Your search keyword '"Ishihama, Yasushi"' showing total 14 results

1. Hybrid-DIA: intelligent data acquisition integrates targeted and discovery proteomics to analyze phospho-signaling in single spheroids.

Author

Martínez-Val A, Fort K, Koenig C, Van der Hoeven L, Franciosa G, Moehring T, Ishihama Y, Chen YJ, Makarov A, Xuan Y, and Olsen JV

Subjects

Humans, HeLa Cells, Tandem Mass Spectrometry methods, Signal Transduction, Proteome metabolism, Proteomics methods, Phosphopeptides metabolism

Abstract

Achieving sufficient coverage of regulatory phosphorylation sites by mass spectrometry (MS)-based phosphoproteomics for signaling pathway reconstitution is challenging, especially when analyzing tiny sample amounts. To address this, we present a hybrid data-independent acquisition (DIA) strategy (hybrid-DIA) that combines targeted and discovery proteomics through an Application Programming Interface (API) to dynamically intercalate DIA scans with accurate triggering of multiplexed tandem mass spectrometry (MSx) scans of predefined (phospho)peptide targets. By spiking-in heavy stable isotope labeled phosphopeptide standards covering seven major signaling pathways, we benchmark hybrid-DIA against state-of-the-art targeted MS methods (i.e., SureQuant) using EGF-stimulated HeLa cells and find the quantitative accuracy and sensitivity to be comparable while hybrid-DIA also profiles the global phosphoproteome. To demonstrate the robustness, sensitivity, and biomedical potential of hybrid-DIA, we profile chemotherapeutic agents in single colon carcinoma multicellular spheroids and evaluate the phospho-signaling difference of cancer cells in 2D vs 3D culture., (© 2023. The Author(s).)

Published

2023

2. Bioinertization of NanoLC/MS/MS Systems by Depleting Metal Ions From the Mobile Phases for Phosphoproteomics.

Author

Komori Y, Niinae T, Imami K, Yanagibayashi J, Yasunaga K, Imamura S, Tomita M, and Ishihama Y

Subjects

Chromatography, Liquid methods, Chromatography, Affinity methods, Ions, Tandem Mass Spectrometry methods, Phosphopeptides chemistry

Abstract

We have successfully developed a bioinertized nanoflow LC/MS/MS (nanoLC/MS/MS) system for the highly sensitive analysis of phosphopeptides by depleting metal ions from the mobile phase. We found that not only direct contact of phosphopeptides with metal components, but also indirect contact with nanoLC pumps through the mobile phase causes significant losses during the recovery of phosphopeptides. Moreover, electrospray ionization was adversely affected by the mobile phase containing multiple metal ions as well as by the sample solvents contaminated with metal ions used in immobilized metal ion affinity chromatography for phosphopeptide enrichment. To solve these problems, metal ions were depleted by inserting an online metal ion removal device containing metal-chelating membranes between the gradient mixer and the autosampler. As a result, the peak areas of the identified phosphopeptides increased an average of 9.9-fold overall and 77-fold for multiply phosphorylated peptides with the insertion of the online metal ion removal system. This strategy would be applicable to the highly sensitive analysis of other phosphorylated biomolecules by microscale-LC/MS/MS., Competing Interests: Conflict of interest The authors declare no competing interests., (Copyright © 2023 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2023

3. Motif-centric phosphoproteomics to target kinase-mediated signaling pathways.

Author

Tsai CF, Ogata K, Sugiyama N, and Ishihama Y

Subjects

Phosphorylation, Mass Spectrometry, Phosphopeptides, Signal Transduction

Abstract

Identifying cellular phosphorylation pathways based on kinase-substrate relationships is a critical step to understanding the regulation of physiological functions in cells. Mass spectrometry-based phosphoproteomics workflows have made it possible to comprehensively collect information on individual phosphorylation sites in a variety of samples. However, there is still no generic approach to uncover phosphorylation networks based on kinase-substrate relationships in rare cell populations. Here, we describe a motif-centric phosphoproteomics approach combined with multiplexed isobaric labeling, in which in vitro kinase reactions are used to generate targeted phosphopeptides, which are spiked into one of the isobaric channels to increase detectability. Proof-of-concept experiments demonstrate selective and comprehensive quantification of targeted phosphopeptides by using multiple kinases for motif-centric channels. More than 7,000 tyrosine phosphorylation sites were quantified from several tens of micrograms of starting materials. This approach enables the quantification of multiple phosphorylation pathways under physiological or pathological regulation in a motif-centric manner., Competing Interests: The authors declare no competing interests., (© 2021 The Author(s).)

