The UBE2C/CDH1/DEPTOR axis is an oncogene and tumor suppressor cascade in lung cancer cells
Shizhen Zhang, … , Xiufang Xiong, Yi Sun
Shizhen Zhang, … , Xiufang Xiong, Yi Sun
Published December 22, 2022
Citation Information: J Clin Invest. 2023;133(4):e162434. https://doi.org/10.1172/JCI162434.
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Research Article Cell biology Oncology

The UBE2C/CDH1/DEPTOR axis is an oncogene and tumor suppressor cascade in lung cancer cells

Abstract

Ubiquitin-conjugating enzyme E2C (UBE2C) mediates ubiquitylation chain formation via the K11 linkage. While previous in vitro studies showed that UBE2C plays a growth-promoting role in cancer cell lines, the underlying mechanism remains elusive. Still unknown is whether and how UBE2C plays a promoting role in vivo. Here we report that UBE2C was indeed essential for growth and survival of lung cancer cells harboring Kras mutations, and UBE2C was required for KrasG12D-induced lung tumorigenesis, since Ube2c deletion significantly inhibited tumor formation and extended the lifespan of mice. Mechanistically, KrasG12D induced expression of UBE2C, which coupled with APC/CCDH1 E3 ligase to promote ubiquitylation and degradation of DEPTOR, leading to activation of mTORC signaling. Importantly, DEPTOR levels fluctuated during cell cycle progression in a manner dependent on UBE2C and CDH1, indicating their physiological connection. Finally, Deptor deletion fully rescued the tumor inhibitory effect of Ube2c deletion in the KrasG12D lung tumor model, indicating a causal role of Deptor. Taken together, our study shows that the UBE2C/CDH1/DEPTOR axis forms an oncogene and tumor suppressor cascade that regulates cell cycle progression and autophagy and validates UBE2C an attractive target for lung cancer associated with Kras mutations.

Authors

Shizhen Zhang, Xiahong You, Yawen Zheng, Yanwen Shen, Xiufang Xiong, Yi Sun

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Figure 6

DEPTOR knockdown rescues the phenotypes induced by UBE2C knockdown in lung cancer cells.

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DEPTOR knockdown rescues the phenotypes induced by UBE2C knockdown in l...
(A and B) A427 (A) and H1792 (B) cells were transfected with indicated siRNAs for 24 hours; one portion of cells was analyzed by IB (inset), and the other portion was seeded in 96-well plates with medium containing 2% FBS in triplicate and analyzed by CCK-8 cell proliferation assay on the indicated days. (C) A427 and H1792 cells were transfected with the indicated siRNAs for 24 hours, followed by clonogenic survival assay. A representative dish from each indicated group was photographed (left) and colonies were counted and are shown as mean ± SEM (n = 3) (right). (D) H1792 and A427 cells were transfected with indicated siRNAs for 48 hours, followed by IB with indicated antibodies. (E) Knockdown of UBE2C or CDH1 induced autophagy, which was rescued by DEPTOR knockdown. H358 cell were transfected with indicated siRNAs for 48 hours and stained with the indicated Abs, followed by photography under a fluorescence microscope (left). Data are the mean ± SEM of 4 independent experiments (right). *P < 0.05; **P < 0.01 by 1-way ANOVA test (AC and E). Scale bar: 20 μm.