Enigma negatively regulates p53 through MDM2 and promotes tumor cell survival in mice
Cho-Rok Jung, … , Seung-Moo Noh, Dong-Soo Im
Cho-Rok Jung, … , Seung-Moo Noh, Dong-Soo Im
Published November 8, 2010
Citation Information: J Clin Invest. 2010;120(12):4493-4506. https://doi.org/10.1172/JCI42674.
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Research Article Oncology

Enigma negatively regulates p53 through MDM2 and promotes tumor cell survival in mice

Abstract

The human E3 ubiquitin ligase murine double minute 2 (MDM2) targets the tumor suppressor p53 for ubiquitination and degradation but also promotes its own ubiquitination and subsequent degradation. As the balance between MDM2 and p53 levels plays a crucial role in regulating cell proliferation and apoptosis, we sought to identify factors selectively inhibiting MDM2 self-ubiquitination. Here we have shown that the LIM domain protein Enigma directly interacts with MDM2 to form a ternary complex with p53 in vitro and in human hepatoma and colon carcinoma cell lines and mouse embryonic fibroblasts. We found that Enigma elicited p53 degradation by inhibiting MDM2 self-ubiquitination and increasing its ubiquitin ligase activity toward p53 in cells. Moreover, mitogenic stimuli such as serum, FGF, and HGF increased Enigma transcription via induction of serum response factor (SRF), leading to MDM2 stabilization and subsequent p53 degradation. We observed similar results in the livers of mice treated with HGF. In humans, we found SRF and Enigma coexpressed with MDM2 but not p53 in several liver and stomach tumors. Finally, we showed that Enigma promoted cell survival and chemoresistance by suppressing p53-mediated apoptosis in both cell lines and a mouse xenograft model. Our findings suggest a role for Enigma in tumorigenesis and uncover a mechanism whereby mitogens attenuate p53 antiproliferative activity through an SRF/Enigma/MDM2 pathway.

Authors

Cho-Rok Jung, Jung Hwa Lim, Yoonjung Choi, Dae-Ghon Kim, Koo Jeong Kang, Seung-Moo Noh, Dong-Soo Im

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Figure 3

Enigma inhibits MDM2 self-ubiquitination and enhances MDM2-mediated ubiquitination of p53.

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Enigma inhibits MDM2 self-ubiquitination and enhances MDM2-mediated ubiq...
(A) We transfected HLK3 cells with His-Ub (5 μg), F-Enigma (0, 5, 10 μg), F-EniΔLIM3 (10 μg), siEnigma (10, 15 μg), or siControl (15 μg) vectors and treated them with 10 μM MG132 for 12 hours before analysis as indicated. (B) We performed an in vitro ubiquitination assay with GST-MDM2 (2 μg), GST-MDM2(C464A) (2 μg), Enigma (0.5, 1 μg), His-PCAF (1 μg), GST (2 μg). After assay, we analyzed the reaction mixtures as indicated. F-Ub, Flag-tagged Ub. (C) We transfected MEFs with or without F-PCAF (5 μg), HA-Enigma (2, 5 μg), GST-MDM2 (10 μg), GST-MDM2(C464A) (10 μg), or GST (10 μg) vectors and prepared cell lysates at 48 hours after transfection before IB as indicated. (D) We performed an in vitro ubiquitination assay with His-MDM2 (2 μg), Enigma (0.5, 1 μg), EniΔLIM3 (1 μg), GST-p53 (1 μg), or GST (1 μg) and analyzed the reaction mixtures as indicated. Protein components in B and D were purified from bacteria. Molecular size markers are indicated at the left in A, B, and D.