Comprehensive identification of protein disulfide bonds with pepsin/trypsin digestion, Orbitrap HCD and Spectrum Identification Machine

Chuanlong Cui; Tong Liu; Tong Chen; Johanna Lu; Ian Casaren; Diogo Borges Lima; Paulo Costa Carvalho; Annie Beuve; Hong Li

doi:10.1016/j.jprot.2018.12.010

Comprehensive identification of protein disulfide bonds with pepsin/trypsin digestion, Orbitrap HCD and Spectrum Identification Machine

J Proteomics. 2019 Apr 30:198:78-86. doi: 10.1016/j.jprot.2018.12.010. Epub 2018 Dec 14.

Authors

Chuanlong Cui¹, Tong Liu¹, Tong Chen¹, Johanna Lu¹, Ian Casaren¹, Diogo Borges Lima², Paulo Costa Carvalho³, Annie Beuve⁴, Hong Li⁵

Affiliations

¹ Center for Advanced Proteomics Research and Department of Microbiology, Biochemistry and Molecular Genetics, Rutgers University - New Jersey Medical School and Cancer Institute of New Jersey, Newark, NJ 07103, USA.
² Mass Spectrometry for Biology Unit, Institut Pasteur, CNRS USR 2000, Paris, France.
³ Laboratory for Structural and Computational Proteomics, Carlos Chagas Institute, Fiocruz Paraná, Brazil.
⁴ Department of Pharmacology, Physiology and Neuroscience, Rutgers University - New Jersey Medical School, Newark, NJ 07103, USA.
⁵ Center for Advanced Proteomics Research and Department of Microbiology, Biochemistry and Molecular Genetics, Rutgers University - New Jersey Medical School and Cancer Institute of New Jersey, Newark, NJ 07103, USA. Electronic address: liho2@rutgers.edu.

Abstract

Disulfide bonds (SS) are post-translational modifications important for the proper folding and stabilization of many cellular proteins with therapeutic uses, including antibodies and other biologics. With budding advances of biologics and biosimilars, there is a mounting need for a robust method for accurate identification of SS. Even though several mass spectrometry methods have emerged for this task, their practical use rests on the broad effectiveness of both sample preparation methods and bioinformatics tools. Here we present a new protocol tailored toward mapping SS; it uses readily available reagents, instruments, and software. For sample preparation, a 4-h pepsin digestion at pH 1.3 followed by an overnight trypsin digestion at pH 6.5 can maximize the release of SS-containing peptides from non-reduced proteins, while minimizing SS scrambling. For LC/MS/MS analysis, SS-containing peptides can be efficiently fragmented with HCD in a Q Exactive Orbitrap mass spectrometer, preserving SS for subsequent identification. Our bioinformatics protocol describes how we tailored our freely downloadable and easy-to-use software, Spectrum Identification Machine for Cross-Linked Peptides (SIM-XL), to minimize false identification and facilitate manual validation of SS-peptide mass spectra. To substantiate this optimized method, we've comprehensively identified 14 out of 17 known SS in BSA. SIGNIFICANCE: Comprehensive and accurate identification of SS in proteins is critical for elucidating protein structures and functions. Yet, it is far from routine to accomplish this task in many analytical or core laboratories. Numerous published methods require complex sample preparation methods, specialized mass spectrometers and cumbersome or proprietary software tools, thus cannot be easily implemented in unspecialized laboratories. Here, we describe a robust and rapid SS mapping approach that utilizes readily available reagents, instruments, and software; it can be easily implemented in any analytical core laboratories, and tested for its impact on the research community.

Keywords: HCD; Pepsin; Protein disulfide bond; SIM-XL; Tandem mass spectrometry; Trypsin.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Cattle
Chickens
Disulfides / analysis*
Disulfides / chemistry
Mass Spectrometry*
Pepsin A / chemistry*
Peptides / analysis*
Peptides / chemistry
Trypsin / chemistry*

Substances

Disulfides
Peptides
Trypsin
Pepsin A

Abstract

Publication types

MeSH terms

Substances

Grants and funding