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Nanoscale 3D DNA tracing in non-denatured cells resolves the Cohesin-dependent loop architecture of the genome in situ

Nature Communications. 2025-07; 
K S Beckwith, Ø Ødegård-Fougner, N R Morero, C Barton, F Schueder, W Tang, S Alexander, J-M Peters, R Jungmann, E Birney, J Ellenberg Cell Biology and Biophysics Unit, European Molecular Biology Laboratory, Heidelberg, Germany
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Oligo pool Docking sequences for secondary imagers (two identical barcodes for each position and one for each region per oligo) and amplification primers were appended, and probe libraries were ordered from Genscript (Precise Synthetic Oligo Pools) and amplified (see below). Get A Quote

摘要

The spatial organization of the genome is essential for its functions, including gene expression and chromosome segregation. Phase separation and loop extrusion have been proposed to underlie compartments and topologically associating domains, however, whether the fold of genomic DNA inside the nucleus is consistent with such mechanisms has been difficult to establish in situ. Here, we present a 3D DNA-tracing workflow that resolves genome architecture in single structurally well-preserved cells with nanometre resolution. Our findings reveal that genomic DNA generally behaves as a flexible random coil at the 100-kb scale. At CTCF sites however, we find Cohesin-dependent loops in a subset of cells, in variable c... More

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