A Robust Method for Quantitative High-throughput Analysis of Proteomes by 18O Labeling

Bonzón-Kulichenko, Elena; Pérez-Hernández, Daniel; Núñez, Estefanía; Martínez-Acedo, Pablo; Navarro, Pedro J.; Trevisán-Herraz, Marco; Ramos, María C.; Sierra, Saleta; Martı́nez-Martı́nez, Sara; Ruiz‐Meana, Marisol; Miró-Casas, Elizabeth; Garcı́a-Dorado, David; Redondo, Juan Miguel; Burgos, Javier S.; Vázquez, Jesús

doi:10.1074/mcp.m110.003335

Cited by 87 publications

(136 citation statements)

References 55 publications

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“…After 5 washes with lysis buffer, the beads were resuspended in Laemmli buffer and resolved by SDS-PAGE. After staining with Coomassie blue, gel samples were digested in gel with trypsin, and the resulting peptides were identified by mass spectrometry (MS) as described previously (23). Selected tandem MS (MS/MS) ion monitoring was performed as described previously (24).…”

Section: Methodsmentioning

confidence: 99%

The Leukocyte Activation Receptor CD69 Controls T Cell Differentiation through Its Interaction with Galectin-1

Fuente

Cruz-Adalia

Martín

et al. 2014

Molecular and Cellular Biology

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f CD69 is involved in immune cell homeostasis, regulating the T cell-mediated immune response through the control of Th17 cell differentiation. However, natural ligands for CD69 have not yet been described. Using recombinant fusion proteins containing the extracellular domain of CD69, we have detected the presence of a ligand(s) for CD69 on human dendritic cells (DCs). Pulldown followed by mass spectrometry analyses of CD69-binding moieties on DCs identified galectin-1 as a CD69 counterreceptor. Surface plasmon resonance and anti-CD69 blocking analyses demonstrated a direct and specific interaction between CD69 and galectin-1 that was carbohydrate dependent. Functional assays with both human and mouse T cells demonstrated the role of CD69 in the negative effect of galectin-1 on Th17 differentiation. Our findings identify CD69 and galectin-1 to be a novel regulatory receptor-ligand pair that modulates Th17 effector cell differentiation and function. C D69, a C-type lectin, is a member of the natural killer (NK) receptor family and is induced early following activation of leukocytes (1). The physiological role of this receptor, which is persistently expressed by infiltrating leukocytes in different chronic inflammatory diseases, has been studied in CD69-deficient mice in multiple different models of chronic inflammation (2-5). Thus, we have previously described that CD69 Ϫ/Ϫ mice develop an exacerbated form of collagen-induced arthritis (CIA) (3), a Th1 and Th17 cell-mediated autoimmune condition. Moreover, in an experimental model of autoimmune myocarditis (EAM), CD69 negatively regulates cardiac inflammation through the regulation of heart-specific Th17 responses (4). In this regard, we have detected that CD69 modulates the in vitro differentiation of T cells toward the Th17 lineage through the activation of the Jak3/Stat5 inhibitory pathway (5). On the other hand, CD69 negatively regulates the chemotactic responses of effector lymphocytes and dendritic cells (DCs) to sphingosine 1 phosphate (S1P); CD69 can associate with S1P1 in the cell membrane and induce a conformation of S1P1 that favors its internalization and degradation (6-8). It is clear that the identification of cellular ligands for CD69 is a critical next step to better understand the physiological role of this receptor.Galectins are characterized by a common structural fold and a conserved carbohydrate recognition domain (CRD) with a high affinity for beta-galactosides (9). Despite being soluble proteins, galectins are also expressed on the cell surface due to their association with membrane glycoproteins. Thus, galectin-1 (Gal-1) is expressed by most activated but not resting T and B cells, and it is significantly upregulated in activated macrophages and T regulatory lymphocytes (10). In addition, tolerogenic DCs show a high expression of Gal-1 (11), which is rapidly downregulated in response to maturation signals. Furthermore, Gal-1-deficient DCs show a greater immunogenic potential and an impaired ability to halt the inflammatory phenomenon in a ...

