Abstract
Although it is well established that the majority of eukaryotic DNA is sequestered as nucleosomes, the higher-order structure resulting from nucleosome interactions as well as the dynamics of nucleosome stability are not as well understood. To characterize the structural and functional contribution of individual nucleosomal sites, we have developed a chromatin model system containing up to four nucleosomes, where the array composition, saturation, and length can be varied via the ordered ligation of distinct mononucleosomes. Using this system we find that the ligated tetranucleosomal arrays undergo intra-array compaction. However, this compaction is less extensive than for longer arrays and is histone H4 tail-independent, suggesting that well ordered stretches of four or fewer nucleosomes do not fully compact to the 30-nm fiber. Like longer arrays, the tetranucleosomal arrays exhibit cooperative self-association to form species composed of many copies of the array. This propensity for self-association decreases when the fraction of nucleosomes lacking H4 tails is systematically increased. However, even tetranucleosomal arrays with only two octamers possessing H4 tails recapitulate most of the inter-array self-association. Varying array length shows that systems as short as dinucleosomes demonstrate significant self-association, confirming that relatively few determinants are required for inter-array interactions and suggesting that in vivo multiple interactions of short runs of nucleosomes might contribute to complex fiber-fiber interactions. Additionally, we find that the stability of nucleosomes toward octamer loss increases with array length and saturation, suggesting that in vivo stretches of ordered, saturated nucleosomes could serve to protect these regions from histone ejection.
Highlights
Intra-array Compaction— it was expected that the stability of an intra-array compacted tetranucleosomal array would be less than that for longer nucleosomal arrays, the strong propensity of 601 sequences for compaction as well as the precedent of a fully compacted
We found that ligated tetranucleosomal arrays do demonstrate intraarray compaction at 1.75 mM MgCl2 but exhibit less complete compaction than can be achieved for longer nucleosomal arrays and do so in a manner seemingly independent of the histone H4 tail
A possible interpretation is that chromatin compaction is
Summary
Nucleosomes can interact with one another, generating chromatin structures that affect DNA-based biological processes such as transcription, replication, and repair. The mechanism by which this repression is achieved is still not well defined in vivo, in vitro these proteins facilitate the creation of short and long range higher order chromatin structures through their interaction with various aspects of histone modifications, histone tails, the nucleosome core, and/or the linker DNA (14 –22). During transcriptional initiation, nucleosomes can be disassembled to generate stretches of DNA that are largely free of nucleosomes (24 –26). This disassembly process involves many factors, including nucleosome remodeling complexes, histone modifying enzymes, and histone chaperones [27]. In this study we ligate mononucleosomes to assemble well ordered di-, tri, and tetranucleosomal arrays to better understand various features of higher-order chromatin structure and nucleosome stability
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