Molecular signature of retinoic acid treatment in acute promyelocytic leukemia

被引:0
|
作者
Natalia Meani
Simone Minardi
Silvia Licciulli
Vania Gelmetti
Francesco Lo Coco
Clara Nervi
Pier Giuseppe Pelicci
Heiko Müller
Myriam Alcalay
机构
[1] IFOM – Institute of Molecular Oncology of the Italian Foundation for Cancer Research,Department of Biopathology
[2] European Institute of Oncology,undefined
[3] San Raffaele Bio-medical Science Park of Rome,undefined
[4] University of Tor Vergata,undefined
来源
Oncogene | 2005年 / 24卷
关键词
differentiation therapy; acute myeloid leukemia; transcriptional regulation; expression profiling; transcription factor binding sites;
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摘要
Acute promyelocytic leukemia (APL) is a distinct subtype of acute myeloid leukemia characterized by a block of differentiation at the promyelocytic stage. APL patients respond to pharmacological concentrations of all-trans retinoic acid (RA) and disease remission correlates with terminal differentiation of leukemic blasts. The PML/RAR oncogenic transcription factor is responsible for both the pathogenesis of APL and for its sensitivity to RA. In order to identify physiological targets of RA therapy, we analysed gene expression profiles of RA-treated APL blasts and found 1056 common target genes. Comparing these results to those obtained in RA-treated U937 cell lines revealed that transcriptional response to RA is largely dependent on the expression of PML/RAR. Several genes involved in the control of differentiation and stem cell renewal are early targets of RA regulation, and may be important effectors of RA response. Modulation of chromatin modifying genes was also observed, suggesting that specific structural changes in local chromatin domains may be required to promote RA-mediated differentiation. Computational analysis of upstream genomic regions in RA target genes revealed nonrandom distribution of transcription factor binding sites, indicating that specific transcriptional regulatory complexes may be involved in determining RA response.
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页码:3358 / 3368
页数:10
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