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- W2360441420 abstract "Objective We constructed an expression vector containing EGFP fused to the viral TAT transduction domain and driven by the prostate-specific antigen promoter(pPSA-TAT-EGFP) by gene cloning technology.The targeting expression of pPSA-TAT-EGFP was examined in prostate cancer cells and colon cells.Methods The vector pEGFP-1 served as the framework,and the fragment with the TAT sequence and EGFP was produced by using polymerase chain reaction.After digestion with SalI and NotI enzymes,the fragment was inserted into the T cloning vector.The EGFP expression plasmid driven by the PSA promoter(pPSA-EGFP) was digested overnight with SalI and NotI,and a large fragment containing the PSA promoter was purified by gel purification.The TAT-EGFP,cut with SalI and NotI from the T-vector,was linked with the large fragment with the PSA promoter sequence and generated the pPSA-TAT-EGFP construct.The construct was confirmed by restriction enzyme digestion and DNA sequencing,and tested by transfection assay.Result The expression vector pPSA-TAT-EGFP was constructed.It was expressed in prostate carcinoma cells,but was not detected in colon cells.Conclusion A slightly higher expression was observed in cells transfected with EGFP fused to TAT compared to the EGFP control plasmid in prostate cancer cells,but no detectable expression was shown in colon cells." @default.
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- W2360441420 date "2008-01-01" @default.
- W2360441420 modified "2023-09-26" @default.
- W2360441420 title "Targeting expression of TAT-EGFP driven by the prostate specific antigen promoter" @default.
- W2360441420 hasPublicationYear "2008" @default.
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