Your search keyword '"Ubiquitinated Proteins analysis"' showing total 27 results

1. Antibody-free approach for ubiquitination profiling by selectively clicking the ubiquitination sites.

Author

Sun M, Zhang Q, Zhao B, Huang Q, Wu W, Fan P, Zhang L, and Zhang X

Subjects

Humans, Chromatography, Liquid, Reproducibility of Results, Ubiquitination, Ubiquitin, Ubiquitinated Proteins analysis, Ubiquitinated Proteins chemistry, Ubiquitinated Proteins metabolism, Peptides chemistry, Antibodies metabolism, Amines, Ubiquitin Thiolesterase metabolism, Ubiquitin-Conjugating Enzymes metabolism, Lysine metabolism, Tandem Mass Spectrometry

Abstract

Ubiquitination is a reversible post-translational modification that plays a pivotal role in numerous biological processes. Antibody-based approaches, as the most used methods for identifying ubiquitination sites, exist sequence recognition bias, high cost, and ubiquitin-like protein modification interference, limiting their widespread application. Here, we proposed an Antibody-Free approach for Ubiquitination Profiling, termed AFUP, by selectively clicking the ubiquitinated lysine to enrich and profile endogenous ubiquitinated peptides using mass spectrometry. Briefly, protein amines were blocked with formaldehyde, and then the ubiquitin molecules were hydrolyzed from the ubiquitinated proteins by non-specific deubiquitinases USP2 and USP21 to release the free ε-amine of lysine. Peptides containing free ε-amines were selectively enriched with streptavidin beads upon NHS-SS-biotin labeling. Finally, the enriched peptides were eluted by DTT and analyzed by LC-MS/MS, resulting in ubiquitination profiling. Preliminary experiment showed that 349 ± 7 ubiquitination sites were identified in 0.8 mg HeLa lysates with excellent reproducibility (CV = 2%) and high quantitative stability (Pearson, r ≥ 0.91) using our method. With the combination of AFUP and simple basic C18 pre-fractionation, approximately 4000 ubiquitination sites were identified in a single run of 293T cells. In addition, we showed that 209 ubiquitination sites were significantly regulated in UBE2O knockdown cells after normalized to protein abundance. In conclusion, our results demonstrated that AFUP is a robust alternative strategy for ubiquitomics research., 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 Elsevier B.V. All rights reserved.)

Published

2023

2. Polyubiquitin Profile in Down Syndrome and Alzheimer's Disease Brain.

Author

Tramutola A and Perluigi M

Subjects

Analytic Sample Preparation Methods, Animals, Disease Models, Animal, Humans, Mass Spectrometry, Proteolysis, Ubiquitination, Alzheimer Disease metabolism, Brain metabolism, Down Syndrome metabolism, Electrophoresis, Gel, Two-Dimensional, Proteomics, Ubiquitinated Proteins analysis

Abstract

Posttranslational modifications (PTMs) of a protein are chemical modifications that play a key role because they regulate almost all cellular events, including gene expression, signal transduction, protein-protein interaction, cell-cell interaction, and communication. Defects in PTMs have been linked to numerous developmental disorders and human diseases, highlighting the importance of PTMs in maintaining normal cellular states. PTMs reversibly or irreversibly alter the structure and properties of proteins through biochemical reactions, thus extending protein function beyond what is dictated by gene transcripts. As analytical approaches have evolved, the biological influences of many types of PTMs have been identified and are routinely analyzed in many systems.Among several types of PTMs, polyubiquitination-addition of ubiquitin (often in the form of polymers) to substrates-governs a variety of biological processes ranging from proteolysis to DNA damage response. The functional flexibility of this modification correlates with the existence of a large number of ubiquitinating enzymes that form distinct ubiquitin polymers, which in turn result in different signals. Thus, the need of specific and sensitive methods for the analysis of the complexity of ubiquitin chain linkage is needed to understand how this structural diversity could translate into various cellular functions. In this section, we described a detailed protocol to enrich polyubiquitinated proteins.

Published

2021

3. Monitoring protein ubiquitination and SUMOylation in real-time by NMR.

Author

Habibullah BI, Tripathi V, Surana P, and Das R

Subjects

Humans, Models, Molecular, Time Factors, Ubiquitin chemistry, Nuclear Magnetic Resonance, Biomolecular, Sumoylation, Ubiquitin metabolism, Ubiquitinated Proteins analysis, Ubiquitinated Proteins chemistry, Ubiquitination

Abstract

The covalent conjugation of ubiquitin (Ub), known as ubiquitination, is a multi-step reaction involving multiple enzymes. We report a real-time, tag-free method to monitor protein ubiquitination by NMR spectroscopy under physiological conditions. The approach is also applicable for monitoring other ubiquitin-like modifications, and the disassembly of Ub polymers.

Published

2020

4. Detection of Protein Ubiquitination Sites by Peptide Enrichment and Mass Spectrometry.

Author

Bezstarosti K, van der Wal L, and Demmers JAA

Subjects

Amino Acid Sequence, Animals, Bortezomib pharmacology, Cell Line, Tumor, Humans, Isotope Labeling, Mice, Peptides chemistry, Ubiquitinated Proteins chemistry, Mass Spectrometry methods, Peptides metabolism, Ubiquitinated Proteins analysis, Ubiquitination

Abstract

The posttranslational modification of proteins by the small protein ubiquitin is involved in many cellular events. After tryptic digestion of ubiquitinated proteins, peptides with a diglycine remnant conjugated to the epsilon amino group of lysine ('K-ε-diglycine' or simply 'diGly') can be used to track back the original modification site. Efficient immunopurification of diGly peptides combined with sensitive detection by mass spectrometry has resulted in a huge increase in the number of ubiquitination sites identified up to date. We have made several improvements to this workflow, including offline high pH reverse-phase fractionation of peptides prior to the enrichment procedure, and the inclusion of more advanced peptide fragmentation settings in the ion routing multipole. Also, more efficient cleanup of the sample using a filter-based plug in order to retain the antibody beads results in a greater specificity for diGly peptides. These improvements result in the routine detection of more than 23,000 diGly peptides from human cervical cancer cells (HeLa) cell lysates upon proteasome inhibition in the cell. We show the efficacy of this strategy for in-depth analysis of the ubiquitinome profiles of several different cell types and of in vivo samples, such as brain tissue. This study presents an original addition to the toolbox for protein ubiquitination analysis to uncover the deep cellular ubiquitinome.

