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Heterogeneity in leukemia cells that escape drug-induced senescence-like state

David F. Miller, Kyra Kerkhofs, Farnoosh Abbas‐Aghababazadeh, Sahib Singh Madahar, Mark D. Minden, Josée Hébert, Benjamin Haibe‐Kains, Mark A. Bayfield, Samuel Benchimol

2023Cell Death and Disease12 citationsDOIOpen Access PDF

Abstract

Erythropoietin (EPO) suppresses drug-induced apoptosis in EPO-receptor-positive leukemia cells and allows cells to persist after drug treatment by promoting cellular senescence. Importantly a small proportion of senescent cells can re-enter the cell cycle and resume proliferation after drug treatment, resulting in disease recurrence/persistence. Using a single-cell assay to track individual cells that exit a drug-induced senescence-like state, we show that cells exhibit asynchronous exit from a senescent-like state, and display different rates of proliferation. Escaped cells retain sensitivity to drug treatment, but display inter-clonal variability. We also find heterogeneity in gene expression with some of the escaped clones retaining senescence-associated gene expression. Senescent leukemia cells exhibit changes in gene expression that affect metabolism and senescence-associated secretory phenotype (SASP)-related genes. Herein, we generate a senescence gene signature and show that this signature is a prognostic marker of worse overall survival in AML and multiple other cancers. A portion of senescent leukemia cells depend on lysosome activity; chloroquine, an inhibitor of lysosome activity, promotes senolysis of some senescent leukemia cells. Our study indicates that the serious risks associated with the use of erythropoietin-stimulating agents (ESAs) in anemic cancer patients may be attributed to their ability to promote drug-tolerant cancer cells through the senescence program.

Topics & Concepts

SenescenceBiologyLeukemiaCancer cellCancer researchPhenotypeLysosomeCell growthCell biologyApoptosisCancerGeneImmunologyGeneticsBiochemistryEnzymeTelomeres, Telomerase, and SenescenceAcute Myeloid Leukemia ResearchSingle-cell and spatial transcriptomics
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