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Highly efficient baculovirus-mediated multigene delivery in primary cells

Mansouri, M. and Bellon-Echeverria, I. and Rizk, A. and Ehsaei, Z. and Cianciolo Cosentino, C. and Silva, C. S. and Xie, Y. and Boyce, F. M. and Davis, M. W. and Neuhauss, S. C. and Taylor, V. and Ballmer-Hofer, K. and Berger, I. and Berger, P.. (2016) Highly efficient baculovirus-mediated multigene delivery in primary cells. Nature Communications, 7. p. 11529.

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Official URL: https://edoc.unibas.ch/62481/

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Abstract

Multigene delivery and subsequent cellular expression is emerging as a key technology required in diverse research fields including, synthetic and structural biology, cellular reprogramming and functional pharmaceutical screening. Current viral delivery systems such as retro- and adenoviruses suffer from limited DNA cargo capacity, thus impeding unrestricted multigene expression. We developed MultiPrime, a modular, non-cytotoxic, non-integrating, baculovirus-based vector system expediting highly efficient transient multigene expression from a variety of promoters. MultiPrime viruses efficiently transduce a wide range of cell types, including non-dividing primary neurons and induced-pluripotent stem cells (iPS). We show that MultiPrime can be used for reprogramming, and for genome editing and engineering by CRISPR/Cas9. Moreover, we implemented dual-host-specific cassettes enabling multiprotein expression in insect and mammalian cells using a single reagent. Our experiments establish MultiPrime as a powerful and highly efficient tool, to deliver multiple genes for a wide range of applications in primary and established mammalian cells.
Faculties and Departments:03 Faculty of Medicine > Departement Biomedizin > Division of Anatomy > Embryology and Stem Cell Biology (Taylor)
UniBasel Contributors:Taylor, Verdon
Item Type:Article, refereed
Article Subtype:Research Article
Publisher:Nature Publishing Group
e-ISSN:2041-1723
Note:Publication type according to Uni Basel Research Database: Journal article
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Last Modified:11 Dec 2018 17:26
Deposited On:11 Dec 2018 17:26

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