4.7 Article

Directed Evolution of Replication-Competent Double-Stranded DNA Bacteriophage toward New Host Specificity

Journal

ACS SYNTHETIC BIOLOGY
Volume 11, Issue 2, Pages 634-643

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/acssynbio.1c00319

Keywords

phage engineering; directed evolution; phage specificity; synthetic phage platform; tail fiber engineering

Funding

  1. HBMS IAF-PP grant [H17/01/a0/0V9]
  2. A*STAR Visiting Investigator Prog r a m [1535j00137]

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Bacteriophages are a promising alternative to antibiotics in combating antimicrobial resistance. This study presents a strategy for generating large libraries of phage variants, allowing for engineering of phage specificity and improved qualities. The findings demonstrate the potential of directed evolution in enhancing phage therapy for therapeutic applications.
In the fight against antimicrobial resistance, bacteriophages are a promising alternative to antibiotics. However, due to their narrow spectra, phage therapy requires the careful matching between the host and bacteriophage to be effective. Despite our best efforts, nature remains as the only source of novel phage specificity. Directed evolution can potentially open an avenue for engineering phage specificity and improving qualities of phages that are not strongly selected for in their natural environments but are important for therapeutic applications. In this work, we present a strategy that generates large libraries of replication-competent phage variants directly from synthetic DNA fragments, with no restriction on their host specificity. Using the T7 bacteriophage as a proof-of-concept, we created a large library of tail fiber mutants with at least 10(7) unique variants. From this library, we identified mutants that have broadened specificity as evidenced by their novel lytic activity against Yersinia enterocolitica, a strain that the wild-type T7 was unable to lyse. Using the same concept, mutants with improved lytic efficiency and characteristics, such as lytic condition tolerance and resistance suppression, were also identified. However, the observed limitations in altering host specificity by tail fiber mutagenesis suggest that other bottlenecks could be of equal or even greater importance.

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