Chancellery Research - Research Publications

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Author: Corbett, Alexandra × End date: 2019 × Start date: 2017 ×

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    IL-23 costimulates antigen-specific MAIT cell activation and enables vaccination against bacterial infection
    Wang, H ; Kjer-Nielsen, L ; Shi, M ; D'Souza, C ; Pediongco, TJ ; Cao, H ; Kostenko, L ; Lim, XY ; Eckle, SBG ; Meehan, BS ; Zhu, T ; Wang, B ; Zhao, Z ; Mak, JYW ; Fairlie, DP ; Teng, MWL ; Rossjohn, J ; Yu, D ; de St Groth, BF ; Lovrecz, G ; Lu, L ; McCluskey, J ; Strugnell, RA ; Corbett, AJ ; Chen, Z (AMER ASSOC ADVANCEMENT SCIENCE, 2019-11-01)
    Mucosal-associated invariant T (MAIT) cells are activated in a TCR-dependent manner by antigens derived from the riboflavin synthesis pathway, including 5-(2-oxopropylideneamino)-6-D-ribitylaminouracil (5-OP-RU), bound to MHC-related protein-1 (MR1). However, MAIT cell activation in vivo has not been studied in detail. Here, we have found and characterized additional molecular signals required for optimal activation and expansion of MAIT cells after pulmonary Legionella or Salmonella infection in mice. We show that either bone marrow–derived APCs or non–bone marrow–derived cells can activate MAIT cells in vivo, depending on the pathogen. Optimal MAIT cell activation in vivo requires signaling through the inducible T cell costimulator (ICOS), which is highly expressed on MAIT cells. Subsequent expansion and maintenance of MAIT-17/1-type responses are dependent on IL-23. Vaccination with IL-23 plus 5-OP-RU augments MAIT cell–mediated control of pulmonary Legionella infection. These findings reveal cellular and molecular targets for manipulating MAIT cell function under physiological conditions.
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    Drugs and drug-like molecules can modulate the function of mucosal-associated invariant T cells
    Keller, AN ; Eckle, SBG ; Xu, W ; Liu, L ; Hughes, VA ; Mak, JYW ; Meehan, BS ; Pediongco, T ; Birkinshaw, RW ; Chen, Z ; Wang, H ; D'Souza, C ; Kjer-Nielsen, L ; Gherardin, NA ; Godfrey, DI ; Kostenko, L ; Corbett, AJ ; Purcell, AW ; Fairlie, DP ; McCluskey, J ; Rossjohn, J (NATURE PUBLISHING GROUP, 2017-04)
    The major-histocompatibility-complex-(MHC)-class-I-related molecule MR1 can present activating and non-activating vitamin-B-based ligands to mucosal-associated invariant T cells (MAIT cells). Whether MR1 binds other ligands is unknown. Here we identified a range of small organic molecules, drugs, drug metabolites and drug-like molecules, including salicylates and diclofenac, as MR1-binding ligands. Some of these ligands inhibited MAIT cells ex vivo and in vivo, while others, including diclofenac metabolites, were agonists. Crystal structures of a T cell antigen receptor (TCR) from a MAIT cell in complex with MR1 bound to the non-stimulatory and stimulatory compounds showed distinct ligand orientations and contacts within MR1, which highlighted the versatility of the MR1 binding pocket. The findings demonstrated that MR1 was able to capture chemically diverse structures, spanning mono- and bicyclic compounds, that either inhibited or activated MAIT cells. This indicated that drugs and drug-like molecules can modulate MAIT cell function in mammals.
