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225 results on '"Ion-mobility spectrometry–mass spectrometry"'

1. Analysis of Peptide Stereochemistry in Single Cells by Capillary Electrophoresis–Trapped Ion Mobility Spectrometry Mass Spectrometry

Author

Jonathan V. Sweedler, Hsiao Wei Liao, David H. Mast, and Elena V. Romanova

Subjects
Proteomics, chemistry.chemical_classification, Neuropeptide Gene, Ion-mobility spectrometry, Stereochemistry, 010401 analytical chemistry, Cell, Electrophoresis, Capillary, Peptide, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Mass Spectrometry, Article, 0104 chemical sciences, Analytical Chemistry, medicine.anatomical_structure, Capillary electrophoresis, Ion-mobility spectrometry–mass spectrometry, chemistry, Single-cell analysis, Ion Mobility Spectrometry, medicine, Peptides
Abstract

Single cell analysis strives to probe molecular heterogeneity in morphologically similar cell populations through quantitative or qualitative measurements of genetic, proteomic, or metabolic products. Here, we applied mass analysis of single neurons to investigate cell-cell signaling peptides. The multiplicity of endogenous cell-cell signaling peptides is a common source of chemical diversity among cell populations. Certain peptides can undergo post-translational isomerization of select residues, which has important physiological consequences. The limited number of single cell analysis techniques that are sensitive to peptide stereochemistry make it challenging to study isomerization at the individual cell level. We performed capillary electrophoresis (CE) with mass spectrometry (MS) detection to characterize the peptide content of single cells. Using complementary trapped ion mobility spectrometry (TIMS) separations, we measured the stereochemical configurations of three neuropeptide gene products derived from the pleurin precursor in individual neurons (N = 3) isolated from the central nervous system of Aplysia californica. An analysis of the resultant mobility profiles indicated >98% of the detectable pleurin-derived peptides exist as the non-isomerized, all-L forms in individual neuron cell bodies. However, we observed 44% of the Plrn2 peptide from the pleurin precursor was present as the isomerized, D-residue-containing form in the nerve tissue. These findings demonstrate an unusual distribution of isomerized peptides in A. californica and establish CE–TIMS MS as a powerful analytical tool for investigating peptide stereochemistry at the single cell level.

Published
2021

2. Rapid Characterization of Emerging Per- and Polyfluoroalkyl Substances in Aqueous Film-Forming Foams Using Ion Mobility Spectrometry–Mass Spectrometry

Author

James N. Dodds, Weihsueh A. Chiu, Yu-Syuan Luo, Noor A. Aly, Ivan Rusyn, Erin S. Baker, Mark J. Strynar, and James McCord

Subjects
Fluorocarbons, Aqueous solution, Chromatography, Chemistry, Ion-mobility spectrometry, Water, General Chemistry, 010501 environmental sciences, Contamination, Mass spectrometry, 01 natural sciences, Article, Homologous series, chemistry.chemical_compound, Ion-mobility spectrometry–mass spectrometry, Tandem Mass Spectrometry, Adverse health effect, Ion Mobility Spectrometry, Environmental Chemistry, Water Pollutants, Chemical, 0105 earth and related environmental sciences
Abstract

Aqueous film-forming foams (AFFF) are mixtures formulated with numerous hydrocarbon- and fluoro-containing surfactants. AFFF use leads to environmental releases of unknown per- and polyfluoroalkyl substances (PFAS). AFFF composition is seldom disclosed, and their use elicits concerns from both regulatory agencies and the public because PFAS are persistent in the environment and potentially associated with adverse health effects. In this study, we demonstrate the use of coupled liquid chromatography, ion mobility spectrometry, and mass spectrometry (LC-IMS-MS) to rapidly characterize both known and unknown PFAS in AFFF. Ten AFFF formulations from seven brands were analyzed using LC-IMS-MS in both negative and positive ion modes. Untargeted analysis of the formulations was followed by feature identification of PFAS-like features utilizing database matching, mass defect and homologous series evaluation, and MS/MS fragmentation experiments. Across the tested AFFF formulations, we identified 33 homologous series; only ten of these homologous series have been previously reported. Among tested AFFF, the FireStopper (n = 85) contained the greatest number of PFAS-like features and Phos-Check contained zero. This work demonstrates that LC-IMS-MS-enabled untargeted analysis of complex formulations, followed by feature identification using data-processing algorithms, can be used for rapid exposure characterization of known and putative PFAS during fire suppression-related contamination events.

Published
2020

3. Structural Analysis of the Glycoprotein Complex Avidin by Tandem-Trapped Ion Mobility Spectrometry–Mass Spectrometry (Tandem-TIMS/MS)

Author

Tyler C. Cropley, Mark E. Ridgeway, Melvin A. Park, Fanny C. Liu, and Christian Bleiholder

Subjects
biology, Protein Conformation, Chemistry, Ion-mobility spectrometry, 010401 analytical chemistry, Avidin, 010402 general chemistry, Mass spectrometry, Tandem mass spectrometry, 01 natural sciences, Article, 0104 chemical sciences, Analytical Chemistry, Ion-mobility spectrometry–mass spectrometry, Protein structure, Tetramer, Tandem Mass Spectrometry, Glycoprotein complex, Ion Mobility Spectrometry, biology.protein, Biophysics
Abstract

Glycoproteins play a central role in many biological processes including disease mechanisms. Nevertheless, because glycoproteins are heterogeneous entities, it remains unclear how glycosylation modulates the protein structure and function. Here, we assess the ability of tandem-trapped ion mobility spectrometry – mass spectrometry (tandem-TIMS/MS) to characterize the structure and sequence of the homo-tetrameric glycoprotein avidin. We show that (1) tandem-TIMS/MS retains native-like avidin tetramers with deeply buried solvent particles; (2) applying high activation voltages in the interface of tandem-TIMS results in collision-induced dissociation (CID) of avidin tetramers into compact monomers, dimers, and trimers with cross sections consistent with x-ray structures and reports from surface-induced dissociation (SID); (3) avidin oligomers are best described as heterogeneous ensembles with (essentially) random combinations of monomer glycoforms; (4) native top-down sequence analysis of the avidin tetramer is possible by CID in tandem-TIMS. Overall, our results demonstrate that tandem-TIMS/MS has the potential to correlate individual proteoforms to variations in protein structure.

Published
2020

4. Rapid Characterization of Per- and Polyfluoroalkyl Substances (PFAS) by Ion Mobility Spectrometry–Mass Spectrometry (IMS-MS)

Author

Zachary R. Hopkins, James N. Dodds, Erin S. Baker, and Detlef R.U. Knappe

Subjects
Pollutant, Pollution, Drift tube, Hydrocarbons, Fluorinated, Molecular Structure, Polymers, Ion-mobility spectrometry, Chemistry, media_common.quotation_subject, 010401 analytical chemistry, 010402 general chemistry, Health outcomes, 01 natural sciences, Mass Spectrometry, Article, 0104 chemical sciences, Analytical Chemistry, Characterization (materials science), Ion-mobility spectrometry–mass spectrometry, Environmental water, Environmental chemistry, Ion Mobility Spectrometry, media_common
Abstract

Per- and polyfluoroalkyl substances (PFAS) are an ensemble of persistent organic pollutants of global interest because of their associations with adverse health outcomes. Currently, environmental PFAS pollution is prolific as a result of the widespread manufacturing of these compounds and their chemical persistence. In this work, we demonstrate the advantages of adding ion mobility spectrometry (IMS) separation to existing LC-MS workflows for PFAS analysis. Using a commercially available drift tube IMS-MS, we characterized PFAS species and isomeric content in both analytical standards and environmental water samples. Molecular trendlines based on intrinsic mass and structural relationships were also explored for individual PFAS subclasses (e.g. PFSA, PFCA, etc.). Results from rapid IMS-MS analyses provided a link between mass and collision cross sections (CCS) for specific PFAS families and are linked to compositional differences in molecular structure. In addition, CCS values provide additional confidence of annotating prioritized features in untargeted screening studies for potential environmental pollutants. Results from this study show that the IMS separation provides novel information to support traditional LC-MS PFAS analyses and will greatly benefit the evaluation of unknown pollutants in future environmental studies.

Published
2020

5. Predicting Breast Cancer by Paper Spray Ion Mobility Spectrometry Mass Spectrometry and Machine Learning

Author

Ewelina P. Dutkiewicz, Chih-Lin Chen, Hua-Yi Hsieh, Cheng-Chih Hsu, Ying-Chen Huang, Ming-Yang Wang, Hsin-Hsiang Chung, and Bo-Rong Chen

Subjects
Paper, Core needle, Spectrometry, Mass, Electrospray Ionization, Ion-mobility spectrometry, Electrospray ionization, Breast Neoplasms, 010402 general chemistry, Machine learning, computer.software_genre, Mass spectrometry, 01 natural sciences, Analytical Chemistry, Machine Learning, Breast cancer, Ion Mobility Spectrometry, medicine, Humans, business.industry, Chemistry, 010401 analytical chemistry, medicine.disease, Mass spectrometric, 0104 chemical sciences, Ion-mobility spectrometry–mass spectrometry, Female, Artificial intelligence, Asymmetric waveform, business, computer, Algorithms
Abstract

Paper spray ionization has been used as a fast sampling/ionization method for the direct mass spectrometric analysis of biological samples at ambient conditions. Here, we demonstrated that by utilizing paper spray ionization-mass spectrometry (PSI-MS) coupled with field asymmetric waveform ion mobility spectrometry (FAIMS), predictive metabolic and lipidomic profiles of routine breast core needle biopsies could be obtained effectively. By the combination of machine learning algorithms and pathological examination reports, we developed a classification model, which has an overall accuracy of 87.5% for an instantaneous differentiation between cancerous and noncancerous breast tissues utilizing metabolic and lipidomic profiles. Our results suggested that paper spray ionization-ion mobility spectrometry-mass spectrometry (PSI-IMS-MS) is a powerful approach for rapid breast cancer diagnosis based on altered metabolic and lipidomic profiles.

Published
2019

6. Improving the Speed and Selectivity of Newborn Screening Using Ion Mobility Spectrometry-Mass Spectrometry

Author

James N. Dodds and Erin S. Baker

Subjects
Newborn screening, Drift tube, Chromatography, Chemistry, Ion-mobility spectrometry, Infant, Newborn, food and beverages, Mass spectrometry, Mass Spectrometry, Article, Analytical Chemistry, High-Throughput Screening Assays, Ion-mobility spectrometry–mass spectrometry, Neonatal Screening, embryonic structures, Ion Mobility Spectrometry, Humans, Dried blood, Biomarkers
Abstract

Detection and diagnosis of congenital disorders is the principal aim of newborn screening (NBS) programs worldwide. Mass spectrometry (MS) has become the preferred primary testing method for high-throughput NBS sampling because of its speed and selectivity. However, the ever-increasing list of NBS biomarkers included in expanding panels creates unique analytical challenges for multiplexed MS assays due to isobaric/isomeric overlap and chimeric fragmentation spectra. Since isobaric and isomeric systems limit the diagnostic power of current methods and require costly follow-up exams due to many false-positive results, here, we explore the utility of ion mobility spectrometry (IMS) to enhance the accuracy of MS assays for primary (tier 1) screening. Our results suggest that ∼400 IMS resolving power would be required to confidently assess most NBS biomarkers of interest in dried blood spots (DBSs) that currently require follow-up testing. While this level of selectivity is unobtainable with most commercially available platforms, the separations detailed here for a commercially available drift tube IMS (Agilent 6560 with high-resolution demultiplexing, HRdm) illustrate the unique capabilities of IMS to separate many diagnostic NBS biomarkers from interferences. Furthermore, to address the need for increased speed of NBS analyses, we utilized an automated solid-phase extraction (SPE) system for ∼10 s sampling of simulated NBS samples prior to IMS-MS. This proof-of-concept work demonstrates the unique capabilities of SPE-IMS-MS for high-throughput sample introduction and enhanced separation capacity conducive for increasing speed and accuracy for NBS.

