Your search keyword '"Chromatography, Reverse-Phase"' showing total 326 results

1. Ultra-short columns for the chromatographic analysis of large molecules.

Author

Fekete S and Guillarme D

Subjects

Chromatography, High Pressure Liquid, Chromatography, Ion Exchange methods, Hydrophobic and Hydrophilic Interactions, Chromatography, Reverse-Phase, Proteins chemistry

Abstract

Today, reverse phase liquid chromatography (RPLC) analysis of proteins is almost exclusively performed on conventional columns (100-150 mm) in gradient elution mode. However, it was shown many years ago that large molecules present an on/off retention mechanism, and that only a very short inlet segment of the chromatographic column retains effectively the large molecules. Much shorter columns - like only a few centimetres or even a few millimetres - can therefore be used to efficiently analyse such macromolecules. The aim of this review is to summarise the historical and more recent works related to the use of very short columns for the analysis of model and therapeutic proteins. To this end, we have outlined the theoretical concepts behind the use of short columns, as well as the instrumental limitations and potential applications. Finally, we have shown that these very short columns were also possibly interesting for other chromatographic modes, such as ion exchange chromatography (IEX), hydrophilic interaction chromatography (HILIC) or hydrophobic interaction chromatography (HIC), as analyses in these chromatographic modes are performed in gradient elution mode., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2023. Published by Elsevier B.V.)

Published

2023

2. Understanding and managing peak shape for basic solutes in reversed-phase high performance liquid chromatography.

Author

McCalley DV

Subjects

Chromatography, High Pressure Liquid methods, Chromatography, Reverse-Phase, Proteins

Abstract

While other separation mechanisms can challenge the dominance of reversed phase (for example in the separation of native proteins), reversed phase liquid chromatography is the method of choice for the analysis of a wide variety of samples. However, basic solutes (including small molecules, peptides and proteins) can give broad peaks, ofteh with severe peak tailing, which negatively affects peak identification and quantitation. In this feature article, the causes of low efficiency and peak asymmetry are discussed, including the choices of stationary and mobile phases that can minimise these detrimental effects. The contributory effects of column overloading to peak asymmetry are also considered although the exact causes of these effects remain of considerable debate.

Published

2023

3. Design Guidelines and Kinetic Performance Limits for Spatial Comprehensive Three-Dimensional Chromatography for the Analysis of Intact Proteins.

Author

Themelis T, De Vos J, and Eeltink S

Subjects

Chromatography, Liquid methods, Chromatography, Reverse-Phase methods, Proteins

Abstract

The design aspects of microfluidic chips for spatial three-dimensional chromatography featuring an interconnected channel network and targeting protein analysis are discussed, and the corresponding kinetic performance limits have been established using a Pareto-optimality approach. The pros and cons to integrate different separation mechanisms (IEF, CE, SEC, RPLC, HILIC, HIC, and IEX) are discussed considering development stages in the spatial domain ( x LC) in the first and second dimension and time domain ( t LC) for the third dimension. Based on Pareto-optimization, we discuss the considerations of the channel length, particle diameter, and the effect of number of second- and third-dimension channels on the resulting peak capacity of a spatial x IEF × x SEC × t RPLC device. Novel equations are proposed to determine the peak capacity in x SEC and to account for sample modulation affected by the number of second- and third-dimension channels. The corresponding Pareto fronts have been constructed demonstrating the resolving power, in terms of peak capacity and analysis time, considering current state-of-the-art prototyping methodologies. A microfluidic spatial prototype chip with an integrated channel layout (64 2 D and 4096 3 D channels) has been created, which has the potential to yield a peak capacity of 32,600 within only 44 min of the total analysis time, by implementing x IEF × x SEC × t RPLC separation stages.

Published

2022

4. A simple mathematical treatment for predicting linear solvent strength behavior in gradient elution: Application to biomolecules.

Author

Guillarme D, Bouvarel T, Rouvière F, and Heinisch S

Subjects

Chromatography, High Pressure Liquid methods, Peptides chemistry, Solvents chemistry, Chromatography, Reverse-Phase, Proteins

Abstract

This paper describes an approach to rapidly and easily calculate the linear solvent strength parameters, namely log k 0 and S, under reversed-phase liquid chromatography conditions. This approach, which requires two preliminary gradient experiments to determine the retention parameters, was applied to various representative compounds including small molecules, peptides, and proteins. The retention time prediction errors were compared to the ones obtained with a commercial HPLC modeling software, and a good correlation was found between the values. However, two important constraints have to be accounted for to maintain good predictions with this new approach: i) the retention factor at the initial composition of the preliminary gradient series have to be large enough (i.e., log k i above 2.1) and ii) the retention models have to be sufficiently linear. While these two conditions are not always met with small molecules or even peptides, the situation is different with large biomolecules. This is why our simple calculation method should be preferentially applied to calculate the linear solvent strength parameters of protein samples., (© 2022 The Authors. Journal of Separation Science published by Wiley-VCH GmbH.)

Published

2022

5. High-Throughput Chromatographic Separation of Oligonucleotides: A Proof of Concept Using Ultra-Short Columns.

Author

Lardeux H, Fekete S, Lauber M, D'Atri V, and Guillarme D

Subjects

Chromatography, High Pressure Liquid methods, Chromatography, Reverse-Phase methods, Ions, Oligonucleotides chemistry, Proteins

Abstract

Ion-pairing reversed-phase liquid chromatography (IP-RPLC) is the reference separation technique for characterizing oligonucleotides (ONs) and their related impurities. The aim of this study was to better understand the retention mechanism of ONs, evaluate the applicability of the linear solvent strength (LSS) retention model, and explore the potential of ultra-short columns having a length of only 5 mm for the separation of model ONs. First, the validity of the LSS model was evaluated for ONs having sizes comprised between 3 and 30 kDa, and the accuracy of retention time predictions was assessed. It was found that ONs in IP-RPLC conditions follow an "on-off" elution behavior, despite a molecular weight lower than that of proteins. For most linear gradient separation conditions, a column length between 5 and 35 mm was found to be appropriate. Ultra-short columns of only 5 mm were therefore explored to speed up separations by considering the impact of the instrumentation on the efficiency. Interestingly, the impacts of injection volume and post-column connection tubing on peak capacity were found to be negligible. Finally, it was demonstrated that longer columns would not improve selectivity or separation efficiency, but baseline separation of three model ONs mixtures was enabled in as little as 30 s on the 5 mm column. This proof-of-concept work paves the way for future investigations using more complex therapeutic ONs and their related impurities.

Published

2023

6. Relative Quantification of Phosphorylated and Glycosylated Peptides from the Same Sample Using Isobaric Chemical Labelling with a Two-Step Enrichment Strategy.

Author

Silbern I, Fang P, Ji Y, Christof L, Urlaub H, and Pan KT

Subjects

Animals, Cell Line, Glycosylation, Humans, Phosphorylation, Research Design, Chromatography, High Pressure Liquid, Chromatography, Reverse-Phase, Isotope Labeling, Protein Processing, Post-Translational, Proteins analysis, Proteomics, Tandem Mass Spectrometry

Abstract

Post-translational modifications (PTMs) are essential for the regulation of all cellular processes. The interplay of various PTMs on a single protein or different proteins comprises a complexity that we are far from understanding in its entirety. Reliable strategies for the enrichment and accurate quantification of PTMs are needed to study as many PTMs on proteins as possible. In this protocol we present a liquid chromatography-tandem mass spectrometry (LC/MS/MS)-based workflow that enables the enrichment and quantification of phosphorylated and N-glycosylated peptides from the same sample. After extraction and digestion of proteins, we label the peptides with stable isotope-coded tandem mass tags (TMTs) and enrich N-glycopeptides and phosphopeptides by using zwitterionic hydrophilic interaction chromatography (ZIC-HILIC) and titanium dioxide (TiO 2 ) beads, respectively. Labelled and enriched N-glycopeptides and phosphopeptides are further separated by high pH (basic) reversed-phase chromatography and analyzed by LC/MS/MS. The enrichment strategies, together with quantification of two different PTM types from the same sample, allow investigation of the interplay of those two PTMs, which are important for signal transduction inside the cell (phosphorylation), as well as for messaging between cells through decoration of the cellular surface (glycosylation).

Published

2021

7. Making Sharper Peaks for Reverse-Phase Liquid Chromatography of Proteins.

Author

Bupp CR and Wirth MJ

Subjects

Particle Size, Surface Properties, Chromatography, Reverse-Phase, Proteins analysis

Abstract

Protein separations have gained increasing interest over the past two decades owing to the dramatic growth of proteins as therapeutics and the completion of the Human Genome Project. About every decade, the field of protein high-performance liquid chromatography (HPLC) seems to mature, having reached what appears to be a theoretical limit. But then scientists well versed in the basic principles of HPLC invented a way around the limit, generating another decade of exciting progress. There is still the need for higher resolution and better compatibility with mass spectrometry because it is an essential tool for identification of proteins and their modifications. To make advances, the fundamental principles need to be understood. This review covers recent advances and current needs in the context of the principles that underlie the many contributions to peak broadening.

Published

2020

8. A comprehensive investigation of the peak capacity for the reversed-phase gradient liquid-chromatographic analysis of intact proteins using a polymer-monolithic capillary column.

Author

Fernández-Pumarega A, Dores-Sousa JL, and Eeltink S

Subjects

Chromatography, Reverse-Phase instrumentation, Diffusion, Molecular Weight, Polymers chemistry, Proteins chemistry, Chromatography, Reverse-Phase methods, Proteins isolation & purification

Abstract

The present study reports on the analysis of different factors affecting the magnitude of the peak capacity for intact protein separations conducted in gradient reversed-phase liquid chromatography. Experiments were conducted using a 200 µm i.d. capillary styrene-co-divinylbenzene monolithic column that was developed in-house and was characterized by a mode globule cluster size of 1.2 µm and a mode macropore size of 1.0 µm (based on scanning electron microscopy). The monolith yielded a minimum plate-height value of 13.3 µm for uracil. The use of trifluoroacetic acid instead of formic acid as ion-pairing agent generally led to better peak symmetry, narrower peak widths which effect is protein-dependent, and improved loadability characteristics. The peak capacity has been systematically assessed at different flow rates and gradient duration. The highest peak capacity of 247 was obtained at a flow rate of 1 µL min -1 and a gradient time of 120 min, which corresponds to an optimal t G /t 0 ratio of ∼60. While the optimum van Deemter velocity for intact proteins was approximated to be 0.065 µL min -1 , the highest peak capacity was achieved at approximately 20-fold higher flow rate, depending on the gradient duration applied and the molecular weight of the proteins. The optimum velocity increased with decreasing gradient time and is a compromise between the magnitude of the mass-transfer contribution (decreasing the peak capacity with velocity) affected by molecular diffusion, and the increase in peak capacity induced by the more favorable gradient-volume ratio., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2020

9. Fabrication of a monolithic, macroporous diallyl maleate-based material and its application for fast separation of intact proteins from human plasma with reversed-phase chromatography.

