I'm going to edit a disease-causing mutation using CRISPR/cas9-base gene editing strategy for my PHD thesis. I'm going to replace 1608 bp of genome with nearly 3700 bp of donor template. Each of homologous arms is 1000 bp, Do you have similar experience? Is replasment of this large fragment possible using CRISPR/cas9 gene editing strategy, I would be wondering if you could direct me
Amr Salem
Hi, Lotfi
The answer for your question is yes, its possible to insert even larger fragments, to start correctly you should make sure that your sgRNAs are highly efficient, specific, to the directed locus, I suggest to test them firstly in cell lines using T7E1 before proceeding to IVT and zygote micro-injection.
Best of Luck with your project
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