Differential Expression of ETS Family Transcription Factors in NCCIT Human Embryonic Carcinoma Cells upon Retinoic Acid-Induced Differentiation

Park, Sung-Won; Do, Hyun-Jin; Ha, Woo Tae; Han, Mi-Hee; Song, Hyuk; Uhm, Sang Jun; Chung, Hak-Jae; Kim, Jaehwan

doi:10.1248/bpb.b13-00985

Cited by 8 publications

(9 citation statements)

References 40 publications

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“…38) We also previously reported that OCT4 and GDF3 are highly expressed in pluripotent human EC NCCIT cells and that this expression is reduced upon RA treatment in a time-dependent manner. 30,36,37,39,40) However, there is no report concerning the interaction between OCT4 and GDF3 at the transcriptional level. Therefore, to investigate their transcriptional relationship in pluripotent germ cell-derived EC cells, we first examined the expression of GDF3 and OCT4 in NCCIT cells during RA-mediated differentiation.…”

Section: Resultsmentioning

confidence: 99%

Growth and Differentiation Factor 3 Is Transcriptionally Regulated by OCT4 in Human Embryonic Carcinoma Cells

Han

Park

et al. 2016

Biological & Pharmaceutical Bulletin

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Growth and differentiation factor 3 (GDF3), a mammalian-specific transforming growth factor β ligand, and OCT4, one of key stem cell transcription factors, are expressed in testicular germ cell tumors (TGCTs) as well as pluripotent stem cells. To understand the molecular mechanism by which OCT4 and GDF3 function in tumorigenesis as well as stemness, we investigated the transcriptional regulation of GDF3 mediated by OCT4 in human embryonic carcinoma (EC) NCCIT cells, which are pluripotent stem cells of TGCTs. GDF3 and OCT4 was highly expressed in undifferentiated NCCIT cells and then significantly decreased upon retinoic acid-induced differentiation in a time-dependent manner. Moreover, GDF3 expression was reduced by short hairpin RNA-mediated knockdown of OCT4 and increased by OCT4 overexpression, suggesting that GDF3 and OCT4 have a functional relationship in pluripotent stem cells. A promoter-reporter assay revealed that the GDF3 promoter ( 1721-Luc) activity was significantly activated by OCT4 in a dose-dependent manner. Moreover, the minimal promoter ( 183-Luc) was sufficient for OCT4-mediated transcriptional activation and provided a potential binding site for the direct interaction with OCT4. Collectively, this study provides the evidence about the regulatory mechanism of GDF3 mediated by OCT4 in pluripotent EC cells.

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Section: Resultsmentioning

confidence: 99%

Growth and Differentiation Factor 3 Is Transcriptionally Regulated by OCT4 in Human Embryonic Carcinoma Cells

Han

Park

et al. 2016

Biological & Pharmaceutical Bulletin

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“…FLI1 is a member of the large ETS transcription factor family 43 and has been associated with an increased proliferation, differentiation and evasion from apoptosis in human cancer cells. 44 , 45 Aberrant FLI1 activation induces dysregulated cell division and malignant transformation, 46 , 47 and in the NIH3T3 murine cell line with induced overexpression of FLI1, drug-induced apoptosis was inhibited. 47 In endothelial cells, ETS phosphorylation via the RAS/MAPK pathway is required for CD13 induction, 48 suggesting that there may be a link between the ETS transcription factor family and CD13.…”

Section: Discussionmentioning

confidence: 99%

Silencing FLI or targeting CD13/ANPEP lead to dephosphorylation of EPHA2, a mediator of BRAF inhibitor resistance, and induce growth arrest or apoptosis in melanoma cells

et al. 2017

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A majority of patients with BRAF-mutated metastatic melanoma respond to therapy with BRAF inhibitors (BRAFi), but relapses are common owing to acquired resistance. To unravel BRAFi resistance mechanisms we have performed gene expression and mass spectrometry based proteome profiling of the sensitive parental A375 BRAF V600E-mutated human melanoma cell line and of daughter cell lines with induced BRAFi resistance. Increased expression of two novel resistance candidates, aminopeptidase-N (CD13/ANPEP) and ETS transcription factor FLI1 was observed in the BRAFi-resistant daughter cell lines. In addition, increased levels of the previously reported resistance mediators, receptor tyrosine kinase ephrine receptor A2 (EPHA2) and the hepatocyte growth factor receptor MET were also identified. The expression of these proteins was assessed in matched tumor samples from melanoma patients obtained before BRAFi and after disease progression. MET was overexpressed in all progression samples while the expression of the other candidates varied between the individual patients. Targeting CD13/ANPEP by a blocking antibody induced apoptosis in both parental A375- and BRAFi-resistant daughter cells as well as in melanoma cells with intrinsic BRAFi resistance and led to dephosphorylation of EPHA2 on S897, previously demonstrated to cause inhibition of the migratory capacity. AKT and RSK, both reported to induce EPHA2 S897 phosphorylation, were also dephosphorylated after inhibition of CD13/ANPEP. FLI1 silencing also caused decreases in EPHA2 S897 phosphorylation and in total MET protein expression. In addition, silencing of FLI1 sensitized the resistant cells to BRAFi. Furthermore, we show that BRAFi in combination with the multi kinase inhibitor dasatinib can abrogate BRAFi resistance and decrease both EPHA2 S897 phosphorylation and total FLI1 protein expression. This is the first report presenting CD13/ANPEP and FLI1 as important mediators of resistance to BRAF inhibition with potential as drug targets in BRAFi refractory melanoma.