Author

Lan D, Bai L, Liu H, Guo H, and Yan H

Subjects

Chromatography, High Pressure Liquid, Humans, Plasma chemistry, Proteomics, Blood Chemical Analysis methods, Chromatography, Reverse-Phase, Maleates chemistry, Proteins isolation & purification

Abstract

A monolithic diallyl maleate-based column was developed and used to separate intact proteins from complex bio-samples with high-performance liquid chromatography. The resulting monolith exhibited a relatively uniform porous structure with macro-pores. A sample of standard proteins mixture was used to explore the reversed-phase mechanism for fast separation on the homemade monolithic column. The observed retention time increased with the values of the diameters, relative hydrophobicities and molecular weights of the standard proteins, which mainly depends on the relative hydrophobicity of the proteins. It is worth mentioning that the mask of the three most abundant proteins in human plasma can be avoided, thus providing an opportunity for the middle- and low-abundance proteins to be detected. According to this exploration, the fast separation of human plasma proteins on the diallyl maleate-based monolithic column was achieved in 15 min. The chromatographic fractions were identified by liquid chromatography-tandem mass spectrometry, and the results indicate that the present method is an outstanding method for the fast and efficient fractionation of human plasma that will be significant sense for plasma proteomics research, especially for exploring new disease marker and drug target., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2019

10. Quantification of In Vitro Protein Lysine Acetylation by Reversed Phase HPLC.

Author

Njeri CW, Ononye OE, and Balakrishnan L

Subjects

Acetyl Coenzyme A chemistry, Acetyl Coenzyme A metabolism, Acetylation, Lysine metabolism, Lysine Acetyltransferases chemistry, Lysine Acetyltransferases metabolism, Proteins metabolism, Chromatography, High Pressure Liquid methods, Chromatography, Reverse-Phase methods, Lysine chemistry, Proteins chemistry

Abstract

Protein lysine acetylation is a reversible posttranslational modification that is catalyzed by a group of enzymes that are collectively referred to as lysine (K) acetyltransferases (KATs). These enzymes catalyze the transfer of the acetyl group from acetyl coenzyme A (Ac-CoA) to the ε-amino group of lysine amino acid. Protein lysine acetylation plays a critical role in the regulation of important cellular processes and it is therefore paramount that we understand the catalytic mechanisms of these enzymes. While there is a variety of methods that have been developed to analyze the enzymatic properties of KATs, majority of the proposed methods have considerable limitations. We describe here a reversed phase HPLC based method that monitors substrate consumption and product formation simultaneously. This method is highly reproducible and optimally suited for the determination of accurate kinetic parameters of KATs.

Published

2019

11. Two-dimensional chromatographic analysis using three second-dimension columns for continuous comprehensive analysis of intact proteins.

Author

Zhu Z, Chen H, Ren J, Lu JJ, Gu C, Lynch KB, Wu S, Wang Z, Cao C, and Liu S

Subjects

Animals, Chromatography, High Pressure Liquid instrumentation, Chromatography, Ion Exchange instrumentation, Chromatography, Reverse-Phase instrumentation, Complex Mixtures chemistry, Electrophoresis, Polyacrylamide Gel, Escherichia coli chemistry, Humans, Chromatography, High Pressure Liquid methods, Chromatography, Ion Exchange methods, Chromatography, Reverse-Phase methods, Proteins isolation & purification

Abstract

We develop a new two-dimensional (2D) high performance liquid chromatography (HPLC) approach for intact protein analysis. Development of 2D HPLC has a bottleneck problem - limited second-dimension (second-D) separation speed. We solve this problem by incorporating multiple second-D columns to allow several second-D separations to be proceeded in parallel. To demonstrate the feasibility of using this approach for comprehensive protein analysis, we select ion-exchange chromatography as the first-dimension and reverse-phase chromatography as the second-D. We incorporate three second-D columns in an innovative way so that three reverse-phase separations can be performed simultaneously. We test this system for separating both standard proteins and E. coli lysates and achieve baseline resolutions for eleven standard proteins and obtain more than 500 peaks for E. coli lysates. This is an indication that the sample complexities are greatly reduced. We see less than 10 bands when each fraction of the second-D effluents are analyzed by sodium dodecyl sulfate - polyacrylamide gel electrophoresis (SDS-PAGE), compared to hundreds of SDS-PAGE bands as the original sample is analyzed. This approach could potentially be an excellent and general tool for protein analysis., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2018

12. Generic multicriteria approach to determine the best precipitation agent for removal of biomacromolecules prior to non-targeted metabolic analysis.

Author

Knudsen SB, Nielsen NJ, Qvist J, Andersen KB, and Christensen JH

Subjects

Acetonitriles chemistry, Algorithms, Chemical Precipitation, Methanol chemistry, Principal Component Analysis, Proteins chemistry, Solvents chemistry, Chromatography, High Pressure Liquid methods, Chromatography, Reverse-Phase methods, Metabolomics methods, Proteins isolation & purification

Abstract

The removal of biomacromolecules from biofluids decreases the sample complexity and lower electrospray suppression effects. Furthermore, it can increase the analysis sensitivity, precision, and selectivity. Often removal approaches evaluate the model based on a single criterion, like protein removed or response of one of few specific metabolites. In this study, we used a multicriteria approach to test the effect of using the solvents methanol and acetonitrile (organic solvent precipitation), trichloroacetic acid (acidic precipitation) and ammonium sulphate (salting out) to remove biomacromolecules from a downstream recovery process from a bacillus fermentation. The downstream recovery process intermediates were analysed using reversed-phase ultra-high-pressure liquid chromatography with electrospray ionisation and high-resolution time-of-flight mass spectrometry detection. To evaluate the pre-treatment agents the following multicriteria was applied i) practical considerations, ii) total amino acid in the precipitated pellet, iii) putative identification of the molecules removed or created by the different treatments, iv) coherence between high quality extracted ion chromatograms (repeatability of DW-CODA) and v) replicate consistency from principal component analysis score values obtained by using the CHEMometric analysis of sections of Selected Ion Chromatograms (CHEMSIC) method. This study presents a generic workflow to find the best pre-treatment for removing bio-macromolecules from biofluids with a multicriteria approach. In our case, the best protein removal strategy for downstream recovery intermediates was acetonitrile precipitation. This method showed high precision, created few artefact peaks compared to simple sample dilution, and mainly removed small peptides., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

13. Charge variant analysis of protein-based biopharmaceuticals using two-dimensional liquid chromatography hyphenated to mass spectrometry.

Author

Jaag S, Shirokikh M, and Lämmerhofer M

Subjects

Antibodies, Monoclonal, Humanized analysis, Chromatography, High Pressure Liquid, Rheology, Biological Products analysis, Chromatography, Reverse-Phase methods, Proteins analysis, Spectrometry, Mass, Electrospray Ionization

Abstract

The profile of charge variants represents an important critical quality attribute of protein-based biopharmaceuticals, in particular of monoclonal antibodies, and must therefore becontrolled. In this work, 2D-LC methods for charge variant analysis were developed using a strong cation-exchange chromatography (SCX) as first dimension ( 1 D) separation. Non-porous SCX (3 µm) particle columns and different mobile phases were evaluated using a test mixture of some standard proteins of different size and pI (comprising myoglobin, bovine serum albumin, cytochrome c, lysozyme and β-lactoglobulin) and two monoclonal IgG1 antibodies (NIST mAb and Secukinumab). The most promising 1 D eluent for SCX was a salt-mediated pH-gradient system using a ternary mobile phase system with 2-(N-morpholino)ethanesulfonic acid, 1,3-diamino-2-propanol and sodium chloride. For the second dimension ( 2 D), a desalting reversed-phase liquid chromatography (RP-LC) was chosen to enable the hyphenation of the charge variant separation with mass spectrometric (MS) detection. While for intact mAbs the 2 D just served for desalting without additional selectivity, the 2 D contributed some orthogonal selectivity for the mAb fragment separation. Various core-shell and monolithic columns were tested and variables such as gradient time and flow rate systematically optimized. Unexpectedly, a C4 400 Å column (3.4 µm diameter with 0.2 µm porous shell) provided higher peak capacities compared to the same 1000 Å column (2.7 µm diameter with 0.5 µm porous shell). A thinner shell appeared to be more advantageous than wider pores under high flow regime. An ultra-fast RP-LC method with a run time of one minute was developed using trifluoroacetic acid which was later replaced by formic acid as additive for better MS compatibility. The successful hyphenation of the two orthogonal separation modes, SCX and RP-LC, could be demonstrated in the multiple heart-cutting and the full comprehensive mode. MS analysis using a high-resolution quadrupole time-of-flight instrument enabled to identify different glycoforms and some major charge variants of the antibody at the intact protein level as well as on the subunit level (Fc/2, Lc, Fd') in a middle-up approach by 2D-LC-ESI-MS analysis., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2020. Published by Elsevier B.V.)

Published

2021

14. Quantification and Identification of Post-Translational Modifications Using Modern Proteomics Approaches.

Author

Holtz A, Basisty N, and Schilling B

Subjects

Acetylation, Animals, Chromatography, High Pressure Liquid, Chromatography, Reverse-Phase, High-Throughput Screening Assays, Liver chemistry, Mice, Research Design, Protein Processing, Post-Translational, Proteins analysis, Proteomics, Spectrometry, Mass, Electrospray Ionization, Tandem Mass Spectrometry

Abstract

Post-translational modifications (PTMs) occur dynamically, allowing cells to quickly respond to changes in the environment. Lysine residues can be targeted by several modifications including acylations (acetylation, succinylation, malonylation, glutarylation, and others), methylation, ubiquitination, and other modifications. One of the most efficient methods for the identification of post-translational modifications is utilizing immunoaffinity enrichment followed by high-resolution mass spectrometry. This workflow can be coupled with comprehensive data-independent acquisition (DIA) mass spectrometry to be a high-throughput, label-free PTM quantification approach. Below we describe a detailed protocol to process tissue by homogenization and proteolytically digest proteins, followed by immunoaffinity enrichment of lysine-acetylated peptides to identify and quantify relative changes of acetylation comparing different conditions.

