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| June 2000, Volume 7, Number 12, Pages 1063-1066 |
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| Viral transfer technology |
| Plat-E: an efficient and stable system for transient packaging of retroviruses |
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| S Morita, T Kojima and T Kitamura |
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Department of Hematopoietic Factors, Institute of Medical Science, University of Tokyo, 4-6-1 Shirokanedai Minato-ku, Tokyo 108-8639, Japan
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Correspondence to: T Kitamura |
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| Abstract |
 | A potent retrovirus packaging cell line named Platinum-E (Plat-E) was generated based on the 293T cell line. Plat-E is superior to existing packaging cell lines regarding efficiency, stability and safety. The novel packaging constructs utilized in establishment of Plat-E ensure high and stable expression of viral structural proteins. Conventional packaging constructs made use of the promoter of MuLV-LTR for expression of viral structural genes gag-pol and env, while our packaging constructs utilized the EF1 promoter, which is 100-fold more potent than the MuLV-LTR in 293T cells in combination with the Kozak's consensus sequence upstream of the initiation codon resulting in high expression of virus structural proteins in Plat-E cells. To maintain the high titers of retroviruses under drug selection pressure, we inserted the IRES (internal ribosome entry site) sequence between the gene encoding gag-pol or env, and the gene encoding a selectable marker in the packaging constructs. Plat-E cells can stably produce retroviruses with an average titer of 1 ´ 107/ml for at least 4 months. In addition, as we used only the coding sequences of viral structural genes to avoid inclusion of unnecessary retrovirus sequences in the packaging constructs, the probability of generating the replication competent retroviruses (RCR) by recombination can virtually be ruled out. Gene Therapy (2000) 7, 1063-1066. |
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| Keywords |
 | packaging cell; retroviruses; ecotropic; EF1 promoter |
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| Received 3 November 1999; accepted 3 March 2000 |
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| June 2000, Volume 7, Number 12, Pages 1063-1066 |
| Table of contents Previous Abstract Next Full text PDF |
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