Sequential Window Acquisition of all Theoretical Mass Spectra (SWATH) Analysis for Characterization and Quantification of Histone Post-translational Modifications

Simone Sidoli,Shu Lin,Lei Xiong,Natarajan V Bhanu,Kelly R Karch,Eric Johansen,Christie Hunter,Sahana Mollah,Benjamin A Garcia

doi:10.1074/mcp.o114.046102

Abstract

Histone post-translational modifications (PTMs) have a fundamental function in chromatin biology, as they model chromatin structure and recruit enzymes involved in gene regulation, DNA repair, and chromosome condensation. High throughput characterization of histone PTMs is mostly performed by using nano-liquid chromatography coupled to mass spectrometry. However, limitations in speed and stochastic sampling of data dependent acquisition methods in MS lead to incomplete discrimination of isobaric peptides and loss of low abundant species. In this work, we analyzed histone PTMs with a data-independent acquisition method, namely SWATH™ analysis. This approach allows for MS/MS-based quantification of all analytes without upfront assay development and no issues of biased and incomplete sampling. We purified histone proteins from human embryonic stem cells and mouse trophoblast stem cells before and after differentiation, and prepared them for MS analysis using the propionic anhydride protocol. Results on histone H3 peptides verified that sequential window acquisition of all theoretical mass spectra could accurately quantify peptides (<9% average coefficient of variation, CV) over four orders of magnitude, and we could discriminate isobaric and co-eluting peptides (e.g. H3K18ac and H3K23ac) using MS/MS-based quantification. This method provided high sensitivity and precision, supported by the fact that we could find significant differences for remarkably low abundance PTMs such as H3K9me2S10ph (relative abundance <0.02%). We performed relative quantification for few sample peptides using different fragment ions and observed high consistency (CV <15%) between the fragments. This indicated that different fragment ions can be used independently to achieve the same peptide relative quantification. Taken together, sequential window acquisition of all theoretical mass spectra proved to be an easy-to-use MS acquisition method to perform high quality MS/MS-based quantification of histone-modified peptides.

Highlights

We prove that SWATHTM-Mass spectrometry (MS) is a reliable and simple-to-use acquisition method to perform epigenetic histone post-translational modifications (PTMs) analysis
We tested SWATHTM-MS as acquisition method to evaluate the advantages of the MS/MS-based label-free quantification
Because histone peptides are decorated with multiple variable PTMs, we used SWATHTM to perform MS/MS fragmentation through the entire elution and separately quantify isobaric species

Summary

Technological Innovations and Resources

Sequential Window Acquisition of all Theoretical Mass Spectra (SWATH) Analysis for Characterization and Quantification of Histone Post-translational Modifications*□S. The most widely adopted in shotgun or discovery proteomics is the data-dependent acquisition (DDA) mode Such acquisition method does not require any previous knowledge about the analyte, as it automatically selects precursor ions detectable at the full scan level in a given order (commonly from the most intense) to perform MS/MS fragmentation [11]. LC-MS/MS analysis of histone peptides is commonly performed by integrating shotgun and targeted acquisition within the same MS method [13] This method requires previous knowledge about retention time and mass of coeluting isobaric species, and tedious manual peak integration or dedicated software to deconvolute such complex raw data. We prove that SWATHTM-MS is a reliable and simple-to-use acquisition method to perform epigenetic histone PTM analysis

EXPERIMENTAL PROCEDURES

RESULTS

DISCUSSION