Transduction of CD34+ cells by a vesicular stomach virus protein G (VSV-G) pseudotyped HIV-1 vector. Stable gene expression in progeny cells, including dendritic cells.

Journal of human virology Pub Date : 1998-07-01

X Li, T Mukai, D Young, S Frankel, P Law, F Wong-Staal

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引用次数: 0

Abstract

Objective: To use HIV-1 vectors to mediate stable gene transfer into hematopoietic stem/progenitor cells.

Study design/methods: Purified human CD34+ cells were transduced with HIV-1 vectors pseudotyped with VSV-G and subjected to colony-forming assays and differentiation in liquid culture. Transduction was determined by DNA-polymerase chain reaction (PCR) for the transgene. GFP reporter gene expression and phenotypes of progeny cells were assessed by microscopy and flow cytometry.

Results: The HIV-1 vector transduced CD34+ cells with high efficiency. Transduction did not interfere with CD34+ cells differentiation in vitro. Transduced genes are expressed in different subsets of progeny cells, including those with normal dendritic cells (DC) morphology and phenotypes (HLADR+/CD1a+/CD86+/CD14-).

Conclusions: We have demonstrated efficient transduction of hematopoietic progenitor cells by HIV-1 vectors. The transgenes are expressed in different subsets of progeny cells, which suggests stable integration. The generation of DCs stably expressing HIV antigens provides a new approach for vaccine development.

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泡状胃病毒蛋白G (VSV-G)假型HIV-1载体对CD34+细胞的转导包括树突状细胞在内的后代细胞中稳定的基因表达。

目的:利用HIV-1载体介导稳定基因转染造血干细胞/祖细胞。研究设计/方法:纯化的人CD34+细胞用VSV-G伪型HIV-1载体进行转导，并在液体培养中进行集落形成试验和分化。通过dna -聚合酶链反应(PCR)检测该基因的转导。用显微镜和流式细胞术检测GFP报告基因的表达和后代细胞的表型。结果:HIV-1载体能高效转染CD34+细胞。转导不干扰CD34+细胞的体外分化。转导的基因在后代细胞的不同亚群中表达，包括那些具有正常树突状细胞(DC)形态和表型(HLADR+/CD1a+/CD86+/CD14-)的细胞。结论:我们已经证明了HIV-1载体对造血祖细胞的有效转导。这些转基因在后代细胞的不同亚群中表达，这表明它们的整合是稳定的。稳定表达HIV抗原的dc的产生为疫苗的研制提供了新的途径。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Journal of human virology

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