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pHUSH: a single vector system for conditional gene expression
Authors:Daniel C Gray  Klaus P Hoeflich  Li Peng  Zhenyu Gu  Alvin Gogineni  Lesley J Murray  Mike Eby  Noelyn Kljavin  Somasekar Seshagiri  Mary J Cole  David P Davis
Institution:1. Department of Molecular Biology, Genentech Inc, South San Francisco, California, USA
2. Department of Translational Oncology Genentech Inc, South San Francisco, California, USA
3. Department of Biomedical Imaging Group, Genentech Inc, South San Francisco, California, USA
4. Department of Internal Medicine, UC Davis Cancer Center, University of California, Davis, California, USA
5. Antibody Discovery and Protein Engineering Department, MedImmune Inc, Gaithersburg, Maryland, USA
Abstract:

Background

Conditional expression vectors have become a valuable research tool to avoid artefacts that may result from traditional gene expression studies. However, most systems require multiple plasmids that must be independently engineered into the target system, resulting in experimental delay and an increased potential for selection of a cell subpopulation that differs significantly from the parental line. We have therefore developed pHUSH, an inducible expression system that allows regulated expression of shRNA, miRNA or cDNA cassettes on a single viral vector.

Results

Both Pol II and Pol III promoters have been successfully combined with a second expression cassette containing a codon-optimized tetracycline repressor and selectable marker. We provide examples of how pHUSH has been successfully employed to study the function of target genes in a number of cell types within in vitro and in vivo assays, including conditional gene knockdown in a murine model of brain cancer.

Conclusion

We have successfully developed and employed a single vector system that enables Doxycycline regulated RNAi or transgene expression in a variety of in vitro and in vivo model systems. These studies demonstrate the broad application potential of pHUSH for conditional genetic engineering in mammalian cells.
Keywords:
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