Abstract
Airway inflammation is a critical feature of the airway diseases asthma and chronic obstructive pulmonary disease (COPD). There is emerging evidence that structural cells play a key role in the development and perpetuation of the inflammatory response and are pivotal in the development of the changes in the airway structures that lead to airway remodelling.
To date, little attention has been given to the localisation of inflammatory cells to airway structures or the potential interactions between these intimately located cells. However, it is likely that interactions between inflammatory and structural cells in the airway contribute enormously to the pathophysiology of asthma and COPD.
Indeed, recent evidence suggests that mast cells localised to the airway smooth muscle bundle may be important in the development of airway hyperresponsiveness in asthma.
In the present article, the authors aim to summarise: 1) the current understanding of which inflammatory cells locate to airway structures; 2) the proposed mechanisms that may be involved in mediating this microlocalisation; 3) the possible consequences of interactions between inflammatory and structural cells; and 4) the pressing need to investigate whether modulating these interactions is beneficial in asthma and chronic obstructive pulmonary disease.
The prevalence of obstructive airway diseases, namely asthma and chronic obstructive pulmonary disease (COPD), are increasing. Asthma affects 10% of children and 5% of adults 1, 2, and by 2020 it is predicted that COPD will be the third leading cause of mortality worldwide 3. Both conditions are defined in terms of typical symptoms and abnormal airway physiology, but it is also well recognised that airway inflammation and airway remodelling are key components of both diseases 4, 5.
Asthma is characterised by airway hyperresponsiveness (AHR) and variable airflow obstruction. The airway inflammation in asthma is typically eosinophilic with increased expression of T-helper cell (Th) type 2 cytokines 6. Airway remodelling in asthma encompasses several structural changes in the airway wall, including reticular lamina and basement membrane thickening, an increased number of subepithelial myofibroblasts and increased airway smooth muscle (ASM) mass 7, 8.
The hallmark of COPD is irreversible airflow obstruction. Pathologically, COPD consists of a combination of emphysema and obliteration of the small airways. These two pathologies are distinct, in that emphysema can occur without narrowing of the small airways and vice versa, although the conditions usually coexist 9. Small airway narrowing results as a consequence of mucus hypersecretion, inflammation and remodelling due to fibrosis, and increased ASM mass 4. The inflammatory infiltration in the airway in COPD comprises of T-cells with a relative preponderance of CD8+ cells, macrophages and neutrophils 4, 10.
Although the features of the disordered airway physiology, inflammatory profile and structural changes in the airway in asthma and COPD are well described, the interactions between these components of airway disease are poorly understood. To date, little attention has been paid to the localisation of inflammatory cells within structural compartments of the airway wall. Recently, enthusiasm for the view that microlocalisation is important in obstructive airway diseases has been fuelled by studies showing inflammatory cells within the ASM in asthma 11–18 and COPD 19, but not in normal controls. Most notably, in asthma the ASM is infiltrated by mast cells and the number of mast cells within the ASM bundle was associated with the degree of AHR 11.
Communication between cells within the airway predominately occurs across distances of only a few microns, as many inflammatory mediators are rapidly inactivated once they leave the cell. Thus, direct cell–cell interactions are likely to be critical in modulating cellular function. It is therefore likely that microlocalisation between inflammatory and structural cells is a fundamental organising principle of airway inflammation and repair.
The present study will: review the evidence that inflammatory cells localise to structural cells focused particularly on mast cell localisation to the ASM bundle; review the functional consequences of interactions between these cells; review the mechanisms driving this co-location; consider how these interactions may be further studied; and speculate on the therapeutic potential of modifying these interactions.