Published
2021

7. Tandem‐trapped ion mobility spectrometry/mass spectrometry coupled with ultraviolet photodissociation

Author

Mark E. Ridgeway, Melvin A. Park, Christian Bleiholder, Christopher A. Wootton, Fanny C. Liu, Alina Theisen, J. S. Raaj Vellore Winfred, Jusung Lee, and Nick C. Polfer

Subjects
Tandem, Ion-mobility spectrometry, Chemistry, Organic Chemistry, Photodissociation, Analytical chemistry, Mass spectrometry, Proteomics, Article, Dissociation (chemistry), Analytical Chemistry, Ion, Ion-mobility spectrometry–mass spectrometry, Spectroscopy
Abstract

RATIONALE Tandem-ion mobility spectrometry/mass spectrometry methods have recently gained traction for the structural characterization of proteins and protein complexes. However, ion activation techniques currently coupled with tandem-ion mobility spectrometry/mass spectrometry methods are limited in their ability to characterize structures of proteins and protein complexes. METHODS Here, we describe the coupling of the separation capabilities of tandem-trapped ion mobility spectrometry/mass spectrometry (tTIMS/MS) with the dissociation capabilities of ultraviolet photodissociation (UVPD) for protein structure analysis. RESULTS We establish the feasibility of dissociating intact proteins by UV irradiation at 213 nm between the two TIMS devices in tTIMS/MS and at pressure conditions compatible with ion mobility spectrometry (2-3 mbar). We validate that the fragments produced by UVPD under these conditions result from a radical-based mechanism in accordance with prior literature on UVPD. The data suggest stabilization of fragment ions produced from UVPD by collisional cooling due to the elevated pressures used here ("UVnoD2"), which otherwise do not survive to detection. The data account for a sequence coverage for the protein ubiquitin comparable to recent reports, demonstrating the analytical utility of our instrument in mobility-separating fragment ions produced from UVPD. CONCLUSIONS The data demonstrate that UVPD carried out at elevated pressures of 2-3 mbar yields extensive fragment ions rich in information about the protein and that their exhaustive analysis requires IMS separation post-UVPD. Therefore, because UVPD and tTIMS/MS each have been shown to be valuable techniques on their own merit in proteomics, our contribution here underscores the potential of combining tTIMS/MS with UVPD for structural proteomics.

Published
2021

8. Analysis of Per- and Polyfluoroalkyl Substances in Houston Ship Channel and Galveston Bay Following a Large-Scale Fire Using Ion-Mobility-Spectrometry-Mass Spectrometry

Author

Alexandra C Cordova, Gaston A. Casillas, Ivan Rusyn, MaKayla Foster, Yu-Syuan Luo, Erin S. Baker, Alan Valdiviezo, and Noor A. Aly

Subjects
Pollutant, Fluorocarbons, Environmental Engineering, Deer, General Medicine, Contamination, Mass spectrometry, Industrial fire, Article, Ion-mobility spectrometry–mass spectrometry, Bays, Tandem Mass Spectrometry, Environmental chemistry, Ion Mobility Spectrometry, Environmental Chemistry, Environmental science, Animals, Surface water, Bay, Water Pollutants, Chemical, General Environmental Science, Exposure assessment, Chromatography, Liquid
Abstract

Per- and polyfluoroalkyl substances (PFAS) are persistent organic pollutants of concern because of their ubiquitous presence in surface and ground water; analytical methods that can be used for rapid comprehensive exposure assessment and fingerprinting of PFAS are needed. Following the fires at the Intercontinental Terminals Company (ITC) in Deer Park, TX in 2019, large quantities of PFAS-containing firefighting foams were deployed. The release of these substances into the Houston Ship Channel/Galveston Bay (HSC/GB) prompted concerns over the extent and level of PFAS contamination. A targeted liquid chromatography-tandem mass spectrometry (LC-MS/MS)-based study of temporal and spatial patterns of PFAS associated with this incident revealed presence of 7 species; their levels gradually decreased over a 6-month period. Because the targeted LC-MS/MS analysis was focused on about 30 PFAS molecules, it may have missed other PFAS compounds present in firefighting foams. Therefore, we utilized untargeted LC-ion mobility spectrometry-mass spectrometry (LC-IMS-MS)-based analytical approach for a more comprehensive characterization of PFAS in these water samples. We analyzed 31 samples from 9 sites in the HSC/GB that were collected over 5 months after the incident. Our data showed that additional 19 PFAS were detected in surface water of HSC/GB, most of them decreased gradually after the incident. PFAS features detected by LC-MS/MS correlated well in abundance with LC-IMS-MS data; however, LC-IMS-MS identified a number of additional PFAS, many known to be components of firefighting foams. These findings therefore illustrate that untargeted LC-IMS-MS improved our understanding of PFAS presence in complex environmental samples.

Published
2021

9. Data Processing Workflow to Identify Structurally Related Compounds in Petroleum Substances Using Ion Mobility Spectrometry-Mass Spectrometry

Author

Ivan Rusyn, Alexandra C Cordova, Thomas J. McDonald, Alina T. Roman-Hubers, Noor A. Aly, Weihsueh A. Chiu, Erin S. Baker, Fred A. Wright, and Dillon T Lloyd

Subjects
Chromatography, Kendrick mass, Ion-mobility spectrometry, General Chemical Engineering, Energy Engineering and Power Technology, Mass spectrometry, Article, Characterization (materials science), Homologous series, chemistry.chemical_compound, Fuel Technology, Workflow, Ion-mobility spectrometry–mass spectrometry, chemistry, Gasoline
Abstract

Ion mobility spectrometry coupled with mass spectrometry (IMS-MS) is a post-ionization separation technique that can be used for rapid multidimensional analyses of complex samples. IMS-MS offers untargeted analysis, including ion-specific conformational data derived as collisional cross section (CCS) values. Here, we combine nitrogen gas drift tube CCS ((DT)CCS(N2)) and Kendrick mass defect (KMD) analyses based on CH2 and H functional units to enable compositional analyses of petroleum substances. First, polycyclic aromatic compound standards were analyzed by IMS-MS to demonstrate how CCS assists the identification of isomeric species in homologous series. Next, we used case studies of a gasoline standard previously characterized for paraffin, isoparaffin, aromatic, naphthene, and olefinic (PIANO) compounds, and a crude oil sample to demonstrate the application of the KMD analyses and CCS filtering. Finally, we propose a workflow that enables confident molecular formula assignment to the IMS-MS-derived features in petroleum samples. Collectively, this work demonstrates how rapid untargeted IMS-MS analysis and the proposed data processing workflow can be used to provide confident compositional characterization of hydrocarbon-containing substances.

Published
2021

10. Utilizing ion mobility spectrometry-mass spectrometry for the characterization and detection of persistent organic pollutants and their metabolites

Author

Ivan Rusyn, MaKayla Foster, Yu-Syuan Luo, Erin S. Baker, James N. Dodds, Noor A. Aly, and Fabian A. Grimm

Subjects
Pollutant, Ion-mobility spectrometry, Electrospray ionization, Mass spectrometry, Biochemistry, Environmental impact of pharmaceuticals and personal care products, Polychlorinated Biphenyls, Mass Spectrometry, Article, Analytical Chemistry, chemistry.chemical_compound, Persistent Organic Pollutants, Ion-mobility spectrometry–mass spectrometry, chemistry, Pharmaceutical Preparations, Environmental chemistry, Ion Mobility Spectrometry, Humans, Pesticides, Xenobiotic, Exposure assessment, Environmental Monitoring
Abstract

Persistent organic pollutants (POPs) are xenobiotic chemicals of global concern due to their long-range transport capabilities, persistence, ability to bioaccumulate, and potential to have negative effects on human health and the environment. Identifying POPs in both the environment and human body is therefore essential for assessing potential health risks, but their diverse range of chemical classes challenge analytical techniques. Currently, platforms coupling chromatography approaches with mass spectrometry (MS) are the most common analytical methods employed to evaluate both parent POPs and their respective metabolites and/or degradants in samples ranging from d rinking water to biofluids. Unfortunately, different types of analyses are commonly needed to assess both the parent and metabolite/degradant POPs from the various chemical classes. The multiple time-consuming analyses necessary thus present a number of technical and logistical challenges when rapid evaluations are needed and sample volumes are limited. To address these challenges, we characterized 64 compounds including parent per- and polyfluoroalkyl substances (PFAS), pesticides, polychlorinated biphenyls (PCBs), industrial chemicals, and pharmaceuticals and personal care products (PPCPs), in addition to their metabolites and/or degradants, using ion mobility spectrometry coupled with MS (IMS-MS) as a potential rapid screening technique. Different ionization sources including electrospray ionization (ESI) and atmospheric pressure photoionization (APPI) were employed to determine optimal ionization for each chemical. Collectively, this study advances the field of exposure assessment by structurally characterizing the 64 important environmental pollutants, assessing their best ionization sources, and evaluating their rapid screening potential with IMS-MS.

Published
2021

11. Exploring the Conformational Space of Growth-Hormone-Releasing Hormone Analogues Using Dopant Assisted Trapped Ion Mobility Spectrometry–Mass Spectrometry

Author

Javier Moreno, Francisco Fernandez-Lima, and Kevin Jeanne Dit Fouque

Subjects
Models, Molecular, Dopant, Protein Conformation, Chemistry, Growth Hormone-Releasing Hormone, Growth hormone–releasing hormone, Surfaces, Coatings and Films, Ion-mobility spectrometry–mass spectrometry, Ion Mobility Spectrometry, Solvents, Materials Chemistry, Biophysics, Physical and Theoretical Chemistry, Structural motif, Hormone
Abstract

Recently, we proposed a high-throughput screening workflow for the elucidation of agonistic or antagonistic growth hormone-releasing hormone (GHRH) potencies based on structural motif descriptors as a function of the starting solution. In the present work, we revisited the influence of solution and gas-phase GHRH molecular microenvironment using trapped ion mobility-mass spectrometry (TIMS-MS). The effect of the starting solvent composition (10 mM ammonium acetate (NH

Published
2019

12. Substance P in the Gas Phase: Conformational Changes and Dissociations Induced by Collisional Activation in a Drift Tube

Author

David H. Russell, Zhichao Zhang, Daniel R. Fuller, Daniel W. Woodall, Christopher R. Conant, and David E. Clemmer

Subjects
Ion-mobility spectrometry, Chemistry, digestive, oral, and skin physiology, 010401 analytical chemistry, Activation energy, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Potential energy, Article, 0104 chemical sciences, Ion, Ion-mobility spectrometry–mass spectrometry, Structural Biology, Chemical physics, Thermochemistry, Conformational isomerism, Spectroscopy
Abstract

The work presented below is related to our companion paper in this issue, entitled: Substance P in solution: trans-to-cis configurational changes of penultimate prolines initiate non-enzymatic peptide bond cleavages. Two-dimensional ion mobility spectrometry (IMS-IMS) and mass spectrometry techniques are used to investigate structural transitions for [M+3H](3+) ions of substance P (subP) upon collisional activation (CA) in the gas phase. In this approach, different conformations of ions having a specified mobility are selected after an initial IMS separation, collisionally activated to produce new conformers, and these product structures are separated again using a second IMS region. In this way it is possible to follow folding and unfolding transitions of different conformations. The analysis shows evidence for five conformations. Unlike other systems, every transition is irreversible. Studies as a function of activation voltage are used to discern pathways of structural changes prior to reaching the energy required for dissociation. Thresholds associated with the onsets of transitions are calibrated to obtain estimates of the energetic barriers between different structures and semi-quantitative potential-energy diagrams are presented. Overall, barriers associated with structural transitions of [subP+3H](3+) in the absence of solvent are on the order of ~40 kJ∙mol(−1), substantially lower than the ~90 kJ∙mol(−1) required for some similar structural transitions in solutions of ethanol. Comparisons of the transition energies in the gas-phase with thermochemistry for similar transitions in solution provide clues about why reverse transitions are prohibited.

