Your search keyword '"Luke C. Davies"' showing total 40 results

1. Oxylipin metabolism is controlled by mitochondrial β-oxidation during bacterial inflammation

Author

Mariya Misheva, Konstantinos Kotzamanis, Luke C. Davies, Victoria J. Tyrrell, Patricia R. S. Rodrigues, Gloria A. Benavides, Christine Hinz, Robert C. Murphy, Paul Kennedy, Philip R. Taylor, Marcela Rosas, Simon A. Jones, James E. McLaren, Sumukh Deshpande, Robert Andrews, Nils Helge Schebb, Magdalena A. Czubala, Mark Gurney, Maceler Aldrovandi, Sven W. Meckelmann, Peter Ghazal, Victor Darley-Usmar, Daniel A. White, and Valerie B. O’Donnell

Subjects

Science

Abstract

Oxylipins are lipid mediators generated during infection for regulating inflammatory responses, but how they are removed is not completely clear. Here the authors show that cellular oxylipin removal is linked to mitochondria β-oxidation by CPT1, a mitochondria lipid importer protein, to serve as a metabolic checkpoint for oxylipin homeostasis and inflammation.

Published

2022

2. Effective In Vivo Gene Modification in Mouse Tissue-Resident Peritoneal Macrophages by Intraperitoneal Delivery of Lentiviral Vectors

Author

Natacha Ipseiz, Magdalena A. Czubala, Valentina M.T. Bart, Luke C. Davies, Robert H. Jenkins, Paul Brennan, and Philip R. Taylor

Subjects

Genetics, QH426-470, Cytology, QH573-671

Abstract

Tissue-resident macrophages exhibit specialized phenotypes dependent on their in vivo physiological niche. Investigation of their function often relies upon complex whole mouse transgenic studies. While some appropriate lineage-associated promoters exist, there are no options for tissue-specific targeting of macrophages. We have developed full protocols for in vivo productive infection (defined by stable transgene expression) of tissue-resident macrophages with lentiviral vectors, enabling RNA and protein overexpression, including expression of small RNA species such as shRNA, to knock down and modulate gene expression. These approaches allow robust infection of peritoneal tissue-resident macrophages without significant infection of other cell populations. They permit rapid functional study of macrophages in homeostatic and inflammatory settings, such as thioglycolate-induced peritonitis, while maintaining the cells in their physiological context. Here we provide detailed protocols for the whole workflow: viral production, purification, and quality control; safety considerations for administration of the virus to mice; and assessment of in vivo transduction efficiency and the low background levels of inflammation induced by the virus. In summary, we present a quick and accessible protocol for the rapid assessment of gene function in peritoneal tissue-resident macrophages in vivo.

Published

2020

3. Nitric oxide orchestrates metabolic rewiring in M1 macrophages by targeting aconitase 2 and pyruvate dehydrogenase

Author

Erika M. Palmieri, Marieli Gonzalez-Cotto, Walter A. Baseler, Luke C. Davies, Bart Ghesquière, Nunziata Maio, Christopher M. Rice, Tracey A. Rouault, Teresa Cassel, Richard M. Higashi, Andrew N. Lane, Teresa W.-M. Fan, David A. Wink, and Daniel W. McVicar

Subjects

Science

Abstract

Production of inflammatory mediators by M1-polarized macrophages is thought to rely on suppression of mitochondrial metabolism in favor of glycolysis. Refining this concept, here the authors define metabolic targets of nitric oxide as responsible for the mitochondrial rewiring resulting from polarization.

Published

2020

4. Tumour-elicited neutrophils engage mitochondrial metabolism to circumvent nutrient limitations and maintain immune suppression

Author

Christopher M. Rice, Luke C. Davies, Jeff J. Subleski, Nunziata Maio, Marieli Gonzalez-Cotto, Caroline Andrews, Nimit L. Patel, Erika M. Palmieri, Jonathan M. Weiss, Jung-Min Lee, Christina M. Annunziata, Tracey A. Rouault, Scott K. Durum, and Daniel W. McVicar

Subjects

Science

Abstract

Neutrophils normally fulfil their metabolic demands by glycolysis and have limited mitochondrial activity. Here the authors show that tumours promote neutrophils adapted to oxidative mitochondria metabolism that function in the glucose-restrained tumour microenvironment to promote tumour growth by maintaining local immune suppression.

Published

2018

5. Peritoneal tissue-resident macrophages are metabolically poised to engage microbes using tissue-niche fuels

Author

Luke C. Davies, Christopher M. Rice, Erika M. Palmieri, Philip R. Taylor, Douglas B. Kuhns, and Daniel W. McVicar

Subjects

Science

Abstract

Tissue-resident marcophages have both generic and tissue-specific functions, but how the latter functions are imbued is still unclear. Here the authors show that peritoneal macrophages express a specialised genetic programme to utilise the locally enriched glutamate for a metabolic setting that facilitates protective in situ immunity.

Published

2017

6. Autocrine IL-10 functions as a rheostat for M1 macrophage glycolytic commitment by tuning nitric oxide production

Author

Walter A. Baseler, Luke C. Davies, Laura Quigley, Lisa A. Ridnour, Jonathan M. Weiss, S. Perwez Hussain, David A. Wink, and Daniel W. McVicar

Subjects

Medicine (General), R5-920, Biology (General), QH301-705.5

Abstract

Inflammatory maturation of M1 macrophages by proinflammatory stimuli such as toll like receptor ligands results in profound metabolic reprogramming resulting in commitment to aerobic glycolysis as evidenced by repression of mitochondrial oxidative phosphorylation (OXPHOS) and enhanced glucose utilization. In contrast, “alternatively activated” macrophages adopt a metabolic program dominated by fatty acid-fueled OXPHOS. Despite the known importance of these developmental stages on the qualitative aspects of an inflammatory response, relatively little is know regarding the regulation of these metabolic adjustments. Here we provide evidence that the immunosuppressive cytokine IL-10 defines a metabolic regulatory loop. Our data show for the first time that lipopolysaccharide (LPS)-induced glycolytic flux controls IL-10-production via regulation of mammalian target of rapamycin (mTOR) and that autocrine IL-10 in turn regulates macrophage nitric oxide (NO) production. Genetic and pharmacological manipulation of IL-10 and nitric oxide (NO) establish that metabolically regulated autocrine IL-10 controls glycolytic commitment by limiting NO-mediated suppression of OXPHOS. Together these data support a model where autocine IL-10 production is controlled by glycolytic flux in turn regulating glycolytic commitment by preserving OXPHOS via suppression of NO. We propose that this IL-10-driven metabolic rheostat maintains metabolic equilibrium during M1 macrophage differentiation and that perturbation of this regulatory loop, either directly by exogenous cellular sources of IL-10 or indirectly via limitations in glucose availability, skews the cellular metabolic program altering the balance between inflammatory and immunosuppressive phenotypes.

Published

2016

7. Immune and metabolic markers for identifying and investigating severe Coronavirus disease and Sepsis in children and young people (pSeP/COVID ChYP study): protocol for a prospective cohort study

Author

Richard Skone, Daniel White, Bethan Phillips, Jennifer Evans, Robert Andrews, Benjamin Saunders, Kerry Hood, Mallinath Chakraborty, Sarah Edkins, Barbara Paquete, Sian Foulkes, Anna Barrow, Siske Struik, Valerie O'Donnell, Sara Ali, Patrícia R S Rodrigues, Angela Strang, Summia Zaher, Simran Sharma, Luke C Davies, Linda Moet, James E McLaren, Gareth L Watson, Peter Ghazal, Edward Parkinson, Sivakumar Oruganti, William John Watkins, Selyf Shapey, Rim al Samsam, Malcolm Gajraj, Michelle Jardine, Jong Eun Song, Lloyd Abood, Sarah Joanne Kotecha, Awen Evans, Iona Buchanan, Susan Bowes, Begum Ali, Maya Gore, Rhian Thomas-Turner, Federico Liberatore, and Thomas Woolley

Subjects

Medicine

Abstract

Introduction Early recognition and appropriate management of paediatric sepsis are known to improve outcomes. A previous system’s biology investigation of the systemic immune response in neonates to sepsis identified immune and metabolic markers that showed high accuracy for detecting bacterial infection. Further gene expression markers have also been reported previously in the paediatric age group for discriminating sepsis from control cases. More recently, specific gene signatures were identified to discriminate between COVID-19 and its associated inflammatory sequelae. Through the current prospective cohort study, we aim to evaluate immune and metabolic blood markers which discriminate between sepses (including COVID-19) from other acute illnesses in critically unwell children and young persons, up to 18 years of age.Methods and analysis We describe a prospective cohort study for comparing the immune and metabolic whole-blood markers in patients with sepsis, COVID-19 and other illnesses. Clinical phenotyping and blood culture test results will provide a reference standard to evaluate the performance of blood markers from the research sample analysis. Serial sampling of whole blood (50 μL each) will be collected from children admitted to intensive care and with an acute illness to follow time dependent changes in biomarkers. An integrated lipidomics and RNASeq transcriptomics analyses will be conducted to evaluate immune-metabolic networks that discriminate sepsis and COVID-19 from other acute illnesses. This study received approval for deferred consent.Ethics and dissemination The study has received research ethics committee approval from the Yorkshire and Humber Leeds West Research Ethics Committee 2 (reference 20/YH/0214; IRAS reference 250612). Submission of study results for publication will involve making available all anonymised primary and processed data on public repository sites.Trial registration number NCT04904523.