INFLAMMATORY CELL MICROLOCALISATION TO STRUCTURAL COMPONENTS WITHIN THE AIRWAY
Most immunopathological descriptions of asthma and COPD have focused on the number of inflammatory cells that infiltrate the airway submucosa. Often, structural components of the airway are excluded. There is an increasing recognition that inflammatory cells selectively localise to different airway structures in disease (as summarised in table 1⇓) and it is biologically plausible that this microlocalisation has important functional consequences. For example, bronchoconstriction is a consequence of ASM contraction. Therefore, the localisation of inflammatory cells within the ASM bundle is likely to modulate AHR and variable airflow obstruction.
The recognition of the importance of microlocalisation is not confined to inflammatory cells and ASM cells but is equally critical in interactions with other structural cells, such as the epithelium, fibroblasts, mucosal glands and nerve cells.
Inflammatory cell localisation to ASM bundle
In asthma and, according to some reports, in nonasthmatic subjects, the ASM bundle is infiltrated by mast cells, predominately of the chymase-positive phenotype 11–18. Mast cell–ASM interactions in asthma are summarised in figure 1⇓. Mast cells adhere avidly to ASM, in part via a tumour suppressor in lung cancer-1 heterophilic adhesion molecule and in part via an unidentified Ca2+ independent pathway 47. Mast cell number correlated positively with the degree of AHR 11 and with the bronchoconstrictor response to a deep inspiration 44, suggesting that mast cell–ASM cell interactions are likely to be central in the development of the disordered physiology in asthma. The strength of this assertion was underpinned by the paucity of mast cells within the ASM bundle in eosinophilic bronchitis, a condition that presents with chronic cough and shares many of the immunopatholgical features of asthma but is not associated with airflow obstruction or AHR 11, 25, 48–50. Although most studies have reported an increase in the number of mast cells in the ASM bundle in asthma, some have not been able to confirm this observation 42. However, although Balzar et al. 51 did not report a significant increase in the number of mast cells in the ASM bundle in asthma, the numbers were double that observed in normal controls and this almost reached statistical significance (p = 0.06). Importantly, there is evidence that mast cells infiltrating the ASM bundle are activated with increased expression of Th2 cytokines interleukin (IL)-4 and IL-13 43. A post mortem study of fatal and nonfatal asthma has shown that there was a marked increase in mast cell degranulation in the ASM bundle in both the large and small airways 12. Another study demonstrated that increased numbers of mast cells (degranulated and intact) are associated with increased ASM shortening in fatal asthma 37. Interestingly, there was a paucity of other inflammatory cells, with only one study reporting the presence of T-cells in the ASM bundle 18, suggesting that it is predominantly mast cells that are selectively recruited to the ASM bundle.
Inflammatory cell localisation to the ASM bundle is also a phenomenon of COPD. Baraldo et al. 19 found increased numbers of neutrophils and CD8+ cells, but not mast cells, in the small airways of smokers with COPD, and noted that the neutrophil number was inversely related to lung function. This is consistent with an earlier study showing that the number of neutrophils in the ASM bundle in small airways in smokers is related to air trapping determined by computed tomography scanning 45. In the latter report, there was also a relationship between air trapping, reflecting peripheral obstruction and infiltration of ASM by chymase-positive mast cells. This result indicates that mast cells may also play a role in COPD, at least at the peripheral level. This picture is not replicated in the large airway in COPD as, although T-cells, macrophages and mast cells were present in the ASM bundle, the number of inflammatory cells in the ASM bundle was not different between subjects with COPD (Global Initiative for Obstructive Lung Disease (GOLD) I-II) and non-COPD smoking and nonsmoking controls 39, 42, 46. However, in contrast to studies in asthma, macrophages, neutrophils and T-cells were observed in the ASM bundle in low numbers in resection specimens from subjects with and without COPD. Most of the subjects in these studies were older and had undergone lung resection for cancer; thus, although the airways studied were considered to be from unaffected areas, there remains the possibility of the underlying lung cancer contributing to the inflammatory changes described. Nevertheless, the body of evidence strongly suggests that microlocalisation of inflammatory cells within the ASM bundle is an important feature in the small airway in COPD and in both the large and small airway in asthma.
