Expression profiling of p53-/- shPU.1 AML cells single cell clones

We have utilized advanced RNAi technology to dynamically restore endogenous PU.1 expression in p53-deficient shPU.1 AML single cell clones in vitro. This causes rapid cell cycle shutdown and reversible myeloid differentiation. Overall design: RNA-seq was performed in biological triplicate single cell clones that were either untreated, treated with Dox for 14 days or treated with Dox for 14 days washed and left untreated