Daunorubicin-induced variations in gene transcription: commitment to proliferation arrest, senescence and apoptosis

Author:

MANSILLA Sylvia1,PIÑA Benjamin1,PORTUGAL José1

Affiliation:

1. Departamento de Biología Molecular y Celular, Instituto de Biología Molecular de Barcelona, CSIC, Jordi Girona, 18-26, 08034 Barcelona, Spain

Abstract

We used a human cDNA macroarray containing various oncogenes and tumour suppressor genes to assess gene expression profiles in early-passage Jurkat T lymphocytes treated with clinically relevant concentrations of the antitumour antibiotic daunorubicin. Several oncogenes and tumour suppressor genes were either up- or down-regulated depending on the daunorubicin concentration used. The expression levels of some of these genes were confirmed by semi-quantitative reverse transcriptase–PCR. We also compared the changes in cell-cycle distribution and the apoptotic morphological characteristics of the cells treated with daunorubicin, using flow cytometry and fluorescence microscopy. Exposure to 182 nM daunorubicin (its IC75 in Jurkat T cells: where IC75 is the drug concentration that inhibits growth by 75%) resulted in cell-cycle arrest in G1 and almost immediate apoptosis. In contrast, decreasing the drug concentration to 91 nM (close to the IC50) caused G2 arrest and cell senescence-like growth arrest, whereas features of apoptosis and necrosis appeared only after longer incubation times. Gene expression profiles, cell-cycle distribution, the presence of DNA damage and the time-dependent response of Jurkat T cells to cell death were correlated clearly. The general behaviour of the genes suggests that cell-cycle arrest and cell death follow distinct pathways depending on drug concentration.

Publisher

Portland Press Ltd.

Subject

Cell Biology,Molecular Biology,Biochemistry

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