Negative Regulation of p53 Functions by Daxx and the Involvement of MDM2

Zhao, Lisa; Liu, Jilin; Sidhu, G. S.; Niu, Yuxin; Liu, Yue; Wang, Ruipeng; Liao, Daiqing

doi:10.1074/jbc.m406743200

Cited by 55 publications

(71 citation statements)

References 51 publications

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“…We then wished to assess whether p53-activating chemotherapeutical agents could relieve E1B-mediated repression. In keeping with published reports (26,35) 8). A similar pattern of p21 expression was also observed in cells treated with both TSA and 5-FU (lanes 10 -12 in Fig.…”

Section: E1b Represses P21 Expression In Glioblastoma Ln-229supporting

confidence: 77%

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Repression of p53-mediated Transcription by Adenovirus E1B 55-kDa Does Not Require Corepressor mSin3A and Histone Deacetylases

Zhao

Santiago

Liu³

2007

Journal of Biological Chemistry

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The Ad E1B 55-kDa protein (E1B) is a potent transcriptional repressor. In vitro biochemical studies revealed that direct p53-E1B interaction is essential for E1B to block p53-activated transcription and a corepressor may be involved. To understand how E1B represses p53-mediated transcription in vivo, we expressed E1B in several tumor cell lines that express wild type p53. Here we show that E1B strongly suppresses the expression of p53 target genes such as p21 and Puma-␣ in normal growth conditions or after cells were treated with p53-activating chemotherapeutic agents, suggesting that E1B-mediated gene repression is dominant and cannot be reversed via p53 activation. Interestingly, we found that E1B binds to corepressor mSin3A. Mutagenesis analysis indicated that the sequence motif "LHLLA" near the NH 2 terminus of E1B is responsible for mSin3A binding, and this motif is conserved among E1B proteins from different Ad serotypes. The conserved paired amphipathic helix domain 1 of mSin3A is critical for mSin3A-E1B interaction. Surprisingly, E1B mutants that cannot bind to mSin3A can still repress p53 target genes, indicating that it is not the corepressor required for E1B-mediated gene repression. In support of this notion, repression of p53 target genes by E1B is insensitive to HDAC inhibitor trichostatin A. We further show that both the NH 2 -and COOH-terminal domains of E1B are required for the repression function. Therefore, E1B employs a unique repression mechanism to block p53-mediated transcription.The p53 and pRb tumor suppressor pathways are inactivated in virtually all human cancers regardless of their etiology (1, 2). Understanding the precise molecular mechanisms of these pathways is at the center stage of current research efforts in cancer biology. Small DNA tumor viruses such as adenoviruses (Ad), 3 human papillomaviruses, and SV40 can transform cells and cause cancer (3, 4). Each of these viruses produces several proteins that disable both p53 and pRb tumor suppressor pathways in infected cells. Ad E1A proteins physically associate with pRb and release it from E2F transcription factors that activate expression of genes required for DNA replication and cell cycle progression. The Ad 1B region encodes two major proteins in two overlapping ORFs: E1B 55-and 19-kDa, both of which are required for efficient cell transformation. The E1B 19-kDa functions as an inhibitor of apoptosis by binding to proapoptotic proteins Bax and Bak (5), and E1B 55-kDa (hereafter called E1B) participates in transformation by inactivating the p53 pathway (6).Several functions of E1B contribute to the inhibition of p53. Apart from sequestration of p53 in the cytoplasm that blocks p53-mediated apoptosis (7), E1B can inhibit acetylation of p53 and disrupt the interaction between p53 and coactivator p300/ CBP-associated protein (8). Early studies clearly showed that the transcriptional repression function of E1B, but not p53-E1B interaction per se, is critical for Ad-mediated cell transformation (9, 10). These studies demonstrated t...

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Section: E1b Represses P21 Expression In Glioblastoma Ln-229supporting

confidence: 77%

“…The cells were then processed for dual-luciferase assays (Promega) 48 h after transfection. Firefly luciferase activity was normalized against sea pansy luciferase activity as described previously (26).…”

Section: Methodsmentioning

confidence: 99%

Repression of p53-mediated Transcription by Adenovirus E1B 55-kDa Does Not Require Corepressor mSin3A and Histone Deacetylases

Zhao

Santiago

Liu³

2007

Journal of Biological Chemistry

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“…In contrast, Daxx-␤ and Daxx-␥ lacking this domain displayed a strongly diminished interaction with p53. However, analogous to the reduced interaction with PML, the binding of Daxx-␤/-␥ to p53 was not totally absent which confirms prior observations that N-terminal parts of Daxx could be also implicated in p53 binding (19,20). This interaction (Daxx/p53) is accompanied with a recruitment of p53 to PODs, thereby corroborating recent reports that p53 co-localizes with PML in PODs and that Daxx display a co-localization pattern with p53 in subnuclear dot-like structures (19,28,29).…”

