Your search keyword '"Wagstaffe HR"' showing total 13 results

1. The Effect of Viral Vaccines on Natural Killer Cell Effector Function

Author

Wagstaffe, HR, Goodier, MR, and Riley, E

Abstract

Natural killer cells are large, granular, innate lymphoid cells that lie at the interface between innate and adaptive immunity and facilitate bidirectional crosstalk between the two systems. This has led to an abundance of research into vaccination induced priming of ‘adaptive’ or memory-like NK cell responses. Using human peripheral blood mononuclear cells for cross-sectional and vaccination studies in two distinct virus models, cytokine-dependent NK cell activation, and the effect of vaccination on these responses was investigated. Very low concentrations of IL-15 enhanced NK cell activation in response to inactivated influenza virus stimulation in vitro via augmented innate cytokine secretion from accessory cells, in particular IL-12 from myeloid dendritic cells. Similarly, after seasonal influenza vaccination, both accessory cell cytokine secretion and NK cell activation were enhanced compared to before vaccination in response to low dose IL-15 stimulation in vitro. This suggested that together with a vaccination-induced enhanced responsiveness to innate cytokines at the NK cell level (the generation of cytokine-induced memory like NK cells), an increased production of innate cytokines at the accessory cell level contributed to the overall enhancement in NK cell response post-vaccination. The effect of vaccination on NK cell effector function was further investigated in PBMC from heathy volunteers vaccinated with an Ebola glycoprotein expressing, vectored, prime-boost regimen vaccine (Ad26.ZEBOV/MVA-BN-Filo). Both inactivated influenza vaccination and Ebola vaccination increased the frequency and proliferation of less differentiated, CD56bright NK cells. Data described in this thesis also demonstrate for the first time that NK cells were activated indirectly by Ebola glycoprotein induced IL-12 and IL-18, independently of Ebola vaccination, and in contrast to influenza vaccination, there was no evidence of vaccine induced boosting of these responses. NK cell responses to Ebola GP were dependent on accessory cell TLR-4 engagement but were tightly regulated by CD14+ monocyte-derived IL-10. In addition to soluble antigen driven cytokinedependent activation, 21-day post-boost vaccination serum induced robust antibody-dependent NK cell activation of more differentiated subsets that varied with vaccine arm and correlated with antibody titre. Together, these studies demonstrate that two different types of vaccines against distinct viruses have similar impacts on the activation of less differentiated NK cells. Priming of both NK cells and myeloid cells for enhanced cytokinedependent NK cell responses after vaccination was not replicated across different vaccination models and may be a function dependent on the unique cytokine signatures induced by the respective antigens. These studies further our understanding of NK cells in post-vaccination effector responses, and may represent an avenue for improving future design of vaccines and adjuvants.

2. Mucosal and systemic immune correlates of viral control after SARS-CoV-2 infection challenge in seronegative adults.

Author

Wagstaffe HR, Thwaites RS, Reynaldi A, Sidhu JK, McKendry R, Ascough S, Papargyris L, Collins AM, Xu J, Lemm NM, Siggins MK, Chain BM, Killingley B, Kalinova M, Mann A, Catchpole A, Davenport MP, Openshaw PJM, and Chiu C

Subjects

Humans, SARS-CoV-2, Vaccination, CD8-Positive T-Lymphocytes, Nasal Mucosa, COVID-19

Abstract

Human infection challenge permits in-depth, early, and pre-symptomatic characterization of the immune response, enabling the identification of factors that are important for viral clearance. Here, we performed intranasal inoculation of 34 young adult, seronegative volunteers with a pre-Alpha severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) strain. Of these participants, 18 (53%) became infected and showed an interferon-dominated mediator response with divergent kinetics between nasal and systemic sites. Peripheral CD4 + and CD8 + T cell activation and proliferation were early and robust but showed distinct kinetic and phenotypic profiles; antigen-specific T cells were largely CD38 + Ki67 + and displayed central and effector memory phenotypes. Both mucosal and systemic antibodies became detectable around day 10, but nasal antibodies plateaued after day 14 while circulating antibodies continued to rise. Intensively granular measurements in nasal mucosa and blood allowed modeling of immune responses to primary SARS-CoV-2 infection that revealed CD8 + T cell responses and early mucosal IgA responses strongly associated with viral control, indicating that these mechanisms should be targeted for transmission-reducing intervention.