Published
2019

13. Structural signatures of the class III lasso peptide BI-32169 and the branched-cyclic topoisomers using trapped ion mobility spectrometry–mass spectrometry and tandem mass spectrometry

Author

Sylvie Rebuffat, Séverine Zirah, Vikash Bisram, Kevin Jeanne Dit Fouque, Francisco Fernandez-Lima, and Julian D. Hegemann

Subjects
chemistry.chemical_classification, Topoisomer, Collision-induced dissociation, Electron-capture dissociation, Protein Conformation, Stereochemistry, Chemistry, 010401 analytical chemistry, Peptide, 02 engineering and technology, 021001 nanoscience & nanotechnology, Tandem mass spectrometry, Mass spectrometry, Peptides, Cyclic, 01 natural sciences, Biochemistry, 0104 chemical sciences, Analytical Chemistry, Ion-mobility spectrometry–mass spectrometry, Tandem Mass Spectrometry, Covalent bond, Ion Mobility Spectrometry, Protein Isoforms, 0210 nano-technology
Abstract

Lasso peptides are a class of bioactive ribosomally synthesized and post-translationally modified peptides (RiPPs) characterized by a mechanically interlocked topology, where the C-terminal tail of the peptide is threaded and trapped within an N-terminal macrolactam ring. BI-32169 is a class III lasso peptide containing one disulfide bond that further stabilizes the lasso structure. In contrast to its branched-cyclic analog, BI-32169 has higher stability and is known to exert a potent inhibitory activity against the human glucagon receptor. In the present work, tandem mass spectrometry, using collision-induced dissociation (CID) and electron capture dissociation (ECD), and trapped ion mobility spectrometry-mass spectrometry (TIMS-MS) experiments were carried out to evidence specific structural signatures of the two topologies. CID experiments showed similar fragmentation patterns for the two topoisomers, where a part of the C-terminal tail remains covalently linked to the macrolactam ring by the disulfide bond, which cannot clearly constitute a signature of the lasso topology. ECD experiments of BI-32169 showed an increase of hydrogen migration events in the loop region when compared with those of its branched-cyclic topoisomer evidencing specific structural signatures for the lasso topology. The high mobility resolving power of TIMS resulted in the identification of multiple conformations for the protonated species but did not allow the clear differentiation of the two topologies in mixture. When in complex with cesium metal ions, a reduced number of conformations led to a clear identification of the two structures. Experiments reducing and alkylating the disulfide bond of BI-32169 showed that the lasso structure is preserved and heat stable and the associated conformational changes provide new insights about the role of the disulfide bond in the inhibitory activity against the human glucagon receptor. Graphical abstract ᅟ.

Published
2019

14. Validation of ion mobility spectrometry - mass spectrometry as a screening tool to identify type II kinase inhibitors of FGFR1 kinase

Author

Richard A. Norman, Julie A. Tucker, Malcolm Anderson, Helen S. Beeston, Tobias Klein, Alison E. Ashcroft, and Geoffrey A. Holdgate

Subjects
Ion-mobility spectrometry, Kinase, Chemistry, 010401 analytical chemistry, Organic Chemistry, Ligand (biochemistry), Mass spectrometry, 01 natural sciences, 0104 chemical sciences, Analytical Chemistry, Folding (chemistry), stomatognathic diseases, Ion-mobility spectrometry–mass spectrometry, Biochemistry, Unfolded protein response, Protein kinase A, Spectroscopy
Abstract

Rationale The protein kinase FGFR1 regulates cellular processes in human development. As over-activity of FGFR1 is implicated with cancer, effective inhibitors are in demand. Type I inhibitors, which bind to the active form of FGFR1, are less effective than type II inhibitors, which bind to the inactive form. Screening to distinguish between type I and type II inhibitors is required. Methods X-ray crystallography was used to indicate whether a range of potential inhibitors bind to the active or inactive FGFR1 kinase conformation. The binding affinity of each ligand to FGFR1 was measured using biochemical methods. Electrospray ionisation - ion mobility spectrometry - mass spectrometry (ESI-IMS-MS) in conjunction with collision-induced protein unfolding generated a conformational profile of each FGFR1-ligand complex. The results indicate that the protein's conformational profile depends on whether the inhibitor is type I or type II. Results X-ray crystallography confirmed which of the kinase inhibitors bind to the active or inactive form of FGFR1 kinase. Collision-induced unfolding combined with ESI-IMS-MS showed distinct differences in the FGFR1 folding landscape for type I and type II inhibitors. Biochemical studies indicated a similar range of FGFR1 affinities for both types of inhibitors, thus providing confidence that the conformational variations detected using ESI-IMS-MS can be interpretated unequivocally and that this is an effective screening method. Conclusions A robust ESI-IMS-MS method has been implemented to distinguish between the binding mode of type I and type II inhibitors by monitoring the conformational unfolding profile of FGFR1. This rapid method requires low sample concentrations and could be used as a high-throughput screening technique for the characterisation of novel kinase inhibitors.

Published
2021

15. A Comparative Analysis of Analytical Techniques for Rapid Oil Spill Identification

Author

Ivan Rusyn, Alina T. Roman-Hubers, Weihsueh A. Chiu, Erin S. Baker, and Thomas J. McDonald

Subjects
Health, Toxicology and Mutagenesis, Sample (statistics), 010501 environmental sciences, 01 natural sciences, Article, Gas Chromatography-Mass Spectrometry, chemistry.chemical_compound, Environmental Chemistry, Petroleum Pollution, Gasoline, 0105 earth and related environmental sciences, business.industry, 010401 analytical chemistry, Hydrocarbons, 0104 chemical sciences, Ion-mobility spectrometry–mass spectrometry, Petroleum, Petroleum industry, chemistry, Principal component analysis, Environmental science, Biochemical engineering, Gas chromatography, business, Chemical fingerprinting
Abstract

The complex chemical composition of crude oils presents many challenges for rapid chemical characterization in the case of a spill. A number of approaches are currently used to "fingerprint" petroleum-derived samples. Gas chromatography coupled with mass spectrometry (GC-MS) is the most common, albeit not very rapid, technique; however, with GC-MS alone, it is difficult to resolve the complex substances in crude oils. The present study examined the potential application of ion mobility spectrometry-mass spectrometry (IMS-MS) coupled with chem-informatic analyses as an alternative high-throughput method for the chemical characterization of crude oils. We analyzed 19 crude oil samples from on- and offshore locations in the Gulf of Mexico region in the United States using both GC-MS (biomarkers, gasoline range hydrocarbons, and n-alkanes) and IMS-MS (untargeted analysis). Hierarchical clustering, principal component analysis, and nearest neighbor-based classification were used to examine sample similarity and geographical groupings. We found that direct-injection IMS-MS performed either equally or better than GC-MS in the classification of the origins of crude oils. In addition, IMS-MS greatly increased the sample analysis throughput (minutes vs hours per sample). Finally, a tabletop science-to-practice exercise, utilizing both the GC-MS and IMS-MS data, was conducted with emergency response experts from regulatory agencies and the oil industry. This activity showed that the stakeholders found the IMS-MS data to be highly informative for rapid chemical fingerprinting of complex substances in general and specifically advantageous for accurate and confident source-grouping of crude oils. Collectively, the present study shows the utility of IMS-MS as a technique for rapid fingerprinting of complex samples and demonstrates its advantages over traditional GC-MS-based analyses when used for decision-making in emergency situations. Environ Toxicol Chem 2021;40:1034-1049. © 2020 SETAC.

Published
2021

16. AutoCCS: Automated collision cross section calculation software for ion mobility spectrometry-mass spectrometry

Author

Ian K. Webb, Christopher R. Conant, Aivett Bilbao, Mowei Zhou, Yehia M. Ibrahim, Kent J. Bloodsworth, Richard D. Smith, Samuel H. Payne, Joon-Yong Lee, Ailin Li, Thomas O. Metz, John C. Fjeldsted, Christer Jansson, Xueyun Zheng, Kim K. Hixson, Jesse W. Wilson, and Daniel J. Orton

Subjects
Statistics and Probability, Analyte, Computer science, business.industry, Ion-mobility spectrometry, 010401 analytical chemistry, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Biochemistry, Pipeline (software), 0104 chemical sciences, Computer Science Applications, Computational science, Characterization (materials science), Computational Mathematics, Ion-mobility spectrometry–mass spectrometry, Software, Computational Theory and Mathematics, Calibration, business, Molecular Biology
Abstract

Motivation Ion mobility spectrometry (IMS) separations are increasingly used in conjunction with mass spectrometry (MS) for separation and characterization of ionized molecular species. Information obtained from IMS measurements includes the ion’s collision cross section (CCS), which reflects its size and structure and constitutes a descriptor for distinguishing similar species in mixtures that cannot be separated using conventional approaches. Incorporating CCS into MS-based workflows can improve the specificity and confidence of molecular identification. At present, there is no automated, open-source pipeline for determining CCS of analyte ions in both targeted and untargeted fashion, and intensive user-assisted processing with vendor software and manual evaluation is often required. Results We present AutoCCS, an open-source software to rapidly determine CCS values from IMS-MS measurements. We conducted various IMS experiments in different formats to demonstrate the flexibility of AutoCCS for automated CCS calculation: (i) stepped-field methods for drift tube-based IMS (DTIMS), (ii) single-field methods for DTIMS (supporting two calibration methods: a standard and a new enhanced method) and (iii) linear calibration for Bruker timsTOF and non-linear calibration methods for traveling wave based-IMS in Waters Synapt and Structures for Lossless Ion Manipulations. We demonstrated that AutoCCS offers an accurate and reproducible determination of CCS for both standard and unknown analyte ions in various IMS-MS platforms, IMS-field methods, ionization modes and collision gases, without requiring manual processing. Availability and implementation https://github.com/PNNL-Comp-Mass-Spec/AutoCCS. Supplementary information Supplementary data are available at Bioinformatics online. Demo datasets are publicly available at MassIVE (Dataset ID: MSV000085979).

Published
2020

17. Comparison of gaseous ubiquitin ion structures obtained from a solid and solution matrix using ion mobility spectrometry/mass spectrometry

Author

Andjoe A S Sampat, Dean R. Jarois, Tarick J. El-Baba, Ellen D. Inutan, Christopher B. Lietz, Sarah Trimpin, Efstathios A. Elia, Casey D. Foley, David E. Clemmer, and Santosh Karki

Subjects
Ions, Ubiquitin, Chemistry, Electrospray ionization, 010401 analytical chemistry, Organic Chemistry, Analytical chemistry, Mass spectrometry, 01 natural sciences, Mass Spectrometry, 0104 chemical sciences, Analytical Chemistry, Ion, law.invention, Solvent, Ion-mobility spectrometry–mass spectrometry, law, Ionization, Desorption, Ion Mobility Spectrometry, Solvents, Gases, Crystallization, Spectroscopy
Abstract

Rationale Examining surface protein conformations, and especially achieving this with spatial resolution, is an important goal. The recently discovered ionization processes offer spatial-resolution measurements similar to matrix-assisted laser desorption/ionization (MALDI) and produce charge states similar to electrospray ionization (ESI) extending higher-mass protein applications directly from surfaces on high-performance mass spectrometers. Studying a well-interrogated protein by ion mobility spectrometry-mass spectrometry (IMS-MS) to access effects on structures using a solid vs. solvent matrix may provide insights. Methods Ubiquitin was studied by IMS-MS using new ionization processes with commercial and homebuilt ion sources and instruments (Waters SYNAPT G2(S)) and homebuilt 2 m drift-tube instrument; MS™ sources). Mass-to-charge and drift-time (td )-measurements are compared for ubiquitin ions obtained by inlet and vacuum ionization using laserspray ionization (LSI), matrix- (MAI) and solvent-assisted ionization (SAI), respectively, and compared with those from ESI under conditions that are most comparable. Results Using the same solution conditions with SYNAPT G2(S) instruments, td -distributions of various ubiquitin charge states from MAI, LSI, and SAI are similar to those from ESI using a variety of solvents, matrices, extraction voltages, a laser, and temperature only, showing subtle differences in more compact features within the elongated distribution of structures. However, on a homebuilt drift-tube instrument, within the elongated distribution of structures, both similar and different td -distributions are observed for ubiquitin ions obtained by MAI and ESI. MAI-generated ions are frequently narrower in their td -distributions. Conclusions Direct comparisons between ESI and the new ionization methods operational directly from surfaces suggest that the protein in its solution structure prior to exposure to the ionization event is either captured (frozen out) at the time of crystallization, or that the protein in the solid matrix is associated with sufficient solvent to maintain the solution structure, or, alternatively, that the observed structures are those related to what occurs in the gas phase with ESI- or MAI-generated ions and not with the solution structures.

