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CRISPR-mediated promoter de/methylation technologies for gene regulation

Authors
Sung, Chang K.Yim, Hyungshin
Issue Date
Jul-2020
Publisher
PHARMACEUTICAL SOC KOREA
Keywords
Epigenetic regulation; DNA methyltransferase; DNA demethylase; CRISPR-dCas9
Citation
ARCHIVES OF PHARMACAL RESEARCH, v.43, no.7, pp 705 - 713
Pages
9
Indexed
SCIE
SCOPUS
KCI
Journal Title
ARCHIVES OF PHARMACAL RESEARCH
Volume
43
Number
7
Start Page
705
End Page
713
URI
https://scholarworks.bwise.kr/erica/handle/2021.sw.erica/1036
DOI
10.1007/s12272-020-01257-8
ISSN
0253-6269
1976-3786
Abstract
DNA methylation on cytosines of CpG dinucleotides is well established as a basis of epigenetic regulation in mammalian cells. Since aberrant regulation of DNA methylation in promoters of tumor suppressor genes or proto-oncogenes may contribute to the initiation and progression of various types of human cancer, sequence-specific methylation and demethylation technologies could have great clinical benefit. The CRISPR-Cas9 protein with a guide RNA can target DNA sequences regardless of the methylation status of the target site, making this system superb for precise methylation editing and gene regulation. Targeted methylation-editing technologies employing the dCas9 fusion proteins have been shown to be highly effective in gene regulation without altering the DNA sequence. In this review, we discuss epigenetic alterations in tumorigenesis as well as various dCas9 fusion technologies and their usages in site-specific methylation editing and gene regulation.
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