![Gene and protein expression changes upon menin-MLL inhibition in NPM1mut and MLL-r AML. (A) Human (left) and murine (right) AML cells were treated for 11 days with MI-503. Viable (4′,6-diamidino-2-phenylindole [DAPI]–negative) cells were assessed by flow cytometry, and IC50 values were calculated with GraphPad Prism software. (B) Summary of IC50 values (MI-503), MLL-rearrangement, and NPM1 and FLT3 mutation status in the AML cells assessed. (C) Venn diagram showing downregulated genes identified by RNA-seq (more than twofold decrease; adjusted P < .05), in NPM1mut OCI-AML3, MLL-r MOLM13, and MV411 cells after MI-503 treatment (2.5 µM) compared with the DMSO control. (D) Volcano plots of RNA-seq data obtained from OCI-AML3, MOLM13, and MV411 cells treated with MI-503 (2.5 µM). FLT3 and selected MLL-fusion targets are labeled. (E) FLT3 and MEIS1 mRNA expression in human and murine leukemia cells after 4 days of MI-503 treatment (2.5 µM), as assessed by qRT-PCR. ChIP was performed with antibodies against menin (F) or MLL1 (G) and IgG as the negative control, followed by qPCR to detect a sequence within the MEIS1 gene body or SOX2 as negative control. Cells were treated with MI-503 (2.5 µM) or vehicle control for 4 days. (H) FLT3 protein (cell surface) expression assessed by flow cytometry in human and murine NPM1mut and MLL-rearranged AML cells after MI-503 treatment (2.5 µM for 4 or 7 days, as indicated). Representative histograms of 3 independent experiments are shown. Bar graphs in panels A and E-G represent the mean of 3 independent experiments, each performed in technical triplicate. Bar graph in panel H showing Npm1CA/+Flt3ITD/+ cells represents 2 independent experiments performed in technical triplicate. Error bars represent standard deviation.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/136/21/10.1182_blood.2020005037/1/bloodbld2020005037f1.png?Expires=1719009503&Signature=T6u4x6yVJ7Y9nLUCaOJKEA~W1rXW3x7mqD8IP50pQWGl6uatFmjS2OfM~9404LwOhRsytKg2XxcrQqO6zPcZkp3rroJuRgGTvvD83uY2Dc2QQxTvi4IL9y9O-fa3K7srCY16NJ3fJWXTI0BuBYmB5-AhaVCH~nsyMn7hp3MGQ3oVmNps-JjvefVD8duh~XyLGlbG9jQJaGYmFe3c4EGChmbB2bAXjYDMaLskuSaKUUczJTnMasNa9tzZB7LLJGD~lFqXTMNSlxwcb1wQax6glJOJ-0EGOep2-QRPv37fp6yzx3kVJPLxeyjNdrKfAHnwJKx2q8ZZfZzszrQe4hpXrQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Gene and protein expression changes upon menin-MLL inhibition in NPM1mut and MLL-r AML. (A) Human (left) and murine (right) AML cells were treated for 11 days with MI-503. Viable (4′,6-diamidino-2-phenylindole [DAPI]–negative) cells were assessed by flow cytometry, and IC50 values were calculated with GraphPad Prism software. (B) Summary of IC50 values (MI-503), MLL-rearrangement, and NPM1 and FLT3 mutation status in the AML cells assessed. (C) Venn diagram showing downregulated genes identified by RNA-seq (more than twofold decrease; adjusted P < .05), in NPM1mut OCI-AML3, MLL-r MOLM13, and MV411 cells after MI-503 treatment (2.5 µM) compared with the DMSO control. (D) Volcano plots of RNA-seq data obtained from OCI-AML3, MOLM13, and MV411 cells treated with MI-503 (2.5 µM). FLT3 and selected MLL-fusion targets are labeled. (E) FLT3 and MEIS1 mRNA expression in human and murine leukemia cells after 4 days of MI-503 treatment (2.5 µM), as assessed by qRT-PCR. ChIP was performed with antibodies against menin (F) or MLL1 (G) and IgG as the negative control, followed by qPCR to detect a sequence within the MEIS1 gene body or SOX2 as negative control. Cells were treated with MI-503 (2.5 µM) or vehicle control for 4 days. (H) FLT3 protein (cell surface) expression assessed by flow cytometry in human and murine NPM1mut and MLL-rearranged AML cells after MI-503 treatment (2.5 µM for 4 or 7 days, as indicated). Representative histograms of 3 independent experiments are shown. Bar graphs in panels A and E-G represent the mean of 3 independent experiments, each performed in technical triplicate. Bar graph in panel H showing Npm1CA/+Flt3ITD/+ cells represents 2 independent experiments performed in technical triplicate. Error bars represent standard deviation.