Journal
MEDICAL SCIENCE MONITOR
Volume 24, Issue -, Pages 6735-6741Publisher
INT SCIENTIFIC INFORMATION, INC
DOI: 10.12659/MSM.910325
Keywords
Apoptosis; Cell Proliferation; Iron Chelating Agents; Leukemia, Myeloid, Acute
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Funding
- Nanjing Municipal Health Bureau [YKK15087]
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Background: This study aimed to investigate the effect of deferoxamine (DFO) on leukemia in vitro, and to explore the underlying molecular mechanism. Material/Methods: K562 leukemia cells were treated with various concentrations of DFO (10, 50, and 100 mu mol/l) with or with- out 10 mu mol/l ferric chloride for 12 h. Then, total cellular iron was detected. CCK-8 kit and flow cytometry were used for cell viability and apoptosis detection. In addition, expression of apoptosis-related genes was determined by Western blotting and qRT-PCR, respectively. Results: The results suggested that DFO significantly inhibited K562 cell viability and induced cell apoptosis in a dose- dependent manner. We also found that the protein and mRNA levels of Bax, p53, and Fas dose-dependently increased in DFO-treated K562 cells, while the level of Bcl-2 markedly decreased in a dose-dependent manner. Moreover, the findings showed that ferric chloride eliminated these effects on K562 cells caused by DFO treatment. Conclusions: Our results indicate that DFO plays a protective role in leukemia via inhibiting leukemia cell viability and inducing cell apoptosis by the regulation of apoptosis-related genes expression.
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