基因分型方法,对广西HIV-1重组毒株env基因区进行亚型鉴定。方法从HIV阳性样品中提取核酸,使用HIV-1M组通用引物对env区进行第一轮扩增,第二轮则使用分别检测B′/C或C亚型和CRF01-AE亚型的二套特异性引物放入同一反应管中进行扩增,根据不同亚型扩增的目的带位置不同来判断亚型。将通用引物扩增出的所有样本均进行基因测序和系统树分析以验证结果。结果50份样本中,经基因测序和系统树分析证实CRF08-BC样本3份(6%),CRF01-AE样本43份(86%),4份(8%)样本无法确定亚型。经亚型特异性引物PCR法检测得出B′/C或C亚型样本3份(100%),CRF01-AE样本39份(90.7%),灵敏度为91.3%,特异度为100%。两种方法检测结果经差异性检验显示X^2=2.25,P〉0.05,差异无统计学意义,结果一致者占92%。与基因分析结果吻合。重复实验显示CRF08-BC平均重复性为100%(10/10),CRF01.AE为93.8%(61/65)。结论该方法是一种简便、快速、低成本,具有高度灵敏性和特异性的HIV-1毒株env基因区分型法,能够直接对广西HIV-1 CRF01-AE重组毒株进行鉴定。 |
| 关 键 词: | HIV-1 基因型 聚合酶链反应 |
| 收稿时间: | 2005-09-27 |
| 修稿时间: | 2005年9月27日 |
Development of a rapid subtype-screening assay for the env region of HIV-1 CRF strains in Guangxi |
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| LIANG Hao,LUO Hao,SHAO Yi-ming,LIU Wei,ZHANG Zhi-yong,XING Hui,LU Can-jian,SHEN Jing,MAI Zhi-dan.Development of a rapid subtype-screening assay for the env region of HIV-1 CRF strains in Guangxi[J].Chinese Journal of Experimental and Clinical Virology,2006,20(3):282-284. | |
| Authors: | LIANG Hao LUO Hao SHAO Yi-ming LIU Wei ZHANG Zhi-yong XING Hui LU Can-jian SHEN Jing MAI Zhi-dan |
| Institution: | Guangxi Medical Univeristy, Nanning 530021, China |
| Abstract: | BACKGROUND: To develop a simple and rapid subtype-screening assay for the env region of the circulating recombinant form (CRF) of human immunodeficiency virus type 1 (HIV-1) in Guangxi. METHODS: Proviral DNA from HIV-1 positive samples were extracted and subjected to the first round PCR with universal primers for the env region that can detect HIV-1 M group isolates. In the second round PCR, two pairs of subtype-specific primers that were designed to detect subtype C or B'/C and CRF01-AE respectively were added into one tube. The PCR products of different subtypes could be distinguished in agarose-gel electrophoresis. Additionally, all of these samples were sequenced and analyzed phylogenetically. RESULTS: Phylogenetic analysis of the env region of 50 samples showed that 3 samples (6%) were infected with CRF08-BC, 43 (86%) with CRF01-AE, and 4 (8%) remained unclassifiable. Detection of the subtype-specific primer sets revealed that 3 were subtype C or B'/C (100%), 39 were CRF01-AE (90.7%), with an adequate sensitivity (91.3%) and a high specificity (100%). Non-specific bands occasionally appeared but did not interfere with interpretation of the results. The phylogenetic analysis was consistent with subtype-specific primer sets and the consistency rate was 92%. The average reproducibility was 100% for CRF08-BC samples and 93.8% for CRF01-AE samples. CONCLUSION: A simple, rapid and low cost assay was developed for subtype-screening of CRF01-AE in Guangxi. |
| Keywords: | HIV-1 Genotype Polymerase chain reaction |
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