Efficient directional cloning of recombinant adenovirus vectors using DNA-protein complex

Artigo Acesso aberto Revisado por pares

Efficient directional cloning of recombinant adenovirus vectors using DNA-protein complex

1998; Oxford University Press; Volume: 26; Issue: 8 Linguagem: Inglês

10.1093/nar/26.8.1947

ISSN

1362-4962

Autores

Takashi Okada,

Tópico(s)

CAR-T cell therapy research

Resumo

We describe an efficient cloning system utilizing adenoviral DNA-protein complexes which allows the directional cloning of genes into adenoviral expression vectors in a single step. DNA-protein complexes derived from a recombinant adenovirus (AVC2.null) were isolated by sequential use of CsCl step gradients followed by isopycnic centrifugation in a mixture of CsCl and guanidine HCl. AVC2.null is an adenoviral expression vector containing unique restriction sites between the human CMV-IE promoter and the SV40 intron/polyadenylation site. Transgenes were prepared for cloning into this vector by introduction of compatible restriction sites by PCR. A vector expressing rat granulocyte-macrophage colony-stimulating factor (GM-CSF) was constructed using DNA-protein complex as well as by traditional recombination techniques. The efficacy of our adenoviral cloning system utilizing DNA-protein complex was two logs higher than that seen using homologous recombination. All viruses generated by directional ligation of the insert into the vector DNA-protein complexes contained the desired transgene in the correct orientation. This technique greatly simplifies and accelerates the generation of recombinant adenoviral vectors.

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Efficient directional cloning of recombinant adenovirus vectors using DNA-protein complex