Activation of the inflammatory cells within the ASM bundle would be predicted to have important consequences on ASM function. Following mast cell degranulation, the mediators histamine, prostaglandin (PG)D2 and leukotriene (LT)C4 are released, which are all potent agonists for ASM contraction 52. Mast cell cytokines may further contribute to AHR. The mast cells in the ASM bundles in asthma, but not in COPD, express IL-13 53. IL-13 has been shown to attenuate relaxation to β-agonists and augment contractility to acetylcholine 54, 55. Similarly, the mast cell protease may be important in modulating ASM contractility and AHR 56. The effect of neutrophil-derived mediators on ASM function is less clear, with conflicting reports from animal studies showing that elastase can increase and diminish smooth muscle responsiveness 57, 58.
The interactions between inflammatory cells and ASM cells may have more long-term consequences. Mast cells co-cultured with ASM promote ASM differentiation with increased α-smooth muscle actin expression 59. Similarly, mast cell differentiation towards the chymase-positive phenotype observed within the ASM bundle may be mediated by mast cell–ASM interactions. Increased ASM mass is a well-established feature of both asthma 60 and COPD 10. A number of mast cell mediators, including histamine 61, tryptase 62 and LTD4 63, as well as the neutrophil product elastase 64, promote ASM proliferation. Alternatively, increased ASM mass may be a consequence of recruitment of ASM progenitors. This view is supported by the increased number of fibrocytes that migrate into the airway following allergen challenge 65. Recent evidence suggests that ASM migration towards the ASM bundle is mediated by activation of CC chemokine receptor (CCR)7, ASM- and mast cell-derived CC chemokine ligand (CCL)19 26. In asthma, increased ASM mass occurs predominantly in the large airway and in COPD in the small airways. Small ASM mass is inversely associated with post-bronchodilator forced expiratory volume in one second in COPD 10. Using a computational model, increased muscle mass has been shown to be probably the most important abnormality responsible for the increased airflow resistance observed in response to bronchoconstricting stimuli in both asthma and COPD 66. Consistent with this view, in a cross-sectional study of the immunopathology of asthma across severity using a multiple regression model, increased ASM mass and ASM hypertrophy were the features of remodelling that were associated most strongly with impairment in lung function 7. The relative contribution of ASM mass to overall airway wall thickness in the small airways is much greater than that in the large airways. Thus, increased ASM mass in the small airways is likely to make a significant contribution to the development of fixed airflow obstruction characteristic of COPD and sometimes seen in persistent chronic severe asthma.
Therefore, mast cell interactions with ASM in asthma are likely to be important in the development of AHR and may play a critical role in the development of increased ASM mass and the development of fixed airflow obstruction seen in severe disease. The role of inflammatory cell–ASM interactions in COPD in the small airway may be related to gas trapping, but in the large airway the role of ASM–inflammatory cell interactions is uncertain and needs to be further explored.
Inflammatory cell localisation to (myo)fibroblasts
In asthma, interactions between the airway epithelium and mesenchymal cells, known as the epithelial-mesenchymal trophic unit, are well described 67, 68. There are increased numbers of subepithelial myofibroblasts in asthma, which are correlated with the degree of reticular basement membrane thickening 69. This layer of mesenchymal cells is in close proximity to the epithelium and the activation of the airway epithelium, secondary to epithelial damage, is likely to be critical in regulating the activation of the airway mesenchyme. Whether inflammatory cells are co-localised to subepithelial mesenchymal cells is unclear. However, there is evidence that implicates mast cells, eosinophils and T-cells in playing a key role in perpetuating interactions between epithelial and mesenchymal cells. For example, in co-culture with mast cells, primary bronchial fibroblasts from asthmatics increase their expression of pro-collagen 1 expression mediated by mast cell-derived IL-4 70. Cytokines IL-4 and IL-13 activate epithelial cells in vitro to produce transforming growth factor (TGF)-β2, as well as having a direct effect upon myofibroblasts promoting CCL11 release and eosinophil recruitment to the subepithelium 71. Submucosal mast cells, eosinophils 43, 72 and T-cells 73 are important sources of these cytokines.