Published

2024

3. Author Correction: Human SARS-CoV-2 challenge uncovers local and systemic response dynamics.

Author

Lindeboom RGH, Worlock KB, Dratva LM, Yoshida M, Scobie D, Wagstaffe HR, Richardson L, Wilbrey-Clark A, Barnes JL, Kretschmer L, Polanski K, Allen-Hyttinen J, Mehta P, Sumanaweera D, Boccacino JM, Sungnak W, Elmentaite R, Huang N, Mamanova L, Kapuge R, Bolt L, Prigmore E, Killingley B, Kalinova M, Mayer M, Boyers A, Mann A, Swadling L, Woodall MNJ, Ellis S, Smith CM, Teixeira VH, Janes SM, Chambers RC, Haniffa M, Catchpole A, Heyderman R, Noursadeghi M, Chain B, Mayer A, Meyer KB, Chiu C, Nikolić MZ, and Teichmann SA

Published

2024

4. Human SARS-CoV-2 challenge uncovers local and systemic response dynamics.

Author

Lindeboom RGH, Worlock KB, Dratva LM, Yoshida M, Scobie D, Wagstaffe HR, Richardson L, Wilbrey-Clark A, Barnes JL, Kretschmer L, Polanski K, Allen-Hyttinen J, Mehta P, Sumanaweera D, Boccacino JM, Sungnak W, Elmentaite R, Huang N, Mamanova L, Kapuge R, Bolt L, Prigmore E, Killingley B, Kalinova M, Mayer M, Boyers A, Mann A, Swadling L, Woodall MNJ, Ellis S, Smith CM, Teixeira VH, Janes SM, Chambers RC, Haniffa M, Catchpole A, Heyderman R, Noursadeghi M, Chain B, Mayer A, Meyer KB, Chiu C, Nikolić MZ, and Teichmann SA

Subjects

Female, Humans, Male, Epithelial Cells immunology, Gene Expression Profiling, Interferons immunology, Macrophages immunology, Macrophages virology, Nasopharynx virology, Nasopharynx immunology, T-Lymphocytes cytology, T-Lymphocytes immunology, T-Lymphocytes metabolism, T-Lymphocytes virology, Time Factors, Virus Replication, COVID-19 genetics, COVID-19 immunology, COVID-19 pathology, COVID-19 virology, Multiomics, SARS-CoV-2 growth & development, SARS-CoV-2 immunology, SARS-CoV-2 pathogenicity, SARS-CoV-2 physiology, Single-Cell Analysis

Abstract

The COVID-19 pandemic is an ongoing global health threat, yet our understanding of the dynamics of early cellular responses to this disease remains limited 1 . Here in our SARS-CoV-2 human challenge study, we used single-cell multi-omics profiling of nasopharyngeal swabs and blood to temporally resolve abortive, transient and sustained infections in seronegative individuals challenged with pre-Alpha SARS-CoV-2. Our analyses revealed rapid changes in cell-type proportions and dozens of highly dynamic cellular response states in epithelial and immune cells associated with specific time points and infection status. We observed that the interferon response in blood preceded the nasopharyngeal response. Moreover, nasopharyngeal immune infiltration occurred early in samples from individuals with only transient infection and later in samples from individuals with sustained infection. High expression of HLA-DQA2 before inoculation was associated with preventing sustained infection. Ciliated cells showed multiple immune responses and were most permissive for viral replication, whereas nasopharyngeal T cells and macrophages were infected non-productively. We resolved 54 T cell states, including acutely activated T cells that clonally expanded while carrying convergent SARS-CoV-2 motifs. Our new computational pipeline Cell2TCR identifies activated antigen-responding T cells based on a gene expression signature and clusters these into clonotype groups and motifs. Overall, our detailed time series data can serve as a Rosetta stone for epithelial and immune cell responses and reveals early dynamic responses associated with protection against infection., (© 2024. The Author(s).)

Published

2024

5. The Development of Immunological Assays to Evaluate the Level and Function of Antibodies Induced by Klebsiella pneumoniae O-Antigen Vaccines.

