Abstract

Bone disease occurs in over 80% of Multiple Myeloma (MM) patients and is characterized by severe osteolytic bone destruction accompanied by profoundly suppressed or absent bone formation that has devastating consequences for patients These consequences include pathologic fractures, severe bone pain and derangements in mineral metabolism that negatively impact survival, performance status and quality of life. Adhesive interactions between bone marrow stromal cells (BMSC) and MM cells play a key role in pathogenesis of MMBD because they activate multiple signaling pathways and induce potent mediators that regulate osteoclast (OCL) and osteoblast (OB) activity as well as promote tumor growth. Although new MM therapies have greatly improved progression-free and overall survival, MM still remains incurable for most patients. Thus, novel treatments that effectively target the multiplicity of mediators and signaling pathways induced by the interactions of MM cells with their microenvironment are needed if we are to cure MM. In studies leading to this proposal, we identified Sequestosome-1 (p62), as a potential target to block the effects of key signal pathways in MMBD. p62 is a multidomain adapter protein that serves as a signaling hub for formation of multiple signaling complexes induced in BMSC by adhesive interactions with MM cells resulting in activation of NF-kB, p38 MAPK and JNK. Activation of these signaling pathways increases MM cell growth, OCL activity, and production of IL-6, RANKL and TNF? in BMSC as well as suppresses OB differentiation of patient BMSCs (MM-BMSC). Importantly, knockdown (KD) of p62 in MM-BMSC markedly decreases the capacity of MM cells to upregulate VCAM1, IL-6, TNF? and RANKL production, and enhances MM growth and OCL formation. Recently, we showed that when mice with established MM were treated with a small molecule antagonist to the p62-ZZ domain, the domain that mediates many of the effects of enhanced p62-mediated signaling in MM-BMSC, dramatic new bone formation occurred exclusively in MM-involved bones. In addition we found that: 1) the transcriptional repressor Gfi1 (growth factor independence1) is increased in MM-BMSC and MM cells from a majority of patients; 2) direct co-culture of MM cells with wild type (WT), but not p62 knockout (KO) BMSC, as well as IL-6 treatment markedly increased Gfi1 expression in MM cells and BMSC; 3) upregulation of Gfi1 in MM-BMSC inhibits OB differentiation by repressing transcription of the critical OB transcription factor Runx2; 4) knock-down (KD) of Gfi1 allows MM-BMSC to differentiate to OB and 5) KD of Gfi1 in MM cells decreased their growth and induced apoptosis. However, the role of the p62/Gfi1 signaling axis in MMBD is not established. It is our hypotheses that adhesive interactions between BMSC and MM cells enhance p62-mediated signaling in BMSC, which increases Gfi1, IL-6, RANKL, VCAM1, and TNF? in BMSC and results in suppressed OB differentiation, increased bone destruction and Gfi1 upregulation in MM cells. Increased Gfi1 expression in MM cells suppresses transcription of pro- apoptotic genes and increases STAT3 signaling in MM cells to promote MM survival and growth. To test these hypotheses, we will use novel ex vivo and in vivo approaches to determine:
Aim 1) the contributions of the p62/Gfi1 axis in MM-BMSC to the suppression of OB differentiation, MM-BMSC enhancement of MM cell growth and MMBD and the mechanisms mediating these effects in vitro and in vivo.
Aim 2) the contributions of increased Gfi1 expression in MM cells to MM cell growth and survival and the mechanisms mediating these effects in vitro and in vivo. Results of these studies should provide important new information on the role of the p62/Gfi1 axis in MM, and provide a basis for development of novel mechanism-based therapies that target the p62/Gfi1 axis as treatment for Veterans with MM.

Public Health Relevance

This Merit Review proposal will use novel ex vivo and in vivo approaches to assess the mechanisms responsible for p62/Gfi1's enhancement of Myeloma Bone Disease (MMBD) and MM cell growth and survival, and the potential of targeting the p62/Gfi1 axis as a novel treatment for Veterans with MM. The project will test the hypotheses that adhesive interactions between BMSC and MM cells enhance p62-mediated signaling in bone marrow stromal cells (BMSC) and increase bone destruction and Gfi1 expression in MM cells. Increased Gfi1 expression in MM cells suppresses transcription of pro-apoptotic genes and increases STAT3 signaling by blocking PIAS3 binding to STAT3, to promote MM survival and growth. The study will determine: 1) the contributions of the p62/Gfi1 axis in MM-BMSC to MM cell growth and MMBD and the mechanisms mediating these effects in vitro and in vivo and 2) the contributions of increased Gfi1 expression in MM cells to MM cell growth and survival and the mechanism mediating these effects in vitro and in vivo.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
Veterans Affairs (VA)
Type
Non-HHS Research Projects (I01)
Project #
5I01CX000623-06
Application #
9323824
Study Section
Hematology (HEMA)
Project Start
2012-07-01
Project End
2020-06-30
Budget Start
2017-07-01
Budget End
2018-06-30
Support Year
6
Fiscal Year
2017
Total Cost
Indirect Cost

  Institution

Name
Rlr VA Medical Center
Department
Type
DUNS #
608434697
City
Indianapolis
State
IN
Country
United States
Zip Code
46202

  Publications

Marino, Silvia; Roodman, G David (2018) Multiple Myeloma and Bone: The Fatal Interaction. Cold Spring Harb Perspect Med 8:
Adamik, Juraj; Silbermann, Rebecca; Marino, Silvia et al. (2018) XRK3F2 Inhibition of p62-ZZ Domain Signaling Rescues Myeloma-Induced GFI1-Driven Epigenetic Repression of the Runx2 Gene in Pre-osteoblasts to Overcome Differentiation Suppression. Front Endocrinol (Lausanne) 9:344
Petrusca, Daniela N; Toscani, Denise; Wang, Feng-Ming et al. (2018) Growth factor independence 1 expression in myeloma cells enhances their growth, survival, and osteoclastogenesis. J Hematol Oncol 11:123
Adamik, Juraj; Jin, Shunqian; Sun, Quanhong et al. (2017) EZH2 or HDAC1 Inhibition Reverses Multiple Myeloma-Induced Epigenetic Suppression of Osteoblast Differentiation. Mol Cancer Res 15:405-417
Hiasa, Masahiro; Okui, Tatsuo; Allette, Yohance M et al. (2017) Bone Pain Induced by Multiple Myeloma Is Reduced by Targeting V-ATPase and ASIC3. Cancer Res 77:1283-1295
Delgado-Calle, J; Anderson, J; Cregor, M D et al. (2017) Genetic deletion of Sost or pharmacological inhibition of sclerostin prevent multiple myeloma-induced bone disease without affecting tumor growth. Leukemia 31:2686-2694
Hao, M; Franqui-Machin, R; Xu, H et al. (2017) NEK2 induces osteoclast differentiation and bone destruction via heparanase in multiple myeloma. Leukemia 31:1648-1650
Teramachi, J; Silbermann, R; Yang, P et al. (2016) Blocking the ZZ domain of sequestosome1/p62 suppresses myeloma growth and osteoclast formation in vitro and induces dramatic bone formation in myeloma-bearing bones in vivo. Leukemia 30:390-8