A RUNX1/ETO-SKP2-CDKN1B axis regulates expression of telomerase in t (8;21) acute myeloid leukemia

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作者
Emmanuel J. Moses
Adam Azlan
Kang Zi Khor
Yee Yik Mot
Saleem Mohamed
Azman Seeni
Farnaz Barneh
Olaf Heidenreich
Narazah Yusoff
机构
[1] Advanced Medical and Dental Institute,Department of Biomedical Sciences
[2] Universiti Sains Malaysia,Department of Toxicology, Advanced Medical and Dental Institute
[3] Princess Maxima Center for Pediatric Oncology,undefined
[4] Wolfson Childhood Cancer Research Centre,undefined
[5] Translational and Clinical Research Institute,undefined
[6] Newcastle University,undefined
[7] Advanced Medical and Dental Institute,undefined
[8] Universiti Sains Malaysia,undefined
[9] Universiti Sains Malaysia,undefined
来源
关键词
RUNX1/ETO; Acute Myeloid Leukaemia (AML); Transcription factor; Telomerase Reverse Transcriptase (TERT); Self renewal; Cell cycle;
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摘要
The fusion oncoprotein RUNX1/ETO which results from the chromosomal translocation t (8;21) in acute myeloid leukemia (AML) is an essential driver of leukemic maintenance. We have previously shown that RUNX1/ETO knockdown impairs expression of the protein component of telomerase, TERT. However, the underlying molecular mechanism of how RUNX1/ETO controls TERT expression has not been fully elucidated. Here we show that RUNX1/ETO binds to an intergenic region 18 kb upstream of the TERT transcriptional start site and to a site located in intron 6 of TERT. Loss of RUNX1/ETO binding precedes inhibition of TERT expression. Repression of TERT expression is also dependent on the destabilization of the E3 ubiquitin ligase SKP2 and the resultant accumulation of the cell cycle inhibitor CDKN1B, that are both associated with RUNX1/ETO knockdown. Increased CDKN1B protein levels ultimately diminished TERT transcription with E2F1/Rb involvement. Collectively, our results show that RUNX1/ETO controls TERT expression directly by binding to its locus and indirectly via a SKP2—CDKN1B—E2F1/Rb axis.
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