Scc2/Nipbl hops between chromosomal cohesin rings after loading

Author:

Rhodes James1ORCID,Mazza Davide23ORCID,Nasmyth Kim1ORCID,Uphoff Stephan1ORCID

Affiliation:

1. Department of Biochemistry, Oxford University, Oxford, United Kingdom

2. Istituto Scientifico Ospedale San Raffaele, Centro di Imaging Sperimentale, Milano, Italy

3. Fondazione CEN, European Center for Nanomedicine, Milano, Italy

Abstract

The cohesin complex mediates DNA-DNA interactions both between (sister chromatid cohesion) and within chromosomes (DNA looping). It has been suggested that intra-chromosome loops are generated by extrusion of DNAs through the lumen of cohesin’s ring. Scc2 (Nipbl) stimulates cohesin’s ABC-like ATPase and is essential for loading cohesin onto chromosomes. However, it is possible that the stimulation of cohesin’s ATPase by Scc2 also has a post-loading function, for example driving loop extrusion. Using fluorescence recovery after photobleaching (FRAP) and single-molecule tracking in human cells, we show that Scc2 binds dynamically to chromatin, principally through an association with cohesin. Scc2’s movement within chromatin is consistent with a 'stop-and-go' or 'hopping' motion. We suggest that a low diffusion coefficient, a low stoichiometry relative to cohesin, and a high affinity for chromosomal cohesin enables Scc2 to move rapidly from one chromosomal cohesin complex to another, performing a function distinct from loading.

Funder

Wellcome

H2020 European Research Council

Cancer Research UK

Publisher

eLife Sciences Publications, Ltd

Subject

General Immunology and Microbiology,General Biochemistry, Genetics and Molecular Biology,General Medicine,General Neuroscience

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