Chinnasamy Dhanalakshmi, Milsom Michael D, Shaffer James, Neuenfeldt James, Shaaban Aimen F, Margison Geoffrey P, Fairbairn Leslie J, Chinnasamy Nachimuthu
Vince Lombardi Gene Therapy Laboratory, Immunotherapy Program, Aurora St. Luke's Medical Center, Milwaukee, WI 53215, USA.
Virol J. 2006 Mar 15;3:14. doi: 10.1186/1743-422X-3-14.
A number of gene therapy applications would benefit from vectors capable of expressing multiple genes. In this study we explored the feasibility and efficiency of expressing two or three transgenes in HIV-1 based lentiviral vector. Bicistronic and tricistronic self-inactivating lentiviral vectors were constructed employing the internal ribosomal entry site (IRES) sequence of encephalomyocarditis virus (EMCV) and/or foot-and-mouth disease virus (FMDV) cleavage factor 2A. We employed enhanced green fluorescent protein (eGFP), O6-methylguanine-DNA-methyltransferase (MGMT), and homeobox transcription factor HOXB4 as model genes and their expression was detected by appropriate methods including fluorescence microscopy, flow cytometry, immunocytochemistry, biochemical assay, and western blotting.
All the multigene vectors produced high titer virus and were able to simultaneously express two or three transgenes in transduced cells. However, the level of expression of individual transgenes varied depending on: the transgene itself; its position within the construct; the total number of transgenes expressed; the strategy used for multigene expression and the average copy number of pro-viral insertions. Notably, at limiting MOI, the expression of eGFP in a bicistronic vector based on 2A was approximately 4 times greater than that of an IRES based vector.
The small and efficient 2A sequence can be used alone or in combination with an IRES for the construction of multicistronic lentiviral vectors which can express encoded transgenes at functionally relevant levels in cells containing an average of one pro-viral insert.
许多基因治疗应用将受益于能够表达多个基因的载体。在本研究中,我们探索了在基于HIV-1的慢病毒载体中表达两个或三个转基因的可行性和效率。利用脑心肌炎病毒(EMCV)的内部核糖体进入位点(IRES)序列和/或口蹄疫病毒(FMDV)切割因子2A构建了双顺反子和三顺反子自失活慢病毒载体。我们使用增强型绿色荧光蛋白(eGFP)、O6-甲基鸟嘌呤-DNA甲基转移酶(MGMT)和同源盒转录因子HOXB4作为模型基因,并通过包括荧光显微镜、流式细胞术、免疫细胞化学、生化分析和蛋白质印迹在内的适当方法检测它们的表达。
所有多基因载体均产生高滴度病毒,并能够在转导细胞中同时表达两个或三个转基因。然而,单个转基因的表达水平因以下因素而异:转基因本身;其在构建体中的位置;表达的转基因总数;用于多基因表达的策略以及前病毒插入的平均拷贝数。值得注意的是,在限制感染复数(MOI)时,基于2A的双顺反子载体中eGFP的表达比基于IRES的载体高约4倍。
小而高效的2A序列可单独使用或与IRES结合使用,用于构建多顺反子慢病毒载体,该载体可在平均含有一个前病毒插入的细胞中以功能相关水平表达编码的转基因。
