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Details

Autor(en) / Beteiligte
Titel
In Vitro Binding of H1 Histone Subtypes to Nucleosomal Organized Mouse Mammary Tumor Virus Long Terminal Repeat Promotor
Ist Teil von
  • The Journal of biological chemistry, 1998-11, Vol.273 (48), p.32236-32243
Ort / Verlag
United States: Elsevier Inc
Erscheinungsjahr
1998
Quelle
MEDLINE
Beschreibungen/Notizen
  • The binding of all known linker histones, named H1a through H1e, including H10 and H1t, to a model chromatin complex based on a DNA fragment containing the mouse mammary tumor virus long terminal repeat promotor was systematically studied. As for the histone subtype H1b, we found a dissociation constant of 8–16 nm to a single mononucleosome (210 base pairs), whereas the binding constant of all other subtypes varied between 2 and 4 nm. Most of the H1 histones, namely H1a, H1c, H1d/e, and H10, completely aggregate polynucleosomes (1.3 kilobase pairs, 6 nucleosomes) at 270–360 nm, corresponding to a molar ratio of six to eight H1 molecules per reconstituted nucleosome. To form aggregates with the histones H1t and H1b, however, greater amounts of protein were required. Furthermore, our results show that specific types of in vivo phosphorylation of the linker histone tails influence both the binding to mononucleosomes and the aggregation of polynucleosomes. S phase-specific phosphorylation with one to three phosphate groups at specific sites in the C terminus influences neither the binding to a mononucleosome nor the aggregation of polynucleosomes. In contrast, highly phosphorylated H1 histones with four to five phosphate groups in the C and N termini reveal a very high binding affinity to a mononucleosome but a low chromatin aggregation capability. These findings suggest that specific S phase or mitotic phosphorylation sites act independently and have distinct functional roles.

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