ETO, fusion partner in t(8;21) acute myeloid leukemia, represses transcription by interaction with the human N-CoR/mSin3/HDAC1 complex

Wang, Jianxiang; Hoshino, Taizo; Redner, Robert L.; Kajigaya, Sachiko; Liu, Johnson M.

doi:10.1073/pnas.95.18.10860

Cited by 480 publications

(415 citation statements)

References 32 publications

(43 reference statements)

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“…Since the MYND domain is a putative interaction molecule for the nuclear co-repressors N-CoR and SMRT (Lutterbach et al, 1998a;Gelmetti et al, 1998;Wang et al, 1998) we tested whether the MYND domain of BS69 also mediates N-CoR binding in a coimmunoprecipitation experiment. We transfected human U2OS osteosarcoma cells with expression vectors for FLAG tagged N-CoR and full-length human BS69 fused to the DNA binding domain of the yeast transcription factor GAL4 at the N-terminus ( Figure 2).…”

Section: Interaction Of Bs69 With N-cor Through the Mynd Domainmentioning

confidence: 99%

“…The C-terminus harbours a region with homology to the MYND domain, a two zinc ®nger motif ®rst identi®ed in DEAF-1 (Gross and McGinnis, 1996) and in MTG8/ETO (Lutterbach et al, 1998a). This domain was shown to be required for both repression of basal transcription by the AML/ETO fusion protein and binding of the transcriptional corepressors N-CoR and SMRT (Lutterbach et al, 1998b;Gelmetti et al, 1998;Wang et al, 1998). N-CoR and its close homologue SMRT were cloned as co-repressors of the thyroidhormone and retinoic acid receptors (Chen and Evans, 1995;Horlein et al, 1995).…”

Section: Introductionmentioning

confidence: 99%

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The adenovirus E1A binding protein BS69 is a corepressor of transcription through recruitment of N-CoR

Masselink

Bernards

2000

Oncogene

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BS69 was ®rst identi®ed as a protein that interacts directly with the transactivation domain (conserved region 3) of the 289R adenovirus type 5 E1A protein.We show here that BS69 is a potent repressor of transcription. BS69 mediates repression, at least in part, through interaction with the co-repressor N-CoR. BS69 interacts with N-CoR through a MYND domain in its carboxyl terminus. A recently cloned splice variant of BS69, designated BRAM1, is also capable of interacting with N-CoR and E1A, but unlike BS69, is not able to repress transcription, indicating that N-CoR interaction is necessary but not su cient for BS69 repression. Expression of E1A inhibits repression mediated by BS69. Our data suggest that BS69 participates in transcriptional repressor complexes and that E1A can modulate these complexes through interaction with BS69. Oncogene (2000) 19, 1538 ± 1546.

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Section: Interaction Of Bs69 With N-cor Through the Mynd Domainmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

The adenovirus E1A binding protein BS69 is a corepressor of transcription through recruitment of N-CoR

Masselink

Bernards

2000

Oncogene

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“…The resulting AML1-ETO fusion protein is expressed in E12% of AML of the M2 subtype (Look, 1997). AML1-ETO has been shown to interact with a number of proteins present in corepressor complexes, suggesting that AML1-ETO may act as a transcriptional repressor (Meyers et al, 1995;Gelmetti et al, 1998;Lutterbach et al, 1998;Wang et al, 1998;Westendorf et al, 1998;Amann et al, 2001;Hildebrand et al, 2001;Zhang et al, 2001;Linggi et al, 2002;Lausen et al, 2004). However, there have been very few studies that correlate a DNA binding event by AML1-ETO at a target gene's promoter with a direct consequence on transcription (see, e.g.…”

