Your search keyword '"Jahnsen, Frode L."' showing total 13 results

1. CD1c-Expression by Monocytes - Implications for the Use of Commercial CD1c+ Dendritic Cell Isolation Kits.

Author

Schrøder M, Melum GR, Landsverk OJ, Bujko A, Yaqub S, Gran E, Aamodt H, Bækkevold ES, Jahnsen FL, and Richter L

Subjects

Antigens, CD1 genetics, CD4-Positive T-Lymphocytes cytology, Cell Communication, Coculture Techniques, Dendritic Cells cytology, Gene Expression, Glycoproteins genetics, Humans, Lymphocyte Activation, Monocytes cytology, Primary Cell Culture, Reagent Kits, Diagnostic, Antigens, CD1 immunology, CD4-Positive T-Lymphocytes immunology, Cell Separation methods, Dendritic Cells immunology, Flow Cytometry standards, Glycoproteins immunology, Monocytes immunology

Abstract

Conventional dendritic cells (cDCs) comprise a heterogeneous population of cells that are important regulators of immunity and homeostasis. CD1c+ cDCs are present in human blood and tissues, and found to efficiently activate naïve CD4+ T cells. While CD1c is thought to specifically identify this subset of human cDCs, we show here that also classical and intermediate monocytes express CD1c. Accordingly, the commercial CD1c (BDCA-1)+ Dendritic Cell Isolation Kit isolates two distinct cell populations from blood: CD1c+CD14- cDCs and CD1c+CD14+ monocytes. CD1c+ cDCs and CD1c+ monocytes exhibited strikingly different properties, including their differential regulation of surface marker expression, their levels of cytokine production, and their ability to stimulate naïve CD4+ T cells. These results demonstrate that a commercial CD1c (BDCA-1)+ Dendritic Cell Isolation Kit isolates two functionally different cell populations, which has important implications for the interpretation of previously generated data using this kit to characterize CD1c+ cDCs.

Published

2016

2. A thymic stromal lymphopoietin-responsive dendritic cell subset mediates allergic responses in the upper airway mucosa.

Author

Melum GR, Farkas L, Scheel C, Van Dieren B, Gran E, Liu YJ, Johansen FE, Jahnsen FL, and Baekkevold ES

Subjects

Adolescent, Adult, Aged, Allergens immunology, Antigens, CD1 metabolism, Cell Differentiation immunology, Cell Movement, Cells, Cultured, Cytokines metabolism, Female, Glycoproteins metabolism, Humans, Immunologic Memory, Lymphocyte Activation, Male, Middle Aged, Receptors, CCR7 genetics, Receptors, CCR7 metabolism, Receptors, Cytokine metabolism, Up-Regulation, Young Adult, Thymic Stromal Lymphopoietin, Cytokines immunology, Dendritic Cells immunology, Myeloid Cells immunology, Respiratory Mucosa immunology, Rhinitis, Allergic immunology, Th2 Cells immunology

Abstract

Background: Thymic stromal lymphopoietin (TSLP) controls allergic TH2 inflammatory responses through induction of distinct activation programs in dendritic cells (DCs). However, knowledge about TSLP receptor expression and functional consequences of receptor activation by DCs residing in the human respiratory tract is limited., Objective: We wanted to identify TSLP-responding DC populations in the human upper airway mucosa and assess the TSLP-mediated effects on such DCs in allergic airway responses., Results: We found that the TSLP receptor was constitutively and preferentially expressed by myeloid CD1c(+) DCs in the human airway mucosa and that the density of this DC subset in nasal mucosa increased significantly after in vivo allergen challenge of patients with allergic rhinitis. In vitro, TSLP strongly enhanced the capacity of CD1c(+) DCs to activate allergen-specific memory CD4(+) T cells. Moreover, TSLP rapidly induced CCR7 expression on CD1c(+) DCs. However, TH2 cytokines attenuated TSLP-mediated CCR7 induction, thus inhibiting the TSLP-induced DC migration potential to the draining lymph nodes., Conclusion: Our results suggest that TSLP-mediated activation of human nasal mucosal CD1c(+) DCs triggers CCR7-dependent migration to the draining lymph nodes and enhances their capacity to initiate TH2 responses. However, the observation that TH2 cytokines abrogate the induction of CCR7 implies that during a TH2-mediated inflammatory reaction, TLSP-activated CD1c(+) DCs are retained in the inflamed tissue to further exacerbate local inflammation by activating local antigen-specific memory TH2 cells., (Copyright © 2014 American Academy of Allergy, Asthma & Immunology. All rights reserved.)

