INTRODUCTION: Multiple Myeloma (MM) is an aggressive, debilitating and deadly hematological malignancy, arising from clonal expansion of plasma cells at multiple sites in the bone marrow. Recently, MM proved sensitive to a new class of drugs, proteasome inhibitors (PI), but the mechanisms of action and bases of individual susceptibility remain still largely unclear. Recent work linked PI sensitivity to protein synthesis and proteasome activity (1-2), raising the question of whether different levels of proteasome expression and workload underlie PI sensitivity in normal and transformed plasma cells. RESULTS: To test this hypothesis we first adopted different models of B cell activation in mouse, and observed that following polyclonal activation, proteasome activity decreases even more than previously reported in vitro (3). This decrease is linked to enhanced apoptosis after treatment with the potent anti-myeloma proteasome inhibitor bortezomib (PS-341, Velcade™). Accordingly, in vivo treatment with PS-341 decreases Ab titres in T-dependent and -independent mouse immunization models, therefore providing the rationale for limiting the activity of Ab-secreting cells in vivo by impacting proteasome function. Furthermore, to asses whether the exquisite sensitivity of certain MM cells (MMC) to PI may also be due to their intense protein secretion function, we directly assessed protein degradation by proteasomes in two human MM cell lines - U266 and MM.1S - that display a differential sensitivity to bortezomib. These two lines reveal a striking direct correlation between the degradative flux of proteins through proteasomes and the apoptotic response to bortezomib. In particular, proteasomal degradation within 30 minutes of chase is fivefold higher in MM.1S, the far more sensitive line, indicating that these cells are intensively degrading short-lived protein species. Paradoxically, cell extracts from MM.1S cells show nearly half the proteasomal activity of U266 cells, suggesting a decreased pool of proteasomes as compared to the resistant line. In this scenario, accumulation of poly-ubiquitinated proteins and the accompanying decrease of free ubiquitin reveal proteasome stress in PI-sensitive MMC. Altogether, our data indicate that the balance between proteasome workload and degradative capacity represents a critical determinant of apoptotic sensitivity of MMC to PI, providing both a novel predictive tool of potential prognostic value and the framework for novel combination therapies.
Imbalance between synthetic load and proteasomal capacity sensitizes normal and malignant plasma cells to proteasome inhibitors
CASCIO, Paolo;CERRUTI, Fulvia;
2008-01-01
Abstract
INTRODUCTION: Multiple Myeloma (MM) is an aggressive, debilitating and deadly hematological malignancy, arising from clonal expansion of plasma cells at multiple sites in the bone marrow. Recently, MM proved sensitive to a new class of drugs, proteasome inhibitors (PI), but the mechanisms of action and bases of individual susceptibility remain still largely unclear. Recent work linked PI sensitivity to protein synthesis and proteasome activity (1-2), raising the question of whether different levels of proteasome expression and workload underlie PI sensitivity in normal and transformed plasma cells. RESULTS: To test this hypothesis we first adopted different models of B cell activation in mouse, and observed that following polyclonal activation, proteasome activity decreases even more than previously reported in vitro (3). This decrease is linked to enhanced apoptosis after treatment with the potent anti-myeloma proteasome inhibitor bortezomib (PS-341, Velcade™). Accordingly, in vivo treatment with PS-341 decreases Ab titres in T-dependent and -independent mouse immunization models, therefore providing the rationale for limiting the activity of Ab-secreting cells in vivo by impacting proteasome function. Furthermore, to asses whether the exquisite sensitivity of certain MM cells (MMC) to PI may also be due to their intense protein secretion function, we directly assessed protein degradation by proteasomes in two human MM cell lines - U266 and MM.1S - that display a differential sensitivity to bortezomib. These two lines reveal a striking direct correlation between the degradative flux of proteins through proteasomes and the apoptotic response to bortezomib. In particular, proteasomal degradation within 30 minutes of chase is fivefold higher in MM.1S, the far more sensitive line, indicating that these cells are intensively degrading short-lived protein species. Paradoxically, cell extracts from MM.1S cells show nearly half the proteasomal activity of U266 cells, suggesting a decreased pool of proteasomes as compared to the resistant line. In this scenario, accumulation of poly-ubiquitinated proteins and the accompanying decrease of free ubiquitin reveal proteasome stress in PI-sensitive MMC. Altogether, our data indicate that the balance between proteasome workload and degradative capacity represents a critical determinant of apoptotic sensitivity of MMC to PI, providing both a novel predictive tool of potential prognostic value and the framework for novel combination therapies.
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