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53 Role of the MSC-Derived Exosomal and Endogenous JAK2-SET/PP2A-Beta Catenin-Modulator Mir-300 in Leukemic Stem/Progenitor Proliferation and Survival in CML

Chronic Myeloid Leukemia: Biology and Pathophysiology, excluding Therapy
Program: Oral and Poster Abstracts
Type: Oral
Session: 631. Chronic Myeloid Leukemia: Biology and Pathophysiology, excluding Therapy: Targeting Leukemic Stem Cells in Chronic Myeloid Leukemia
Saturday, December 5, 2015: 10:30 AM
W340, Level 3 (Orange County Convention Center)

Giovannino Silvestri, PhD1*, Lorenzo Stramucci, PhD1*, Justin Ellis2*, Justine Yu3*, Jason Harb, PhD4*, Paolo Neviani, PhD5, Guido Marcucci, MD6*, Klara Srutova7*, Katerina Machova Polakova8*, Denis-Claude Roy, MD9, Peter Hokland, M.D.10, Michael W. Deininger11, Ravi Bhatia, MD12*, Carlo Gambacorti-Passerini13, Dragana Milojkovic14*, Alistair G Reid, BSc, PhD15*, Jane F. Apperley, MD16, Ferenc Livak, PhD17*, Maria R. Baer, MD18, Rossana Trotta, PhD19* and Danilo Perrotti, MD, PhD20

1The Greenebaum Cancer Center, Dept. of Medicine, University of Maryland Baltimore, school of Medicine, Baltimore, MD
2The Ohio State University Comprehensive Cancer Center, Columbus, OH
3the Greenebaum Cancer Center, Dept. of Medicine, University of Maryland Baltimore, school of Medicine, Baltimore, MD
4Blood Research Institute BloodCenter of Wisconsin, Milwaukee, WI
5Norris Comprehensive Cancer Center, Children's Hospital Los Angeles, Los Angeles, CA
6Division of Hematopoietic Stem Cell and Leukemia Research of Beckman Research Institute, Gehr Family Center for Leukemia Research, City of Hope National Medical Center, Duarte, CA
7Institute of Hematology and Blood Transfusion, Prague, Czech Republic
8Institute of Hematology and Blood Transfusion, University of Prague, Prague, Czech Republic
9Department of Hematology and Cellular Therapy Laboratory, Hôpital Maisonneuve-Rosemont, University of Montreal, Montreal, QC, Canada
10Department of Hematology, Aarhus University Hospital, Aarhus, Denmark
11Huntsman Cancer Institute, University of Utah, Salt Lake City, UT
12University of Alabama Birmingham, Birmingham, AL
13Azienda Ospedaliera San Gerardo/University of Milano-Bicocca, Monza, Italy
14Department of Haematology, Hammersmith Hospital (Imperial College Healthcare NHS Trust), London, United Kingdom
15Haematology Department, Hammersmith Hospital (Imperial College Healthcare NHS Trust), London, United Kingdom
16Department of Haematology, Imperial College London, Hammersmith Hospital, London, United Kingdom
17Microbiology and Immunology, University of Maryland Baltimore, school of Medicine, Baltimore, MD
18Greenebaum Cancer Center, University of Maryland Baltimore, Baltimore, MD
19Dept. microbiology and Immunology, University of Maryland Baltimore, school of Medicine, Baltimore, MD
20Dept. Medicine, University of Maryland - Greenebaum Cancer Center, Baltimore, MD

MiR-300 is a microRNA predicted to target multiple components of the BCR-ABL1 / JAK2 / hnRNPA1 / SET / PP2A / β-catenin pathway, which is essential for survival/self-renewal of leukemic progenitors and quiescent TKI-resistant Ph+ hematopoietic stem cells (HSCs). Nanostring arrays analysis of bone marrow (BM) cells from healthy individuals (n=5) and CML patients (n=10) showed gradual inhibition of miR-300 expression (CML-CPmiR-300>CML-BCmiR-300).

MiR-300 transduction in CMLCD34+ cells and BCR-ABL1+ cell lines decreased JAK2, β-catenin, hnRNPA1 and SET expression and increased PP2A activity. Targets were confirmed by miR-300 expression in BCR-ABL1+ cells expressing Flag-tagged miR-300-targets lacking or carrying a wild-type or mutated 3’UTR. Restored miR-300 expression in CMLCD34+ cells and/or BCR-ABL1+ cell lines impaired cell cycle progression, proliferation and clonogenic potential, markedly reduced LTC-ICs, and increased TKI sensitivity. Notably, miR-300 expression was inhibited by BCR-ABL1 in proliferating cells. Accordingly, imatinib restored miR-300 expression in CD34+ dividing progenitors and BCR-ABL1+ cell lines without altering miR-300 levels in quiescent (CFSEMAX) CMLCD34+ cells (n=3), consistent with the BCR-ABL1 kinase-dependent activation of the Jak2/SET/PP2A/β-catenin pathway in CML progenitors but not quiescent Ph+ HSCs. Indeed, ectopic SET expression counteracted the negative effects of mir-300 on cell proliferation and survival.  Surprisingly, miR-300 levels were increased in CD34+CD38- compared to CD34+CD38+ CML cells, and >20-fold higher in CFSEMAX compared to dividing CMLCD34+ cells (n=4).  

To determine whether enhanced miR-300 expression in quiescent cells depends on cell autonomous events or is induced by the BM microenvironment, we exposed BCR-ABL+ cells to conditioned medium (CM) of HS-5 or hTERT mesenchymal stem cells (MSC). CM strongly decreased proliferation, induced imatinib but not FTY720 (PP2A activator) resistance, increased miR-300 levels, decreased BCR-ABL1 activity and Jak2 expression but not its activity, and did not alter b-catenin levels or PP2A activity. Interestingly, miR-300 was found in MSC-derived exosomes, and its expression increased in BCR-ABL1+ cells exposed to exosomes. Accordingly, proliferation of CML-BCCD34+and LAMA-84 cells was strongly reduced upon exposure to MSC-derived exosomes. These effects were abolished when we used CM from MSCs transduced with a miR-300 antagomir.

Altogether our results indicate that downregulation of miR-300 appears necessary for the activation of JAK2/SET/PP2A/b-catenin survival signals in CML progenitors. Conversely, increased miR-300 levels (endogenous and MSC-derived) seem to be required for HSC quiescence.

Disclosures: Deininger: Novartis: Other: Consulting or Advisory Role , Research Funding ; BMS: Other: Consulting & Advisory Role , Research Funding ; Celgene: Research Funding ; Genzyme: Research Funding ; Gilead: Research Funding ; ARIAD Pharmaceutical Inc.: Other: Consulting or Advisory Role ; Incyte: Other: Consulting or Advisory Role ; Pfizer: Other: Consulting or Advisory Role . Milojkovic: BMS: Honoraria ; ARIAD Pharmaceuticals Inc.: Honoraria ; Novartis: Honoraria ; Pfizer: Honoraria .

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