N-Pyrenemaleimide, a fluorescent probe that specifically labels histone H3 of rat liver chromatin in situ, was used to monitor the accessibility of histone H3 in chromatin isolated from rat liver at different times during degeneration. At times of maximum DNA synthesis (18–24 h after hepatectomy), the accessibility of the probe was found to be markedly (40–50%) increased. This increase is abolished, however, by treatment of the chromatin fibres with high salt (2 M-NaCl) or detergent. Tryptophan fluorescence was also enhanced at points of maximum DNA synthesis, suggesting that some non-histone tryptophan-containing protein was being synthesized. The polarization of the labelled histone H3 is not markedly altered, suggesting that fibre aggregation or dissociation does not occur. Mononucleosomes extracted from sham-operated and hepatectomized animals did not exhibit any difference in binding to the probe. Also, analysis of the chromatin protein by electrophoresis on detergent- and acid/urea/ Triton-X-100-containing polyacrylamide gels showed no detectable difference in histone H3 : 1, H3 : 2 or H3 : 3 subclasses.
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March 1981
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Research Article|
March 01 1981
Conformational changes in rat liver chromatin after liver regeneration
Publisher: Portland Press Ltd
Online ISSN: 1470-8728
Print ISSN: 0264-6021
© 1981 London: The Biochemical Society
1981
Biochem J (1981) 193 (3): 671–678.
Citation
H Simpkins, L M Thompson, N Waldeck, D S Gross, D Mooney; Conformational changes in rat liver chromatin after liver regeneration. Biochem J 1 March 1981; 193 (3): 671–678. doi: https://doi.org/10.1042/bj1930671
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