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j.ultramic.2009.03.014.pdf | 633.87 kB | Adobe PDF | 見る/開く |
タイトル: | Removal of histone tails from nucleosome dissects the physical mechanisms of salt-induced aggregation, linker histone H1-induced compaction, and 30-nm fiber formation of the nucleosome array |
著者: | Hizume, Kohji Nakai, Tonau Araki, Sumiko Prieto, Eloise Yoshikawa, Kenichi Takeyasu, Kunio |
著者名の別形: | 日詰, 光治 竹安, 邦夫 |
キーワード: | Atomic force microscopy Chromatin Electron microscopy Histone tail Nucleosome Scanning tunneling and atomic force microscopy |
発行日: | Jul-2009 |
出版者: | Elsevier |
誌名: | Ultramicroscopy |
巻: | 109 |
号: | 8 |
開始ページ: | 868 |
終了ページ: | 873 |
抄録: | In order to reveal the roles of histone tails in the formation of higher-order chromatin structures, we employed atomic force microscopy (AFM), and an in vitro reconstitution system to examine the properties of reconstituted chromatin composed of tail-less histones and a long DNA (106-kb plasmid) template. The tail-less nucleosomes did not aggregate at high salt concentrations or with an excess amount of core histones, in contrast with the behavior of nucleosomal arrays composed of nucleosomes containing normal, N-terminal tails. Analysis of our nucleosome distributions reveals that the attractive interaction between tail-less nucleosomes is weakened. Addition of linker histone H1 into the tail-less nucleosomal array failed to promote the formation of 30 nm chromatin fibers that are usually formed in the normal nucleosomal array. These results demonstrate that the attractive interaction between nucleosomes via histone tails plays a critical role in the formation of the uniform 30-nm chromatin fiber. |
著作権等: | c 2009 Elsevier B.V. All rights reserved. この論文は出版社版でありません。引用の際には出版社版をご確認ご利用ください。 This is not the published version. Please cite only the published version. |
URI: | http://hdl.handle.net/2433/84728 |
DOI(出版社版): | 10.1016/j.ultramic.2009.03.014 |
PubMed ID: | 19328628 |
出現コレクション: | 学術雑誌掲載論文等 |
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