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Nucleic Acids Research Advance Access published online on October 2, 2008

Nucleic Acids Research, doi:10.1093/nar/gkn646
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© 2008 The Author(s)
This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/2.0/uk/) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.


Methods online

Rapid and reliable universal cloning of influenza A virus genes by target-primed plasmid amplification

Jürgen Stech1,*, Olga Stech1, Astrid Herwig2, Hermann Altmeppen2, Jana Hundt1, Sandra Gohrbandt1, Anne Kreibich1, Siegfried Weber1, Hans-Dieter Klenk2 and Thomas C. Mettenleiter1

1Friedrich-Loeffler-Institute, Federal Research Institute for Animal Health, Südufer 10, 17493 Greifswald - Insel Riems and 2Institute for Virology, Philipps-University Marburg, Hans-Meerwein-Straße 2, 35043 Marburg, Germany

*To whom correspondence should be addressed. Tel: +49 383517237; Fax: +49 383517275; Email: juergen.stech{at}fli.bund.de

Received August 18, 2008. Accepted September 16, 2008.

Reverse genetics has become pivotal in influenza virus research relying on rapid generation of tailored recombinant influenza viruses. They are rescued from transfected plasmids encoding the eight influenza virus gene segments, which have been cloned using restriction endonucleases and DNA ligation. However, suitable restriction cleavage sites often are not available. Here, we describe a cloning method universal for any influenza A virus strain which is independent of restriction sites. It is based on target-primed plasmid amplification in which the insert provides two megaprimers and contains termini homologous to plasmid regions adjacent to the insertion site. For improved efficiency, a cloning vector was designed containing the negative selection marker ccdB flanked by the highly conserved influenza A virus gene termini. Using this method, we generated complete sets of functional gene segments from seven influenza A strains and three haemagglutinin genes from different serotypes amounting to 59 cloned influenza genes. These results demonstrate that this approach allows rapid and reliable cloning of any segment from any influenza A strain without any information about restriction sites. In case the PCR amplicon ends are homologous to the plasmid annealing sites only, this method is suitable for cloning of any insert with conserved termini.


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