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Section: Methodsmentioning

confidence: 99%

The Leukocyte Activation Receptor CD69 Controls T Cell Differentiation through Its Interaction with Galectin-1

Fuente

Cruz-Adalia

Martín

et al. 2014

Molecular and Cellular Biology

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“…SIGMA ProteoPrep20) to remove some of the most abundant plasma proteins (91), or protein equalizer technology like combinatorial peptide ligand library (BioRad ProteoMiner) (77 ,92);; sometimes the two technologies are used to allow enrichment of proteins in biological fluids for in-depth proteomic analysis (11).…”

Section: Culture Media and Sample Preparationmentioning

confidence: 99%

Redox Proteomics Applied to the Thiol Secretome

Ghezzi

Chan

2017

Antioxidants & Redox Signaling

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Word count: 6800 excluding references Number of references: 113Number of greyscale and color illustrations: 7 greyscale and 5 color (online only)Ghezzi 2 AbstractStudies of redox proteomics to identify glutathionylated proteins have so far been focused on intracellular proteins. However, plasma proteins have been described as glutathionylated. The present review discusses the redox state of protein cysteines in relation to their cellular distribution. We focus in particular on the redox state of proteins secreted under inflammatory conditions and that may act as soluble mediators (cytokines). We describe the various approaches used to detect secreted glutathionylated proteins, the only thiol modification studied so far in secreted proteins, and the specific problems presented in the study of the secretome. This review will deal with a particular aspect of redox proteomics, the analysis of secreted proteins and their possible function. Ghezzi 3 Redox state of proteins in the context of their localization Redox proteomics of the thiol proteomeAccording to the Oxford English Dictionary, proteomics is "the study or analysis of the set of proteins expressed by an organism" and we commonly apply the term to high-throughput techniques of protein identification. As such, the history of redox proteomics started in 2002 when various groups published the first reports of the identification of oxidized proteins by modifying the existing proteomic techniques.Two of these papers were aimed at carbonylated proteins (19,20) and others at protein glutathionylation (33,37,61) or overall protein thiol oxidation (60) .This review will deal with the redox states of protein thiols. Biochemistry textbooks and protein databases classify cysteines in proteins as either free or engaged in a disulfide bond. However, "free" cysteines can be reversibly or irreversibly oxidized to various forms. In particular, in addition to forming structural disulfides, cysteines can form transient, reversible disulfides with another protein cysteine, with free cysteine (cysteinylation) or with the cysteine in the tripeptide glutathione (GSH;; glutamylcystenyl-glycine). Fig. 1 lists the most important oxidation state of sulfur in cysteine.These forms of oxidation, due to their reversibility, are of great interest in the context of redox regulation, as a means by which the redox state of the cell can regulate protein functions (43-45).Specific proteins undergoing glutathionylation were described even before the term "proteomics" became popular (in the late 1990s, according to Google books ngram viewer -https://books.google.com/ngrams). Two proteins have been identified as undergoing glutathionylation in two separate papers, an unidentified 30 kDa cytosolic Ghezzi 4protein in oxidant-treated rat liver (79), and actin in human neutrophils during oxidative burst (22). Although these were not the result of high-throughput studies, some of the technologies used were then adapted for two-dimensional gels for further studies and are at the basis of current red...

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“…Sepharose beads coming from the pull-down assays were directly resuspended in Laemmli buffer, applied onto a SDS-PAGE gel, and subjected to the one-step in-gel trypsin digestion method (46). The resulting peptides were analyzed by LC-MS/MS using a Surveyor LC system coupled to an LTQ linear ion trap mass spectrometer (Thermo-Fisher, San Jose, CA) as previously described (47,48).…”

Section: Mass Spectrometrymentioning

confidence: 99%

EWI-2 Association with α-Actinin Regulates T Cell Immune Synapses and HIV Viral Infection

Gordon-Alonso

Sala-Valdés

Rocha-Perugini

et al. 2012

The Journal of Immunology

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EWI motif-containing protein 2 (EWI-2) is a member of the Ig superfamily that links tetraspanin-enriched microdomains to the actin cytoskeleton. We found that EWI-2 colocalizes with CD3 and CD81 at the central supramolecular activation cluster of the T cell immune synapse. Silencing of the endogenous expression or overexpression of a cytoplasmic truncated mutant of EWI-2 in T cells increases IL-2 secretion upon Ag stimulation. Mass spectrometry experiments of pull-downs with the C-term intracellular domain of EWI-2 revealed the specific association of EWI-2 with the actin-binding protein α-actinin; this association was regulated by PIP2. α-Actinin regulates the immune synapse formation and is required for efficient T cell activation. We extended these observations to virological synapses induced by HIV and found that silencing of either EWI-2 or α-actinin-4 increased cell infectivity. Our data suggest that the EWI-2–α-actinin complex is involved in the regulation of the actin cytoskeleton at T cell immune and virological synapses, providing a link between membrane microdomains and the formation of polarized membrane structures involved in T cell recognition.

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A Robust Method for Quantitative High-throughput Analysis of Proteomes by 18O Labeling

Cited by 87 publications

References 55 publications

The Leukocyte Activation Receptor CD69 Controls T Cell Differentiation through Its Interaction with Galectin-1

The Leukocyte Activation Receptor CD69 Controls T Cell Differentiation through Its Interaction with Galectin-1

Redox Proteomics Applied to the Thiol Secretome

EWI-2 Association with α-Actinin Regulates T Cell Immune Synapses and HIV Viral Infection

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