Published

2021

15. High-Throughput Profiling of Proteome and Posttranslational Modifications by 16-Plex TMT Labeling and Mass Spectrometry.

Author

Yu K, Wang Z, Wu Z, Tan H, Mishra A, and Peng J

Subjects

Alzheimer Disease metabolism, Chromatography, Reverse-Phase, Frontal Lobe chemistry, Humans, Phosphorylation, Research Design, Ubiquitination, High-Throughput Screening Assays, Protein Processing, Post-Translational, Proteins analysis, Proteome, Proteomics, Tandem Mass Spectrometry

Abstract

Mass spectrometry (MS)-based proteomic profiling of whole proteome and protein posttranslational modifications (PTMs) is a powerful technology to measure the dynamics of proteome with high throughput and deep coverage. The reproducibility of quantification benefits not only from the fascinating developments in high-performance liquid chromatography (LC) and high-resolution MS with enhanced scan rates but also from the invention of multiplexed isotopic labeling strategies, such as the tandem mass tags (TMT). In this chapter, we introduce a 16-plex TMT-LC/LC-MS/MS protocol for proteomic profiling of biological and clinical samples. The protocol includes protein extraction, enzymatic digestion, PTM peptide enrichment, TMT labeling, and two-dimensional reverse-phase liquid chromatography fractionation coupled with tandem mass spectrometry (MS/MS) analysis, followed by computational data processing. In general, more than 10,000 proteins and tens of thousands of PTM sites (e.g., phosphorylation and ubiquitination) can be confidently quantified. This protocol provides a general protein measurement tool, enabling the dissection of protein dysregulation in any biological samples and human diseases.

Published

2021

16. Quantitative Proteomic Analysis Using Formalin-Fixed, Paraffin-Embedded (FFPE) Human Cardiac Tissue.

Author

Azimzadeh O, Atkinson MJ, and Tapio S

Subjects

Autopsy, Chromatography, Reverse-Phase, Humans, Tandem Mass Spectrometry, Fixatives chemistry, Formaldehyde chemistry, Myocardium metabolism, Paraffin Embedding, Proteins analysis, Proteome, Proteomics, Tissue Fixation

Abstract

Clinical tissue archives represent an invaluable source of biological information. Formalin-fixed, paraffin-embedded (FFPE) tissue can be used for retrospective investigation of biomarkers of diseases and prognosis.Recently, the number of studies using proteome profiling of samples from clinical archives has markedly increased. However, the application of conventional quantitative proteomics technologies remains a challenge mainly due to the harsh fixation process resulting in protein cross-linking and protein degradation. In the present chapter, we demonstrate a protocol for label-free proteomic analysis of FFPE tissue prepared from human cardiac autopsies. The data presented here highlight the applicability and suitability of FFPE heart tissue for understanding the molecular mechanism of cardiac injury using a proteomics approach.

Published

2021

17. Missing Value Monitoring to Address Missing Values in Quantitative Proteomics.

Author

Matafora V and Bachi A

Subjects

Animals, Chromatography, Reverse-Phase, Humans, Research Design, Workflow, Proteins analysis, Proteome, Proteomics, Tandem Mass Spectrometry

Abstract

Many classes of key functional proteins such as transcription factors or cell cycle proteins are present in the proteome at a very low concentration. These low-abundance proteins are almost entirely invisible to systematic quantitative analysis by classical data dependent proteomics methods (DDA). Moreover, DDA runs in shotgun proteomics experiments are plenty of missing values among the replicates due to the stochastic nature of the acquisition method, thus hampering the robustness of the quantitative analysis. Here, we have overcome these obstacles designing a robust workflow named missing value monitoring (MvM) in order to follow low abundance proteins dynamics.

Published

2021

18. Quantifying Proteome and Protein Modifications in Activated T Cells by Multiplexed Isobaric Labeling Mass Spectrometry.

Author

Tan H, Blanco DB, Xie B, Li Y, Wu Z, Chi H, and Peng J

Subjects

Acetylation, Animals, Chromatography, High Pressure Liquid, Chromatography, Reverse-Phase, Humans, Immunomagnetic Separation, Methylation, Phosphorylation, Research Design, T-Lymphocytes immunology, Workflow, Lymphocyte Activation, Protein Processing, Post-Translational, Proteins analysis, Proteome, Proteomics, T-Lymphocytes metabolism, Tandem Mass Spectrometry

Abstract

The dynamic regulation of protein function by altered protein expression and post-translational modifications (PTMs) is essential for T cell function, but it has remained difficult to systemically quantify such events. Mass spectrometry (MS)-based proteomics has become a mainstream tool for comprehensive profiling of proteome and PTMs, especially with the development of multiplexed isobaric labeling methods, such as tandem mass tag (TMT), coupled with high-resolution two-dimensional liquid chromatography and tandem mass spectrometry (LC/LC-MS/MS). Here, we introduce a deep proteomics profiling protocol with an optimized 11-plex TMT-LC/LC-MS/MS platform to quantitate whole proteome, phosphoproteome, acetylome, and methylome in activated T cells. The major steps include preparation of activated T cells, protein extraction and digestion, TMT labeling, basic pH reverse phase LC, modified peptide enrichment, acidic pH reverse phase LC-MS/MS, and computational data processing. Approximately 10,000 proteins, 30,000 phosphosites, 2,000 lysine acetylated sites, and 1,000 lysine methylated sites can be identified and quantified from 1 mg of proteins per sample. Quality control steps are implemented in this protocol, and future development, such as nanoscale 16-plex TMT analysis, is discussed. This multiplexed and robust method provides a powerful tool for dissecting proteomic and PTM signatures in T cells at the systems level, and it is equally suitable for other biological samples, including effector T cell subsets.

Published

2021

19. Comprehensive Protocol to Simultaneously Study Protein Phosphorylation, Acetylation, and N-Linked Sialylated Glycosylation.

Author

Melo-Braga MN, Ibáñez-Vea M, Kulej K, and Larsen MR

Subjects

Acetylation, Chromatography, Affinity, Chromatography, Reverse-Phase, Glycosylation, Immunoprecipitation, Phosphorylation, Spectrometry, Mass, Electrospray Ionization, Tandem Mass Spectrometry, Titanium chemistry, Workflow, Protein Processing, Post-Translational, Proteins analysis, Proteomics

Abstract

Posttranslational modifications (PTMs) such as phosphorylation, acetylation, and glycosylation are an essential regulatory mechanism of protein function and interaction, and they are associated with a wide range of biological processes. Since most PTMs alter the molecular mass of a protein, mass spectrometry (MS) is the ideal analytical tool for studying various PTMs. However, PTMs are often present in substoichiometric levels, and therefore their unmodified counterpart often suppresses their signal in MS. Consequently, PTM analysis by MS is a challenging task, requiring highly specialized and sensitive PTM-specific enrichment methods. Currently, several methods have been implemented for PTM enrichment, and each of them has its drawbacks and advantages as they differ in selectivity and specificity toward specific protein modifications. Unfortunately, for the vast majority of more than 400 known modifications, we have no or poor tools for selective enrichment.Here, we describe a comprehensive workflow to simultaneously study phosphorylation, acetylation, and N-linked sialylated glycosylation from the same biological sample. The protocol involves an initial titanium dioxide (TiO 2 ) step to enrich for phosphopeptides and sialylated N-linked glycopeptides followed by glycan release and post-fractionation using sequential elution from immobilized metal affinity chromatography (SIMAC) to separate mono-phosphorylated and deglycosylated peptides from multi-phosphorylated ones. The IMAC flow-through and acidic elution are subsequently subjected to a next round of TiO 2 enrichment for further separation of mono-phosphopeptides from deglycosylated peptides. Furthermore, the lysine-acetylated peptides present in the first TiO 2 flow-through fraction are enriched by immunoprecipitation (IP) after peptide cleanup. Finally, the samples are fractionated by high pH reversed phase chromatography (HpH) or hydrophilic interaction liquid chromatography (HILIC ) to reduce sample complexity and increase the coverage in the subsequent LC-MS /MS analysis. This allows the analysis of multiple types of modifications from the same highly complex biological sample without decreasing the quality of each individual PTM study.

Published

2021

20. Isolation of Extracellular Vesicles for Proteomic Profiling.

Author

Choi D, Rak J, and Gho YS

Subjects

Cell Line, Tumor, Centrifugation, Density Gradient, Chromatography, Reverse-Phase, Humans, Mass Spectrometry, Proteolysis, Ultracentrifugation, Analytic Sample Preparation Methods, Exosomes metabolism, Proteins isolation & purification, Proteome, Proteomics

Abstract

Extracellular vesicles (EVs) are nano-sized lipid bilayer surrounded by structures released from most cells, including archaea, bacteria, and eukaryotic cells. EVs play multiple roles in cell-to-cell communication, including immune modulation, angiogenesis, and phenotypic transformation of cells by transferring genetic material and functional proteins. They contain specific subsets of proteins, DNA, RNA, and lipids that represent their cellular origin. Furthermore, EVs are enriched in cell type- or disease-specific proteins, especially plasma membrane proteins, which have pathophysiological functions; many of these vesicular proteins are investigated as novel diagnostic biomarkers, as well as therapeutic targets. To profile the global EV proteome, their various purification methods have been developed, of which density gradient ultracentrifugation is considered especially promising. In this chapter, we describe the isolation of EVs derived from SW480 cells with serum-free media and from U373 cells with EV-depleted serum-containing media, and the preparation of tryptic peptides for mass-spectrometry-based proteomic analysis.

Published

2021

21. Applicability of linear and nonlinear retention-time models for reversed-phase liquid chromatography separations of small molecules, peptides, and intact proteins.

