Golden Gate assembly of BioBrick-compliant parts using Type II restriction endonucleases

Author:

Matsumura Ichiro12ORCID

Affiliation:

1. Department of Biochemistry, Emory University School of Medicine, Department of Biochemistry, O. Wayne Rollins Research Center, 1510 Clifton Road NE, Room 4001, Atlanta, GA 30322, USA

2. Bond Pet Foods, 3200 Carbon Place, #104, Boulder, CO 80301, USA

Abstract

Aims: New methods of DNA recombination that capture the principal advantages of the BioBrick standard (ease of design) and Golden Gate assembly (decreased labor) are demonstrated here. Methods & materials: Both methods employ DNA methyltransferase expression vectors, available from Addgene, that protect selected sites on different plasmids from particular Type II restriction endonucleases. No other reagents are required. Results: The 4R/2M discontinuous DNA assembly is more efficient (produces more desired recombinant plasmids) and as specific (produces few undesired recombination products) as conventional subcloning. The 5RM continuous DNA assembly is approximately as efficient and specific as conventional Golden Gate assembly, even though in vivo methylation of one plasmid is incomplete. Conclusion: Both methylase-assisted methods streamline BioBrick assembly workflows without complicating the design of synthetic parts.

Publisher

Future Science Ltd

Subject

General Biochemistry, Genetics and Molecular Biology,Biotechnology

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