Published

2014

3. Plasmacytoid DCs regulate recall responses by rapid induction of IL-10 in memory T cells.

Author

Kvale EO, Fløisand Y, Lund-Johansen F, Rollag H, Farkas L, Ghanekar S, Brandtzaeg P, Jahnsen FL, and Olweus J

Subjects

Antigens, Viral immunology, Antigens, Viral pharmacology, Bystander Effect drug effects, Bystander Effect immunology, CD11c Antigen immunology, Cells, Cultured, Coculture Techniques, Dendritic Cells cytology, Enterotoxins immunology, Enterotoxins pharmacology, Humans, Interferon Type I immunology, Interferon Type I metabolism, Interferon-gamma immunology, Interleukin-10 metabolism, Plasma Cells cytology, T-Lymphocytes, Regulatory metabolism, Dendritic Cells immunology, Immunologic Memory drug effects, Interleukin-10 immunology, Plasma Cells immunology, T-Lymphocytes, Regulatory immunology

Abstract

Dendritic cells (DCs) are believed to regulate T cell-mediated immunity primarily by directing differentiation of naive T cells. Here, we show that a large fraction of CD4(+) memory cells produce IL-10 within the first hours after interaction with plasmacytoid DCs (PDCs). In contrast, CD11c(+) DCs induce IFN-gamma and little IL-10. IL-10-secreting T cells isolated after 36 hours of culture with PDCs suppressed antigen-induced T-cell proliferation by an IL-10-dependent mechanism, but were distinct from natural and type 1 regulatory T cells. They proliferated strongly and continued to secrete IL-10 during expansion with PDCs, and after restimulation with immature monocyte-derived DCs or CD11c(+) DCs. The IL-10-producing T cells acquired the ability to secrete high levels of IFN-gamma after isolation and subsequent coculture with PDCs or CD11c(+) DCs. Compared to CD11c(+) DCs, PDCs were superior in their ability to selectively expand T cells that produced cytokines on repeated antigenic challenge. The DC-dependent differences in cytokine profiles were observed with viral recall antigen or staphylococcal enterotoxin B and were independent of extracellular type I interferon or IL-10. Our results show that DCs can regulate memory responses and that PDCs rapidly induce regulatory cytokines in effector T cells that can suppress bystander activity.

Published

2007

4. Accelerated antigen sampling and transport by airway mucosal dendritic cells following inhalation of a bacterial stimulus.

Author

Jahnsen FL, Strickland DH, Thomas JA, Tobagus IT, Napoli S, Zosky GR, Turner DJ, Sly PD, Stumbles PA, and Holt PG

Subjects

Administration, Inhalation, Aerosols, Animals, Antigen-Presenting Cells immunology, Antigens, Bacterial metabolism, Cell Movement, Coculture Techniques, Lymph Nodes immunology, Protein Transport, Rats, Rats, Inbred Strains, Antigen Presentation immunology, Dendritic Cells immunology, Immunologic Surveillance, Moraxella catarrhalis immunology, Respiratory Mucosa immunology, Respiratory Mucosa microbiology

