Ultrastructure of transcriptionally competent chromatin

doi:10.1093/nar/18.23.7015

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Nucleic Acids Research, 1990, Vol. 18, No. 23 7015-7024
© 1990

Articles

Ultrastructure of transcriptionally competent chromatin

Lonzell Locklear, Jr, Andrew J. Ridsdale¹, David P. Bazett-Jones^* and James R. Davie¹

Department of Medical Biochemistry, The University of Calgary 3330 Hospital Drive NW, Calgary, Alberta T2N 4N1, Canada ¹Department of Biochemistry and Molecular Biology, University of Manitoba 770 Bannatyne Avenue, Winnipeg, Manitoba R3E 0W3, Canada

^* To whom correspondence should be addressed

Received July 26, 1990. Revised November 2, 1990. Accepted November 2, 1990.

We have examined a salt-soluble, transcriptionally competentgene-enriched fraction of chicken erythrocyte chromatin andcompared it to bulk chromatin using the unique mlcroanalyticalcapabilities of Electron Spectroscopic Imaging (ESI). The saltsoluble fraction is enriched 48 fold in (ß-globlngene sequences and is also enriched in histones that are post-syntheticallymodified, including acetylation and ubiquitination. Differencesbetween the two fractions are also apparent In the distributionof the two major forms of nucleoprotein structures, Including(1) particles which present a circular profile and possess proteinand DNA content nearly identical to that of the canonical nucleosomeand account for 89% of particles In the bulk fraction but accountfor only 66% of the particles in the competent fraction, and(2) u-shaped particles which possess about 20% less proteinmass than particles of circular profile and are about 10x moreprevalent In the transcriptionally competent fraction than inthe bulk. Additionally, elongated particles with protein andDNA content similar to the u-shaped objects are also seen inthe competent fraction.

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