Genomic insertion of lentiviral DNA circles directed by the yeast Flp recombinase

Moldt, B., Staunstrup, N. H., Jakobsen, M., Yáñez-Muñoz, R. J. and Mikkelsen, J. G.

(2008)

Moldt, B., Staunstrup, N. H., Jakobsen, M., Yáñez-Muñoz, R. J. and Mikkelsen, J. G. (2008) Genomic insertion of lentiviral DNA circles directed by the yeast Flp recombinase. BMC Biotechnology, 8

Our Full Text Deposits

Full text access: Open

Full text file - 985.79 KB

Links to Copies of this Item Held Elsewhere

Link to publisher copy

Abstract

BACKGROUND: Circular forms of viral genomic DNA are generated during infection of cells with retroviruses like HIV-1. Such circles are unable to replicate and are eventually lost as a result of cell division, lending support to the prevalent notion that episomal retroviral DNA forms are dead-end products of reverse transcription. RESULTS: We demonstrate that circular DNA generated during transduction with HIV-1-based lentiviral vectors can be utilized as substrate for gene insertion directed by nonviral recombinases co-expressed in the target cells. By packaging of lentiviral genomic RNA in integrase-defective lentiviral vectors, harboring an inactive form of the viral integrase, the normal pathway for viral integration is blocked and circular vector DNA accumulates in transduced cells as a result. We find that the amount of DNA circles is increased 4-fold in cells transduced with integration-defective vectors relative to cells treated with integrase-proficient vectors. By transduction of target cells harboring engineered recognition sites for the yeast Flp recombinase with integration-defective lentiviral vectors containing an ATG-deficient hygromycin B selection gene we demonstrate precise integration of lentiviral vector-derived DNA circles in a drug-selective approach. Moreover, it is demonstrated that trans-acting Flp recombinase can be delivered by Flp-encoding transfected plasmid DNA or, alternatively, by co-transduced integrase-defective lentiviral vectors carrying a Flp expression cassette. CONCLUSION: Our data provide proof-of-principle that nonviral recombinases, like Flp, produced by plasmid DNA or non-integrating lentiviral vectors can gain access to circular viral recombination substrates and facilitate site-directed genomic insertion of such episomal DNA forms. Replacement of the normal viral integration machinery with nonviral mediators of integration represents a new platform for creation of lentiviral vectors with an altered integration profile.

Information about this Version

This is a Submitted version
This version's date is: 2008
This item is not peer reviewed

Link to this Version

https://repository.royalholloway.ac.uk/items/c45abbd7-e6a7-807b-7552-ce6a39a65bd5/6/

Item TypeJournal Article
TitleGenomic insertion of lentiviral DNA circles directed by the yeast Flp recombinase
AuthorsMoldt, B.
Staunstrup, N. H.
Jakobsen, M.
Yáñez-Muñoz, R. J.
Mikkelsen, J. G.
Uncontrolled KeywordsDNA Nucleotidyltransferases/*metabolism DNA, Circular/*genetics Fungal Proteins/metabolism Genetic Vectors/*genetics Genome, Viral/*genetics Lentivirus/*genetics Mutagenesis, Insertional/*methods Transfection/*methods
DepartmentsFaculty of Science\Biological Science

Identifiers
doihttp://dx.doi.org/10.1186/1472-6750-8-60

Deposited by Research Information System (atira) on 22-Jul-2014 in Royal Holloway Research Online.Last modified on 22-Jul-2014

Notes

Moldt, Brian Staunstrup, Nicklas H Jakobsen, Maria Yáñez-Muñoz, Rafael J Mikkelsen, Jacob G Research Support, Non-U.S. Gov't England BMC biotechnology BMC Biotechnol. 2008 Aug 9;8:60.

Details