Author

Wagstaffe HR, Johnson M, Osman G, Martin P, Carranza P, and Goldblatt D

Subjects

Animals, Rabbits, Antibodies, Bacterial, Phagocytosis, Bacterial Vaccines, O Antigens, Klebsiella pneumoniae

Abstract

Klebsiella pneumoniae, a Gram-negative bacterium, has been listed as a critical pathogen for urgent intervention by the World Health Organization. With no licensed vaccine and increasing resistance to antibiotics, Klebsiella pneumoniae causes a high incidence of hospital- and community-acquired infections. Recently, there has been progress in anti-Klebsiella pneumoniae vaccine development, which has highlighted the lack of standardized assays to measure vaccine immunogenicity. We have developed and optimized methods to measure antibody level and function after vaccination with an in-development Klebsiella pneumoniae O-antigen vaccine. We describe the qualification of a Luminex-based multiplex antibody binding assay and both an opsonophagocytic killing assay and serum bactericidal assay to measure antibody function. Serum from immunized animals were immunogenic and capable of binding to and killing specific Klebsiella serotypes. Cross-reactivity was observed but limited among serotypes sharing antigenic epitopes. In summary, these results demonstrate the standardization of assays that can be used to test new anti-Klebsiella pneumoniae vaccine candidates, which is important for moving them into clinical trials. IMPORTANCE There is no licensed vaccine for the prevention of Klebsiella pneumoniae infections, and increasing levels of antibiotic resistance make this pathogen a high priority for vaccine and therapeutic development. Standardized assays for testing vaccine immunogenicity are paramount for the development of vaccines, and so in this study, we optimized and standardized both antibody-level and function assays for evaluating in-development K. pneumoniae bioconjugate vaccine response in rabbits.

Published

2023

6. NK Cell Subset Redistribution and Antibody Dependent Activation after Ebola Vaccination in Africans.

Author

Wagstaffe HR, Anzala O, Kibuuka H, Anywaine Z, Sirima SB, Thiébaut R, Richert L, Levy Y, Lacabaratz C, Bockstal V, Luhn K, Douoguih M, and Goodier MR

Abstract

Natural killer cells play an important role in the control of viral infections both by regulating acquired immune responses and as potent innate or antibody-mediated cytotoxic effector cells. NK cells have been implicated in control of Ebola virus infections and our previous studies in European trial participants have demonstrated durable activation, proliferation and antibody-dependent NK cell activation after heterologous two-dose Ebola vaccination with adenovirus type 26.ZEBOV followed by modified vaccinia Ankara-BN-Filo. Regional variation in immunity and environmental exposure to pathogens, in particular human cytomegalovirus, have profound impacts on NK cell functional capacity. We therefore assessed the NK cell phenotype and function in African trial participants with universal exposure to HCMV. We demonstrate a significant redistribution of NK cell subsets after vaccine dose two, involving the enrichment of less differentiated CD56 dim CD57 - and CD56 dim FcεR1γ + (canonical) cells and the increased proliferation of these subsets. Sera taken after vaccine dose two support robust antibody-dependent NK cell activation in a standard NK cell readout; these responses correlate strongly with the concentration of anti-Ebola glycoprotein specific antibodies. These sera also promote comparable IFN-γ production in autologous NK cells taken at baseline and post-vaccine dose two. However, degranulation responses of post-vaccination NK cells were reduced compared to baseline NK cells and these effects could not be directly attributed to alterations in NK cell phenotype after vaccination. These studies demonstrate consistent changes in NK cell phenotypic composition and robust antibody-dependent NK cell function and reveal novel characteristics of these responses after heterologous two dose Ebola vaccination in African individuals.

Published

2022

7. Antibody-Dependent Natural Killer Cell Activation After Ebola Vaccination.

Author

Wagstaffe HR, Clutterbuck EA, Bockstal V, Stoop JN, Luhn K, Douoguih M, Shukarev G, Snape MD, Pollard AJ, Riley EM, and Goodier MR

Subjects

Antibodies, Viral blood, Ebolavirus immunology, Glycoproteins immunology, Humans, Vaccination, Viral Proteins immunology, Antibody-Dependent Cell Cytotoxicity, Ebola Vaccines immunology, Hemorrhagic Fever, Ebola prevention & control, Killer Cells, Natural immunology

