Trinh Alice T, Ball Bret G, Weber Erin, Gallaher Timothy K, Gluzman-Poltorak Zoya, Anderson French, Basile Lena A
Neumedicines Inc, Pasadena, California 91107, USA.
Genet Vaccines Ther. 2009 Dec 30;7:13. doi: 10.1186/1479-0556-7-13.
Murine retroviral vectors have been used in several hundred gene therapy clinical trials, but have fallen out of favor for a number of reasons. One issue is that gene expression from viral or internal promoters is highly variable and essentially unregulated. Moreover, with retroviral vectors, gene expression is usually silenced over time. Mammalian genes, in contrast, are characterized by highly regulated, precise levels of expression in both a temporal and a cell-specific manner. To ascertain if recapitulation of endogenous adenosine deaminase (ADA) expression can be achieved in a vector construct we created a new series of Moloney murine leukemia virus (MuLV) based retroviral vector that carry human regulatory elements including combinations of the ADA promoter, the ADA locus control region (LCR), ADA introns and human polyadenylation sequences in a self-inactivating vector backbone.
A MuLV-based retroviral vector with a self-inactivating (SIN) backbone, the phosphoglycerate kinase promoter (PGK) and the enhanced green fluorescent protein (eGFP), as a reporter gene, was generated. Subsequent vectors were constructed from this basic vector by deletion or addition of certain elements. The added elements that were assessed are the human ADA promoter, human ADA locus control region (LCR), introns 7, 8, and 11 from the human ADA gene, and human growth hormone polyadenylation signal. Retroviral vector particles were produced by transient three-plasmid transfection of 293T cells. Retroviral vectors encoding eGFP were titered by transducing 293A cells, and then the proportion of GFP-positive cells was determined using fluorescence-activated cell sorting (FACS). Non T-cell and T-cell lines were transduced at a multiplicity of infection (MOI) of 0.1 and the yield of eGFP transgene expression was evaluated by FACS analysis using mean fluorescent intensity (MFI) detection.
Vectors that contained the ADA LCR were preferentially expressed in T-cell lines. Further improvements in T-cell specific gene expression were observed with the incorporation of additional cis-regulatory elements, such as a human polyadenylation signal and intron 7 from the human ADA gene.
These studies suggest that the combination of an authentically regulated ADA gene in a murine retroviral vector, together with additional locus-specific regulatory refinements, will yield a vector with a safer profile and greater efficacy in terms of high-level, therapeutic, regulated gene expression for the treatment of ADA-deficient severe combined immunodeficiency.
鼠逆转录病毒载体已用于数百项基因治疗临床试验,但由于多种原因已不再受青睐。一个问题是病毒或内部启动子的基因表达高度可变且基本不受调控。此外,对于逆转录病毒载体,基因表达通常会随着时间的推移而沉默。相比之下,哺乳动物基因的特征是在时间和细胞特异性方面都具有高度调控、精确的表达水平。为了确定在载体构建体中是否可以实现内源性腺苷脱氨酶(ADA)表达的重现,我们创建了一系列基于莫洛尼鼠白血病病毒(MuLV)的新型逆转录病毒载体,这些载体在自失活载体骨架中携带人类调控元件,包括ADA启动子、ADA基因座控制区(LCR)、ADA内含子和人类聚腺苷酸化序列的组合。
构建了一种基于MuLV的具有自失活(SIN)骨架、磷酸甘油酸激酶启动子(PGK)和增强型绿色荧光蛋白(eGFP)作为报告基因的逆转录病毒载体。随后的载体通过删除或添加某些元件从该基本载体构建而成。评估添加的元件包括人类ADA启动子、人类ADA基因座控制区(LCR)、人类ADA基因的内含子7、8和11以及人类生长激素聚腺苷酸化信号。通过对293T细胞进行瞬时三质粒转染产生逆转录病毒载体颗粒。通过转导293A细胞对编码eGFP的逆转录病毒载体进行滴度测定,然后使用荧光激活细胞分选(FACS)确定GFP阳性细胞的比例。以0.1的感染复数(MOI)转导非T细胞和T细胞系,并使用平均荧光强度(MFI)检测通过FACS分析评估eGFP转基因表达的产量。
含有ADA LCR的载体在T细胞系中优先表达。通过加入额外的顺式调控元件,如人类聚腺苷酸化信号和人类ADA基因的内含子7,观察到T细胞特异性基因表达有进一步改善。
这些研究表明,在鼠逆转录病毒载体中真实调控的ADA基因与额外的基因座特异性调控优化相结合,将产生一种在治疗ADA缺陷的严重联合免疫缺陷方面具有更安全的特征和更高疗效的载体,可实现高水平、治疗性、受调控的基因表达。
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