Published
2020

18. Following Structural Changes by Thermal Denaturation Using Trapped Ion Mobility Spectrometry-Mass Spectrometry

Author

Francisco Fernandez-Lima and Kevin Jeanne Dit Fouque

Subjects
Protein Denaturation, Materials science, Analytical chemistry, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Mass Spectrometry, Article, Ion, chemistry.chemical_compound, Ionization, 0103 physical sciences, Ion Mobility Spectrometry, Materials Chemistry, Physical and Theoretical Chemistry, Bovine serum albumin, Spectroscopy, Aqueous solution, 010304 chemical physics, biology, Temperature, Proteins, 0104 chemical sciences, Surfaces, Coatings and Films, Monomer, Ion-mobility spectrometry–mass spectrometry, chemistry, biology.protein
Abstract

The behavior of biomolecules as a function of the solution temperature is often crucial to assess their biological activity and function. While heat-induced changes of biomolecules are traditionally monitored using optical spectroscopy methods, their conformational changes and unfolding transitions remain challenging to interpret. In the present work, the structural transitions of bovine serum albumin (BSA) in native conditions (100 mM aqueous ammonium acetate) were investigated as a function of the starting solution temperature (T = ~23-70 °C) using a temperature-controlled nano-electrospray ionization source (nESI) coupled to a trapped ion mobility spectrometry – mass spectrometry (TIMS-MS) instrument. The charge state distribution of the monomeric BSA changed from a native-like, narrow charge state ([M + 12H](12+) - [M + 16H](16+) at ~23 °C) and narrow mobility distribution towards an unfolded-like, broad charge state (up to [M + 46H](46+) at ~70 °C) and broad mobility distribution. Inspection of the average charge state and collision cross section (CCS) distribution suggested a two-state unfolding transition with a melting temperature T(m) ~56 ± 1 °C; however, the inspection of the CCS profiles at the charge state level as a function of the solution temperature showcase at least six structural transitions (T1-T7). If the starting solution concentration is slightly increased (from 2 to 25 μM), this method can detect non-specific BSA dimers and trimers which dissociate early (T(d) ~34 ± 1 °C) and may disturb the melting curve of the BSA monomer. In a single experiment, this technology provides a detailed view of the solution, protein structural landscape (mobility vs solution temperature vs relative intensity for each charge state).

Published
2020

19. High-Resolution Ion Mobility Spectrometry-Mass Spectrometry of Isomeric/Isobaric Ribonucleotide Variants

Author

Jakub Ujma, Reza Nemati, Thomas Kenderdine, Daniele Fabris, Andrew Baker, Molly FitzGibbon, Limin Deng, Martin Palmer, James I. Langridge, and Maksim Royzen

Subjects
Analyte, Ribonucleotide, Molecular mass, 010405 organic chemistry, Chemistry, 010401 analytical chemistry, Analytical chemistry, Ribonucleotides, Mass spectrometry, 01 natural sciences, Article, Mass Spectrometry, 0104 chemical sciences, Ion, Metabolomics, Ion-mobility spectrometry–mass spectrometry, Fragmentation (mass spectrometry), Isomerism, Ion Mobility Spectrometry, Humans, Spectroscopy, HeLa Cells
Abstract

In this report, we explored the benefits of cyclic ion mobility (cIM) mass spectrometry in the analysis of isomeric post-transcriptional modifications of RNA. Standard methyl-cytidine samples were initially utilized to test the ability to correctly distinguish different structures sharing the same elemental composition, and thus molecular mass. Analyzed individually, the analytes displayed characteristic arrival times (t(D)) determined by the different positions of the modifying methyl groups onto the common cytidine scaffold. Analyzed in mixture, the widths of the respective signals resulted in significant overlap that initially prevented their resolution on the t(D) scale. The separation of the four isomers was achieved by increasing the number of passes through the cIM device, which enabled to fully differentiate the characteristic ion mobility behaviors associated with very subtle structural variations. The placement of the cIM device between the mass-selective quadrupole and the time-of-flight analyzer allowed us to perform gas-phase activation of each of these ion populations, which had been first isolated according to a common mass-to-charge ratio, and then separated on the basis of different ion mobility behaviors. The observed fragmentation patterns confirmed the structures of the various isomers, thus substantiating the benefits of complementing unique t(D) information with specific fragmentation data to reach more stringent analyte identification. These capabilities were further tested by analyzing natural mono-nucleotide mixtures obtained by exonuclease digestion of total RNA extracts. In particular, the combination of cIM separation and post-mobility dissociation allowed us to establish the composition of methyl-cytidine and methyl-adenine components present in the entire transcriptome of HeLa cells. For this reason, we expect that this technique will benefit not only epitranscriptomics studies requiring the determination of identity and expression levels of RNA modifications, but also metabolomics investigations involving the analysis of natural extracts that may possibly contain subsets of isomeric/isobaric species.

Published
2020

20. Analysis of Multiply Charged Poly(ethylene oxide-co-propylene oxide) Using Electrospray Ionization-Ion Mobility Spectrometry-Mass Spectrometry

Author

Shinya Kitagawa, Hajime Ohtani, and Kanako Ito

Subjects
Electrospray, Ethylene oxide, Chemistry, Electrospray ionization, 010401 analytical chemistry, Oxide, Analytical chemistry, 02 engineering and technology, 021001 nanoscience & nanotechnology, Mass spectrometry, 01 natural sciences, 0104 chemical sciences, Analytical Chemistry, chemistry.chemical_compound, Ion-mobility spectrometry–mass spectrometry, Copolymer, Propylene oxide, 0210 nano-technology
Abstract

Poly(ethylene oxide), poly(propylene oxide), and their copolymer (poly(EO-co-PO)) were analyzed by electrospray ionization-ion mobility spectrometry-mass spectrometry (ESI-IMS-MS). ESI produced multiply charged analytes of 2 to 5 Na+ additions, and they were separately observed in a 2D map of m/z value vs. drift time. The collision cross-section of the analyte polymers was almost linearly proportional to (molecular weight)0.644, except for the analytes with 2Na+ addition; a nonlinear relation called "folding" was significantly observed for the analytes with 2Na+ addition. An increase in electrostatic repulsion, because of the increase in Na+ addition, suppressed the folding of the polymer. Analyses of poly(EO-co-PO) with different EO compositions revealed that the copolymer with high EO composition tended to show folding. The separation of highly multiply charged poly(EO-co-PO)s with different EO contents by ESI-IMS-MS was successfully demonstrated.

Published
2018

21. Solvent Mediation of Peptide Conformations: Polyproline Structures in Water, Methanol, Ethanol, and 1-Propanol as Determined by Ion Mobility Spectrometry-Mass Spectrometry

Author

David H. Russell, David A. Hales, Daniel R. Fuller, David E. Clemmer, and Tarick J. El-Baba

Subjects
Circular dichroism, Chemistry, 010401 analytical chemistry, 010402 general chemistry, 01 natural sciences, Article, 0104 chemical sciences, Solvent, chemistry.chemical_compound, Crystallography, 1-Propanol, Ion-mobility spectrometry–mass spectrometry, Enthalpy–entropy compensation, Structural Biology, Methanol, Conformational isomerism, Spectroscopy, Polyproline helix
Abstract

Ion mobility spectrometry and circular dichroism spectroscopy are used to examine the populations of the small model peptide, polyproline-13 in water, methanol, ethanol, and 1-propanol over a range of solution temperatures (from 288 to 318 K). At low temperatures, the less-polar solvents (1-propanol and ethanol) favor the all-cis polyproline I helix (PPI); as the temperature is increased, the trans-configured polyproline II helix (PPII) is formed. In polar solvents (methanol and water), PPII is favored at all temperatures. From the experimental data, we determine the relative stabilities of the eight structures in methanol, ethanol, and 1-propanol, as well as four in water, all with respect to PPII. Although these conformers show relatively small differences in free energies, substantial variability is observed in the enthalpies and entropies across the structures and solvents. This requires that enthalpies and entropies be highly correlated: in 1-propanol, cis-configured PPI conformations are energetically favorable but entropically disfavored. In more polar solvents, PPI is enthalpically less favorable and entropy favors trans-configured forms. While either ΔH(0) or ΔS(0) can favor different structures, no conformation in any solvent is simultaneously energetically and entropically stabilized. These data present a rare opportunity to examine the origin of conformational stability.

Published
2018

22. Magnifying ion mobility spectrometry–mass spectrometry measurements for biomolecular structure studies

Author

Kushani Attanyake, Elinore Loch, Ahmad Kiani Karanji, Hossein Maleki, Stephen J. Valentine, and Sandra N. Majuta

Subjects
Materials science, Molecular Structure, Biochemical Phenomena, Extramural, 010401 analytical chemistry, Buffer gas, Biomolecular structure, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Biochemistry, Mass Spectrometry, Article, 0104 chemical sciences, Analytical Chemistry, Ion, Ion-mobility spectrometry–mass spectrometry, Chemical physics, Ion Mobility Spectrometry, Molecule, Instrumentation (computer programming)
Abstract

Ion mobility spectrometry – mass spectrometry (IMS-MS) provides information about the structures of gas-phase ions in the form of a collision cross section (CCS) with a neutral buffer gas. Indicating relative ion size, a CCS value alone is of limited utility. Although such information can be used to propose different conformer types, finer details of structure are not captured. The increased accessibility of IMS-MS measurements with commercial instrumentation in recent years has ballooned its usage in combination with separate measurements to provide enhanced data from which greater structural inferences can be drawn. This short review presents recent outstanding developments in scientific research that employs complementary measurements that when combined with IMS-MS data are used to characterize the structures of a wide range of compounds.

