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Activation of the chicken Ig-beta locus by the collaboration of scattered regulatory regions through changes in chromatin structure.


ABSTRACT: A total of 10 B-lymphocyte-specific DNase I hypersensitive sites located in the chicken Ig-beta locus were divided into four regions and combinations of deletions of these regions were carried out. A decrease in transcription of the Ig-beta gene to <3% was demonstrated in cells with deletions in all four regions. The Ig-beta chromatin was resistant to DNase I digestion in these cells. Thus, the collaboration is shown to convert the Ig-beta chromatin from the condensed state to a relaxed state. H3 and H4 acetylation decreased to <8% but H3K4 hypermethylation was observed at the Ig-beta promoter and exon 3. The collaboration of four regions had virtually no effect on CG hypomethylation in the region upstream the transcriptional start site. Accordingly, neither the DNase I general sensitive state in the Ig-beta chromatin nor hyperacetylation of H3 and H4 histones in the promoter proximal region causes H3K4 di-methylation or CG hypomethylation in the promoter. From these analyses, a chromatin situation was found in which both an active state, such as enhanced H3K4 methylation, or CG hypomethylation, and an inactive state, such as DNase I resistance in the Ig-beta chromatin or hypoacetylation of H3 and H4 histones in the Ig-beta locus, coexist.

SUBMITTER: Shimada N 

PROVIDER: S-EPMC1540724 | biostudies-literature | 2006

REPOSITORIES: biostudies-literature

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Activation of the chicken Ig-beta locus by the collaboration of scattered regulatory regions through changes in chromatin structure.

Shimada Naoko N   Matsudo Hiroki H   Osano Kyoichi K   Arakawa Hiroshi H   Buerstedde Jean-Marie JM   Matsumoto Yasuyuki Y   Chayahara Kozue K   Torihata Atsushi A   Ono Masao M  

Nucleic acids research 20060811 13


A total of 10 B-lymphocyte-specific DNase I hypersensitive sites located in the chicken Ig-beta locus were divided into four regions and combinations of deletions of these regions were carried out. A decrease in transcription of the Ig-beta gene to <3% was demonstrated in cells with deletions in all four regions. The Ig-beta chromatin was resistant to DNase I digestion in these cells. Thus, the collaboration is shown to convert the Ig-beta chromatin from the condensed state to a relaxed state. H  ...[more]

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