Scientific Reports (Jul 2017)

Targeted DNA methylation in human cells using engineered dCas9-methyltransferases

  • Tina Xiong,
  • Glenna E. Meister,
  • Rachael E. Workman,
  • Nathaniel C. Kato,
  • Michael J. Spellberg,
  • Fulya Turker,
  • Winston Timp,
  • Marc Ostermeier,
  • Carl D. Novina

DOI
https://doi.org/10.1038/s41598-017-06757-0
Journal volume & issue
Vol. 7, no. 1
pp. 1 – 14

Abstract

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Abstract Mammalian genomes exhibit complex patterns of gene expression regulated, in part, by DNA methylation. The advent of engineered DNA methyltransferases (MTases) to target DNA methylation to specific sites in the genome will accelerate many areas of biological research. However, targeted MTases require clear design rules to direct site-specific DNA methylation and minimize the unintended effects of off-target DNA methylation. Here we report a targeted MTase composed of an artificially split CpG MTase (sMTase) with one fragment fused to a catalytically-inactive Cas9 (dCas9) that directs the functional assembly of sMTase fragments at the targeted CpG site. We precisely map RNA-programmed DNA methylation to targeted CpG sites as a function of distance and orientation from the protospacer adjacent motif (PAM). Expression of the dCas9-sMTase in mammalian cells led to predictable and efficient (up to ~70%) DNA methylation at targeted sites. Multiplexing sgRNAs enabled targeting methylation to multiple sites in a single promoter and to multiple sites in multiple promoters. This programmable de novo MTase tool might be used for studying mechanisms of initiation, spreading and inheritance of DNA methylation, and for therapeutic gene silencing.