Abstract

An increase in the tempo of local dendritic cell (DC)-mediated immune surveillance is a recognized feature of the response to acute inflammation at airway mucosal surfaces, and transient up-regulation of the APC functions of these DC preceding their emigration to regional lymph nodes has recently been identified as an important trigger for T cell-mediated airway tissue damage in diseases such as asthma. In this study, using a rat model, we demonstrate that the kinetics of the airway mucosal DC (AMDC) response to challenge with heat-killed bacteria is considerably more rapid and as a consequence more effectively compartmentalized than that in recall responses to soluble Ag. Notably, Ag-bearing AMDC expressing full APC activity reach regional lymph nodes within 30 min of cessation of microbial exposure, and in contrast to recall responses to nonpathogenic Ags, there is no evidence of local expression of APC activity within the airway mucosa preceding DC emigration. We additionally demonstrate that, analogous to that reported in the gut, a subset of airway intraepithelial DC extend their processes into the airway lumen. This function is constitutively expressed within the AMDC population, providing a mechanism for continuous immune surveillance of the airway luminal surface in the absence of "danger" signals.

Published

2006

5. A unique dendritic cell subset accumulates in the celiac lesion and efficiently activates gluten-reactive T cells.

Author

Ráki M, Tollefsen S, Molberg Ø, Lundin KE, Sollid LM, and Jahnsen FL

Subjects

Adolescent, Adult, Aged, Aged, 80 and over, Antigens, CD immunology, Antigens, Differentiation, Myelomonocytic immunology, Biopsy, CD11 Antigens immunology, Celiac Disease immunology, Celiac Disease pathology, Dendritic Cells pathology, Humans, In Vitro Techniques, Intestinal Mucosa immunology, Middle Aged, Dendritic Cells immunology, Duodenum pathology, Glutens pharmacology, HLA-DQ Antigens immunology, Intestinal Mucosa pathology, Lymphocyte Activation immunology, T-Lymphocytes immunology

Abstract

Background & Aims: Celiac disease is a chronic inflammation of the duodenal mucosa driven by gluten-reactive T cells restricted by the disease-associated HLA-DQ2 molecule. The mechanisms that regulate the activation of mucosal T cells are, however, understood poorly. The aim of this study was to identify the antigen-presenting cells that are responsible for the activation of gluten-reactive T cells in the celiac lesion., Methods: Intestinal biopsy specimens obtained from untreated and treated celiac patients and normal controls were either snap-frozen directly or incubated for 24 hours with or without gluten peptides. Cryosections were subjected to multicolor immunofluorescence applying monoclonal antibodies to a range of antigen-presenting cell markers. Macrophages and dendritic cells were isolated from enzymatically digested small intestinal biopsies of untreated patients and incubated with gluten-reactive T-cell clones to measure their antigen-presenting capacity., Results: HLA-DQ2+ cells in the normal duodenal mucosa consisted of 2 distinct cell populations: about 80% were CD68+ DC-lysosome intercellular adhesion molecule-3-grabbing nonintegrin+ macrophages and 20% were CD11c+ dendritic cells. Importantly, the CD11c+ dendritic cells accumulated in the celiac lesion and revealed an activated phenotype expressing CD86 and DC-specific-associated membrane protein. Moreover, when isolated from challenged biopsy specimens, the CD11c+ dendritic cells efficiently activated gluten-reactive T cells., Conclusions: Our results suggest that a unique subset of dendritic cells are responsible for local activation of gluten-reactive T cells in the celiac lesion.