Published

2023

8. mSep: investigating physiological and immune-metabolic biomarkers in septic and healthy pregnant women to predict feto-maternal immune health – a prospective observational cohort study protocol

Author

Daniel White, Sarah Bell, Shaun Oram, Robert Andrews, Mallinath Chakraborty, Sarah Edkins, W John Watkins, Patrícia R S Rodrigues, Angela Strang, Summia Zaher, Simran Sharma, Luke C Davies, Linda Moet, James E McLaren, Valerie B O’Donnell, Peter Ghazal, Edward Parkinson, Nicos Angelopoulos, Freya Shepherd, Kate Megan Megan Davies, Kate Siddall, Vikki Keeping, Kathryn Simpson, Federica Faggian, Maryanne Bray, Claire Bertorelli, Rachel E Collis, and Mario Labeta

Subjects

Medicine

Abstract

Introduction Maternal sepsis remains a leading cause of death in pregnancy. Physiological adaptations to pregnancy obscure early signs of sepsis and can result in delays in recognition and treatment. Identifying biomarkers that can reliably diagnose sepsis will reduce morbidity and mortality and antibiotic overuse. We have previously identified an immune-metabolic biomarker network comprising three pathways with a >99% accuracy for detecting bacterial neonatal sepsis. In this prospective study, we will describe physiological parameters and novel biomarkers in two cohorts—healthy pregnant women and pregnant women with suspected sepsis—with the aim of mapping pathophysiological drivers and evaluating predictive biomarkers for diagnosing maternal sepsis.Methods and analysis Women aged over 18 with an ultrasound-confirmed pregnancy will be recruited to a pilot and two main study cohorts. The pilot will involve blood sample collection from 30 pregnant women undergoing an elective caesarean section. Cohort A will follow 100 healthy pregnant women throughout their pregnancy journey, with collection of blood samples from participants at routine time points in their pregnancy: week 12 ‘booking’, week 28 and during labour. Cohort B will follow 100 pregnant women who present with suspected sepsis in pregnancy or labour and will have at least two blood samples taken during their care pathway. Study blood samples will be collected during routine clinical blood sampling. Detailed medical history and physiological parameters at the time of blood sampling will be recorded, along with the results of routine biochemical tests, including C reactive protein, lactate and white blood cell count. In addition, study blood samples will be processed and analysed for transcriptomic, lipidomic and metabolomic analyses and both qualitative and functional immunophenotyping.Ethics and dissemination Ethical approval has been obtained from the Wales Research Ethics Committee 2 (SPON1752-19, 30 October 2019).Trial registration number NCT05023954.

Published

2022

9. Immune and metabolic markers for identifying and investigating severe Coronavirus disease and Sepsis in children and young people (pSeP/COVID ChYP study): protocol for a prospective cohort study

Author

Sivakumar Oruganti, Patrícia R S Rodrigues, Daniel White, William John Watkins, Selyf Shapey, Anna Barrow, Rim al Samsam, Sara Ali, Malcolm Gajraj, Richard Skone, Michelle Jardine, Jennifer Evans, Siske Struik, Jong Eun Song, Lloyd Abood, Barbara Paquete, Sian Foulkes, Benjamin Saunders, Angela Strang, Sarah Joanne Kotecha, Bethan Phillips, Awen Evans, Iona Buchanan, Susan Bowes, Begum Ali, Maya Gore, Rhian Thomas-Turner, Robert Andrews, Summia Zaher, Simran Sharma, Mallinath Chakraborty, Edward Parkinson, Federico Liberatore, Thomas Woolley, Sarah Edkins, Luke C Davies, Linda Moet, James E McLaren, Gareth L Watson, Valerie O'Donnell, Kerry Hood, and Peter Ghazal

Subjects

General Medicine

Abstract

IntroductionEarly recognition and appropriate management of paediatric sepsis are known to improve outcomes. A previous system’s biology investigation of the systemic immune response in neonates to sepsis identified immune and metabolic markers that showed high accuracy for detecting bacterial infection. Further gene expression markers have also been reported previously in the paediatric age group for discriminating sepsis from control cases. More recently, specific gene signatures were identified to discriminate between COVID-19 and its associated inflammatory sequelae. Through the current prospective cohort study, we aim to evaluate immune and metabolic blood markers which discriminate between sepses (including COVID-19) from other acute illnesses in critically unwell children and young persons, up to 18 years of age.Methods and analysisWe describe a prospective cohort study for comparing the immune and metabolic whole-blood markers in patients with sepsis, COVID-19 and other illnesses. Clinical phenotyping and blood culture test results will provide a reference standard to evaluate the performance of blood markers from the research sample analysis. Serial sampling of whole blood (50 μL each) will be collected from children admitted to intensive care and with an acute illness to follow time dependent changes in biomarkers. An integrated lipidomics and RNASeq transcriptomics analyses will be conducted to evaluate immune-metabolic networks that discriminate sepsis and COVID-19 from other acute illnesses. This study received approval for deferred consent.Ethics and disseminationThe study has received research ethics committee approval from the Yorkshire and Humber Leeds West Research Ethics Committee 2 (reference 20/YH/0214; IRAS reference 250612). Submission of study results for publication will involve making available all anonymised primary and processed data on public repository sites.Trial registration numberNCT04904523.

Published

2023

10. nSeP: immune and metabolic biomarkers for early detection of neonatal sepsis—protocol for a prospective multicohort study

Author

Mallinath Chakraborty, Patrícia R S Rodrigues, W John Watkins, Angela Hayward, Alok Sharma, Rachel Hayward, Elisa Smit, Rebekka Jones, Nitin Goel, Amar Asokkumar, Jennifer Calvert, David Odd, Ian Morris, Cora Doherty, Sian Elliott, Angela Strang, Robert Andrews, Summia Zaher, Simran Sharma, Sarah Bell, Siva Oruganti, Claire Smith, Judith Orme, Sarah Edkins, Marie Craigon, Daniel White, Widad Dantoft, Luke C Davies, Linda Moet, James E McLaren, Samantha Clarkstone, Gareth L Watson, Kerenza Hood, Sailesh Kotecha, B. Paul Morgan, Valerie B O’Donnell, and Peter Ghazal

Subjects

immunology, perinatology, neonatal intensive & critical care, Paediatrics, General Medicine

Abstract

IntroductionDiagnosing neonatal sepsis is heavily dependent on clinical phenotyping as culture-positive body fluid has poor sensitivity, and existing blood biomarkers have poor specificity.A combination of machine learning, statistical and deep pathway biology analyses led to the identification of a tripartite panel of biologically connected immune and metabolic markers that showed greater than 99% accuracy for detecting bacterial infection with 100% sensitivity. The cohort study described here is designed as a large-scale clinical validation of this previous work.Methods and analysisThis multicentre observational study will prospectively recruit a total of 1445 newborn infants (all gestations)—1084 with suspected early—or late-onset sepsis, and 361 controls—over 4 years. A small volume of whole blood will be collected from infants with suspected sepsis at the time of presentation. This sample will be used for integrated transcriptomic, lipidomic and targeted proteomics profiling. In addition, a subset of samples will be subjected to cellular phenotype and proteomic analyses. A second sample from the same patient will be collected at 24 hours, with an opportunistic sampling for stool culture. For control infants, only one set of blood and stool sample will be collected to coincide with clinical blood sampling. Along with detailed clinical information, blood and stool samples will be analysed and the information will be used to identify and validate the efficacy of immune-metabolic networks in the diagnosis of bacterial neonatal sepsis and to identify new host biomarkers for viral sepsis.Ethics and disseminationThe study has received research ethics committee approval from the Wales Research Ethics Committee 2 (reference 19/WA/0008) and operational approval from Health and Care Research Wales. Submission of study results for publication will involve making available all anonymised primary and processed data on public repository sites.Trial registration numberNCT03777670

Published

2021

11. Immune-metabolic adaptations in pregnancy: A potential stepping-stone to sepsis

Author

Simran Sharma, Patricia R.S. Rodrigues, Summia Zaher, Luke C. Davies, and Peter Ghazal

Subjects

Pregnancy, Placenta, Sepsis, Humans, Homeostasis, Female, General Medicine, Pregnancy Complications, Infectious, Adaptation, Physiological, General Biochemistry, Genetics and Molecular Biology

Abstract

Physiological shifts during pregnancy predispose women to a higher risk of developing sepsis resulting from a maladapted host-response to infection. Insightful studies have delineated subtle point-changes to the immune system during pregnancy. Here, we present an overlay of these point-changes, asking what changes and when, at a physiological, cellular, and molecular systems-level in the context of sepsis. We identify distinct immune phases in pregnancy delineated by placental hormone-driven changes in homeostasis setpoints of the immune and metabolic systems that subtly mirrors changes observed in sepsis. We propose that pregnancy immune-metabolic setpoint changes impact feedback thresholds that increase risk for a maladapted host-response to infection and thus act as a stepping-stone to sepsis. Defining maternal immune-metabolic setpoint changes is not only vital for tailoring the right diagnostic tools for early management of maternal sepsis but will facilitate an unravelling of the pathophysiological pathways that predispose an individual to sepsis.

Published

2022

12. P042 CHARACTERIZATION OF INNATE AND ADAPTIVE IMMUNE CELLS INVOLVED IN THE FOREIGN BODY REACTION TO POLYPROPYLENE MESHES IN THE HUMAN ABDOMEN

Author

Pascal Achenbach, Uwe Klinge, Luke C. Davies, and Axel Dievernich

Subjects

medicine.anatomical_structure, Immune system, business.industry, medicine, Abdomen, Surgery, Foreign body, medicine.disease, business, Cell biology

Abstract

Aim Polypropylene (PP) mesh is widely used to reinforce tissues. The foreign body reaction (FBR) to the implant is dominated by innate immune cells, especially macrophages. However, considerable numbers of adaptive immune cells have also been regularly observed, which appear to play a crucial role in the long-term host response. This study investigated the FBR to seven human PP meshes, which were removed from the abdomen for recurrence after a median of one year. Material and Methods Using immunofluorescence microscopy and distance maps, the FBR was spatially analyzed for various innate (e.g., CD68+ macrophages, CD56+ NK) and adaptive immune cells (CD3+ T, CD4+ T-helper, CD8+ cytotoxic, FoxP3+ T-regulatory, CD20+ B) as well as “conventional” immune cells (defined as cells expressing their specific immune cell marker without co-expressing CD68). Results T-helper cells (19%) and regulatory T-cells (25%) were present at comparable rates to macrophages, and clustered significantly toward the mesh fibers. For all cell types the lowest proportions of “conventional” cells (< 60%) were observed at the mesh–tissue interface, but increased considerably at about 50–100 µm, indicating reduced stimulation with rising distance to the mesh fibers. Conclusions Both innate and adaptive immune cells participate in the chronic FBR to PP meshes with T cells and macrophages being the predominant cell types, respectively. Furthermore, many cells present a “hybrid” pattern near the mesh fibers. The complexity of the local immune reaction may explain why approaches focusing on specific cell types have not been very successful in reducing the chronic FBR.