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“…4,5,32,[47][48][49] In our previous studies, treatment of NCCIT cells with RA was found to repress the expression of OCT4 and induces differentiation. 33,34,37,38 Therefore, this study demonstrates that GCNF expression transiently increased to the highest at day 2 and then dropped down afterward throughout the period of RA treatment for 10 days, whereas OCT4 expression gradually decreased upon RA treatment in NCCIT cells (Figure 1). We further confirmed that OCT4 expression is reduced by GCNF overexpression and induced by GCNF shRNA (Figure 2), suggesting that the level of OCT4 expression is dependent on GCNF expression.…”

Section: Discussionmentioning

confidence: 55%

“…We also used the pGL3-ti minimal promoter (an adenovirus major late promoter TATA box and mouse terminal deoxynucleotidyl transferase gene initiator sequence, 35 reporter construct containing the OCT4 promoter conserved region 2 (CR2-ti-Luc) and mutants (CR2-ti-Luc [second binding site mutant, M6], CR2-ti-Luc [third binding site mutant, M7], CR2-ti-Luc [second & third binding site mutant, M8]), which have been described previously. 33,34,[36][37][38] Full-length human GCNF complementary cDNA (cDNA) was obtained from the PCR amplification of NCCIT cells and inserted into Flag-tagged pcDNA3.1+ vector. Target sequence for human GCNF RNA interference was obtained from the previous report.…”

Section: Cell Culture and Differentiationmentioning

confidence: 99%

“…Chromatin immunoprecipitation (ChIP) assay was performed as described previously 37,38 with a minor modification using the chromatin DNA purified from NCCIT cells differentiated by RA treatment for 2 days. Lysate was precleared using protein G-agarose beads (Santa Cruz Biotechnology) and incubated with mouse monoclonal antibody against GCNF (Santa Cruz Biotechnology) or normal mouse IgG antibody (Santa Cruz Biotechnology).…”

Section: Chromatin Immunoprecipitation Analysismentioning

confidence: 99%

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GCNF regulates OCT4 expression through its interactions with nuclear receptor binding elements in NCCIT cells

Park

Choi

et al. 2017

J of Cellular Biochemistry

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We demonstrate that OCT4 expression is regulated by germ cell nuclear factor (GCNF) via its interactions with three nuclear receptor (NR) binding sites within OCT4 promoter conserved regions (CRs) in human embryonic carcinoma (EC) NCCIT cells. OCT4 expression is gradually reduced during the retinoic acid-induced differentiation, while GCNF temporarily increased after 2 days and then significantly decreased. In addition, OCT4 expression is significantly reduced by overexpression of exogenous GCNF, but increased by GCNF shRNA-mediated knockdown. The transcriptional activity of OCT4 is significantly inhibited by dose-dependent overexpression of GCNF. While mutants at each of the NR binding sites retain the repressive effects of GCNF on OCT4 promoter activity, the repressive effect was completely eliminated in the reporter construct with all binding sites mutated even in the presence of GCNF. Furthermore, the transcriptional activity of native minimal promoter (CR1-Luc) containing the first NR binding site was significantly reduced by GCNF overexpression, while the mutant retained basal activity to some extent. Next, an exogenous minimal ti promoter-inserted CR2 reporter construct containing the second and third NR binding sites (CR2-ti-Luc) was co-transfected with GCNF expression vector. The transcriptional activity of CR2-ti-Luc was significantly decreased by GCNF overexpression, while mutation of both binding sites retained the transcriptional activity of the reporter construct. Binding assays confirmed the direct interaction of GCNF with all three NR binding sites cooperatively. Taken together, GCNF acts as a transcriptional repressor in the regulation of OCT4 gene expression through cooperative interaction with three NR binding elements in pluripotent NCCIT cells.

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Differential Expression of ETS Family Transcription Factors in NCCIT Human Embryonic Carcinoma Cells upon Retinoic Acid-Induced Differentiation

Cited by 8 publications

References 40 publications

Growth and Differentiation Factor 3 Is Transcriptionally Regulated by OCT4 in Human Embryonic Carcinoma Cells

Growth and Differentiation Factor 3 Is Transcriptionally Regulated by OCT4 in Human Embryonic Carcinoma Cells

Silencing FLI or targeting CD13/ANPEP lead to dephosphorylation of EPHA2, a mediator of BRAF inhibitor resistance, and induce growth arrest or apoptosis in melanoma cells

GCNF regulates OCT4 expression through its interactions with nuclear receptor binding elements in NCCIT cells

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