Biophys J. 2022 Nov 02. pii: S0006-3495(22)00898-0. [Epub ahead of print]
The spatial organization of the eukaryotic genome plays an important role in regulating transcriptional activity. In the nucleus, chromatin forms loops that assemble into fundamental units called topologically associating domains that facilitate or inhibit long-range contacts. These loops are formed and held together by the ring-shaped cohesin protein complex, and this can involve binding of CCCTC-binding factor (CTCF). High-resolution conformation capture experiments provide the frequency at which two DNA fragments physically associate in 3D space. However, technical limitations of this approach, such as low throughput, low resolution or noise in contact maps make data interpretation and identification of chromatin intra-loop contacts, e.g. between distal regulatory elements and their target genes, challenging. Herein, an existing coarse-grained model of chromatin at single nucleosome resolution was extended by integrating potentials describing CTCF and cohesin. We performed replica exchange Monte Carlo simulations with regularly spaced nucleosomes, and experimentally determined nucleosome positions in the presence of cohesin-CTCF, as well as depleted systems as controls. In fully extruded loops caused by the presence of cohesin and CTCF, the number of contacts within the formed loops was increased. The number and types of these contacts were impacted by the nucleosome distribution and loop size. Micro loops were observed within cohesin mediated loops due to thermal fluctuations without additional influence of other factors, and the number, size, and shape of micro loops were determined by nucleosome distribution and loop size. Nucleosome positions directly affect the spatial structure and contact probability within a loop, with presumed consequences for transcriptional activity.