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Gene transfer of human TCR in primary murine T cells is improved by pseudo‐typing with amphotropic and ecotropic envelopes

转导(生物物理学) T细胞受体 生物 分子生物学 T细胞 抗原 病毒学 转染 链霉菌 细胞毒性T细胞 转基因 小鼠白血病病毒 细胞培养 基因 病毒 体外 免疫系统 免疫学 遗传学 生物化学
作者
Nadine Pouw,Elike J. Westerlaken,Ralph A. Willemsen,Reno Debets
出处
期刊:Journal of Gene Medicine [Wiley]
卷期号:9 (7): 561-570 被引量:17
标识
DOI:10.1002/jgm.1047
摘要

Abstract Background T cell receptor (TCR) gene therapy represents an attractive anti‐cancer treatment but requires further optimization of its efficacy and safety in clinically relevant models, such as those using a tumor antigen and TCR of human origin. Currently, however, there is no consensus as to what protocol is most optimal for retroviral human TCR gene transfer into primary murine T cells, most notably with respect to virus pseudo‐type. Methods Primary murine T cells were transduced, expanded and subsequently tested for transgene expression, proliferation and antigen‐specific function. To this end, murine leukemia virus (MLV) retroviruses were produced upon transfection of various packaging cells with genes encoding either green fluorescent protein (GFP) or TCRαβ specific for human melanoma antigen gp100 280–288 and the helper elements GAG/POL and ENV. Next to viral pseudotyping, the following parameters were studied: T cell densities; T cell activation; the amounts of IL‐2 and the source of serum used to supplement medium. Results The pseudo‐type of virus produced by packaging cells critically determines T cell transduction efficiencies. In fact, MLV‐A and MLV‐E pseudo‐typed viruses derived from a co‐culture of Phoenix‐A and 293T cells resulted in T cell transduction efficiencies that were two‐fold higher than those based on retroviruses expressing either VSV‐G, GALV, MLV‐A or MLV‐E envelopes. In addition, T cell densities during transduction were inversely related to transduction efficiencies. Further optimization resulted in transduction efficiencies of over 90% for GFP, and 68% for both a murine and a human (i.e. murinized) TCR. Importantly, TCR‐transduced T cells proliferate (i.e. showing a log increase in cell number in a few days) and show antigen‐specific function. Conclusions We set up a quick and versatile method to genetically modify primary murine T cells based on transient production of TCR‐positive retroviruses, and show that retroviral gene transfer of a human TCR into primary murine T cells is critically improved by viral pseudo‐typing with both MLV‐A and MLV‐E envelopes. Copyright © 2007 John Wiley & Sons, Ltd.
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