Published

2020

5. Proteome-wide identification and functional analysis of ubiquitinated proteins in peach leaves.

Author

Song Y, Shi X, Zou Y, Guo J, Huo N, Chen S, Zhao C, Li H, Wu G, and Peng Y

Subjects

Amino Acid Sequence, Plant Leaves chemistry, Plant Proteins analysis, Proteomics, Prunus persica chemistry, Ubiquitinated Proteins analysis, Ubiquitination, Plant Leaves metabolism, Plant Proteins metabolism, Prunus persica metabolism, Ubiquitinated Proteins metabolism

Abstract

Ubiquitination is a critical post-translational modification machinery that governs a wide range of cellular functions by regulating protein homeostasis. Identification of ubiquitinated proteins and lysine residues can help researchers better understand the physiological roles of ubiquitin modification in different biological systems. In this study, we report the first comprehensive analysis of the peach ubiquitome by liquid chromatography-tandem mass spectrometry-based diglycine remnant affinity proteomics. Our systematic profiling revealed a total of 544 ubiquitination sites on a total of 352 protein substrates. Protein annotation and functional analysis suggested that ubiquitination is involved in modulating a variety of essential cellular and physiological processes in peach, including but not limited to carbon metabolism, histone assembly, translation and vesicular trafficking. Our results could facilitate future studies on how ubiquitination regulates the agricultural traits of different peach cultivars and other crop species.

Published

2020

6. Proteome-wide identification of ubiquitin interactions using UbIA-MS.

Author

Zhang X, Smits AH, van Tilburg GB, Ovaa H, Huber W, and Vermeulen M

Subjects

Binding Sites, Carrier Proteins, Chromatography, Affinity methods, Mass Spectrometry methods, Polyubiquitin, Protein Binding, Protein Processing, Post-Translational, Proteome, Software, Tandem Mass Spectrometry methods, Ubiquitin metabolism, Ubiquitinated Proteins chemistry, Ubiquitination physiology, Computational Biology methods, Ubiquitin chemistry, Ubiquitinated Proteins analysis

Abstract

Ubiquitin-binding proteins play an important role in eukaryotes by translating differently linked polyubiquitin chains into proper cellular responses. Current knowledge about ubiquitin-binding proteins and ubiquitin linkage-selective interactions is mostly based on case-by-case studies. We have recently reported a method called ubiquitin interactor affinity enrichment-mass spectrometry (UbIA-MS), which enables comprehensive identification of ubiquitin interactors for all ubiquitin linkages from crude cell lysates. One major strength of UbIA-MS is the fact that ubiquitin interactors are enriched from crude cell lysates, in which proteins are present at endogenous levels, contain biologically relevant post-translational modifications (PTMs) and are assembled in native protein complexes. In addition, UbIA-MS uses chemically synthesized nonhydrolyzable diubiquitin, which mimics native diubiquitin and is inert to cleavage by endogenous deubiquitinases (DUBs). Here, we present a detailed protocol for UbIA-MS that proceeds in five stages: (i) chemical synthesis of ubiquitin precursors and click chemistry for the generation of biotinylated nonhydrolyzable diubiquitin baits, (ii) in vitro affinity purification of ubiquitin interactors, (iii) on-bead interactor digestion, (iv) liquid chromatography (LC)-MS/MS analysis and (v) data analysis to identify differentially enriched proteins. The computational analysis tools are freely available as an open-source R software package, including a graphical interface. Typically, UbIA-MS allows the identification of dozens to hundreds of ubiquitin interactors from any type of cell lysate, and can be used to study cell type or stimulus-dependent ubiquitin interactions. The nonhydrolyzable diubiquitin synthesis can be completed in 3 weeks, followed by ubiquitin interactor enrichment and identification, which can be completed within another 2 weeks.

Published

2018

7. Ubiquitin Conjugation Probed by Inflammation in Myeloid-Derived Suppressor Cell Extracellular Vesicles.

Author

Adams KR, Chauhan S, Patel DB, Clements VK, Wang Y, Jay SM, Edwards NJ, Ostrand-Rosenberg S, and Fenselau C

Subjects

Animals, Binding Sites, Cell Movement, Mice, Ubiquitinated Proteins analysis, Ubiquitination, Extracellular Vesicles pathology, Inflammation, Myeloid-Derived Suppressor Cells ultrastructure, Ubiquitin metabolism

Abstract

Ubiquitinated proteins carried by the extracellular vesicles (EV) released by myeloid-derived suppressor cells (MDSC) have been investigated using proteomic strategies to examine the effect of tumor-associated inflammation. EV were collected from MDSC directly following isolation from tumor-bearing mice with low and high inflammation. Among the 1092 proteins (high inflammation) and 925 proteins (low inflammation) identified, more than 50% were observed as ubiquitinated proteoforms. More than three ubiquitin-attachment sites were characterized per ubiquitinated protein, on average. Multiple ubiquitination sites were identified in the pro-inflammatory proteins S100 A8 and S100 A9, characteristic of MDSC and in histones and transcription regulators among other proteins. Spectral counting and pathway analysis suggest that ubiquitination occurs independently of inflammation. Some ubiquitinated proteins were shown to cause the migration of MDSC, which has been previously connected with immune suppression and tumor progression. Finally, MDSC EV are found collectively to carry all the enzymes required to catalyze ubiquitination, and the hypothesis is presented that a portion of the ubiquitinated proteins are produced in situ.

Published

2018

8. Quantitative Proteomics Reveals Extensive Changes in the Ubiquitinome after Perturbation of the Proteasome by Targeted dsRNA-Mediated Subunit Knockdown in Drosophila.

Author

Sap KA, Bezstarosti K, Dekkers DHW, Voets O, and Demmers JAA

Subjects

Animals, Gene Knockdown Techniques, Proteasome Endopeptidase Complex deficiency, Proteasome Endopeptidase Complex metabolism, Protein Subunits genetics, RNA, Double-Stranded genetics, Ubiquitin analysis, Ubiquitin metabolism, Ubiquitination, Drosophila chemistry, Proteomics methods, Ubiquitinated Proteins analysis

Abstract

The ubiquitin-proteasome system (UPS), a highly regulated mechanism including the active marking of proteins by ubiquitin to be degraded, is critical in regulating proteostasis. Dysfunctioning of the UPS has been implicated in diseases such as cancer and neurodegenerative disorders. Here we investigate the effects of proteasome malfunctioning on global proteome and ubiquitinome dynamics using SILAC proteomics in Drosophila S2 cells. dsRNA-mediated knockdown of specific proteasome target subunits is used to inactivate the proteasome. Upon this perturbation, both the global proteome and the ubiquitinome become modified to a great extent, with the overall impact on the ubiquitinome being the most dramatic. The abundances of ∼10% of all proteins are increased, while the abundances of the far majority of over 14 000 detected diGly peptides are increased, suggesting that the pool of ubiquitinated proteins is highly dynamic. Remarkably, several proteins show heterogeneous ubiquitination dynamics, with different lysine residues on the same protein showing either increased or decreased ubiquitination. This suggests the occurrence of simultaneous and functionally different ubiquitination events. This strategy offers a powerful tool to study the response of the ubiquitinome upon interruption of normal UPS activity by targeted interference and opens up new avenues for the dissection of the mode of action of individual components of the proteasome. Because this is to our knowledge the first comprehensive ubiquitinome screen upon proteasome malfunctioning in a fruit fly cell system, this data set will serve as a valuable repository for the Drosophila community.

Published

2017

9. Optimising methods for the preservation, capture and identification of ubiquitin chains and ubiquitylated proteins by immunoblotting.