Published

2021

13. mSep: investigating physiological and immune-metabolic biomarkers in septic and healthy pregnant women to predict feto-maternal immune health – a prospective observational cohort study protocol

Author

Simran Sharma, Summia Zaher, Patrícia R S Rodrigues, Luke C Davies, Sarah Edkins, Angela Strang, Mallinath Chakraborty, W John Watkins, Robert Andrews, Edward Parkinson, Nicos Angelopoulos, Linda Moet, Freya Shepherd, Kate Megan Megan Davies, Daniel White, Shaun Oram, Kate Siddall, Vikki Keeping, Kathryn Simpson, Federica Faggian, Maryanne Bray, Claire Bertorelli, Sarah Bell, Rachel E Collis, James E McLaren, Mario Labeta, Valerie B O’Donnell, and Peter Ghazal

Subjects

Adult, Adolescent, Cesarean Section, Infant, Newborn, General Medicine, Anti-Bacterial Agents, Cohort Studies, Observational Studies as Topic, C-Reactive Protein, Pre-Eclampsia, Pregnancy, Sepsis, Lactates, Humans, Female, Pregnant Women, Prospective Studies, Pregnancy Complications, Infectious, Biomarkers

Abstract

IntroductionMaternal sepsis remains a leading cause of death in pregnancy. Physiological adaptations to pregnancy obscure early signs of sepsis and can result in delays in recognition and treatment. Identifying biomarkers that can reliably diagnose sepsis will reduce morbidity and mortality and antibiotic overuse. We have previously identified an immune-metabolic biomarker network comprising three pathways with a >99% accuracy for detecting bacterial neonatal sepsis. In this prospective study, we will describe physiological parameters and novel biomarkers in two cohorts—healthy pregnant women and pregnant women with suspected sepsis—with the aim of mapping pathophysiological drivers and evaluating predictive biomarkers for diagnosing maternal sepsis.Methods and analysisWomen aged over 18 with an ultrasound-confirmed pregnancy will be recruited to a pilot and two main study cohorts. The pilot will involve blood sample collection from 30 pregnant women undergoing an elective caesarean section. Cohort A will follow 100 healthy pregnant women throughout their pregnancy journey, with collection of blood samples from participants at routine time points in their pregnancy: week 12 ‘booking’, week 28 and during labour. Cohort B will follow 100 pregnant women who present with suspected sepsis in pregnancy or labour and will have at least two blood samples taken during their care pathway. Study blood samples will be collected during routine clinical blood sampling. Detailed medical history and physiological parameters at the time of blood sampling will be recorded, along with the results of routine biochemical tests, including C reactive protein, lactate and white blood cell count. In addition, study blood samples will be processed and analysed for transcriptomic, lipidomic and metabolomic analyses and both qualitative and functional immunophenotyping.Ethics and disseminationEthical approval has been obtained from the Wales Research Ethics Committee 2 (SPON1752-19, 30 October 2019).Trial registration numberNCT05023954.

Published

2022

14. Effective In Vivo Gene Modification in Mouse Tissue-Resident Peritoneal Macrophages by Intraperitoneal Delivery of Lentiviral Vectors

Author

Robert H. Jenkins, Luke C. Davies, Valentina M T Bart, Philip R. Taylor, Natacha Ipseiz, Magdalena A. Czubala, and Paul Brennan

Subjects

0301 basic medicine, Small RNA, lcsh:QH426-470, Transgene, Cell, Inflammation, Biology, Article, Small hairpin RNA, Transduction (genetics), 03 medical and health sciences, 0302 clinical medicine, In vivo, Gene expression, medicine, Genetics, lcsh:QH573-671, Molecular Biology, 030304 developmental biology, 0303 health sciences, lcsh:Cytology, Correction, Cell biology, 3. Good health, lcsh:Genetics, 030104 developmental biology, medicine.anatomical_structure, 030220 oncology & carcinogenesis, Molecular Medicine, medicine.symptom

Abstract

Tissue-resident macrophages exhibit specialized phenotypes dependent on their in vivo physiological niche. Investigation of their function often relies upon complex whole mouse transgenic studies. While some appropriate lineage-associated promoters exist, there are no options for tissue-specific targeting of macrophages. We have developed full protocols for in vivo productive infection (defined by stable transgene expression) of tissue-resident macrophages with lentiviral vectors, enabling RNA and protein overexpression, including expression of small RNA species such as shRNA, to knock down and modulate gene expression. These approaches allow robust infection of peritoneal tissue-resident macrophages without significant infection of other cell populations. They permit rapid functional study of macrophages in homeostatic and inflammatory settings, such as thioglycolate-induced peritonitis, while maintaining the cells in their physiological context. Here we provide detailed protocols for the whole workflow: viral production, purification, and quality control; safety considerations for administration of the virus to mice; and assessment of in vivo transduction efficiency and the low background levels of inflammation induced by the virus. In summary, we present a quick and accessible protocol for the rapid assessment of gene function in peritoneal tissue-resident macrophages in vivo., Graphical Abstract

Published

2019

15. Prostaglandin E2 promotes intestinal inflammation via inhibiting microbiota-dependent regulatory T cells

Author

Marie Goepp, Konstantinos Gkikas, Konstantinos Gerasimidis, Luke C. Davies, Stephen M. Anderton, Jürgen Schwarze, Xue-Feng Li, Calum T. Robb, Valerie B. O'Donnell, Sarah E. M. Howie, Gwo-Tzer Ho, Victoria J. Tyrrell, Bin-Zhi Qian, Chengcan Yao, Alexander Adima, Hatti X. Yao, Shuh Narumiya, Richard M. Breyer, Adriano G. Rossi, John P. Iredale, Robert Andrews, Xiaozhong Zheng, Danielle J. Smyth, Amil Mair, Sonja Vermeren, Rick M. Maizels, Damian J. Mole, Richard A. O’Connor, You Zhou, Jolinda Pollock, Siobhan Crittenden, and Mark J. Arends

Subjects

Immunology, Inflammation, chemical and pharmacologic phenomena, Biology, Gut flora, T-Lymphocytes, Regulatory, digestive system, Dinoprostone, 03 medical and health sciences, 0302 clinical medicine, Mediator, Interferon, Intestinal inflammation, medicine, Humans, Prostaglandin E2, Receptor, Research Articles, 030304 developmental biology, 0303 health sciences, Multidisciplinary, SciAdv r-articles, hemic and immune systems, Receptors, Prostaglandin E, EP2 Subtype, biology.organism_classification, Gastrointestinal Microbiome, Cell biology, stomatognathic diseases, 030220 oncology & carcinogenesis, Type I Interferon Receptor, lipids (amino acids, peptides, and proteins), medicine.symptom, Research Article, medicine.drug

Abstract

PGE2 inhibits Tregs and promotes intestinal inflammation through actions on mononuclear phagocytes and the gut microbiota., The gut microbiota fundamentally regulates intestinal homeostasis and disease partially through mechanisms that involve modulation of regulatory T cells (Tregs), yet how the microbiota-Treg cross-talk is physiologically controlled is incompletely defined. Here, we report that prostaglandin E2 (PGE2), a well-known mediator of inflammation, inhibits mucosal Tregs in a manner depending on the gut microbiota. PGE2 through its receptor EP4 diminishes Treg-favorable commensal microbiota. Transfer of the gut microbiota that was modified by PGE2-EP4 signaling modulates mucosal Treg responses and exacerbates intestinal inflammation. Mechanistically, PGE2-modified microbiota regulates intestinal mononuclear phagocytes and type I interferon signaling. Depletion of mononuclear phagocytes or deficiency of type I interferon receptor diminishes PGE2-dependent Treg inhibition. Together, our findings provide emergent evidence that PGE2-mediated disruption of microbiota-Treg communication fosters intestinal inflammation.

Published

2021

16. Innate immunology in COVID-19 - a living review. Part II: dysregulated inflammation drives immunopathology

Author

Ellie Pring, Ruth Jones, F Lu, Rodrigues Prs., Bart Vmt., Michael Tellier, Ester Gea-Mallorquí, S Maleki-Toyserkani, Aljawharah Alrubayyi, Felix Richter, D O Scourfield, Luke C. Davies, and C.R. Coveney

Subjects

0301 basic medicine, Neutrophils, Short Communication, Inflammation, NK cells, Monocytes, 03 medical and health sciences, 0302 clinical medicine, Immune system, Fibrosis, Interferon, Immunopathology, medicine, Innate immune system, business.industry, Macrophages, COVID-19, Interleukin, General Medicine, Neutrophil extracellular traps, medicine.disease, 030104 developmental biology, 030220 oncology & carcinogenesis, Immunology, Innate immunology, medicine.symptom, business, medicine.drug

Abstract

The current pandemic of coronavirus disease 2019 (COVID-19) caused by severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) poses a global health crisis and will likely continue to impact public health for years. As the effectiveness of the innate immune response is crucial to patient outcome, huge efforts have been made to understand how dysregulated immune responses may contribute to disease progression. Here we have reviewed current knowledge of cellular innate immune responses to SARS-CoV-2 infection, highlighting areas for further investigation and suggesting potential strategies for intervention. We conclude that in severe COVID-19 initial innate responses, primarily type I interferon, are suppressed or sabotaged which results in an early interleukin (IL)-6, IL-10 and IL-1β-enhanced hyperinflammation. This inflammatory environment is driven by aberrant function of innate immune cells: monocytes, macrophages and natural killer cells dispersing viral pathogen-associated molecular patterns and damage-associated molecular patterns into tissues. This results in primarily neutrophil-driven pathology including fibrosis that causes acute respiratory distress syndrome. Activated leukocytes and neutrophil extracellular traps also promote immunothrombotic clots that embed into the lungs and kidneys of severe COVID-19 patients, are worsened by immobility in the intensive care unit and are perhaps responsible for the high mortality. Therefore, treatments that target inflammation and coagulation are promising strategies for reducing mortality in COVID-19., Graphical Abstract Graphical Abstract

Published

2021

17. Neutrophilia, lymphopenia and myeloid dysfunction: a living review of the quantitative changes to innate and adaptive immune cells which define COVID-19 pathology

