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A novel affinity gene fusion system allowing protein A-based recovery of non-immunoglobulin gene products
Authors:Gräslund Susanne  Eklund Malin  Falk Ronny  Uhlén Mathias  Nygren Per-Ake  Ståhl Stefan
Affiliation:Deltagen Proteomics Inc., 615 Arapeen Drive, Suite 300, Salt Lake City, UT 84108, USA. rsandrock@deltagenpro.com
Abstract:The capacity to produce large amounts of protein in mammalian cells is important in several contexts, including large-scale generation of biologically useful proteins, gene therapy, and transdominant genetics in cultured cells. For transdominant genetics, retroviral vectors are especially useful for delivery of expression libraries. However, even the potent CMV promoter is often unable to stimulate single-copy production of protein beyond the 1 microM level. We have adapted the HIV2/Tat expression system to retroviral vectors to boost expression above levels attainable with CMV promoters. We show that the system produces protein levels in four cell types tested which exceed levels attained by wild-type CMV or modified CMV promoters. In one cell line, the increase is 10-fold above CMV. Coupled with a stable expressed protein, levels of about 4 microM can be produced from presumptive single-copy retroviral transductants, and 30 microM from multicopy transductants.
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