In COPD, subepithelial fibrosis is an important component of small airway obliteration. However, the importance of inflammatory cells localised and interacting with mesenchymal cells in this disease is unclear.
Inflammatory cell localisation to mucus glands
Mucus production is a cardinal feature of asthma and COPD and mucus gland hyperplasia is a feature of both conditions 39, 74–76. Patients with asthma across the spectrum of severity, including fatal asthma, demonstrate increased numbers of degranulated mast cells 12, 37 and neutrophils 38 within submucosal glands compared with controls. However, the degree of mucus-related obstruction expressed as the percentage of the airway lumen occupied by mucus only correlated with mast cell numbers and not with neutrophil numbers 38. In COPD, the submucosal glands are infiltrated by neutrophils and macrophages 31. Whether mast cells infiltrate the mucus glands in COPD is controversial, with two reports supporting 32, 39 and another refuting 31 the location of mast cells in glands. Eosinophils and T-cells were not increased in number in submucosal glands in asthma or COPD. A recent report has demonstrated that plasma cells are increased in the submucosal glands in patients with COPD and chronic bronchitis without airflow limitation, compared with smoking controls 39. Furthermore, there was a close correlation between the number of plasma cells in glands and the number of IL-4 mRNA cells and protein expressing cells within the glands, and an increase in mucus in the glandular epithelium compared with smoking controls. Mast cells were present but not increased in glands and the ASM in COPD, chronic bronchitis and smoking controls in the study 39.
Mast cell proteases, tryptase and chymase are potent stimuli for mucus secretion and other mast cell mediators, PGD2 and LTC4 40, together with mast cell-derived cytokines, IL-6, IL-13 77 and IL-4 78, have also been implicated in glandular hyperplasia and mucus production. More recently, mast cell expression of amphiregullin, a member of the epidermal growth factor family, was increased in asthma and this upregulates mucin gene expression by epithelial cells, implicating amphiregullin in goblet cell metaplasia and mucus hypersecretion 79, 80. Similarly, neutrophils may promote mucus hypersecretion by upregulation of MUC5AC by neutrophil elastase 81, 82.
Inflammatory cell localisation to airway epithelium
A variety of inflammatory cells infiltrate the airway epithelium. This is likely to be important, as it places these cells at the mucosal interface with pathogenic and allergic stimuli promoting an effector role for inflammatory cells in the ongoing immune response and facilitating cellular interactions. In asthma and healthy subjects, T-cells are the most abundant inflammatory cell in the epithelium 20, 25, 27, 28 but increased numbers of T-cells in the epithelium in disease is rarely reported 20, and most studies do not support the view that T-cells are selectively recruited to the epithelium 21, 27. Similarly, in COPD, both granulocytes and T-cell numbers have been shown to be increased in the epithelium in some studies 31, 35 but not in all 31, 33, 34. In contrast, eosinophils and dendritic cells are consistently reported to be increased in the epithelium in asthma 20, 22, 25, 29, 30. In most reports 13, 20–24, 32, 33, but not all 25, 27–29, 31, 37, mast cell numbers are increased in the airway epithelium in asthma and COPD. In addition, neutrophil infiltration into the airway epithelium is a feature of COPD 27.
Mast cells adhere avidly to airway epithelium via a carbohydrate-dependent mechanism 83 and mast cell survival is promoted by epithelial cell-derived stem cell factor 84. Mast cells activate epithelial cells through release of IL-4, IL-13 and tryptase 43, 85, but in contrast epithelial cells attenuate both constitutive and immunoglobulin (Ig)E-dependent histamine release from human lung mast cells 86.