Author

Tehmina Bharuchq, Bruce MacLachlan, Ceri Fielding, Adrian L Smith, Fadi Issa, Emily Thornton, Raphael Sanches Peres, Calliope A Dendrou, Dorothée L Berthold, Liliana Cifuentes, Alicia Teijeira Crespo, Elizabeth H Mann, Arvind Sami, Anne Chauveau, Dominic S Alonzi, Anís Gammage, Fabian Fischer, Valentina M T Bart, Fangfang Lu, Miriam O'Hanlon, Lynn B Dustin, Pragati Sabberwal, Ewoud B. Compeer, Mariana Borsa, Rowie Borst, Hannah Almuttaqi, David J Ahern, Eleanor J Pring, Emma Jones, Ester Gea-Mallorquí, Kate Liddiard, Dingxi Zhou, Amy Cross, Sara Danielli, Max Quastel, Shayda Maleki-Toyserkani, Owen R Moon, Ruban Rex Peter Durairaj, Vicky Batchelor, Barbora Schonfeldova, Angus K T Wann, Lorenzo Capitani, Petros Ligoxygakis, Sandra Dimonte, Clara Eléonore Pavillet, Lion F K Uhl, Luke C Davies, Kristin Ladell, Stephanie Jean Hanna, Felix Richter, Freya R Shepherd, Sarah Hulin-Curtis, Stephanie Burnell, Amy Susan Codd, Anita Milicic, Quentin Sattentau, Juliane Brun, David Oliver Scourfield, Sophie Reed, Jan Rehwinkel, Ghada Alsaleh, D Oliver Scourfield, Michael Tellier, Reginald James Matthews, Eleanor Pring, Emma Mitchell, Anna Katharina Simon, Joseph D Wilson, Niamh Richmond, Van Dien Nguyen, Sarah N Lauder, Zihan Zhu, Tharini A Selvakumar, Ana Pires, Cariad Shorten, Richard Williams, Erinke van Grinsven, Sarah Galloway, Aljawharah Alrubayyi, Stephanie J. Hanna, Felix Clemens Richter, Julie M Mazet, Dimitra Peppa, Clarissa Coveney, Awen Gallimore, Cornelia Heuberger, Owen Moon, Ruth Jones, Helene Borrmann, Arthur Dyer, Lucy Chapman, Jelena S Bezbradica, Andrew Godkin, Rebecca Bayliss, Amy S. Codd, Anna M Marzeda, Athena Cavounidis, Patrícia R S Rodrigues, Alice J B Robinson, and Ewoud Bernardus Compeer

Subjects

Myeloid, Coronavirus disease 2019 (COVID-19), severity, Review Article, clinical, AcademicSubjects/MED00160, cell counts, recovery, Immune system, neutrophils, Lymphopenia, neutrophilia, Medicine, Lymphocytes, B cells, SARS-CoV-2, business.industry, General Medicine, Neutrophilia, medicine.anatomical_structure, Immunology, AcademicSubjects/SCI00960, prognosis, AcademicSubjects/MED00770, medicine.symptom, monocytes, business, AcademicSubjects/MED00690

Abstract

Destabilization of balanced immune cell numbers and frequencies is a common feature of viral infections. This occurs due to, and further enhances, viral immune evasion and survival. Since the discovery of the Severe Acute Respiratory Syndrome coronavirus 2 (SARS-CoV-2), which manifests in coronavirus disease 2019 (COVID-19), a great number of studies have described the association between this virus and pathologically increased or decreased immune cell counts. In this review, we consider the absolute and relative changes to innate and adaptive immune cell numbers, in COVID-19. In severe disease particularly, neutrophils are increased, which can lead to inflammation and tissue damage. Dysregulation of other granulocytes, basophils and eosinophils represents an unusual COVID-19 phenomenon. Contrastingly, the impact on the different types of monocytes leans more strongly to an altered phenotype, e.g. HLA-DR expression, rather than numerical changes. However, it is the adaptive immune response that bears the most profound impact of SARS-CoV-2 infection. T cell lymphopenia correlates with increased risk of intensive care unit admission and death; therefore, this parameter is particularly important for clinical decision-making. Mild and severe diseases differ in the rate of immune cell counts returning to normal levels post disease. Tracking the recovery trajectories of various immune cell counts may also have implications for long-term COVID-19 monitoring. This review represents a snapshot of our current knowledge, showing that much has been achieved in a short period of time. Alterations in counts of distinct immune cells represent an accessible metric to inform patient care decisions or predict disease outcomes.

Published

2021

18. Characterization of innate and adaptive immune cells involved in the foreign body reaction to polypropylene meshes in the human abdomen

Author

Axel Dievernich, Uwe Klinge, Luke C. Davies, and Pascal Achenbach

Subjects

medicine.medical_specialty, Cell type, Myeloid, Polypropylenes, 03 medical and health sciences, 0302 clinical medicine, Immune system, Abdomen, medicine, Cytotoxic T cell, Humans, Herniorrhaphy, 030304 developmental biology, 0303 health sciences, Innate immune system, business.industry, Foreign-Body Reaction, FOXP3, Surgical Mesh, Acquired immune system, digestive system diseases, humanities, Cell biology, Surgery, stomatognathic diseases, medicine.anatomical_structure, surgical procedures, operative, 030220 oncology & carcinogenesis, business, CD8

Abstract

Hernia : the journal of hernias and abdominal wall surgery 26(1), 309-323 (2022). doi:10.1007/s10029-021-02396-7, Published by Springer, Paris

Published

2020

19. Prostaglandin E2 promotes intestinal inflammation via inhibiting microbiota-dependent regulatory T cells

Author

John P. Iredale, Stephen M. Anderton, Jürgen Schwarze, Sarah E. M. Howie, Luke C. Davies, Jolinda Pollock, Gwo-Tzer Ho, Alexander Adima, Xue-Feng Li, Amil Mair, Hatti X. Yao, Valerie B. O'Donnell, Richard M. Breyer, Adriano G. Rossi, Danielle J. Smyth, Xiaozhong Zheng, Victoria J. Tyrrell, Damian J. Mole, Shuh Narumiya, Bin-Zhi Qian, Chengcan Yao, Rick M. Maizels, Mark J. Arends, Richard A. O’Connor, You Zhou, Calum T. Robb, Robert Andrews, Siobhan Crittenden, Sonja Vermeren, and Marie Goepp

Subjects

Inflammation, Biology, Gut flora, biology.organism_classification, digestive system, Cell biology, Crosstalk (biology), Mediator, Interferon, Intestinal inflammation, medicine, lipids (amino acids, peptides, and proteins), Prostaglandin E2, medicine.symptom, Receptor, medicine.drug

Abstract

The gut microbiota fundamentally regulates intestinal homeostasis and disease partially through mechanisms that involve modulation of regulatory T cells (Tregs), yet how the microbiota-Treg crosstalk is physiologically controlled is incompletely defined. Here, we report that prostaglandin E2 (PGE2), a well-known mediator of inflammation, inhibits mucosal Tregs in a manner depending on the gut microbiota. PGE2 through its receptor EP4 diminishes Treg-favorable commensal microbiota. Transfer of the gut microbiota that was modified by PGE2-EP4 signaling modulates mucosal Treg responses and exacerbates intestinal inflammation. Mechanistically, PGE2-modified microbiota regulates intestinal mononuclear phagocytes and type I interferon signaling. Depletion of mononuclear phagocytes or deficiency of type I interferon receptor contracts PGE2-dependent Treg inhibition. Taken together, our findings provide emergent evidence that PGE2-mediated disruption of microbiota-Treg communication fosters intestinal inflammation.

Published

2020

20. Tissue‐resident macrophages actively suppress IL‐1beta release via a reactive prostanoid/IL‐10 pathway

Author

Magdalena A. Czubala, Robert J. Pickering, Avril A. B. Robertson, Valerie B. O'Donnell, Selinda J. Orr, Luke C. Davies, Victoria J. Tyrrell, Dina Fathalla, Marcela Rosas, Philip R. Taylor, Natacha Ipseiz, and Clare E. Bryant

Subjects

Lipopolysaccharide, medicine.medical_treatment, Immunology, Interleukin-1beta, Mice, Transgenic, Prostacyclin, Article, IL‐10, General Biochemistry, Genetics and Molecular Biology, Prostacyclin synthase, Mice, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, GATA6 Transcription Factor, medicine, Animals, Molecular Biology, Transcription factor, 030304 developmental biology, Inflammation, 0303 health sciences, General Immunology and Microbiology, biology, prostacyclin, Activator (genetics), General Neuroscience, Inflammasome, Articles, Epoprostenol, macrophages, Interleukin-10, 3. Good health, Cell biology, Interleukin 10, Cytokine, chemistry, Macrophages, Peritoneal, biology.protein, 030217 neurology & neurosurgery, IL‐1beta, medicine.drug

Abstract

The alarm cytokine interleukin‐1β (IL‐1β) is a potent activator of the inflammatory cascade following pathogen recognition. IL‐1β production typically requires two signals: first, priming by recognition of pathogen‐associated molecular patterns leads to the production of immature pro‐IL‐1β; subsequently, inflammasome activation by a secondary signal allows cleavage and maturation of IL‐1β from its pro‐form. However, despite the important role of IL‐1β in controlling local and systemic inflammation, its overall regulation is still not fully understood. Here we demonstrate that peritoneal tissue‐resident macrophages use an active inhibitory pathway, to suppress IL‐1β processing, which can otherwise occur in the absence of a second signal. Programming by the transcription factor Gata6 controls the expression of prostacyclin synthase, which is required for prostacyclin production after lipopolysaccharide stimulation and optimal induction of IL‐10. In the absence of secondary signal, IL‐10 potently inhibits IL‐1β processing, providing a previously unrecognized control of IL‐1β in tissue‐resident macrophages., Resident peritoneal macrophages limit IL‐1β release following TLR activation, via a novel GATA6‐induced pathway involving prostacyclin and IL‐10.

