Abstract
The rise in the frequency of antibiotic resistance has made bacterial infections, specifically Pseudomonas aeruginosa, a cause for greater concern. Phage therapy is a promising solution that uses naturally isolated phages to treat bacterial infections. Ecological limitations, which stipulate a discrete host range and the inevitable evolution of resistance, may be overcome through a better understanding of phage biology and the utilization of engineered phages. In this study, we developed a synthetic biology approach to construct tailed phages that naturally target clinically relevant strains of Pseudomonas aeruginosa. As proof of concept, we successfully cloned and assembled the JG024 and DMS3 phage genomes in yeast using transformation-associated recombination cloning and rebooted these two phage genomes in two different strains of P. aeruginosa. We identified factors that affected phage reboot efficiency like the phage species or the presence of antiviral defense systems in the bacterial strain. We have successfully extended this method to two other phage species and observed that the method enables the reboot of phages that are naturally unable to infect the strain used for reboot. This research represents a critical step toward the construction of clinically relevant, engineered P. aeruginosa phages. IMPORTANCE Pseudomonas aeruginosa is a bacterium responsible for severe infections and a common major complication in cystic fibrosis. The use of antibiotics to treat bacterial infections has become increasingly difficult as antibiotic resistance has become more prevalent. Phage therapy is an alternative solution that is already being used in some European countries, but its use is limited by the narrow host range due to the phage receptor specificity, the presence of antiviral defense systems in the bacterial strain, and the possible emergence of phage resistance. In this study, we demonstrate the use of a synthetic biology approach to construct and reboot clinically relevant P. aeruginosa tailed phages. This method enables a significant expansion of possibilities through the construction of engineered phages for therapy applications.
| Original language | English (US) |
|---|---|
| Journal | Microbiology Spectrum |
| Volume | 12 |
| Issue number | 3 |
| DOIs | |
| State | Published - Mar 2024 |
Funding
This work was funded in part by the Northwestern University McCormick School of Engineering Research Catalyst Program, the Walder Foundation (Innovation Top-Up Award; Hartmann AGMT 12/16/21), the National Science Foundation Graduate Research Fellowship (Grant number: DGE-2234667), the National Science Foundation Research Trainee Program Understandng the Rules of Life Synthetic Biology Across Scales (Grant number: 2021900) and the National Institutes of Health’s National Center for Advancing Translational Sciences (Grant number: TL1TR001423). The content is solely the responsibility of the authors and does not necessarily represent the views of the National Institutes of Health or any other funding agency. National Science Foundation (NSF) National Science Foundation (NSF) NRT-URoL SynBAS
Keywords
- Pseudomonas aeruginosa
- phage reboot
- phage therapy
- synthetic biology
ASJC Scopus subject areas
- Physiology
- Ecology
- General Immunology and Microbiology
- Genetics
- Microbiology (medical)
- Cell Biology
- Infectious Diseases
