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High-performance capillary electrophoresis of core histones and their acetylated modified derivatives.

机译:核心组蛋白及其乙酰化修饰衍生物的高效毛细管电泳。

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摘要

By using high-performance capillary electrophoresis, we have successfully separated rat liver core histones into several subfractions. Inconvenient interactions of the highly basic proteins with the capillary wall were eliminated by a phosphate buffer system containing 0.03% hydroxyprophylmethylcellulose. Sample amounts of a few nanolitres were analysed within about 20 min. Multiacetylated histones H4 and H3 from induced Friend erythroleukaemic cells prepurified by h.p.l.c. were clearly separated into their non-acetylated and distinct acetylated forms. Our results illustrate that the application of capillary zone electrophoresis on its own or in combination with h.p.l.c. to the analysis of histones provides an important new alternative to traditional gel electrophoreses.
机译:通过使用高效毛细管电泳,我们已成功地将大鼠肝核心组蛋白分离为几个亚组分。高碱性蛋白与毛细管壁的不便相互作用通过包含0.03%羟丙基甲基纤维素的磷酸盐缓冲系统消除了。在约20分钟内分析了几纳升的样品量。来自经h.p.l.c.预纯化的诱导的Friend红白血病细胞的多乙酰化组蛋白H4和H3。清楚地分为非乙酰化和独特的乙酰化形式。我们的结果表明,毛细管区带电泳本身或与h.p.l.c结合使用。对组蛋白的分析为传统的凝胶电泳提供了重要的新选择。

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