Eosinophils adhere to epithelial cells via a CD18-dependent mechanism closely regulated by the local cytokine milieu 87, 88, and survival is maintained, in part, by release of nerve growth factor and brain-derived growth factor. Adhesion leads to eosinophil activation, release of eosinophil cationic protein 89 and promotes epithelial apoptosis 90. T-cells also promote epithelial apoptosis 90, activation via release of cytokines and, reciprocally, epithelial cells augment T-cell proliferation and activation 91. The increase in epithelial apoptosis may contribute to the increased epithelial fragility and shedding often described in asthma 8, although whether this is a real feature of asthma or a biopsy artefact remains unclear 92, 93.
Survival of dendritic cells in the airway epithelium is maintained in part by granulocyte-macrophage colony-stimulating factor (GM-CSF) released by the epithelium in response to protease-activated receptor-2 activation 94. Retention is augmented by enhanced epithelial intercellular adhesion molecule-1 expression and activation with Th2 polarisation by release of a variety of mediators, in particular PGE2 and IL-10 95, 96. Reciprocally, the expression of CD40L by dendritic cells enhances production of chemokines, pro-inflammatory cytokines and epithelial defensins by the asthmatic epithelium, and represents an important arm of the innate epithelial immune response 97.
Inflammatory cell localisation to airway nerves
To date, interest has focused on eosinophil–airway nerve interactions. Eosinophils have been shown to cluster around cholinergic nerves in patients with fatal asthma 41. There are no reports in human disease that describe the presence or absence of other inflammatory cells co-localised to airway nerves, but a guinea pig model of asthma suggests that there may be selective localisation of esoinophils to airway nerves as there was a paucity of other inflammatory cells.
The dominant nervous innervation of the airways is vagally mediated via the parasympathetic nervous system 98. Release of acetylcholine from these nerves has a variety of consequences regulated by local muscarinic receptors, including bronchoconstriction 98, release of mucus from glands 99 and vasodilatation 100. Cholinergic-mediated AHR seems to be related to loss of muscarinic 2 receptor (M2R) inhibition rather than increased expression/altered function of M3R on ASM 101, 102. The interaction of eosinophils with M2Rs is important to the pathogenesis of neuronal AHR. Eosinophils co-cultured with human Caucasian neruoblastoma cell line cell leads to increased expression of the M2R, which is mediated via an adhesion-dependent release of eosinophil proteins, including major basic protein and nerve growth factor, increasing acetylcholine release and potentiating vagally mediated bronchoconstriction 103.
Eosinophilic bronchitis, cough, variant asthma and idiopathic chronic cough are associated with increased concentration of mast cell products in sputum 104, 105. Therefore, it is possible, but as yet unproven, that localisation of mast cells to sensory nerve endings might be important in the development of cough reflex hypersensitivity and cough. A rather similar interaction is thought to be important in the genesis of itch 106, 107. In COPD, the potential role of airway nerve–inflammatory cell interactions has not been investigated.
Inflammatory cell localisation to vasculature
Vascular remodelling occurs in asthma and COPD 108–111 and is associated with airflow obstruction 108. The role of vascular remodelling in the development of AHR in asthma is contentious. Kanazawa et al. 112 demonstrated that vascular epidermal growth factor (VEGF) was increased in the sputum in asthma, but not in nonasthmatic eosinophilic bronchitis, and correlated with increased airway vascular permeability and AHR. However, the duration of disease in the nonasthmatic eosinophilic bronchitis cohort in the study by Kanazawa et al. 112 is unclear and disease duration is critical in assessing the impact of some features of airway remodelling 113. The current authors have recently demonstrated in patients with chronic nonasthmatic eosinophilic bronchitis that vascular remodelling does occur to a similar degree as in moderate-to-severe persistent asthma and is, therefore, unlikely to be related to AHR 114. The increased vascularity in asthma was related to disease duration and airflow obstruction, but not AHR.
