doi: 10.1016/j.bcp.2016.08.009.
Epub 2016 Aug 9.
Epigenetic blockade of neoplastic transformation by bromodomain and extra-terminal (BET) domain protein inhibitor JQ-1
Affiliations
- PMID: 27520485
- PMCID: PMC5031540
- DOI: 10.1016/j.bcp.2016.08.009
Item in Clipboard
Epigenetic blockade of neoplastic transformation by bromodomain and extra-terminal (BET) domain protein inhibitor JQ-1
Biochem Pharmacol.
.
Abstract
The neoplastic transformation of cells and inflammation are processes that contribute to tumor initiation. Recently, emerging evidence has suggested that epigenetic alterations are also implicated in the early stages of carcinogenesis. Therefore, potent small molecules targeting epigenetic regulators have been developed as novel cancer therapeutic and preventive strategies. Bromodomain and extraterminal domain (BET) proteins are epigenetic readers that play key roles at the interface between chromatin modification and transcriptional regulation. In this study, we investigated the effect of the BET inhibitor JQ-1 on malignant transformation induced by 12-O-tetradecanoylphorbol-13-acetate (TPA) in mouse skin epidermal JB6 P+ cells. Treatment with JQ-1 effectively impaired TPA-induced colony formation in vitro. At the molecular level, the expression of several key TPA-induced pro-survival and pro-proliferative genes (Bcl2, Cyclin D1, and c-Myc) decreased rapidly after BET inhibition. In addition, JQ-1 treatment attenuated the activation of inflammatory NF-κB signaling triggered by TPA. Luciferase reporter assays using plasmids carrying different elements from the COX2 or IL6 promoters demonstrated that JQ-1 does not directly inhibit interactions between NF-κB and its binding sequence; rather, it affects CRE-element-associated transcriptional enhancement. Through siRNA gene silencing, we found that JQ-1 inhibits the p300-dependent transcriptional activation of COX2, which correlates with the results of the luciferase assay. Chromatin immunoprecipitation assays showed that TPA elevated H3K27Ac enrichment in the COX2 promoter region, which is mediated by p300, and Brd4. JQ-1 treatment did not change H3K27Ac levels but decreased the recruitment of Brd4 and RNA Polymerase II. Collectively, our study reveals that the BET inhibitor JQ-1 exerts potent anti-cancer and anti-inflammatory effects by interfering with the core transcriptional program of neoplastic transformation.
Keywords: Brd4; Bromodomain; JQ-1; NF-κB; Neoplastic transformation.
Copyright © 2016 Elsevier Inc. All rights reserved.
Conflict of interest statement
of potential conflicts of interest: No potential conflicts of interest were disclosed.
Figures
Cells were seeded in soft agar containing DMSO (vehicle control), 20ng/mL TPA or a combination of TPA and indicated concentration of JQ-1 in 6-well plates and were allowed to grow for 14 days. The colonies exhibiting anchorage-independent growth were imaged under a microscope, and the colony numbers were counted using ImageJ software. A) Representative images of each treatment group. B) Graphical data of colony numbers in each group are presented as the mean ± SD from three independent experiments. JB6 P+ cells in the vehicle control group rarely formed colonies in agar plate unless treated with TPA. JQ-1 significantly inhibited the TPA-induced anchorage independent growth of JB6 P+ cells. *P<0.05 and **P<0.01 indicate significant differences between the JQ-1-treated group and cells treated with TPA alone.
JB6 P+ or HaCaT cells were treated with the indicated concentrations of JQ-1 for 4 h, followed by 20 ng/ml TPA treatment. Cells were harvested 8 h post TPA treatment for RNA extraction and 24 h for protein sample preparation. A) JQ-1 attenuated the TPA-induced phosphorylation of ERK1/2 in JB6 P+ cells; band intensity of the blots were digitized and normalized to the vehicle control as fold change, presented as the mean ± SD in the right panel. B) JQ-1 treatment decreased the TPA-induced transcription of Cyclin D1 and c-Myc in JB6 P+ cells. C) Western blotting images of Bcl2, Cyclin D1, and c-Myc in JB6 P+ cells after JQ-1 treatment; right panel shows the bar graph of relative band intensity as the mean ± SD. D) JQ-1 treatment attenuated c-MYC mRNA levels in HaCaT cells. E) JQ-1 treatment decreased c-MYC and Bcl2 protein levels in HaCaT cells; right panel shows the bar graph of relative band intensity. *P<0.05, **P<0.01, and #P<0.001 indicate significant differences between the JQ-1-treated group and the cells treated with TPA alone.
