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慢病毒载体转导的小干扰RNA对在SCID-hu小鼠中分化的T淋巴细胞及CD34+祖细胞来源的巨噬细胞中HIV-1的抑制作用

Inhibition of HIV-1 by lentiviral vector-transduced siRNAs in T lymphocytes differentiated in SCID-hu mice and CD34+ progenitor cell-derived macrophages.

作者信息

Banerjea Akhil, Li Ming-Jie, Bauer Gerhard, Remling Leila, Lee Nan-Sook, Rossi John, Akkina Ramesh

机构信息

Department of Microbiology, Immunology and Pathology, Colorado State University, 1619 Campus Drive, Fort Collins, Colorado 80523, USA.

出版信息

Mol Ther. 2003 Jul;8(1):62-71. doi: 10.1016/s1525-0016(03)00140-0.

Abstract

The phenomenon of RNA interference mediated by small interfering RNAs (siRNAs) is a potent gene-silencing mechanism. A number of recent studies demonstrated inhibition of HIV-1 replication in cultured cells using this approach. To make further progress and harness this technology for HIV-1 gene therapy in a stem cell setting, in vivo studies using primary hematopoietic cells are needed. Using an HIV-based lentiviral vector we introduced an anti-Rev siRNA construct into CD34(+) hematopoietic progenitor cells. The siRNA-transduced progenitor cells were allowed to mature into macrophages in vitro and T cells in vivo in SCID-hu mouse thy/liv grafts. Phenotypically normal T cells and macrophages displaying characteristic surface markers were obtained. In vitro HIV-1 challenge of the siRNA-expressing macrophages and T cells with macrophage-tropic and T-cell-tropic HIV-1, respectively, showed marked viral resistance. These experiments demonstrate the utility of siRNAs delivered into hematopoietic stem cells via lentiviral vectors for future in vivo applications.

摘要

由小干扰RNA(siRNA)介导的RNA干扰现象是一种强大的基因沉默机制。最近的一些研究表明,使用这种方法可抑制培养细胞中的HIV-1复制。为了取得进一步进展并将该技术应用于干细胞环境下的HIV-1基因治疗,需要使用原代造血细胞进行体内研究。我们使用基于HIV的慢病毒载体将抗Rev siRNA构建体导入CD34(+)造血祖细胞。经siRNA转导的祖细胞在体外成熟为巨噬细胞,并在SCID-hu小鼠甲状腺/肝脏移植物中在体内成熟为T细胞。获得了表型正常且显示特征性表面标志物的T细胞和巨噬细胞。分别用嗜巨噬细胞型和嗜T细胞型HIV-1对表达siRNA的巨噬细胞和T细胞进行体外HIV-1攻击,结果显示出明显的病毒抗性。这些实验证明了通过慢病毒载体将siRNA导入造血干细胞在未来体内应用中的实用性。

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