Part:BBa_K2429007:Experience
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Applications of BBa_K2429007
In our experiment, we tested five plain guides, Guide1 through Guide5.The guides were co-transfected with dCas13a, which uses the guide to locate the target intron and block the spliceosome from recognizing the splice site. (For a detailed explanation of how to plan a mammalian transfection click here)
Guide Tiling
Tre:mKate DOX Induction
Guides and Cas13a need to be produced by the cell before they are able to affect the splicing of mKate-ff4. In order to add a time delay between when they were being produced and when mKate was being produced, we put mKate downstream of a DOX inducible promoter. DOX was added to cells 24 hours after the initial transfection, allowing the cells to undergo a doubling before producing mKate. We want to compare the results of the Cas-affected output with a normal Tre:mKate-ff4 DOX induction. We expect that the Cas will cause a disruption in what would otherwise be a normal mKate induction curve. These expected results are compared side by side below. The different colored lines corrispond to different transfection bins
In our experiment, we used Guide3, and a well with just mKate for control. DOX was added to the system 24 hours after transfection. Each cell was transfected with optimized amounts of plasmid from previous experiments (For a detailed explanation of how to plan a mammalian transfection click here)
Guide 3 Tre:mKate-ff4 DOX Induction Plain Tre:mKate-ff4 DOX Induction
Unfortunately, there was no significant difference between the control titration and the Guide3 or Junk guide induction. However, even the control in this experiment was not showing clear results, so the experiment should be rerun before drawing conclusions about the system. All the guides will have to be tested in this way before determining whether or not this system is effective.
User Reviews
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