Section: Introductionmentioning

confidence: 99%

ELA2 is regulated by hematopoietic transcription factors, but not repressed by AML1-ETO

et al. 2005

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A 117 bp fragment of the human ELA2 promoter has been characterized that can act as a minimal promoter for the expression of neutrophil elastase. Chromatin immunoprecipitation and siRNAs revealed that expression of ELA2 is regulated by the acute myeloid human leukemia 1 protein (AML1), C/EBPa, PU.1 and c-Myb transcription factors. ELA2 has also been investigated as a possible target of the leukemic fusion protein AML1-ETO resulting from the t(8;21) chromosomal translocation. AML1-ETO, like AML1, binds the ELA2 promoter in the myeloid cell lines Kasumi-1 and U937, but unexpectedly fails to significantly alter expression of ELA2. Although AML1-ETO downregulates the expression of C/EBPa, changes in C/EBPa expression do not correlate with changes in the expression of ELA2. Our observations indicate that AML1-ETO may not be a constitutive repressor of gene expression in every case in which it can associate with DNA, either on its own or in conjunction with C/EBPa. Since neither ETO nor AML1-ETO are typically expressed in hematopoietic progenitors, we hypothesize that it is the interactions between AML1-ETO and regulatory cofactors in disease-state cells that alter gene expression programs during hematopoiesis. These protein-protein interactions may not require simultaneous DNA binding by AML1-ETO for the deleterious effects of the fusion protein to be realized.

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“…Indeed, AML1-ETO has been shown to act as a dominant negative inhibitor of AML1 [50]. Multiple repressors of transcription, such as Sin3A, HDAC, N-CoR, and SMRT, interact with the ETO portion of the fusion protein [17][18][19][20], which provides the molecular mechanisms of repression. AML1-ETO has been reported to repress the MDR1 promoter in hematopoietic HEL cells and non-hematopoietic C33A cells [26].…”

Section: Discussionmentioning

confidence: 99%

“…Furthermore, reporter-gene assays and protein-protein interaction data provide a further molecular mechanism for this effect. AML1-ETO binds to transcription repressor complexes, such as NCoR, Sin3A, SMRT, and class 1 histone deacetylases (HDACs), which actively shut down transcription from AML1 responsive promoters [15][16][17][18][19][20]. However, AML1-ETO does not always function as a transcriptional repressor.…”

Section: Introductionmentioning

confidence: 99%

Cell type dependent regulation of multidrug resistance-1 gene expression by AML1-ETO

Hines¹,

Boyapati²,

Zhang³

2007

Blood Cells, Molecules, and Diseases

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The AML1-ETO fusion protein is generated from the 8;21 chromosome translocation that is commonly identified in acute myeloid leukemia. AML1-ETO is a DNA binding transcription factor and has been demonstrated to play a critical role in promoting leukemogenesis. Therefore, it is important to define the molecular mechanism of AML1-ETO in the regulation of gene expression. Here, we report that the effect of AML1-ETO on the promoter of multidrug resistance-1 (MDR1) gene, a known AML1-ETO target, is highly cell type specific. Besides observing repression of the MDR1 promoter in C33A and CV-1 cells as reported previously, AML1-ETO strongly activated the promoter in K562 and B210 cells. More importantly, this activation required both the AML1 and ETO portions of the fusion protein, but did not depend on the AML1 binding site in MDR1 promoter. Furthermore, results from promoter deletion analysis and chromatin immunoprecipitation assays suggested that this activation effect was likely through the influence of the general transcription machinery rather than promoter-specific factors. Based on these data, we propose that AML1-ETO may have opposing effects on gene expression depending on the various conditions of the cellular environment.

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ETO, fusion partner in t(8;21) acute myeloid leukemia, represses transcription by interaction with the human N-CoR/mSin3/HDAC1 complex

Cited by 480 publications

References 32 publications

The adenovirus E1A binding protein BS69 is a corepressor of transcription through recruitment of N-CoR

The adenovirus E1A binding protein BS69 is a corepressor of transcription through recruitment of N-CoR

ELA2 is regulated by hematopoietic transcription factors, but not repressed by AML1-ETO

Cell type dependent regulation of multidrug resistance-1 gene expression by AML1-ETO

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