Abstract

Background: Antibody Fc-mediated functions, such as antibody-dependent cellular cytotoxicity, contribute to vaccine-induced protection against viral infections. Fc-mediated function of anti-Ebola glycoprotein (GP) antibodies suggest that Fc-dependent activation of effector cells, including natural killer (NK) cells, could play a role in vaccination against Ebola virus disease., Methods: We analyzed the effect on primary human NK cell activation of anti-Ebola GP antibody in the serum of United Kingdom-based volunteers vaccinated with the novel 2-dose heterologous adenovirus type 26.ZEBOV, modified vaccinia Ankara-BN-Filo vaccine regimen., Results: We demonstrate primary human NK cell CD107a and interferon γ expression, combined with down-regulation of CD16, in response to recombinant Ebola virus GP and post-vaccine dose 1 and dose 2 serum samples. These responses varied significantly with vaccine regimen, and NK cell activation was found to correlate with anti-GP antibody concentration. We also reveal an impact of NK cell differentiation phenotype on antibody-dependent NK cell activation, with highly differentiated CD56dimCD57+ NK cells being the most responsive., Conclusions: These findings highlight the dual importance of vaccine-induced antibody concentration and NK cell differentiation status in promoting Fc-mediated activation of NK cells after vaccination, raising a potential role for antibody-mediated NK cell activation in vaccine-induced immune responses., (© The Author(s) 2019. Published by Oxford University Press for the Infectious Diseases Society of America.)

Published

2021

8. Durable natural killer cell responses after heterologous two-dose Ebola vaccination.

Author

Wagstaffe HR, Susannini G, Thiébaut R, Richert L, Lévy Y, Bockstal V, Stoop JN, Luhn K, Douoguih M, Riley EM, Lacabaratz C, and Goodier MR

Abstract

Natural killer (NK) cells are implicated among immune effectors after vaccination against viral pathogens, including Ebola virus. The two-dose heterologous Ebola virus vaccine regimen, adenovirus type 26.ZEBOV followed by modified vaccinia Ankara-BN-Filo (EBOVAC2 consortium, EU Innovative Medicines Initiative), induces NK cell activation and anti-Ebola glycoprotein (GP) antibody-dependent NK cell activation post-dose 1, which is further elevated post-dose 2. Here, in a multicentre, phase 2 clinical trial (EBL2001), we demonstrate durable ex vivo NK cell activation 180 days after dose 2, with responses enriched in CD56 bright NK cells. In vitro antibody-dependent responses to immobilised Ebola GP increased after dose 1, and remained elevated compared to pre-vaccination levels in serum collected 180 days later. Peak NK cell responses were observed post-dose 2 and NK cell IFN-γ responses remained significantly elevated at 180 days post-dose 2. Individual variation in NK cell responses were influenced by both anti-Ebola GP antibody concentrations and intrinsic interindividual differences in NK cell functional capacity. In summary, this study demonstrates durable NK cell responses after Ad26.ZEBOV, MVA-BN-Filo Ebola virus vaccination and could inform the immunological evaluation of future iterations of the vaccine regimen and vaccination schedules.

Published

2021

9. Evaluation of a novel multiplexed assay for determining IgG levels and functional activity to SARS-CoV-2.

Author

Johnson M, Wagstaffe HR, Gilmour KC, Mai AL, Lewis J, Hunt A, Sirr J, Bengt C, Grandjean L, and Goldblatt D

Subjects

Adult, Betacoronavirus, COVID-19, COVID-19 Testing, Clinical Laboratory Techniques, Coronavirus Infections immunology, Coronavirus Nucleocapsid Proteins, Female, Humans, Luminescent Measurements methods, Male, Middle Aged, Nucleocapsid Proteins immunology, Pandemics, Phosphoproteins, Pneumonia, Viral immunology, SARS-CoV-2, Sensitivity and Specificity, Spike Glycoprotein, Coronavirus immunology, Antibodies, Viral blood, Antigens, Viral immunology, Coronavirus Infections diagnosis, Immunoassay methods, Immunoglobulin G blood, Pneumonia, Viral diagnosis

Abstract

Background: The emergence of SARS-CoV-2 has led to the development of serological assays that could aid in an understanding of the burden of COVID-19 disease. Many available tests lack rigorous evaluation and therefore results may be misleading., Objectives: The aim of this study was to assess the performance of a novel multiplexed immunoassay for the simultaneous detection of antibodies against SARS-CoV-2 trimeric spike (S), spike receptor binding domain (RBD), spike N terminal domain and nucleocapsid antigen and a novel pseudo-neutralisation assay., Methods: A multiplexed solid-phase chemiluminescence assay (Meso Scale Discovery) was evaluated for the simultaneous detection of IgG binding to four SARS-CoV-2 antigens and the quantification of antibody-induced ACE-2 binding inhibition (pseudo-neutralisation assay). Sensitivity was evaluated with a total of 196 COVID-19 serum samples (169 confirmed PCR positive and 27 anti-nucleocapsid IgG positive) from individuals with mild symptomatic or asymptomatic disease. Specificity was evaluated with 194 control serum samples collected from adults prior to December 2019., Results: The specificity and sensitivity of the binding IgG assay was highest for S protein with a specificity of 97.4 % and sensitivity of 96.2 % for samples taken 14 days and 97.9 % for samples taken 21 days following the onset of symptoms. IgG concentration to S and RBD correlated strongly with percentage inhibition measured by the pseudo-neutralisation assay., Conclusion: Excellent sensitivity for IgG detection was obtained over 14 days since onset of symptoms for three SARS-CoV-2 antigens (S, RBD and N) in this multiplexed assay which can also measure antibody functionality., (Copyright © 2020 The Author(s). Published by Elsevier B.V. All rights reserved.)

