Flow cytometric application of helper adenovirus (HAd) containing GFP gene flanked by two parallel loxP sites to evaluation of 293 cre-complementing cell line and monitoring of HAd in gutless Ad production

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Gutless adenoviruses (GAds), namely, all gene-deleted adenoviruses, were developed to minimize their immune responses and toxic effects for a successful gene delivery tool in gene therapy. The Cre/loxP system has been widely used for GAd production. To produce GAd with a low amount of helper adenovirus (HAd) as byproduct, it is indispensable to use 293Cre cells expressing a high level of Cre for GAd production. In this study, we constructed the HAd containing enhanced green fluorescent protein gene flanked by two parallel loxP sites (HAd/GFP). The use of HAd/GFP with flow cytometry allows one to select 293Cre cells expressing a high level of Cre without using conventional Western blot analysis. Unlike conventional HAd titration methods such as plaque assay and end-point dilution assay, it also allows one to monitor rapidly the HAd as byproduct in earlier stages of GAd amplification. Taken together, the use of HAd/GFP with flow cytometry facilitates bioprocess development for efficient GAA production.
Publisher
AMER CHEMICAL SOC
Issue Date
2004-05
Language
English
Article Type
Article
Keywords

GREEN FLUORESCENT PROTEIN; DEPENDENT VECTOR; IN-VIVO; SYSTEM; EXPRESSION; EXCISION; IMMUNITY; THERAPY; CULTURE

Citation

BIOTECHNOLOGY PROGRESS, v.20, pp.913 - 920

ISSN
8756-7938
DOI
10.1021/bp034248e
URI
http://hdl.handle.net/10203/85274
Appears in Collection
BS-Journal Papers(저널논문)
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