Author

Tyteca E, De Vos J, Vankova N, Cesla P, Desmet G, and Eeltink S

Subjects

Chromatography, High Pressure Liquid, Models, Molecular, Molecular Weight, Peptides chemistry, Phenols chemistry, Proteins chemistry, Time Factors, Chromatography, Reverse-Phase, Peptides isolation & purification, Phenols isolation & purification, Proteins isolation & purification

Abstract

The applicability and predictive properties of the linear solvent strength model and two nonlinear retention-time models, i.e., the quadratic model and the Neue model, were assessed for the separation of small molecules (phenol derivatives), peptides, and intact proteins. Retention-time measurements were conducted in isocratic mode and gradient mode applying different gradient times and elution-strength combinations. The quadratic model provided the most accurate retention-factor predictions for small molecules (average absolute prediction error of 1.5%) and peptides separations (with a prediction error of 2.3%). An advantage of the Neue model is that it can provide accurate predictions based on only three gradient scouting runs, making tedious isocratic retention-time measurements obsolete. For peptides, the use of gradient scouting runs in combination with the Neue model resulted in better prediction errors (<2.2%) compared to the use of isocratic runs. The applicability of the quadratic model is limited due to a complex combination of error and exponential functions. For protein separations, only a small elution window could be applied, which is due to the strong effect of the content of organic modifier on retention. Hence, the linear retention-time behavior of intact proteins is well described by the linear solvent strength model. Prediction errors using gradient scouting runs were significantly lower (2.2%) than when using isocratic scouting runs (3.2%)., (© 2016 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2016

22. Investigation of a Pharmacological Approach for Reduction of Renal Uptake of Radiolabeled ADAPT Scaffold Protein.

Author

Vorobyeva A, Oroujeni M, Lindbo S, Hober S, Xu T, Liu Y, Rinne SS, and Garousi J

Subjects

Animals, Autoradiography, Chromatography, High Pressure Liquid, Chromatography, Reverse-Phase, Female, Mice, Proteins administration & dosage, Proteins metabolism, Radiopharmaceuticals administration & dosage, Tissue Distribution drug effects, Kidney metabolism, Proteins pharmacology, Radiopharmaceuticals pharmacology

Abstract

Albumin binding domain-Derived Affinity ProTeins (ADAPTs) are small (5 kDa) engineered scaffold proteins that are promising targeting agents for radionuclide-based imaging. A recent clinical study has demonstrated that radiolabeled ADAPTs can efficiently visualize human epidermal growth factor receptor 2 (HER2) expression in breast cancer using SPECT imaging. However, the use of ADAPTs directly labeled with radiometals for targeted radionuclide therapy is limited by their high reabsorption and prolonged retention of activity in kidneys. In this study, we investigated whether a co-injection of lysine or gelofusin, commonly used for reduction of renal uptake of radiolabeled peptides in clinics, would reduce the renal uptake of [ 99m Tc]Tc(CO) 3 -ADAPT6 in NMRI mice. In order to better understand the mechanism behind the reabsorption of [ 99m Tc]Tc(CO) 3 -ADAPT6, we included several compounds that act on various parts of the reabsorption system in kidneys. Administration of gelofusine, lysine, probenecid, furosemide, mannitol, or colchicine did not change the uptake of [ 99m Tc]Tc(CO) 3 -ADAPT6 in kidneys. Sodium maleate reduced the uptake of [ 99m Tc]Tc(CO) 3 -ADAPT6 to ca. 25% of the uptake in the control, a high dose of fructose (50 mmol/kg) reduced the uptake by ca. two-fold. However, a lower dose (20 mmol/kg) had no effect. These results indicate that common clinical strategies are not effective for reduction of kidney uptake of [ 99m Tc]Tc(CO) 3 -ADAPT6 and that other strategies for reduction of activity uptake or retention in kidneys should be investigated for ADAPT6.

Published

2020

23. Proteomic Profiling of Emiliania huxleyi Using a Three-Dimensional Separation Method Combined with Tandem Mass Spectrometry.

Author

Yun G, Park JM, Duong VA, Mok JH, Jeon J, Nam O, Lee J, Jin E, and Lee H

Subjects

Chromatography, Reverse-Phase methods, Gene Ontology, Peptides analysis, Peptides isolation & purification, Proteins chemistry, Proteins isolation & purification, Proteome analysis, Proteome genetics, Proteome isolation & purification, Workflow, Haptophyta chemistry, Proteins analysis, Proteomics methods, Tandem Mass Spectrometry methods

Abstract

Emiliania huxleyi is one of the most abundant marine planktons, and it has a crucial feature in the carbon cycle. However, proteomic analyses of Emiliania huxleyi have not been done extensively. In this study, a three-dimensional liquid chromatography (3D-LC) system consisting of strong cation exchange, high- and low-pH reversed-phase liquid chromatography was established for in-depth proteomic profiling of Emiliania huxleyi . From tryptic proteome digest, 70 fractions were generated and analyzed using liquid chromatography-tandem mass spectrometry. In total, more than 84,000 unique peptides and 10,000 proteins groups were identified with a false discovery rate of ≤0.01. The physicochemical properties of the identified peptides were evaluated. Using ClueGO, approximately 700 gene ontology terms and 15 pathways were defined from the identified protein groups with p -value ≤0.05, covering a wide range of biological processes, cellular components, and molecular functions. Many biological processes associated with CO 2 fixation, photosynthesis, biosynthesis, and metabolic process were identified. Various molecular functions relating to protein binding and enzyme activities were also found. The 3D-LC strategy is a powerful approach for comparative proteomic studies on Emiliania huxleyi to reveal changes in its protein level and related mechanism.

Published

2020

24. Enhancing online protein isolation as intact species from soy flour samples by actively modulated two-dimensional liquid chromatography (2D-LC).

Author

Nardiello D, Melfi MT, Pignatelli C, and Centonze D

Subjects

Plant Extracts analysis, Reference Standards, Chromatography, Gel instrumentation, Chromatography, Liquid methods, Chromatography, Reverse-Phase instrumentation, Flour analysis, Proteins analysis, Glycine max chemistry

Abstract

In this study, an enhanced fully automated approach is described for the protein isolation from soy flour samples by two-dimensional liquid chromatography with active modulation interface. The use of two multi-port switching valves is proposed to on-line connect the first to the second dimension column, thus overcoming the problems associated with the re-mixing effects and incompatibility of eluent composition and pH. A 5-cm long C4 analytical column installed in the interface device allows to focus the proteins coming from the first column (size exclusion chromatography), before their selective elution in the second column (reversed-phase). A trap washing step was included in the total workflow, as a desalting step to remove buffer residues from the eluent of the first column and to enhance the chromatographic performances of the second column. The experimental conditions were optimized by analyses of mixed standard solutions of bovine serum albumin, glucose oxidase, immunoglobulin A, thyroglobulin and myoglobin. Then, the optimized 2D-LC method was applied to the protein analysis in extracts of soy flour, known worldwide as one of the major food allergen sources, with the final aim to recovery sufficient protein amounts for the molecular characterization and the assessment of the pattern of allergenic components., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2020

25. Retention Time Prediction and Protein Identification.

Author

Henneman A and Palmblad M

Subjects

Amino Acid Sequence, Chromatography, Reverse-Phase methods, Electrophoresis, Hydrogen-Ion Concentration, Hydrophobic and Hydrophilic Interactions, Chromatography, Liquid methods, Peptides isolation & purification, Proteins isolation & purification, Proteomics methods, Tandem Mass Spectrometry methods

Abstract

In bottom-up proteomics, proteins are typically identified by enzymatic digestion into peptides, tandem mass spectrometry and comparison of the tandem mass spectra with those predicted from a sequence database for peptides within measurement uncertainty from the experimentally obtained mass. Although now decreasingly common, isolated proteins or simple protein mixtures can also be identified by measuring only the masses of the peptides resulting from the enzymatic digest, without any further fragmentation. Separation methods such as liquid chromatography and electrophoresis are often used to fractionate complex protein or peptide mixtures prior to analysis by mass spectrometry. Although the primary reason for this is to avoid ion suppression and improve data quality, these separations are based on physical and chemical properties of the peptides or proteins and therefore also provide information about them. Depending on the separation method, this could be protein molecular weight (SDS-PAGE), isoelectric point (IEF), charge at a known pH (ion exchange chromatography), or hydrophobicity (reversed phase chromatography). These separations produce approximate measurements on properties that to some extent can be predicted from amino acid sequences. In the case of molecular weight of proteins without posttranslational modifications this is straightforward: simply add the molecular weights of the amino acid residues in the protein. For IEF, charge and hydrophobicity, the order of the amino acids, and folding state of the peptide or protein also matter, but it is nevertheless possible to predict the behavior of peptides and proteins in these separation methods to a degree which renders such predictions useful. This chapter reviews the topic of using data from separation methods for identification and validation in proteomics, with special emphasis on predicting retention times of tryptic peptides in reversed-phase chromatography under acidic conditions, as this is one of the most commonly used separation methods in bottom-up proteomics.

Published

2020

26. Evaluation and comparison of n-alkyl chain and polar ligand bonded stationary phases for protein separation in reversed-phase liquid chromatography.

Author

Ding L, Guo Z, Xiao Y, Xue X, Zhang X, and Liang X

Subjects

Ligands, Proteins chemistry, Chromatography, Reverse-Phase, Proteins isolation & purification

Abstract

Protein retention is very sensitive to the change of solvent composition in reversed-phase liquid chromatography for so called "on-off" mechanism, leading to difficulty in mobile phase optimization. In this study, a novel 3-chloropropyl trichlorosilane ligand bonded column was prepared for protein separation. The differences in retention characteristics between the 3-chloropropyl trichlorosilane ligand bonded column and n-alkyl chain modified (C2, C4, C8) stationary phases were elucidated by the retention equation l nk=a+cC(B). Retention parameters (a and c) of nine standard proteins with different molecular weights were calculated by using homemade software. Results showed that retention times of nine proteins were similar on four columns, but the 3-chloropropyl trichlorosilane ligand bonded column obtained the lowest retention parameter values of larger proteins. It meant that their retention behavior affected by acetonitrile concentration would be different due to lower |c| values. More specifically, protein elution windows were broader, and retentions were less sensitive to the change of acetonitrile concentration on the 3-chloropropyl trichlorosilane ligand bonded column than that on other columns. Meanwhile, the 3-chloropropyl trichlorosilane ligand bonded column displayed distinctive selectivity for some proteins. Our results indicated that stationary phase with polar ligand provided potential solutions to the "on-off" problem and optimization in protein separation., (© 2014 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2014

27. High-throughput absolute quantification of proteins using an improved two-dimensional reversed-phase separation and quantification concatemer (QconCAT) approach.