Published
2018

23. A four dimensional separation method based on continuous heart-cutting gas chromatography with ion mobility and high resolution mass spectrometry

Author

Oliver J. Schmitz, Christian Lipok, and Jörg Hippler

Subjects
Chromatography, Resolution (mass spectrometry), Chemistry, Ion-mobility spectrometry, 010401 analytical chemistry, Organic Chemistry, Chemie, Analytical chemistry, General Medicine, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Biochemistry, Chemistry Techniques, Analytical, Gas Chromatography-Mass Spectrometry, 0104 chemical sciences, Analytical Chemistry, Ion, Ion-mobility spectrometry–mass spectrometry, Comprehensive two-dimensional gas chromatography, Gas chromatography, Pesticides, Gas chromatography–mass spectrometry
Abstract

A two-dimensional GC (2D-GC) method was developed and coupled to an ion mobility-high resolution mass spectrometer, which enables the separation of complex samples in four dimensions (2D-GC, ion mobilility spectrometry and mass spectrometry). This approach works as a continuous multiheart-cutting GC-system (GC+GC), using a long modulation time of 20s, which allows the complete transfer of most of the first dimension peaks to the second dimension column without fractionation, in comparison to comprehensive two-dimensional gas chromatography (GCxGC). Hence, each compound delivers only one peak in the second dimension, which simplifies the data handling even when ion mobility spectrometry as a third and mass spectrometry as a fourth dimension are introduced. The analysis of a plant extract from Calendula officinales shows the separation power of this four dimensional separation method. The introduction of ion mobility spectrometry provides an additional separation dimension and allows to determine collision cross sections (CCS) of the analytes as a further physicochemical constant supporting the identification. A CCS database with more than 800 standard substances including drug-like compounds and pesticides was used for CCS data base search in this work.

Published
2018

24. On-line analysis of coffee roasting with ion mobility spectrometry–mass spectrometry (IMS–MS)

Author

Alexia N. Gloess, Michael Groessl, R. Knochenmuss, and Chahan Yeretzian

Subjects
Ion-mobility spectrometry, Coffee roasting, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Ion, coffee roasting, Physical and Theoretical Chemistry, Instrumentation, Spectroscopy, Aroma, Alkyl, Roasting, chemistry.chemical_classification, Chromatography, biology, Chemistry, 010401 analytical chemistry, food and beverages, Ion mobility spectrometry, Condensed Matter Physics, biology.organism_classification, 0104 chemical sciences, Ion-mobility spectrometry–mass spectrometry, Pyrazines, 663: Getränketechnologie, On-line analysis, Ionisation
Abstract

On-line analysis of coffee roasting was performed using ion mobility spectrometry–mass spectrometry (IMS–MS) with corona discharge ionization. This is the first time that formation of volatile organic compounds (VOCs) during coffee roasting was monitored not only in positive but also in negative ion mode, and not only with mass spectrometry, but also with ion mobility spectrometry. The temporal evolution of more than 150 VOCs was monitored during the roasting of Brazilian Coffea arabica. Mass-selective ion mobility spectrometry allowed a separation of isobaric and isomeric compounds. In positive ion mode, isomers of alkyl pyrazines were found to exhibit distinct time-intensity profiles during roasting, providing a unique insight into the complex chemistry of this important class of aroma active compounds. Negative ion mode gave access to species poorly detectable by other on-line methods, such as acids. In this study, the release of fatty acids during coffee roasting was investigated in detail. These increase early on in the roasting process followed by a decrease at the same time as other VOCs start to be formed.

Published
2018

25. Characterizing the lipid and metabolite changes associated with placental function and pregnancy complications using ion mobility spectrometry-mass spectrometry and mass spectrometry imaging

Author

Erin S. Baker, Kristin E. Burnum-Johnson, and Thomas O. Metz

Subjects
0301 basic medicine, Spectrometry, Mass, Electrospray Ionization, medicine.medical_specialty, Placenta, Spectrometry, Mass, Secondary Ion, Bioinformatics, Mass spectrometry, Models, Biological, 01 natural sciences, Article, Mass spectrometry imaging, 03 medical and health sciences, Metabolomics, Pregnancy, Internal medicine, Ion Mobility Spectrometry, medicine, Metabolome, Animals, Humans, Embryo Implantation, Chromatography, High Pressure Liquid, Chemistry, 010401 analytical chemistry, Obstetrics and Gynecology, Placentation, Lipidome, Lipid Metabolism, medicine.disease, 0104 chemical sciences, Pregnancy Complications, 030104 developmental biology, Endocrinology, Ion-mobility spectrometry–mass spectrometry, Reproductive Medicine, Female, Developmental Biology
Abstract

Successful pregnancy is dependent upon discrete biological events, which include embryo implantation, decidualization, and placentation. Problems associated with each of these events can cause infertility or conditions such as preeclampsia. A greater understanding of the molecular changes associated with these complex processes is necessary to aid in identifying treatments for each condition. Previous nuclear magnetic resonance spectroscopy and mass spectrometry studies have been used to identify metabolites and lipids associated with pregnancy-related complications. However, due to limitations associated with conventional implementations of both techniques, novel technology developments are needed to more fully understand the initiation and development of pregnancy related problems at the molecular level. In this perspective, we describe current analytical techniques for metabolomic and lipidomic characterization of pregnancy complications and discuss the potential for new technologies such as ion mobility spectrometry-mass spectrometry and mass spectrometry imaging to contribute to a better understanding of the molecular changes that affect the placenta and pregnancy outcomes.

Published
2017

26. Structure-elucidation of human CCL5 by integrating trapped ion mobility spectrometry-mass spectrometry (TIMS-MS) with Structure Relaxation Approximation (SRA) analysis

Author

Mengqi Chai and Christian Bleiholder

Subjects
Proton, Chemistry, Ion-mobility spectrometry, Condensed Matter Physics, Mass spectrometry, Ligand (biochemistry), Spectral line, Ion, Cross section (physics), Ion-mobility spectrometry–mass spectrometry, Chemical physics, Physical and Theoretical Chemistry, Instrumentation, Spectroscopy
Abstract

Ion mobility spectrometry-mass spectrometry offers the potential to characterize structures of transient protein assemblies and protein isoforms by means of their orientationally-averaged momentum transfer cross-sections. A commonly observed phenomenon is the compaction of a protein in the ion mobility measurement, that is, the cross section measured for the protein by ion mobility spectrometry is smaller than the cross section expected for its native structure. Consequently, this compaction means that at least some structural changes of the protein must have occurred during the ion mobility measurement. A major challenge is then to identify which aspects of the solution structure are retained in the ion mobility measurement and which ones are not. Here, we apply our recently developed Structure Relaxation Approximation (SRA) method in conjunction with trapped ion mobility spectrometry-mass spectrometry (TIMS-MS) to probe compaction of the human protein chemokine (C-C motif) ligand 5 (also CCL5). Ion mobility spectra are recorded for various charge states and solution conditions of CCL5 under both “soft” and collisionally-activated conditions. Our data show that the SRA reproduces the overall trends in the experimental spectra: (1) the compaction of the CCL5 structure as seen in the experiments; (2) the general increase in the cross section for the various charge states; and (3) the increase in cross section after collisional-activation. The SRA attributes the compaction of the CCL5 structure mainly to the folding of the unstructured N-terminus onto the central Greek key motif of CCL5. By contrast, the SRA indicates that native residue-residue contacts present in the NMR structure are largely retained. Additionally, our analysis indicates that accurate treatment of proton transfer processes during the structural relaxation process would significantly improve the structural interpretation of ion mobility data by the SRA.

Published
2021

27. Characterization of Intramolecular Interactions of Cytochrome c Using Hydrogen–Deuterium Exchange-Trapped Ion Mobility Spectrometry–Mass Spectrometry and Molecular Dynamics

Author

Mark E. Ridgeway, Melvin A. Park, Francisco Fernandez-Lima, Juan Camilo Molano-Arevalo, Kevin Jeanne Dit Fouque, Khoa N. Pham, and Jaroslava Miksovska

Subjects
Hydrogen, Protein Conformation, Analytical chemistry, chemistry.chemical_element, Molecular Dynamics Simulation, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Mass Spectrometry, Article, Analytical Chemistry, Ion, Ion Mobility Spectrometry, Animals, Horses, Protein Unfolding, Chemistry, Hydrogen bond, 010401 analytical chemistry, Cytochromes c, Deuterium Exchange Measurement, 0104 chemical sciences, Ion-mobility spectrometry–mass spectrometry, Deuterium, Hydrogen–deuterium exchange
Abstract

Globular proteins, such as cytochrome c (cyt c), display an organized native conformation, maintained by a hydrogen bond interaction network. In the present work, the structural interrogation of kinetically trapped intermediates of cyt c was performed by correlating the ion-neutral collision cross section (CCS) and charge state with the starting solution conditions and time after desolvation using collision induced activation (CIA), time resolved hydrogen/deuterium back exchange (HDX) and trapped ion mobility spectrometry - mass spectrometry (TIMS-MS). The high ion mobility resolving power of the TIMS analyzer allowed the identification of new ion mobility bands, yielding a total of 63 mobility bands over the +6 to +21 charge states and 20 mobility bands over the −5 to −10 charge states. Mobility selected HDX rates showed that for the same charge state, conformers with larger CCS present faster HDX rates in both positive and negative ion mode, suggesting that the charge sites and neighboring exchange sites on the accessible surface area define the exchange rate regardless of the charge state. Complementary molecular dynamic simulations permitted the generation of candidate structures and a mechanistic model of the folding transitions from native (N) to molten globule (MG) to kinetic intermediates (U) pathways. Our results suggest that cyt c major structural unfolding is associated with the distancing of the N- and C- terminal helices and subsequent solvent exposure of the hydrophobic, heme-containing cavity.

Published
2017

28. Structural Elucidation of cis/trans Dicaffeoylquinic Acid Photoisomerization Using Ion Mobility Spectrometry-Mass Spectrometry

Author

Yehia M. Ibrahim, Dennis G. Thomas, Mwadham M. Kabanda, Mpho M. Makola, Richard D. Smith, Xueyun Zheng, Heino M. Heyman, Niranjan Govind, Ntakadzeni E. Madala, Erin S. Baker, Ryan S. Renslow, Ian K. Webb, Liulin Deng, and Ian A. Dubery

Subjects
Photoisomerization, 010405 organic chemistry, Chemistry, Ion-mobility spectrometry, Stereochemistry, 010401 analytical chemistry, Dicaffeoylquinic acid, Health benefits, Mass spectrometry, 01 natural sciences, Article, 0104 chemical sciences, Ion-mobility spectrometry–mass spectrometry, General Materials Science, Physical and Theoretical Chemistry, Cis–trans isomerism
Abstract

Due to the recently uncovered health benefits and anti-HIV activities of dicaffeoylquinic acids (diCQAs), understanding their structures and functions is of great interest for drug discovery efforts. DiCQAs are analytically challenging to identify and quantify since they commonly exist as a diverse mixture of positional and geometric (cis/trans) isomers. In this work, we utilized ion mobility spectrometry coupled with mass spectrometry to separate the various isomers before and after UV irradiation. The experimental collision cross sections were then compared with theoretical structures to differentiate and identify the diCQA isomers. Our analyses found that naturally the diCQAs existed predominantly as trans/trans isomers, but after 3 h of UV irradiation, cis/cis, cis/trans, trans/cis, and trans/trans isomers were all present in the mixture. This is the first report of successful differentiation of cis/trans diCQA isomers individually, which shows the great promise of IMS coupled with theoretical calculations for determining the structure and activity relationships of different isomers in drug discovery studies.