Published

2020

21. Nitric oxide orchestrates metabolic rewiring in M1 macrophages by targeting aconitase 2 and pyruvate dehydrogenase

Author

Christopher M. Rice, Tracey A. Rouault, Richard M. Higashi, Teresa Cassel, Andrew N. Lane, Nunziata Maio, David A. Wink, Daniel W. McVicar, Marieli Gonzalez-Cotto, Teresa W.-M. Fan, Walter A. Baseler, Luke C. Davies, Erika M. Palmieri, and Bart Ghesquière

Subjects

0301 basic medicine, Science, Citric Acid Cycle, Nitric Oxide Synthase Type II, General Physics and Astronomy, Nitric Oxide, Article, Citric Acid, General Biochemistry, Genetics and Molecular Biology, Nitric oxide, Mice, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Mediator, Pyruvic Acid, Animals, Humans, lcsh:Science, Acute inflammation, Aconitate Hydratase, Inflammation, Mice, Knockout, Phagocytes, Multidisciplinary, Macrophages, Pyruvate Dehydrogenase Acetyl-Transferring Kinase, ACO2, Energy metabolism, General Chemistry, Metabolism, Hypoxia-Inducible Factor 1, alpha Subunit, Pyruvate dehydrogenase complex, In vitro, Mitochondria, Cell biology, Mice, Inbred C57BL, Glutamine, Citric acid cycle, 030104 developmental biology, Electron Transport Chain Complex Proteins, chemistry, 030220 oncology & carcinogenesis, lcsh:Q, Oxidoreductases

Abstract

Profound metabolic changes are characteristic of macrophages during classical activation and have been implicated in this phenotype. Here we demonstrate that nitric oxide (NO) produced by murine macrophages is responsible for TCA cycle alterations and citrate accumulation associated with polarization. 13C tracing and mitochondrial respiration experiments map NO-mediated suppression of metabolism to mitochondrial aconitase (ACO2). Moreover, we find that inflammatory macrophages reroute pyruvate away from pyruvate dehydrogenase (PDH) in an NO-dependent and hypoxia-inducible factor 1α (Hif1α)-independent manner, thereby promoting glutamine-based anaplerosis. Ultimately, NO accumulation leads to suppression and loss of mitochondrial electron transport chain (ETC) complexes. Our data reveal that macrophages metabolic rewiring, in vitro and in vivo, is dependent on NO targeting specific pathways, resulting in reduced production of inflammatory mediators. Our findings require modification to current models of macrophage biology and demonstrate that reprogramming of metabolism should be considered a result rather than a mediator of inflammatory polarization., Production of inflammatory mediators by M1-polarized macrophages is thought to rely on suppression of mitochondrial metabolism in favor of glycolysis. Refining this concept, here the authors define metabolic targets of nitric oxide as responsible for the mitochondrial rewiring resulting from polarization.

Published

2020

22. Tissue remodeling macrophages morphologically dominate at the interface of polypropylene surgical meshes in the human abdomen

Author

Uwe Klinge, Axel Dievernich, Pascal Achenbach, and Luke C. Davies

Subjects

Pathology, medicine.medical_specialty, Macrophage, Cell, Inflammation, Matrix (biology), Immunofluorescence, Polypropylenes, 03 medical and health sciences, 0302 clinical medicine, Foreign body reaction, Medicine, Animals, Humans, 030304 developmental biology, Mesh, Fluorescence microscopy, 0303 health sciences, medicine.diagnostic_test, business.industry, Macrophages, Abdominal Wall, Surgical Mesh, M2 Macrophage, Phenotype, Surgery, medicine.anatomical_structure, Microscopy, Fluorescence, 030220 oncology & carcinogenesis, Original Article, Collagen, medicine.symptom, business, CD163

Abstract

Background Mesh implants are widely used to reinforce the abdominal wall, although the inevitable inflammatory foreign body reaction (FBR) at the interface leads to complications. Macrophages are suspected to regulate the subsequent scar formation, but it is still unclear whether adequate fibrous scar formation with collagen deposition depends mainly on the presence of M1 or M2 macrophages. Methods This study investigated the FBR to seven human polypropylene meshes, which were removed after a median incorporation time of 1 year due to the primary complaint of recurrence. Using immunofluorescence, the FBR was examined in six regional zones with increasing distance from the mesh fibers up to 350 µm, based on the cell densities, macrophage M1 (CD86) and M2 (CD163, CD206) phenotypes, deposition of collagen-I and -III, and expression of matrix metalloproteinase-2 (MMP-2) and -8 as indicator of collagen degradation. Results All mesh–tissue complexes demonstrated a decrease in cell density and macrophages with distance to the mesh fibers. Overall, about 60% of the macrophages presented an M2 phenotype, whereas only 6% an M1 phenotype. Over 70% of macrophages showed co-expression with collagen-I or -III and over 50% with MMP-2. Conclusions The chronic FBR to polypropylene meshes is associated with an M2 macrophage response, which is accompanied by collagen deposition and MMP-2 expression. These findings challenge the idea that mainly M1 macrophages are related to inflammation and highlights that iatrogenic attempts to polarize these cells towards the M2 phenotype may not be a solution to ameliorate the long-term foreign body reaction.

Published

2020

23. CD68+ macrophages as crucial components of the foreign body reaction demonstrate an unconventional pattern of functional markers quantified by analysis with double fluorescence staining

Author

Luke C. Davies, Rene Tolba, Axel Dievernich, Uwe Klinge, and Bernd Klosterhalfen

Subjects

0301 basic medicine, Cell type, Materials science, Cell Survival, CD3, Lymphocyte, Biomedical Engineering, CD34, Antigens, Differentiation, Myelomonocytic, CD16, Polypropylenes, Antibodies, Biomaterials, 03 medical and health sciences, 0302 clinical medicine, Antigens, CD, medicine, Macrophage, Humans, Herniorrhaphy, Cell Proliferation, Fluorescent Dyes, Inflammation, biology, Foreign-Body Reaction, Macrophages, Surgical Mesh, Cell biology, Extracellular Matrix, 030104 developmental biology, medicine.anatomical_structure, Microscopy, Fluorescence, 030220 oncology & carcinogenesis, biology.protein, Polyvinyls, Stem cell, CD8, Biomarkers

Abstract

Implants like meshes for the reinforcement of tissues implement the formation of a persistent inflammation with an ambient fibrotic reaction. In the inflammatory infiltrate several distinct cell types have been identified, but CD68+ macrophages are supposed to be most important. To investigate the collaboration among the various cell types within the infiltrate we performed at explanted meshes from humans double fluorescence staining with CD68 as a constant marker and a variety of other antibodies as the second marker. The list of second markers includes lymphocytes (CD3, CD4, CD8, CD16, CD56, FoxP3, and CD11b) stem cells (CD34), leucocytes (CD45, CD15), macrophages (CD86, CD105, CD163, and CD206); deposition of EC matrix (collagen‐I, collagen‐III, MMP2, and MMP8); Ki67 as a marker for proliferation; and the tyrosine‐protein kinase receptor AXL. The present study demonstrates within the inflammatory infiltrate the abundant capability of CD68+ cells to co‐express a huge variety of other markers, including those of lymphocytes, varying between 5 and 83% of investigated cells. The observation of co‐staining was not restricted to a specific polymer but was seen with polypropylene fibers as well as with fibers made of polyvinylidene fluoride, although with differences in co‐expression rates. The persisting variability of these cells without the functional reduction toward differentiated mature cell types may favor the lack of healing at the interface of meshes.

Published

2019

24. Autocrine IL-10 functions as a rheostat for M1 macrophage glycolytic commitment by tuning nitric oxide production

Author

Jonathan M. Weiss, David A. Wink, Laura Quigley, S. Perwez Hussain, Lisa A. Ridnour, Luke C. Davies, Daniel W. McVicar, and Walter A. Baseler

Subjects

Lipopolysaccharides, 0301 basic medicine, medicine.medical_treatment, Clinical Biochemistry, Biology, Nitric Oxide, Autocrine Communication, Biochemistry, Oxidative Phosphorylation, Proinflammatory cytokine, Nitric oxide, Mice, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, medicine, Animals, Humans, Glycolysis, Autocrine signalling, lcsh:QH301-705.5, Cells, Cultured, PI3K/AKT/mTOR pathway, lcsh:R5-920, Macrophages, TOR Serine-Threonine Kinases, Organic Chemistry, Cell Differentiation, Macrophage Activation, Interleukin-10, Mitochondria, Glucose, 030104 developmental biology, Cytokine, lcsh:Biology (General), chemistry, Anaerobic glycolysis, 030220 oncology & carcinogenesis, lcsh:Medicine (General), Research Paper

Abstract

Inflammatory maturation of M1 macrophages by proinflammatory stimuli such as toll like receptor ligands results in profound metabolic reprogramming resulting in commitment to aerobic glycolysis as evidenced by repression of mitochondrial oxidative phosphorylation (OXPHOS) and enhanced glucose utilization. In contrast, “alternatively activated” macrophages adopt a metabolic program dominated by fatty acid-fueled OXPHOS. Despite the known importance of these developmental stages on the qualitative aspects of an inflammatory response, relatively little is know regarding the regulation of these metabolic adjustments. Here we provide evidence that the immunosuppressive cytokine IL-10 defines a metabolic regulatory loop. Our data show for the first time that lipopolysaccharide (LPS)-induced glycolytic flux controls IL-10-production via regulation of mammalian target of rapamycin (mTOR) and that autocrine IL-10 in turn regulates macrophage nitric oxide (NO) production. Genetic and pharmacological manipulation of IL-10 and nitric oxide (NO) establish that metabolically regulated autocrine IL-10 controls glycolytic commitment by limiting NO-mediated suppression of OXPHOS. Together these data support a model where autocine IL-10 production is controlled by glycolytic flux in turn regulating glycolytic commitment by preserving OXPHOS via suppression of NO. We propose that this IL-10-driven metabolic rheostat maintains metabolic equilibrium during M1 macrophage differentiation and that perturbation of this regulatory loop, either directly by exogenous cellular sources of IL-10 or indirectly via limitations in glucose availability, skews the cellular metabolic program altering the balance between inflammatory and immunosuppressive phenotypes., Graphical abstract fx1, Highlights • Optimal macrophage IL-10 production requires un-restricted utilization of glucose. • IL-10 production is limited by AMP Kinase activation and subsequent TORC suppression. • Macrophage glycolytic commitment is wholly dependent on nitric oxide. • Autocrine IL-10 inhibits NO production, limiting macrophage glycolytic commitment. • Autocrine IL-10 is a rheostat for glycolytic commitment of macrophages.

