Literature DB >> 26657151

Excess of NPM-ALK oncogenic signaling promotes cellular apoptosis and drug dependency.

Monica Ceccon1, Maria Elena Boggio Merlo2,3, Luca Mologni1, Teresa Poggio2,3, Lydia M Varesio2,3, Matteo Menotti2,3, Silvia Bombelli1, Roberta Rigolio4, Andrea D Manazza2,3, Filomena Di Giacomo2,3, Chiara Ambrogio5, Giovanni Giudici6, Cesare Casati7, Cristina Mastini2,3, Mara Compagno2,3,8, Suzanne D Turner9, Carlo Gambacorti-Passerini1,10, Roberto Chiarle2,3,8, Claudia Voena2,3.   

Abstract

Most of the anaplastic large-cell lymphoma (ALCL) cases carry the t(2;5; p23;q35) that produces the fusion protein NPM-ALK (nucleophosmin-anaplastic lymphoma kinase). NPM-ALK-deregulated kinase activity drives several pathways that support malignant transformation of lymphoma cells. We found that in ALK-rearranged ALCL cell lines, NPM-ALK was distributed in equal amounts between the cytoplasm and the nucleus. Only the cytoplasmic portion was catalytically active in both cell lines and primary ALCL, whereas the nuclear portion was inactive because of heterodimerization with NPM1. Thus, about 50% of the NPM-ALK is not active and sequestered as NPM-ALK/NPM1 heterodimers in the nucleus. Overexpression or relocalization of NPM-ALK to the cytoplasm by NPM genetic knockout or knockdown caused ERK1/2 (extracellular signal-regulated protein kinases 1 and 2) increased phosphorylation and cell death through the engagement of an ATM/Chk2- and γH2AX (phosphorylated H2A histone family member X)-mediated DNA-damage response. Remarkably, human NPM-ALK-amplified cell lines resistant to ALK tyrosine kinase inhibitors (TKIs) underwent apoptosis upon drug withdrawal as a consequence of ERK1/2 hyperactivation. Altogether, these findings indicate that an excess of NPM-ALK activation and signaling induces apoptosis via oncogenic stress responses. A 'drug holiday' where the ALK TKI treatment is suspended could represent a therapeutic option in cells that become resistant by NPM-ALK amplification.

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Year:  2015        PMID: 26657151      PMCID: PMC4907875          DOI: 10.1038/onc.2015.456

Source DB:  PubMed          Journal:  Oncogene        ISSN: 0950-9232            Impact factor:   9.867


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