Engineering an Escherichia coli strain for production of long single-stranded DNA

Author:

Shen Konlin1,Flood Jake J2,Zhang Zhihuizi1,Ha Alvin345,Shy Brian R345,Dueber John E26,Douglas Shawn M1ORCID

Affiliation:

1. Department of Cellular and Molecular Pharmacology, University of California, San Francisco , San Francisco , CA , 94158 USA

2. Department of Bioengineering, University of California, Berkeley , Berkeley , CA , 94720 USA

3. Department of Laboratory Medicine, University of California, San Francisco , San Francisco , CA , 94143  USA

4. Gladstone-UCSF Institute of Genomic Immunology , San Francisco , CA , 94158  USA

5. Department of Medicine, University of California, San Francisco , San Francisco , CA , 94143  USA

6. Biological Systems & Engineering Division, Lawrence Berkeley National Laboratory , Berkeley , CA , 94720 USA

Abstract

Abstract Long single-stranded DNA (ssDNA) is a versatile molecular reagent with applications including RNA-guided genome engineering and DNA nanotechnology, yet its production is typically resource-intensive. We introduce a novel method utilizing an engineered Escherichia coli ‘helper’ strain and phagemid system that simplifies long ssDNA generation to a straightforward transformation and purification procedure. Our method obviates the need for helper plasmids and their associated contamination by integrating M13mp18 genes directly into the E. coli chromosome. We achieved ssDNA lengths ranging from 504 to 20 724 nt with titers up to 250 μg/l following alkaline lysis purification. The efficacy of our system was confirmed through its application in primary T-cell genome modifications and DNA origami folding. The reliability, scalability and ease of our approach promise to unlock new experimental applications requiring large quantities of long ssDNA.

Funder

National Science Foundation

National Institutes of Health

Publisher

Oxford University Press (OUP)

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