Production and purification of high-titer foamy virus vector for the treatment of leukocyte adhesion deficiency

被引:11
|
作者
Nasimuzzaman, Md [1 ,2 ]
Lynn, Danielle [1 ]
Ernst, Rebecca [1 ]
Beuerlein, Michele [1 ]
Smith, Richard H. [3 ]
Shrestha, Archana [1 ,2 ]
Cross, Scott [1 ,4 ]
Link, Kevin [1 ]
Lutzko, Carolyn [1 ,2 ,5 ]
Nordling, Diana [1 ]
Russell, David W. [6 ]
Larochelle, Andre [3 ]
Malik, Punam [1 ,2 ]
Van der Loo, Johannes C. M. [1 ,2 ,7 ]
机构
[1] Cincinnati Childrens Hosp Med Ctr, Div Expt Hematol & Canc Biol, Cincinnati, OH 45229 USA
[2] Univ Cincinnati, Coll Med, Cincinnati, OH 45220 USA
[3] NHLBI, Hematol Branch, NIH, Bethesda, MD 20892 USA
[4] Florida Biologix, Alachua, FL USA
[5] Univ Cincinnati, Hoxworth Blood Ctr, Div Regenerat Med & Cellular Therapies, Cincinnati, OH USA
[6] Univ Washington, Div Hematol, Seattle, WA 98195 USA
[7] Childrens Hosp Philadelphia, Ctr Cellular & Mol Therapeut, Philadelphia, PA 19104 USA
关键词
GENE-THERAPY; RETROVIRAL VECTORS; LENTIVIRAL VECTORS; INTEGRATION SITES; HEPARAN-SULFATE; VIRAL VECTOR; TRANSDUCTION; PROTEINS; CELLS;
D O I
10.1038/mtm.2016.4
中图分类号
R-3 [医学研究方法]; R3 [基础医学];
学科分类号
1001 ;
摘要
Compared to other integrating viral vectors, foamy virus (FV) vectors have distinct advantages as a gene transfer tool, including their nonpathogenicity, the ability to carry larger transgene cassettes, and increased stability of virus particles due to DNA genome formation within the virions. Proof of principle of its therapeutic utility was provided with the correction of canine leukocyte adhesion deficiency using autologous CD34(+) cells transduced with FV vector carrying the canine CD18 gene, demonstrating its long-term safety and efficacy. However, infectious titers of FV-human(h) CD18 were low and not suitable for manufacturing of clinical-grade product. Herein, we developed a scalable production and purification process that resulted in 60-fold higher FV-hCD18 titers from similar to 1.7 x 10(4) to 1.0 x 10(6) infectious units (IU)/ml. Process development improvements included use of polyethylenimine-based transfection, use of a codon-optimized gag, heparin affinity chromatography, tangential flow filtration, and ultracentrifugation, which reproducibly resulted in 5,000-fold concentrated and purified virus, an overall yield of 19 +/- 3%, and final titers of 1-2 x 10(9) IU/ml. Highly concentrated vector allowed reduction of final dimethyl sulfoxide (DMSO) concentration, thereby avoiding DMSO-induced toxicity to CD34(+) cells while maintaining high transduction efficiencies. This process development results in clinically relevant, high titer FV which can be scaled up for clinical grade production.
引用
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页数:8
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