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− | <strong>Figure 1: Toxin repression in <em>C. difficile</em> using antisense RNA.</strong> (starting with the image on the bottom left and going clockwise) Once the therapy is administered and in the gut, the genetically modified bacteriophage binds to a toxin-producing <em>C. difficile</em> cell and injects its genetic material (our antisense RNA constructs) into the cell. The phage genome is subsequently integrated into the host (<em>C. difficile</em>) chromosome. Later, the constructs are transcribed along with the host genome, resulting in the expression of antisense RNA. The antisense RNA binds the toxin mRNA hence preventing | + | <strong>Figure 1: Toxin repression in <em>C. difficile</em> using antisense RNA.</strong> (starting with the image on the bottom left and going clockwise) Once the therapy is administered and in the gut, the genetically modified bacteriophage binds to a toxin-producing <em>C. difficile</em> cell and injects its genetic material (our antisense RNA constructs) into the cell. The phage genome is subsequently integrated into the host (<em>C. difficile</em>) chromosome. Later, the constructs are transcribed along with the host genome, resulting in the expression of antisense RNA. The antisense RNA binds the toxin mRNA hence preventing translation of the toxin mRNA to the protein. The RNA-RNA duplex is degraded in the cell. As a result, the <em>C. difficile</em> cell is no longer producing toxins, converting to into a non-toxigenic cell.</h6> |
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Revision as of 19:13, 17 October 2018