Author

Emmerich CH and Cohen P

Subjects

Animals, Electrophoresis, Polyacrylamide Gel methods, Humans, Immunoprecipitation methods, Ubiquitin genetics, Ubiquitin metabolism, Ubiquitin-Specific Proteases metabolism, Ubiquitinated Proteins metabolism, Ubiquitination, Up-Regulation, Immunoblotting methods, Ubiquitin analysis, Ubiquitinated Proteins analysis

Abstract

Immunoblotting is a powerful technique for the semi-quantitative analysis of ubiquitylation events, and remains the most commonly used method to study this process due to its high specificity, speed, sensitivity and relatively low cost. However, the ubiquitylation of proteins is complex and, when the analysis is performed in an inappropriate manner, it can lead to the misinterpretation of results and to erroneous conclusions being reached. Here we discuss the advantages and disadvantages of the methods currently in use to analyse ubiquitin chains and protein ubiquitylation, and describe the procedures that we have found to be most useful for optimising the quality and reliability of the data that we have generated. We also highlight commonly encountered problems and the pitfalls inherent in some of these methods. Finally, we introduce a set of recommendations to help researchers obtain high quality data, especially those new to the field of ubiquitin signalling. The specific topics addressed in this article include sample preparation, the separation, detection and identification of particular ubiquitin chains by immunoblotting, and the analysis of ubiquitin chain topology through the combined use of ubiquitin-binding proteins and ubiquitin linkage-specific deubiquitylases., (Copyright © 2015 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2015

10. ETD Outperforms CID and HCD in the Analysis of the Ubiquitylated Proteome.

Author

Porras-Yakushi TR, Sweredoski MJ, and Hess S

Subjects

Databases, Protein, Mass Spectrometry methods, Proteome analysis, Proteome chemistry, Ubiquitinated Proteins analysis, Ubiquitinated Proteins chemistry

Abstract

Comprehensive analysis of the ubiquitylome is a prerequisite to fully understand the regulatory role of ubiquitylation. However, the impact of key mass spectrometry parameters on ubiquitylome analyses has not been fully explored. In this study, we show that using electron transfer dissociation (ETD) fragmentation, either exclusively or as part of a decision tree method, leads to ca. 2-fold increase in ubiquitylation site identifications in K-ε-GG peptide-enriched samples over traditional collisional-induced dissociation (CID) or higher-energy collision dissociation (HCD) methods. Precursor ions were predominantly observed as 3+ charged species or higher and in a mass range 300-1200 m/z. N-ethylmaleimide was used as an alkylating agent to reduce false positive identifications resulting from overalkylation with halo-acetamides. These results demonstrate that the application of ETD fragmentation, in addition to narrowing the mass range and using N-ethylmaleimide yields more high-confidence ubiquitylation site identification than conventional CID and HCD analysis.

Published

2015

11. Development of two novel high-throughput assays to quantify ubiquitylated proteins in cell lysates: application to screening of new anti-malarials.

Author

Mata-Cantero L, Cid C, Gomez-Lorenzo MG, Xolalpa W, Aillet F, Martín JJ, and Rodriguez MS

Subjects

Malaria, Falciparum drug therapy, Proteasome Endopeptidase Complex metabolism, Ubiquitins metabolism, Antimalarials pharmacology, Drug Discovery methods, High-Throughput Screening Assays methods, Plasmodium falciparum drug effects, Protozoan Proteins analysis, Ubiquitinated Proteins analysis

Abstract

Background: The ubiquitin proteasome system (UPS) is one of the main proteolytical pathways in eukaryotic cells and plays an essential role in key cellular processes such as cell cycle, stress response, signal transduction, and transcriptional regulation. Many components of this pathway have been implicated in diverse pathologies including cancer, neurodegeneration and infectious diseases, such as malaria. The success of proteasome inhibitors in clinical trials underlines the potential of the UPS in drug discovery., Methods: Plasmodium falciparum, the malaria causative pathogen, has been used to develop two assays that allow the quantification of the parasite protein ubiquitylation levels in a high-throughput format that can be used to find new UPS inhibitors., Results: In both assays tandem ubiquitin binding entities (TUBEs), also known as ubiquitin traps, have been used to capture ubiquitylated proteins from cell lysates. The primary assay is based on AlphaLISA technology, and the orthogonal secondary assay relies on a dissociation-enhanced lanthanide fluorescent immunoassay (DELFIA) system. A panel of well-known proteasome inhibitors has been used to validate both technologies. An excellent correlation was obtained between these biochemical assays and the standard whole cell assay that measures parasite growth inhibition., Conclusions: The two assays presented can be used in a high-throughput format to find new UPS inhibitors for P. falciparum and could help to identify new targets within this system. This methodology is also applicable to other cellular contexts or pathologies.

Published

2015

12. Deubiquitinase-based analysis of ubiquitin chain architecture using Ubiquitin Chain Restriction (UbiCRest).

Author

Hospenthal MK, Mevissen TET, and Komander D

Subjects

Blotting, Western, Ubiquitin chemistry, Ubiquitin metabolism, Ubiquitin-Specific Proteases chemistry, Ubiquitination, Biochemistry methods, Ubiquitin analysis, Ubiquitin-Specific Proteases metabolism, Ubiquitinated Proteins analysis, Ubiquitinated Proteins chemistry

Abstract

Protein ubiquitination is a versatile protein modification that regulates virtually all cellular processes. This versatility originates from polyubiquitin chains, which can be linked in eight distinct ways. The combinatorial complexity of eight linkage types in homotypic (one chain type per polymer) and heterotypic (multiple linkage types per polymer) chains poses significant problems for biochemical analysis. Here we describe UbiCRest, in which substrates (ubiquitinated proteins or polyubiquitin chains) are treated with a panel of linkage-specific deubiquitinating enzymes (DUBs) in parallel reactions, followed by gel-based analysis. UbiCRest can be used to show that a protein is ubiquitinated, to identify which linkage type(s) are present on polyubiquitinated proteins and to assess the architecture of heterotypic polyubiquitin chains. DUBs used in UbiCRest can be obtained commercially; however, we include details for generating a toolkit of purified DUBs and for profiling their linkage preferences in vitro. UbiCRest is a qualitative method that yields insights into ubiquitin chain linkage types and architecture within hours, and it can be performed on western blotting quantities of endogenously ubiquitinated proteins., Competing Interests: DK is part of the DUB Alliance that includes Cancer Research Technology and FORMA Therapeutics, and is a consultant for FORMA Therapeutics. A patent application has been filed for the described method. Boston Biochem / Biotechne distribute an enzyme kit for performing UbiCRest analysis.

Published

2015

13. Polyubiquitinated proteins, proteasome, and glycogen characterize the particle-rich cytoplasmic structure (PaCS) of neoplastic and fetal cells.

