Molecular cloning using in vivo DNA assembly
Resumen: Here we describe the in vivo DNA assembly approach, where molecular cloning procedures are performed using an E. coli recA-independent recombination pathway, which assembles linear fragments of DNA with short homologous termini. This pathway is present in all standard laboratory E. coli strains and, by bypassing the need for in vitro DNA assembly, allows simplified molecular cloning to be performed without the plasmid instability issues associated with specialized recombination-cloning bacterial strains. The methodology requires specific primer design and can perform all standard plasmid modifications (insertions, deletions, mutagenesis, and sub-cloning) in a rapid, simple, and cost-efficient manner, as it does not require commercial kits or specialized bacterial strains. Additionally, this approach can be used to perform complex procedures such as multiple modifications to a plasmid, as up to 6 linear fragments can be assembled in vivo by this recombination pathway. Procedures generally require less than 3 h, involving PCR amplification, DpnI digestion of template DNA, and transformation, upon which circular plasmids are assembled. In this chapter we describe the requirements, procedure, and potential pitfalls when using this technique, as well as protocol variations to overcome the most common issues.
Idioma: Inglés
DOI: 10.1007/978-1-0716-3004-4_3
Año: 2023
Publicado en: Methods in Molecular Biology 2633 (2023), 33-44
ISSN: 1064-3745

Factor impacto CITESCORE: 2.0 - Genetics (Q4) - Molecular Biology (Q4)

Factor impacto SCIMAGO: 0.399 - Genetics (Q3) - Molecular Biology (Q4)

Tipo y forma: Artículo (PostPrint)
Área (Departamento): Área Bioquímica y Biolog.Mole. (Dpto. Bioq.Biolog.Mol. Celular)

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Artículos > Artículos por área > Bioquímica y Biología Molecular



 Registro creado el 2023-05-04, última modificación el 2024-07-31


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