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- Engineering Phages for Eukaryotic Payload Expression in Cancer Associated Fusobacterium Nucleatum
To address these challenges, a de novo molecular system was established. Initially, a shuttle vector was generated using a native FN plasmid. Two promoters that drive strong bacterial gene expression in FN were identified using both bioinformatic tools and mass spectrometry and their activity was validated using a luciferase-based detection tag.
Payload protein expression was further improved using various algorithms for exposing the ribosome binding site and optimizing codon usage and ribosome elongation speed. After determining the optimal conditions for payload expression via a plasmid, a FN phage was engineered to carry the payload within its genome. Following phage infection, payload expression by the bacterial host was observed.