Author

Necchi V, Sommi P, Vitali A, Vanoli A, Savoia A, Ricci V, and Solcia E

Subjects

Cytoplasm chemistry, Cytoplasm ultrastructure, Glycogen analysis, Humans, Immunohistochemistry, Microscopy, Confocal, Microscopy, Electron, Transmission, Proteasome Endopeptidase Complex analysis, Ubiquitinated Proteins analysis, Cytoplasm metabolism, Fetus cytology, Glycogen metabolism, Neoplasms pathology, Proteasome Endopeptidase Complex metabolism, Ubiquitinated Proteins metabolism

Abstract

A particle-rich cytoplasmic structure (PaCS) concentrating ubiquitin-proteasome system (UPS) components and barrel-like particles in clear, cytoskeleton- and organelle-free areas has recently been described in some neoplasms and in genetic or infectious diseases at risk of neoplasia. Ultrastructurally similar particulate cytoplasmic structures, interpreted as glycogen deposits, have previously been reported in clear-cell neoplasms and some fetal tissues. It remains to be investigated whether the two structures are the same, colocalize UPS components and polysaccharides, and have a role in highly proliferative cells such as fetal and neoplastic cells. We used immunogold electron microscopy and confocal immunofluorescence microscopy to examine human and mouse fetal tissues and human neoplasms. Fetal and neoplastic cells both showed colocalization of polyubiquitinated proteins, 19S and 20S proteasomes, and polysaccharides, both glycogen and chondroitin sulfate, inside cytoplasmic structures showing all distinctive features of PaCSs. Poorly demarcated and/or hybrid (ribosomes admixed) UPS- and glycogen-enriched areas, likely stages in PaCS development, were also seen in some fetal cells, with special reference to those, like primary alveolar pulmonary cells or pancreatic centroacinar cells, having a crucial role in organogenesis. UPS- and glycogen-rich PaCSs developed extensively in clear-cell neoplasms of the kidney, ovary, pancreas, and other organs, as well as, in infantile, development-related tumors replicating fetal patterns, such as choroid plexus papilloma. UPS-mediated, ATP-dependent proteolysis and its potential energy source, glycogen metabolism, may have a crucial, synergic role in embryo-/organogenesis and carcinogenesis.

Published

2014

14. Decreased histone H2B monoubiquitination in malignant gastric carcinoma.

Author

Wang ZJ, Yang JL, Wang YP, Lou JY, Chen J, Liu C, and Guo LD

Subjects

Carcinoma mortality, Carcinoma secondary, Carcinoma surgery, Case-Control Studies, Cell Differentiation, Down-Regulation, Female, Humans, Immunohistochemistry, Kaplan-Meier Estimate, Lymphatic Metastasis, Male, Methylation, Middle Aged, Multivariate Analysis, Neoplasm Staging, Predictive Value of Tests, Proportional Hazards Models, Risk Factors, Stomach Neoplasms mortality, Stomach Neoplasms pathology, Stomach Neoplasms surgery, Ubiquitination, Biomarkers, Tumor analysis, Carcinoma chemistry, Histones analysis, Stomach Neoplasms chemistry, Ubiquitinated Proteins analysis

Abstract

Aim: To investigate H2B monoubiquitination (uH2B) and H3K4 di- and tri-methylation (H3K4-2me, H3K4-3me) levels and their clinical significance in gastric cancer (GC)., Methods: Immunohistochemistry (IGC) was used to detect the differential levels of uH2B, H3K4-2me and H3K4-3me modifications in GC specimens from chemo/radiotherapy-naïve patients who underwent potentially curative surgical resection (n = 159) and in a random sampling of non-tumor gastric epithelium specimens (normal controls, n = 20). The immunohistochemistry (IHC)-detected modifications were classified as negative, low-level, or high-level using a dual-rated (staining intensity and percentage of positively-stained cells) semi-quantitative method. The relationships between uH2B modification levels and clinicopathological parameters of GC were assessed by a Wilcoxon rank sum test (pairwise comparisons) and the Kruskal-Wallis H test (multiple comparisons). The correlation between uH2B modification and survival was estimated by Kaplan-Meier analysis, and the role of uH2B as an independent prognostic factor for survival was assessed by multivariate Cox regression analysis., Results: The presence and level of H3K4-2me and H3K4-3me IHC staining was similar between the normal controls and GC specimens. In contrast, the level of uH2B was significantly lower in the malignant gastric tissues (vs normal control tissues) and decreased along with increases in dedifferentiation (well differentiated > moderately differentiated > poorly differentiated). The level of uH2B correlated with tumor differentiation (P < 0.001), Lauren's diffuse- and intestinal-type classification (P < 0.001), lymph node metastasis (P = 0.049) and tumor-node-metastasis stage (P = 0.005). Patients with uH2B+ staining had higher 5-year survival rates than patients with uH2B-staining (52.692 ± 2.452 vs 23.739 ± 5.207, P < 0.001). The uH2B level was an independent prognostic factor for cancer-specific survival (95%CI: 0.237-0.677, P = 0.001)., Conclusion: uH2B displays differential IHC staining patterns corresponding to progressive stages of GC. uH2B may contribute to tumorigenesis and could be a potential therapeutic target.

Published

2013

15. Evaluation of ubiquitinated proteins by proteomics reveals the role of the ubiquitin proteasome system in the regulation of Grp75 and Grp78 chaperone proteins during intestinal inflammation.

Author

Bertrand J, Tennoune N, Marion-Letellier R, Goichon A, Chan P, Mbodji K, Vaudry D, Déchelotte P, and Coëffier M

Subjects

Animals, Cell Line, Tumor, Colitis chemically induced, Colitis metabolism, Colon chemistry, Endoplasmic Reticulum Chaperone BiP, HSP70 Heat-Shock Proteins analysis, HSP70 Heat-Shock Proteins chemistry, Heat-Shock Proteins analysis, Heat-Shock Proteins chemistry, Humans, Interleukin-8 analysis, Interleukin-8 metabolism, Intestinal Mucosa chemistry, Intestinal Mucosa metabolism, Male, Membrane Proteins analysis, Membrane Proteins chemistry, Rats, Rats, Wistar, Trinitrobenzenesulfonic Acid toxicity, Ubiquitin chemistry, Ubiquitin metabolism, Ubiquitinated Proteins chemistry, Ubiquitinated Proteins metabolism, Colon metabolism, HSP70 Heat-Shock Proteins metabolism, Heat-Shock Proteins metabolism, Membrane Proteins metabolism, Proteasome Endopeptidase Complex metabolism, Proteomics methods, Ubiquitinated Proteins analysis

