TY - JOUR
T1 - The small inhibitor WM-1119 effectively targets KAT6A-rearranged AML, but not KMT2A-rearranged AML, despite shared KAT6 genetic dependency
AU - Sheridan, Mathew
AU - Maqbool, Muhammad Ahmad
AU - Largeot, Anne
AU - Clayfield, Liam
AU - Xu, Jingru
AU - Moncaut, Natalia
AU - Sellers, Robert
AU - Whittle, Jessica
AU - Paggetti, Jerome
AU - Iqbal, Mudassar
AU - Aucagne, Romain
AU - Delva, Laurent
AU - Baker, Syed Murtuza
AU - Lie-a-Ling, Michael
AU - Kouskoff, Valerie
AU - Lacaud, Georges
N1 - Funding:
The study was supported by Cancer Research UK (C5759/A20971 (G.L.),
C5759/A27412 (G.L.), C19941/A31313 (M.S), Blood Cancer UK 19014 (G.L.),
and an MSCA Postdoctoral Fellowship (658625, A.L.). Research in the Kouskoff
laboratory is supported by the Medical Research Council (MR/P000673/1; MR/
T000384/1) and the Biotechnology and Biological Sciences Research Council
(BB/R007209/1). Work in the A.L. laboratory is supported by grants from the
Luxembourg National Research Fund (FNR) and Fondation Cancer (C20/
BM/14582635, C20/BM/14592342, and C23/BM/17987391).
Publisher Copyright:
© The Author(s) 2024.
© 2024. The Author(s).
PY - 2024/10/8
Y1 - 2024/10/8
N2 - Background: The epigenetic factors KAT6A (MOZ/MYST3) and KMT2A (MLL/MLL1) interact in normal hematopoiesis to regulate progenitors’ self-renewal. Both proteins are recurrently translocated in AML, leading to impairment of critical differentiation pathways in these malignant cells. We evaluated the potential of different KAT6A therapeutic targeting strategies to alter the growth of KAT6A and KMT2A rearranged AMLs. Methods: We investigated the action and potential mechanisms of the first-in-class KAT6A inhibitor, WM-1119 in KAT6A and KMT2A rearranged (KAT6Ar and KMT2Ar) AML using cellular (flow cytometry, colony assays, cell growth) and molecular (shRNA knock-down, CRISPR knock-out, bulk and single-cell RNA-seq, ChIP-seq) assays. We also used two novel genetic murine KAT6A models combined with the most common KMT2Ar AML, KMT2A::MLLT3 AML. In these murine models, the catalytic activity of KAT6A, or the whole protein, can be conditionally abrogated or deleted. These models allowed us to compare the effects of specific KAT6A KAT activity inhibition with the complete deletion of the whole protein. Finally, we also tested these therapeutic approaches on human AML cell lines and primary patient AMLs. Results: We found that WM-1119 completely abrogated the proliferative and clonogenic potential of KAT6Ar cells in vitro. WM-1119 treatment was associated with a dramatic increase in myeloid differentiation program. The treatment also decreased stemness and leukemia pathways at the transcriptome level and led to loss of binding of the fusion protein at critical regulators of these pathways. In contrast, our pharmacologic and genetic results indicate that the catalytic activity of KAT6A plays a more limited role in KMT2Ar leukemogenicity, while targeting the whole KAT6A protein dramatically affects leukemic potential in murine KMT2A::MLLT3 AML. Conclusion: Our study indicates that inhibiting KAT6A KAT activity holds compelling promise for KAT6Ar AML patients. In contrast, targeted degradation of KAT6A, and not just its catalytic activity, may represent a more appropriate therapeutic approach for KMT2Ar AMLs.
AB - Background: The epigenetic factors KAT6A (MOZ/MYST3) and KMT2A (MLL/MLL1) interact in normal hematopoiesis to regulate progenitors’ self-renewal. Both proteins are recurrently translocated in AML, leading to impairment of critical differentiation pathways in these malignant cells. We evaluated the potential of different KAT6A therapeutic targeting strategies to alter the growth of KAT6A and KMT2A rearranged AMLs. Methods: We investigated the action and potential mechanisms of the first-in-class KAT6A inhibitor, WM-1119 in KAT6A and KMT2A rearranged (KAT6Ar and KMT2Ar) AML using cellular (flow cytometry, colony assays, cell growth) and molecular (shRNA knock-down, CRISPR knock-out, bulk and single-cell RNA-seq, ChIP-seq) assays. We also used two novel genetic murine KAT6A models combined with the most common KMT2Ar AML, KMT2A::MLLT3 AML. In these murine models, the catalytic activity of KAT6A, or the whole protein, can be conditionally abrogated or deleted. These models allowed us to compare the effects of specific KAT6A KAT activity inhibition with the complete deletion of the whole protein. Finally, we also tested these therapeutic approaches on human AML cell lines and primary patient AMLs. Results: We found that WM-1119 completely abrogated the proliferative and clonogenic potential of KAT6Ar cells in vitro. WM-1119 treatment was associated with a dramatic increase in myeloid differentiation program. The treatment also decreased stemness and leukemia pathways at the transcriptome level and led to loss of binding of the fusion protein at critical regulators of these pathways. In contrast, our pharmacologic and genetic results indicate that the catalytic activity of KAT6A plays a more limited role in KMT2Ar leukemogenicity, while targeting the whole KAT6A protein dramatically affects leukemic potential in murine KMT2A::MLLT3 AML. Conclusion: Our study indicates that inhibiting KAT6A KAT activity holds compelling promise for KAT6Ar AML patients. In contrast, targeted degradation of KAT6A, and not just its catalytic activity, may represent a more appropriate therapeutic approach for KMT2Ar AMLs.
KW - Leukemia, Myeloid, Acute/genetics
KW - Animals
KW - Myeloid-Lymphoid Leukemia Protein/genetics
KW - Humans
KW - Mice
KW - Histone-Lysine N-Methyltransferase/genetics
KW - Histone Acetyltransferases/genetics
KW - Gene Rearrangement
KW - Cell Line, Tumor
UR - http://www.scopus.com/inward/record.url?scp=85206068162&partnerID=8YFLogxK
UR - https://pubmed.ncbi.nlm.nih.gov/39380002/
U2 - 10.1186/s13045-024-01610-0
DO - 10.1186/s13045-024-01610-0
M3 - Article
C2 - 39380002
AN - SCOPUS:85206068162
SN - 1756-8722
VL - 17
SP - 91
JO - Journal of Hematology and Oncology
JF - Journal of Hematology and Oncology
IS - 1
M1 - 91
ER -