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HIF-1α promotes autophagic proteolysis of Dicer and enhances tumor metastasis
Hui-Huang Lai, … , Hiroshi I. Suzuki, Pai-Sheng Chen
Hui-Huang Lai, … , Hiroshi I. Suzuki, Pai-Sheng Chen
Published December 18, 2017
Citation Information: J Clin Invest. 2018;128(2):625-643. https://doi.org/10.1172/JCI89212.
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Research Article Cell biology

HIF-1α promotes autophagic proteolysis of Dicer and enhances tumor metastasis

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Abstract

HIF-1α, one of the most extensively studied oncogenes, is activated by a variety of microenvironmental factors. The resulting biological effects are thought to depend on its transcriptional activity. The RNAse enzyme Dicer is frequently downregulated in human cancers, which has been functionally linked to enhanced metastatic properties; however, current knowledge of the upstream mechanisms regulating Dicer is limited. In the present study, we identified Dicer as a HIF-1α–interacting protein in multiple types of cancer cell lines and different human tumors. HIF-1α downregulated Dicer expression by facilitating its ubiquitination by the E3 ligase Parkin, thereby enhancing autophagy-mediated degradation of Dicer, which further suppressed the maturation of known tumor suppressors, such as the microRNA let-7 and microRNA-200b. Consequently, expression of HIF-1α facilitated epithelial-mesenchymal transition (EMT) and metastasis in tumor-bearing mice. Thus, this study uncovered a connection between oncogenic HIF-1α and the tumor-suppressive Dicer. This function of HIF-1α is transcription independent and occurs through previously unrecognized protein interaction–mediated ubiquitination and autophagic proteolysis.

Authors

Hui-Huang Lai, Jie-Ning Li, Ming-Yang Wang, Hsin-Yi Huang, Carlo M. Croce, Hui-Lung Sun, Yu-Jhen Lyu, Jui-Wen Kang, Ching-Feng Chiu, Mien-Chie Hung, Hiroshi I. Suzuki, Pai-Sheng Chen

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Figure 9

HIF-1α–induced miR-200b suppression facilitates cancer metastasis.

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HIF-1α–induced miR-200b suppression facilitates cancer metastasis.
(A–C)...
(A–C) CT-26/Luc mouse colon cancer cells stably expressing WT or HLH-truncated HIF-1α were restored with miR-200b for metastasis animal experiments (A). After intrasplenic injection, tumor metastasis was monitored by in vivo images of mouse (A) liver and lung (B). (C) The photon intensities of the metastatic signals in the livers and lungs were calculated 18 days after intrasplenic injection (n = 7 per group). Data are presented as mean ± SD, with at least n = 3 per group. Multigroup comparisons were analyzed by 1-way ANOVA with Tukey’s post hoc test. *P < 0.05; **P < 0.01; ***P < 0.001.

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