Formamide denaturation of double-stranded DNA for fluorescence in situ hybridization (FISH) distorts nanoscale chromatin structure

Author:

Shim Anne R.,Frederick JaneORCID,Pujadas Emily M.,Kuo Tiffany,Ye I. ChaeORCID,Pritchard Joshua A.,Dunton Cody L.,Gonzalez Paola CarrilloORCID,Acosta Nicolas,Jain Surbhi,Anthony Nicholas M.,Almassalha Luay M.ORCID,Szleifer IgalORCID,Backman VadimORCID

Abstract

As imaging techniques rapidly evolve to probe nanoscale genome organization at higher resolution, it is critical to consider how the reagents and procedures involved in sample preparation affect chromatin at the relevant length scales. Here, we investigate the effects of fluorescent labeling of DNA sequences within chromatin using the gold standard technique of three-dimensional fluorescence in situ hybridization (3D FISH). The chemical reagents involved in the 3D FISH protocol, specifically formamide, cause significant alterations to the sub-200 nm (sub-Mbp) chromatin structure. Alternatively, two labeling methods that do not rely on formamide denaturation, resolution after single-strand exonuclease resection (RASER)-FISH and clustered regularly interspaced short palindromic repeats (CRISPR)-Sirius, had minimal impact on the three-dimensional organization of chromatin. We present a polymer physics-based analysis of these protocols with guidelines for their interpretation when assessing chromatin structure using currently available techniques.

Funder

National Science Foundation

National Cancer Institute

Center for Physical Genomics and Engineering

K. Hudson and R. Goldman

S. Brice and J. Esteve

M.E. Holliday and I. Schneider

Christina Carinato Charitable Foundation

D. Sachs

Chemistry of Life Processes Institute

NU Office for Research

Department of Molecular Biosciences

Rice Foundation

National Institutes of Health

Publisher

Public Library of Science (PLoS)

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