Very few studies have examined the association of cellular interactions and vascular remodelling in asthma and COPD. Chetta et al. 111 demonstrated that the number of mast cells in the subepithelium correlates with the number of vessels in asthma; however, a similar correlation was not observed for eosinophilic airway inflammation. Although studies have described an association with sputum VEGF and percentage of eosinophilia in sputum 115, a similar relationship in vivo has not been described. Despite the lack of data linking airway inflammation and vascular remodelling in asthma, growth factors (VEGF, β-fibroblast growth factor and angiogenin) co-localise predominantly to eosinophils, macrophages and CD34+ cells in vivo, and the expression of these growth factors correlates with the percentage of vascularity of the airway wall 116. Furthermore, the expression of the main signalling receptor for VEGF (FLT-1) is increased in vessels in asthmatics 109. Taken together, these observations suggest that eosinophils, macrophages and mesenchymal cells may be important in regulating vascular remodelling in asthma. However, it remains unclear whether inflammatory cells are selectively co-localised to vessels in asthma or COPD.
IS THE PATTERN OF LOCALISATION OF INFLAMMATORY CELLS TO AIRWAY STRUCTURES CONSISTENT BETWEEN SMALL AND LARGE AIRWAYS?
Although a large number of studies have examined cellular localisation to the airway wall in large and small airways, few have assessed the distribution of inflammatory cells to specific structures within the airway wall according to airway size.
Mast cell smooth muscle mysotitis has been consistently observed in proximal ASM and has also been reported in small airway wall smooth muscle in asthma 11, 12, 13, 16–18, 37. Although mast cell density was increased in membranous compared with cartilaginous airway in the epithelium and ASM in one study 12, mast cell numbers were not increased in COPD compared with controls in the proximal airway smooth muscle 39, 46 and conflicting data exist for the distal airways. One study showed increased mast cells in the ASM 45 and another reported that numbers were not increased compared with healthy controls 19. Similarly, T-cells, neutrophils and macrophages (but not eosinophils) have been observed in the ASM in large and small airways in COPD, but only small airway CD8+ T-cells and neutrophils have been shown to be increased compared with healthy controls 19, 46.
Further studies are required to establish whether the localisation of inflammatory cells to airway structures is consistent between large and small airways in asthma and COPD.
WHAT MECHANISMS ARE INVOLVED IN SELECTIVE LOCALISATION?
Inflammatory cells microlocalise to specific compartments within the airway, with an abundance of some and a paucity of other cells within airway structures. Inflammatory cell localisation is a feature of asthma and COPD, but interestingly the pattern of this microlocalisaion is different. This raises the question: what are the mechanisms controlling the selective recruitment of inflammatory cells to structural compartments within the airway?
Granulocyte trafficking has been extensively studied and characterised 117. For example, the recruitment of eosinophils into the airway is mediated by a multi-step process directed by Th cytokines. The first step is increased production and release of eosinophils from the bone marrow under the influence of IL-5 118, 119 and specific chemoattractants, such as CCL11 (eotaxin) 120, CCL5 (RANTES) 121, CCL12 (monocyte chemotactic protein-5) 121 and CCL3 (macrophage inhibitory protein-1α) 121. Secondary target organ vasculature has increased adhesiveness for eosinophils through the specific effects of locally generated IL-4 and IL-13. These cytokines induce the expression of vascular cell adhesion molecule (VCAM)-1 that binds to eosinophils through the very late activation antigen-4 receptor, which is not expressed by neutrophils, and P-selectin, to which eosinophils bind with greater avidity than neutrophils 122–124. The interaction of the eosinophil with these adhesion molecules is mediated by integrins (α4β1 and α4β7) 125, 126, which have been shown to bind to VCAM-1 127. Following adhesion, transmigration across the endothelium is mediated by complement proteins such as C5a 128. The final phase of trafficking involves chemotaxis, which is mediated by chemokines, such as CCL11 129, and involves encryption and passage through the matrix network of the airway wall. CCL11 has been shown to bind to CCR3, a high-affinity receptor expressed by eosinophils, and mediates directional migration through tissue 130. Survival of eosinophils is augmented by IL-5 131 and GM-CSF 132. In contrast, the mechanisms involved in the recruitment of inflammatory cells in tissue to structural components is poorly understood.
