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High-resolution fractionation of nucleosomes: minor particles, 'whiskers,' and separation of mononucleosomes containing and lacking A24 semihistone

机译:核小体的高分辨率分级分离:细小颗粒,“须晶”和包含和缺乏A24半组蛋白的单核小体的分离

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摘要

Staphylococcal nuclease digests of HeLa chromatin fractionated on low ionic strength nucleoprotein gels have been further analyzed by second-dimension DNA and protein gel electrophoresis. In vivo radioactive labeling of chromatin components and use of longer gels allowed a higher sensitivity and resolution than has been previously reported for this approach. A number of nonhistone protein spots and about 20 DNA spots can be detected in the mononucleosomal region of the second-dimension gel. In particular, there are three DNA spots identical in DNA size that correspond to three discrete kinds of core mononucleosomes resolved on the first-dimension nucleoprotein gel. Analysis of protein composition shows that the most rapidly migrating particle contains all four core histones but no A24 semihistone (A24 is a covalent conjugate of histone H2A and a specific nonhistone protein, ubiquitin), whereas the other two core mononucleosomes contain A24 semihistone. Thus, one can now quantitatively separate the A24-lacking core mononucleosomes from those containing A24, making it possible to directly address the question of whether A24 is associated with nucleosomes containing a specific subset of DNA sequences. Additional features of two-dimensional nucleoprotein-DNA patterns are "whiskers," which run slower than core mononucleosomes in the nucleoprotein dimension and both faster and slower than core-length DNA in the DNA dimension. In more extensive digests, "secondary whiskers" are observed, which run faster than core mononucleosomes in both dimensions and appear to coincide with previously described subnucleosomal particles SN7 and SN8 [Bakayev, V., Bakayeva, T. & Varshavsky, A. (1977) Cell 11, 619-629]. Possible mechanisms of whisker formation are discussed.
机译:已通过二维DNA和蛋白质凝胶电泳进一步分析了在低离子强度核蛋白凝胶上分离的HeLa染色质的葡萄球菌核酸酶消化物。染色质组分的体内放射性标记和更长的凝胶的使用比以前报道的这种方法具有更高的灵敏度和分辨率。在第二维凝胶的单核小体区域中可以检测到许多非组蛋白蛋白斑点和大约20个DNA斑点。特别地,存在三个DNA大小相同的DNA斑点,它们对应于在第一维核蛋白凝胶上解析的三种离散种类的核心单核小体。蛋白质组成分析表明,迁移最快的颗粒包含所有四个核心组蛋白,但不含A24半组蛋白(A24是组蛋白H2A和特定的非组蛋白蛋白质泛素的共价缀合物),而其他两个核心单核小体则包含A24半组蛋白。因此,现在可以定量地将缺乏A24的核心单核小体与含有A24的核心单核小体分开,从而有可能直接解决A24是否与含有特定DNA序列子集的核小体相关的问题。二维核蛋白-DNA模式的其他特征是“晶须”,其在核蛋白维度上的运行速度比核心单核小体慢,而在DNA维度上的运行速度则慢于核心长度DNA。在更广泛的消化中,观察到“二级晶须”,在两个方面的运行速度都比核心单核小体快,并且似乎与先前描述的亚核小体颗粒SN7和SN8一致[Bakayev,V.,Bakayeva,T.&Varshavsky,A.(1977)。 (Cell 11,619-629)。讨论了晶须形成的可能机制。

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