Microbiology & Immunology - Research Publications

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Author: Godfrey, Dale × Author: Uldrich, Adam ×

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    Biparatopic nanobodies targeting the receptor binding domain efficiently neutralize SARS-CoV-2
    Pymm, P ; Redmond, SJ ; Dolezal, O ; Mordant, F ; Lopez, E ; Cooney, JP ; Davidson, KC ; Haycroft, ER ; Tan, CW ; Seneviratna, R ; Grimley, SL ; Purcell, DFJ ; Kent, SJ ; Wheatley, AK ; Wang, L-F ; Leis, A ; Glukhova, A ; Pellegrini, M ; Chung, AW ; Subbarao, K ; Uldrich, AP ; Tham, W-H ; Godfrey, DI ; Gherardin, NA (CELL PRESS, 2022-11-18)
    The development of therapeutics to prevent or treat COVID-19 remains an area of intense focus. Protein biologics, including monoclonal antibodies and nanobodies that neutralize virus, have potential for the treatment of active disease. Here, we have used yeast display of a synthetic nanobody library to isolate nanobodies that bind the receptor-binding domain (RBD) of SARS-CoV-2 and neutralize the virus. We show that combining two clones with distinct binding epitopes within the RBD into a single protein construct to generate biparatopic reagents dramatically enhances their neutralizing capacity. Furthermore, the biparatopic nanobodies exhibit enhanced control over clinically relevant RBD variants that escaped recognition by the individual nanobodies. Structural analysis of biparatopic binding to spike (S) protein revealed a unique binding mode whereby the two nanobody paratopes bridge RBDs encoded by distinct S trimers. Accordingly, biparatopic nanobodies offer a way to rapidly generate powerful viral neutralizers with enhanced ability to control viral escape mutants.
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    CD8 coreceptor engagement of MR1 enhances antigen responsiveness by human MAIT and other MR1-reactive T cells
    Souter, MNT ; Awad, W ; Li, S ; Pediongco, T ; Meehan, BS ; Meehan, LJ ; Tian, Z ; Zhao, Z ; Wang, H ; Nelson, A ; Le Nours, J ; Khandokar, Y ; Praveena, T ; Wubben, J ; Lin, J ; Sullivan, LC ; Lovrecz, G ; Mak, JYW ; Liu, L ; Kostenko, L ; Kedzierska, K ; Corbett, AJ ; Fairlie, DP ; Brooks, AG ; Gherardin, NA ; Uldrich, AP ; Chen, Z ; Rossjohn, J ; Godfrey, DI ; MCCLUSKEY, J ; Pellicci, DG ; Eckle, SBG (Rockefeller University Press, 2022)
    Mucosal-associated invariant T (MAIT) cells detect microbial infection via recognition of riboflavin-based antigens presented by the major histocompatibility complex class I (MHC-I)-related protein 1 (MR1). Most MAIT cells in human peripheral blood express CD8αα or CD8αβ coreceptors, and the binding site for CD8 on MHC-I molecules is relatively conserved in MR1. Yet, there is no direct evidence of CD8 interacting with MR1 or the functional consequences thereof. Similarly, the role of CD8αα in lymphocyte function remains ill-defined. Here, using newly developed MR1 tetramers, mutated at the CD8 binding site, and by determining the crystal structure of MR1-CD8αα, we show that CD8 engaged MR1, analogous to how it engages MHC-I molecules. CD8αα and CD8αβ enhanced MR1 binding and cytokine production by MAIT cells. Moreover, the CD8-MR1 interaction was critical for the recognition of folate-derived antigens by other MR1-reactive T cells. Together, our findings suggest that both CD8αα and CD8αβ act as functional coreceptors for MAIT and other MR1-reactive T cells.
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    CD36 family members are TCR-independent ligands for CD1 antigen-presenting molecules.