Published
2017

29. Increasing Peak Capacity in Nontargeted Omics Applications by Combining Full Scan Field Asymmetric Waveform Ion Mobility Spectrometry with Liquid Chromatography–Mass Spectrometry

Author

Matthew A. Turner, Kayleigh L. Arthur, Colin S. Creaser, and James C. Reynolds

Subjects
0301 basic medicine, Analyte, Chromatography, Collision-induced dissociation, Chemistry, Ion-mobility spectrometry, Hydrophilic interaction chromatography, 010401 analytical chemistry, Analytical chemistry, Mass spectrometry, 01 natural sciences, 0104 chemical sciences, Analytical Chemistry, 03 medical and health sciences, 030104 developmental biology, Metabolomics, Ion-mobility spectrometry–mass spectrometry, Liquid chromatography–mass spectrometry
Abstract

Full scan field asymmetric waveform ion mobility spectrometry (FAIMS) combined with liquid chromatography and mass spectrometry (LC-FAIMS-MS) is shown to enhance peak capacity for omics applications. A miniaturized FAIMS device capable of rapid compensation field scanning has been incorporated into an ultrahigh performance liquid chromatography (UHPLC) and time-of-flight mass spectrometry analysis, allowing the acquisition of full scan FAIMS and MS nested data sets within the time scale of a UHPLC peak. Proof of principle for the potential of scanning LC-FAIMS-MS in omics applications is demonstrated for the nontargeted profiling of human urine using a HILIC column. The high level of orthogonality between FAIMS and MS provides additional unique compound identifiers with detection of features based on retention time, FAIMS dispersion field and compensation field (DF and CF), and mass-to-charge (m/z). Extracted FAIMS full scan data can be matched to standards to aid the identification of unknown analytes. The peak capacity for features detected in human urine using LC-FAIMS-MS was increased approximately threefold compared to LC-MS alone due to a combination of the reduction of chemical noise and separation of coeluting isobaric species across the entire analytical space. The use of FAIMS-selected in source collision induced dissociation (FISCID) yields fragmentation of ions, which reduces sample complexity associated with overlapping fragmentation patterns and provides structural information on the selected precursor ions.

Published
2017

30. Ion Mobility Mass Spectrometry

Author

Akio Hayashi, Ushio Takeda, Nobutake Sato, and Haruo Hosoda

Subjects
Ion-mobility spectrometry–mass spectrometry, Chromatography, Ion-mobility spectrometry, Chemistry, Selected reaction monitoring, Thermal ionization mass spectrometry, Mass spectrometry, Top-down proteomics
Published
2017

32. Advances in MS Based Strategies for Probing Ligand-Target Interactions: Focus on Soft Ionization Mass Spectrometric Techniques

Author

Guilin Chen, Minxia Fan, Ye Liu, Baoqing Sun, Meixian Liu, Jianlin Wu, Na Li, and Mingquan Guo

Subjects
Electrospray ionization, soft ionization, Binding energy, 02 engineering and technology, Review, 010402 general chemistry, Mass spectrometry, 01 natural sciences, MALDI-MS, drug discovery, lcsh:Chemistry, Molecule, ligand-target interactions, mass spectrometry, Drug discovery, Chemistry, ESI-MS, General Chemistry, 021001 nanoscience & nanotechnology, Combinatorial chemistry, 0104 chemical sciences, Matrix-assisted laser desorption/ionization, Ion-mobility spectrometry–mass spectrometry, lcsh:QD1-999, 0210 nano-technology, Stoichiometry
Abstract

The non-covalent interactions between small drug molecules and disease-related proteins (ligand-target interactions) mediate various pharmacological processes in the treatment of different diseases. The development of the analytical methods to assess those interactions, including binding sites, binding energies, stoichiometry and association-dissociation constants, could assist in clarifying the mechanisms of action, precise treatment of targeted diseases as well as the targeted drug discovery. For the last decades, mass spectrometry (MS) has been recognized as a powerful tool to study the non-covalent interactions of the ligand-target complexes with the characteristics of high sensitivity, high-resolution, and high-throughput. Soft ionization mass spectrometry, especially the electrospray mass spectrometry (ESI-MS) and matrix assisted laser desorption ionization mass spectrometry (MALDI-MS), could achieve the complete transformation of the target analytes into the gas phase, and subsequent detection of the small drug molecules and disease-related protein complexes, and has exerted great advantages for studying the drug ligands-protein targets interactions, even in case of identifying active components as drug ligands from crude extracts of medicinal plants. Despite of other analytical techniques for this purpose, such as the NMR and X-ray crystallography, this review highlights the principles, research hotspots and recent applications of the soft ionization mass spectrometry and its hyphenated techniques, including hydrogen-deuterium exchange mass spectrometry (HDX-MS), chemical cross-linking mass spectrometry (CX-MS), and ion mobility spectrometry mass spectrometry (IMS-MS), in the study of the non-covalent interactions between small drug molecules and disease-related proteins.

Published
2019

33. Determination of the collision cross sections of cardiolipins and phospholipids from Pseudomonas aeruginosa by traveling wave ion mobility spectrometry-mass spectrometry using a novel correction strategy

Author

Annick Schaumann, Corinne Loutelier-Bourhis, Stéphane Alexandre, Isabelle Schmitz-Afonso, Emmanuelle Dé, Estelle Deschamps, Carlos Afonso, Chimie Organique et Bioorganique : Réactivité et Analyse (COBRA), Institut Normand de Chimie Moléculaire Médicinale et Macromoléculaire (INC3M), Institut de Chimie du CNRS (INC)-École Nationale Supérieure d'Ingénieurs de Caen (ENSICAEN), Normandie Université (NU)-Normandie Université (NU)-Institut national des sciences appliquées Rouen Normandie (INSA Rouen Normandie), Institut National des Sciences Appliquées (INSA)-Normandie Université (NU)-Institut National des Sciences Appliquées (INSA)-Université Le Havre Normandie (ULH), Normandie Université (NU)-Université de Rouen Normandie (UNIROUEN), Normandie Université (NU)-Centre National de la Recherche Scientifique (CNRS)-Université de Caen Normandie (UNICAEN), Normandie Université (NU)-Institut de Chimie du CNRS (INC)-École Nationale Supérieure d'Ingénieurs de Caen (ENSICAEN), Normandie Université (NU)-Centre National de la Recherche Scientifique (CNRS)-Institut de Chimie Organique Fine (IRCOF), Université de Rouen Normandie (UNIROUEN), Institut National des Sciences Appliquées (INSA)-Normandie Université (NU)-Institut National des Sciences Appliquées (INSA)-Centre National de la Recherche Scientifique (CNRS)-Centre National de la Recherche Scientifique (CNRS), Polymères Biopolymères Surfaces (PBS), Institut national des sciences appliquées Rouen Normandie (INSA Rouen Normandie), Institut National des Sciences Appliquées (INSA)-Normandie Université (NU)-Institut National des Sciences Appliquées (INSA)-Normandie Université (NU)-Institut de Chimie du CNRS (INC)-Institut Normand de Chimie Moléculaire Médicinale et Macromoléculaire (INC3M), Normandie Université (NU)-École Nationale Supérieure d'Ingénieurs de Caen (ENSICAEN), Normandie Université (NU)-Université Le Havre Normandie (ULH), and Normandie Université (NU)-Centre National de la Recherche Scientifique (CNRS)

Subjects
CCS calibration, Ion-mobility spectrometry, Cardiolipins, Analytical chemistry, medicine.disease_cause, Mass spectrometry, 01 natural sciences, Biochemistry, Mass Spectrometry, Analytical Chemistry, Ion, 03 medical and health sciences, [CHIM.ANAL]Chemical Sciences/Analytical chemistry, Ion Mobility Spectrometry, medicine, [SDV.BBM.BC]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Biochemistry [q-bio.BM], Phospholipids, 030304 developmental biology, 0303 health sciences, biology, Chemistry, Pseudomonas aeruginosa, fungi, 010401 analytical chemistry, Pseudomonas, biology.organism_classification, 0104 chemical sciences, 3. Good health, Membrane, Ion-mobility spectrometry–mass spectrometry, Calibration
Abstract

International audience; Collision cross section (CCS) values are descriptors of the 3D structure of ions which can be determined by ion mobility spectrometry (IMS). Currently, most lipidomic studies involving CCS value determination concern eukaryote samples (e.g. human, bovine) and to a lower extent prokaryote samples (e.g. bacteria). Here, we report CCS values obtained from traveling wave ion mobility spectrometry (TWCCSN2) measurements from the bacterial membrane of Pseudomonas aeruginosa—a bacterium ranked as priority 1 for the R&D of new antibiotics by the World Health Organization. In order to cover the lack of reference compounds which could cover the m/z and CCS ranges of the membrane lipids of P. aeruginosa, three calibrants (polyalanine, dextran and phospholipids) were used for the TWCCSN2 calibration. A shift from the published lipid CCS values was systematically observed (ΔCCS% up to 9%); thus, we proposed a CCS correction strategy. This correction strategy allowed a reduction in the shift (ΔCCS%) between our measurements and published values to less than 2%. This correction was then applied to determine the CCS values of Pseudomonas aeruginosa lipids which have not been published yet. As a result, 32 TWCCSN2 values for [M+H]+ ions and 24 TWCCSN2 values for [M−H]− ions were obtained for four classes of phospholipids (phosphatidylethanolamines (PE), phosphatidylcholines (PC), phosphatidylglycerols (PG) and diphosphatidylglycerols—known as cardiolipins (CL)).

Published
2019

35. Ion mobility spectrometry–mass spectrometry (IMS–MS) for on- and offline analysis of atmospheric gas and aerosol species

Author

Ying Hsuan Lin, Haofei Zhang, Xuan Zhang, Michael Groessl, Richard Knochenmuss, Jordan E. Krechmer, Jose-Luis Jimenez, Douglas R. Worsnop, Michael J. Cubison, Joel R. Kimmel, Sri Hapsari Budisulistiorini, Jason D. Surratt, John T. Jayne, Manjula R. Canagaratna, Andrew T. Lambe, Paola Massoli, Heikki Junninen, Stephan Graf, Department of Physics, Polar and arctic atmospheric research (PANDA), and Earth Observatory of Singapore

Subjects
Atmospheric Science, 010504 meteorology & atmospheric sciences, Electrospray ionization, Analytical chemistry, UNITED-STATES, Geology [Science], 2013 SOUTHERN OXIDANT, 010501 environmental sciences, Mass spectrometry, 114 Physical sciences, 01 natural sciences, REACTIVE UPTAKE, 03 medical and health sciences, chemistry.chemical_compound, Fragmentation (mass spectrometry), SECONDARY ORGANIC AEROSOL, CHEMICAL-IONIZATION, AMBIENT AEROSOL, lcsh:TA170-171, Isoprene, 030304 developmental biology, 0105 earth and related environmental sciences, Atmospheric Gas, 0303 health sciences, Chemical ionization, Aerosol Species, OZONOLYSIS PRODUCTS, lcsh:TA715-787, lcsh:Earthwork. Foundations, ISOPRENE EPOXYDIOLS, OXIDATION-PRODUCTS, lcsh:Environmental engineering, Ion-mobility spectrometry–mass spectrometry, chemistry, 13. Climate action, Mass spectrum, PLASMA CHROMATOGRAPHY, Organosulfate
Abstract

Measurement techniques that provide molecular-level information are needed to elucidate the multi-phase processes that produce secondary organic aerosol (SOA) species in the atmosphere. Here we demonstrate the application of ion mobility spectrometry-mass spectrometry (IMS-MS) to the simultaneous characterization of the elemental composition and molecular structures of organic species in the gas and particulate phases. Molecular ions of gas-phase organic species are measured online with IMS-MS after ionization with a custom build nitrate chemical ionization (CI) source. This CI-IMS-MS technique is used to obtain time-resolved measurements (5 min) of highly oxidized organic molecules during the 2013 Southern Oxidant and Aerosol Study (SOAS) ambient field campaign in the forested SE US. The ambient IMS-MS signals are consistent with laboratory IMS-MS spectra obtained from single-component carboxylic acids and multicomponent mixtures of isoprene and monoterpene oxidation products. Mass-mobility correlations in the 2-dimensional IMS-MS space provide a means of identifying ions with similar molecular structures within complex mass spectra and are used to separate and identify monoterpene oxidation products in the ambient data that are produced from different chemical pathways. Water-soluble organic carbon (WSOC) constituents of fine aerosol particles that are not resolvable with standard analytical separation methods, such as liquid chromatography (LC), are shown to be separable with IMS-MS coupled to an electrospray ionization (ESI) source. The capability to use ion mobility to differentiate between isomers is demonstrated for organosulfates derived from the reactive uptake of isomers of isoprene epoxydiols (IEPOX) onto wet acidic sulfate aerosol. Controlled fragmentation of precursor ions by collisional dissociation (CID) in the transfer region between the IMS and the MS is used to validate MS peak assignments, elucidate structures of oligomers, and confirm the presence of the organosulfate functional group.

