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How chromosome topologies get their shape: views from proximity ligation and microscopy methods

FEBS Lett. 2020 Nov;594(21):3439-3449. doi: 10.1002/1873-3468.13961. Epub 2020 Nov 3.

Abstract

The 3D organization of our genome is an important determinant for the transcriptional output of a gene in (patho)physiological contexts. The spatial organization of linear chromosomes within nucleus is dominantly inferred using two distinct approaches, chromosome conformation capture (3C) and DNA fluorescent in situ hybridization (DNA-FISH). While 3C and its derivatives score genomic interaction frequencies based on proximity ligation events, DNA-FISH methods measure physical distances between genomic loci. Despite these approaches probe different characteristics of chromosomal topologies, they provide a coherent picture of how chromosomes are organized in higher-order structures encompassing chromosome territories, compartments, and topologically associating domains. Yet, at the finer topological level of promoter-enhancer communication, the imaging-centered and the 3C methods give more divergent and sometimes seemingly paradoxical results. Here, we compare and contrast observations made applying visual DNA-FISH and molecular 3C approaches. We emphasize that the 3C approach, due to its inherently competitive ligation step, measures only 'relative' proximities. A 3C interaction enriched between loci, therefore does not necessarily translates into a decrease in absolute spatial distance. Hence, we advocate caution when modeling chromosome conformations.

Keywords: DNA fluorescent in situ hybridization; chromosome conformation capture; gene regulation; genome organization; live-cell imaging; loop extrusion; promoter-enhancer interaction.

Publication types

  • Research Support, Non-U.S. Gov't
  • Review

MeSH terms

  • Animals
  • Chromosomes / chemistry*
  • Chromosomes / metabolism*
  • Humans
  • Microscopy / methods*
  • Models, Molecular
  • Molecular Conformation