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Transcriptional Regulation

Reconstitution of Enhancer Function in Paternal Pronuclei of One-Cell Mouse Embryos

, , &
Pages 5531-5540 | Received 10 Nov 2000, Accepted 11 May 2001, Published online: 28 Mar 2023
 

Abstract

How chromatin-mediated transcription regulates the beginning of mammalian development is currently unknown. Factors responsible for promoter repression and enhancer-mediated relief of this repression are not present in the paternal pronuclei of one-cell mouse embryos but are present in the zygotic nuclei of two-cell embryos. Here we show that coinjection of purified histones and a plasmid-encoded reporter gene into the paternal pronuclei of one-cell embryos at a specific histone-DNA concentration could recreate the behavior observed in two-cell embryos: acquisition of promoter repression and subsequent relief of this repression either by functional enhancers or by histone deacetylase inhibitors. Furthermore, the extent of enhancer-mediated stimulation in one-cell embryos depended on the acetylation status of the injected histones, on the treatment of embryos with a histone deacetylase inhibitor, and on the developmentally regulated appearance of enhancer-specific coactivator activity. The coinjected plasmids in one-cell embryos also exhibited chromatin assembly, as determined by a supercoiling assay. Thus, injection of histones into one-cell embryos faithfully reproduced the chromatin-mediated transcription observed in two-cell embryos. These results suggest that the need for enhancers to stimulate promoters through relief of chromatin-mediated repression occurs once the parental genomes are organized into chromatin. Furthermore, we present a model mammalian system in which the role of individual histones, and particular domains within the histones that are targeted in enhancer function, can be examined using purified mutant histones.

ACKNOWLEDGMENTS

We regret that we could not cite many outstanding research articles because of space limitations and so cite only a few review articles. We are grateful to the two anonymous reviewers and to Mel DePamphilis, Jim Kadonaga, Richard Schultz, and Maureen Goode for their invaluable ideas and suggestions.

This work was supported in part by a grant to S.M. from the National Institutes of Health (GM53454). L.R. was supported by a Translational Research Award from the American Brain Tumor Association.

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