Simultaneous Insertion of Two Expression Cassettes into Adenovirus Vectors | Zendy

Xavier Danthinne | Zendy

AI Assistant Blog Pricing

Home ZAIA Blog

Open Access

Simultaneous Insertion of Two Expression Cassettes into Adenovirus Vectors

Author(s) -

Xavier Danthinne

Publication year - 2001

Publication title -

biotechniques

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.617

H-Index - 131

eISSN - 1940-9818

pISSN - 0736-6205

DOI - 10.2144/01303rr06

Subject(s) - insert (composites) , plasmid , cloning (programming) , restriction enzyme , biology , recombinant dna , genome , computational biology , transfection , transgene , cloning vector , expression cassette , virus , genetics , dna , microbiology and biotechnology , vector (molecular biology) , gene , computer science , mechanical engineering , engineering , programming language

We have designed AdenoQuick, a fast and versatile method to construct first-generation adenoviral vectors that contain one or two transgenes in the E1 and/or the E3 region. The method is based on the reconstitution of the entire genome of the desired recombinant virus in E. coli and the subsequent transfection of the DNA in a helper cell line. Since the construction of large adenoviral plasmids is generally difficult and therefore rebuffing for inexperienced researchers, we have optimized the cloning strategy by using bacterial positive-selection markers and a set of specific restriction enzymes that allow for directional cloning. The system is 99% efficient and allows one to insert simultaneously two expression cassettes into the E1 and E3 regions of the adenovirus genome.

The content you want is available to Zendy users.

Already have an account? Click here to sign in.

Having issues? You can contact us here

Accelerating Research