Published

2006

6. Human dendritic cell expression of HLA-DO is subset specific and regulated by maturation.

Author

Hornell TM, Burster T, Jahnsen FL, Pashine A, Ochoa MT, Harding JJ, Macaubas C, Lee AW, Modlin RL, and Mellins ED

Subjects

Cells, Cultured, Gene Expression Regulation, HLA-D Antigens genetics, Humans, Myeloid Cells metabolism, Skin metabolism, Cell Differentiation, Dendritic Cells cytology, Dendritic Cells metabolism, HLA-D Antigens metabolism

Abstract

Expression of HLA-DO (DO) in cells that express HLA-DM (DM) results in an altered repertoire of MHC class II/peptide complexes, indicating that DO modulates DM function. Human and murine B cells and thymic epithelial cells express DO, while monocytes/macrophages do not. Monocyte-derived dendritic cells (DC) also have been found to be DO-negative, leading to the assumption that DC do not express DO. In this study, we report that, in fact, certain types of human primary DC express DO. These include Langerhans cells (LC) and some subtypes of circulating blood DC. Specifically, the majority of BDCA-3(+) DC, a small subset of uncertain function, are DO(+), while smaller proportions of CD11c(+), BDCA-1(+) (myeloid) DC, at most a minority of CD123(+)/BDCA-2(+) (plasmacytoid) DC, and no detectable CD16(+) (myeloid) DC, express DO. Immunohistochemistry of human tonsil sections demonstrates that tonsillar interdigitating DC are also DO(+). In a subset of immature LC with higher DO expression, an increased fraction of surface DR molecules carry CLIP peptides, indicating that DO functions as a DM inhibitor in these cells. LC expression of DO is down-regulated by maturation stimuli. DM levels also decrease under these conditions, but the DM:DO ratio generally increases. In the myeloid cell types tested, DO expression correlates with levels of DObeta, but not DOalpha, implying that modulation of DObeta regulates DO dimer abundance in these cells. The range of APC types shown to express DO suggests a broader role for DO in immune function than previously appreciated.

Published

2006

7. CD11c+ dendritic cells and plasmacytoid DCs are activated by human cytomegalovirus and retain efficient T cell-stimulatory capability upon infection.

Author

Kvale EØ, Dalgaard J, Lund-Johansen F, Rollag H, Farkas L, Midtvedt K, Jahnsen FL, Brinchmann JE, and Olweus J

Subjects

Autocrine Communication immunology, Cells, Cultured, Dendritic Cells virology, Humans, Interferon Type I immunology, Kidney Transplantation, Lymphocyte Activation immunology, Plasma Cells virology, Antigen Presentation immunology, CD11c Antigen immunology, Cytomegalovirus immunology, Cytomegalovirus Infections immunology, Dendritic Cells immunology, Plasma Cells immunology, T-Lymphocytes immunology

Abstract

It has been suggested that human cytomegalovirus (HCMV) evades the immune system by infecting and paralyzing antigen-presenting cells. This view is based mainly on studies of dendritic cells (DCs) obtained after culture of monocytes (moDCs). It is contradicted by the asymptomatic course of HCMV infection in healthy persons, indicating that other key antigen-presenting cells induce an efficient immune response. Here we show that HCMV activates CD11c+ DCs and plasmacytoid DCs (PDCs). In contrast to moDCs, CD11c+ DCs and PDCs produced interferon (IFN) type 1 when exposed to HCMV. Autocrine IFN type 1 partially protected CD11c+ DCs against infection, whereas PDCs were resistant to HCMV even when IFN type 1 activity was inhibited. HCMV exposure induced the maturation of CD11c+ DCs by IFN type 1-dependent and -independent mechanisms. Importantly, CD11c+ DCs infected by inhibiting IFN type 1 activity retained full capacity to stimulate T cells. Renal transplant recipients receiving immunosuppressive treatment had lower frequencies of CD11c+ DCs and PDCs in blood than did healthy controls. The results show that HCMV activates the immune system by interacting with CD11c+ DCs and PDCs and that recipients of renal transplants have low frequencies of these cell types in blood.

Published

2006

8. Differential capability for phagocytosis of apoptotic and necrotic leukemia cells by human peripheral blood dendritic cell subsets.

