Demethylation of specific sites in the 5' region of the inactive X-linked human phosphoglycerate kinase gene correlates with the appearance of nuclease sensitivity and gene expression.

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Mol Cell Biol. 1988 November; 8(11): 4692-4699

Demethylation of specific sites in the 5' region of the inactive X-linked human phosphoglycerate kinase gene correlates with the appearance of nuclease sensitivity and gene expression.

R S Hansen, N A Ellis and S M Gartler

Department of Medicine, University of Washington, Seattle 98195.

ABSTRACT

X8/6T2, a hamster-human hybrid cell line which contains an inactivehuman X chromosome, was treated with 5-azacytidine and selectedfor derepression of hypoxanthine-guanine phosphoribosyltransferase.Clones were examined for coreactivation of the phosphoglyceratekinase gene (Pgk). Of 68 of these hybrids, approximately 20%expressed measurable human phosphoglycerate kinase (PGK) activity.A 600-base-pair region of the Pgk 5' CpG cluster was examinedfor the methylation status of eight CCGG sites (site 1 being5'-most) in a number of PGK-negative and PGK-positive cell lines.The inactive X chromosome is normally methylated at all eightsites, and this was also true for the majority of X8/6T2 cells.However, several PGK-negative hybrids were demethylated in thesite 3 to site 6 region. PGK activity correlated with demethylationat both sites 6 and 7. The data for PGK-positive and -negativehybrids indicate that demethylation at or near site 7 was necessaryfor reactivation of Pgk. Chromatin sensitivity to MspI digestionin the nuclei of male lymphoblastoid cells and several PGK-positiveand PGK-negative hybrids was examined. PGK-positive cell lineswere hypersensitive to digestion, while PGK-negative hybridswere resistant. Cleavage at sites 6 and 7 was observed in allPGK-positive cell lines at each MspI concentration examined.Sites 7 and 8 were less accessible to digestion than site 6.Cleavage in the site 2 to site 5 region was observable at thelowest MspI concentration. In most PGK-positive hybrids, a nonspecificendogenous nuclease detected the presence of a hypersensitiveregion spanning at least 450 base pairs, bounded at the 3' endnear HpaII site 6. Nuclease hypersensitivity appears to be relatedto promoter activity, because sites 7 and 8 are in transcribedregions of the gene. These data indicate that specific siteswithin the CpG cluster have a dominant controlling influenceover the Pgk promoter conformation and the transcriptional activationof Pgk.

Mol Cell Biol. 1988 November; 8(11): 4692-4699

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