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CRISPR-Cas knockout of miR21 reduces glioma growth


Citation

Nieland, Lisa and Solinge, Thomas S. van and Cheah, Pike See and Morsett, Liza M. and Khoury, Joseph El and Rissman, Joseph I. and Kleinstiver, Benjamin P. and Broekman, Marike L. D. and Breakefield, Xandra O. and Abels, Erik R. (2022) CRISPR-Cas knockout of miR21 reduces glioma growth. Molecular Therapy: Oncolytics, 25. 121 - 136. ISSN 2372-7705

Abstract

Non-coding RNAs, including microRNAs (miRNAs), support the progression of glioma. miR-21 is a small, non-coding transcript involved in regulating gene expression in multiple cellular pathways, including the regulation of proliferation. High expression of miR-21 has been shown to be a major driver of glioma growth. Manipulating the expression of miRNAs is a novel strategy in the development of therapeutics in cancer. In this study we aimed to target miR-21. Using CRISPR genome-editing technology, we disrupted the miR-21 coding sequences in glioma cells. Depletion of this miRNA resulted in the upregulation of many downstream miR-21 target mRNAs involved in proliferation. Phenotypically, CRISPR-edited glioma cells showed reduced migration, invasion, and proliferation in vitro. In immunocompetent mouse models, miR-21 knockout tumors showed reduced growth resulting in an increased overall survival. In summary, we show that by knocking out a key miRNA in glioma, these cells have decreased proliferation capacity both in vitro and in vivo. Overall, we identified miR-21 as a potential target for CRISPR-based therapeutics in glioma.


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Additional Metadata

Item Type: Article
Divisions: Faculty of Medicine and Health Science
DOI Number: https://doi.org/10.1016/j.omto.2022.04.001
Publisher: Cell Press
Keywords: Glioblastoma; CRISPR; Gene editing; MicroRNA; miR-21
Depositing User: Ms. Nur Faseha Mohd Kadim
Date Deposited: 22 Aug 2023 03:45
Last Modified: 22 Aug 2023 03:45
Altmetrics: http://www.altmetric.com/details.php?domain=psasir.upm.edu.my&doi=10.1016/j.omto.2022.04.001
URI: http://psasir.upm.edu.my/id/eprint/100836
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