Author

Dalgaard J, Beckstrøm KJ, Jahnsen FL, and Brinchmann JE

Subjects

Cell Differentiation drug effects, Cell Differentiation immunology, Culture Media, Serum-Free, Dendritic Cells cytology, Dendritic Cells drug effects, Granulocyte-Macrophage Colony-Stimulating Factor pharmacology, Humans, Integrin beta Chains immunology, Interleukin-4 pharmacology, K562 Cells, Leukemia, Erythroblastic, Acute pathology, Monocytes cytology, Monocytes drug effects, Monocytes immunology, Necrosis immunology, Phagocytosis drug effects, Plasma Cells cytology, Plasma Cells drug effects, Transforming Growth Factor beta pharmacology, Transforming Growth Factor beta1, Apoptosis immunology, CD11c Antigen immunology, Dendritic Cells immunology, Phagocytosis immunology, Plasma Cells immunology

Abstract

CD11c+ dendritic cells (DC) and plasmacytoid DC (PDC) are the two major DC subsets in human peripheral blood. For the purpose of immunotherapy with DC, it is important to investigate the phagocytosis of killed tumor cells by different DC subsets. Using immature monocyte-derived DC (iMoDC) as reference, we have compared the ability of CD11c+ DC and PDC to phagocytose apoptotic and necrotic K562 leukemia cells. Freshly isolated CD11c+ DC phagocytosed apoptotic and necrotic K562 cells, whereas PDC did not show any evidence of uptake of dead cells. Blocking studies showed that CD36 is importantly involved in uptake of apoptotic and necrotic material. CD91 and CD11c were also involved. In addition, we found that beta5 integrin was expressed on CD11c+ DC but not in its classical association with alphaV. Uptake of apoptotic K562 cells by CD11c+ DC was increased following incubation with granulocyte macrophage-colony stimulating factor (GM-CSF) and interleukin (IL)-4, alone or in combination with transforming growth factor-beta1, to levels comparable with those observed for iMoDC. Phagocytosis of dead cellular material by the GM-CSF/IL-4-treated CD11c+ DC was largely restricted to a subset expressing low levels of human leukocyte antigen-DR and CD83. Thus, the relationship between phagocytosis of antigenic material and expression of maturation-related cell-surface molecules is similar for CD11c+ DC and MoDC. We conclude that CD11c+ DC in peripheral blood are precursor cells, which under the influence of cytokines, differentiate to cells with DC phenotype and function.

Published

2005

9. Plasmacytoid dendritic cells activate allergen-specific TH2 memory cells: modulation by CpG oligodeoxynucleotides.

Author

Farkas L, Kvale EO, Johansen FE, Jahnsen FL, and Lund-Johansen F

Subjects

Adult, Cytokines biosynthesis, Dendritic Cells physiology, Female, Humans, Interferon-alpha physiology, Interferon-beta physiology, Interferon-gamma biosynthesis, Male, Middle Aged, Poaceae immunology, Rhinitis, Allergic, Perennial immunology, Adjuvants, Immunologic pharmacology, Allergens immunology, Dendritic Cells drug effects, Immunologic Memory, Lymphocyte Activation, Oligodeoxyribonucleotides pharmacology, Th2 Cells immunology

Abstract

Background: Plasmacytoid dendritic cells (PDCs) accumulate in the nasal mucosa of allergic rhinitis patients, but their function in upper airway allergy has not been determined. CpG oligodeoxynucleotides, potent adjuvants in immunotherapeutic strategies in animal models, are especially effective at activating PDCs. These cells are therefore potential targets for immunomodulation in humans., Objective: In this study, PDCs were compared with CD11c+ dendritic cells (DCs), a very potent antigen-presenting cell type, for their capacity to induce allergen-dependent activation of TH2 memory cells. Then, we investigated whether CpG-activated PDCs were able to modulate the allergen-specific TH2 memory response., Methods: DCs were isolated from patients with upper airway allergy and cocultured with autologous CD4+ T cells with or without grass pollen extract and CpG. In some experiments cells were restimulated with allergen-pulsed monocyte-derived DCs. T-cell activation was measured by their proliferative response and cytokine production., Results: PDCs stimulated allergen-dependent T-cell proliferation and TH2 cytokine production as efficiently as CD11c+ DCs. CpG-activated PDCs inhibited allergen-dependent proliferation of TH2 memory cells and markedly increased IFN-gamma production in PDC/T-cell cocultures; the former effect depended on the CpG-induced IFN-alpha/beta production by the PDCs., Conclusion: Our results demonstrated that PDCs efficiently drive allergen-dependent TH2 memory responses, suggesting that they play an active role in the allergic reaction. However, in the presence of CpG, PDCs were responsible for increased production of the TH1-related cytokines IFN-alpha and IFN-gamma, indicating that mucosal PDCs may be targets for CpG-based immunotherapeutic strategies against airway allergy.