Abstract

The ubiquitin proteasome system (UPS) is the major pathway of intracellular protein degradation and may be involved in the pathophysiology of inflammatory bowel diseases or irritable bowel syndrome. UPS specifically degrades proteins tagged with an ubiquitin chain. We aimed to identify polyubiquitinated proteins during inflammatory response in intestinal epithelial HCT-8 cells by a proteomic approach. HCT-8 cells were incubated with interleukin 1β, tumor necrosis factor-α, and interferon-γ for 2 h. Total cellular protein extracts were separated by 2D gel electrophoresis and analyzed by an immunodetection using antiubiquitin antibody. Differential ubiquitinated proteins were then identified by LC-ESI MS/MS. Seven proteins were differentially ubiquitinated between control and inflammatory conditions. Three of them were chaperones: Grp75 and Hsc70 were more ubiquitinated (p < 0.05) and Grp78 was less ubiquitinated (p < 0.05) under inflammatory conditions. The results for Grp75 and Grp78 were then confirmed in HCT-8 cells and in 2-4-6-trinitrobenzen sulfonic acid induced colitis in rats mimicking inflammatory bowel disease by immunoprecipitation. No difference was observed in irritable bowel syndrome like model. In conclusion, we showed that a proteomic approach is suitable to identify ubiquitinated proteins and that UPS-regulated expression of Grp75 and Grp78 may be involved in inflammatory response. Further studies should lead to the identification of ubiquitin ligases responsible for Grp75 and Grp78 ubiquitination., (© 2013 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2013

16. Using glycinylation, a chemical derivatization technique, for the quantitation of ubiquitinated proteins.

Author

Fiedler KL and Cotter RJ

Subjects

Chromatography, Liquid methods, Humans, Protein Processing, Post-Translational genetics, Saccharomyces cerevisiae genetics, Ubiquitinated Proteins genetics, Glycine chemistry, Tandem Mass Spectrometry methods, Ubiquitinated Proteins analysis

Abstract

The quantitation of lysine post-translational modifications (PTMs) by bottom-up mass spectrometry is convoluted by the need for analogous derivatives and the production of different tryptic peptides from the unmodified and modified versions of a protein. Chemical derivatization of lysines prior to enzymatic digestion circumvents these problems and has proven to be a successful method for lysine PTM quantitation. The most notable example is the use of deuteroacetylation to quantitate lysine acetylation. In this work, levels of lysine ubiquitination were quantitated using a structurally homologous label that is chemically similar to the diglycine (GlyGly) tag, which is left at the ubiquitination site upon trypsinolysis. The LC-MS analysis of a chemically equivalent monoglycine (Gly) tag that is analogous to the corresponding GlyGly tag proved that the monoglycine tag can be used for the quantitation of ubiquitination. A glycinylation protocol was then established for the derivatization of proteins to label unmodified lysine residues with a single glycine tag. Ubiquitin multimers were used to show that after glycinylation and tryptic digestion, the mass spectrometric response from the corresponding analogous tagged peptides could be compared for relative quantitation. For a proof of principle regarding the applicability of this technique to the analysis of ubiquitination in biological samples, the glycinylation technique was used to quantitate the increase in monoubiquitinated histone H2B that is observed in yeast which lacks the enzyme responsible for deubiquitinating H2B-K123, compared to wild-type yeast.

Published

2013

17. Refined preparation and use of anti-diglycine remnant (K-ε-GG) antibody enables routine quantification of 10,000s of ubiquitination sites in single proteomics experiments.

Author

Udeshi ND, Svinkina T, Mertins P, Kuhn E, Mani DR, Qiao JW, and Carr SA

Subjects

Amino Acids metabolism, Antibodies chemistry, Antibodies immunology, Binding Sites, Chromatography, Liquid methods, Cross-Linking Reagents chemistry, Cysteine Proteinase Inhibitors pharmacology, Glycylglycine immunology, Humans, Isotope Labeling methods, Jurkat Cells, Leupeptins pharmacology, Proteasome Endopeptidase Complex metabolism, Proteome chemistry, Proteome metabolism, Reproducibility of Results, Tandem Mass Spectrometry methods, Ubiquitinated Proteins analysis, Ubiquitinated Proteins chemistry, Ubiquitinated Proteins metabolism, Proteome analysis, Proteomics methods, Ubiquitination

Abstract

Detection of endogenous ubiquitination sites by mass spectrometry has dramatically improved with the commercialization of anti-di-glycine remnant (K-ε-GG) antibodies. Here, we describe a number of improvements to the K-ε-GG enrichment workflow, including optimized antibody and peptide input requirements, antibody cross-linking, and improved off-line fractionation prior to enrichment. This refined and practical workflow enables routine identification and quantification of ∼20,000 distinct endogenous ubiquitination sites in a single SILAC experiment using moderate amounts of protein input.

Published

2013

18. Ubiquitin - omics reveals novel networks and associations with human disease.

Author

Kessler BM

Subjects

Animals, Bacterial Infections metabolism, Humans, Inflammation metabolism, Mass Spectrometry methods, Models, Molecular, Neoplasms metabolism, Neurodegenerative Diseases metabolism, Signal Transduction, Ubiquitin analysis, Ubiquitinated Proteins analysis, Ubiquitination, Ubiquitins analysis, Ubiquitins metabolism, Virus Diseases metabolism, Protein Interaction Mapping methods, Proteomics methods, Ubiquitin metabolism, Ubiquitinated Proteins metabolism

Abstract

Human neurodegenerative and infectious diseases and tumorigenesis are associated with alterations in ubiquitin pathways. Over 10% of the genome encode for genes that either bind or manipulate ubiquitin to affect a large proportion of biological processes. This has been the basis for the development of approaches allowing the enrichment of ubiquitinated proteins for comparisons using proteomics and mass spectrometry. Tools such as tagged tandem ubiquitin binding domains, chemically derivatized ubiquitin or anti-gly-gly-lys antibodies combined with mass spectrometry have contributed to surveys of poly-ubiquitinated proteins, poly-ubiquitin linkage diversity and protein ubiquitination sites and their relation to other posttranslational modifications at a proteome wide level, providing insights in to how dynamic alterations in ubiquitination and deubiquitination steps are associated with normal physiology and pathogenesis., (Copyright © 2013 Elsevier Ltd. All rights reserved.)

Published

2013

19. Development of a homogeneous AlphaLISA ubiquitination assay using ubiquitin binding matrices as universal components for the detection of ubiquitinated proteins.

Author

Schneider S, Chen H, Tang J, Emkey R, and Andrews PS

Subjects

Enzyme-Linked Immunosorbent Assay, Humans, Recombinant Proteins metabolism, Ubiquitinated Proteins metabolism, Ubiquitination, Polyubiquitin chemistry, Polyubiquitin metabolism, Recombinant Proteins analysis, Tandem Repeat Sequences, Ubiquitinated Proteins analysis

Abstract

The Ubiquitin Proteasome Pathway (UPP) has become a target rich pathway for therapeutic intervention as its role in pathogenic disease is better understood. In particular many E3 ligases within this pathway have been implicated in cancer, inflammation and metabolic diseases. It has been of great interest to develop biochemical assays to identify inhibitors of catalytic E3 ubiquitination activity as a means of abrogating the disease mechanism. Here we describe a homogeneous biochemical assay that utilizes native ubiquitin and Tandem-repeated Ubiquitin-Binding Entities (TUBEs) as a detection technology for ubiquitination activity. We developed a TUBEs based proximity AlphaLisa® assay for Mdm2, which is an E3 ligase that negatively regulates p53 tumor suppressor protein. We further demonstrate that this assay strategy or design can also be applied to the development of assays to detect autoubiquitination of other E3 ligases that are also of interest for therapeutic intervention. This article is part of a Special Issue entitled: Ubiquitin Drug Discovery and Diagnostics., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published