Published

2022

4. Mass Spectrometry-Compatible Subcellular Fractionation for Proteomics.

Author

Masuda T, Sugiyama N, Tomita M, Ohtsuki S, and Ishihama Y

Subjects

Chemical Fractionation, Mass Spectrometry, Proteins, Subcellular Fractions, Phosphopeptides, Proteomics

Abstract

We found that nuclear envelopes stabilize against surfactants in the presence of ethylene glycol (EG). We, therefore, developed a novel subcellular fractionation approach for proteomics using RIPA buffer containing EG and phase transfer surfactants. This method involves separating the cells into the cytoplasm, organelles, and nucleus, including intermediate filaments without ultracentrifugation. These fractions are directly applicable to sample preparation for shotgun proteomics as they have no mass spectrometry (MS)-incompatible chemicals, whereas those separated by traditional fractionation protocols require desalting. This protocol is successfully applied to subcellular fractionation with only 3.5 × 10 5 cells. Here, it was combined with phosphoproteomics and proteomics to identify phosphorylation sites regulating protein subcellular localization. In total, 59 phosphorylation sites on 42 phosphopeptides and 32 proteins showing different enrichment patterns between phosphoproteomics and the corresponding proteomics were identified, which are potential candidate sites to regulate the protein subcellular localization, including serine 706 on CD44 and serine 22 on lamin A/C.

Published

2020

5. Retention Order Reversal of Phosphorylated and Unphosphorylated Peptides in Reversed-Phase LC/MS.

Author

Ogata K, Krokhin OV, and Ishihama Y

Subjects

Phosphorylation, Chromatography, Reverse-Phase, Phosphopeptides chemistry, Tandem Mass Spectrometry

Abstract

Protein phosphorylation is one of the most ubiquitous post-translational modifications in humans, and trypsin-digested phosphorylated peptides have been analyzed by reversed phase LC/MS using C18-silica columns under acidic conditions to profile human phosphoproteomes. Here, we report that phosphopeptides generally exhibit stronger retention than their unphosphorylated counterparts when C18-silica columns are used with acetic acid or formic acid as an ion-pairing reagent, whereas the retention order is reversed when less hydrophobic stationary phases such as C4-silica columns are employed. Similarly the retention reversal is observed when more hydrophobic ion-pairing reagents such as trifluoroacetic acid are used with C18-silica columns. These phenomena could be explained by the smaller S-values of phosphopeptides in linear solvation strength theory, based on the reduced net charge caused by intramolecular interaction between phosphate and basic groups.

Published

2018

6. Identifications of Putative PKA Substrates with Quantitative Phosphoproteomics and Primary-Sequence-Based Scoring.

Author

Imamura H, Wagih O, Niinae T, Sugiyama N, Beltrao P, and Ishihama Y

Subjects

Amino Acid Sequence genetics, Cyclic AMP-Dependent Protein Kinases chemistry, Cyclic AMP-Dependent Protein Kinases genetics, Humans, Phosphopeptides chemistry, Phosphopeptides genetics, Phosphorylation, Protein Serine-Threonine Kinases chemistry, Protein Serine-Threonine Kinases genetics, Signal Transduction genetics, Substrate Specificity, Cyclic AMP-Dependent Protein Kinases metabolism, High-Throughput Screening Assays, Phosphopeptides isolation & purification, Tandem Mass Spectrometry

