Rapid Assessment of Pepsin Column Activity for Reliable HDX-MS Studies

Vorauer, Clint; Wrigley, Michael S.; Pabon, Juan P. Rincon; Watson, Michael J.; Mundorff, Charlie C.; Weis, David D.; Guttman, Miklós

doi:10.1021/jasms.1c00080

Cited by 5 publications

(13 citation statements)

References 21 publications

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“…Using a standard peptide or well-established protein to quantitatively assess proteolytic efficiency is an effective way to achieve more reproducible digestion profiles among data sets and across different laboratories. 635 …”

Section: Precision and Reproducibility Of Hdx-ms Measurementsmentioning

confidence: 99%

“…These observations point out that standardization of conditions and reagents is critical for generating consistent digests so that peptides can be compared directly between sample sets. Using a standard peptide or well-established protein to quantitatively assess proteolytic efficiency is an effective way to achieve more reproducible digestion profiles among data sets and across different laboratories …”

Section: Precision and Reproducibility Of Hdx-ms Measurementsmentioning

confidence: 99%

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Advances in Hydrogen/Deuterium Exchange Mass Spectrometry and the Pursuit of Challenging Biological Systems

et al. 2021

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Solution-phase hydrogen/deuterium exchange (HDX) coupled to mass spectrometry (MS) is a widespread tool for structural analysis across academia and the biopharmaceutical industry. By monitoring the exchangeability of backbone amide protons, HDX-MS can reveal information about higher-order structure and dynamics throughout a protein, can track protein folding pathways, map interaction sites, and assess conformational states of protein samples. The combination of the versatility of the hydrogen/deuterium exchange reaction with the sensitivity of mass spectrometry has enabled the study of extremely challenging protein systems, some of which cannot be suitably studied using other techniques. Improvements over the past three decades have continually increased throughput, robustness, and expanded the limits of what is feasible for HDX-MS investigations. To provide an overview for researchers seeking to utilize and derive the most from HDX-MS for protein structural analysis, we summarize the fundamental principles, basic methodology, strengths and weaknesses, and the established applications of HDX-MS while highlighting new developments and applications.

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Section: Precision and Reproducibility Of Hdx-ms Measurementsmentioning

confidence: 99%

Section: Precision and Reproducibility Of Hdx-ms Measurementsmentioning

confidence: 99%

Advances in Hydrogen/Deuterium Exchange Mass Spectrometry and the Pursuit of Challenging Biological Systems

et al. 2021

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“…13 Labeling of spike's "hinge" is a novel HDX-MS result, completely based on the coverage of deuterated glycopeptides containing glycan-modified N1134 (Figures 6 and S2). Robust labeling (24-30%) was observed in the fusion peptide (823-851), N-terminus, [19][20][21][22][23][24][25][26][27][28][29][30][31] and middle helix of the stalk (1174-1197).…”

Section: Localization Of These Patterns On a Model Based Upon Protein...mentioning

confidence: 99%

“…22 A key step in modern HDX-MS analysis for obtaining sequence coverage is on-line proteolytic digestion 23 of the (glyco)protein of interest to generate peptides amenable to liquid chromatography (LC)/MS detection. HDX-MS sample preparation typically includes a low-pH ($2.5) quenching step immediately before proteolytic digestion, 12 limiting digestion to acid-tolerant proteases such as pepsin 24 or aspergillopepsin. 23,25 These proteases generate overlapping, mostly nonspecific 26 peptides that are nonetheless reproducible for a given protein substrate.…”

Section: Introductionmentioning

confidence: 99%

Inclusion of deuterated glycopeptides provides increased sequence coverage in hydrogen/deuterium exchange mass spectrometry analysis of SARS‐CoV‐2 spike glycoprotein