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    Guidelines for the use of flow cytometry and cell sorting in immunological studies (second edition)
    Cossarizza, A ; Chang, H-D ; Radbruch, A ; Acs, A ; Adam, D ; Adam-Klages, S ; Agace, WW ; Aghaeepour, N ; Akdis, M ; Allez, M ; Almeida, LN ; Alvisi, G ; Anderson, G ; Andrae, I ; Annunziato, F ; Anselmo, A ; Bacher, P ; Baldari, CT ; Bari, S ; Barnaba, V ; Barros-Martins, J ; Battistini, L ; Bauer, W ; Baumgart, S ; Baumgarth, N ; Baumjohann, D ; Baying, B ; Bebawy, M ; Becher, B ; Beisker, W ; Benes, V ; Beyaert, R ; Blanco, A ; Boardman, DA ; Bogdan, C ; Borger, JG ; Borsellino, G ; Boulais, PE ; Bradford, JA ; Brenner, D ; Brinkman, RR ; Brooks, AES ; Busch, DH ; Buescher, M ; Bushnell, TP ; Calzetti, F ; Cameron, G ; Cammarata, I ; Cao, X ; Cardell, SL ; Casola, S ; Cassatella, MA ; Cavani, A ; Celada, A ; Chatenoud, L ; Chattopadhyay, PK ; Chow, S ; Christakou, E ; Cicin-Sain, L ; Clerici, M ; Colombo, FS ; Cook, L ; Cooke, A ; Cooper, AM ; Corbett, AJ ; Cosma, A ; Cosmi, L ; Coulie, PG ; Cumano, A ; Cvetkovic, L ; Dang, VD ; Dang-Heine, C ; Davey, MS ; Davies, D ; De Biasi, S ; Del Zotto, G ; Dela Cruz, GV ; Delacher, M ; Della Bella, S ; Dellabona, P ; Deniz, G ; Dessing, M ; Di Santo, JP ; Diefenbach, A ; Dieli, F ; Dolf, A ; Doerner, T ; Dress, RJ ; Dudziak, D ; Dustin, M ; Dutertre, C-A ; Ebner, F ; Eckle, SBG ; Edinger, M ; Eede, P ; Ehrhardt, GRA ; Eich, M ; Engel, P ; Engelhardt, B ; Erdei, A ; Esser, C ; Everts, B ; Evrard, M ; Falk, CS ; Fehniger, TA ; Felipo-Benavent, M ; Ferry, H ; Feuerer, M ; Filby, A ; Filkor, K ; Fillatreau, S ; Follo, M ; Foerster, I ; Foster, J ; Foulds, GA ; Frehse, B ; Frenette, PS ; Frischbutter, S ; Fritzsche, W ; Galbraith, DW ; Gangaev, A ; Garbi, N ; Gaudilliere, B ; Gazzinelli, RT ; Geginat, J ; Gerner, W ; Gherardin, NA ; Ghoreschi, K ; Gibellini, L ; Ginhoux, F ; Goda, K ; Godfrey, DI ; Goettlinger, C ; Gonzalez-Navajas, JM ; Goodyear, CS ; Gori, A ; Grogan, JL ; Grummitt, D ; Gruetzkau, A ; Haftmann, C ; Hahn, J ; Hammad, H ; Haemmerling, G ; Hansmann, L ; Hansson, G ; Harpur, CM ; Hartmann, S ; Hauser, A ; Hauser, AE ; Haviland, DL ; Hedley, D ; Hernandez, DC ; Herrera, G ; Herrmann, M ; Hess, C ; Hoefer, T ; Hoffmann, P ; Hogquist, K ; Holland, T ; Hollt, T ; Holmdahl, R ; Hombrink, P ; Houston, JP ; Hoyer, BF ; Huang, B ; Huang, F-P ; Huber, JE ; Huehn, J ; Hundemer, M ; Hunter, CA ; Hwang, WYK ; Iannone, A ; Ingelfinger, F ; Ivison, SM ; Jaeck, H-M ; Jani, PK ; Javega, B ; Jonjic, S ; Kaiser, T ; Kalina, T ; Kamradt, T ; Kaufmann, SHE ; Keller, B ; Ketelaars, SLC ; Khalilnezhad, A ; Khan, S ; Kisielow, J ; Klenerman, P ; Knopf, J ; Koay, H-F ; Kobow, K ; Kolls, JK ; Kong, WT ; Kopf, M ; Korn, T ; Kriegsmann, K ; Kristyanto, H ; Kroneis, T ; Krueger, A ; Kuehne, J ; Kukat, C ; Kunkel, D ; Kunze-Schumacher, H ; Kurosaki, T ; Kurts, C ; Kvistborg, P ; Kwok, I ; Landry, J ; Lantz, O ; Lanuti, P ; LaRosa, F ; Lehuen, A ; LeibundGut-Landmann, S ; Leipold, MD ; Leung, LYT ; Levings, MK ; Lino, AC ; Liotta, F ; Litwin, V ; Liu, Y ; Ljunggren, H-G ; Lohoff, M ; Lombardi, G ; Lopez, L ; Lopez-Botet, M ; Lovett-Racke, AE ; Lubberts, E ; Luche, H ; Ludewig, B ; Lugli, E ; Lunemann, S ; Maecker, HT ; Maggi, L ; Maguire, O ; Mair, F ; Mair, KH ; Mantovani, A ; Manz, RA ; Marshall, AJ ; Martinez-Romero, A ; Martrus, G ; Marventano, I ; Maslinski, W ; Matarese, G ; Mattioli, AV ; Maueroder, C ; Mazzoni, A ; McCluskey, J ; McGrath, M ; McGuire, HM ; McInnes, IB ; Mei, HE ; Melchers, F ; Melzer, S ; Mielenz, D ; Miller, SD ; Mills, KHG ; Minderman, H ; Mjosberg, J ; Moore, J ; Moran, B ; Moretta, L ; Mosmann, TR ; Mueller, S ; Multhoff, G ; Munoz, LE ; Munz, C ; Nakayama, T ; Nasi, M ; Neumann, K ; Ng, LG ; Niedobitek, A ; Nourshargh, S ; Nunez, G ; O'Connor, J-E ; Ochel, A ; Oja, A ; Ordonez, D ; Orfao, A ; Orlowski-Oliver, E ; Ouyang, W ; Oxenius, A ; Palankar, R ; Panse, I ; Pattanapanyasat, K ; Paulsen, M ; Pavlinic, D ; Penter, L ; Peterson, P ; Peth, C ; Petriz, J ; Piancone, F ; Pickl, WF ; Piconese, S ; Pinti, M ; Pockley, AG ; Podolska, MJ ; Poon, Z ; Pracht, K ; Prinz, I ; Pucillo, CEM ; Quataert, SA ; Quatrini, L ; Quinn, KM ; Radbruch, H ; Radstake, TRDJ ; Rahmig, S ; Rahn, H-P ; Rajwa, B ; Ravichandran, G ; Raz, Y ; Rebhahn, JA ; Recktenwald, D ; Reimer, D ; Reis e Sousa, C ; Remmerswaal, EBM ; Richter, L ; Rico, LG ; Riddell, A ; Rieger, AM ; Robinson, JP ; Romagnani, C ; Rubartelli, A ; Ruland, J ; Saalmueller, A ; Saeys, Y ; Saito, T ; Sakaguchi, S ; Sala-de-Oyanguren, F ; Samstag, Y ; Sanderson, S ; Sandrock, I ; Santoni, A ; Sanz, RB ; Saresella, M ; Sautes-Fridman, C ; Sawitzki, B ; Schadt, L ; Scheffold, A ; Scherer, HU ; Schiemann, M ; Schildberg, FA ; Schimisky, E ; Schlitzer, A ; Schlosser, J ; Schmid, S ; Schmitt, S ; Schober, K ; Schraivogel, D ; Schuh, W ; Schueler, T ; Schulte, R ; Schulz, AR ; Schulz, SR ; Scotta, C ; Scott-Algara, D ; Sester, DP ; Shankey, TV ; Silva-Santos, B ; Simon, AK ; Sitnik, KM ; Sozzani, S ; Speiser, DE ; Spidlen, J ; Stahlberg, A ; Stall, AM ; Stanley, N ; Stark, R ; Stehle, C ; Steinmetz, T ; Stockinger, H ; Takahama, Y ; Takeda, K ; Tan, L ; Tarnok, A ; Tiegs, G ; Toldi, G ; Tornack, J ; Traggiai, E ; Trebak, M ; Tree, TIM ; Trotter, J ; Trowsdale, J ; Tsoumakidou, M ; Ulrich, H ; Urbanczyk, S ; van de Veen, W ; van den Broek, M ; van der Pol, E ; Van Gassen, S ; Van Isterdael, G ; van Lier, RAW ; Veldhoen, M ; Vento-Asturias, S ; Vieira, P ; Voehringer, D ; Volk, H-D ; von Borstel, A ; von