miR-107 promotes tumor progression by targeting the let-7 microRNA in mice and humans
Pai-Sheng Chen, … , Pan-Chyr Yang, Min-Liang Kuo
Pai-Sheng Chen, … , Pan-Chyr Yang, Min-Liang Kuo
Published August 15, 2011
Citation Information: J Clin Invest. 2011;121(9):3442-3455. https://doi.org/10.1172/JCI45390.
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Research Article

miR-107 promotes tumor progression by targeting the let-7 microRNA in mice and humans

Abstract

MicroRNAs (miRNAs) influence many biological processes, including cancer. They do so by posttranscriptionally repressing target mRNAs to which they have sequence complementarity. Although it has been postulated that miRNAs can regulate other miRNAs, this has never been shown experimentally to our knowledge. Here, we demonstrate that miR-107 negatively regulates the tumor suppressor miRNA let-7 via a direct interaction. miR-107 was found to be highly expressed in malignant tissue from patients with advanced breast cancer, and its expression was inversely correlated with let-7 expression in tumors and in cancer cell lines. Ectopic expression of miR-107 in human cancer cell lines led to destabilization of mature let-7, increased expression of let-7 targets, and increased malignant phenotypes. In contrast, depletion of endogenous miR-107 dramatically increased the stability of mature let-7 and led to downregulation of let-7 targets. Accordingly, miR-107 expression increased the tumorigenic and metastatic potential of a human breast cancer cell line in mice via inhibition of let-7 and upregulation of let-7 targets. By mutating individual sites within miR-107 and let-7, we found that miR-107 directly interacts with let-7 and that the internal loop of the let-7/miR-107 duplex is critical for repression of let-7 expression. Altogether, we have identified an oncogenic role for miR-107 and provide evidence of a transregulational interaction among miRNAs in human cancer development.

Authors

Pai-Sheng Chen, Jen-Liang Su, Shih-Ting Cha, Woan-Yuh Tarn, Ming-Yang Wang, Hsing-Chih Hsu, Ming-Tsan Lin, Chia-Yu Chu, Kuo-Tai Hua, Chiung-Nien Chen, Tsang-Chih Kuo, King-Jen Chang, Michael Hsiao, Yi-Wen Chang, Jin-Shing Chen, Pan-Chyr Yang, Min-Liang Kuo

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Figure 5

The internal loop of the miR-107–let-7 duplex is crucial for their activities.

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The internal loop of the miR-107–let-7 duplex is crucial for their activ...
(A) Duplex structures formed between mutant forms of miR-107 and let-7a (bottom). Design of mutated miR-107 constructs. The top panel shows the wild-type miR-107–let-7a duplex structure, which exhibits several mismatched regions; mutations in miR-107 eliminating those mismatches are indicated (M1–M6). (B and C) The internal loop is required for miR-107 to antagonize let-7 function. The effects of structure-based miR-107 mutants on lin-41 activity (B) and let-7a levels (C) were measured in T47D cells. Luciferase activity of wild-type lin-41 in the control group served as the reference (100%). (D) Effect of the mutant forms of miR-107 on NF1A suppression. The activity of NF1A, a known mRNA target of miR-107, was measured using a luciferase reporter assay. The wild type and mutant refer to the NF1A constructs used in the reporter assay. (E) Requirement of miR-107’s internal loop for in vitro tumorigenesis. The effect of miR-107M2 mutants on colony formation, as measured by AIG assays. Data are presented as mean ± SD.