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Transcriptional Regulation

The Dynamic Mobility of Histone H1 Is Regulated by Cyclin/CDK Phosphorylation

, , , , &
Pages 8626-8636 | Received 13 May 2003, Accepted 20 Aug 2003, Published online: 27 Mar 2023
 

Abstract

The linker histone H1 is involved in maintaining higher-order chromatin structures and displays dynamic nuclear mobility, which may be regulated by posttranslational modifications. To analyze the effect of H1 tail phosphorylation on the modulation of the histone's nuclear dynamics, we generated a mutant histone H1, referred to as M1-5, in which the five cyclin-dependent kinase phosphorylation consensus sites were mutated from serine or threonine residues into alanines. Cyclin E/CDK2 or cyclin A/CDK2 cannot phosphorylate the mutant in vitro. Using the technique of fluorescence recovery after photobleaching, we observed that the mobility of a green fluorescent protein (GFP)-M1-5 fusion protein is decreased compared to that of a GFP-wild-type H1 fusion protein. In addition, recovery of H1 correlated with CDK2 activity, as GFP-H1 mobility was decreased in cells with low CDK2 activity. Blocking the activity of CDK2 by p21 expression decreased the mobility of GFP-H1 but not that of GFP-M1-5. Finally, the level and rate of recovery of cyan fluorescent protein (CFP)-M1-5 were lower than those of CFP-H1 specifically in heterochromatic regions. These data suggest that CDK2 phosphorylates histone H1 in vivo, resulting in a more open chromatin structure by destabilizing H1-chromatin interactions.

ACKNOWLEDGMENTS

We thank D. Randy Garza and M. G. Mancini for technical assistance and J. W. Harper and M. Rijnkels for generously providing the adenovirus expressing p21 and β-Gal, respectively.

This work was supported by supplemental grant RO1-CA16303-27 from the Comprehensive Minority Biomedical Branch of the National Institutes of Health (J.M.R.) and by the American Cancer Society (R.E.H.).

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