Author

Wei J, Ding C, Zhang J, Mi W, Zhao Y, Liu M, Fu T, Zhang Y, Ying W, Cai Y, Qin J, and Qian X

Subjects

Amino Acid Sequence, Animals, Chromatography, Reverse-Phase instrumentation, Glutathione Transferase chemistry, High-Throughput Screening Assays instrumentation, Liver metabolism, Mice, Molecular Sequence Data, Proteins metabolism, Proteomics instrumentation, Proteomics methods, Chromatography, Reverse-Phase methods, High-Throughput Screening Assays methods, Liver chemistry, Mass Spectrometry methods, Peptides chemistry, Proteins chemistry

Abstract

Stable isotope dilution-selective reaction monitoring-mass spectrometry (SID-SRM-MS) has been widely used for the absolute quantitative analysis of proteins. However, when performing the large-scale absolute quantification of proteins from a more complex tissue sample, such as mouse liver, in addition to a high-throughput approach for the preparation and calibration of large amounts of stable-isotope-labelled internal standards, a more powerful separation method prior to SRM analysis is also urgently needed. To address these challenges, a high-throughput absolute quantification strategy based on an improved two-dimensional reversed-phase (2D RP) separation and quantification concatemer (QconCAT) approach is presented in this study. This strategy can be used to perform the simultaneous quantification of hundreds of proteins from mouse liver within one week of total MS measurement time. By using calibrated synthesised peptides from the protein glutathione S-transferase (GST), large amounts of GST-tagged QconCAT internal standards corresponding to hundreds of proteins can be accurately and rapidly quantified. Additionally, using an improved 2D RP separation method, a mixture containing a digested sample and QconCAT standards can be efficiently separated and absolutely quantified. When a maximum gradient of 72 min is employed in the first LC dimension, resulting in 72 fractions, identification and absolute quantification experiments for all fractions can be completed within one week of total MS measurement time. The quantification approach developed here can further extend the dynamic range and increase the analytical sensitivity of SRM analysis of complex tissue samples, thereby helping to increase the coverage of absolute quantification in a whole proteome.

Published

2014

28. Improved separation of fluorogenic derivatized intact proteins with high resolution and efficiency using a reversed-phase liquid chromatographic system.

Author

Ichibangase T, Nakata K, and Imai K

Subjects

Chromatography, Reverse-Phase instrumentation, Hepatocytes metabolism, Humans, Proteins chemistry, Proteomics, Chromatography, Reverse-Phase methods, Hepatocytes chemistry, Proteins isolation & purification

Abstract

Although the efficient separation of intact protein mixtures is extremely difficult, reversed-phase chromatography is an important technique for performing quantitative, accurate and reproducible proteomics analyses. Here, we show that, despite the operating constraints of conventional high-performance liquid chromatography, such as column temperature, operating pressure and separation time, comprehensive separation of fluorogenic derivatized intact proteins could be achieved with high resolution and separation efficiency. First, amylin was chosen as a model peptide and used to estimate the separation efficiency with respect to column temperature and flow rate, as indicated by peak capacity. Then, an extract of human primary hepatocytes was used to model complex component mixtures and the separation conditions were optimized. The effects of mobile-phase pH, the separation time and the column length were also investigated. Consequently, more than 890 peaks could be separated efficiently in the extract, which is 1.5-fold greater than when using conventional conditions. Finally, it was demonstrated that both longer separation time and column length contributed greatly to the effective separation of the protein mixture. These results are expected to provide insights into the separation of intact proteins., (Copyright © 2014 John Wiley & Sons, Ltd.)

Published

2014

29. Utilization of a precolumn with size exclusion and reversed-phase modes for size-exclusion chromatographic analysis of polysorbate-containing protein aggregates.

Author

Fukuda J, Iura T, Yanagihara S, and Kano K

Subjects

Chromatography, Gel methods, Chromatography, Reverse-Phase methods, Proteins isolation & purification, Temperature, Chromatography, Gel instrumentation, Chromatography, Reverse-Phase instrumentation, Polysorbates chemistry, Proteins analysis, Proteins chemistry

Abstract

Size-exclusion chromatography (SEC) is a useful method for quantification of protein aggregates because of its high throughput capacity and highly quantitative performance. One of the problems in this method concerns polysorbates, which are well-known additives for protein-containing products to prevent protein aggregation, but frequently interfere with the photometric detection of protein aggregates. We developed a new SEC method that can separate polysorbates from protein sample solutions in an on-line mode with a precolumn with size exclusion and reversed-phase mixed modes. The precolumn can effectively trap polysorbates in aqueous mobile phase, and the trapped polysorbates are easily eluted with acetonitrile-containing aqueous mobile phase to clean the precolumn. Small parts of protein aggregates may be also trapped on the precolumn depending on temperature and proteins. Setting appropriate column temperature can minimize such inconvenient trapping of aggregates., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published

2014

30. Qualitative evaluation of high pH mass spectrometry-compatible reversed phase liquid chromatography for altered selectivity in separations of intact proteins.

Author

Baghdady YZ and Schug KA

Subjects

Hydrogen-Ion Concentration, Polymers chemistry, Silicon Dioxide chemistry, Chemistry Techniques, Analytical methods, Chromatography, Reverse-Phase standards, Mass Spectrometry, Proteins isolation & purification

Abstract

Intact proteins are increasingly being recognized as potential biomarkers and biotherapeutic agents for cancer and other serious diseases. Low pH reversed phase plays an important role in both single and multidimensional protein separations for resolving complex protein samples prior to mass spectrometric detection. In this work, we evaluated the use of high pH reversed phase liquid chromatography as an alternative chromatographic separation to gain different selectivity while maintaining the high resolving power and MS compatibility of reversed phase separations. The altered selectivity gained by high pH reversed phase liquid chromatography can further help to separate unresolved protein peaks or to increase peak capacity and resolving power of a multidimensional setup for complex biological samples. Hence, we evaluated the use of different MS-friendly buffers, ion pairing reagents, and stationary phases (silica- and polymer-based) at alkaline pH for intact protein separations. The best chromatographic separation, with complementary selectivity to low pH reversed phase, was achieved using triethylammonium bicarbonate at pH 10 and hybrid silica particles., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2019

31. Identification of the Secreted Proteins Originated from Primary Human Hepatocytes and HepG2 Cells.

Author

Franko A, Hartwig S, Kotzka J, Ruoß M, Nüssler AK, Königsrainer A, Häring HU, Lehr S, and Peter A

Subjects

Chromatography, Reverse-Phase, Hep G2 Cells, Humans, Primary Cell Culture, Proteomics methods, Secretory Pathway, Spectrometry, Mass, Electrospray Ionization, Tandem Mass Spectrometry, Hepatocytes metabolism, Proteins metabolism

Abstract

The liver plays a pivotal role in whole-body carbohydrate, lipid, and protein metabolism. One of the key regulators of glucose and lipid metabolism are hepatokines, which are found among the liver secreted proteins, defined as liver secretome. To elucidate the composition of the human liver secretome and identify hepatokines in primary human hepatocytes (PHH), we conducted comprehensive protein profiling on conditioned medium (CM) of PHH. Secretome profiling using liquid chromatography-electrospray ionization tandem mass spectrometry (LC-MS/MS) identified 691 potential hepatokines in PHH. Subsequently, pathway analysis assigned these proteins to acute phase response, coagulation, and complement system pathways. The secretome of PHH was compared to the secreted proteins of the liver hepatoma cell line HepG2. Although the secretome of PHH and HepG2 cells show a high overlap, the HepG2 secretome rather mirrors the fetal liver with some cancer characteristics. Collectively, our study represents one of the most comprehensive secretome profiling approaches for PHH, allowing new insights into the composition of the secretome derived from primary human material, and points out strength and weakness of using HepG2 cell secretome as a model for the analysis of the human liver secretome.

Published

2019

32. Computer-aided gradient optimization of hydrophilic interaction liquid chromatographic separations of intact proteins and protein glycoforms.

Author

van Schaick G, Pirok BWJ, Haselberg R, Somsen GW, and Gargano AFG

Subjects

Acetonitriles chemistry, Adsorption, Amides chemistry, Chromatography, Reverse-Phase, Hydrophobic and Hydrophilic Interactions, Software, Solvents chemistry, Tandem Mass Spectrometry, Chemistry Techniques, Analytical methods, Chromatography, Liquid, Glycoproteins isolation & purification, Proteins isolation & purification

Abstract

Protein glycosylation is one of the most common and critical post-translational modification, which results from covalent attachment of carbohydrates to protein backbones. Glycosylation affects the physicochemical properties of proteins and potentially their function. Therefore it is important to establish analytical methods which can resolve glycoforms of glycoproteins. Recently, hydrophilic-interaction liquid chromatography (HILIC)-mass spectrometry has demonstrated to be a useful tool for the efficient separation and characterization of intact protein glycoforms. In particular, amide-based stationary phases in combination with acetonitrile-water gradients containing ion-pairing agents, have been used for the characterization of glycoproteins. However, finding the optimum gradient conditions for glycoform resolution can be quite tedious as shallow gradients (small decrease of acetonitrile percentage in the elution solvent over a long time) are required. In the present study, the retention mechanism and peak capacity of HILIC for non-glycosylated and glycosylated proteins were investigated and compared to reversed-phase liquid chromatography (RPLC). For both LC modes, ln k vs. φ plots of a series of test proteins were calculated using linear solvent strength (LSS) analysis. For RPLC, the plots were spread over a wider φ range than for HILIC, suggesting that HILIC methods require shallower gradients to resolve intact proteins. Next, the usefulness of computer-aided method development for the optimization of the separation of intact glycoform by HILIC was examined. Five retention models including LSS, adsorption, and mixed-mode, were tested to describe and predict glycoprotein retention under gradient conditions. The adsorption model appeared most suited and was applied to the gradient prediction for the separation of the glycoforms of six glycoproteins (Ides-digested trastuzumab, alpha-acid glycoprotein, ovalbumin, fetuin and thyroglobulin) employing the program PIOTR. Based on the results of three scouting gradients, conditions for high-efficiency separations of protein glycoforms varying in the degree and complexity of glycosylation was achieved, thereby significantly reducing the time needed for method optimization., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2019

33. Assessing the Relationship Between Mass Window Width and Retention Time Scheduling on Protein Coverage for Data-Independent Acquisition.

