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J. Biol. Chem., Vol. 256, Issue 17, 8892-8895, Sep, 1981
R Sterner, G Vidali and VG Allfrey
Duck erythrocytes were incubated with [3H]acetate both in the presence and
absence of sodium butyrate. Subsequent perchloric acid extraction of the
nuclei, followed by selective acetone precipitation, CM-Sephadex ion
exchange chromatography, and gel filtration yielded radioactively labeled
high mobility group (HMG) proteins HMG-14 and HMG-17 in pure form.
Extensive enzymatic degradation of the proteins followed by amino acid
analysis of the digests yielded a significant amount of material eluting in
the position of epsilon-N-acetyllysine. Furthermore, automated Edman
degradation of intact 3H-labeled HMG-14 and HMG-17 identified the specific
sites of acetylation of these proteins. In both erythrocyte HMGs isolated
from cells not exposed to butyrate, the lysine residue at position 2 was
the only one found to be labeled. However, one additional site in HMG-14
and two additional sites in HMG- 17 were found in the proteins from cells
incubated in butyrate. Finally, studies of the enzymatic deacetylation of
HMG-14 and HMG-17 confirmed that both nuclear proteins serve as deacetylase
substrates and that butyrate inhibits their deacetylation, just as in the
case of other HMG proteins and nucleosomal core histones.
Studies of acetylation and deacetylation in high mobility group proteins. Identification of the sites of acetylation in high mobility group proteins 14 and 17
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