2012

20. Synaptic protein ubiquitination in rat brain revealed by antibody-based ubiquitome analysis.

Author

Na CH, Jones DR, Yang Y, Wang X, Xu Y, and Peng J

Subjects

Amino Acid Sequence, Animals, Antibodies chemistry, Antibodies metabolism, Brain Chemistry physiology, Chromatography, Ion Exchange, Databases, Protein, Iodoacetamide, Lysine chemistry, Lysine metabolism, Molecular Sequence Data, Nerve Tissue Proteins chemistry, Nerve Tissue Proteins metabolism, Peptide Fragments analysis, Peptide Fragments chemistry, Peptide Fragments metabolism, Proteome chemistry, Proteome metabolism, Rats, Synapses, Tandem Mass Spectrometry, Ubiquitin chemistry, Ubiquitinated Proteins chemistry, Ubiquitinated Proteins metabolism, Ubiquitination, Brain metabolism, Nerve Tissue Proteins analysis, Proteome analysis, Proteomics methods, Ubiquitin metabolism, Ubiquitinated Proteins analysis

Abstract

Protein ubiquitination is an essential post-translational modification regulating neurodevelopment, synaptic plasticity, learning, and memory, and its dysregulation contributes to the pathogenesis of neurological diseases. Here we report a systematic analysis of ubiquitinated proteome (ubiquitome) in rat brain using a newly developed monoclonal antibody that recognizes the diglycine tag on lysine residues in trypsinized peptides (K-GG peptides). Initial antibody specificity analysis showed that the antibody can distinguish K-GG peptides from linear GG peptides or pseudo K-GG peptides derived from iodoacetamide. To evaluate the false discovery rate of K-GG peptide matches during database search, we introduced a null experiment using bacterial lysate that contains no such peptides. The brain ubiquitome was then analyzed by this antibody enrichment with or without strong cation exchange (SCX) prefractionation. During SCX chromatography, although the vast majority of K-GG peptides were detected in the fractions containing at least three positive charged peptides, specific K-GG peptides with two positive charges (e.g., protein N-terminal acetylated and C-terminal non-K/R peptides) were also identified in early fractions. The reliability of C-terminal K-GG peptides was also extensively investigated. Finally, we collected a data set of 1786 K-GG sites on 2064 peptides in 921 proteins and estimated their abundance by spectral counting. The study reveals a wide range of ubiquitination events on key components in presynaptic region (e.g., Bassoon, NSF, SNAP25, synapsin, synaptotagmin, and syntaxin) and postsynaptic density (e.g., PSD-95, GKAP, CaMKII, as well as receptors for NMDA, AMPA, GABA, serotonin, and acetylcholine). We also determined ubiquitination sites on amyloid precursor protein and alpha synuclein that are thought to be causative agents in Alzhermer's and Parkinson's disorders, respectively. As K-GG peptides can also be produced from Nedd8 or ISG15 modified proteins, we quantified these proteins in the brain and found that their levels are less than 2% of ubiquitin. Together, this study demonstrates that a large number of neuronal proteins are modified by ubiquitination and provides a feasible method for profiling the ubiquitome in the brain.

Published

2012

21. Proteomic analysis of salt-responsive ubiquitin-related proteins in rice roots.

Author

Liu CW, Hsu YK, Cheng YH, Yen HC, Wu YP, Wang CS, and Lai CC

Subjects

Amino Acid Sequence, Blotting, Western, Chromatography, Liquid, Molecular Sequence Data, Oryza enzymology, Oryza genetics, Oryza metabolism, Plant Proteins chemistry, Plant Proteins metabolism, Plant Roots chemistry, Plant Roots physiology, Proteome metabolism, Proteomics methods, Salt Tolerance, Salt-Tolerant Plants enzymology, Salt-Tolerant Plants genetics, Salt-Tolerant Plants metabolism, Sodium Chloride, Tandem Mass Spectrometry, Ubiquitinated Proteins chemistry, Ubiquitinated Proteins metabolism, Oryza chemistry, Plant Proteins analysis, Salt-Tolerant Plants chemistry, Ubiquitinated Proteins analysis

Abstract

Rationale: Ubiquitination of proteins plays an important role in regulating a myriad of physiological functions in plants such as xylogenesis, senescence, cell cycle control, and stress response. However, only a limited number of proteins in plants have been identified as being ubiquitinated in response to salt stress. The relationships between ubiquitination and salt-stress responses in plants are not clear., Methods: Rice (Oryza sativa) seedlings from the same genetic background with various salt tolerances exposed to salt stress were studied. The proteins of roots were extracted then analyzed using western blotting against ubiquitin. Differentially expressed ubiquitinated proteins were identified by nanospray liquid chromatography/tandem mass spectrometry (nano-LC/MS/MS) and quantified by label-free methods based on the Exponentially Modified Protein Abundance Index (emPAI) and on the peak areas of XIC spectra derived from ubiquitinated peptides. In addition, we performed a gel-based shotgun proteomic analysis to detect the ubiquitinated proteome that may be involved in response to salt stress., Results: The expressions of ubiquitination on pyruvate phosphate dikinase 1, heat shock protein 81-1, probable aldehyde oxidase 3, plasma membrane ATPase, cellulose synthase A catalytic subunit 4 [UDP-forming] and cyclin-C1-1 were identified and compared before and after salt treatment. The functions of those ubiquitinated proteins were further discussed for defence against salt stress. In addition, a large number of ubiquitinated proteins were successfully identified as well in this study., Conclusions: The ubiquitination of proteins affected the protective mechanisms in rice seedlings to resist the salt stress during the initial phase. The findings in the present study also demonstrate that the regulated mechanisms through protein ubiquitination are important for rice seedlings against salt stress., (Copyright © 2012 John Wiley & Sons, Ltd.)