Published

2004

10. Bidirectional interactions between antigen-bearing respiratory tract dendritic cells (DCs) and T cells precede the late phase reaction in experimental asthma: DC activation occurs in the airway mucosa but not in the lung parenchyma.

Author

Huh JC, Strickland DH, Jahnsen FL, Turner DJ, Thomas JA, Napoli S, Tobagus I, Stumbles PA, Sly PD, and Holt PG

Subjects

Animals, Antigens, CD analysis, B7-2 Antigen, Histocompatibility Antigens Class II analysis, Immunologic Memory, Lymphocyte Activation, Membrane Glycoproteins analysis, Mucous Membrane immunology, Ovalbumin immunology, Rats, T-Lymphocytes immunology, Asthma immunology, Cell Communication, Dendritic Cells physiology, Lung immunology, Respiratory System immunology, T-Lymphocytes physiology

Abstract

The airway mucosal response to allergen in asthma involves influx of activated T helper type 2 cells and eosinophils, transient airflow obstruction, and airways hyperresponsiveness (AHR). The mechanism(s) underlying transient T cell activation during this inflammatory response is unclear. We present evidence that this response is regulated via bidirectional interactions between airway mucosal dendritic cells (AMDC) and T memory cells. After aerosol challenge, resident AMDC acquire antigen and rapidly mature into potent antigen-presenting cells (APCs) after cognate interactions with T memory cells. This process is restricted to dendritic cells (DCs) in the mucosae of the conducting airways, and is not seen in peripheral lung. Within 24 h, antigen-bearing mature DCs disappear from the airway wall, leaving in their wake activated interleukin 2R+ T cells and AHR. Antigen-bearing activated DCs appear in regional lymph nodes at 24 h, suggesting onward migration from the airway. Transient up-regulation of CD86 on AMDC accompanies this process, which can be reproduced by coculture of resting AMDC with T memory cells plus antigen. The APC activity of AMDC can be partially inhibited by anti-CD86, suggesting that CD86 may play an active role in this process and/or is a surrogate for other relevant costimulators. These findings provide a plausible model for local T cell activation at the lesional site in asthma, and for the transient nature of this inflammatory response.

Published

2003

11. Involvement of plasmacytoid dendritic cells in human diseases.

Author

Jahnsen FL, Farkas L, Lund-Johansen F, and Brandtzaeg P

Subjects

Dendritic Cells immunology, Dendritic Cells metabolism, Dendritic Cells virology, Humans, Lupus Erythematosus, Systemic immunology, Lupus Erythematosus, Systemic metabolism, Dendritic Cells pathology, Interferon-alpha biosynthesis, Lupus Erythematosus, Systemic pathology

Abstract

In vitro studies have reported that plasmacytoid dendritic cells (PDCs) exert multiple functions, including production of interferon (IFN)-alpha as effector cells and regulation of T-cell responses as mature DCs. Here we review recent data obtained in situ showing that PDCs accumulate in lesions of type I IFN-related disorders (virus infections and lupus erythematosus), Th2 cell-dominated allergic reactions, and ovarian carcinoma. These results demonstrate that PDCs do migrate to peripheral tissues during inflammation, which lends further support to the view that PDCs most likely are important players in innate and adaptive immunity in vivo. Future research should aim at defining the exact pathogenic or defense roles of PDCs in such disorders and determine whether these cells are potential targets for therapeutic intervention in microbial infections, allergy, autoimmunity, or cancer.

