| Literature DB >> 32369019 |
Taro Tsujimura1,2, Osamu Takase1,2, Masahiro Yoshikawa1,2, Etsuko Sano1,2, Matsuhiko Hayashi3, Kazuto Hoshi4,5, Tsuyoshi Takato4,5, Atsushi Toyoda6, Hideyuki Okano2, Keiichi Hishikawa1,2.
Abstract
While regulation of gene-enhancer interaction is intensively studied, its application remains limited. Here, we reconstituted arrays of CTCF-binding sites and devised a synthetic topological insulator with tetO for chromatin-engineering (STITCH). By coupling STITCH with tetR linked to the KRAB domain to induce heterochromatin and disable the insulation, we developed a drug-inducible system to control gene activation by enhancers. In human induced pluripotent stem cells, STITCH inserted between MYC and the enhancer down-regulated MYC. Progressive mutagenesis of STITCH led to a preferential escalation of the gene-enhancer interaction, corroborating the strong insulation ability of STITCH. STITCH also altered epigenetic states around MYC. Time-course analysis by drug induction uncovered deposition and removal of H3K27me3 repressive marks follows and reflects, but does not precede and determine, the expression change. Finally, STITCH inserted near NEUROG2 impaired the gene activation in differentiating neural progenitor cells. Thus, STITCH should be broadly useful for functional genetic studies.Entities:
Keywords: CTCF; MYC; chromatin conformation; chromosomes; enhancer; epigenetic manipulation; gene expression; genetics; genomics; human; mouse
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Year: 2020 PMID: 32369019 PMCID: PMC7200164 DOI: 10.7554/eLife.47980
Source DB: PubMed Journal: Elife ISSN: 2050-084X Impact factor: 8.140