Restoration of DNA‐binding and growth‐suppressive activity of mutant forms of p53 via a PCAF‐mediated acetylation pathway

Perez, Ricardo E.; Knights, Chad D.; Sahu, Geetaram; Catania, Jason; Kolukula, Vamsi Krishna; Stoler, Daniel L.; Graessmann, A.; Ogryzko, Vasily; Pishvaian, Michael J.; Albanese, Christopher; Avantaggiati, Maria Laura

doi:10.1002/jcp.22285

Cited by 36 publications

(40 citation statements)

References 55 publications

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“…4). This result, while unexpected, is not unparalleled, as a number of studies have shown that mutant p53 protein is capable of binding to its target gene sequences and regulating their expression (Pan and Haines, 2000;O'Farrell et al, 2004;Weisz et al, 2007;Chandrachud and Gal, 2009;Perez et al, 2010;Rasti et al, 2012). Since the mutant p53 did not associate with the 14-3-3s promoter in the absence of plakoglobin (SCC9 cells), this suggests a role for plakoglobin in associating p53 with its target gene promoter(s).…”

Section: Discussionmentioning

confidence: 84%

Plakoglobin interacts with the transcription factor p53 and regulates the expression of 14-3-3σ

Aktary

Kulak

Mackey

et al. 2013

Journal of Cell Science

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SummaryPlakoglobin (c-catenin), a constituent of the adherens junction and desmosomes, has signaling capabilities typically associated with tumor/metastasis suppression through mechanisms that remain undefined. To determine the role of plakoglobin during tumorigenesis and metastasis, we expressed plakoglobin in human tongue squamous cell carcinoma (SCC9) cells and compared the mRNA profiles of parental SCC9 cells and their plakoglobin-expressing transfectants (SCC9-PG). We detected several p53-target genes whose levels were altered upon plakoglobin expression. In this study, we identified the p53 regulated tumor suppressor 14-3-3s as a direct plakoglobin-p53 target gene. Coimmunoprecipitation experiments revealed that plakoglobin and p53 interact, and chromatin immunoprecipitation and electrophoretic mobility shift assays revealed that plakoglobin and p53 associate with the 14-3-3s promoter. Furthermore, luciferase reporter assays showed that p53 transcriptional activity is increased in the presence of plakoglobin. Finally, knockdown of plakoglobin in MCF-7 cells followed by luciferase assays confirmed that p53 transcriptional activity is enhanced in the presence of plakoglobin. Our data suggest that plakoglobin regulates gene expression in conjunction with p53 and that plakoglobin may regulate p53 transcriptional activity, which may account, in part, for the tumor/metastasis suppressor activity of plakoglobin.

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Section: Discussionmentioning

confidence: 84%

Plakoglobin interacts with the transcription factor p53 and regulates the expression of 14-3-3σ

Aktary

Kulak

Mackey

et al. 2013

Journal of Cell Science

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“…The expression of p53R175H, p53G281D or p53G245A in the p53 null H1299 cell lines increased the levels of endogenous CIC protein compared to naive H1299 cells (Figure 2AB), while wild-type p53 did not (Figure 2A, lane 2). In isogenic murine mammary breast cancer cell lines either lacking p53, harboring a wild-type gene or carrying the p53G242A codon (equivalent to the human G245A mutation) [24-26], high CIC levels were seen in cells expressing mutant but not wild-type p53 (Figure 2C). Additionally, down-regulation of p53R280K or p53R273H in MDA-231 or MDA-468 cells, respectively, with the previously described specific p53shRNA [9,24] reduced the levels of endogenous CIC (Figure 2DE).…”

Section: Resultsmentioning

confidence: 99%

SLC25A1, or CIC, is a novel transcriptional target of mutant p53 and a negative tumor prognostic marker

et al. 2014

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Mutations of the p53 gene hallmark many human cancers. Several p53 mutant proteins acquire the capability to promote cancer progression and metastasis, a phenomenon defined as Gain of Oncogenic Function (GOF). The downstream targets by which GOF p53 mutants perturb cellular programs relevant to oncogenesis are only partially known. We have previously demonstrated that SLC25A1 (CIC) promotes tumorigenesis, while its inhibition blunts tumor growth. We now report that CIC is a direct transcriptional target of several p53 mutants. We identify a novel interaction between mutant p53 (mutp53) and the transcription factor FOXO-1 which is responsible for regulation of CIC expression levels. Tumor cells harboring mutp53 display higher CIC levels relative to p53 null or wild-type tumors, and inhibition of CIC activity blunts mutp53-driven tumor growth, partially overcoming GOF activity. CIC inhibition also enhances the chemotherapeutic potential of platinum-based agents. Finally, we found that elevated CIC levels predict poor survival outcome in tumors hallmarked by high frequency of p53 mutations. Our results identify CIC as a novel target of mutp53 and imply that the employment of CIC inhibitors may improve survival rates and reduce chemo-resistance in tumors harboring these types of mutations, which are among the most intractable forms of cancers.

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“…Previously, acetylation of the mutant p53 has been found to restore the DNA binding ability and the growth suppression function. 44 Since p53 methylation at K372 promotes its subsequent acetylation, 40,45 it is possible that KDM3A knockdown might reactivate mutant p53 by increasing p53 acetylation. Growing evidence suggests that breast CSCs are chemoresistant and highly invasive which might be associated with disease relapse.…”

Section: Discussionmentioning

confidence: 99%

Lysine demethylase KDM3A regulates breast cancer cell invasion and apoptosis by targeting histone and the non-histone protein p53

Sivakumar¹,

Guo²,

2016

Oncogene

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Invasive growth and apoptosis resistance of breast cancer cells are associated with metastasis and disease relapse. Here we identified that the lysine-specific demethylase KDM3A played a dual role in breast cancer cell invasion and apoptosis by demethylating histone and the non-histone protein p53, respectively. While inducing pro-invasive genes by erasing repressive histone H3 lysine 9 methylation, KDM3A promotes chemoresistance by demethylating p53. KDM3A suppressed pro-apoptotic functions of p53 by erasing p53-K372me1 as this methylation site is crucial for the stability of chromatin-bound p53. Unexpectedly, depletion of KDM3A was capable of reactivating mutated p53 to induce the expression of pro-apoptotic genes in breast cancer with mutant p53. Moreover, KDM3A knockdown also potently inhibited tumorigenic potentials of breast cancer stem-like cells and rendered them sensitive to apoptosis induced by chemotherapeutic drugs. Taken together, our results suggest that KDM3A might be a potential therapeutic target for human breast cancer treatment and prevention.

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Restoration of DNA‐binding and growth‐suppressive activity of mutant forms of p53 via a PCAF‐mediated acetylation pathway

Cited by 36 publications

References 55 publications

Plakoglobin interacts with the transcription factor p53 and regulates the expression of 14-3-3σ

Plakoglobin interacts with the transcription factor p53 and regulates the expression of 14-3-3σ

SLC25A1, or CIC, is a novel transcriptional target of mutant p53 and a negative tumor prognostic marker

Lysine demethylase KDM3A regulates breast cancer cell invasion and apoptosis by targeting histone and the non-histone protein p53

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