Published

2002

12. CD1c-Expression by Monocytes – Implications for the Use of Commercial CD1c+ Dendritic Cell Isolation Kits.

Author

Schrøder, Martine, Melum, Guro Reinholt, Landsverk, Ole J. B., Bujko, Anna, Yaqub, Sheraz, Gran, Einar, Aamodt, Henrik, Bækkevold, Espen S., Jahnsen, Frode L., and Richter, Lisa

Subjects

MONOCYTES, DENDRITIC cells, HOMEOSTASIS, T cells, CELL surface antigens

Abstract

Conventional dendritic cells (cDCs) comprise a heterogeneous population of cells that are important regulators of immunity and homeostasis. CD1c+ cDCs are present in human blood and tissues, and found to efficiently activate naïve CD4+ T cells. While CD1c is thought to specifically identify this subset of human cDCs, we show here that also classical and intermediate monocytes express CD1c. Accordingly, the commercial CD1c (BDCA-1)+ Dendritic Cell Isolation Kit isolates two distinct cell populations from blood: CD1c+CD14− cDCs and CD1c+CD14+ monocytes. CD1c+ cDCs and CD1c+ monocytes exhibited strikingly different properties, including their differential regulation of surface marker expression, their levels of cytokine production, and their ability to stimulate naïve CD4+ T cells. These results demonstrate that a commercial CD1c (BDCA-1)+ Dendritic Cell Isolation Kit isolates two functionally different cell populations, which has important implications for the interpretation of previously generated data using this kit to characterize CD1c+ cDCs. [ABSTRACT FROM AUTHOR]

Published

2016

13. Pathogenic Mechanisms of Allergic Inflammation : Atopic Asthma as a Paradigm.

Author

Holt, Patrick G., Strickland, Deborah H., Bosco, Anthony, and Jahnsen, Frode L.

Subjects

ALLERGIES, INFLAMMATION, ASTHMA, RESPIRATORY infections, ALLERGENS, DENDRITIC cells, EPITHELIAL cells, T cells

Abstract

Prospective studies tracking birth cohorts over periods of years indicate that the seeds for atopic asthma in adulthood are sewn during early life. The key events involve programming of functional phenotypes within the immune and respiratory systems which determine long-term responsiveness to ubiquitous environmental stimuli, particularly respiratory viruses and aeroallergens. A crucial component of asthma pathogenesis is early sensitization to aeroallergens stemming from a failure of mucosal tolerance mechanisms during the preschool years, which is associated with delayed postnatal maturation of a range of adaptive and innate immune functions. These maturationa[ defects also increase risk for severe respiratory infections, and the combination of sensitization and infections maximizes risk for early development of the persistent asthma phenotype. Interactions between immunoinflammatory pathways stimulated by these agents also sustain the disease in later life as major triggers of asthma exacerbations. Recent studies on the nature of these interactions suggest the operation of an infection-associated lung:bone marrow axis involving upregulation of FcERlα on myeloid precursor populations prior to their migration to the airways, thus amplifying local inflammation via IgE-mediated recruitment of bystander atopic effector mechanisms. The key participants in the disease process are airway mucosal dendritic cells and adjacent epithelial cells, and transiting CD4+ effector and regulatory T-cell populations, and increasingly detailed characterization of their roles at different stages of pathogenesis is opening up novel possibilities for therapeutic control of asthma. Of particular interest is the application of genomics-based approaches to drug target identification in cell populations of interest, exemplified by recent findings discussed below relating to the gene network(s) triggered by activation of Th2-memory cells from atopics. [ABSTRACT FROM AUTHOR]

Published

2009