Methods for the Differential Analysis of Hi-C Data

染色质 染色体构象捕获 嘉雅宠物 支架/基质附着区域 增强子 计算生物学 生物 基因组 染色体 遗传学 染色质重塑 基因 转录因子
作者
Chiara Nicoletti
出处
期刊:Methods in molecular biology [Springer Science+Business Media]
卷期号:: 61-95 被引量:5
标识
DOI:10.1007/978-1-0716-1390-0_4
摘要

The 3D organization of chromatin within the nucleus enables dynamic regulation and cell type-specific transcription of the genome. This is true at multiple levels of resolution: on a large scale, with chromosomes occupying distinct volumes (chromosome territories); at the level of individual chromatin fibers, which are organized into compartmentalized domains (e.g., Topologically Associating Domains-TADs), and at the level of short-range chromatin interactions between functional elements of the genome (e.g., enhancer-promoter loops).The widespread availability of Chromosome Conformation Capture (3C)-based high-throughput techniques has been instrumental in advancing our knowledge of chromatin nuclear organization. In particular, Hi-C has the potential to achieve the most comprehensive characterization of chromatin 3D interactions, as it is theoretically able to detect any pair of restriction fragments connected as a result of ligation by proximity.This chapter will illustrate how to compare the chromatin interactome in different experimental conditions, starting from pre-computed Hi-C contact matrices, how to visualize the results, and how to correlate the observed variations in chromatin interaction strength with changes in gene expression.
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