Enhanced targeted DNA methylation of the CMV and endogenous promoters with dCas9-DNMT3A3L entails distinct subsequent histone modification changes in CHO cells

Nicolas Marx; Heena Dhiman; Valerie Schmieder; Catarina Martins Freire; Ly Ngoc Nguyen; Gerald Klanert; Nicole Borth

doi:10.1016/j.ymben.2021.04.014

Enhanced targeted DNA methylation of the CMV and endogenous promoters with dCas9-DNMT3A3L entails distinct subsequent histone modification changes in CHO cells

Metab Eng. 2021 Jul:66:268-282. doi: 10.1016/j.ymben.2021.04.014. Epub 2021 May 16.

Authors

Nicolas Marx¹, Heena Dhiman¹, Valerie Schmieder¹, Catarina Martins Freire², Ly Ngoc Nguyen¹, Gerald Klanert³, Nicole Borth⁴

Affiliations

¹ BOKU University of Natural Resources and Life Sciences, Vienna, Austria; Austrian Center for Industrial Biotechnology GmbH, Vienna, Austria.
² BOKU University of Natural Resources and Life Sciences, Vienna, Austria.
³ Austrian Center for Industrial Biotechnology GmbH, Vienna, Austria.
⁴ BOKU University of Natural Resources and Life Sciences, Vienna, Austria; Austrian Center for Industrial Biotechnology GmbH, Vienna, Austria. Electronic address: nicole.borth@boku.ac.at.

PMID: 33965614
DOI: 10.1016/j.ymben.2021.04.014

Abstract

With the emergence of new CRISPR/dCas9 tools that enable site specific modulation of DNA methylation and histone modifications, more detailed investigations of the contribution of epigenetic regulation to the precise phenotype of cells in culture, including recombinant production subclones, is now possible. These also allow a wide range of applications in metabolic engineering once the impact of such epigenetic modifications on the chromatin state is available. In this study, enhanced DNA methylation tools were targeted to a recombinant viral promoter (CMV), an endogenous promoter that is silenced in its native state in CHO cells, but had been reactivated previously (β-galactoside α-2,6-sialyltransferase 1) and an active endogenous promoter (α-1,6-fucosyltransferase), respectively. Comparative ChIP-analysis of histone modifications revealed a general loss of active promoter histone marks and the acquisition of distinct repressive heterochromatin marks after targeted methylation. On the other hand, targeted demethylation resulted in autologous acquisition of active promoter histone marks and loss of repressive heterochromatin marks. These data suggest that DNA methylation directs the removal or deposition of specific histone marks associated with either active, poised or silenced chromatin. Moreover, we show that de novo methylation of the CMV promoter results in reduced transgene expression in CHO cells. Although targeted DNA methylation is not efficient, the transgene is repressed, thus offering an explanation for seemingly conflicting reports about the source of CMV promoter instability in CHO cells. Importantly, modulation of epigenetic marks enables to nudge the cell into a specific gene expression pattern or phenotype, which is stabilized in the cell by autologous addition of further epigenetic marks. Such engineering strategies have the added advantage of being reversible and potentially tunable to not only turn on or off a targeted gene, but also to achieve the setting of a desirable expression level.

Keywords: CHO; CMV promoter; CRISPR/dCas9; DNA methylation; Epigenetic editing; Histone modifications.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
CHO Cells
Cricetinae
Cricetulus
Cytomegalovirus Infections*
DNA Methylation* / genetics
Epigenesis, Genetic / genetics
Histone Code / genetics