Published

2020

10. Ebola virus glycoprotein stimulates IL-18-dependent natural killer cell responses.

Author

Wagstaffe HR, Clutterbuck EA, Bockstal V, Stoop JN, Luhn K, Douoguih M, Shukarev G, Snape MD, Pollard AJ, Riley EM, and Goodier MR

Subjects

Adolescent, Adult, Antibodies, Viral immunology, Ebola Vaccines administration & dosage, Ebola Vaccines genetics, Ebolavirus genetics, Female, Humans, Male, Middle Aged, Viral Envelope Proteins administration & dosage, Viral Envelope Proteins genetics, Ebola Vaccines immunology, Ebolavirus immunology, Interleukin-18 immunology, Killer Cells, Natural immunology, Viral Envelope Proteins immunology

Abstract

BACKGROUNDNK cells are activated by innate cytokines and viral ligands to kill virus-infected cells. These functions are enhanced during secondary immune responses and after vaccination by synergy with effector T cells and virus-specific antibodies. In human Ebola virus infection, clinical outcome is strongly associated with the initial innate cytokine response, but the role of NK cells has not been thoroughly examined.METHODSThe novel 2-dose heterologous Adenovirus type 26.ZEBOV (Ad26.ZEBOV) and modified vaccinia Ankara-BN-Filo (MVA-BN-Filo) vaccine regimen is safe and provides specific immunity against Ebola glycoprotein, and is currently in phase 2 and 3 studies. Here, we analyzed NK cell phenotype and function in response to Ad26.ZEBOV, MVA-BN-Filo vaccination regimen and in response to in vitro Ebola glycoprotein stimulation of PBMCs isolated before and after vaccination.RESULTSWe show enhanced NK cell proliferation and activation after vaccination compared with baseline. Ebola glycoprotein-induced activation of NK cells was dependent on accessory cells and TLR-4-dependent innate cytokine secretion (predominantly from CD14+ monocytes) and enriched within less differentiated NK cell subsets. Optimal NK cell responses were dependent on IL-18 and IL-12, whereas IFN-γ secretion was restricted by high concentrations of IL-10.CONCLUSIONThis study demonstrates the induction of NK cell effector functions early after Ad26.ZEBOV, MVA-BN-Filo vaccination and provides a mechanism for the activation and regulation of NK cells by Ebola glycoprotein.TRIAL REGISTRATIONClinicalTrials.gov NCT02313077.FUNDINGUnited Kingdom Medical Research Council Studentship in Vaccine Research, Innovative Medicines Initiative 2 Joint Undertaking, EBOVAC (grant 115861) and Crucell Holland (now Janssen Vaccines and Prevention B.V.), European Union's Horizon 2020 research and innovation programme and European Federation of Pharmaceutical Industries and Associations (EFPIA).

Published

2020

11. Influenza Vaccination Primes Human Myeloid Cell Cytokine Secretion and NK Cell Function.

Author

Wagstaffe HR, Pickering H, Houghton J, Mooney JP, Wolf AS, Prevatt N, Behrens RH, Holland MJ, Riley EM, and Goodier MR

Subjects

Adult, Aged, Female, Humans, Influenza A Virus, H3N2 Subtype immunology, Interferon-gamma immunology, Interleukin-15 immunology, Leukocytes, Mononuclear immunology, Lymphocyte Activation immunology, Male, Middle Aged, Vaccination methods, Young Adult, Cytokines immunology, Influenza Vaccines immunology, Influenza, Human immunology, Killer Cells, Natural immunology, Myeloid Cells immunology