Selective recruitment of inflammatory cells to the ASM is likely to be mediated by smooth muscle-derived chemoattractants and by the maintenance of the correct microenvironment to maintain cell differentiation and survival. ASM has a significant secretory capacity, so it clearly has the potential to recruit inflammatory cells 133. For example, CXC chemokine ligand (CXCL)8 (IL-8) and CXCL10 (interferon-inducible protein-10) released by activated ASM in COPD may mediate neutrophil and CD8+ cell migration into the ASM bundle in the small airway 134, 135. A plethora of chemotactic factors for mast cells are released by ASM, notably stem cell factor 16, CCL11 (eotaxin) 136–138, CXCL8 (IL-8) 136, 139, CX3C chemokine receptor 1 17 and TGF-β 16. CXC chemokine receptor (CXCR)3 is the most abundantly expressed chemokine receptor on human lung mast cells within the ASM bundle. Human lung mast cell migration is induced by the CXCR3 ligand CXCL10, which is released preferentially from Th1-stimulated asthmatic ASM cells compared with those from healthy controls 140 and is released in response to Toll-like receptor-3 activation 141. Interestingly, Th2-stimulated ASM from asthmatics is chemotactic for mast cells compared with nonasthmatic ASM mediated via activation of CCR3 and CXCR1. This is not due to differential expression of chemokines but is likely to be due to the release of a factor that inhibits mast cell migration released by the nonasthmatic ASM 138. It is also important to consider why some inflammatory cells, notably eosinophils and T-cells, are rarely seen in the ASM in spite of appropriate chemotactic signals. Eosinophil paucity in ASM may be explained by selective cleavage of eosinophil chemoattractants CCL5 (RANTES) and CCL11 (eotaxin) by mast cell β-tryptase 142. Similar interactions may explain the lack of other cells, such as T-lymphocytes from ASM bundles, in asthma as Lazaar et al. 143 demonstrated that mast cell chymase inhibited integrin-mediated T-cell adhesion to ASM cells.
Similarly, the airway epithelium has the capacity to secrete a number of chemokines that are involved in the recruitment of inflammatory cells 144, 145. The induced sputum CXCL10 concentration from subjects with nonasthmatic eosinophilic bronchitis is increased and mediates mast cell migration via CXCR3 activation 146. Airway epithelium is an important source of CCR3 ligands, which play a role in the recruitment of mast cells, eosinophils and Th2 cells. CXCL8 is an important neutrophil and mast cell chemoattractant, and its expression is increased in induced sputum from subjects with COPD 147, 148 and neutrophilic asthma 149, and is increased in response to cigarette smoke 150. How chemokines interact to recruit inflammatory cells to the airway epithelium is poorly understood and it is unknown why there is less selection in cell recruitment than observed in the ASM.
Chemokine expression by airway mucus glands has not been extensively examined. CXCL8 mRNA expression by mucus glands is increased in response to Pseudomonas infection in bronchiectasis 151. However, to date, there are no data to explain the selective recruitment of mast cells and neutrophils to the airway mucus glands in asthma, and neutrophils and macrophages in COPD. The mechanisms described to date involved in the selective microlocalisation of mast cells to ASM, epithelium and mucosal glands in asthma are summarised in figure 2⇓.
Eosinophil localisation to airway nerves is mediated by the release of CCR3 ligands by nerves 152. It would be predicted that airway nerve-derived CCL11 would also recruit Th2 cells and mast cells, but whether eosinophil localisation to the airway nerves in human disease is selective is unclear.