Published

2016

25. Diversity and environmental adaptation of phagocytic cell metabolism

Author

Luke C, Davies, Christopher M, Rice, Daniel W, McVicar, and Jonathan M, Weiss

Subjects

Phagocytes, Neutrophils, Macrophages, oxidative phosphorylation, Reviews, Review, glycolysis, Adaptation, Physiological, niche diversity, Neoplasms, phagocyte metabolism, Animals, Humans, Metabolic Networks and Pathways

Abstract

Phagocytes are cells of the immune system that play important roles in phagocytosis, respiratory burst and degranulation—key components of innate immunity and response to infection. This diverse group of cells includes monocytes, macrophages, dendritic cells, neutrophils, eosinophils, and basophils—heterogeneous cell populations possessing cell and tissue‐specific functions of which cellular metabolism comprises a critical underpinning. Core functions of phagocytic cells are diverse and sensitive to alterations in environmental‐ and tissue‐specific nutrients and growth factors. As phagocytic cells adapt to these extracellular cues, cellular processes are altered and may contribute to pathogenesis. The considerable degree of functional heterogeneity among monocyte, neutrophil, and other phagocytic cell populations necessitates diverse metabolism. As we review our current understanding of metabolism in phagocytic cells, gaps are focused on to highlight the need for additional studies that hopefully enable improved cell‐based strategies for counteracting cancer and other diseases.

Published

2018

26. Itaconic acid mediates crosstalk between macrophage metabolism and peritoneal tumors

Author

Lisa A. Ridnour, Luke C. Davies, Jonathan M. Weiss, Daniel W. McVicar, Michelle K. Ozaki, Lilia Ileva, David A. Wink, Robert Y.S. Cheng, Christina M. Annunziata, and Megan Karwan

Subjects

0301 basic medicine, Carboxy-Lyases, Metabolite, Cell, Melanoma, Experimental, Oxidative phosphorylation, Mouse models, Monocytes, Oxidative Phosphorylation, 03 medical and health sciences, chemistry.chemical_compound, Mice, Downregulation and upregulation, Cell Line, Tumor, medicine, Animals, Humans, Glycolysis, Itaconic acid, RNA, Small Interfering, Hydro-Lyases, Peritoneal Neoplasms, Mice, Knockout, Ovarian Neoplasms, Catabolism, Fatty Acids, Proteins, Succinates, General Medicine, 3. Good health, Tumor Burden, Mice, Inbred C57BL, 030104 developmental biology, medicine.anatomical_structure, Metabolism, chemistry, Oncology, Tumor progression, Intermediary metabolism, Cancer research, Disease Progression, Macrophages, Peritoneal, Female, Reactive Oxygen Species, Research Article

Abstract

Control of cellular metabolism is critical for efficient cell function, although little is known about the interplay between cell subset–specific metabolites in situ, especially in the tumor setting. Here, we determined how a macrophage-specific (Mϕ-specific) metabolite, itaconic acid, can regulate tumor progression in the peritoneum. We show that peritoneal tumors (B16 melanoma or ID8 ovarian carcinoma) elicited a fatty acid oxidation–mediated increase in oxidative phosphorylation (OXPHOS) and glycolysis in peritoneal tissue–resident macrophages (pResMϕ). Unbiased metabolomics identified itaconic acid, the product of immune-responsive gene 1–mediated (Irg1-mediated) catabolism of mitochondrial cis-aconitate, among the most highly upregulated metabolites in pResMϕ of tumor-bearing mice. Administration of lentivirally encoded Irg1 shRNA significantly reduced peritoneal tumors. This resulted in reductions in OXPHOS and OXPHOS-driven production of ROS in pResMϕ and ROS-mediated MAPK activation in tumor cells. Our findings demonstrate that tumors profoundly alter pResMϕ metabolism, leading to the production of itaconic acid, which potentiates tumor growth. Monocytes isolated from ovarian carcinoma patients’ ascites fluid expressed significantly elevated levels of IRG1. Therefore, IRG1 in pResMϕ represents a potential therapeutic target for peritoneal tumors.

Published

2018

27. Tumour-elicited neutrophils engage mitochondrial metabolism to circumvent nutrient limitations and maintain immune suppression

Author

Jonathan M. Weiss, Scott K. Durum, Luke C. Davies, Jung-Min Lee, Tracey A. Rouault, Christopher M. Rice, Caroline Andrews, Daniel W. McVicar, Jeff J. Subleski, Christina M. Annunziata, Erika M. Palmieri, Marieli Gonzalez-Cotto, Nimit L. Patel, and Nunziata Maio

Subjects

0301 basic medicine, Neutrophils, Science, T cell, Lymphocyte, Immunoblotting, General Physics and Astronomy, Oxidative phosphorylation, medicine.disease_cause, General Biochemistry, Genetics and Molecular Biology, Article, Oxidative Phosphorylation, 03 medical and health sciences, Mice, 0302 clinical medicine, Immune system, Cell Line, Tumor, medicine, Animals, Glycolysis, lcsh:Science, Cells, Cultured, chemistry.chemical_classification, Mice, Knockout, Reactive oxygen species, Multidisciplinary, Microscopy, Confocal, General Chemistry, Metabolism, Flow Cytometry, Immunohistochemistry, Cell biology, Mitochondria, Oxidative Stress, 030104 developmental biology, medicine.anatomical_structure, chemistry, 030220 oncology & carcinogenesis, lcsh:Q, CRISPR-Cas Systems, Reactive Oxygen Species, Oxidation-Reduction, Oxidative stress, Signal Transduction

Abstract

Neutrophils are a vital component of immune protection, yet in cancer they may promote tumour progression, partly by generating reactive oxygen species (ROS) that disrupts lymphocyte functions. Metabolically, neutrophils are often discounted as purely glycolytic. Here we show that immature, c-Kit+ neutrophils subsets can engage in oxidative mitochondrial metabolism. With limited glucose supply, oxidative neutrophils use mitochondrial fatty acid oxidation to support NADPH oxidase-dependent ROS production. In 4T1 tumour-bearing mice, mitochondrial fitness is enhanced in splenic neutrophils and is driven by c-Kit signalling. Concordantly, tumour-elicited oxidative neutrophils are able to maintain ROS production and T cell suppression when glucose utilisation is restricted. Consistent with these findings, peripheral blood neutrophils from patients with cancer also display increased immaturity, mitochondrial content and oxidative phosphorylation. Together, our data suggest that the glucose-restricted tumour microenvironment induces metabolically adapted, oxidative neutrophils to maintain local immune suppression., Neutrophils normally fulfil their metabolic demands by glycolysis and have limited mitochondrial activity. Here the authors show that tumours promote neutrophils adapted to oxidative mitochondria metabolism that function in the glucose-restrained tumour microenvironment to promote tumour growth by maintaining local immune suppression.

Published

2017

28. Tissue-resident macrophages

Author

Judith E. Allen, Stephen J. Jenkins, Philip R. Taylor, and Luke C. Davies

Subjects

Inflammation, Wound Healing, Innate immune system, Macrophages, Immunology, Immunity, Macrophage Activation, Biology, Article, Haematopoiesis, Immune system, Organ Specificity, medicine, Animals, Humans, Immunology and Allergy, Macrophage, medicine.symptom, Wound healing, Immunologic Surveillance, Tissue homeostasis

Abstract

Tissue-resident macrophages are a heterogeneous population of immune cells that fulfill tissue-specific and niche-specific functions. These range from dedicated homeostatic functions, such as clearance of cellular debris and iron processing, to central roles in tissue immune-surveillance, response to infection and the resolution of inflammation. Recent studies highlight marked heterogeneity in the origins of tissue macrophages that arise from hematopoietic versus self-renewing embryo-derived populations. We discuss the tissue–niche-specific factors that dictate cell phenotype, the definition of which will allow novel strategies to promote the restoration of tissue homeostasis. Understanding the mechanisms that dictate tissue macrophage heterogeneity should explain why simplified paradigms of macrophage activation do not explain the extent of heterogeneity seen in vivo.

Published

2013

29. Macrophage heterogeneity and acute inflammation

Author

Philip R. Taylor, Marcela Rosas, Luke C. Davies, Simon Arnett Jones, and Kate Liddiard

Subjects

Adult, Inflammation, Macrophages, Immunology, Cell Differentiation, Macrophage Activation, Biology, Cell biology, Cellular heterogeneity, Acute Disease, medicine, Animals, Homeostasis, Humans, Regeneration, Immunology and Allergy, Macrophage, Effector functions, medicine.symptom, Function (biology)

Abstract

In this Viewpoint, we concentrate on the aspects of macrophage biology that we believe are fundamental for an appropriate contextual understanding of macrophage function during acute inflammation. These are the different origins of macrophage populations (and the implications of this for the renewal of these populations in the adult); and the impact of specific homeostatic or disease-associated microenvironments upon cellular heterogeneity, activation and effector functions.

Published

2011

30. Nitric oxide dictates the reprogramming of carbon flux during M1 macrophage polarization

Author

Erika M. Palmieri, Walter A. Baseler, Luke C. Davies, Marieli Gonzalez-Cotto, Bart Ghesquiere, Teresa W. M. Fan, Andrew N. Lane, David A. Wink, and Daniel W. McVicar

Subjects

Immunology, Immunology and Allergy

Abstract

Classical pro-inflammatory activation of macrophages is characterized by profound intracellular metabolic changes, with increased glycolytic usage of carbon, away from Oxidative Phosphorylation (OXPHOS). We previously demonstrated that Nitric Oxide (NO) levels induced in Bone Marrow Derived Macrophages (BMDMs) from Wild Type (WT) mice are necessary and sufficient for the repression of OXPHOS. Here we demonstrate that NO is also responsible for the “break” in the mitochondrial TCA cycle and citrate accumulation during LPS/IFNγ stimulation; macrophages that lack NO maintain indeed substantial levels of Oxygen Consumption Rates (OCR) and TCA cycle intermediates. Carbon tracing experiments in the presence of U13C-glucose show almost undetected labelled α-ketoglutarate from citrate in WT but a conserved pattern of heavy carbon fate in Nos2−/− macrophages. Moreover we found that mitochondrial respiration elicited through citrate was decreased in WT M1 macrophages, but isocitrate was a full substrate for complex I-dependent OCR suggesting suppression of metabolism at mitochondrial Aconitase (ACO2). Consistent with this data, we found ACO2 enzymatic activity blunted in WT vs Nos2−/−. In addition we observed that M1 macrophages reroute pyruvate away from Pyruvate Dehydrogenase (PDH) in an NO dependent manner since only WT show halted flux through PDH. Surprisingly, we demonstrate this mechanism to be independent on the activation of Hif1α and its suggested effect on limiting acetyl-coA for the TCA. With these data together we hypothesize that NO orchestrates macrophage metabolism during inflammation inhibiting OXPHOS by blocking Krebs Cycle, therefore depriving of substrates the mitochondrial electron transport chain.