Volkmann, K ; Waisman, A ; Walker, RV ; Wallace, PK ; Wang, SA ; Wang, XM ; Ward, MD ; Ward-Hartstonge, KA ; Warnatz, K ; Warnes, G ; Warth, S ; Waskow, C ; Watson, JV ; Watzl, C ; Wegener, L ; Weisenburger, T ; Wiedemann, A ; Wienands, J ; Wilharm, A ; Wilkinson, RJ ; Willimsky, G ; Wing, JB ; Winkelmann, R ; Winkler, TH ; Wirz, OF ; Wong, A ; Wurst, P ; Yang, JHM ; Yang, J ; Yazdanbakhsh, M ; Yu, L ; Yue, A ; Zhang, H ; Zhao, Y ; Ziegler, SM ; Zielinski, C ; Zimmermann, J ; Zychlinsky, A (WILEY, 2019-10)
    These guidelines are a consensus work of a considerable number of members of the immunology and flow cytometry community. They provide the theory and key practical aspects of flow cytometry enabling immunologists to avoid the common errors that often undermine immunological data. Notably, there are comprehensive sections of all major immune cell types with helpful Tables detailing phenotypes in murine and human cells. The latest flow cytometry techniques and applications are also described, featuring examples of the data that can be generated and, importantly, how the data can be analysed. Furthermore, there are sections detailing tips, tricks and pitfalls to avoid, all written and peer-reviewed by leading experts in the field, making this an essential research companion.
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    An overview on the identification of MAIT cell antigens
    Kjer-Nielsen, L ; Corbett, AJ ; Chen, Z ; Liu, L ; Mak, JYW ; Godfrey, DI ; Rossjohn, J ; Fairlie, DP ; McCluskey, J ; Eckle, SBG (WILEY, 2018-07)
    Mucosal associated invariant T (MAIT) cells are restricted by the monomorphic MHC class I-like molecule, MHC-related protein-1 (MR1). Until 2012, the origin of the MAIT cell antigens (Ags) was unknown, although it was established that MAIT cells could be activated by a broad range of bacteria and yeasts, possibly suggesting a conserved Ag. Using a combination of protein chemistry, mass spectrometry, cellular biology, structural biology and small molecule chemistry, we discovered MR1 ligands derived from folic acid (vitamin B9) and from an intermediate in the microbial biosynthesis of riboflavin (vitamin B2). While the folate derivative 6-formylpterin generally inhibited MAIT cell activation, two riboflavin pathway derivatives, 5-(2-oxopropylideneamino)-6-D-ribitylaminouracil and 5-(2-oxoethylideneamino)-6-D-ribitylaminouracil, were potent MAIT cell agonists. Other intermediates and derivatives of riboflavin synthesis displayed weak or no MAIT cell activation. Collectively, these studies revealed that in addition to peptide and lipid-based Ags, small molecule natural product metabolites are also ligands that can activate T cells expressing αβ T-cell receptors, and here we recount this discovery.