Section: Discussionsupporting

confidence: 75%

“…7B). This is consistent with recent observations that N-terminal parts of Daxx could also be implicated in binding to p53 (19,20). After co-expression of Daxx with empty GFP vector, which served as negative control, even with longer exposure no Daxx protein could be detected in the corresponding precipitate.…”

Section: Neither Daxx Nor Daxx-␤ or Daxx-␥ Is An Enhancer Of Cd95-medsupporting

confidence: 79%

Daxx-β and Daxx-γ, Two Novel Splice Variants of the Transcriptional Co-repressor Daxx

Wethkamp

Funke

Suschek³

et al. 2011

Journal of Biological Chemistry

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Daxx is involved in transcriptional control and apoptosis. It comprises several domains, including a regulatory C terminus that is responsible for the interaction with numerous proteins such as p53, promyelocytic leukemia protein (PML), and Hsp27. Here, we describe the identification and characterization of two novel variants of Daxx termed Daxx-␤ and Daxx-␥, which are generated by alternative splicing. Alternative splicing results in a truncated regulatory C terminus in both proteins. As a consequence, Daxx-␤ and Daxx-␥ show a markedly decreased affinity to PML, which in turn is associated with a different subnuclear localization of these proteins compared with Daxx. Although Daxx is localized mainly in PML-oncogenic domains (PODs) Daxx-␤ and Daxx-␥ display a distinct distribution pattern. Furthermore, Daxx-␤ and Daxx-␥ show a decreased affinity to p53 also due to the truncated C terminus. We provide evidence that the p53 recruitment into PODs is Daxx isoform-dependent. The decreased affinity of Daxx-␤/-␥ to p53 and PML results in a diffuse localization of p53 throughout the nucleus. In contrast to Daxx, Daxx-␤ and Daxx-␥ are unable to repress p53-mediated transcription. Therefore, alternative splicing of Daxx might indicate an additional level in the cellular apoptosis network.

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“…More recently, it was found that Daxx can modulate the function of mdm2 regulating therefore DNA damage-induced p53 activation. 12,13 The importance of Fas and FasL in lymphocyte homeostasis and peripheral tolerance is revealed by the identification of mutations in their genes in both mice and humans where both lymphoproliferation and autoimmunity are observed. 14 Mice deficient in FADD, caspase 8 or FLIP (through either a germline deficiency or an overexpression of a dominant-negative form (DN) form) do not develop such pathological features, but present an unexpected defect in T-cell activation.…”

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confidence: 99%

Requirement for Daxx in mature T-cell proliferation and activation

et al. 2006

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The protein Daxx promotes Fas-mediated cell death through activation of apoptosis signal-regulating kinase 1, leading to the activation of the MAPKs JNK and p38. Owing to the in utero lethality of daxx-deficient mice, the in vivo role of Daxx has been so far difficult to analyze. We have generated transgenic mice expressing a dominant-negative form of Daxx (Daxx-DN) in the T-cell lineage. We show that Daxx is recruited to the Fas receptor upon FasL engagement and that Daxx-DN expression protects activated T cells from Fas-induced cell death, by preventing the death-inducing signal complex to be properly formed. Normal lymphocyte development and homeostasis are nevertheless observed. Interestingly, we report that both in vitro and in vivo stimulation of Daxx-DN T-lymphocytes leads to increased proliferative T-cell responses. This increased proliferation is associated with a marked increase in tyrosine phosphorylation of LAT and ZAP70 as Daxx-DN favor their recruitment to the T-cell receptor (TCR) complex. These findings identify Daxx as a critical regulator of T-lymphocyte homeostasis by decreasing TCRinduced cell proliferation and by promoting Fas-mediated cell death.

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Negative Regulation of p53 Functions by Daxx and the Involvement of MDM2

Cited by 55 publications

References 51 publications

Repression of p53-mediated Transcription by Adenovirus E1B 55-kDa Does Not Require Corepressor mSin3A and Histone Deacetylases

Repression of p53-mediated Transcription by Adenovirus E1B 55-kDa Does Not Require Corepressor mSin3A and Histone Deacetylases

Daxx-β and Daxx-γ, Two Novel Splice Variants of the Transcriptional Co-repressor Daxx

Requirement for Daxx in mature T-cell proliferation and activation

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