Published

2012

22. Integrative analysis of the ubiquitin proteome isolated using Tandem Ubiquitin Binding Entities (TUBEs).

Author

Lopitz-Otsoa F, Rodriguez-Suarez E, Aillet F, Casado-Vela J, Lang V, Matthiesen R, Elortza F, and Rodriguez MS

Subjects

Adenocarcinoma metabolism, Adenocarcinoma pathology, Biomarkers, Tumor analysis, Biomarkers, Tumor isolation & purification, Biomarkers, Tumor metabolism, Breast Neoplasms metabolism, Breast Neoplasms pathology, Cells, Cultured, Female, Humans, Mass Spectrometry, Models, Biological, Protein Binding physiology, Protein Interaction Maps, Proteomics methods, Recombinant Proteins analysis, Recombinant Proteins metabolism, Systems Integration, Tandem Repeat Sequences, Ubiquitin genetics, Ubiquitination, Proteome analysis, Proteome isolation & purification, Ubiquitin metabolism, Ubiquitinated Proteins analysis, Ubiquitinated Proteins isolation & purification

Abstract

The successful use of proteasome inhibitors in clinical trials revealed the potential of the Ubiquitin Proteasome System for drug development. Protein remodeling through ubiquitylation is known to regulate the stability and activity of essential cellular factors through largely uncharacterized mechanisms. Here, we used Tandem repeated Ubiquitin Binding Entities (TUBEs) under non-denaturing conditions followed by mass spectrometry analysis to study global ubiquitylation events that may lead to the identification of potential drug targets. Using this approach we identified 643 proteins including known and unknown ubiquitin targets from human breast adenocarcinoma MCF7 cells treated with Adriamycin. Coherent with a global cellular response to this genotoxic insult, cellular factors identified are involved in protein synthesis, cellular transport, RNA post-transcriptional modification and signaling pathways regulating early stress responses. This includes components of large macromolecular complexes such as subunits and regulators of the proteasome, supporting the use of this method to characterize networks of molecular interactions coordinated by ubiquitylation. Further in vitro and in silico analysis confirmed that 84% of the total proteins identified here, are ubiquitylated. More importantly the enrichment of known biomarkers and targets for drug development, underlined the potential of this approach for the identification of this clinically relevant information. This article is part of a Special Issue entitled: Proteomics: The clinical link., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published

2012

23. Ubiquitin/proteasome-mediated proteolysis is involved in the response to flooding stress in soybean roots, independent of oxygen limitation.

Author

Yanagawa Y and Komatsu S

Subjects

Cell Hypoxia, Cysteine Proteinase Inhibitors pharmacology, Electrophoresis, Gel, Two-Dimensional, Floods, Immersion adverse effects, Leupeptins pharmacology, Oxygen metabolism, Plant Proteins analysis, Plant Roots drug effects, Plant Roots metabolism, Plant Roots physiology, Proteasome Endopeptidase Complex drug effects, Proteasome Endopeptidase Complex immunology, Proteolysis, Seedlings drug effects, Seedlings metabolism, Seedlings physiology, Glycine max drug effects, Glycine max physiology, Time Factors, Ubiquitinated Proteins analysis, Ubiquitinated Proteins metabolism, Water adverse effects, Plant Proteins metabolism, Proteasome Endopeptidase Complex metabolism, Glycine max metabolism, Stress, Physiological physiology, Ubiquitin metabolism

Abstract

Ubiquitin/proteasome-mediated proteolysis plays an important role in the response to several environmental stresses. Here, we described the relationship of the proteolysis in the flooding stress in soybean (Glycine max L. cultivar Enrei). Immunoblot analyses were performed using antibodies against two subunits of 26S proteasome, Rpt5 and Rpn10, 20S proteasome and two subunits of COP9 signalosome (CSN), CSN4 and CSN5, to compare between flooded and untreated roots. We also examined their protein amounts in the condition of low oxygen. Moreover, crude extracts from flooded or untreated roots incubated with or without a proteasome inhibitor MG132 were analyzed by proteomics technique. We revealed that the amount of ubiquitinated proteins in soybean roots decreased after flooding treatment and increased to levels similar to controls after de-submergence. Both CSN4 and CSN5 accumulated following flooding treatment, although no significant difference was observed in proteasome. Low oxygen had no effect on the amount of ubiquitinated proteins or CSN4. By 2D-PAGE, the amount of 6 proteins changed significantly following MG132 treatment in flooding stressed plants. We conclude that the accumulation of CSN proteins might enhance the degradation of ubiquitinated proteins independent of hypoxia caused by flooding, thereby lowering their abundance during flooding stress., (Copyright © 2011 Elsevier Ireland Ltd. All rights reserved.)

Published

2012

24. Critical role of proteostasis-imbalance in pathogenesis of COPD and severe emphysema.

Author

Min T, Bodas M, Mazur S, and Vij N

Subjects

Adenosine Triphosphatases biosynthesis, Adenosine Triphosphatases genetics, Aged, Animals, Apoptosis, Bronchi cytology, Cell Cycle Proteins biosynthesis, Cell Cycle Proteins genetics, Cinnamates pharmacology, Cinnamates therapeutic use, Endopeptidases metabolism, Epithelial Cells, Female, HEK293 Cells, Histone Deacetylase 2 metabolism, Humans, Male, Mice, Middle Aged, NF-E2-Related Factor 2 metabolism, NF-kappa B metabolism, Oxidative Stress, Proteostasis Deficiencies pathology, Pulmonary Disease, Chronic Obstructive pathology, Pulmonary Emphysema pathology, Receptors, Autocrine Motility Factor, Receptors, Cytokine biosynthesis, Receptors, Cytokine genetics, Smoking, Thiourea analogs & derivatives, Thiourea pharmacology, Thiourea therapeutic use, Transcription Factor CHOP biosynthesis, Ubiquitin Thiolesterase metabolism, Ubiquitin-Protein Ligases biosynthesis, Ubiquitin-Protein Ligases genetics, Ubiquitinated Proteins analysis, Valosin Containing Protein, Proteins metabolism, Proteostasis Deficiencies metabolism, Pulmonary Disease, Chronic Obstructive metabolism, Pulmonary Emphysema metabolism

Abstract

The environmental, genetic, and/or age-related changes in proteostasis induce inflammation, oxidative stress, and apoptosis. We quantified the correlation of protein expression of critical proteostasis mediators to severity of chronic lung disease using lung tissue samples from control and chronic obstructive pulmonary disease (COPD) subjects (GOLD stage 0-IV) and cigarette smoke (CS)-induced murine model. The human bronchial epithelial cells, HEK-293, and Beas2B cells were used for in vitro experiments to verify the mechanisms. Our data verifies the correlation of higher expression of valosin-containing protein (VCP) retrograde translocation complex (VCP-Rma1-gp78) with severity of emphysema in COPD lung tissues and over-expression of inflammatory, ER stress and apoptotic mediators like NFκB, GADD-153/CHOP, and p-eIF2α. Moreover, subjects with severe emphysema had a higher accumulation of ubiquitinated proteins and deubiquitinating enzyme, UCHL-1, indicating towards the aggregation of misfolded or damaged proteins. The modulation of both protein degradation and synthesis rates by CS-extract substantiates the pathogenetic role of proteostasis-imbalance in emphysema and COPD. We identified that VCP also mediates proteasomal degradation of HDAC2 and Nrf2, as a potential mechanism for increased oxidative stress and corticosteroid resistance in COPD subjects with emphysema. Next, we confirmed that higher VCP expression associates with increased inflammation and apoptosis using in vitro and murine models. Our data clearly shows aberrant proteostasis in COPD subjects with severe emphysema. In addition, we evaluate therapeutic efficacy of salubrinal (ER stress inhibitor) to correct the proteostasis-imbalance based on its ability to control VCP expression and ubiquitin accumulation. Overall, our data demonstrate for the first time the critical role of proteostasis-imbalance in pathogenesis of severe emphysema.