HCT116 cells were treated with the indicated concentrations of JQ-1 for 24 h. A, B) JQ-1 suppressed cell cycle-related markers such as c-Myc and Cyclins A and D1 at both the mRNA and protein levels; relative mRNA expression or blot band intensity are presented as the mean ± SD; C) JQ-1 significantly induced G1 cell cycle arrest in HCT116 cells. Representative results from three independent experiments are provided in the upper panel whereas the lower panel shows the cell percentage in each phase as the mean ± SD. The statistical analyses were performed using one-way ANOVA with post-hoc Dunnett's test. *P<0.05, **P<0.01, and #P<0.001 indicate significant differences between the JQ-1-treated group and the vehicle control.
The protein expression of HDAC1–4 was determined by western blotting. The relative band intensity (fold change) was calculated by normalizing the intensity of each sample to the vehicle control. Representative bands are shown in the left panel, whereas the bar chart in the right panel presents the mean ± SD of three independent experiments. *P<0.05 indicates significant differences between the JQ-1-treated group and the vehicle control.
A) JQ-1 treatment decreased the TPA-induced transcription of IL6, uPAR, and COX2 in JB6 P+ cells. B) Western blot images of COX2 expression in JB6 P+ cells after JQ-1 treatment. C) JQ-1 treatment attenuated IL6 and COX2 mRNA levels in HaCaT cells. D) JQ-1 treatment decreased COX2 protein levels in HaCaT cells. *P<0.05, **P<0.01, and #P<0.001 indicate significant differences between the JQ-1-treated group and cells treated with TPA alone.
A) Different constructs of luciferase reporter genes. B) HaCaT cells were co-transfected with 400 ng of the designated pGL4.15 firefly luciferase reporters and 100 ng of pGL4.75 [hRluc/CMV] Renilla luciferase plasmids as an internal control. The transfected cells were treated with DMSO, 20 ng/ml TPA, 500 nM JQ-1, or the combination for 20 h. The firefly luciferase readings were normalized to the Renilla luciferase reading first; then, the fold changes were calculated by comparing each treatment group to the vehicle control. JQ-1 inhibits the luciferase activity in the cells transfected with the plasmids carrying CRE elements (#P<0.001). No significant changes were observed after JQ-1 treatment in the cells transfected with the plasmids carrying the NF-κB binding sequence alone.
ChIP assays were performed to analyze the enrichment of H3K27Ac, Brd4, and Pol II on the promoter or transcription start site of COX2 in JB6 P+ cells. The immunoprecipitated DNA was used as a template for qPCR and the enrichment was quantified as the proportion ratio of its self- input. Relative fold change was then calculated by normalizing the ratio to that of the vehicle control. *P<0.05 and **P<0.01 indicate significant differences between the TPA-treated group and the indicated groups.
JB6 P+ cells were transfected with siRNA against p300 or non-specific negative control, and the cells were then further treated with DMSO, 20 ng/ml TPA alone or 20 ng/ml TPA in combination with 500 nM JQ-1 for 24 h. ChIP assays were performed to examine the enrichment of H3K27Ac and Brd4 after TPA stimulation in the p300 or negative control siRNA treated cells. The mRNA and protein levels of COX2 were assessed respectively. A) TPA increased the Ac-H3K27 enrichment on COX2 gene promoter and Brd4 enrichment on TSS. Knock down of p300 attenuated these TPA induced alterations. B) The mRNA levels of p300 and COX2 were determined by quantitative PCR. C) Representative western blot images of p300 and COX2 protein levels. Transfection of p300 siRNA attenuated TPA-induced COX2 expression at both the mRNA and protein levels. JQ-1 treatment did not show further inhibitory effects after p300 knockdown.
Similar articles
-
Involvement of the antioxidative property of morusin in blocking phorbol ester-induced malignant transformation of JB6 P+ mouse epidermal cells.Chem Biol Interact. 2017 Feb 25;264:34-42. doi: 10.1016/j.cbi.2017.01.009. Epub 2017 Jan 17. Chem Biol Interact. 2017. PMID: 28108223
-
Disruption of BRD4 at H3K27Ac-enriched enhancer region correlates with decreased c-Myc expression in Merkel cell carcinoma.Epigenetics. 2015;10(6):460-6. doi: 10.1080/15592294.2015.1034416. Epub 2015 May 5. Epigenetics. 2015. PMID: 25941994 Free PMC article.
