Nanopores Suggest a Negligible Influence of CpG Methylation on Nucleosome Packaging and Stability
Author(s) -
Martin Langecker,
Andrey Ivankin,
Spencer Carson,
Shan R. Morey Kinney,
Friedrich C. Simmel,
Meni Wanunu
Publication year - 2014
Publication title -
nano letters
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 4.853
H-Index - 488
eISSN - 1530-6992
pISSN - 1530-6984
DOI - 10.1021/nl504522n
Subject(s) - nucleosome , force spectroscopy , dna methylation , chromatin , dna , biophysics , nanopore , epigenetics , histone , linker dna , cpg site , chemistry , magnetic tweezers , biology , genetics , nanotechnology , atomic force microscopy , materials science , gene , gene expression
Nucleosomes are the fundamental repeating units of chromatin, and dynamic regulation of their positioning along DNA governs gene accessibility in eukaryotes. Although epigenetic factors have been shown to influence nucleosome structure and dynamics, the impact of DNA methylation on nucleosome packaging remains controversial. Further, all measurements to date have been carried out under zero-force conditions. In this paper, we present the first automated force measurements that probe the impact of CpG DNA methylation on nucleosome stability. In solid-state nanopore force spectroscopy, a nucleosomal DNA tail is captured into a pore and pulled on with a time-varying electrophoretic force until unraveling is detected. This is automatically repeated for hundreds of nucleosomes, yielding statistics of nucleosome lifetime vs electrophoretic force. The force geometry, which is similar to displacement forces exerted by DNA polymerases and helicases, reveals that nucleosome stability is sensitive to DNA sequence yet insensitive to CpG methylation. Our label-free method provides high-throughput data that favorably compares with other force spectroscopy experiments and is suitable for studying a variety of DNA-protein complexes.
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