Abstract

Protein kinase A (PKA or cAMP-dependent protein kinase) is a serine/threonine kinase that plays essential roles in the regulation of proliferation, differentiation, and apoptosis. To better understand the functions of PKA, it is necessary to elucidate the direct interplay between PKA and their substrates in living human cells. To identify kinase target substrates in a high-throughput manner, we first quantified the change of phosphoproteome in the cells of which PKA activity was perturbed by drug stimulations. LC-MS/MS analyses identified 2755 and 3191 phosphopeptides from experiments with activator or inhibitor of PKA. To exclude potential indirect targets of PKA, we built a computational model to characterize the kinase sequence specificity toward the substrate target site based on known kinase-substrate relationships. Finally, by combining the sequence recognition model with the quantitative changes in phosphorylation measured in the two drug perturbation experiments, we identified 29 reliable candidates of PKA targeting residues in living cells including 8 previously known substrates. Moreover, 18 of these sites were confirmed to be site-specifically phosphorylated in vitro. Altogether this study proposed a confident list of PKA substrate candidates, expanding our knowledge of PKA signaling network.

Published

2017

7. Phosphoproteomics Identifies CK2 as a Negative Regulator of Beige Adipocyte Thermogenesis and Energy Expenditure.

Author

Shinoda K, Ohyama K, Hasegawa Y, Chang HY, Ogura M, Sato A, Hong H, Hosono T, Sharp LZ, Scheel DW, Graham M, Ishihama Y, and Kajimura S

Subjects

Adipose Tissue, Brown drug effects, Adipose Tissue, White drug effects, Adipose Tissue, White metabolism, Animals, Casein Kinase II antagonists & inhibitors, Casein Kinase II genetics, Cyclic AMP metabolism, Histone Deacetylases chemistry, Histone Deacetylases metabolism, Ion Channels genetics, Ion Channels metabolism, Male, Mice, Mice, Inbred C57BL, Mitochondrial Proteins genetics, Mitochondrial Proteins metabolism, Naphthyridines pharmacology, Norepinephrine pharmacology, Obesity etiology, Oxides pharmacology, Phenazines, Receptors, Adrenergic, beta-3 metabolism, Signal Transduction, Thermogenesis drug effects, Uncoupling Protein 1, Vanadium Compounds pharmacology, Adipose Tissue, Brown metabolism, Casein Kinase II metabolism, Energy Metabolism drug effects, Phosphopeptides analysis, Proteomics

Abstract

Catecholamines promote lipolysis both in brown and white adipocytes, whereas the same stimuli preferentially activate thermogenesis in brown adipocytes. Molecular mechanisms for the adipose-selective activation of thermogenesis remain poorly understood. Here, we employed quantitative phosphoproteomics to map global and temporal phosphorylation profiles in brown, beige, and white adipocytes under β3-adrenenoceptor activation and identified kinases responsible for the adipose-selective phosphorylation profiles. We found that casein kinase2 (CK2) activity is preferentially higher in white adipocytes than brown/beige adipocytes. Genetic or pharmacological blockade of CK2 in white adipocytes activates the thermogenic program in response to cAMP stimuli. Such activation is largely through reduced CK2-mediated phosphorylation of class I HDACs. Notably, inhibition of CK2 promotes beige adipocyte biogenesis and leads to an increase in whole-body energy expenditure and ameliorates diet-induced obesity and insulin resistance. These results indicate that CK2 is a plausible target to rewire the β3-adrenenoceptor signaling cascade that promotes thermogenesis in adipocytes., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2015

8. Microscale phosphoproteome analysis of 10,000 cells from human cancer cell lines.

Author

Masuda T, Sugiyama N, Tomita M, and Ishihama Y

Subjects

Cell Line, Tumor, Chromatography, Affinity, Chromatography, High Pressure Liquid, Humans, Mass Spectrometry, Miniaturization, Neoplasms, Phosphopeptides isolation & purification, Phosphorylation, Phosphopeptides analysis, Proteomics