-
Bromodomain and extraterminal (BET) protein inhibition suppresses human T cell leukemia virus 1 (HTLV-1) Tax protein-mediated tumorigenesis by inhibiting nuclear factor κB (NF-κB) signaling.J Biol Chem. 2013 Dec 13;288(50):36094-105. doi: 10.1074/jbc.M113.485029. Epub 2013 Nov 4. J Biol Chem. 2013. PMID: 24189064 Free PMC article.
-
BET Bromodomain as a Target of Epigenetic Therapy.Chem Pharm Bull (Tokyo). 2016;64(6):540-7. doi: 10.1248/cpb.c16-00225. Chem Pharm Bull (Tokyo). 2016. PMID: 27250788 Review.
-
BET bromodomain inhibitors--a novel epigenetic approach in castration-resistant prostate cancer.Cancer Biol Ther. 2014;15(12):1583-5. doi: 10.4161/15384047.2014.962297. Cancer Biol Ther. 2014. PMID: 25535892 Free PMC article. Review.
Cited by
-
The BET family in immunity and disease.Signal Transduct Target Ther. 2021 Jan 19;6(1):23. doi: 10.1038/s41392-020-00384-4. Signal Transduct Target Ther. 2021. PMID: 33462181 Free PMC article. Review.
-
Epoxymicheliolide, a novelguaiane-type sesquiterpene lactone, inhibits NF‑κB/COX‑2 signaling pathways by targeting leucine 281 and leucine 25 in IKKβ in renal cell carcinoma.Int J Oncol. 2018 Sep;53(3):987-1000. doi: 10.3892/ijo.2018.4460. Epub 2018 Jun 29. Int J Oncol. 2018. PMID: 29956738 Free PMC article.
-
Chemoprevention of Preclinical Breast and Lung Cancer with the Bromodomain Inhibitor I-BET 762.Cancer Prev Res (Phila). 2018 Mar;11(3):143-156. doi: 10.1158/1940-6207.CAPR-17-0264. Epub 2017 Dec 15. Cancer Prev Res (Phila). 2018. PMID: 29246957 Free PMC article.
-
Combined inhibition of BET proteins and class I HDACs synergistically induces apoptosis in urothelial carcinoma cell lines.Clin Epigenetics. 2018 Jan 4;10:1. doi: 10.1186/s13148-017-0434-3. eCollection 2018. Clin Epigenetics. 2018. PMID: 29312470 Free PMC article.
-
Isoalantolactone inhibits IKKβ kinase activity to interrupt the NF-κB/COX-2-mediated signaling cascade and induces apoptosis regulated by the mitochondrial translocation of cofilin in glioblastoma.Cancer Med. 2019 Apr;8(4):1655-1670. doi: 10.1002/cam4.2013. Epub 2019 Feb 10. Cancer Med. 2019. PMID: 30740911 Free PMC article.
References
-
- Fujiwara K, Ghosh S, Liang P, Morien E, Soma M, Nagase H. Genome-wide screening of aberrant DNA methylation which associated with gene expression in mouse skin cancers. Molecular carcinogenesis. 2013 - PubMed
-
- Gambichler T, Sand M, Skrygan M. Loss of 5-hydroxymethylcytosine and ten-eleven translocation 2 protein expression in malignant melanoma. Melanoma research. 2013;23(3):218–20. - PubMed
-
- Ceol CJ, Houvras Y, Jane-Valbuena J, Bilodeau S, Orlando DA, Battisti V, Fritsch L, Lin WM, Hollmann TJ, Ferre F, Bourque C, Burke CJ, Turner L, Uong A, Johnson LA, Beroukhim R, Mermel CH, Loda M, Ait-Si-Ali S, Garraway LA, Young RA, Zon LI. The histone methyltransferase SETDB1 is recurrently amplified in melanoma and accelerates its onset. Nature. 2011;471(7339):513–7. - PMC - PubMed
Publication types
MeSH terms
Substances
Grants and funding
LinkOut - more resources
Full Text Sources
Other Literature Sources
Research Materials
Miscellaneous
