| Literature DB >> 33067435 |
Alexandra Stützer1, Luisa M Welp1, Monika Raabe1, Timo Sachsenberg2,3, Christin Kappert1,4, Alexander Wulf1, Andy M Lau5, Stefan-Sebastian David6,7, Aleksandar Chernev1, Katharina Kramer8, Argyris Politis5, Oliver Kohlbacher2,3,9,10, Wolfgang Fischle6,7, Henning Urlaub11,12.
Abstract
Protein-DNA interactions are key to the functionality and stability of the genome. Identification and mapping of protein-DNA interaction interfaces and sites is crucial for understanding DNA-dependent processes. Here, we present a workflow that allows mass spectrometric (MS) identification of proteins in direct contact with DNA in reconstituted and native chromatin after cross-linking by ultraviolet (UV) light. Our approach enables the determination of contact interfaces at amino-acid level. With the example of chromatin-associated protein SCML2 we show that our technique allows differentiation of nucleosome-binding interfaces in distinct states. By UV cross-linking of isolated nuclei we determined the cross-linking sites of several factors including chromatin-modifying enzymes, demonstrating that our workflow is not restricted to reconstituted materials. As our approach can distinguish between protein-RNA and DNA interactions in one single experiment, we project that it will be possible to obtain insights into chromatin and its regulation in the future.Entities:
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Year: 2020 PMID: 33067435 PMCID: PMC7567871 DOI: 10.1038/s41467-020-19047-7
Source DB: PubMed Journal: Nat Commun ISSN: 2041-1723 Impact factor: 14.919