Haynes,

Keppel,

Mekonnen

et al. 2024

Rapid Comm Mass Spectrometry

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RationaleHydrogen/deuterium exchange mass spectrometry (HDX‐MS) can provide precise analysis of a protein's conformational dynamics across varied states, such as heat‐denatured versus native protein structures, localizing regions that are specifically affected by such conditional changes. Maximizing protein sequence coverage provides high confidence that regions of interest were located by HDX‐MS, but one challenge for complete sequence coverage is N‐glycosylation sites. The deuteration of peptides post‐translationally modified by asparagine‐bound glycans (glycopeptides) has not always been identified in previous reports of HDX‐MS analyses, causing significant sequence coverage gaps in heavily glycosylated proteins and uncertainty in structural dynamics in many regions throughout a glycoprotein.MethodsWe detected deuterated glycopeptides with a Tribrid Orbitrap Eclipse mass spectrometer performing data‐dependent acquisition. An MS scan was used to identify precursor ions; if high‐energy collision‐induced dissociation MS/MS of the precursor indicated oxonium ions diagnostic for complex glycans, then electron transfer low‐energy collision‐induced dissociation MS/MS scans of the precursor identified the modified asparagine residue and the glycan's mass. As in traditional HDX‐MS, the identified glycopeptides were then analyzed at the MS level in samples labeled with D2O.ResultsWe report HDX‐MS analysis of the SARS‐CoV‐2 spike protein ectodomain in its trimeric prefusion form, which has 22 predicted N‐glycosylation sites per monomer, with and without heat treatment. We identified glycopeptides and calculated their average isotopic mass shifts from deuteration. Inclusion of the deuterated glycopeptides increased sequence coverage of spike ectodomain from 76% to 84%, demonstrated that glycopeptides had been deuterated, and improved confidence in results localizing structural rearrangements.ConclusionInclusion of deuterated glycopeptides improves the analysis of the conformational dynamics of glycoproteins such as viral surface antigens and cellular receptors.

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“…The MS equipment and techniques used to measure HDX are continually evolving. Key challenges include limiting the back-exchange of absorbed deuterium , and improving both the throughput and coverage of the protein digestion step. , Many excellent reviews cover the current applications and practice of HDX-MS. ,,,,,− As such, the discussion below focuses mainly on the application of HDX-MS for the assessment of protein stability. The earliest examples of such experiments focus on model proteins, such as ubiquitin and lysozyme, with the latter protein probed under conditions promoting both intact and reduced disulfide bonds .…”

Section: Survey Of Ms-based Protein Stability Measurement Techniquesmentioning

confidence: 99%

Mass Spectrometry Methods for Measuring Protein Stability

et al. 2022

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Mass spectrometry is a central technology in the life sciences, providing our most comprehensive account of the molecular inventory of the cell. In parallel with developments in mass spectrometry technologies targeting such assessments of cellular composition, mass spectrometry tools have emerged as versatile probes of biomolecular stability. In this review, we cover recent advancements in this branch of mass spectrometry that target proteins, a centrally important class of macromolecules that accounts for most biochemical functions and drug targets. Our efforts cover tools such as hydrogen–deuterium exchange, chemical cross-linking, ion mobility, collision induced unfolding, and other techniques capable of stability assessments on a proteomic scale. In addition, we focus on a range of application areas where mass spectrometry-driven protein stability measurements have made notable impacts, including studies of membrane proteins, heat shock proteins, amyloidogenic proteins, and biotherapeutics. We conclude by briefly discussing the future of this vibrant and fast-moving area of research.

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Rapid Assessment of Pepsin Column Activity for Reliable HDX-MS Studies

Cited by 5 publications

References 21 publications

Advances in Hydrogen/Deuterium Exchange Mass Spectrometry and the Pursuit of Challenging Biological Systems

Advances in Hydrogen/Deuterium Exchange Mass Spectrometry and the Pursuit of Challenging Biological Systems

Inclusion of deuterated glycopeptides provides increased sequence coverage in hydrogen/deuterium exchange mass spectrometry analysis of SARS‐CoV‐2 spike glycoprotein

Mass Spectrometry Methods for Measuring Protein Stability

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