Microbiology & Immunology - Research Publications

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Author: Godfrey, Dale × Start date: 2010 × End date: 2019 ×

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    Powdery mildew fungal effector candidates share N-terminal Y/F/WxC-motif.
    Godfrey, D ; Böhlenius, H ; Pedersen, C ; Zhang, Z ; Emmersen, J ; Thordal-Christensen, H (Springer Science and Business Media LLC, 2010-05-20)
    BACKGROUND: Powdery mildew and rust fungi are widespread, serious pathogens that depend on developing haustoria in the living plant cells. Haustoria are separated from the host cytoplasm by a plant cell-derived extrahaustorial membrane. They secrete effector proteins, some of which are subsequently transferred across this membrane to the plant cell to suppress defense. RESULTS: In a cDNA library from barley epidermis containing powdery mildew haustoria, two-thirds of the sequenced ESTs were fungal and represented approximately 3,000 genes. Many of the most highly expressed genes encoded small proteins with N-terminal signal peptides. While these proteins are novel and poorly related, they do share a three-amino acid motif, which we named "Y/F/WxC", in the N-terminal of the mature proteins. The first amino acid of this motif is aromatic: tyrosine, phenylalanine or tryptophan, and the last is always cysteine. In total, we identified 107 such proteins, for which the ESTs represent 19% of the fungal clones in our library, suggesting fundamental roles in haustoria function. While overall sequence similarity between the powdery mildew Y/F/WxC-proteins is low, they do have a highly similar exon-intron structure, suggesting they have a common origin. Interestingly, searches of public fungal genome and EST databases revealed that haustoria-producing rust fungi also encode large numbers of novel, short proteins with signal peptides and the Y/F/WxC-motif. No significant numbers of such proteins were identified from genome and EST sequences from either fungi which do not produce haustoria or from haustoria-producing Oomycetes. CONCLUSION: In total, we identified 107, 178 and 57 such Y/F/WxC-proteins from the barley powdery mildew, the wheat stem rust and the wheat leaf rust fungi, respectively. All together, our findings suggest the Y/F/WxC-proteins to be a new class of effectors from haustoria-producing pathogenic fungi.
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    A non-canonical function of Ezh2 preserves immune homeostasis
    Vasanthakumar, A ; Xu, D ; Lun, ATL ; Kueh, AJ ; van Gisbergen, KPJM ; Iannarella, N ; Li, X ; Yu, L ; Wang, D ; Williams, BRG ; Lee, SCW ; Majewski, IJ ; Godfrey, DI ; Smyth, GK ; Alexander, WS ; Herold, MJ ; Kallies, A ; Nutt, SL ; Allan, RS (WILEY, 2017-04)
    Enhancer of zeste 2 (Ezh2) mainly methylates lysine 27 of histone-H3 (H3K27me3) as part of the polycomb repressive complex 2 (PRC2) together with Suz12 and Eed. However, Ezh2 can also modify non-histone substrates, although it is unclear whether this mechanism has a role during development. Here, we present evidence for a chromatin-independent role of Ezh2 during T-cell development and immune homeostasis. T-cell-specific depletion of Ezh2 induces a pronounced expansion of natural killer T (NKT) cells, although Ezh2-deficient T cells maintain normal levels of H3K27me3. In contrast, removal of Suz12 or Eed destabilizes canonical PRC2 function and ablates NKT cell development completely. We further show that Ezh2 directly methylates the NKT cell lineage defining transcription factor PLZF, leading to its ubiquitination and subsequent degradation. Sustained PLZF expression in Ezh2-deficient mice is associated with the expansion of a subset of NKT cells that cause immune perturbation. Taken together, we have identified a chromatin-independent function of Ezh2 that impacts on the development of the immune system.
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    Total Synthesis of Mycobacterium tuberculosis Dideoxymy-cobactin-838 and Stereoisomers: Diverse CD1a-Restricted T Cells Display a Common Hierarchy of Lipopeptide Recognition
    Cheng, JMH ; Liu, L ; Pellicci, DG ; Reddiex, SJJ ; Cotton, RN ; Cheng, T-Y ; Young, DC ; Van Rhijn, I ; Moody, DB ; Rossjohn, J ; Fairlie, DP ; Godfrey, DI ; Williams, SJ (WILEY-V C H VERLAG GMBH, 2017-01)
    Mycobacterium tuberculosis produces dideoxymycobactin-838 (DDM-838), a lipopeptide that potently activates T cells upon binding to the MHC-like antigen-presenting molecule CD1a. M. tuberculosis produces DDM-838 in only trace amounts and a previous solid-phase synthesis provided sub-milligram quantities. We describe a high-yielding solution-phase synthesis of DDM-838 that features a Mitsunobu substitution that avoids yield-limiting epimerization at lysine during esterification, and amidation conditions that prevent double-bond isomerization of the Z-C20:1 acyl chain, and provides material with equivalent antigenicity to natural DDM-838. Isomers of DDM-838 that varied in stereochemistry at the central lysine and the C20:1 acyl chain were compared for their ability to be recognised by CD1a-restricted T cell receptors (TCRs). These TCRs, derived from unrelated human donors, exhibited a similar spectrum of reactivity towards the panel of DDM-838 isomers, highlighting the exquisite sensitivity of lipopeptide-reactive T cells for the natural DDM stereochemistry.
