Mass Spectrometric Determination of Disulfide Linkages in Recombinant Therapeutic Proteins Using Online LC−MS with Electron-Transfer Dissociation

Wu, Shiaw‐Lin; Jiang, Haitao; Lu, Qiaozhen; Dai, Shujia; Hancock, William S.; Karger, Barry L.

doi:10.1021/ac801560k

Cited by 128 publications

(133 citation statements)

References 42 publications

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“…1C). Purified IGFBP-5 was digested with trypsin under non-reducing conditions and subjected to a MS3 protocol with ETD (ETD-MS2) followed by CID (CID-MS3) (40). CID-MS2 also was employed to help identify disulfide-linked peptides (Fig.…”

Section: An Ms Approach To Mapping Disulfide Bonds In Igfbp-5-mentioning

confidence: 99%

“…Mass spectrometric (MS) methods for identifying disulfide bonds have improved over the last few years, and several proteins recently have been mapped using a tandem MS approach in which peptides, including disulfide-linked species, are selected in the MS1 scan and then subjected to ETD (ETD-MS2) followed by CID (CID-MS3) (39,40). ETD fragments peptides via electron transfer from a radical anion to a protonated peptide, causing cleavage between C␣-N bonds which results in c and z ions (41).…”

mentioning

confidence: 99%

“…Traditional MS disulfide mapping methodologies have employed CID, but only to compare protease-digested peptides in proteins treated with or without reducing agents (44). However, because ETD preferentially cleaves disulfide bonds, this approach may be applied to protein samples without prior chemical reduction (40), as subsequent CID fragmentation of the peptides liberated by ETD will then identify the cysteines involved in disulfide bonds (40).…”

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confidence: 99%

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Defining the Disulfide Bonds of Insulin-like Growth Factor-binding Protein-5 by Tandem Mass Spectrometry with Electron Transfer Dissociation and Collision-induced Dissociation

Nili¹,

Mukherjee

Shinde

et al. 2012

Journal of Biological Chemistry

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Background: Only 2 of 9 putative disulfide bonds have been mapped for IGFBP-5. Results: Using a MS-based strategy combining ETD and CID, and ab initio molecular modeling, we have mapped all 9 disulfide bonds in IGFBP-5. Conclusion: Our results provide new insights into the IGFBP-5 structure. Significance: We define an approach using tandem MS and ab initio molecular modeling to characterize unknown disulfide linkages in proteins.

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Section: An Ms Approach To Mapping Disulfide Bonds In Igfbp-5-mentioning

confidence: 99%

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confidence: 99%

mentioning

confidence: 99%

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Defining the Disulfide Bonds of Insulin-like Growth Factor-binding Protein-5 by Tandem Mass Spectrometry with Electron Transfer Dissociation and Collision-induced Dissociation

Nili¹,

Mukherjee

Shinde

et al. 2012

Journal of Biological Chemistry

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“…15,17,19,27–30 Several mass spectrometry (MS)/MS approaches for characterizing disulfide linkages have been described using collision-induced dissociation (CID), electron-transfer dissociation (ETD), or electron-capture dissociation (ECD). 11–13,29,31–35 These approaches often require multiple analysis, comparison of reduced and non-reduced peptide maps, interpretation of complex data sets, or large sample consumption. Electrospray ionization MS/MS characterization of IgG2 hinge disulfides can also be difficult due to the large size of hinge peptides (5 – 10 kDa, depending on disulfide configuration and number of missed cleavages) that generate low-intensity, multiply charged peak clusters that complicate the deconvolution of the MS/MS spectra.…”

Section: Introductionmentioning

confidence: 99%

Rapid, automated characterization of disulfide bond scrambling and IgG2 isoform determination

Resemann

Liu-Shin

Tremintin

et al. 2018

mAbs

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Human antibodies of the IgG2 subclass exhibit complex inter-chain disulfide bonding patterns that result in three structures, namely A, A/B, and B. In therapeutic applications, the distribution of disulfide isoforms is a critical product quality attribute because each configuration affects higher order structure, stability, isoelectric point, and antigen binding. The current standard for quantification of IgG2 disulfide isoform distribution is based on chromatographic or electrophoretic techniques that require additional characterization using mass spectrometry (MS)-based methods to confirm disulfide linkages. Detailed characterization of the IgG2 disulfide linkages often involve MS/MS approaches that include electrospray ionization or electron-transfer dissociation, and method optimization is often cumbersome due to the large size and heterogeneity of the disulfide-bonded peptides. As reported here, we developed a rapid LC-MALDI-TOF/TOF workflow that can both identify the IgG2 disulfide linkages and provide a semi-quantitative assessment of the distribution of the disulfide isoforms. We established signature disulfide-bonded IgG2 hinge peptides that correspond to the A, A/B, and B disulfide isoforms and can be applied to the fast classification of IgG2 isoforms in heterogeneous mixtures.

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“…17 By preserving the post translational modifications (PTMs) to the greatest extent, it is considered to be an ideal tool for elucidation of sequences and identification of PTMs including disulfide bonding sites. 18 Despite these advantages, ETD still suffers from a low fragmentation rate of precursor ions with weak intensity just like other fragmentation techniques.…”

mentioning

confidence: 99%

High-Efficiency Recognition and Identification of Disulfide Bonded Peptides in Rat Neuropeptidome Using Targeted Electron Transfer Dissociation Tandem Mass Spectrometry

Khani

et al. 2015

Anal. Chem.

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ABSTRACT:The main goal of the present study is to develop a method to recognize and identify endogenous intrachain disulfide bonded peptide, which are rarely sequenced in current peptidomics studies. In order to achieve highly efficient detection of these peptides in a neuropeptidome analysis, we alkylated the peptides, mined the raw mass spectrometry data, and then recognized the candidates of untreated disulfide bonded peptides from unalkylated peptide extracts. After removing more than 90% features, targeted electron transfer dissociation fragmentation was performed for detecting and fragmenting disulfide bonded peptides, and even most of them were present in low abundance in the original sample. Diverse endogenous disulfide bonded peptides were then detected and sequenced, opening up new perspectives for comprehensively understanding the response of a neuropeptidome.

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Mass Spectrometric Determination of Disulfide Linkages in Recombinant Therapeutic Proteins Using Online LC−MS with Electron-Transfer Dissociation

Cited by 128 publications

References 42 publications

Defining the Disulfide Bonds of Insulin-like Growth Factor-binding Protein-5 by Tandem Mass Spectrometry with Electron Transfer Dissociation and Collision-induced Dissociation

Defining the Disulfide Bonds of Insulin-like Growth Factor-binding Protein-5 by Tandem Mass Spectrometry with Electron Transfer Dissociation and Collision-induced Dissociation

Rapid, automated characterization of disulfide bond scrambling and IgG2 isoform determination

High-Efficiency Recognition and Identification of Disulfide Bonded Peptides in Rat Neuropeptidome Using Targeted Electron Transfer Dissociation Tandem Mass Spectrometry

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