Abstract

We developed a miniaturized LC-MS system with a high-recovery phosphopeptide enrichment protocol that allows phosphoproteome analysis of 10(4) cells. In the enrichment protocol, the key step is to add sodium deoxycholate and sodium lauroyl sarcosinate to the buffer solution for protein extraction and digestion and to omit any subsequent desalt/desurfactant step before phosphopeptide enrichment. The phosphopeptides enriched by hydroxy acid-modified metal oxide chromatography (HAMMOC) are directly injected onto a miniaturized LC column using a nitrogen-pressure-driven cell, instead of switching valve-type injectors. The miniaturized analytical column of 25 μm diameter provided a 3.6-fold improvement in sensitivity over the conventional 100 μm diameter column. Overall, our analytical system provided approximately 80-fold improvement on average in the LC-MS response, and we identified 1011 unique phosphorylated sites based on 995 unique phosphopeptides from a single analysis of 10(4) HeLa cells (approximately 1 μg of proteins). This is the most sensitive phosphoproteomics system that has so far been reported for proteome-wide analysis of in vivo phosphorylation in mammalian cells., (© 2011 American Chemical Society)

Published

2011

9. Chemical dephosphorylation for identification of multiply phosphorylated peptides and phosphorylation site determination.

Author

Kyono Y, Sugiyama N, Tomita M, and Ishihama Y

Subjects

Arabidopsis chemistry, Arabidopsis Proteins chemistry, Arabidopsis Proteins isolation & purification, Chromatography, Liquid, Mass Spectrometry, Molecular Structure, Phosphopeptides isolation & purification, Phosphoproteins chemistry, Phosphorylation, Phosphopeptides chemistry

Abstract

We have developed a novel strategy to improve the efficiency of identification of multiply phosphorylated peptides isolated by hydroxy acid modified metal oxide chromatography (HAMMOC). This strategy consists of alkali-induced chemical dephosphorylation (beta-elimination reaction) of phosphopeptides isolated by HAMMOC prior to analysis by liquid chromatography/mass spectrometry (LC/MS). This approach identified 1.9-fold more multiply phosphorylated peptides than the conventional approach without beta-elimination from a digested mixture of three standard phosphoproteins. In addition, the accuracy of phosphorylation site determination in synthetic phosphopeptides was significantly improved. Finally, we applied this approach to a cell lysate. By combining this dephosphorylation approach with the conventional approach, we successfully identified 1649 unique phosphopeptides, including 325 multiply phosphorylated phosphopeptides, from 200 microg of cultured Arabidopsis cells. These results indicate that chemical dephosphorylation prior to LC/MS analysis increases the efficiency of identification of multiply phosphorylated peptides, as well as the accuracy of phosphorylation site determination., (Copyright (c) 2010 John Wiley & Sons, Ltd.)

Published

2010

10. Ser/Thr/Tyr phosphoproteome analysis of pathogenic and non-pathogenic Pseudomonas species.

Author

Ravichandran A, Sugiyama N, Tomita M, Swarup S, and Ishihama Y

Subjects

Bacterial Proteins metabolism, Chromatography, Liquid, Cyclic GMP analogs & derivatives, Cyclic GMP metabolism, Mass Spectrometry, Phosphoamino Acids metabolism, Phosphopeptides metabolism, Phosphorylation, Protein Kinases metabolism, Proteome metabolism, Pseudomonas aeruginosa metabolism, Pseudomonas putida metabolism, Serine metabolism, Signal Transduction, Threonine metabolism, Tyrosine metabolism, Amino Acids metabolism, Bacterial Proteins analysis, Phosphopeptides analysis, Proteome analysis, Pseudomonas aeruginosa chemistry, Pseudomonas putida chemistry

Abstract

Protein phosphorylation on serine, threonine, and tyrosine is well established as a crucial regulatory posttranslational modification in eukaryotes. With the recent whole-genome sequencing projects reporting the presence of serine/threonine kinases and two-component proteins both in prokaryotes and eukaryotes, the importance of protein phosphorylation in archaea and bacteria is gaining acceptance. While conventional biochemical methods failed to obtain a snapshot of the bacterial phosphoproteomes, advances in MS methods have paved the way for in-depth mapping of phosphorylation sites. Here, we present phosphoproteomes of two ecologically diverse non-enteric Gram-negative bacteria captured by a nanoLC-MS-based approach combined with a novel phosphoenrichment method. While the phosphoproteome data from the two species are not very similar, the results reflect high similarity to the previously published dataset in terms of the pathways the phosphoproteins belong to. This study additionally provides evidence to prior observations that protein phosphorylation is common in bacteria. Notably, phosphoproteins identified in Pseudomonas aeruginosa belong to motility, transport, and pathogenicity pathways that are critical for survival and virulence. We report, for the first time, that motility regulator A, probably acting via the novel secondary messenger cyclic diguanylate monophosphate, significantly affects protein phosphorylation in Pseudomonas putida.

