Quantifying ChIP-seq data: a spiking method providing an internal reference for sample-to-sample normalization

Nicolas Bonhoure; Gergana Bounova; David Bernasconi; Viviane Praz; Fabienne Lammers; Donatella Canella; Ian M. Willis; Winship Herr; Nouria Hernandez; Mauro Delorenzi; The CycliX Consortium; Nouria Hernandez; Mauro Delorenzi; Bart Deplancke; Béatrice Desvergne; Nicolas Guex; Winship Herr; Felix Naef; Jacques Rougemont; Ueli Schibler; Teemu Andersin; Pascal Cousin; Federica Gilardi; Pascal Gos; Fabienne Lammers; Sunil Raghav; Dominic Villeneuve; Roberto Fabbretti; Volker Vlegel; Ioannis Xenarios; Eugenia Migliavacca; Viviane Praz; Fabrice David; Yohan Jarosz; Dmitry Kuznetsov; Robin Liechti; Olivier Martin; Julien Delafontaine; Julia Cajan; Kyle Gustafson; Irina Krier; Marion Leleu; Nacho Molina; Aurélien Naldi; Leonor Rib; Laura Symul; Gergana Bounova

doi:10.1101/gr.168260.113

Quantifying ChIP-seq data: a spiking method providing an internal reference for sample-to-sample normalization

¹Center for Integrative Genomics, Faculty of Biology and Medicine, University of Lausanne, 1015 Lausanne, Switzerland;
²Bioinformatics Core Facility, SIB Swiss Institute of Bioinformatics, 1015 Lausanne, Switzerland;
³Swiss Institute of Bioinformatics, 1015 Lausanne, Switzerland;
⁴Department of Biochemistry, Albert Einstein College of Medicine, Bronx, New York 10461, USA;
⁵Department of Oncology and the Ludwig Center for Cancer Research, Faculty of Biology and Medicine, University of Lausanne, 1011 Lausanne, Switzerland

Abstract

Chromatin immunoprecipitation followed by deep sequencing (ChIP-seq) experiments are widely used to determine, within entire genomes, the occupancy sites of any protein of interest, including, for example, transcription factors, RNA polymerases, or histones with or without various modifications. In addition to allowing the determination of occupancy sites within one cell type and under one condition, this method allows, in principle, the establishment and comparison of occupancy maps in various cell types, tissues, and conditions. Such comparisons require, however, that samples be normalized. Widely used normalization methods that include a quantile normalization step perform well when factor occupancy varies at a subset of sites, but may miss uniform genome-wide increases or decreases in site occupancy. We describe a spike adjustment procedure (SAP) that, unlike commonly used normalization methods intervening at the analysis stage, entails an experimental step prior to immunoprecipitation. A constant, low amount from a single batch of chromatin of a foreign genome is added to the experimental chromatin. This “spike” chromatin then serves as an internal control to which the experimental signals can be adjusted. We show that the method improves similarity between replicates and reveals biological differences including global and largely uniform changes.

Footnotes

↵6 These authors contributed equally to this work.
↵7 A complete list of consortium authors appears at the end of this article.
↵8 Present address: Biocartis SA, EPFL Innovation Square, Lausanne, Switzerland
↵9 Corresponding authors

E-mail nouria.hernandez{at}unil.ch

E-mail mauro.delorenzi{at}unil.ch
[Supplemental material is available for this article.]
Article published online before print. Article, supplemental material, and publication date are at http://www.genome.org/cgi/doi/10.1101/gr.168260.113.

Freely available online through the Genome Research Open Access option.

Received October 11, 2013.
Accepted March 31, 2014.

This article, published in Genome Research, is available under a Creative Commons License (Attribution-NonCommercial 4.0 International), as described at http://creativecommons.org/licenses/by-nc/4.0/.