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    MAIT cells protect against pulmonary Legionella longbeachae infection
    Wang, H ; D'Souza, C ; Lim, XY ; Kostenko, L ; Pediongco, TJ ; Eckle, SBG ; Meehan, BS ; Shi, M ; Wang, N ; Li, S ; Liu, L ; Mak, JYW ; Fairlie, DP ; Iwakura, Y ; Gunnersen, JM ; Stent, AW ; Godfrey, DI ; Rossjohn, J ; Westall, GP ; Kjer-Nielsen, L ; Strugnell, RA ; McCluskey, J ; Corbett, AJ ; Hinks, TSC ; Chen, Z (NATURE RESEARCH, 2018-08-22)
    Mucosal associated invariant T (MAIT) cells recognise conserved microbial metabolites from riboflavin synthesis. Striking evolutionary conservation and pulmonary abundance implicate them in antibacterial host defence, yet their functions in protection against clinically important pathogens are unknown. Here we show that mouse Legionella longbeachae infection induces MR1-dependent MAIT cell activation and rapid pulmonary accumulation of MAIT cells associated with immune protection detectable in immunocompetent host animals. MAIT cell protection is more evident in mice lacking CD4+ cells, and adoptive transfer of MAIT cells rescues immunodeficient Rag2-/-γC-/- mice from lethal Legionella infection. Protection is dependent on MR1, IFN-γ and GM-CSF, but not IL-17A, TNF or perforin, and enhanced protection is detected earlier after infection of mice antigen-primed to boost MAIT cell numbers before infection. Our findings define a function for MAIT cells in protection against a major human pathogen and indicate a potential role for vaccination to enhance MAIT cell immunity.
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    MAIT cells contribute to protection against lethal influenza infection in vivo
    van Wilgenburg, B ; Loh, L ; Chen, Z ; Pediongco, TJ ; Wang, H ; Shi, M ; Zhao, Z ; Koutsakos, M ; Nussing, S ; Sant, S ; Wang, Z ; D'Souza, C ; Jia, X ; Almeida, CF ; Kostenko, L ; Eckle, SBG ; Meehan, BS ; Kallies, A ; Godfrey, DI ; Reading, PC ; Corbett, AJ ; McCluskey, J ; Klenerman, P ; Kedzierska, K ; Hinks, TSC (NATURE PUBLISHING GROUP, 2018-11-09)
    Mucosal associated invariant T (MAIT) cells are evolutionarily-conserved, innate-like lymphocytes which are abundant in human lungs and can contribute to protection against pulmonary bacterial infection. MAIT cells are also activated during human viral infections, yet it remains unknown whether MAIT cells play a significant protective or even detrimental role during viral infections in vivo. Using murine experimental challenge with two strains of influenza A virus, we show that MAIT cells accumulate and are activated early in infection, with upregulation of CD25, CD69 and Granzyme B, peaking at 5 days post-infection. Activation is modulated via cytokines independently of MR1. MAIT cell-deficient MR1-/- mice show enhanced weight loss and mortality to severe (H1N1) influenza. This is ameliorated by prior adoptive transfer of pulmonary MAIT cells in both immunocompetent and immunodeficient RAG2-/-γC-/- mice. Thus, MAIT cells contribute to protection during respiratory viral infections, and constitute a potential target for therapeutic manipulation.
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    Stabilizing short-lived Schiff base derivatives of 5-aminouracils that activate mucosal-associated invariant T cells
    Mak, JYW ; Xu, W ; Reid, RC ; Corbett, AJ ; Meehan, BS ; Wang, H ; Chen, Z ; Rossjohn, J ; McCluskey, J ; Liu, L ; Fairlie, DP (NATURE PUBLISHING GROUP, 2017-03-08)
    Mucosal-associated invariant T (MAIT) cells are activated by unstable antigens formed by reactions of 5-amino-6-D-ribitylaminouracil (a vitamin B2 biosynthetic intermediate) with glycolysis metabolites such as methylglyoxal. Here we show superior preparations of antigens in dimethylsulfoxide, avoiding their rapid decomposition in water (t1/2 1.5 h, 37 °C). Antigen solution structures, MAIT cell activation potencies (EC50 3-500 pM), and chemical stabilities are described. Computer analyses of antigen structures reveal stereochemical and energetic influences on MAIT cell activation, enabling design of a water stable synthetic antigen (EC50 2 nM). Like native antigens, this antigen preparation induces MR1 refolding and upregulates surface expression of human MR1, forms MR1 tetramers that detect MAIT cells in human PBMCs, and stimulates cytokine expression (IFNγ, TNF) by human MAIT cells. These antigens also induce MAIT cell accumulation in mouse lungs after administration with a co-stimulant. These chemical and immunological findings provide new insights into antigen properties and MAIT cell activation.