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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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    CD8+ T Cell Activation Leads to Constitutive Formation of Liver Tissue-Resident Memory T Cells that Seed a Large and Flexible Niche in the Liver
    Holz, LE ; Prier, JE ; Freestone, D ; Steiner, TM ; English, K ; Johnson, DN ; Mollard, V ; Cozijnsen, A ; Davey, GM ; Godfrey, D ; Yui, K ; Mackay, LK ; Lahoud, MH ; Caminschi, I ; McFadden, G ; Bertolino, P ; Fernandez-Ruiz, D ; Heath, WR (CELL PRESS, 2018-10-02)
    Liver tissue-resident memory T (Trm) cells migrate throughout the sinusoids and are capable of protecting against malaria sporozoite challenge. To gain an understanding of liver Trm cell development, we examined various conditions for their formation. Although liver Trm cells were found in naive mice, their presence was dictated by antigen specificity and required IL-15. Liver Trm cells also formed after adoptive transfer of in vitro-activated but not naive CD8+ T cells, indicating that activation was essential but that antigen presentation within the liver was not obligatory. These Trm cells patrolled the liver sinusoids with a half-life of 36 days and occupied a large niche that could be added to sequentially without effect on subsequent Trm cell cohorts. Together, our findings indicate that liver Trm cells form as a normal consequence of CD8+ T cell activation during essentially any infection but that inflammatory and antigenic signals preferentially tailor their development.
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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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    MicroRNA-managing the development of MAIT cells
    Koay, H-F ; Godfrey, DI (WILEY, 2019-02)
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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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    Differential surface phenotype and context-dependent reactivity of functionally diverse NKT cells
    Cameron, G ; Godfrey, DI (WILEY, 2018-08)
    Natural Killer T (NKT) cells are a functionally diverse population that recognizes lipid-based antigens in association with the antigen-presenting molecule CD1d. Here, we define a technique to separate the functionally distinct thymic NKT1, NKT2 and NKT17 cell subsets by their surface expression of CD278 (ICOS) and the activation-associated glycoform of CD43, enabling the investigation of subset-specific effector-functions. We report that all three subsets express the transcription factor GATA-3 and the potential to produce IL-4 and IL-10 following activation. This questions the notion that NKT2 cells are the predominant source of IL-4 within the NKT cell pool, and suggests that IL-10-production may be more indicative of NKT cell plasticity than the existence of a distinct regulatory lineage or subset. We also show that many NKT17 cells are CD4+ and are biased toward Vβ8.3 TCR gene usage. Lastly, we demonstrate that the toll-like receptor (TLR) ligand lipopolysaccharide (LPS) can induce a NKT17 cell-biased response, even in the absence of exogenous antigen, and that combining LPS with α-GalCer resulted in enhanced IL-17A-production, and reduced levels of the immunosuppressive cytokine IL-10. This study provides a novel means to examine the context-dependent reactivity of the functionally heterogeneous NKT cell population and provides important new insight into the functional biology of these subsets.
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    Characterization and Purification of Mouse Mucosal-Associated Invariant T (MAIT) Cells
    Chen, Z ; Wang, H ; D'Souza, C ; Koay, H-F ; Meehan, B ; Zhao, Z ; Pediongco, T ; Shi, M ; Zhu, T ; Wang, B ; Kjer-Nielsen, L ; Eckle, SBG ; Rossjohn, J ; Fairlie, DP ; Godfrey, DI ; Strugnell, RA ; McCluskey, J ; Corbett, AJ (John Wiley & Sons, 2019)
    This unit describes the utility of various mouse models of infection and immunization for studying mucosal-associated invariant T (MAIT) cell immunity: MAIT cells can be isolated from the lungs (or from other tissues/organs) and then identified and characterized by flow cytometry using MR1 tetramers in combination with a range of antibodies. The response kinetics, cytokine profiles, and functional differentiation of lung MAIT cells are studied following infection with the bacterial pathogen Legionella longbeachae or Salmonella enterica Typhimurium or immunization with synthetic MAIT cell antigen plus Toll-like receptor agonist. MAIT cells enriched or expanded during the process can be used for further studies. A step-by-step protocol is provided for MAIT cell sorting and adoptive transfer. Mice can then be challenged and MAIT cells tracked and further examined.