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表达凋亡转基因的腺病毒载体产量的提高。

Improved production of adenovirus vectors expressing apoptotic transgenes.

作者信息

Bruder J T, Appiah A, Kirkman W M, Chen P, Tian J, Reddy D, Brough D E, Lizonova A, Kovesdi I

机构信息

GenVec, Inc., Gaithersburg, MD 20878, USA.

出版信息

Hum Gene Ther. 2000 Jan 1;11(1):139-49. doi: 10.1089/10430340050016229.

DOI:10.1089/10430340050016229
PMID:10646646
Abstract

Adenovirus vectors expressing gene products that can induce apoptosis have potential utility in gene therapy applications ranging from the treatment of proliferative diseases to transplantation. However, adenovirus vectors carrying proapoptotic gene products are difficult to produce, as the apoptotic environment is not conducive to adenovirus gene expression and replication. Production of AdFasL/G, an adenovirus vector that expresses high levels of Fas ligand, was severely reduced in the 293 packaging cell line. Increased yields of AdFasL/G were achieved by inclusion of peptide-based caspase inhibitors in the growth medium. However, use of these inhibitors for large-scale production would be difficult and expensive. A screen for gene products that increase the yield of AdFasL/G in 293 cells revealed that the poxvirus serpin CrmA and the adenovirus 14.7K product were able to increase virus yields significantly. Apoptosis induced by AdFasL/G was attenuated in 293CrmA cell lines and virus titers were increased dramatically. However, serial passage of AdFasL/G on 293CrmA cells resulted in the generation of replication-competent adenovirus. To resolve this problem, the CrmA gene was introduced into AE25 cells, an E1-complementing cell line that has limited sequence identity with the vectors. AdFasL/G titers were increased 100-fold on AE25CrmA cells relative to the AE25 cells and RCA contamination was not detectable. In addition, adenovirus vectors that express FADD, caspase 8, and Fas/APO1 were produced efficiently in AE25CrmA and 293CrmA.

摘要

表达可诱导细胞凋亡的基因产物的腺病毒载体在从增殖性疾病治疗到移植等基因治疗应用中具有潜在效用。然而,携带促凋亡基因产物的腺病毒载体难以生产,因为凋亡环境不利于腺病毒基因表达和复制。在293包装细胞系中,表达高水平Fas配体的腺病毒载体AdFasL/G的产量严重降低。通过在生长培养基中加入基于肽的半胱天冬酶抑制剂,提高了AdFasL/G的产量。然而,使用这些抑制剂进行大规模生产既困难又昂贵。一项筛选可提高AdFasL/G在293细胞中产量的基因产物的研究表明,痘苗病毒丝氨酸蛋白酶抑制剂CrmA和腺病毒14.7K产物能够显著提高病毒产量。在293CrmA细胞系中,AdFasL/G诱导的细胞凋亡减弱,病毒滴度显著提高。然而,AdFasL/G在293CrmA细胞上连续传代导致产生具有复制能力的腺病毒。为了解决这个问题,将CrmA基因导入AE25细胞,AE25细胞是一种与载体序列同源性有限的E1互补细胞系。相对于AE25细胞,AdFasL/G在AE25CrmA细胞上的滴度提高了100倍,且未检测到RCA污染。此外,表达FADD、半胱天冬酶8和Fas/APO1的腺病毒载体在AE25CrmA和293CrmA中高效产生。

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