Allosteric regulation of glycogen phosphorylase solution phase structural dynamics at high spatial resolution

Kish, Monika; Smith, Stacy; Subramanian, Sivaraman; Vollmer, Frank; Lethbridge, Natasha; Cole, Lindsay J.; Bond, Nicholas J.; Phillips, Jonathan J.

doi:10.1101/654665

Cited by 13 publications

(29 citation statements)

References 44 publications

(60 reference statements)

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“…Intrinsic rate calculation and protection factors. HDfleX also calculates the theoretical intrinsic rates for peptides 41 at the experimental pH and temperature. aSyn is incompatible with the Bai and Englander model for the calculation of intrinsic rates 27,44 as all the peptides exchanged faster than the predicted rates.…”

Section: Resultsmentioning

confidence: 99%

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HDfleX: Software for flexible high structural resolution of hydrogen/deuterium-exchange mass spectrometry data

Seetaloo

Kish

Phillips

2021

Preprint

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Hydrogen/deuterium-exchange mass spectrometry (HDX-MS) experiments on protein structures can be performed at three levels: (1) by enzymatically digesting labelled proteins and analyzing the peptides (bottom-up), (2) by further fragmenting peptides following digestion (middle-down), and (3) by fragmenting the intact labelled protein (top-down), using soft gas-phase fragmentation methods, such as electron transfer dissociation (ETD). However, to the best of our knowledge, the software packages currently available for the analysis of HDX-MS data do not enable the peptide- and ETD-levels to be combined - they can only be analyzed separately. Thus, we developed HDfleX - a standalone application for the analysis of flexible high structural resolution of HDX-MS data, which allows data at any level of structural resolution (intact protein, peptide, fragment) to be merged. HDfleX features rapid experimental data fitting, robust statistical significance analyses and optional methods for theoretical intrinsic calculations and a novel empirical correction for comparison between solution conditions.

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Section: Resultsmentioning

confidence: 99%

“…Calculation of intrinsic rates and protection factors. The intrinsic rates and protection factors were fitted and calculated as described previously 41 . Briefly, intrinsic uptake curves are generated, fitted into one-or two stretched exponentials.…”

Section: Methodsmentioning

confidence: 99%

HDfleX: Software for flexible high structural resolution of hydrogen/deuterium-exchange mass spectrometry data

Seetaloo

Kish

Phillips

2021

Preprint

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“…To investigate whether the thermodynamic and kinetic differences associated with the formation of an intramolecular disulfide bond were related to local changes in structure or dynamics, hydrogen-deuterium exchange mass spectrometry (HDX-MS) experiments were conducted. This implementation of HDX-MS uses a novel fully-automated system capable measuring hydrogendeuterium exchange in the millisecond to minutes time scale [21] . Post labelling, online pepsin digestion was conducted and complete sequence coverage achieved in the resulting peptide map (Figure S. 9).…”

Section: Methodsmentioning

confidence: 99%

“…The Fc constructs were used as surrogates for C239i IgG since it has been well established that the antibody binding fragment (Fab) does not affect the stability of the CH2 and CH3 domains [19,20] . Chemical denaturation experiments, differential scanning calorimetry and millisecond HDX mass spectrometry [21] were used to probe the stability, dynamics and structures of the CH2 and CH3 domains in each of the enriched states. Together, these studies provide insight into the conditions under which different thiol states interconvert, their relative stabilities and the conformational changes that occur upon formation of an additional disulfide bond.…”

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confidence: 99%

Interconversion of unexpected thiol states affects stability, structure and dynamics in engineered antibody for site-specific conjugation

Orozco¹,

Edgeworth

Devine

et al. 2020

Preprint

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Antibody drug conjugates have become one of the most actively developed classes of drugs in recent years. Their great potential comes from combining the strengths of large and small molecule therapeutics: the exquisite specificity of antibodies and the highly potent nature of cytotoxic compounds. More recently, the approach of engineering antibody drug conjugate scaffolds to achieve highly controlled drug to antibody ratios has focused on substituting or inserting cysteines to facilitate site-specific conjugation. Herein, we characterise an antibody scaffold engineered with an inserted cysteine that formed an unexpected disulfide bridge. A combination of mass spectrometry and biophysical techniques have been used to understand how the additional disulfide bridge forms, interconverts and changes the stability and structural dynamics of the antibody. Insight is gained into the local and global destabilisation associated with the engineering and subsequent disulfide bonded variant that will inform future engineering strategies.

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“…Kish et al developed a fully automated online flow mixing and quenching system, allowing reproducible HDX measurements between 50 ms and 5 min, with a 1 ms timescale resolution and temperature control (0–25°C) ( Kish et al, 2019 ). The authors used the setup to uncover novel mechanistic details regarding the structural dynamics involved in the allosteric regulation of GlyP.…”

Section: Hydrogen-deuterium Exchange-mass Spectrometrymentioning

confidence: 99%

Structural Proteomics Methods to Interrogate the Conformations and Dynamics of Intrinsically Disordered Proteins

Beveridge

Calabrese

2021

Front. Chem.

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Intrinsically disordered proteins (IDPs) and regions of intrinsic disorder (IDRs) are abundant in proteomes and are essential for many biological processes. Thus, they are often implicated in disease mechanisms, including neurodegeneration and cancer. The flexible nature of IDPs and IDRs provides many advantages, including (but not limited to) overcoming steric restrictions in binding, facilitating posttranslational modifications, and achieving high binding specificity with low affinity. IDPs adopt a heterogeneous structural ensemble, in contrast to typical folded proteins, making it challenging to interrogate their structure using conventional tools. Structural mass spectrometry (MS) methods are playing an increasingly important role in characterizing the structure and function of IDPs and IDRs, enabled by advances in the design of instrumentation and the development of new workflows, including in native MS, ion mobility MS, top-down MS, hydrogen-deuterium exchange MS, crosslinking MS, and covalent labeling. Here, we describe the advantages of these methods that make them ideal to study IDPs and highlight recent applications where these tools have underpinned new insights into IDP structure and function that would be difficult to elucidate using other methods.

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Allosteric regulation of glycogen phosphorylase solution phase structural dynamics at high spatial resolution

Cited by 13 publications

References 44 publications

HDfleX: Software for flexible high structural resolution of hydrogen/deuterium-exchange mass spectrometry data

HDfleX: Software for flexible high structural resolution of hydrogen/deuterium-exchange mass spectrometry data

Interconversion of unexpected thiol states affects stability, structure and dynamics in engineered antibody for site-specific conjugation

Structural Proteomics Methods to Interrogate the Conformations and Dynamics of Intrinsically Disordered Proteins

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