Published

2018

31. Tissue‐resident macrophages: then and now

Author

Philip R. Taylor and Luke C. Davies

Subjects

Gata6, Immunology, Population, Inflammation, Review Article, Biology, Immune system, medicine, Animals, Homeostasis, Humans, Immunology and Allergy, Macrophage, education, Macrophage inflammatory protein, education.field_of_study, Innate immune system, Macrophages, Macrophage Activation, tissue-resident macrophages, Phenotype, Immunity, Innate, Haematopoiesis, Gene Expression Regulation, environmental programming, Inflammation Mediators, medicine.symptom, Signal Transduction, Transcription Factors

Abstract

Macrophages have been at the heart of immune research for over a century and are an integral component of innate immunity. Macrophages are often viewed as terminally differentiated monocytic phagocytes. They infiltrate tissues during inflammation, and form polarized populations that perform pro-inflammatory or anti-inflammatory functions. Tissue-resident macrophages were regarded as differentiated monocytes, which seed the tissues to perform immune sentinel and homeostatic functions. However, tissue-resident macrophages are not a homogeneous population, but are in fact a grouping of cells with similar functions and phenotypes. In the last decade, it has been revealed that many of these cells are not terminally differentiated and, in most cases, are not derived from haematopoiesis in the adult. Recent research has highlighted that tissue-resident macrophages cannot be grouped into simple polarized categories, especially in vivo, when they are exposed to complex signalling events. It has now been demonstrated that the tissue environment itself is a major controller of macrophage phenotype, and can influence the expression of many genes regardless of origin. This is consistent with the concept that cells within different tissues have diverse responses in inflammation. There is still a mountain to climb in the field, as it evolves to encompass not only tissue-resident macrophage diversity, but also categorization of specific tissue environments and the plasticity of macrophages themselves. This knowledge provides a new perspective on therapeutic strategies, as macrophage subsets can potentially be manipulated to control the inflammatory environment in a tissue-specific manner.

Published

2015

32. The transcription factor Gata6 links tissue macrophage phenotype and proliferative renewal§

Author

Bashar Kharfan, Valerie B. O'Donnell, Donald James Fraser, Chia-Te Liao, Luke C. Davies, Peter Giles, Simon Arnett Jones, Timothy Stone, Philip R. Taylor, and Marcela Rosas

Subjects

Population, Inflammation, Biology, Article, Transcriptome, Mice, GATA6 Transcription Factor, medicine, Transcriptional regulation, Macrophage, Animals, Myeloid Cells, education, Transcription factor, Cell Proliferation, Mice, Knockout, education.field_of_study, Multidisciplinary, GATA6, R1, Cell biology, medicine.anatomical_structure, Phenotype, Immunology, Macrophages, Peritoneal, Bone marrow, medicine.symptom

Abstract

Gata6 Controls Peritoneal Macs Macrophages seed tissues throughout the body and are shaped both phenotypically and functionally by the microenvironment they inhabit. Despite such heterogeneity, most tissue macrophages self-renew by local proliferation. How this is regulated, however, is unclear. Rosas et al. (p. 645 , published online 24 April) used gene expression analysis to show that the transcription factor Gata6 is specifically expressed in peritoneal macrophages. Gata6 was critical for maintaining the transcriptional signature of peritoneal macrophages and for their proliferative renewal during homeostasis and under inflammatory conditions.

Published

2014

33. miR-192 Induces G2/M Growth Arrest in Aristolochic Acid Nephropathy

Author

Hideo Akiyama, Donald James Fraser, Luke C. Davies, Cristina Beltrami, Aled O. Phillips, Bevan Cumbes, Timothy Bowen, Robert H. Jenkins, Christopher P. Carrington, and Philip R. Taylor

Subjects

Cell cycle checkpoint, DNA damage, Blotting, Western, Aristolochic acid, Fluorescent Antibody Technique, Pathology and Forensic Medicine, Kidney Tubules, Proximal, chemistry.chemical_compound, Fibrosis, microRNA, Gene expression, medicine, Humans, Immunoprecipitation, Cells, Cultured, Oligonucleotide Array Sequence Analysis, Cyclin-dependent kinase 1, biology, Reverse Transcriptase Polymerase Chain Reaction, Epithelial Cells, Flow Cytometry, medicine.disease, Ubiquitin ligase, G2 Phase Cell Cycle Checkpoints, MicroRNAs, chemistry, Biochemistry, biology.protein, Cancer research, Aristolochic Acids, M Phase Cell Cycle Checkpoints, Kidney Diseases, Signal Transduction

Abstract

Aristolochic acid nephropathy is characterized by rapidly progressive tubulointerstitial nephritis culminating in end-stage renal failure and urothelial malignancy. Profibrotic effects of aristolochic acid are linked to growth arrest of proximal tubular epithelial cells; however, the underlying mechanisms are largely undetermined. miRNAs are small, endogenous, post-transcriptional regulators of gene expression implicated in numerous physiological and pathological processes. In the present study, we characterized the mechanism of aristolochic acid-induced cell cycle arrest and its regulation by miRNAs. Incubation with aristolochic acid led to profound G2/M arrest in proximal tubular epithelial cells via p53-mediated inactivation of the maturation-promoting complex, CDK1/cyclin-B1. Analysis of miRNA expression identified up-regulation of miRNAs, including miR-192, miR-194, miR-450a, and miR-542-3p. The stable overexpression of miR-192 recapitulated G2/M arrest via repression of the E3 ubiquitin ligase, murine double-minute 2, a negative regulator of p53. p53-induced transcription of p21(cip1) and growth arrest and DNA damage 45 and resulted in the inactivation and dissociation of the maturation-promoting complex. These data demonstrate a core role for miR-192 in mediating proximal tubular epithelial cell G2/M arrest after toxic injury by aristolochic acid. Because numerous studies have linked such growth arrest to fibrosis after proximal tubular epithelial cell injury, this mechanism may have widespread relevance to recovery/nonrecovery after acute kidney injury.

Published

2014

34. Distinct bone marrow-derived and tissue-resident macrophage lineages proliferate at key stages during inflammation

Author

Chia-Te Liao, Judith E. Allen, Martin J. Scurr, Frank Brombacher, Stephen J. Jenkins, Marcela Rosas, Simon Arnett Jones, Luke C. Davies, Philip R. Taylor, and Donald James Fraser

Subjects

Lineage (genetic), General Physics and Astronomy, Bone Marrow Cells, Inflammation, Peritonitis, Biology, Article, General Biochemistry, Genetics and Molecular Biology, Mice, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, medicine, Animals, Antigens, Ly, Macrophage, Cell Lineage, Receptor, Macrophage inflammatory protein, Cell Proliferation, 030304 developmental biology, 0303 health sciences, Multidisciplinary, Cell growth, Macrophage Colony-Stimulating Factor, Macrophages, Zymosan, General Chemistry, Receptors, Interleukin-4, Mice, Inbred C57BL, Kinetics, medicine.anatomical_structure, chemistry, Immunology, Female, Interleukin-4, Bone marrow, medicine.symptom, 030215 immunology

Abstract

The general paradigm is that monocytes are recruited to sites of inflammation and terminally-differentiate into macrophages. There has been no demonstration of proliferation of peripherally-derived inflammatory macrophages under physiological conditions. Here we show that proliferation of both bone marrow-derived inflammatory and tissue resident macrophage lineage branches is a key feature of the inflammatory process with major implications for the mechanisms underlying recovery from inflammation. Both macrophage lineage branches are dependent on M-CSF during inflammation, and thus the potential for therapeutic interventions is marked. Furthermore, these observations are independent of Th2 immunity. These studies indicate that the proliferation of distinct macrophage populations provides a general mechanism for macrophage expansion at key stages during inflammation, and separate control mechanisms are implicated.

Published

2013

35. A quantifiable proliferative burst of tissue macrophages restores homeostatic macrophage populations after acute inflammation

Author

Luke C. Davies, Marcela Rosas, Philip R. Taylor, Donald James Fraser, Simon Arnett Jones, and Paul J. Smith

Subjects

Male, Mice, 129 Strain, Time Factors, Cell Survival, Immunology, Cell, Inflammation, Peritonitis, Biology, Flow cytometry, Mice, Peritoneal cavity, medicine, Animals, Homeostasis, Immunology and Allergy, Macrophage, Peritoneal Cavity, Cells, Cultured, Vascular tissue, Cell Proliferation, medicine.diagnostic_test, Cell growth, Macrophages, Monocyte, Cell Cycle, DNA, Flow Cytometry, Mice, Inbred C57BL, medicine.anatomical_structure, Acute Disease, Female, medicine.symptom

Abstract

Macrophage (MØ) biology is routinely modelled in the peritoneal cavity, a vascular tissue readily infiltrated by leukocytes during inflammation. After several decades of study, no consensus has emerged regarding the importance of in situ proliferation versus peripheral monocyte recruitment for the maintenance of tissue resident MØs. By applying specific measures of mitosis, we have monitored tissue MØ proliferation during newborn development, adulthood and acute resolving inflammation in young adult mice. Despite the vascular nature of the tissue and ease of peripheral leukocyte entry, tissue MØs in the newborn increase in number by local proliferation. On the contrary, in the adult, tissue MØ proliferation is considerably reduced and most likely provides homeostatic control of cell numbers. Importantly, during an acute inflammatory response, when substantial numbers of inflammatory MØs are recruited from the circulation, tissue-resident MØs survive and then undergo a transient and intense proliferative burst in situ to repopulate the tissue. Our data indicate that local proliferation is a general mechanism for the self-sufficient renewal of tissue MØs during development and acute inflammation and not one restricted to non-vascular tissues, which has implications for the therapeutic modulation of MØ activity during the resolution of inflammation.

