Mass Spectrometry-Based Structural Proteomics for Metal Ion/Protein Binding Studies

Yan-chun, Lin; Gross, Michael L.

doi:10.3390/biom12010135

Cited by 6 publications

(7 citation statements)

References 150 publications

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“…Variable stoichiometry combinations of hetero‐dodecamers from 12:0 to 0:12 were identified by nMS, SID for each individual hetero‐dodecamers further revealed the lateral symmetry in the subunit arrangement, greatly improve the understanding of catalytic mechanism of PDX heterocomplexes and further explain the correlation between the catalytic activity with PDX1.2‐PDX1.3 stoichiometry (Novikova et al, 2021). Additionally, Lin and co‐workers (Lin & Gross, 2022) recently found that the sialyation, especially Neu5Gc, can stabilize transferrin conformation and inhibit its dimerization, furtherly improving its association with iron and Aβ, ultimately resulting in the transferrin‐mediated Aβ‐iron cellular co‐transporting.…”

Section: Applicationsmentioning

confidence: 99%

Native top‐down mass spectrometry for higher‐order structural characterization of proteins and complexes

Liu

Xia

2022

Mass Spectrometry Reviews

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Progress in structural biology research has led to a high demand for powerful and yet complementary analytical tools for structural characterization of proteins and protein complexes. This demand has significantly increased interest in native mass spectrometry (nMS), particularly native top‐down mass spectrometry (nTDMS) in the past decade. This review highlights recent advances in nTDMS for structural research of biological assemblies, with a particular focus on the extra multi‐layers of information enabled by TDMS. We include a short introduction of sample preparation and ionization to nMS, tandem fragmentation techniques as well as mass analyzers and software/analysis pipelines used for nTDMS. We highlight unique structural information offered by nTDMS and examples of its broad range of applications in proteins, protein‐ligand interactions (metal, cofactor/drug, DNA/RNA, and protein), therapeutic antibodies and antigen‐antibody complexes, membrane proteins, macromolecular machineries (ribosome, nucleosome, proteosome, and viruses), to endogenous protein complexes. The challenges, potential, along with perspectives of nTDMS methods for the analysis of proteins and protein assemblies in recombinant and biological samples are discussed.

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Section: Applicationsmentioning

confidence: 99%

Native top‐down mass spectrometry for higher‐order structural characterization of proteins and complexes

Liu

Xia

2022

Mass Spectrometry Reviews

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“…For more discussion of this point, we cite a recent review of our efforts to understand metal-ion interactions by MS-based footprinting and HDX. 35 ■ EXPERIMENTAL PROCEDURES Materials. All chemicals, proteases, and solvents were purchased from Sigma-Aldrich (St. Louis, MO) unless otherwise stated.…”

Section: ■ Introductionmentioning

confidence: 99%

Hydrogen/Deuterium Exchange Mass Spectrometry Provides Insights into the Role of Drosophila Testis-Specific Myosin VI Light Chain AndroCaM

Li,

Jethva,

Rohrs

et al. 2024

Biochemistry

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In Drosophila testis, myosin VI plays a special role, distinct from its motor function, by anchoring components to the unusual actin-based structures (cones) that are required for spermatid individualization. For this, the two calmodulin (CaM) light-chain molecules of myosin VI are replaced by androcam (ACaM), a related protein with 67% identity to CaM. Although ACaM has a similar bi-lobed structure to CaM, with two EF handtype Ca 2+ binding sites per lobe, only one functional Ca 2+ binding site operates in the amino-terminus. To understand this light chain substitution, we used hydrogen−deuterium exchange mass spectrometry (HDX-MS) to examine dynamic changes in ACaM and CaM upon Ca 2+ binding and interaction with the two CaM binding motifs of myosin VI (insert2 and IQ motif). HDX-MS reveals that binding of Ca 2+ to ACaM destabilizes its N-lobe but stabilizes the entire C-lobe, whereas for CaM, Ca 2+ binding induces a pattern of alternating stabilization/destabilization throughout. The conformation of this stable holo-C-lobe of ACaM seems to be a "prefigured" version of the conformation adopted by the holo-C-lobe of CaM for binding to insert2 and the IQ motif of myosin VI. Strikingly, the interaction of holo-ACaM with either peptide converts the holo-N-lobe to its Ca 2+ -free, more stable, form. Thus, ACaM in vivo should bind the myosin VI light chain sites in an apo-N-lobe/holo-C-lobe state that cannot fulfill the Ca 2+ -related functions of holo-CaM required for myosin VI motor assembly and activity. These findings indicate that inhibition of myosin VI motor activity is a precondition for transition to an anchoring function.

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“…These techniques induce fragmentation of the peptide without major scrambling of hydrogen and deuterium, permitting the location of deuterium to be accurately determined. 15 A recent study by the FDA 16 monitored, using HDX-MS, changes in solvent accessibilities of stressed mAbs relative to an unstressed control incubated at 25 ± 2 °C, 60 ± 5% relative humidity (RH) for 6 months. Although this study provided a broad survey across several antibodies, there are still challenges to improving the spatial resolution (i.e., peptide length or number of unique peptides) and to employing robust statistical analysis for accurate and reliable measurements of subtle structural changes by using HDX-MS methods.…”

Section: ■ Introductionmentioning

confidence: 99%

“…Tandem MS (MS/MS) fragmentation such as electron transfer dissociation, electron capture dissociation, and ultraviolet photon dissociation may also be adopted. These techniques induce fragmentation of the peptide without major scrambling of hydrogen and deuterium, permitting the location of deuterium to be accurately determined . A recent study by the FDA monitored, using HDX-MS, changes in solvent accessibilities of stressed mAbs relative to an unstressed control incubated at 25 ± 2 °C, 60 ± 5% relative humidity (RH) for 6 months.…”

Section: Introductionmentioning

confidence: 99%

Characterization of Higher Order Structural Changes of a Thermally Stressed Monoclonal Antibody via Mass Spectrometry Footprinting and Other Biophysical Approaches

Lin,

Moyle,

Beaumont

et al. 2023

Anal. Chem.

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Mass Spectrometry-Based Structural Proteomics for Metal Ion/Protein Binding Studies

Cited by 6 publications

References 150 publications

Native top‐down mass spectrometry for higher‐order structural characterization of proteins and complexes

Native top‐down mass spectrometry for higher‐order structural characterization of proteins and complexes

Hydrogen/Deuterium Exchange Mass Spectrometry Provides Insights into the Role of Drosophila Testis-Specific Myosin VI Light Chain AndroCaM

Characterization of Higher Order Structural Changes of a Thermally Stressed Monoclonal Antibody via Mass Spectrometry Footprinting and Other Biophysical Approaches

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