    Gherardin, NA ; Redmond, SJ ; McWilliam, HEG ; Almeida, CF ; Gourley, KHA ; Seneviratna, R ; Li, S ; De Rose, R ; Ross, FJ ; Nguyen-Robertson, CV ; Su, S ; Ritchie, ME ; Villadangos, JA ; Moody, DB ; Pellicci, DG ; Uldrich, AP ; Godfrey, DI (American Association for the Advancement of Science, 2021-06-25)
    CD1c presents lipid-based antigens to CD1c-restricted T cells, which are thought to be a major component of the human T cell pool. However, the study of CD1c-restricted T cells is hampered by the presence of an abundantly expressed, non-T cell receptor (TCR) ligand for CD1c on blood cells, confounding analysis of TCR-mediated CD1c tetramer staining. Here, we identified the CD36 family (CD36, SR-B1, and LIMP-2) as ligands for CD1c, CD1b, and CD1d proteins and showed that CD36 is the receptor responsible for non-TCR-mediated CD1c tetramer staining of blood cells. Moreover, CD36 blockade clarified tetramer-based identification of CD1c-restricted T cells and improved identification of CD1b- and CD1d-restricted T cells. We used this technique to characterize CD1c-restricted T cells ex vivo and showed diverse phenotypic features, TCR repertoire, and antigen-specific subsets. Accordingly, this work will enable further studies into the biology of CD1 and human CD1-restricted T cells.
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    Differential location of NKT and MAIT cells within lymphoid tissue
    Johnson, DN ; Ruan, Z ; Petley, E ; Devi, S ; Holz, LE ; Uldrich, AP ; Mak, JYW ; Hor, JL ; Mueller, SN ; McCluskey, J ; Fairlie, DP ; Darcy, PK ; Beavis, PA ; Heath, WR ; Godfrey, D (NATURE PORTFOLIO, 2022-03-08)
    Natural Killer T (NKT) cells and Mucosal-Associated Invariant T (MAIT) cells are innate-like T cells that express semi-invariant αβ T cell receptors (TCRs) through which they recognise CD1d and MR1 molecules, respectively, in complex with specific ligands. These cells play important roles in health and disease in many organs, but their precise intra-organ location is not well established. Here, using CD1d and MR1 tetramer staining techniques, we describe the precise location of NKT and MAIT cells in lymphoid and peripheral organs. Within the thymus, NKT cells were concentrated in the medullary side of the corticomedullary junction. In spleen and lymph nodes, NKT cells were mainly localised within T cell zones, although following in vivo activation with the potent NKT-cell ligand α-GalCer, they expanded throughout the spleen. MAIT cells were clearly detectable in Vα19 TCR transgenic mice and were rare but detectable in lymphoid tissue of non-transgenic mice. In contrast to NKT cells, MAIT cells were more closely associated with the B cell zone and red pulp of the spleen. Accordingly, we have provided an extensive analysis of the in situ localisation of NKT and MAIT cells and suggest differences between the intra-organ location of these two cell types.
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    Immune recognition of phosphoantigen-butyrophilin molecular complexes by γδ T cells
    Uldrich, AP ; Rigau, M ; Godfrey, DI (WILEY, 2020-11)
    Gamma-delta (γδ) T cells are an important component of the immune system. They are often enriched in non-lymphoid tissues and exhibit diverse functional attributes including rapid activation, cytokine production, proliferation, and acquisition of cytotoxicity following both TCR-dependent and TCR-independent stimulation, but poor capacity for immunological memory. They can detect a broad range of antigens, although typically not peptide-MHC complexes in contrast to alpha-beta (αβ) T cells. In humans, a prominent population of γδ T cells, defined as Vγ9Vδ2+ cells, reacts to small phosphorylated non-peptide "phosphoantigens" (pAgs). The molecular mechanism underpinning this recognition is poorly defined, but is known to involve butyrophilin family members and appears to involve indirect pAg recognition via alterations to butyrophilin molecular complexes. In this review, we discuss recent advances in our understanding of pAg recognition by γδ T cells including the role of butyrophilins and in particular, a newly described role for butyrophilin 2A1.