Published

2009

11. Successive and selective release of phosphorylated peptides captured by hydroxy acid-modified metal oxide chromatography.

Author

Kyono Y, Sugiyama N, Imami K, Tomita M, and Ishihama Y

Subjects

Amino Acid Sequence, Biocompatible Materials chemistry, Dental Materials chemistry, HeLa Cells, Humans, Molecular Sequence Data, Proteome analysis, Chromatography, Affinity methods, Hydroxy Acids chemistry, Phosphopeptides chemistry, Titanium chemistry, Zirconium chemistry

Abstract

We developed a novel approach to enlarge phosphoproteome coverage using successive elution of phosphopeptides with various buffers in series from a single microcolumn packed with hydroxy acid-modified metal oxides, such as titania and zirconia. Elution conditions were investigated to maximize the recovery of phosphopeptides from three standard phosphoproteins. Secondary amines, such as piperidine and pyrrolidine, provided better efficiency than the conventional conditions using ammonium hydroxide and phosphate buffers. Furthermore, elution with these secondary amines provided unique phosphopeptides that were not eluted under the conventional conditions in the analysis of HeLa cell lysates. On the basis of these results, we fractionated phosphopeptides captured by a single metal oxide microcolumn using successive elution with 5% ammonium hydroxide solution, 5% piperidine solution and 5% pyrrolidine solution in series. We identified 1,803 nonredundant phosphopeptides from 100 microg of HeLa cells, which represented a 1.6-fold increase in phosphopeptide number and a 1.9-fold increase in total peak area of phosphopeptides in comparison with the results obtained under the conventional conditions. Since this approach is applicable to any single tip-based protocol without coupling with other enrichment methods, this simple strategy can be easily incorporated as an option into existing protocols for phosphopeptide enrichment, and would be suitable for high-throughput analysis in a parallel format.

Published

2008

12. Phosphopeptide enrichment by aliphatic hydroxy acid-modified metal oxide chromatography for nano-LC-MS/MS in proteomics applications.

Author

Sugiyama N, Masuda T, Shinoda K, Nakamura A, Tomita M, and Ishihama Y

Subjects

Amino Acid Sequence, Cell Extracts chemistry, Chromatography, Liquid, Cytoplasm chemistry, Cytoplasm drug effects, HeLa Cells, Humans, Hydroxy Acids pharmacology, Mass Spectrometry, Molecular Sequence Data, Phosphopeptides analysis, Phosphopeptides chemistry, Reproducibility of Results, Hydroxy Acids chemistry, Nanotechnology, Phosphopeptides isolation & purification, Proteomics instrumentation, Proteomics methods

Abstract

We developed novel methods for phosphopeptide enrichment using aliphatic hydroxy acid-modified metal oxide chromatography (MOC). Titania and zirconia were successfully applied to enrich phosphopeptides with the aid of aliphatic hydroxy acids, such as lactic acid and beta-hydroxypropanoic acid, to reduce the interaction between acidic non-phosphopeptides and the metal oxides. These methods removed the vast majority of non-phosphopeptides from phosphoprotein standard digests, and large numbers of phosphopeptides could be readily identified. The methods were coupled with nano-LC-MS/MS systems without difficulty. Recovery of phosphopeptides in MOC varied greatly from peptide to peptide, ranging from a few percent to 100%, and the average was almost 50%. Repeatability and linearity were satisfactory. In an examination of the cytoplasmic fraction of HeLa cells, more than 1000 phosphopeptides were identified using lactic acid-modified titania MOC and beta-hydroxypropanoic acid-modified zirconia MOC, respectively. The overlap between phosphopeptides enriched by these two methods was 40%, and the combined results provided 1646 unique phosphopeptides. To our knowledge, this is the first successful application of a single MOC-based approach to phosphopeptide enrichment from complex biological samples such as cell lysates.