Author

Li W, Chi H, Salovska B, Wu C, Sun L, Rosenberger G, and Liu Y

Subjects

Cell Line, Tumor, Chromatography, Reverse-Phase, Humans, Mass Spectrometry methods, Peptides analysis, Software, Proteins analysis, Proteomics methods

Abstract

Due to the technical advances of mass spectrometers, particularly increased scanning speed and higher MS/MS resolution, the use of data-independent acquisition mass spectrometry (DIA-MS) became more popular, which enables high reproducibility in both proteomic identification and quantification. The current DIA-MS methods normally cover a wide mass range, with the aim to target and identify as many peptides and proteins as possible and therefore frequently generate MS/MS spectra of high complexity. In this report, we assessed the performance and benefits of using small windows with, e.g., 5-m/z width across the peptide elution time. We further devised a new DIA method named RTwinDIA that schedules the small isolation windows in different retention time blocks, taking advantage of the fact that larger peptides are normally eluting later in reversed phase chromatography. We assessed the direct proteomic identification by using shotgun database searching tools such as MaxQuant and pFind, and also Spectronaut with an external comprehensive spectral library of human proteins. We conclude that algorithms like pFind have potential in directly analyzing DIA data acquired with small windows, and that the instrumental time and DIA cycle time, if prioritized to be spent on small windows rather than on covering a broad mass range by large windows, will improve the direct proteome coverage for new biological samples and increase the quantitative precision. These results further provide perspectives for the future convergence between DDA and DIA on faster MS analyzers.

Published

2019

34. Ancient amino acids from fossil feathers in amber.

Author

McCoy VE, Gabbott SE, Penkman K, Collins MJ, Presslee S, Holt J, Grossman H, Wang B, Solórzano Kraemer MM, Delclòs X, and Peñalver E

Subjects

Amino Acids chemistry, Amino Acids history, Animals, Birds anatomy & histology, Chromatography, Reverse-Phase, Dinosaurs anatomy & histology, Extinction, Biological, Feathers anatomy & histology, Fossils anatomy & histology, History, Ancient, Preservation, Biological, Proteins chemistry, Proteins history, Proteolysis, Amber chemistry, Amino Acids isolation & purification, Egg Shell chemistry, Feathers chemistry, Fossils history, Proteins isolation & purification

Abstract

Ancient protein analysis is a rapidly developing field of research. Proteins ranging in age from the Quaternary to Jurassic are being used to answer questions about phylogeny, evolution, and extinction. However, these analyses are sometimes contentious, and focus primarily on large vertebrates in sedimentary fossilisation environments; there are few studies of protein preservation in fossils in amber. Here we show exceptionally slow racemisation rates during thermal degradation experiments of resin enclosed feathers, relative to previous thermal degradation experiments of ostrich eggshell, coral skeleton, and limpet shell. We also recover amino acids from two specimens of fossil feathers in amber. The amino acid compositions are broadly similar to those of degraded feathers, but concentrations are very low, suggesting that much of the original protein has been degraded and lost. High levels of racemisation in more apolar, slowly racemising amino acids suggest that some of the amino acids were ancient and therefore original. Our findings indicate that the unique fossilisation environment inside amber shows potential for the recovery of ancient amino acids and proteins.

Published

2019

35. Phosphorylated proteomics analysis of human coronary artery endothelial cells stimulated by Kawasaki disease patients serum.

Author

Li SM, Liu WT, Yang F, Yi QJ, Zhang S, and Jia HL

Subjects

Case-Control Studies, Cells, Cultured, Child, Preschool, Chromatography, High Pressure Liquid, Chromatography, Reverse-Phase, Female, Humans, Infant, Male, Mucocutaneous Lymph Node Syndrome diagnosis, Phosphorylation, Protein Interaction Maps, Signal Transduction, Spectrometry, Mass, Electrospray Ionization, Tandem Mass Spectrometry, Coronary Vessels metabolism, Endothelial Cells metabolism, Mucocutaneous Lymph Node Syndrome blood, Proteins metabolism, Proteomics methods

Abstract

Background: Kawasaki disease (KD) is an acute febrile childhood systemic vasculitis that disturbs coronary arteries. The pathogenesis remains unknown. The study of phosphorylated proteins helps to elucidate the relevant pathophysiological mechanisms of cardiovascular disease. However, few researches explored phosphorylated proteins in KD patients., Methods: We compared phosphoprotein profiles of HCAECs stimulated by the serum of KD patients and normal children using iTRAQ technology, TiO 2 enrichment phosphorylated peptide and MS analysis. Then we conducted the functional analysis by ClueGO and the biological interaction networking analysis by ReactomeFIViz. Western blotting was performed to identify the hub proteins., Results: Our results revealed that phosphorylation of 148 proteins showed different intensities between the two HCAECs groups, which are enriched in MAPK, VEGFR, EGFR, Angiopoietin receptor, mTOR, FAK signaling pathway and so on. Through the Network Analyzer analysis, the hub proteins are CDKN1A, MAPK1 and POLR2A, which were experimentally validated., Conclusion: In summary, we provided evidence addressing the valuable phosphorylation signaling that could be useful resource to understand the molecular mechanism and the potential targets for novel therapy of KD.

Published

2019

36. Site-Specific Lysine Acetylation Stoichiometry Across Subcellular Compartments.

Author

Lindahl AJ, Lawton AJ, Baeza J, Dowell JA, and Denu JM

Subjects

Acetylation, Cell Culture Techniques, Cell Fractionation, Chromatography, Liquid, Chromatography, Reverse-Phase, Data Interpretation, Statistical, Hydrogen-Ion Concentration, Lysine chemistry, Mass Spectrometry methods, Mitochondria metabolism, Protein Processing, Post-Translational, Proteins chemistry, Proteomics methods, Tandem Mass Spectrometry, Lysine metabolism, Proteins metabolism

Abstract

Posttranslational modifications of proteins control many complex biological processes, including genome expression, chromatin dynamics, metabolism, and cell division through a language of chemical modifications. Improvements in mass spectrometry-based proteomics have demonstrated protein acetylation is a widespread and dynamic modification in the cell; however, many questions remain on the regulation and downstream effects, and an assessment of the overall acetylation stoichiometry is needed. In this chapter, we describe the determination of acetylation stoichiometry using data-independent acquisition mass spectrometry to expand the number of acetylation sites quantified. However, the increased depth of data-independent acquisition is limited by the spectral library used to deconvolute fragmentation spectra. We describe a powerful approach of subcellular fractionation in conjunction with offline prefractionation to increase the depth of the spectral library. This deep interrogation of subcellular compartments provides essential insights into the compartment-specific regulation and downstream functions of protein acetylation.

Published

2019

37. The Use of High Performance Liquid Chromatography for the Characterization of the Unfolding and Aggregation of Dairy Proteins.

Author

Gaspard SJ and Brodkorb A

Subjects

Chromatography, High Pressure Liquid methods, Chromatography, Reverse-Phase methods, Protein Aggregates physiology, Protein Folding, Proteins chemistry

Abstract

High-performance liquid chromatography (HPLC) is routinely used to identify and characterize proteins. HPLC can help to understand protein aggregation processes in dairy products, which are induced by common industrial processing steps such as heat treatment. In this chapter, three complementary chromatographic methods are described, which are based on the principles of size exclusion and reversed-phase chromatography. These methods are used to determine the degree of denaturation and aggregation of proteins, and estimate the molecular weight of these aggregates.

Published

2019

38. Detection and identification of antibacterial proteins in snake venoms using at-line nanofractionation coupled to LC-MS.

Author

Mladic M, Slagboom J, Kool J, Vonk FJ, van Wezel GP, and Richardson MK

Subjects

Animals, Anti-Bacterial Agents analysis, Chemical Fractionation methods, Peptides analysis, Peptides chemistry, Proteins analysis, Snakes, Anti-Bacterial Agents chemistry, Chromatography, Reverse-Phase methods, Mass Spectrometry methods, Nanotechnology methods, Proteins chemistry, Snake Venoms chemistry

Abstract

This study describes the application of at-line nanofractionation to the screening of snake venoms for antibacterial activity against Gram-positive and Gram-negative bacteria, the detection of proteins of interest, and their partial or full identification. A method was developed to identify bioactive peptides in crude snake venoms based on reversed-phase liquid chromatography (LC), with parallel nanofractionation onto 384-well plates and mass spectrometry (MS). Bioactivity assays were based on a resazurin-reduction assay. Accurate masses of the bioactive peptides were determined, and peptides were then identified via nanoLC-MS/MS analysis of tryptic digests, allowing full or partial identification of the bioactive proteins. Crude venoms from 41 species were screened for their antibacterial bioactivity. Venoms showing the highest activity were further screened using at-line nanofractionation, which resulted in the elucidation of 28 bioactive proteins., (Copyright © 2018. Published by Elsevier Ltd.)

Published

2018

39. Size-exclusion chromatography using reverse-phase columns for protein separation.

Author

Huang TY, Chi LM, and Chien KY

Subjects

Chromatography, High Pressure Liquid, Chromatography, Reverse-Phase, Limit of Detection, Mass Spectrometry, Proteins isolation & purification, Temperature, Chromatography, Gel methods, Proteins analysis

Abstract

Reverse-phase (RP) liquid chromatography (RPLC) and size-exclusion chromatography (SEC) are methods commonly used for protein/peptide separation, and they are based on distinct principles. This study develops a method using RP columns for size-based separation of protein mixtures. Results show that high concentrations of acetonitrile with trifluoroacetic acid as an acid modifier successfully suppressed interactions between proteins and the stationary phase and allowed the RP column to act as a SEC column to separate proteins based on their molecular weight. The reduction of protein disulfide bonds resulted in an improved correlation between the retention time and molecular weight in the RP-based SEC, which indicates that conformation-dependent SEC retention is less important for disulfide-reduced proteins using a current mobile phase. Importantly, the employed salt-free mobile phase allowed the RP-based SEC system to be directly coupled with online mass spectrometry (MS) analysis. Furthermore, by reducing the flow rate and increasing the column length, the separation efficiency was further improved and no adverse effects due to the prolonged separation were observed, which indicates the potential of this strategy to serve as a first-dimensional separation method for constructing an online multi-dimensional LC system. The size-based separation phenomenon with RP columns was further evaluated using a complex protein mixture (a cell lysate), and compared to conventional SEC, more proteins of the cell lysate were observed following the SEC separation principle, which implies the better generality of usage of the RP-based SEC method for protein separation. In summary, results show that the RP-based SEC is highly efficient in achieving protein fractionation. In addition, the employed salt-free mobile phase provides excellent compatibility of the RP-based SEC with other separation strategies or online mass spectrometric analysis. We anticipate that laboratories using RP-HPLC for protein separation will easily be able to move to the size-based separation mode using the same RP-HPLC system., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2018

