Mesenchymal stem cells secretomes' affect multiple myeloma translation initiation

H Marcus; O Attar-Schneider; M Dabbah; V Zismanov; S Tartakover-Matalon; M Lishner; L Drucker

doi:10.1016/j.cellsig.2016.03.003

Mesenchymal stem cells secretomes' affect multiple myeloma translation initiation

Cell Signal. 2016 Jun;28(6):620-30. doi: 10.1016/j.cellsig.2016.03.003. Epub 2016 Mar 11.

Authors

H Marcus¹, O Attar-Schneider¹, M Dabbah¹, V Zismanov¹, S Tartakover-Matalon¹, M Lishner², L Drucker³

Affiliations

¹ Oncogenetic Laboratory, Tel Aviv University, Tel Aviv, Israel; Sackler faculty of Medicine, Tel Aviv University, Tel Aviv, Israel.
² Oncogenetic Laboratory, Tel Aviv University, Tel Aviv, Israel; Internal Medicine Department, Meir Medical Center, Kfar Saba, Tel Aviv University, Tel Aviv, Israel; Sackler faculty of Medicine, Tel Aviv University, Tel Aviv, Israel.
³ Oncogenetic Laboratory, Tel Aviv University, Tel Aviv, Israel; Sackler faculty of Medicine, Tel Aviv University, Tel Aviv, Israel. Electronic address: druckerl@clalit.org.il.

PMID: 26976208
DOI: 10.1016/j.cellsig.2016.03.003

Abstract

Bone marrow mesenchymal stem cells' (BM-MSCs) role in multiple myeloma (MM) pathogenesis is recognized. Recently, we have published that co-culture of MM cell lines with BM-MSCs results in mutual modulation of phenotype and proteome (via translation initiation (TI) factors eIF4E/eIF4GI) and that there are differences between normal donor BM-MSCs (ND-MSCs) and MM BM-MSCs (MM-MSCs) in this crosstalk. Here, we aimed to assess the involvement of soluble BM-MSCs' (ND, MM) components, more easily targeted, in manipulation of MM cell lines phenotype and TI with specific focus on microvesicles (MVs) capable of transferring critical biological material. We applied ND and MM-MSCs 72h secretomes to MM cell lines (U266 and ARP-1) for 12-72h and then assayed the cells' (viability, cell count, cell death, proliferation, cell cycle, autophagy) and TI (factors: eIF4E, teIF4GI; regulators: mTOR, MNK1/2, 4EBP; targets: cyclin D1, NFκB, SMAD5, cMyc, HIF1α). Furthermore, we dissected the secretome into >100kDa and <100kDa fractions and repeated the experiments. Finally, MVs were isolated from the ND and MM-MSCs secretomes and applied to MM cell lines. Phenotype and TI were assessed. Secretomes of BM-MSCs (ND, MM) significantly stimulated MM cell lines' TI, autophagy and proliferation. The dissected secretome yielded different effects on MM cell lines phenotype and TI according to fraction (>100kDa- repressed; <100kDa- stimulated) but with no association to source (ND, MM). Finally, in analyses of MVs extracted from BM-MSCs (ND, MM) we witnessed differences in accordance with source: ND-MSCs MVs inhibited proliferation, autophagy and TI whereas MM-MSCs MVs stimulated them. These observations highlight the very complex communication between MM and BM-MSCs and underscore its significance to major processes in the malignant cells. Studies into the influential MVs cargo are underway and expected to uncover targetable signals in the regulation of the TI/proliferation/autophagy cascade.

Keywords: Microvesicles; Multiple myeloma; Translation initiation; bone marrow mesenchymal stem cells (BM-MSCs); eIF4E; eIF4GI.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Autophagy
Cell Line, Tumor
Cell Proliferation
Cells, Cultured
Eukaryotic Initiation Factor-4E / metabolism
Eukaryotic Initiation Factor-4G / metabolism
Humans
Mesenchymal Stem Cells / metabolism*
Multiple Myeloma / genetics*
Multiple Myeloma / metabolism
Multiple Myeloma / pathology
Peptide Chain Initiation, Translational*

Substances

Eukaryotic Initiation Factor-4E
Eukaryotic Initiation Factor-4G