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    Butyrophilin 2A1 is essential for phosphoantigen reactivity by gamma delta T cells
    Rigau, M ; Ostrouska, S ; Fulford, TS ; Johnson, DN ; Woods, K ; Ruan, Z ; McWilliam, HEG ; Hudson, C ; Tutuka, C ; Wheatley, AK ; Kent, SJ ; Villadangos, JA ; Pal, B ; Kurts, C ; Simmonds, J ; Pelzing, M ; Nash, AD ; Hammet, A ; Verhagen, AM ; Vairo, G ; Maraskovsky, E ; Panousis, C ; Gherardin, NA ; Cebon, J ; Godfrey, DI ; Behren, A ; Uldrich, AP (American Association for the Advancement of Science, 2020-02-07)
    Gamma delta (γδ) T cells are essential to protective immunity. In humans, most γδ T cells express Vγ9Vδ2+ T cell receptors (TCRs) that respond to phosphoantigens (pAgs) produced by cellular pathogens and overexpressed by cancers. However, the molecular targets recognized by these γδTCRs are unknown. Here, we identify butyrophilin 2A1 (BTN2A1) as a key ligand that binds to the Vγ9+ TCR γ chain. BTN2A1 associates with another butyrophilin, BTN3A1, and these act together to initiate responses to pAg. Furthermore, binding of a second ligand, possibly BTN3A1, to a separate TCR domain incorporating Vδ2 is also required. This distinctive mode of Ag-dependent T cell activation advances our understanding of diseases involving pAg recognition and creates opportunities for the development of γδ T cell-based immunotherapies.
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    Antigen-loaded MR1 tetramers define T cell receptor heterogeneity in mucosal-associated invariant T cells
    Reantragoon, R ; Corbett, AJ ; Sakala, IG ; Gherardin, NA ; Furness, JB ; Chen, Z ; Eckle, SBG ; Uldrich, AP ; Birkinshaw, RW ; Patel, O ; Kostenko, L ; Meehan, B ; Kedzierska, K ; Liu, L ; Fairlie, DP ; Hansen, TH ; Godfrey, DI ; Rossjohn, J ; McCluskey, J ; Kjer-Nielsen, L (ROCKEFELLER UNIV PRESS, 2013-10-21)
    Mucosal-associated invariant T cells (MAIT cells) express a semi-invariant T cell receptor (TCR) α-chain, TRAV1-2-TRAJ33, and are activated by vitamin B metabolites bound by the major histocompatibility complex (MHC)-related class I-like molecule, MR1. Understanding MAIT cell biology has been restrained by the lack of reagents to specifically identify and characterize these cells. Furthermore, the use of surrogate markers may misrepresent the MAIT cell population. We show that modified human MR1 tetramers loaded with the potent MAIT cell ligand, reduced 6-hydroxymethyl-8-D-ribityllumazine (rRL-6-CH₂OH), specifically detect all human MAIT cells. Tetramer(+) MAIT subsets were predominantly CD8(+) or CD4(-)CD8(-), although a small subset of CD4(+) MAIT cells was also detected. Notably, most human CD8(+) MAIT cells were CD8α(+)CD8β(-/lo), implying predominant expression of CD8αα homodimers. Tetramer-sorted MAIT cells displayed a T(H)1 cytokine phenotype upon antigen-specific activation. Similarly, mouse MR1-rRL-6-CH₂OH tetramers detected CD4(+), CD4(-)CD8(-) and CD8(+) MAIT cells in Vα19 transgenic mice. Both human and mouse MAIT cells expressed a broad TCR-β repertoire, and although the majority of human MAIT cells expressed TRAV1-2-TRAJ33, some expressed TRAJ12 or TRAJ20 genes in conjunction with TRAV1-2. Accordingly, MR1 tetramers allow precise phenotypic characterization of human and mouse MAIT cells and revealed unanticipated TCR heterogeneity in this population.
