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Fast and Accurate Disulfide Bridge Detection.
Heissel, Søren; He, Yi; Jankevics, Andris; Shi, Yuqi; Molina, Henrik; Viner, Rosa; Scheltema, Richard A.
Afiliação
  • Heissel S; Proteomics Resource Center, The Rockefeller University, New York, New York, USA. Electronic address: sheissel@rockefeller.edu.
  • He Y; Thermo Fisher Scientific, San Jose, California, USA.
  • Jankevics A; Biomolecular Mass Spectrometry and Proteomics, Bijvoet Center for Biomolecular Research and Utrecht Institute for Pharmaceutical Sciences, University of Utrecht, Utrecht, The Netherlands; Structural Proteomics Group, Department of Biochemistry and Systems Biology, University of Liverpool, Liverpool,
  • Shi Y; Thermo Fisher Scientific, San Jose, California, USA.
  • Molina H; Proteomics Resource Center, The Rockefeller University, New York, New York, USA.
  • Viner R; Thermo Fisher Scientific, San Jose, California, USA. Electronic address: rosa.viner@thermofisher.com.
  • Scheltema RA; Biomolecular Mass Spectrometry and Proteomics, Bijvoet Center for Biomolecular Research and Utrecht Institute for Pharmaceutical Sciences, University of Utrecht, Utrecht, The Netherlands; Structural Proteomics Group, Department of Biochemistry and Systems Biology, University of Liverpool, Liverpool,
Mol Cell Proteomics ; 23(5): 100759, 2024 May.
Article em En | MEDLINE | ID: mdl-38574859
ABSTRACT
Recombinant expression of proteins, propelled by therapeutic antibodies, has evolved into a multibillion dollar industry. Essential here is the quality control assessment of critical attributes, such as sequence fidelity, proper folding, and posttranslational modifications. Errors can lead to diminished bioactivity and, in the context of therapeutic proteins, an elevated risk for immunogenicity. Over the years, many techniques were developed and applied to validate proteins in a standardized and high-throughput fashion. One parameter has, however, so far been challenging to assess. Disulfide bridges, covalent bonds linking two cysteine residues, assist in the correct folding and stability of proteins and thus have a major influence on their efficacy. Mass spectrometry promises to be an optimal technique to uncover them in a fast and accurate fashion. In this work, we present a unique combination of sample preparation, data acquisition, and analysis facilitating the rapid and accurate assessment of disulfide bridges in purified proteins. Through microwave-assisted acid hydrolysis, the proteins are digested rapidly and artifact-free into peptides, with a substantial degree of overlap over the sequence. The nonspecific nature of this procedure, however, introduces chemical background, which is efficiently removed by integrating ion mobility preceding the mass spectrometric measurement. The nonspecific nature of the digestion step additionally necessitates new developments in data analysis, for which we extended the XlinkX node in Proteome Discoverer to efficiently process the data and ensure correctness through effective false discovery rate correction. The entire workflow can be completed within 1 h, allowing for high-throughput, high-accuracy disulfide mapping.
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Texto completo: 1 Coleções: 01-internacional Base de dados: MEDLINE Assunto principal: Dissulfetos Limite: Humans Idioma: En Revista: Mol Cell Proteomics Ano de publicação: 2024 Tipo de documento: Article

Texto completo: 1 Coleções: 01-internacional Base de dados: MEDLINE Assunto principal: Dissulfetos Limite: Humans Idioma: En Revista: Mol Cell Proteomics Ano de publicação: 2024 Tipo de documento: Article