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    MAIT cells launch a rapid, robust and distinct hyperinflammatory response to bacterial superantigens and quickly acquire an anergic phenotype that impedes their cognate antimicrobial function: Defining a novel mechanism of superantigen-induced immunopathology and immunosuppression
    Shaler, CR ; Choi, J ; Rudak, PT ; Memarnejadian, A ; Szabo, PA ; Tun-Abraham, ME ; Rossjohn, J ; Corbett, AJ ; McCluskey, J ; McCormick, JK ; Lantz, O ; Hernandez-Alejandro, R ; Haeryfar, SMM ; Bhandoola, A (PUBLIC LIBRARY SCIENCE, 2017-06)
    Superantigens (SAgs) are potent exotoxins secreted by Staphylococcus aureus and Streptococcus pyogenes. They target a large fraction of T cell pools to set in motion a "cytokine storm" with severe and sometimes life-threatening consequences typically encountered in toxic shock syndrome (TSS). Given the rapidity with which TSS develops, designing timely and truly targeted therapies for this syndrome requires identification of key mediators of the cytokine storm's initial wave. Equally important, early host responses to SAgs can be accompanied or followed by a state of immunosuppression, which in turn jeopardizes the host's ability to combat and clear infections. Unlike in mouse models, the mechanisms underlying SAg-associated immunosuppression in humans are ill-defined. In this work, we have identified a population of innate-like T cells, called mucosa-associated invariant T (MAIT) cells, as the most powerful source of pro-inflammatory cytokines after exposure to SAgs. We have utilized primary human peripheral blood and hepatic mononuclear cells, mouse MAIT hybridoma lines, HLA-DR4-transgenic mice, MAIThighHLA-DR4+ bone marrow chimeras, and humanized NOD-scid IL-2Rγnull mice to demonstrate for the first time that: i) mouse and human MAIT cells are hyperresponsive to SAgs, typified by staphylococcal enterotoxin B (SEB); ii) the human MAIT cell response to SEB is rapid and far greater in magnitude than that launched by unfractionated conventional T, invariant natural killer T (iNKT) or γδ T cells, and is characterized by production of interferon (IFN)-γ, tumor necrosis factor (TNF)-α and interleukin (IL)-2, but not IL-17A; iii) high-affinity MHC class II interaction with SAgs, but not MHC-related protein 1 (MR1) participation, is required for MAIT cell activation; iv) MAIT cell responses to SEB can occur in a T cell receptor (TCR) Vβ-specific manner but are largely contributed by IL-12 and IL-18; v) as MAIT cells are primed by SAgs, they also begin to develop a molecular signature consistent with exhaustion and failure to participate in antimicrobial defense. Accordingly, they upregulate lymphocyte-activation gene 3 (LAG-3), T cell immunoglobulin and mucin-3 (TIM-3), and/or programmed cell death-1 (PD-1), and acquire an anergic phenotype that interferes with their cognate function against Klebsiella pneumoniae and Escherichia coli; vi) MAIT cell hyperactivation and anergy co-utilize a signaling pathway that is governed by p38 and MEK1/2. Collectively, our findings demonstrate a pathogenic, rather than protective, role for MAIT cells during infection. Furthermore, we propose a novel mechanism of SAg-associated immunosuppression in humans. MAIT cells may therefore provide an attractive therapeutic target for the management of both early and late phases of severe SAg-mediated illnesses.