Issue 34, 2020
From the journal:

Chemical Science

Examining histone modification crosstalk using immobilized libraries established from ligation-ready nucleosomes

Diego Aparicio Pelaz,a   Zhadyra Yerkesh,b   Sören Kirchgäßner, ORCID logo a   Henriette Mahler,c   Vladlena Kharchenko,b   Dulat Azhibek,b   Mariusz Jaremko, ORCID logo b   Henning D. Mootz, ORCID logo d   Łukasz Jaremko,b   Dirk Schwarzer ORCID logo *a  and  Wolfgang Fischle*bc  

* Corresponding authors

a Interfaculty Institute of Biochemistry, University of Tübingen, Auf der Morgenstelle 34, D-72076 Tübingen, Germany
E-mail: dirk.schwarzer@uni-tuebingen.de

b Biological and Environmental Science and Engineering Division, King Abdullah University of Science and Technology, Thuwal 23955, Saudi Arabia
E-mail: wolfgang.fischle@kaust.edu.sa

c Laboratory of Chromatin Biochemistry, Max Planck Institute for Biophysical Chemistry, 37077 Göttingen, Germany

d Institute of Biochemistry, University of Muenster, Corrensstr. 36, 48149 Münster, Germany

Abstract

Chromatin signaling relies on a plethora of posttranslational modifications (PTM) of the histone proteins which package the long DNA molecules of our cells in reoccurring units of nucleosomes. Determining the biological function and molecular working mechanisms of different patterns of histone PTMs requires access to various chromatin substrates of defined modification status. Traditionally, these are achieved by individual reconstitution of single nucleosomes or arrays of nucleosomes in conjunction with modified histones produced by means of chemical biology. Here, we report an alternative strategy for establishing a library of differentially modified nucleosomes that bypasses the need for many individual syntheses, purification and assembly reactions by installing modified histone tails on ligation-ready, immobilized nucleosomes reconstituted in a single batch. Using the ligation-ready nucleosome strategy with sortase-mediated ligation for histone H3 and intein splicing for histone H2A, we generated libraries of up to 280 individually modified nucleosomes in 96-well plate format. Screening these libraries for the effects of patterns of PTMs onto the recruitment of a well-known chromatin factor, HP1 revealed a previously unknown long-range cross-talk between two modifications. H3S28 phosphorylation enhances recruitment of the HP1 protein to the H3K9 methylated H3-tail only in nucleosomal context. Detailed structural analysis by NMR measurements implies negative charges at position 28 to increase nucleosomal H3-tail dynamics and flexibility. Our work shows that ligation-ready nucleosomes enable unprecedented access to the ample space and complexity of histone modification patterns for the discovery and dissection of chromatin regulatory principles.

Graphical abstract: Examining histone modification crosstalk using immobilized libraries established from ligation-ready nucleosomes

About
Cited by
Related
Download options Please wait...

Supplementary files

Article information

DOI
https://doi.org/10.1039/D0SC03407J
Article type
Edge Article
Submitted
19 Jun 2020
Accepted
14 Aug 2020
First published
20 Aug 2020
This article is Open Access

All publication charges for this article have been paid for by the Royal Society of Chemistry
Creative Commons BY-NC license

Chem. Sci., 2020,11, 9218-9225

Permissions

Request permissions

Examining histone modification crosstalk using immobilized libraries established from ligation-ready nucleosomes

D. Aparicio Pelaz, Z. Yerkesh, S. Kirchgäßner, H. Mahler, V. Kharchenko, D. Azhibek, M. Jaremko, H. D. Mootz, Ł. Jaremko, D. Schwarzer and W. Fischle, Chem. Sci., 2020, 11, 9218 DOI: 10.1039/D0SC03407J

This article is licensed under a Creative Commons Attribution-NonCommercial 3.0 Unported Licence. You can use material from this article in other publications, without requesting further permission from the RSC, provided that the correct acknowledgement is given and it is not used for commercial purposes.

To request permission to reproduce material from this article in a commercial publication, please go to the Copyright Clearance Center request page.

If you are an author contributing to an RSC publication, you do not need to request permission provided correct acknowledgement is given.

If you are the author of this article, you do not need to request permission to reproduce figures and diagrams provided correct acknowledgement is given. If you want to reproduce the whole article in a third-party commercial publication (excluding your thesis/dissertation for which permission is not required) please go to the Copyright Clearance Center request page.

Read more about how to correctly acknowledge RSC content.

Social activity

Spotlight

Advertisements