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    Atypical natural killer T-cell receptor recognition of CD1d-lipid antigens
    Le Nours, J ; Praveena, T ; Pellicci, DG ; Gherardin, NA ; Ross, FJ ; Lim, RT ; Besra, GS ; Keshipeddy, S ; Richardson, SK ; Howell, AR ; Gras, S ; Godfrey, DI ; Rossjohn, J ; Uldrich, AP (NATURE PUBLISHING GROUP, 2016-02)
    Crucial to Natural Killer T (NKT) cell function is the interaction between their T-cell receptor (TCR) and CD1d-antigen complex. However, the diversity of the NKT cell repertoire and the ensuing interactions with CD1d-antigen remain unclear. We describe an atypical population of CD1d-α-galactosylceramide (α-GalCer)-reactive human NKT cells that differ markedly from the prototypical TRAV10-TRAJ18-TRBV25-1(+) type I NKT cell repertoire. These cells express a range of TCR α- and β-chains that show differential recognition of glycolipid antigens. Two atypical NKT TCRs (TRAV21-TRAJ8-TRBV7-8 and TRAV12-3-TRAJ27-TRBV6-5) bind orthogonally over the A'-pocket of CD1d, adopting distinct docking modes that contrast with the docking mode of all type I NKT TCR-CD1d-antigen complexes. Moreover, the interactions with α-GalCer differ between the type I and these atypical NKT TCRs. Accordingly, diverse NKT TCR repertoire usage manifests in varied docking strategies and specificities towards CD1d-α-GalCer and related antigens, thus providing far greater scope for diverse glycolipid antigen recognition.
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    α-Glucuronosyl and α-glucosyl diacylglycerides, natural killer T cell-activating lipids from bacteria and fungi
    Burugupalli, S ; Almeida, CF ; Smith, DGM ; Shah, S ; Patel, O ; Rossjohn, J ; Uldrich, AP ; Godfrey, DI ; Williams, SJ (ROYAL SOC CHEMISTRY, 2020-02-28)
    Natural killer T cells express T cell receptors (TCRs) that recognize glycolipid antigens in association with the antigen-presenting molecule CD1d. Here, we report the concise chemical synthesis of a range of saturated and unsaturated α-glucosyl and α-glucuronosyl diacylglycerides of bacterial and fungal origins from allyl α-glucoside with Jacobsen kinetic resolution as a key step. These glycolipids are recognized by a classical type I NKT TCR that uses an invariant Vα14-Jα18 TCR α-chain, but also by an atypical NKT TCR that uses a different TCR α-chain (Vα10-Jα50). In both cases, recognition is sensitive to the lipid fine structure, and includes recognition of glycosyl diacylglycerides bearing branched (R- and S-tuberculostearic acid) and unsaturated (oleic and vaccenic) acids. The TCR footprints on CD1d loaded with a mycobacterial α-glucuronosyl diacylglyceride were assessed using mutant CD1d molecules and, while similar to that for α-GalCer recognition by a type I NKT TCR, were more sensitive to mutations when α-glucuronosyl diacylglyceride was the antigen. In summary, we provide an efficient approach for synthesis of a broad class of bacterial and fungal α-glycosyl diacylglyceride antigens and demonstrate that they can be recognised by TCRs derived from type I and atypical NKT cells.
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    Distinct CD1d docking strategies exhibited by diverse Type II NKT cell receptors
    Almeida, CF ; Sundararaj, S ; Le Nours, J ; Praveena, T ; Cao, B ; Burugupalli, S ; Smith, DGM ; Patel, O ; Brigl, M ; Pellicci, DG ; Williams, SJ ; Uldrich, AP ; Godfrey, DI ; Rossjohn, J (NATURE PORTFOLIO, 2019-11-20)
    Type I and type II natural killer T (NKT) cells are restricted to the lipid antigen-presenting molecule CD1d. While we have an understanding of the antigen reactivity and function of type I NKT cells, our knowledge of type II NKT cells in health and disease remains unclear. Here we describe a population of type II NKT cells that recognise and respond to the microbial antigen, α-glucuronosyl-diacylglycerol (α-GlcADAG) presented by CD1d, but not the prototypical type I NKT cell agonist, α-galactosylceramide. Surprisingly, the crystal structure of a type II NKT TCR-CD1d-α-GlcADAG complex reveals a CD1d F'-pocket-docking mode that contrasts sharply with the previously determined A'-roof positioning of a sulfatide-reactive type II NKT TCR. Our data also suggest that diverse type II NKT TCRs directed against distinct microbial or mammalian lipid antigens adopt multiple recognition strategies on CD1d, thereby maximising the potential for type II NKT cells to detect different lipid antigens.