Published
2016

36. Modular calibrant sets for the structural analysis of nucleic acids by ion mobility spectrometry mass spectrometry

Author

Jennifer L. Lippens, Daniele Fabris, Srivathsan V. Ranganathan, and Rebecca J. D’Esposito

Subjects
Nucleic acid quantitation, Calibration curve, Ion-mobility spectrometry, Analytical chemistry, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Biochemistry, Mass Spectrometry, Article, Analytical Chemistry, Ion, Reference Values, Nucleic Acids, Ion Mobility Spectrometry, Electrochemistry, Calibration, Environmental Chemistry, Spectroscopy, Reproducibility, Chemistry, 010401 analytical chemistry, Reproducibility of Results, 0104 chemical sciences, Ion-mobility spectrometry–mass spectrometry
Abstract

This study explored the use of modular nucleic acid (NA) standards to generate calibration curves capable of translating primary ion mobility readouts into corresponding collision cross section (CCS) data. Putative calibrants consisted of single- (ss) and double-stranded (ds) oligo-deoxynucleotides reaching up to (~)40 kDa in size (i.e., 64 bp) and (~) 5,700 Å(2) in CCS. To ensure self-consistency among reference CCS values, computational data obtained in house were preferred to any experimental or computational data from disparate sources. Such values were obtained by molecular dynamics (MD) simulations and either the exact hard sphere scattering (EHSS) or the projection superposition approximation (PSA) methods, and then plotted against the corresponding experimental values to generate separate calibration curves. Their performance was evaluated on the basis of their correlation coefficient and ability to provide values that matched the CCS of selected test samples mimicking typical unknowns. The results indicated that the predictive power benefitted from the exclusion of higher charged species that were more susceptible to the destabilizing effects of Coulombic repulsion. The results revealed discrepancies between EHSS and PSA data that were ascribable to the different approximations used to describe the ion mobility process. Within the boundaries defined by these approximations and the challenges of modeling NA structure in solvent-free environment, the calibrant sets enabled the experimental determination of CCS with excellent reproducibility (precision) and error (accuracy), which will support the analysis of progressively larger NA samples of biological significance.

Published
2016

37. Liquid chromatography-ion mobility spectrometry-mass spectrometry analysis of multiple classes of steroid hormone isomers in a mixture

Author

Alana L. Rister and Eric D. Dodds

Subjects
Analyte, Resolution (mass spectrometry), Ion-mobility spectrometry, medicine.medical_treatment, Clinical Biochemistry, Mass spectrometry, 030226 pharmacology & pharmacy, 01 natural sciences, Biochemistry, Article, Mass Spectrometry, Analytical Chemistry, Steroid, 03 medical and health sciences, 0302 clinical medicine, Isomerism, Ion Mobility Spectrometry, medicine, Chromatography, Chemistry, 010401 analytical chemistry, Analytical technique, Cell Biology, General Medicine, 0104 chemical sciences, Steroid hormone, Ion-mobility spectrometry–mass spectrometry, Steroids, Chromatography, Liquid
Abstract

Methods for the analysis of steroids have long been of interest due to the multiple uses for such methods in medical applications, sports monitoring, and environmental science. The analysis of steroids involves inherent analytical hurdles due to their low biological concentrations, poor ionization efficiencies, and frequent occurrence of isomerism. One analytical technique that has been recently applied to steroid analysis is ion mobility spectrometry (IMS). While previous work has focused on the use of metal adduction and multimer formation to enhance separation through IMS analysis coupled to mass spectrometry (MS), this work furthers this approach by coupling IMS-MS with liquid chromatography (LC). Three different LC methods with varying tradeoffs between chromatographic resolution and run time were developed, with one of these achieving a resolution above 1.5 for all steroid isomers. These results also indicate that the coupling of LC to IMS-MS can increase the overall resolution of steroid isomers relative to what can be achieved by either LC or IMS alone. Furthermore, the use of LC and IMS in concert can allow for a more rapid analysis of steroid isomers than can be achieved by LC-MS alone. Finally, the IMS dimension provided for measurements of ion-neutral collision cross sections (CCSs), which were found to be in good agreement with previously reported measurements. Thus, this approach provides three complementary quantitative parameters (retention time, CCS, and mass-to-charge ratio) that can contribute the identification of analytes. Overall, the work presented here demonstrates the potential of coupling LC, IMS, and MS for the analysis of isomeric steroid hormones.

Published
2020

38. Characterization and analysis of non-ionic surfactants by supercritical fluid chromatography combined with ion mobility spectrometry-mass spectrometry

Author

Yun Zhang, Zhenxia Du, Junfeng Zhai, Qiang Ma, Wentao Li, Xi Chen, and Hua Bai

Subjects
Chromatography, Resolution (mass spectrometry), Elution, Electrospray ionization, 010401 analytical chemistry, Fatty alcohol, 02 engineering and technology, 021001 nanoscience & nanotechnology, Mass spectrometry, 01 natural sciences, Biochemistry, 0104 chemical sciences, Analytical Chemistry, Ion, chemistry.chemical_compound, Ion-mobility spectrometry–mass spectrometry, chemistry, Supercritical fluid chromatography, 0210 nano-technology
Abstract

Comprehensive separation and analysis of non-ionic surfactants have been conducted by coupling supercritical fluid chromatography (SFC) with ion mobility spectrometry-mass spectrometry (IMS-MS). Representative non-ionic surfactants were investigated, including alkylphenol ethoxylates (APEOs), e.g., octylphenol ethoxylates (OPEOs) and fatty alcohol ethoxylates (FAEs), e.g., lauryl alcohol ethoxylates (LAEs). A sub-2-μm high-density diol column was used for chromatographic separation by the first-dimensional SFC due to the differences in ethoxy chain prior to electrospray ionization (ESI). Maintaining the fidelity of pre-ionization separation in the first dimension, the introduction of IMS provided additional post-ionization resolution by broadly fractionating the oligometric ethoxymers based on their size and electric charge within 13.78 ms. Distinguishable series of singly and multiply charged non-ionic species could be clearly observed. The millisecond timescale ion mobility separation perfectly fits the elution time of a chromatographic peak, while effectively feeding components into the fast-scanning time-of-flight (TOF) mass analyzer for characterization and analysis. The orthogonality of the developed separation and analysis system was evaluated, revealing a correlation coefficient and peak spreading angle of 0.2729 and 74.16° for the studied OPEOs and 0.1962 and 78.69° for LAEs. Significant enhancement in peak capacity was achieved for the developed SFC-IMS-MS system with the actual peak capacity measured to be approximately 41 and 160 times higher than that of the dimensions of SFC and IMS, respectively, when used alone. Graphical abstract.

Published
2018

40. Vacuum ultraviolet photochemistry: I. Unimolecular decomposition studies of small hydrocarbon clusters by molecular beam photoionization mass spectrometry; II. Photofragment dynamics study of carbon disulfide by high resolution molecular beam laser photofragment time-of-flight mass spectrometry

Author

Wen-Bih Tzeng

Subjects
Static secondary-ion mass spectrometry, Ion-mobility spectrometry–mass spectrometry, Collision-induced dissociation, Chemistry, Analytical chemistry, Photoionization, Time-of-flight mass spectrometry, Fast atom bombardment, Mass spectrometry, Photochemistry, Molecular beam
Published
2018

41. Inorganic and biological applications of inductively coupled plasma mass spectrometry and electrospray mass spectrometry

Author

Fumin Li

Subjects
Matrix (chemical analysis), chemistry.chemical_compound, Aqueous solution, Materials science, Ion-mobility spectrometry–mass spectrometry, chemistry, Nitric acid, Liquid chromatography–mass spectrometry, Analytical chemistry, Extractive electrospray ionization, Capillary electrophoresis–mass spectrometry, Inductively coupled plasma mass spectrometry
Abstract

Aqueous acid mixtures at room temperature are used to partially dissolve steel samples. The dissolved elements are washed off the surface, diluted, and then determined by inductively coupled plasma mass spectrometry (ICP-MS) using a magnetic sector mass analyzer. The amount of material removed is measured from the amount of Fe dissolved and increases linearly with HNO3 concentration in the etch acid. Analyte concentrations in the solid are determined from the signal ratio of "(analyte ion)/Fe+". The shape of a plot of mass of element removed vs. nitric acid concentration yields information about the efficiency of the removal process and the likely chemical form of the element in the sample. For elements like Mn, A1 and W in steel, these plots have the same linear shape as that for the major element (Fe), and the measured concentrations agree well with the certified values. For problem elements like Nb and Ta, the plots have two linear regions with different slopes, and measured concentrations are lower than the certified values. Laser ablation ICP-MS and scanning electron microscopy (SEM) measurements show these elements to be associated together in the solid in refractory grains that are not dissolved to the same extent as the Fe matrix. For steel, the amount of Fe dissolved corresponds to an average depth of at least 4 (o,m or 20,000 atomic layers.

Published
2018

42. Sample introduction techniques for inductively coupled plasma mass spectrometry

Author

Shiuh-Jen Jiang

Subjects
Materials science, Ion-mobility spectrometry–mass spectrometry, Chromatography, Selected reaction monitoring, Mass spectrum, Analytical chemistry, Thermal ionization mass spectrometry, Mass spectrometry, Inductively coupled plasma mass spectrometry, Sample preparation in mass spectrometry, Hybrid mass spectrometer
Published
2018

44. Hyphenated Applications of Mass Spectrometry for the Analysis of Biological Compounds

Author

Derrick L. Morast

Subjects
Quantitative Biology::Biomolecules, biology, Proton, Chemistry, Cytochrome c, Analytical chemistry, Charge (physics), Mass spectrometry, Ion, chemistry.chemical_compound, Ion-mobility spectrometry–mass spectrometry, Physics::Plasma Physics, biology.protein, Lysozyme, Ammonium acetate
Abstract

Ion mobility spectrometry mass spectrometry (IMS-MS) is used to measure gas-phase conformations of ubiquitin, cytochrome c, lysozyme, and α-lactalbumin sprayed from an ammonium acetate solution titrated to pH 8.0. Ion mobility drift time measurements are converted to collision cross section values, in Ǻ 2 , and compared to corresponding charge state conformations generated via proton transfer charge reduction ion/ion reactions. Ions made directly from the alkaline solution in low charge states have conformations which are found to be 14 to 36% more compact than ions generated from proton transfer reactions.

Published
2018

45. Profiling ribonucleotide modifications at full-transcriptome level: a step toward MS-based epitranscriptomics

Author

Ryan Quinn, Daniele Fabris, Rebecca E. Rose, and Jackie L. Sayre

Subjects
Ribonucleotide, Systems biology, Electrospray ionization, Reproducibility of Results, Computational biology, Ribonucleotides, Biology, Bioinformatics, Tandem mass spectrometry, Mass spectrometry, Metabolomics, Ion-mobility spectrometry–mass spectrometry, Tandem Mass Spectrometry, Epitranscriptomics, Methods, RNA Processing, Post-Transcriptional, Erratum, Transcriptome, Molecular Biology
Abstract

The elucidation of the biological significance of RNA post-transcriptional modifications is hampered by the dearth of effective high-throughput sequencing approaches for detecting, locating, and tracking their levels as a function of predetermined experimental factors. With the goal of confronting this knowledge gap, we devised a strategy for completing global surveys of all ribonucleotide modifications in a cell, which is based on the analysis of whole cell extracts by direct infusion electrospray ionization mass spectrometry (ESI-MS). Our approach eschews chromatographic separation to promote instead the direct application of MS techniques capable of providing detection, differentiation, and quantification of post-transcriptional modifications (PTMs) in complex ribonucleotide mixtures. Accurate mass analysis was used to carry out database-aided identification of PTMs, whereas multistep tandem mass spectrometry (MSn) and consecutive reaction monitoring (CRM) provided the necessary structural corroboration. We demonstrated that heat-map plots afforded by ion mobility spectrometry mass spectrometry (IMS-MS) can provide comprehensive modification profiles that are unique for different cell types and metabolic states. We showed that isolated tRNA samples can be used as controlled sources of PTMs in standard-additions quantification. Intrinsic internal standards enable direct comparisons of heat-maps obtained under different experimental conditions, thus offering the opportunity to evaluate the global effects of such conditions on the expression levels of all PTMs simultaneously. This type of comparative analysis will be expected to support the investigation of the system biology of RNA modifications, which will be aimed at exploring mutual correlations of their expression levels and providing new valuable insights into their biological significance.

