The outcomes for acute myeloid leukemia (AML) have remained abysmal for the past 30 years. 20- 40% of patients fail to achieve remission with induction chemotherapy, and 50-70% of patients who achieve a complete remission relapse within 3 years. While cytogenetics are the backbone of risk-stratification, nearly 50% of AML cases are cytogenetically normal (CN-AML) and, biologically and clinically, the most heterogenous group. The nucleo-cytoplasmic shuttle protein nucleophosmin (NPM1) is mutated in 50% of CN-AML cases resulting in the nuclear export of this protein. This has been shown in large clinical cohorts to confer a favorable prognosis and obviates the need for a bone marrow transplant in these patients. This subset of AML has been recognized in a unique diagnostic category in the WHO 2008 classification of hematologic malignancies. The mechanism by which mutated NPM1 (NPM1mut) confers this advantage in CN-AML is unclear. It has previously been hypothesized that NPM1mut dislocates other protein partners into the cytoplasm and consequently affecting their function. We have previously demonstrated that FOXM1, an oncogenic transcription factor, co-localizes with NPM1 in cancer cells. In this proposal, using a novel multispectral imaging modality we will study the cellular interaction of FOXM1 and NPM1 in AML primary blast cells. We will also investigate the functional significance of FOXM1 localization in this disease using AML cell lines. Importantly, we will assess the clinical correlation of mislocalized cytoplasmic FOXM1 with outcomes in AML with the goal of examining its role as a favorable prognostic marker in CN-AML. We intend to show that FOXM1 is the oncogenic driver dictating prognosis in AML. Mutations in NPM1 resulting in its nuclear export mislocalizes FOXM1 to the cytoplasm where it is inactive as a transcription factor. This may account for the improved outcome in this sizeable subset of AML patients. In several AML cell lines we will test how FOXM1 knockdown or FOXM1 overexpression will affect sensitivity to chemotherapeutic drugs in vitro and vivo. We will determine whether FOXM1 knockdown in AML cell lines with nuclear localization of FOXM1 makes them more sensitive to chemotherapy. Nude mice will be injected with AML cell lines with stable FOXM1 knockdown or OCI-AML3 cell line with stable FOXM1 knockdown or with FOXM1 overexpression, and with control cell lines to establish xenograft tumors. We expect that FOXM1 knockdown in U937 and HL60 AML cell lines will increase sensitivity to treatment in xenograft tumors induced by these AML cell lines. I contrast, suppression of FOXM1, localized in the cytoplasm, in OCI-AML3 cell line would not affect sensitivity to chemotherapy in xenograft tumors induced by this cell line. The experiments described in our proposal will reveal if cytoplasmic FOXM1 is a novel favorable prognostic factor in AML and whether nuclear expression of FOXM1 determines the resistance of xenograft tumors induced by AML cell lines to chemotherapy.

Public Health Relevance

Nucleophosmin (NPM1) is a nuclear-cytoplasmic shuttle protein mutated in half of the cases of cytogenetically normal acute myeloid leukemia (CN-AML) and associated with a highly favorable prognosis. By identifying cytoplasmic localization of FOXM1 as a relevant biomarker of favorable prognosis in this disease we will answer the question: what molecular properties make AML curable with conventional chemotherapy? We will assess the clinical correlation of cytoplasmic FOXM1 with outcomes in AML with the goal of establishing its role as a favorable prognostic marker for chemotherapy in CN- AML. Moreover, we will test the assumption that nuclear, but not cytoplasmic expression of FOXM1 increases resistance to chemotherapy of xenograft tumors induced by AML cell lines in mouse models. We will investigate whether FOXM1 suppression by RNAi in AML cell lines with nuclear but not cytoplasmic localization of FOXM1 diminishes the resistance to chemotherapy of xenograft tumors induced by these AML cell lines. Moreover by overexpressing FOXM1 in the nucleus of the OCI-AML3 cell line with known cytoplasmic FOXM1, we hope to impart an increased chemoresistance. Development of these ideas will be crucial to come one step closer to the development of novel approaches for the treatment and the diagnosis of AML patients.

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Exploratory/Developmental Grants (R21)
Project #
5R21CA194608-02
Application #
9061641
Study Section
Special Emphasis Panel (ZCA1)
Program Officer
Agrawal, Lokesh
Project Start
2015-05-01
Project End
2017-04-30
Budget Start
2016-05-01
Budget End
2017-04-30
Support Year
2
Fiscal Year
2016
Total Cost
Indirect Cost
Name
University of Illinois at Chicago
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
098987217
City
Chicago
State
IL
Country
United States
Zip Code
60612
Khan, Irum; Halasi, Marianna; Patel, Anand et al. (2018) FOXM1 contributes to treatment failure in acute myeloid leukemia. JCI Insight 3:
Halasi, Marianna; Hitchinson, Ben; Shah, Binal N et al. (2018) Honokiol is a FOXM1 antagonist. Cell Death Dis 9:84
Gartel, Andrei L (2017) FOXM1 in Cancer: Interactions and Vulnerabilities. Cancer Res 77:3135-3139
Khan, I; Halasi, M; Zia, M F et al. (2017) Nuclear FOXM1 drives chemoresistance in AML. Leukemia 31:251-255