Efficient FLPe recombinase enables scalable production of helper-dependent adenoviral vectors with negligible helper-virus contamination

被引:106
|
作者
Umaña, P
Gerdes, CA
Stone, D
Davis, JRE
Ward, D
Castro, MG
Lowenstein, PR
机构
[1] Univ Manchester, Sch Med, Mol Med & Gene Therapy Unit, Manchester M13 9PT, Lancs, England
[2] Univ Manchester, Endocrine Sci Res Grp, Manchester M13 9PT, Lancs, England
[3] Univ Manchester, ARC Epidemiol Unit, Manchester M13 9PT, Lancs, England
基金
英国医学研究理事会; 英国生物技术与生命科学研究理事会; 美国国家卫生研究院;
关键词
D O I
10.1038/89349
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
Helper-dependent (HD), high-capacity adenoviruses are one of the most efficient and safe gene therapy vectors, capable of mediating long-term expression(1-12). Currently, the most widely used system for HD vector production avoids significant contamination with helper virus by using producer cells stably expressing a nuclear-targeted Cre recombinase and an engineered first-generation helper virus with parallel loxP sites flanking its packaging signal(1,3-12). The system requires a final, density-based separation of HD and residual helper viruses by ultracentrifugation to reduce contaminating helper virus to low levels. This separation step hinders large-scale production of clinical-grade HD virus(13), By using a very efficient recombinase, in vitro-evolved FLPe (ref. 14), to excise the helper virus packaging signal in the producer cells, we have developed a scalable HD vector production method. FLP has previously been shown to mediate maximum levels of excision close to 100% compared to 80% for Cre (ref. 15). Utilizing a common HD plasmid backbone(1,7,8,10-12), the FLPe-based system reproducibly yielded HD virus with the same low levels of helper virus contamination before any density-based separation by ultracentrifugation. This should allow large-scale production of HD vectors using column chromatography-based virus purification(13).
引用
收藏
页码:582 / 585
页数:4
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