Abstract

While critical insights into the pathogenesis of acute myeloid leukemia (AML) have come from studying its cytogenetics and genetics, and from modeling myeloid malignancies in mice, these advances have not translated into therapeutic gains. Our goal is to develop targeted therapies for AML driven by AML1-ETO (AE), a chimeric transcription factor (TF) with oncogenic properties that is generated by the most common chromosomal translocation found in AML, t(8;21). We discovered that the leukemogenicity of AE in mouse and human AML models and its ability to activate gene expression required both the binding of the p300 lysine acetyltransferase to AE, and its acetylation at lysine 43 (K43). Given the inherent difficulties of directly targeting a TF, we have explored ways of targeting AE required co- factors, and over the past four years have defined the efficacy of multiple p300/CBP inhibitors in AE+ AML, targeted protein-protein interactions vital for AE-driven oncogenesis (including TAF1) and defined several AE target genes critical for its leukemogenicity (such as ID1). As we continue this work, our hypothesis is that by studying interacting proteins, cooperating mutations, and downstream biological events, we will more fully understand the cellular machinery that drives AE-expressing (AE+) AML and more efficiently devise combinatorial therapeutic strategies against AML. To test this hypothesis, we have proposed the following specific aims: 1. Determine how AE-interacting proteins regulate its transcriptional regulatory and leukemogenic properties. a) Determine how TAF1 regulates the ability of AE to bind chromatin, alter gene expression, and promote HSC self-renewal and leukemogenesis using ChIP-seq and RNA-seq assays. b) Determine how other components of the AE-TAF1 complex (such as TAF7) impact its biological properties, and its activity at gene enhancers and promoters. 2. Determine how the absence of p300/ CBP, and the presence of epigenetic modifier mutations seen in AE+ AML, affects the transcriptional regulatory and leukemogenic properties of AE. a) Define the response of AE+ AML cells to loss of p300 or CBP, compared to chemical inhibition of p300/CBP by knocking out p300 or CBP in AE-driven leukemia mouse models b) Determine how mutations in ASXL1, ASXL2, and TET2 cooperate with AE to drive leukemogenesis by generating compound mice models and c) Determine how these mutations affect the response of AE+ AML to p300/CBP inhibition by treating AE+ mouse cells derived from these compound mice. 3. Develop combination epigenetic and signal transduction therapies that are effective against AE+ AML. a) Evaluate the efficacy of combination, epigenetic-targeted therapies, including inhibitors of p300/CBP and inhibitors of TAF1, on AE-driven AML cells. b) Evaluate the efficacy of combination therapies that target both the signal transduction pathways (e.g. inhibiting ID1/AKT signaling) and the epigenetic factors (p300, TAF1) that drive AE+ AML.

Public Health Relevance

The AML1-ETO fusion transcription factor causes acute leukemia in humans, and we are studying the fundamental mechanisms that regulate its leukemia promoting ability. We are using biochemical approaches and mouse models to better understand the genesis of AML1-ETO driven leukemia and to devise new therapeutic strategies. By inhibiting its required co-factors, including the p300 and CBP enzymes, and impairing the protein-protein interactions vital for its function as an oncogene, we are developing more targeted approaches to this disease.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA166835-09
Application #
9982800
Study Section
Molecular Oncogenesis Study Section (MONC)
Program Officer
Klauzinska, Malgorzata
Project Start
2012-09-17
Project End
2022-07-31
Budget Start
2020-08-01
Budget End
2021-07-31
Support Year
9
Fiscal Year
2020
Total Cost
Indirect Cost

  Institution

Name
University of Miami School of Medicine
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
052780918
City
Coral Gables
State
FL
Country
United States
Zip Code
33146

  Publications

Luo, Huacheng; Wang, Fei; Zha, Jie et al. (2018) CTCF boundary remodels chromatin domain and drives aberrant HOX gene transcription in acute myeloid leukemia. Blood 132:837-848
Guo, Ying; Yang, Hui; Chen, Shi et al. (2018) Reduced BAP1 activity prevents ASXL1 truncation-driven myeloid malignancy in vivo. Leukemia 32:1834-1837
Yang, Hui; Kurtenbach, Stefan; Guo, Ying et al. (2018) Gain of function of ASXL1 truncating protein in the pathogenesis of myeloid malignancies. Blood 131:328-341
Hamard, Pierre-Jacques; Santiago, Gabriel E; Liu, Fan et al. (2018) PRMT5 Regulates DNA Repair by Controlling the Alternative Splicing of Histone-Modifying Enzymes. Cell Rep 24:2643-2657
Greenblatt, Sarah M; Man, Na; Hamard, Pierre-Jacques et al. (2018) CARM1 Is Essential for Myeloid Leukemogenesis but Dispensable for Normal Hematopoiesis. Cancer Cell 33:1111-1127.e5
Li, Zhaomin; Zhang, Peng; Yan, Aimin et al. (2017) ASXL1 interacts with the cohesin complex to maintain chromatid separation and gene expression for normal hematopoiesis. Sci Adv 3:e1601602
Li, Jianping; He, Fuhong; Zhang, Peng et al. (2017) Loss of Asxl2 leads to myeloid malignancies in mice. Nat Commun 8:15456
Huber, Ferdinand M; Greenblatt, Sarah M; Davenport, Andrew M et al. (2017) Histone-binding of DPF2 mediates its repressive role in myeloid differentiation. Proc Natl Acad Sci U S A 114:6016-6021
Man, Na; Tan, Yurong; Sun, Xiao-Jian et al. (2017) Caspase-3 controls AML1-ETO-driven leukemogenesis via autophagy modulation in a ULK1-dependent manner. Blood 129:2782-2792
Cheng, G; Liu, F; Asai, T et al. (2017) Loss of p300 accelerates MDS-associated leukemogenesis. Leukemia 31:1382-1390

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