Published

2011

25. Rapidly progressive diaphragmatic weakness and injury during mechanical ventilation in humans.

Author

Jaber S, Petrof BJ, Jung B, Chanques G, Berthet JP, Rabuel C, Bouyabrine H, Courouble P, Koechlin-Ramonatxo C, Sebbane M, Similowski T, Scheuermann V, Mebazaa A, Capdevila X, Mornet D, Mercier J, Lacampagne A, Philips A, and Matecki S

Subjects

Adult, Calpain analysis, Diaphragm chemistry, Diaphragm pathology, Diaphragm physiopathology, Female, Humans, Male, Middle Aged, Muscle Weakness pathology, Muscle Weakness physiopathology, Muscular Atrophy etiology, Muscular Atrophy pathology, Muscular Atrophy physiopathology, Time Factors, Transcription Factor RelA analysis, Ubiquitinated Proteins analysis, Young Adult, Diaphragm injuries, Muscle Weakness etiology, Respiration, Artificial adverse effects

Abstract

Rationale: Diaphragmatic function is a major determinant of the ability to successfully wean patients from mechanical ventilation (MV). Paradoxically, MV itself results in a rapid loss of diaphragmatic strength in animals. However, very little is known about the time course or mechanistic basis for such a phenomenon in humans., Objectives: To determine in a prospective fashion the time course for development of diaphragmatic weakness during MV; and the relationship between MV duration and diaphragmatic injury or atrophy, and the status of candidate cellular pathways implicated in these phenomena., Methods: Airway occlusion pressure (TwPtr) generated by the diaphragm during phrenic nerve stimulation was measured in short-term (0.5 h; n = 6) and long-term (>5 d; n = 6) MV groups. Diaphragmatic biopsies obtained during thoracic surgery (MV for 2-3 h; n = 10) and from brain-dead organ donors (MV for 24-249 h; n = 15) were analyzed for ultrastructural injury, atrophy, and expression of proteolysis-related proteins (ubiquitin, nuclear factor-κB, and calpains)., Measurements and Main Results: TwPtr decreased progressively during MV, with a mean reduction of 32 ± 6% after 6 days. Longer periods of MV were associated with significantly greater ultrastructural fiber injury (26.2 ± 4.8 vs. 4.7 ± 0.6% area), decreased cross-sectional area of muscle fibers (1,904 ± 220 vs. 3,100 ± 329 μm²), an increase of ubiquitinated proteins (+19%), higher expression of p65 nuclear factor-κB (+77%), and greater levels of the calcium-activated proteases calpain-1, -2, and -3 (+104%, +432%, and +266%, respectively) in the diaphragm., Conclusions: Diaphragmatic weakness, injury, and atrophy occur rapidly in critically ill patients during MV, and are significantly correlated with the duration of ventilator support.

Published

2011

26. Identification, analysis, and prediction of protein ubiquitination sites.

Author

Radivojac P, Vacic V, Haynes C, Cocklin RR, Mohan A, Heyen JW, Goebl MG, and Iakoucheva LM

Subjects

Amino Acid Sequence, Databases, Protein, Endosomal Sorting Complexes Required for Transport metabolism, Humans, Mass Spectrometry, Molecular Sequence Data, Proteome metabolism, Saccharomyces cerevisiae Proteins metabolism, Sequence Analysis, Protein, Ubiquitin-Protein Ligase Complexes metabolism, Ubiquitinated Proteins metabolism, Ubiquitination, Proteome analysis, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins analysis, Ubiquitinated Proteins analysis

Abstract

Ubiquitination plays an important role in many cellular processes and is implicated in many diseases. Experimental identification of ubiquitination sites is challenging due to rapid turnover of ubiquitinated proteins and the large size of the ubiquitin modifier. We identified 141 new ubiquitination sites using a combination of liquid chromatography, mass spectrometry, and mutant yeast strains. Investigation of the sequence biases and structural preferences around known ubiquitination sites indicated that their properties were similar to those of intrinsically disordered protein regions. Using a combined set of new and previously known ubiquitination sites, we developed a random forest predictor of ubiquitination sites, UbPred. The class-balanced accuracy of UbPred reached 72%, with the area under the ROC curve at 80%. The application of UbPred showed that high confidence Rsp5 ubiquitin ligase substrates and proteins with very short half-lives were significantly enriched in the number of predicted ubiquitination sites. Proteome-wide prediction of ubiquitination sites in Saccharomyces cerevisiae indicated that highly ubiquitinated substrates were prevalent among transcription/enzyme regulators and proteins involved in cell cycle control. In the human proteome, cytoskeletal, cell cycle, regulatory, and cancer-associated proteins display higher extent of ubiquitination than proteins from other functional categories. We show that gain and loss of predicted ubiquitination sites may likely represent a molecular mechanism behind a number of disease-associatedmutations. UbPred is available at http://www.ubpred.org., ((c) 2009 Wiley-Liss, Inc.)

Published

2010

27. Ubiquitin-positive foam cells are identified in the aortic and mitral valves with atherosclerotic involvement.

Author

Yamada T, Satoh S, Sueyoshi S, Mitsumata M, Matsumoto T, Ueno T, Uehara K, and Mizutani T

Subjects

Adult, Aged, Aged, 80 and over, Aortic Valve chemistry, Apoptosis, Calcinosis, Female, Fibrosis, Foam Cells pathology, Humans, Male, Middle Aged, Mitral Valve chemistry, Proteasome Endopeptidase Complex, Severity of Illness Index, Ubiquitinated Proteins analysis, Aortic Valve pathology, Atherosclerosis pathology, Foam Cells chemistry, Mitral Valve pathology, Ubiquitin analysis

Abstract

Aim: Our aim was to determine the roles of the ubiquitin (Ub)-proteasome system (UPS) in valvular diseases by immunohistochemically identifying Ub-positive cells in aortic and mitral valves and determining if Ub+cells were associated with the severity of valvular diseases., Methods: We evaluated surgically removed aortic and mitral valves from 60 patients (mean age, 64.5 years) for thickening, fibrosis, foam cell infiltration, thrombus, and atheromatous plaques by using grading scores. U+cells were detected immunohistochemically., Results: We found Ub+cells in 16 (26.7%) of the 60 patients. Eleven (28.2%) of the 39 aortic valves and 5 (23.8%) of the 21 mitral valves were Ub-positive. Ub was found with granular depositions in the cytoplasm of monocyte-derived foam cells that were CD68+. The aortic valvular thickness of the Ub+group was significantly greater than that of the Ub- group (3.9+/-1.6mm vs. 3.2+/-1.6mm, p<0.05). Foam cells and fibrosis were greater in the Ub+group (p<0.05), and calcifications were prominent in aortic valves. There was no difference in the number of apoptotic cells in Ub+ and Ub- groups. Ub+cells were present in the affected valves and ubiquitinated proteins were accumulated in macrophage-derived foam cells., Conclusions: Ub+ foam cells are present in valves that are vulnerable to valvular disease, and UPS may contribute to the development of atherosclerosis through the inflammatory process.

Published

2009