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In Vivo Kinetics of Early, Non-random Methylome and Transcriptome Changes Induced by DNA-hypomethylating Treatment in Primary AML Blasts

by Andreas Neubauer , Andrieux Geoffroy , Björn Hackanson , Dietmar Pfeifer , Gabriele Greve , Gerhard Heil , Hartmut Döhner , Helmut R. Salih , Jürgen Krauter , Konstanze Döhner , Melanie Börries , Michael Heuser , Michael Lübbert , Nadja Blagitko-Dorfs , Pascal Schlosser , Tobias Ma , Usama-Ur Rehman

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Abstract: Despite routine use of DNA-hypomethylating agents (HMAs) in AML/MDS therapy, their mechanisms of action are not yet unraveled. Pleiotropic effects of HMAs include global methylome and transcriptome changes. We asked whether in blasts and T-cells from AML patients HMA-induced in vivo demethylation and remethylation occur randomly or non-randomly, and whether gene demethylation is associated with gene induction. Peripheral blood AML blasts from patients receiving decitabine (20 mg/m2 day 1-5) were serially isolated for methylome analyses (days 0, 8 and 15, n = 28) and methylome-plus-transcriptome analyses (days 0 and 8, n = 23), respectively. T-cells were isolated for methylome analyses (days 0 and 8; n = 16). We noted massive, non-random demethylation at day 8, which was variable between patients. In contrast, T-cells disclosed a thousand-fold lesser, random demethylation, indicating selectivity of the demethylation for the malignant blasts. The integrative analysis of DNA demethylation and transcript induction revealed 87 genes displaying a significant inverse correlation, e.g. the tumor suppressor gene IFI27, whose derepression was validated in two AML cell lines. These results support HMA-induced, non-random early in vivo demethylation events in AML blasts associated with gene induction. Larger patient cohorts are needed to determine whether a demethylation signature may be predictive for response to this treatment

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