Abstract

Cytokine-induced memory-like (CIML) NK cells generated in response to proinflammatory cytokines in vitro and in vivo can also be generated by vaccination, exhibiting heightened responses to cytokine stimulation months after their initial induction. Our previous study demonstrated that in vitro human NK cell responses to inactivated influenza virus were also indirectly augmented by very low doses of IL-15, which increased induction of myeloid cell-derived cytokine secretion. These findings led us to hypothesize that IL-15 stimulation could reveal a similar effect for active influenza vaccination and influence CIML NK cell effector functions. In this study, 51 healthy adults were vaccinated with seasonal influenza vaccine, and PBMC were collected before and up to 30 d after vaccination. Myeloid and lymphoid cell cytokine secretion was measured after in vitro PBMC restimulation with low-dose IL-15, alone or in combination with inactivated H3N2 virus; the associated NK cell response was assessed by flow cytometry. PBMC collected 30 d postvaccination showed heightened cytokine production in response to IL-15 compared with PBMC collected at baseline; these responses were further enhanced when IL-15 was combined with H3N2. NK cell activation in response to IL-15 alone (CD25) and H3N2 plus IL-15 (CD25 and IFN-γ) was enhanced postvaccination. We also observed proliferation of less-differentiated NK cells with downregulation of cytokine receptors as early as 3 d after vaccination, suggesting cytokine stimulation in vivo. We conclude that vaccination-induced "training" of accessory cells combines with the generation of CIML NK cells to enhance the overall NK cell response postvaccination., (Copyright © 2019 by The American Association of Immunologists, Inc.)

Published

2019

12. IL-15 Promotes Polyfunctional NK Cell Responses to Influenza by Boosting IL-12 Production.

Author

Wagstaffe HR, Nielsen CM, Riley EM, and Goodier MR

Subjects

Humans, Influenza, Human immunology, Interleukin-12 immunology, Leukocytes, Mononuclear immunology, Leukocytes, Mononuclear metabolism, Influenza A virus immunology, Interleukin-12 biosynthesis, Interleukin-15 immunology, Killer Cells, Natural immunology, Lymphocyte Activation immunology

Abstract

IL-15 is a key regulator of NK cell maintenance and proliferation and synergizes with other myeloid cell-derived cytokines to enhance NK cell effector function. At low concentrations, trans -presentation of IL-15 by dendritic cells can activate NK cells, whereas at higher concentrations it can act directly on NK cells, independently of accessory cells. In this study, we investigate the potential for IL-15 to boost responses to influenza virus by promoting accessory cell function. We find that coculture of human PBMCs with inactivated whole influenza virus (A/Victoria/361/2011) in the presence of very low concentrations of IL-15 results in increased production of myeloid cell-derived cytokines, including IL-12, IFN-α2, GM-CSF, and IL-1β, and an increased frequency of polyfunctional NK cells (defined by the expression of two or more of CD107a, IFN-γ, and CD25). Neutralization experiments demonstrate that IL-15-mediated enhancement of NK cell responses is primarily dependent on IL-12 and partially dependent on IFN-αβR1 signaling. Critically, IL-15 boosted the production of IL-12 in influenza-stimulated blood myeloid dendritic cells. IL-15 costimulation also restored the ability of less-differentiated NK cells from human CMV-seropositive individuals to respond to influenza virus. These data suggest that very low concentrations of IL-15 play an important role in boosting accessory cell function to support NK cell effector functions., (Copyright © 2018 The Authors.)

Published

2018

13. Vaccinating for natural killer cell effector functions.

Author

Wagstaffe HR, Mooney JP, Riley EM, and Goodier MR

Abstract

Vaccination has proved to be highly effective in reducing global mortality and eliminating infectious diseases. Building on this success will depend on the development of new and improved vaccines, new methods to determine efficacy and optimum dosing and new or refined adjuvant systems. NK cells are innate lymphoid cells that respond rapidly during primary infection but also have adaptive characteristics enabling them to integrate innate and acquired immune responses. NK cells are activated after vaccination against pathogens including influenza, yellow fever and tuberculosis, and their subsequent maturation, proliferation and effector function is dependent on myeloid accessory cell-derived cytokines such as IL-12, IL-18 and type I interferons. Activation of antigen-presenting cells by live attenuated or whole inactivated vaccines, or by the use of adjuvants, leads to enhanced and sustained NK cell activity, which in turn contributes to T cell recruitment and memory cell formation. This review explores the role of cytokine-activated NK cells as vaccine-induced effector cells and in recall responses and their potential contribution to vaccine and adjuvant development.

Published

2018