40. Integrated device for online sample buffer exchange, protein enrichment, and digestion.

Author

Sun L, Ma J, Qiao X, Liang Y, Zhu G, Shan Y, Liang Z, Zhang L, and Zhang Y

Subjects

Amino Acid Sequence, Animals, Cattle, Chromatography, Reverse-Phase economics, Chromatography, Reverse-Phase instrumentation, Cytochromes c isolation & purification, Cytochromes c metabolism, Equipment Design, Horses, Molecular Sequence Data, Myoglobin isolation & purification, Myoglobin metabolism, Serum Albumin, Bovine isolation & purification, Serum Albumin, Bovine metabolism, Spectrometry, Mass, Electrospray Ionization economics, Spectrometry, Mass, Electrospray Ionization instrumentation, Trypsinogen metabolism, Chromatography, Reverse-Phase methods, Enzymes, Immobilized metabolism, Proteins isolation & purification, Proteins metabolism, Spectrometry, Mass, Electrospray Ionization methods

Abstract

An integrated sample treatment device, composed of a membrane interface and a monolithic hybrid silica based immobilized enzymatic reactor (IMER), was developed for the simultaneous sample buffer exchange, protein enrichment, and online digestion, by which for the sample buffer, the acetonitrile content was reduced to approximately 1/10 of the initial one, and the pH value was adjusted from approximately 3.0 to approximately 8.0, compatible for online trypsin digestion. Furthermore, the signal intensity of myoglobin digests was improved by over 10 times. Such an integrated device was successfully applied to the online treatment of three protein eluates obtained by reverse-phase liquid chromatography (RPLC) separation, followed by further protein digest analysis with microreverse-phase liquid chromatography-electrospray ionization-tandem mass spectrometry (microRPLC-ESI-MS/MS). The experimental results showed that the performance of such an integrated sample treatment device was comparable to that of the traditional offline sample treatment method, including lyophilization and in-solution digestion. However, the consumed time was reduced to 1/192. All these results demonstrate that such an integrated sample treatment device could be further online coupled with protein separation, peptide separation, and identification, to achieve high-throughput proteome analysis.

Published

2010

41. Evaluation of recent very efficient wide-pore stationary phases for the reversed-phase separation of proteins.

Author

Fekete S, Berky R, Fekete J, Veuthey JL, and Guillarme D

Subjects

Animals, Cattle, Chickens, Chromatography, High Pressure Liquid, Chromatography, Reverse-Phase methods, Horses, Humans, Particle Size, Porosity, Pressure, Proteins chemistry, Chromatography, Reverse-Phase instrumentation, Proteins isolation & purification

Abstract

In the present contribution, columns packed with fully porous widepore 1.7μm particles (Acquity BEH300) and widepore core-shell 3.6μm particles (Aeris WP) were evaluated for the separation of model and therapeutic proteins of varying sizes, hydrophobicity and isoelectric points. Two types of bonding were compared, namely C4 and C18 in a systematic way. The kinetic performance of these stationary phases was evaluated in a previous paper hence this new work focuses on their retention behaviour, loading capacity and selectivity. Using the Tanaka tests, model proteins, and other confirmatory experiments, it is highly probable that with proteins, strong interaction mechanisms were predominant on the Aeris WP while the hydrophobic interaction was the driving force of the retention on the Acquity BEH300 material. This explained why, despite the lower pore volume of the Aeris WP material, the apparent retention factors of proteins possessing both hydrophobic and charged amino acids residues were very close on the four investigated columns. In terms of peak widths, values for proteins were similar for all the tested stationary phases, despite the probable strong ion exchange mechanisms of Aeris WP column. This could be explained by the excellent mass transfer characteristics afforded by the thin porous layer (∼0.2μm) at the surface of the particle which probably compensates for the slow secondary ionic interaction kinetics. The loading capacity was also evaluated on all the four widepore columns, using model proteins. On average, approximately 2-4 times higher amount of proteins can be injected on the fully porous BEH300 compared to the core-shell Aeris WP columns when avoiding 10% change in peak width or in tailing. However, this result could be strongly influenced by the nature and shape of the protein, its hydrophobicity, folding, size and number of charges. Finally, all of these columns were employed for the highly efficient separation of a therapeutic protein (interferon-α-2A) and some closely related proteins and showed excellent performance and selectivity. This result confirms that RPLC gained interest in the biopharmaceutical field as it provides significantly better peak widths than size-exclusion or ion-exchange and inherent compatibility with MS., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published

2012

42. Evaluation of a new wide pore core-shell material (Aeris WIDEPORE) and comparison with other existing stationary phases for the analysis of intact proteins.

Author

Fekete S, Berky R, Fekete J, Veuthey JL, and Guillarme D

Subjects

Animals, Antibodies, Monoclonal analysis, Antibodies, Monoclonal isolation & purification, Chromatography, Reverse-Phase methods, Humans, Kinetics, Particle Size, Porosity, Proteins isolation & purification, Chromatography, Reverse-Phase instrumentation, Proteins analysis

Abstract

The separation of large biomolecules such as proteins or monoclonal antibodies (mAbs) by RPLC can be drastically enhanced thanks to the use of columns packed with wide-pore porous sub-2 μm particles or shell particles. In this context, a new wide-pore core-shell material has been recently released under the trademark Aeris WIDEPORE. It is made of a 3.2 μm solid inner core surrounded by a 0.2 μm porous layer (total particle size of 3.6 μm). The aim of this study was to evaluate the performance of this new material, compare it to other recently developed and older conventional wide-pore columns and demonstrate its applicability to real-life separations of proteins and mAbs. At first, the traditional h(min) values of the Aeris WIDEPORE column were determined for small model compounds. The h(min) values were equal to 1.7-1.8 and 1.4 for the 2.1 and 4.6 mm I.D. columns, respectively, which are in agreement with the values reported for other core-shell materials. In the case of a small protein Insulin (5.7 kDa), the achievable lowest h value was below 2 and this impressive result confirms that the Aeris WIDEPORE material should be dedicated to protein analysis. This column was then compared with five other commercially available wide-pore and medium-pore stationary phases, in the gradient elution mode, using various flow rates, gradient steepness and model proteins of MW=5.7-66.8 kDa. The Aeris WIDEPORE material often provided the best performance, in terms of peak capacity, peak capacity per time and pressure unit (PPT) and also based on the gradient kinetic plot representation. Finally, real separations of filgrastim (18.8 kDa) and its oxidized and reduced forms were performed on the different columns and the Aeris WIDEPORE material provided the most impressive performance (peak capacity>100 for t(grad)<6 min). Last but not least, this new material was also evaluated on digested and reduced mAb and powerful, high-throughput separations were also attained., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published

2012

43. Sensitive and reproducible intact mass analysis of complex protein mixtures with superficially porous capillary reversed-phase liquid chromatography mass spectrometry.

Author

Roth MJ, Plymire DA, Chang AN, Kim J, Maresh EM, Larson SE, and Patrie SM

Subjects

HeLa Cells, Histones analysis, Humans, Molecular Weight, Ubiquitin analysis, Chromatography, High Pressure Liquid, Chromatography, Reverse-Phase, Mass Spectrometry, Proteins analysis

Abstract

The compatibility of superficially porous (SP) resin for label-free intact protein analysis with online capillary LC/MS is demonstrated to give improved chromatographic resolution, sensitivity, and reproducibility. The robustness of the platform was measured against several samples of varying complexity and sample loading amount. The results indicate that capillary SP columns provide high loading capacities and that ∼6 s chromatographic peak widths are typical for standard proteins in simple mixtures and proteins isolated from cell and tissue lysates. Subfemtomole detection limits for standard proteins were consistently observed, with the lowest levels at 12 amol for ubiquitin. The analysis of total heart homogenates shows that capillary SP columns provide theoretical peak capacity of 106 protein forms with 30 min total analysis time and enabled detection of proteins from complex mixtures with a single high-resolution scan. The SPLC/MS platform also detected 343 protein forms from two HeLa acid extract replicate analyses that consumed 5 × 10(4) cells and 30 min analysis time, each. Comparison of all the species observed in each HeLa replicate showed 90% overlap (309 forms) with a Pearson correlation coefficient of 89.9% for the common forms observed in the replicates. Efficient acid extract of 1 × 10(4) HeLa cells allowed reproducible detection of common modification states and members from all five of the histone families and demonstrated that capillary SPLC/MS supports reproducible label-free profiling of histones in <15 min total analysis time. The data presented demonstrate that a capillary LC/MS platform utilizing superficially porous stationary phase and a LTQ-Orbitrap FT-MS is fast, sensitive, and reproducible for intact protein profiling from small tissue and cell amounts.

Published

2011

44. Preparation and characterization of lauryl methacrylate-based monolithic microbore column for reversed-phase liquid chromatography.

Author

Shu S, Kobayashi H, Kojima N, Sabarudin A, and Umemura T

Subjects

Adsorption, Chromatography, High Pressure Liquid methods, Chromatography, Reverse-Phase methods, Polymers chemistry, Porosity, Proteins chemistry, Chromatography, High Pressure Liquid instrumentation, Chromatography, Reverse-Phase instrumentation, Methacrylates chemistry, Proteins isolation & purification

Abstract

Poly(lauryl methacrylate-co-ethylene dimethacrylate) monoliths were in situ synthesized within the confines of a silicosteel tubing of 1.02 mm i.d. and 1/16" o.d. for microbore reversed-phase HPLC. In order to obtain practically useful monoliths with adequate column efficiency, low flow resistance, and good mechanical strength, some parameters such as total monomer concentration (%T), cross-linking degree (%C) and polymerization temperature were optimized. High-efficiency monoliths were successfully obtained by thermal polymerization of a monomer mixture (40%T, 10%C) with a binary porogenic solvent consisting of 1-propanol and 1,4-butandiol (7:4, v/v) at a high temperature of 90 °C. The morphology and porous structure of the resulting monoliths were assessed by scanning electron microscope (SEM) and inverse size exclusion chromatography (ISEC), while the column performance was evaluated through the separations of a series of alkylbenzenes in acetonitrile-water (50:50, v/v) eluent. At a normal flow rate of 50 μL/min (corresponding to 1.66 mm/s), the optimized monolithic columns typically exhibited theoretical plate numbers of 6000 plates/10 cm-long column for amylbenzene (k>40), and the pressure drop was always less than 1 MPa/10 cm. The monoliths, which were chemically anchored to the tube inner wall surface using a bifunctional silylation agent, exhibited adequate mechanical strength of up to 12-13 MPa, and were properly operated at 10 times higher flow rate than normal, reducing the separation time to one tenth. The lauryl methacrylate-based monolithic column was applied to a rapid and efficient separation of ten common proteins such as aprotinin, ribonuclease A, insulin, cytochrome c, trypsin, transferrin, conalbumin, myoglobin, β-amylase, and ovalbumin in the precipitation-redissolution mode. Using a linear CH(3)CN gradient elution at a flow rate of 500 μL/min (10-times higher flow rate), 10 proteins were baseline separated within 2 min., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published

2011

45. Reversed-phase liquid chromatographic resolution of diastereomers of protein and non-protein amino acids prepared with newly synthesized chiral derivatizing reagents based on cyanuric chloride.

