A sensitive phenotypic assay for the determination of human immunodeficiency virus type 1 tropism

被引:33
作者
Gonzalez, Nuria [1 ]
Perez-Olmeda, Mayte [1 ]
Mateos, Elena [1 ]
Cascajero, Almudena [1 ]
Alvarez, Amparo [1 ]
Spijkers, Sanne [1 ]
Garcia-Perez, Javier [1 ]
Sanchez-Palomino, Sonsoles [2 ]
Ruiz-Mateos, Ezequiel [3 ]
Leal, Manuel [3 ]
Alcami, Jose [1 ]
机构
[1] Inst Salud Carlos III, Ctr Nacl Microbiol, AIDS Immunopathol Unit, Madrid, Spain
[2] Hosp Clin IDIBAPS, Barcelona, Spain
[3] Hosp Univ Virgen del Rocio, Serv Enfermedades Infecciosas, Seville, Spain
关键词
HIV co-receptors; phenotype; CCR5; tropism; HIV-1 CORECEPTOR USAGE; V3; LOOP; MARAVIROC; CCR5; ENV; SUSCEPTIBILITY; COMBINATION; RECEPTOR; TOOLS;
D O I
10.1093/jac/dkq379
中图分类号
R51 [传染病];
学科分类号
100401 ;
摘要
To develop a sensitive phenotypic assay based on recombinant viruses (RVs) for characterizing HIV-1 tropism. Viral tropism was assessed in 159 plasma samples. The env gene was amplified and ligated into pNL-lacZ/env-Ren, which carries a luciferase reporter gene. Resulting constructs were transfected into HEK293T cells to generate RVs. To assess co-receptor tropism, U87.CD4.CXCR4/CCR5 cells were infected and luciferase activity was measured. RVs containing env from different HIV-1 subtypes were replication competent. Minor variants were detectable in 1% of the viral population. Tropism was determined in 65% of samples with a viral load of < 1000 copies/mL. The phenotypic assay described here was validated with the Trofile (TM) and Trofile (TM) ES assays. Considering the Trofile (TM) assay as a reference, the sensitivity for R5 and R5X4/X4 detection was 90% and 77%, and the specificity was 77% and 90%, respectively. Our assay was 86% concordant with Trofile (TM) (90% for R5 and 77% for R5X4/X4). When our system was compared with Trofile (TM) ES, the concordance was 89% (86% for R5 and 92% for R5X4/X4), the sensitivity for R5 was 86% and for R5X4/X4 was 92%, and the specificity for R5 was 92% and for R5X4/X4 was 86%. The phenotypic results were compared with those obtained using the following V3 genotypic prediction tools: position-specific scoring matrix; geno2pheno[coreceptor]; C4.5; C4.5 using positions 8 and 12; PART; support vector machines; and the charge rule. We describe a system to assess co-receptor tropism based on the generation of chimeric replication-competent viruses with high sensitivity in the detection of minor populations. A good correlation of our results with Trofile (TM) assays was found.
引用
收藏
页码:2493 / 2501
页数:9
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