Abstract Lymphoid B-ALL and TCLL leukemia consists of leukemic blast cells (LBCs) arrested at early stages of differentiation which exhibit high proliferative potential and capability for self-renewal. The idea to induce reprogramming of leukemic and other cancer cells, leading to cell maturation and senescence, gained high popularity, but its clinical applications are rarely successful and are mainly limited to the therapy of the APL leukemia with ATRA and arsenic trioxide. This strategy may have been unsuccessful due to a gap in the knowledge of the mechanisms through which transcriptional reprogramming occurs. Our published data suggest that normal hematopoietic progenitor cells (HPCs) undergo transient de-condensation of chromatin to allow lineage-specific transcription factors (TFs) to bind to their gene targets and to activate new transcriptional programs, leading to cell differentiation. This transient de-condensation occurs through very low accumulation of H3K27me3, on DNA just after DNA replication. H3K27me3 is a mark of the most condensed arrays of nucleosomes in the genome and is found at regulatory regions of all repressed genes. Our results suggest that tested cultured and primary lymphoid B-ALL and TCLL cells have lost this inherent ability to ‘open’ nascent chromatin, thus creating a barrier for their transcriptional reprogramming. In this proposal, we will test a new reprogramming strategy, which overcomes these barriers of reprogramming-based therapies and may lead to elimination of leukemic cells. The key feature of this new strategy is the first step, which includes pharmacological inhibition of the H3K27me3 histone methyltransferases (HMTs) EZH1/EZH2, thus creating de- condensed structure of nascent chromatin at regulatory regions of all genes. At the second step, we will use small molecules to activate endogenous inducible TFs, which can then readily bind to their target genes due to the de-condensed structure of nascent chromatin. Tumor cells, including leukemic cells, are commonly known to accumulate mutations in inducible TFs and receptors; thus, screens of small molecule inducers for a variety of TFs/receptors will be performed to determine the best possible inducer for distinct subtypes of B-ALL. Preliminary results suggest that induction by small molecule inducers leads to transcriptional reprogramming of cell lines and primary B-ALL and TCLL cells, changes in their immunophenotype and apoptosis. Moreover, this strategy strongly suppresses lymphoid leukemia burden in mice. The goal of this project is to develop a widely applicable treatment strategy for transcriptional reprogramming and loss of cell viability for many types of lymphoid leukemic cells. To this end, we propose to: 1. Extend and generalize the lymphoid leukemic cells reprogramming approach; 2. Examine the mechanisms and biological outcomes of reprogramming of lymphoid leukemic cells; 3. Examine the effects of our treatment strategy in vivo.