Published

2011

36. Hoxb8 conditionally immortalised macrophage lines model inflammatory monocytic cells with important similarity to dendritic cells

Author

Caetano Reis e Sousa, Simon Arnett Jones, Fabiola Osorio, Marcela Rosas, Matthew J. Robinson, Luke C. Davies, Philip R. Taylor, and Nicola Dierkes

Subjects

CD4-Positive T-Lymphocytes, Lipopolysaccharides, Cell type, Mice, 129 Strain, beta-Glucans, Ovalbumin, Transgene, Immunology, Priming (immunology), Nerve Tissue Proteins, Biology, Monocyte-Macrophage Precursor Cells, Nitric Oxide, Interferon-gamma, Lipopeptides, Mice, Antigen, Transduction, Genetic, Precursor cell, medicine, Immunology and Allergy, Animals, Lectins, C-Type, Cell Line, Transformed, Homeodomain Proteins, Mice, Knockout, Antigen Presentation, Monocyte, Macrophage Colony-Stimulating Factor, Macrophages, Zymosan, Granulocyte-Macrophage Colony-Stimulating Factor, Membrane Proteins, Cell Differentiation, Dendritic Cells, Cell biology, Mice, Inbred C57BL, medicine.anatomical_structure, Cell culture, Antigens, Surface, Mice, Inbred CBA, Cytokines, Interleukin-2, Bone marrow

Abstract

We have examined the potential to generate bona fide macrophages (MØ) from conditionally immortalised murine bone marrow precursors. MØ can be derived from Hoxb8 conditionally immortalised macrophage precursor cell lines (MØP) using either M-CSF or GM-CSF. When differentiated in GM-CSF (GM-MØP) the resultant cells resemble GM-CSF bone marrow-derived dendritic cells (BMDC) in morphological phenotype, antigen phenotype and functional responses to microbial stimuli. In spite of this high similarity between the two cell types and the ability of GM-MØP to effectively present antigen to a T-cell hybridoma, these cells are comparatively poor at priming the expansion of IFN-γ responses from naïve CD4(+) T cells. The generation of MØP from transgenic or genetically aberrant mice provides an excellent opportunity to study the inflammatory role of GM-MØP, and reduces the need for mouse colonies in many studies. Hence differentiation of conditionally immortalised MØPs in GM-CSF represents a unique in vitro model of inflammatory monocyte-like cells, with important differences from bone marrow-derived dendritic cells, which will facilitate functional studies relating to the many 'sub-phenotypes' of inflammatory monocytes.

Published

2010

37. Factors influencing the career aspirations and preferred modes of working in recent dental graduates in Wales

Author

D. R. Thomas, S. J. Sandham, Luke C. Davies, Ivor Gordon Chestnutt, and Elizabeth Treasure

Subjects

Service (business), State Dentistry, Adult, Male, Specialties, Dental, Wales, Career Choice, National Health Programs, business.industry, Project commissioning, Dentists, General Medicine, Contract Services, Private sector, Preference, Work (electrical), Nursing, Vocational education, Workforce, Medicine, Humans, Female, business, Practice Patterns, Dentists'

Abstract

Introduction In England and Wales, National Health Service (NHS) primary dental care services are now commissioned on a local basis. In planning for the future, it is important that commissioning authorities have a clear understanding of the perspectives of recent dental graduates: vocational dental practitioners (VDPs). Objectives This study investigated the career aspirations and preferred modes of working of VDPs in Wales. Methodology Data were collected via a postal questionnaire, comprising 37 closed and open questions, mailed to all 59 VDPs in Wales. Results A total of 53 (90%) VDPs participated, of whom 47 saw their future in general dental practice: 5, 35, and 7 indicating a preference to work in the NHS, mixed (NHS and private), and private sector, respectively. None selected the Community Dental Service as their preferred vocation. More than half of all respondents intended to undertake a postgraduate qualification within the next five years and 22 wished to specialise. Of the 53 VDPs, 44 were concerned that lack of NHS contracts would limit where they could practise, and agreed that family and other social commitments were a significant influence on choice of practice location. Access to high-quality premises and continuing professional development were agreed as important by 41 VDPs. A majority (37) agreed that private dentistry was an attractive alternative to NHS dentistry. Of the respondents, 38 (22 females, 16 males) expected to work part-time at some point in the future and 14 said they would consider a career outside dentistry. Only nine VDPs agreed that they would be happy working in a single-handed practice and even fewer (six) indicated they would be happy working for a corporate body. Conclusions Numerous factors impact on the career aspirations of VDPs. These factors have been quantified in this study, and healthcare-commissioning bodies need to be aware of them when planning future dental care provision in Wales.

Published

2008

38. Summary of: Practitioners' perspectives and experiences of the new National Health Service dental contract

Author

Luke C. Davies, D. R. Thomas, and Ivor Gordon Chestnutt

Subjects

medicine.medical_specialty, Government, business.industry, Project commissioning, National health service, Dental care, Postal questionnaire, Nursing, Family medicine, Cohort, medicine, Remuneration, business, General Dentistry

Abstract

Background In April 2006, fundamental changes were made to the arrangements for commissioning state funded (National Health Service, NHS) dental care in England and Wales. These involved the dissolution of a universal national contract and the introduction of locally commissioned primary dental care services. Suggested advantages included the elimination of a fee-for-item 'treadmill', an increased emphasis on prevention and improved patient access. This change came at a time when many practitioners were opting to provide care outside the NHS. Objectives This study investigated dentists' experience of the new contract and compared this with attitudes determined in a previous survey of the same cohort of dentists conducted immediately before the changed commissioning arrangements. Methods Data were collected via a postal questionnaire, comprising a combination of 60 open and closed questions, mailed to 608 general dental practitioners in Wales. Results Four hundred and ninety-six (77%) questionnaires were returned. Four hundred and seventeen practitioners continued to provide NHS dental care. Only 46 (11%) of the 417 practitioners agreed that they liked the new method of remuneration and the majority (362 [86.8%]) perceived that they still delivered state-funded care in a 'treadmill' environment. This compares with 34.9% of dentists who perceived the new system as a 'treadmill' immediately before its implementation. Three hundred and forty-eight (83.4%) disagreed that they were able to spend more time on prevention and 356 (85.3%) did not feel they had more time to spend with patients – key objectives of the reforms. Two hundred and seventy-five (65.9%) respondents agreed that local NHS commissioners were controlling their business. Conclusion This survey, conducted 18 months after the implementation of the new commissioning arrangements, suggests that practitioners are deeply unhappy with local commissioning. It raises questions as to whether the changes have achieved the Government's stated objectives in reforming state-funded primary dental care.

Published

2009

39. Practitioners' perspectives and experiences of the new National Health Service dental contract

Author

Ivor Gordon Chestnutt, D. R. Thomas, and Luke C. Davies

Subjects

Male, medicine.medical_specialty, Time Factors, Attitude of Health Personnel, Project commissioning, Dentists, Contracts, Health Services Accessibility, Job Satisfaction, Cohort Studies, Reimbursement Mechanisms, Postal questionnaire, Sex Factors, Nursing, Remuneration, medicine, Humans, Dental Care, Workplace, General Dentistry, Health Services Needs and Demand, Government, Wales, Primary Health Care, business.industry, Administrative Personnel, Dental Prophylaxis, National health service, Dental care, England, State Dentistry, Health Care Reform, Family medicine, Cohort, Female, business, Delivery of Health Care

Abstract

Background In April 2006, fundamental changes were made to the arrangements for commissioning state funded (National Health Service, NHS) dental care in England and Wales. These involved the dissolution of a universal national contract and the introduction of locally commissioned primary dental care services. Suggested advantages included the elimination of a fee-for-item 'treadmill', an increased emphasis on prevention and improved patient access. This change came at a time when many practitioners were opting to provide care outside the NHS. Objectives This study investigated dentists' experience of the new contract and compared this with attitudes determined in a previous survey of the same cohort of dentists conducted immediately before the changed commissioning arrangements. Methods Data were collected via a postal questionnaire, comprising a combination of 60 open and closed questions, mailed to 608 general dental practitioners in Wales. Results Four hundred and ninety-six (77%) questionnaires were returned. Four hundred and seventeen practitioners continued to provide NHS dental care. Only 46 (11%) of the 417 practitioners agreed that they liked the new method of remuneration and the majority (362[86.8%]) perceived that they still delivered state-funded care in a 'treadmill' environment. This compares with 34.9% of dentists who perceived the new system as a 'treadmill' immediately before its implementation. Three hundred and forty-eight (83.4%) disagreed that they were able to spend more time on prevention and 356 (85.3%) did not feel they had more time to spend with patients-key objectives of the reforms. Two hundred and seventy-five (65.9%) respondents agreed that local NHS commissioners were controlling their business. Conclusion This survey, conducted 18 months after the implementation of the new commissioning arrangements, suggests that practitioners are deeply unhappy with local commissioning. It raises questions as to whether the changes have achieved the Government's stated objectives in reforming state-funded primary dental care.

Published

2009

40. The protective effect of inflammatory monocytes during systemic C. albicans infection is dependent on collaboration between C-type lectin-like receptors.

Author

Aiysha Thompson, Luke C Davies, Chia-Te Liao, Diogo M da Fonseca, James S Griffiths, Robert Andrews, Adam V Jones, Mathew Clement, Gordon D Brown, Ian R Humphreys, Philip R Taylor, and Selinda J Orr

Subjects

Immunologic diseases. Allergy, RC581-607, Biology (General), QH301-705.5

Abstract

Invasive candidiasis, mainly caused by Candida albicans, is a serious healthcare problem with high mortality rates, particularly in immunocompromised patients. Innate immune cells express pathogen recognition receptors (PRRs) including C-type lectin-like receptors (CLRs) that bind C. albicans to initiate an immune response. Multiple CLRs including Dectin-1, Dectin-2 and Mincle have been proposed individually to contribute to the immune response to C. albicans. However how these receptors collaborate to clear a fungal infection is unknown. Herein, we used novel multi-CLR knockout (KO) mice to decipher the individual, collaborative and collective roles of Dectin-1, Dectin-2 and Mincle during systemic C. albicans infection. These studies revealed an unappreciated and profound role for CLR co-operation in anti-fungal immunity. The protective effect of multiple CLRs was markedly greater than any single receptor, and was mediated through inflammatory monocytes via recognition and phagocytosis of C. albicans, and production of C. albicans-induced cytokines and chemokines. These CLRs were dispensable for mediating similar responses from neutrophils, likely due to lower expression of these CLRs on neutrophils compared to inflammatory monocytes. Concurrent deletion of Dectin-1 and Dectin-2, or all three CLRs, resulted in dramatically increased susceptibility to systemic C. albicans infection compared to mice lacking a single CLR. Multi-CLR KO mice were unable to control fungal growth due to an inadequate early inflammatory monocyte-mediated response. In response to excessive fungal growth, the multi-CLR KO mice mounted a hyper-inflammatory response, likely leading to multiple organ failure. Thus, these data reveal a critical role for CLR co-operation in the effective control of C. albicans and maintenance of organ function during infection.

Published

2019