Published

2007

13. Enhancement of the efficiency of phosphoproteomic identification by removing phosphates after phosphopeptide enrichment.

Author

Ishihama Y, Wei FY, Aoshima K, Sato T, Kuromitsu J, and Oda Y

Subjects

Alkaline Phosphatase metabolism, Animals, Cell Line, Tumor, Cells, Cultured, Mice, Neuroblastoma chemistry, Neuroblastoma pathology, Phosphates metabolism, Phosphorylation, Prosencephalon chemistry, Prosencephalon cytology, Proteomics standards, Serine, Trypsin, Tyrosine, Phosphopeptides analysis, Phosphoproteins analysis, Proteomics methods

Abstract

Immobilized metal affinity chromatography (IMAC) and titanium oxide (TiO2) chromatography are simple, widely used, and cost-effective methods to enrich phosphopeptides, but the sample loading buffer composition, desalting procedure, and control of loading amount are critical to avoid nonspecific interactions and to achieve efficient phosphopeptide enrichment. Although the combination of MS3 analysis and high-resolution mass spectrometry (MS) is helpful to identify phosphopeptides, the quality of many MS/MS spectra having a neutral loss peak of phosphate is still too poor to allow sequence identification, and this results in many false-negative as well as false-positive identifications. Here, we present a novel strategy, which is based on the use of alkaline phosphatase to remove phosphates and analysis of phospho/dephosphopeptide retention times to increase the reliability of identification. The use of phospho/dephosphopeptide retention time ratios allows the identification of phosphopeptides with high confidence with the aid of a focused database of dephosphopeptides. This approach was very effective to identify multiple phophorylations in tryptic peptides. A 'true' phosphorylation data set should contain about 90% phospho-Ser and a few percent phospho-Tyr, and this ratio can be used as a quality criterion for evaluation of data sets. By applying this efficient approach, we were able to identify more than one thousand phosphopeptides.

Published

2007

14. Specificity of immobilized metal affinity-based IMAC/C18 tip enrichment of phosphopeptides for protein phosphorylation analysis.

Author

Kokubu M, Ishihama Y, Sato T, Nagasu T, and Oda Y

Subjects

Amino Acid Sequence, Animals, Brain metabolism, Hydrophobic and Hydrophilic Interactions, Mice, Molecular Sequence Data, Phosphorylation, Sensitivity and Specificity, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Carbon chemistry, Chromatography, Affinity methods, Metals chemistry, Microarray Analysis methods, Phosphopeptides analysis, Phosphopeptides chemistry, Phosphoproteins analysis

Abstract

We have developed a simple, highly specific enrichment procedure for phosphopeptides, by increasing the specificity of an immobilized metal affinity column (IMAC) without using any chemical reaction. The method employs a biphasic IMAC-C18 tip, in which IMAC beads are packed on an Empore C18 disk in a 200-microL pipet tip. Phosphopeptides are separated from non-phosphopeptides on the IMAC in an optimized solvent without any chemical reaction, then desorbed from the IMAC using a phosphate buffer, reconcentrated, and desalted on the C18 disk. The increase in selectivity was achieved by (a) using a strong acid to discriminate phosphates from carboxyl groups of peptides and (b) using a high concentration of acetonitrile to remove hydrophobic non-phosphopeptides. The entire procedure was optimized by using known phosphoproteins such as Akt1 kinase and protein kinase A. Although it was difficult to detect phosphopeptides in MALDI-MS spectra of tryptic peptide mixtures before enrichment, after the IMAC procedure, we could successfully detect phosphopeptides with almost no non-phosphopeptides. Next, we constructed an array of IMAC-IMAC/C18 tips, such that number of arrayed tips on a 96-well plate could easily be changed depending on the loading amount of sample. Applying this approach to mouse forebrain resulted in the identification of 162 phosphopeptides (166 phosphorylation sites) from 135 proteins using nano-LC/MS.

Published

2005