Author

Bhushan R and Agarwal C

Subjects

Amino Acids chemical synthesis, Amino Acids isolation & purification, Chromatography, High Pressure Liquid instrumentation, Chromatography, Reverse-Phase instrumentation, Proteins chemical synthesis, Proteins isolation & purification, Stereoisomerism, Amino Acids chemistry, Chromatography, High Pressure Liquid methods, Chromatography, Reverse-Phase methods, Proteins chemistry, Triazines chemistry

Abstract

Two new chiral monochloro-s-triazines (MCT) were synthesized [viz N-(4-chloro-6-piperidinyl-[1,3,5]-triazine-2-yl)-L-leucine amide and N-(4-chloro-6-piperidinyl-[1,3,5]-triazine-2-yl)-L-leucine) (CDR 1 and 2, respectively)] by the nucleophilic displacement of chlorine atoms in s-triazine moiety. One of the Cl atoms was replaced with piperidine, and the second Cl atom in the 6-piperidinyl derivative was replaced with amino acid amide (viz L-Leu-NH(2)) and amino acid (L-Leu). These reagents were characterized and used as CDRs for chiral separation of protein and non-protein amino acids, and were separated on a reversed-phase C(18) column. The reaction conditions were optimized for the synthesis of diastereomers using one MCT reagent. The separation method was validated for limit of detection, linearity, accuracy, precision, and recovery.

Published

2011

46. High-resolution reversed-phase chromatography of proteins.

Author

Pettersson SW

Subjects

Algorithms, Buffers, Chromatography, High Pressure Liquid instrumentation, Chromatography, Reverse-Phase instrumentation, Hydrogen Bonding, Hydrogen-Ion Concentration, Hydrophobic and Hydrophilic Interactions, Ions, Metals chemistry, Models, Chemical, Peptides chemistry, Proteins chemistry, Reproducibility of Results, Silanes chemistry, Solvents chemistry, Chromatography, High Pressure Liquid methods, Chromatography, Reverse-Phase methods, Peptides isolation & purification, Proteins isolation & purification

Published

2011

47. Online coupling of reverse-phase and hydrophilic interaction liquid chromatography for protein and glycoprotein characterization.

Author

Lam MP, Siu SO, Lau E, Mao X, Sun HZ, Chiu PC, Yeung WS, Cox DM, and Chu IK

Subjects

Amino Acid Sequence, Animals, Cattle, Cell Line, Chromatography, Liquid instrumentation, Chromatography, Liquid methods, Chromatography, Reverse-Phase methods, Equipment Design, Glycoproteins isolation & purification, Humans, Mass Spectrometry methods, Mice, Molecular Sequence Data, Polysaccharides analysis, Polysaccharides isolation & purification, Proteins isolation & purification, Proteomics methods, Serum chemistry, Chromatography, Reverse-Phase instrumentation, Glycoproteins analysis, Proteins analysis, Proteomics instrumentation

Abstract

We have developed a novel system for coupling reverse-phase (RP) and hydrophilic interaction liquid chromatography (HILIC) online in a micro-flow scheme. In this approach, the inherent solvent incompatibility between RP and HILIC is overcome through the use of constant-pressure online solvent mixing, which allows our system to perform efficient separations of both hydrophilic and hydrophobic compounds for mass spectrometry-based proteomics applications. When analyzing the tryptic digests of bovine serum albumin, ribonuclease B, and horseradish peroxidase, we observed near-identical coverage of peptides and glycopeptides when using online RP-HILIC--with only a single sample injection event--as we did from two separate RP and HILIC analyses. The coupled system was also capable of concurrently characterizing the peptide and glycan portions of deglycosylated glycoproteins from one injection event, as confirmed, for example, through our detection of 23 novel glycans from turkey ovalbumin. Finally, we validated the applicability of using RP-HILIC for the analysis of highly complex biological samples (mouse chondrocyte lysate, deglycosylated human serum). The enhanced coverage and efficiency of online RP-HILIC makes it a viable technique for the comprehensive separation of components displaying dramatically different hydrophobicities, such as peptides, glycopeptides, and glycans.

Published

2010

48. Direct analysis of reversed-phase high-performance thin layer chromatography separated tryptic protein digests using a liquid microjunction surface sampling probe/electrospray ionization mass spectrometry system.

Author

Emory JF, Walworth MJ, Van Berkel GJ, Schulz M, and Minarik S

Subjects

Amino Acid Sequence, Animals, Caseins analysis, Caseins isolation & purification, Cattle, Chickens, Chromatography, High Pressure Liquid instrumentation, Chromatography, Reverse-Phase instrumentation, Chromatography, Thin Layer instrumentation, Cytochromes c analysis, Cytochromes c isolation & purification, Equipment Design, Horses, Molecular Sequence Data, Muramidase analysis, Muramidase isolation & purification, Myoglobin analysis, Myoglobin isolation & purification, Proteins isolation & purification, Serum Albumin, Bovine analysis, Serum Albumin, Bovine isolation & purification, Spectrometry, Mass, Electrospray Ionization instrumentation, Chromatography, High Pressure Liquid methods, Chromatography, Reverse-Phase methods, Chromatography, Thin Layer methods, Proteins analysis, Spectrometry, Mass, Electrospray Ionization methods

Abstract

The sampling, ionization and detection of tryptic peptides separated in one-dimension on reversed-phase high-performance thin layer chromatography (HPTLC) plates was performed using liquid microjunction surface sampling probe electrospray ionization mass spectrometry. Tryptic digests of five proteins [cytochrome c, myoglobin, beta-casein, lysozyme and bovine serum albumin (BSA)] were spotted on reversed phase HPTLC RP-8 F254s and HPTLC RP-18 F254s plates. The plates were then developed using 70/30 methanol/water with 0.1M ammonium acetate. A dual purpose extraction/electrospray solution containing 70/30/0.1 water/methanol/formic acid was infused through the sampling probe during analysis of the developed lanes. Both full scan mass spectra and data dependent tandem mass spectra were acquired for each development lane to detect and verify the peptide distributions. Data dependent tandem mass spectra provided both protein identification and sequence coverage information. Highest sequence coverages were achieved for cytochrome c and myoglobin (62.5% and 58.3%, respectively) on reversed phase RP-8 plates. While the tryptic peptides were separated enough for identification, the peptide bands did show some overlap with most peptides located in the lower half of the development lane. Proteins whose peptides were more separated gave higher sequence coverage. Larger proteins such as beta-casein and BSA which were spotted in lower relative amounts gave much lower sequence coverage than the smaller proteins.

Published

2010

49. Online integration of multiple sample pretreatment steps involving denaturation, reduction, and digestion with microflow reversed-phase liquid chromatography-electrospray ionization tandem mass spectrometry for high-throughput proteome profiling.

Author

Ma J, Liu J, Sun L, Gao L, Liang Z, Zhang L, and Zhang Y

Subjects

Animals, Cattle, Liver metabolism, Mice, Myoglobin analysis, Myoglobin isolation & purification, Myoglobin metabolism, Online Systems, Protein Denaturation, Proteins isolation & purification, Serum Albumin, Bovine analysis, Serum Albumin, Bovine isolation & purification, Serum Albumin, Bovine metabolism, Urea, Chromatography, Reverse-Phase, Proteins analysis, Proteins metabolism, Proteome analysis, Spectrometry, Mass, Electrospray Ionization, Tandem Mass Spectrometry

Abstract

A facile integrated platform for proteome profiling was established, in which native proteins were online denatured and reduced within a heater, digested with an immobilized trypsin microreactor, and analyzed by microflow reversed-phase liquid chromatography with electrospray ionization tandem mass spectrometry (microRPLC-ESI-MS/MS). In comparison to the traditional off-line urea denaturation protocol, even more unique peptides were obtained by online heating in triplicate (14 +/- 2 vs 11 +/- 2 for myoglobin and 16 vs 12 +/- 1 for BSA) within a significantly shortened pretreatment time of approximately 3.5 min (including 1 min of thermal denaturation and reduction and approximately 2.5 min of microreactor digestion). Moreover, proteins with concentrations ranging from 50 ng/mL (approximately 6 fmol) to 1 mg/mL (approximately 120 pmol) were positively identified by the online system. Such a platform was further successfully applied for analyzing the soluble fraction of mouse liver extract. Of all the 367 proteins identified from samples pretreated by the urea protocol and online heating, approximately 40% were overlapped, showing the partial complementation of both approaches. All these results demonstrate that the online integrated platform is of great promise for high-throughput proteome profiling and improved identification capacity for low-abundance proteins with a minute sample amount.

Published

2009

50. FractionOptimizer: a method for optimal peptide fractionation in bottom-up proteomics.

Author

Solovyeva EM, Lobas AA, Kopylov AT, Ilina IY, Levitsky LI, Moshkovskii SA, and Gorshkov MV

Subjects

Chromatography, High Pressure Liquid methods, HEK293 Cells, Humans, Proteome chemistry, Software, Tandem Mass Spectrometry methods, Chromatography, Reverse-Phase methods, Peptides analysis, Proteins chemistry, Proteomics methods

Abstract

Recent advances in mass spectrometry and separation technologies created the opportunities for deep proteome characterization using shotgun proteomics approaches. The "real world" sample complexity and high concentration range limit the sensitivity of this characterization. The common strategy for increasing the sensitivity is sample fractionation prior to analysis either at the protein or the peptide level. Typically, fractionation at the peptide level is performed using linear gradient high-performance liquid chromatography followed by uniform fraction collection. However, this way of peptide fractionation results in significantly suboptimal operation of the mass spectrometer due to the non-uniform distribution of peptides between the fractions. In this work, we propose an approach based on peptide retention time prediction allowing optimization of chromatographic conditions and fraction collection procedures. An open-source software implementing the approach called FractionOptimizer was developed and is available at http://hg.theorchromo.ru/FractionOptimizer . The performance of the developed tool was demonstrated for human embryonic kidney (HEK293) cell line lysate. In these experiments, we improved the uniformity of the peptides distribution between fractions. Moreover, in addition to 13,492 peptides, we found 6787 new peptides not identified in the experiments without fractionation and up to 800 new proteins (or 25%). Graphical abstract The analysis workflow employing FractionOptimizer software.

Published

2018