Published
2015

46. Characterization of Compounds inPsoralea corylifoliaUsing High-Performance Liquid Chromatography Diode Array Detection, Time-of-Flight Mass Spectrometry and Quadrupole Ion Trap Mass Spectrometry

Author

Yifeng Chai, Tiehong Yang, Huayan Miao, Hao Chen, Hong Wu, and Guangguo Tan

Subjects
Chromatography, biology, Plant Extracts, Psoralea corylifolia, Chemistry, Selected reaction monitoring, Ficusin, Analytical chemistry, General Medicine, biology.organism_classification, Mass spectrometry, Mass Spectrometry, Sample preparation in mass spectrometry, Psoralea, Analytical Chemistry, Chalcones, Ion-mobility spectrometry–mass spectrometry, Liquid chromatography–mass spectrometry, Fruit, Glycosides, Time-of-flight mass spectrometry, Chromatography, High Pressure Liquid, Benzofurans, Hybrid mass spectrometer
Abstract

High-performance liquid chromatography with diode array detection (HPLC-DAD), time-of-flight mass spectrometry (HPLC-TOFMS) and quadrupole ion trap mass spectrometry (HPLC-QITMS) were used for separation and identification of multi-components in Psoralea corylifolia. Benefiting from combining the accurate mass measurement of HPLC-TOFMS to generate elemental compositions, the complementary multilevel structural information provided by HPLC-QITMS and the characteristic UV spectra obtained from HPLC-DAD, 24 components in P. corylifolia were identified. The five groups of isomers were differentiated based on the fragmentation behaviors in QITMS and UV spectra. It can be concluded that an effective method based on the combination of HPLC-DAD, HPLC-TOFMS and HPLC-QITMS for identification of chemical components in P. corylifolia was established. The results provide essential data for further pharmacological and clinical studies of P. corylifolia and facilitate the rapid quality control of the crude drug.

Published
2015

47. Systematic analysis of the use of amphipathic polymers for studies of outer membrane proteins using mass spectrometry

Author

Antonio N. Calabrese, Sheena E. Radford, Fabrice Giusti, Alison E. Ashcroft, Thomas G. Watkinson, Manuela Zoonens, Physico-chimie moléculaire des membranes biologiques (PCMMB), Université Paris Diderot - Paris 7 (UPD7)-Centre National de la Recherche Scientifique (CNRS), and Centre National de la Recherche Scientifique (CNRS)-Université Paris Diderot - Paris 7 (UPD7)

Subjects
Outer membrane proteins, Mass spectrometry, Ion mobility spectrometry–mass spectrometry, Micelle, Article, Protein structure, [CHIM.ANAL]Chemical Sciences/Analytical chemistry, Amphiphile, Physical and Theoretical Chemistry, Instrumentation, Spectroscopy, ComputingMilieux_MISCELLANEOUS, ComputingMethodologies_COMPUTERGRAPHICS, Chromatography, Amphipols, Chemistry, [SDV.BBM.BM]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Molecular biology, Condensed Matter Physics, OmpT, [SDV.BBM.BC]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Biomolecules [q-bio.BM], Electrospray ionisation–mass spectrometry, Ion-mobility spectrometry–mass spectrometry, [CHIM.POLY]Chemical Sciences/Polymers, Membrane protein, Protein conformation, Biophysics, Bacterial outer membrane
Abstract

Graphical abstract, Highlights • Outer membrane protein conformational analysis. • Use of amphipols for mass spectrometry analyses. • Comparison of a range of amphipols for membrane protein analysis., Membrane proteins (MPs) are essential for numerous important biological processes. Recently, mass spectrometry (MS), coupled with an array of related techniques, has been used to probe the structural properties of MPs and their complexes. Typically, detergent micelles have been employed for delivering MPs into the gas-phase, but these complexes have intrinsic properties that can limit the utility of structural studies of MPs using MS methods. Amphipols (APols) have advantages over detergent micelles and have been shown to be capable of delivering native MPs into the gas-phase. Comparing six different APols which vary in mass and charge, and the detergent n-dodecyl-β-d-maltopyranoside, we aimed to determine which APols are most efficient for delivery of native outer membrane proteins (OMPs) into the gas-phase. We show that maintaining the solution-phase folding and global structures of three different OMPs (PagP, OmpT and tOmpA) are independent of the APol used, but differences in OMP activity can result from the different APol:OMP complexes. ESI-IMS–MS analysis of OMP:APol complexes shows that the A8-35 APol is most proficient at liberating all three OMPs into the gas-phase, without altering their gas-phase conformations.

Published
2015

48. Tip Enhanced Laser Ablation Sample Transfer for Mass Spectrometry

Author

Suman Ghorai, Chinthaka A. Seneviratne, and Kermit K. Murray

Subjects
MALDI imaging, Materials science, Laser ablation, business.industry, Near-field optics, Analytical chemistry, Laser, Mass spectrometry, Mass spectrometry imaging, law.invention, Ion-mobility spectrometry–mass spectrometry, law, Optoelectronics, business, Inductively coupled plasma mass spectrometry
Abstract

Mass spectrometry is one of the primary analysis techniques for biological analysis but there are technological barriers in sampling scale that must be overcome for it to be used to its full potential on the size scale of single cells. Current mass spectrometry imaging methods are limited in spatial resolution when analyzing large biomolecules. The goal of this project is to use atomic force microscope (AFM) tip enhanced laser ablation to remove material from cells and tissue and capture it for subsequent mass spectrometry analysis. The laser ablation sample transfer system uses an AFM stage to hold the metal-coated tip at a distance of approximately 10 nm from a sample surface. The metal tip acts as an antenna for the electromagnetic radiation and enables the ablation of the sample with a spot size much smaller than a laser focused with a conventional lens system. A pulsed nanosecond UV or visible wavelength laser is focused onto the gold-coated silicon tip at an angle nearly parallel with the surface, which results in the removal of material from a spot between 500 nm and 1 µm in diameter and 200 and 500 nm deep. This corresponds to a few picograms of ablated material, which can be captured on a metal surface for MALDI analysis. We have used this approach to transfer small peptides and proteins from a thin film for analysis by mass spectrometry as a first step toward high spatial resolution imaging.

Published
2015

49. Screening and classifying small-molecule inhibitors of amyloid formation using ion mobility spectrometry–mass spectrometry

Author

Ling Hsien Tu, Janet C. Saunders, Daniel P. Raleigh, Alison E. Ashcroft, Richard Foster, Lydia M. Young, Sheena E. Radford, Charlotte H. Revill, and Rachel A. Mahood

Subjects
Aging, Amyloid, Spectrometry, Mass, Electrospray Ionization, General Chemical Engineering, Electrospray ionization, Molecular Sequence Data, Plasma protein binding, Neurodegenerative, Alzheimer's Disease, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Article, Small Molecule Libraries, 03 medical and health sciences, Acquired Cognitive Impairment, Humans, Amino Acid Sequence, Colloids, Peptide sequence, 030304 developmental biology, 0303 health sciences, Nonspecific binding, Amyloid beta-Peptides, Spectrometry, Chemistry, Electrospray Ionization, Organic Chemistry, Alzheimer's Disease including Alzheimer's Disease Related Dementias (AD/ADRD), General Chemistry, Mass, Small molecule, Peptide Fragments, Brain Disorders, Islet Amyloid Polypeptide, 0104 chemical sciences, Ion-mobility spectrometry–mass spectrometry, Biochemistry, 5.1 Pharmaceuticals, Neurological, Chemical Sciences, Dementia, Development of treatments and therapeutic interventions, Protein Binding
Abstract

The search for therapeutic agents which bind specifically to precursor protein conformations and inhibit amyloid assembly is an important challenge. Identifying such inhibitors is difficult since many protein precursors of aggregation are partially folded or intrinsically disordered, ruling out structure-based design. Furthermore, inhibitors can act by a variety of mechanisms, including specific or non-specific binding, as well as colloidal inhibition. Here we report a high throughput method based on ion mobility spectrometry-mass spectrometry (IMS-MS) that is capable of rapidly detecting small molecules that bind to amyloid precursors, identifying the interacting protein species, and defining the mode of inhibition. Using this method we have classified a variety of small molecules that are potential inhibitors of human islet amyloid polypeptide (hIAPP) aggregation or amyloid-beta 1-40 (Aβ40) aggregation as either specific, non-specific, colloidal or non-interacting. We also demonstrate the ability of IMS-MS to screen for inhibitory small molecules in a 96-well plate format and use this to discover a new inhibitor of hIAPP amyloid assembly.

Published
2014

50. Identification of phase-II metabolites of flavonoids by liquid chromatography-ion-mobility spectrometry-mass spectrometry

Author

Hans-Gerd Janssen, Patrick Augustijns, Boudewijn Hollebrands, Guus Duchateau, and Clément Chalet

Subjects
0301 basic medicine, Ion-mobility spectrometry, Tandem mass spectrometry, Mass spectrometry, 01 natural sciences, Biochemistry, Flavones, Mass Spectrometry, Analytical Chemistry, 03 medical and health sciences, Flavonols, Glucuronides, Isomerism, Tandem Mass Spectrometry, Structural isomer, Humans, chemistry.chemical_classification, Flavonoids, Chromatography, Chemistry, 010401 analytical chemistry, 0104 chemical sciences, 030104 developmental biology, Ion-mobility spectrometry–mass spectrometry, Glucuronide, HT29 Cells, Chromatography, Liquid
Abstract

Flavonoids are a class of natural compounds with a broad range of potentially beneficial health properties. They are subjected to an extensive intestinal phase-II metabolism, i.e., conjugation to glucuronic acid, sulfate, and methyl groups. Flavonoids and their metabolites can interact with drug transporters and thus interfere with drug absorption, causing food-drug interactions. The site of metabolism plays a key role in the activity, but the identification of the various metabolites remains a challenge. Here, we developed an analytical method to identify the phase-II metabolites of structurally similar flavonoids. We used liquid chromatography-ion-mobility spectrometry-mass spectrometry (LC-IMS-MS) analysis to identify phase-II metabolites of flavonols, flavones, and catechins produced by HT29 cells. We showed that IMS could bring valuable structural information on the different positional isomers of the flavonols and flavones. The position of the glucuronide moiety had a strong influence on the collision cross section (CCS) of the metabolites, with only minor contribution of hydroxyl and methyl moieties. For the catechins, fragmentation data obtained from MS/MS analysis appeared more useful than IMS to determine the structure of the metabolites, mostly due to the high number of metabolites formed. Nevertheless, CCS information as a molecular fingerprint proved to be useful to identify peaks from complex mixtures. LC-IMS-MS thus appears as a valuable tool for the identification of phase-II metabolites of flavonoids. Graphical abstract Structural identification of phase-II metabolites of flavonoids using LC-IMS-MS. ispartof: Analytical and Bioanalytical Chemistry vol:410 issue:2 pages:471-482 ispartof: location:Germany status: published

Published
2017

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