4.7 Article

Targeting cancer epigenetics with CRISPR-dCAS9: Principles and prospects

Journal

METHODS
Volume 187, Issue -, Pages 77-91

Publisher

ACADEMIC PRESS INC ELSEVIER SCIENCE
DOI: 10.1016/j.ymeth.2020.04.006

Keywords

Cancer epigenetics; Epigenetic editing; CRISPR-dCas9; Off-target effect; sgRNA designing

Funding

  1. National Cancer Institute, United States [R01 CA178441, R01 CA204346]

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Cancer therapeutics is constantly evolving, with CRISPR-dCas9 emerging as a promising precision cancer treatment option that can modify cancer epigenetic features. Challenges such as off-target effects and lack of efficient delivery systems need to be addressed when targeting cancer with sgRNA-dCas9.
Cancer therapeutics is an ever-evolving field due to incessant demands for effective and precise treatment options. Over the last few decades, cancer treatment strategies have shifted somewhat from surgery to targeted precision medicine. CRISPR-dCas9 is an emerging version of precision cancer therapy that has been adapted from the prokaryotic CRISPR-Cas system. Once ligated to epigenetic effectors (EE), CRISPR-dCas9 can function as an epigenetic editing tool and CRISPR-dCas9-EE complexes could be exploited to alter cancerous epigenetic features associated with different cancer hallmarks. In this article, we discuss the rationale of epigenetic editing as a therapeutic strategy against cancer. We also outline how sgRNA-dCas9 was derived from the CRISPR-Cas system. In addition, the current status of sgRNA-dCas9 use (in vivo and in vitro) in cancer is updated with a molecular illustration of CRISPR-dCas9-mediated epigenetic and transcriptional modulation. As sgRNA-dCas9 is still at the developmental phase, challenges are inherent to its use. We evaluate major challenges in targeting cancer with sgRNA-dCas9 such as off-target effects, lack of sgRNA designing rubrics, target site selection dilemmas and deficient sgRNA-dCas9 delivery systems. Finally, we appraise the sgRNA-dCas9 as a prospective cancer therapeutic by summarizing ongoing improvements of sgRNA-dCas9 methodology.

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