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活性染色质的结构:从大鼠肝脏中分离和鉴定转录活性染色质

Structure of active chromatin: isolation and characterization of transcriptionally active chromatin from rat liver.

作者信息

Tikoo K, Gupta S, Hamid Q A, Shah V, Chatterjee B, Ali Z

机构信息

Department of Biochemistry, Banaras Hindu University, Varanasi, India.

出版信息

Biochem J. 1997 Feb 15;322 ( Pt 1)(Pt 1):273-9. doi: 10.1042/bj3220273.

Abstract

Rat liver nuclei were isolated in low-ionic-strength buffer in the absence of bi- and multi-valent cations. Digestion of these nuclei by endogenous nuclease, micrococcal nuclease and DNase I revealed that a minor chromatin fraction was preferentially digested into poly- and oligo-nucleosomes. Southern blot hybridization with various active gene probes confirmed that these chromatin fragments represent coding and 5' upstream regions of transcriptionally active chromatin. Active chromatin fragments were released selectively into the medium, with inactive chromatin remaining inside the nuclei, under the above ionic conditions. The inclusion of bivalent cations during the digestion of nuclei reversed the solubility behaviour of active chromatin. Rearrangement and exchange of histone H1 between chromatin fragments was prevented by using low-salt conditions in all steps in the absence of bivalent cations. All histones, including H1, were present in stoichiometric amounts in this active chromatin fraction. Active nucleosomes showed a lower electrophoretic mobility than bulk nucleosomes in an acrylamide/agarose composite gel in the absence of Mg2+, but were selectively bound to the gel in the presence of this ion.

摘要

在不含二价和多价阳离子的低离子强度缓冲液中分离大鼠肝脏细胞核。用内源性核酸酶、微球菌核酸酶和DNase I消化这些细胞核后发现,一小部分染色质优先被消化成多核小体和寡核小体。用各种活性基因探针进行Southern印迹杂交证实,这些染色质片段代表转录活性染色质的编码区和5'上游区域。在上述离子条件下,活性染色质片段被选择性地释放到培养基中,而无活性染色质则保留在细胞核内。在细胞核消化过程中加入二价阳离子会逆转活性染色质的溶解性。在不存在二价阳离子的所有步骤中使用低盐条件可防止染色质片段之间组蛋白H1的重排和交换。在这个活性染色质组分中,所有组蛋白,包括H1,都以化学计量的量存在。在不存在Mg2+的情况下,活性核小体在丙烯酰胺/琼脂糖复合凝胶中的电泳迁移率低于整体核小体,但在该离子存在的情况下会选择性地结合到凝胶上。

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