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组蛋白H1的超(ADP-核糖基)化

Hyper(ADP-ribosyl)ation of histone H1.

作者信息

Aubin R J, Dam V T, Miclette J, Brousseau Y, Huletsky A, Poirier G G

出版信息

Can J Biochem. 1982 Dec;60(12):1085-94. doi: 10.1139/o82-139.

DOI:10.1139/o82-139
PMID:6299482
Abstract

Nucleosomal chains of various repeat unit lengths were generated by a mild micrococcal nuclease digestion of purified pancreatic nuclei. Maximal nucleosome associated poly(ADP-ribose) polymerase activity was recovered in trimeric to tetrameric chromatin fragments, after which the enzyme activity gradually decreased and stabilized towards oligomeric periodicities of 11 to 16 nucleosomes. Electrophoresis of [32P]ADP-ribosylated histones on first-dimension acid-urea or acid-urea-Triton gels and on second-dimension acid--urea--cetyltriammonium bromide gels revealed that, of all histones, only histone H1 could be significantly poly(ADP-ribosyl)ated while only minimal modification could be recovered with histone H1(0). Furthermore, the extent of ADP-ribosylation present on pancreatic histone H1 is shown to proportionally retard this protein's electrophoretic mobility in all gel systems and to consist of a distinct series of at least 12 modification intermediates which can be evidenced, in nuclei or nucleosomes, and fully recovered along with histone H1 upon its selective extraction with 5% perchloric acid. The generation of these increasingly ADP-ribosylated forms of histone H1 is also demonstrated to be time dependent and the more complex ADP-ribosylated forms of this histone are favored at high NAD+ concentrations. Moreover, the electrophoretic mobilities of all intermediates are unaffected by the presence of the nonionic detergent Triton X-100.

摘要

通过用温和的微球菌核酸酶消化纯化的胰腺细胞核,生成了具有不同重复单元长度的核小体链。在三聚体到四聚体染色质片段中回收了最大的核小体相关聚(ADP-核糖)聚合酶活性,此后酶活性逐渐降低,并朝着11至16个核小体的寡聚周期稳定下来。在一维酸-尿素或酸-尿素- Triton凝胶以及二维酸-尿素-十六烷基三甲基溴化铵凝胶上对[32P] ADP-核糖基化组蛋白进行电泳分析表明,在所有组蛋白中,只有组蛋白H1能被显著地聚(ADP-核糖基)化,而组蛋白H1(0)只能回收极少的修饰。此外,胰腺组蛋白H1上存在的ADP-核糖基化程度显示出在所有凝胶系统中按比例延迟该蛋白的电泳迁移率,并且由至少12种修饰中间体组成的独特系列,这些中间体在细胞核或核小体中可以得到证实,并且在用5%高氯酸选择性提取组蛋白H1时能与之一同完全回收。还证明了这些组蛋白H1的ADP-核糖基化形式的产生是时间依赖性的,并且在高NAD+浓度下更复杂的ADP-核糖基化形式的该组蛋白更受青睐。此外,所有中间体的电泳迁移率不受非离子去污剂Triton X-100存在的影响。

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