Absolute quantification of cohesin, CTCF and their regulators in human cells

Author:

Holzmann Johann,Politi Antonio Z.,Nagasaka KotaORCID,Hantsche-Grininger Merle,Walther NikeORCID,Koch Birgit,Fuchs Johannes,Dürnberger Gerhard,Tang Wen,Ladurner Rene,Stocsits Roman R.,Busslinger Georg A.,Novak BelaORCID,Mechtler KarlORCID,Davidson Iain F.,Ellenberg JanORCID,Peters Jan-MichaelORCID

Abstract

AbstractThe organisation of mammalian genomes into loops and topologically associating domains (TADs) contributes to chromatin structure, gene expression and recombination. Loops and TADs are formed by cohesin and positioned by CTCF. In proliferating cells, cohesin also mediates sister chromatid cohesion, which is essential for chromosome segregation. Current models of chromatin folding and cohesion are based on assumptions of how many cohesin and CTCF molecules organise the genome. Here we have measured absolute copy numbers and dynamics of cohesin, CTCF, NIPBL, WAPL and sororin by mass spectrometry, fluorescence-correlation spectroscopy and fluorescence recovery after photobleaching in HeLa cells. In G1-phase there are ~245,000 cohesin complexes, of which ~139,000 are on chromatin. Comparison with chromatin immunoprecipitation-sequencing data implies that some genomic cohesin and CTCF enrichment sites are unoccupied in single cells at any one time. We discuss the implications of these findings for how cohesin can contribute to genome organisation and cohesion.

Publisher

Cold Spring Harbor Laboratory

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