Novel Cloning Method for Recombinant Adenovirus Construction in Escherichia coli | Zendy

David W. Souza | Zendy; Donna Armentano | Zendy

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Novel Cloning Method for Recombinant Adenovirus Construction in Escherichia coli

Author(s) -

David W. Souza,

Donna Armentano

Publication year - 1999

Publication title -

biotechniques

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.617

H-Index - 131

eISSN - 1940-9818

pISSN - 0736-6205

DOI - 10.2144/99263rr01

Subject(s) - recombinant dna , plasmid , cloning (programming) , restriction enzyme , biology , multiple cloning site , escherichia coli , molecular cloning , intron , microbiology and biotechnology , virology , genetics , computational biology , dna , gene , peptide sequence , vector (molecular biology) , computer science , programming language

pAd(vantage) is a rapid cloning system for generating recombinant adenoviruses. The system is based on manipulating the full-length adenovirus genome as a stable plasmid in E. coli using intron-encoded endonucleases. These intron-encoded endonucleases cut their recognition sequences, which range from 15-39 bp, with high specificity. Their unusual long homing sequence makes them rare-cutting and ideal for use as cloning sites. We report how transgenes can easily be cloned directly into the E1 region of an adenoviral plasmid, followed by transfection into a mammalian packaging cell line, to produce homogeneous recombinant viruses without the need for plaque purification.

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