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Volume 271,
Number 20,
Issue of May 17, 1996 pp. 11852-11857
©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
Histones
Associated with Non-nucleosomal Rat Ribosomal Genes Are Acetylated
while Those Bound to Nucleosome-organized Gene Copies Are Not
(Received for publication, November 17, 1995; and in revised form, March 6, 1996)
Vesco J.
Mutskov,
Valya
R.
Russanova ,
Stefan I.
Dimitrov ,
Iliya G.
Pashev
Acetylation of histones bound to rat rRNA genes has been studied
relative to their organization in chromatin, either as canonical
nucleosomes, containing the inactive copies, or as anucleosomal
nonrepeating structures, corresponding to the transcribed genes
(Conconi, A., Widmer, R. M., Koller, T., and Sogo, J. M.(1989) Cell 57, 753-761). Nuclei from butyrate-treated rat tumor cells
were irradiated with a UV laser to cross-link proteins to DNA, and the
purified covalent complexes were immunofractionated by an antibody that
specifically recognized the acetylated histones. Upon probing with
sequences coding for mature rat 28 S RNA, DNA of the antibody-bound
complexes was 5-20-fold enriched relative to the total rat DNA.
Since the laser cross-links histones to DNA in both active and inactive
genes, one cannot distinguish which one of them, or both, are bound to
acetylated histones. Alternatively, purified mononucleosomes were
immunofractionated, but DNA from the antibody-bound monosomes was not
enriched in coding rDNA. Taken together, these results suggest that
nucleosome-organized rRNA genes are bound to nonmodified histones and
that the acetylated histones are associated with the active,
anucleosomal gene copies.

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Copyright © 1996 by the American Society for Biochemistry and Molecular Biology.
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