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Generation of a high-titer packaging cell line for the production of retroviral vectors in suspension and serum-free media

机译:用于在悬浮液和无血清培养基中生产逆转录病毒载体的高滴度包装细胞系的产生

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摘要

Several patients with severe combined immunodeficiency-X1 disease and adenosine deaminase deficiency have been cured by retroviral-mediated gene therapy. Despite the earlier success, the production of retroviral vectors for clinical gene therapy is cumbersome, costly and lacks safety features because of the adherent nature of packaging cells and the necessity to supplement the culture media with bovine serum. The aim of this study was to generate a retrovirus packaging cell line that could be used for the production of large clinical batch vectors. Bicistronic vectors containing an internal ribosomal entry site followed by a selection gene were used to express Moloney murine leukemia gag-pol and amphotropic envelope viral proteins in HEK293 cells. The candidate clone (293GP-A2) that was selected as the packaging cell line could release recombinant green fluorescent protein retroviruses at 4 times 107 infectious viral particles per ml. Similar titers were achieved after these cells were adapted to grow in suspension and serum-free media. Furthermore, using the same culture conditions viral titers proved to be stable for a 3-month culture period. The 293GP-A2 packaging cell line has the potential to be cultured in bioreactors, opening the possibility for large-scale use of retroviral vectors in late stage clinical trials.
机译:逆转录病毒介导的基因疗法已治愈了几例严重的X1免疫缺陷综合症和腺苷脱氨酶缺乏症患者。尽管取得了较早的成功,但由于包装细胞的粘附性以及必须用牛血清补充培养基,用于临床基因治疗的逆转录病毒载体的生产麻烦,昂贵且缺乏安全性。这项研究的目的是产生一种可用于生产大型临床批次载体的逆转录病毒包装细胞系。含有内部核糖体进入位点和选择基因的双顺反子载体用于在HEK293细胞中表达莫洛尼氏鼠白血病gag-pol和两性包膜病毒蛋白。被选作包装细胞系的候选克隆(293GP-A2)可以释放重组绿色荧光蛋白逆转录病毒,其密度为每毫升107感染病毒颗粒的4倍。在使这些细胞在悬浮液和无血清培养基中生长后,可获得相似的滴度。此外,在相同的培养条件下,病毒滴度在3个月的培养时间内是稳定的。 293GP-A2包装细胞系具有在生物反应器中培养的潜力,这为后期临床试验中大规模使用逆转录病毒载体提供了可能性。

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