It is likely that a number of chemokines, other chemotaxins and inhibitory factors play a role in the selective recruitment of inflammatory cells into the airway. As previously described, it may be that the release of chemotaxins by ASM and other airway structural cells varies in response to different stimuli, such as cigarette smoke, infection or allergen exposure. Future studies should explore the relative importance of these triggers and the associated network of chemotaxins that are released in promoting selective inflammatory cell microlocalisation to structural compartments of the airway.
HOW CAN INFLAMMATORY CELL MICROLOCALISATION AND ITS CONSEQUENCES BE MEASURED OR MODELLED?
Animal models have provided insight into the mechanisms that underlie inflammatory cell migration into the airway. There has been little focus on the localisation of cells to structural components of the airway and currently there is no established animal model to study mast cell localisation to the ASM bundle. Indeed, on the contrary, in a rat model of asthma CD4+ cells were located within the ASM bundle and were implicated in driving ASM proliferation 153. However, whether T-cell localisation to the ASM bundle is a feature of asthma is contentious, with one report supporting this view but most unable to identify T-cells in the ASM bundle. Therefore, the relevance of current animal models to human disease is questionable.
In vitro two-dimensional migration assays have been informative about inflammatory cell migration towards primary structural cells from asthmatics 140, but further work studying cell migration in three-dimensional culture systems and in ex vivo bronchial biopsies using advanced imaging, for example two-photon microscopy 154, may improve current understanding of inflammatory cell migration in more biologically relevant models.
Whether inflammatory cell–structural cell interactions drive airway remodelling is unclear. However, advances in design-based stereological methods in the assessment of bronchial biopsies 155–158 and improvements in imaging techniques 159–162 have provided new objective tools with reduced bias to assess airway remodelling. These approaches will assist in defining the interplay between inflammatory cell localisation to the airway structures, disordered airway physiology and remodelling in obstructive airways disease. It is important that future studies not only use these techniques in cross-sectional studies but are used to study airway remodelling longitudinally and the effects of pharmacological and nonpharmacological interventions.
CAN LOCALISATION BE MODULATED: IS THERE EVIDENCE TO SUGGEST THIS MAY BE HELPFUL?
There are relatively few studies that have examined the inflammatory cell composition of bronchial biopsies in response to anti-inflammatory therapies in asthma and COPD 28, 30, 33, 163–171. To date, none of these have examined the effect of treatment on cellular infiltration into the ASM bundle, mucus gland or localisation to airway nerves. Therefore, it is unknown whether recruitment of inflammatory cells into these compartments is steroid responsive, or indeed responsive to any current therapy, or whether it is refractory to anti-inflammatory therapy.
In asthma, oral and inhaled corticosteroids consistently reduce the number of eosinophils in the airway epithelium 28, 30 and some, but not all, report reductions in T-cells and mast cells 28. A limited number of bronchoscopy studies that have examined the anti-inflammatory effect of corticosteroids in COPD have not identified a consistent anti-inflammatory effect 33, 163, 164. For other anti-inflammatory therapy the picture is also unclear and the data sparse. There are no reports on the effects of anti-LT therapy on cellular localisation to airway structures; anti-IgE in asthma led to a reduction in T-cells in the airway epithelium 172 but there was no change in other cell numbers and the phosphodiersterase-4 inhibitor cilomilast had no effect on neutrophil numbers in the epithelium in COPD 173. There is therefore a pressing need to understand the effect of current treatment on modulating inflammatory cell localisation to structural cells.
Recruitment of inflammatory cells into the airway is an important target for treatment of asthma and COPD. In addition to treatments with broad anti-inflammatory actions, a number of antibody and small-molecule therapies have been developed, or are in development, to target specific aspects of cell trafficking 174. For example, anti-IL-5 reduces the number of eosinophils in the airway 175 but whether this has an impact on eosinophil infiltration into the epithelium is unknown and, more importantly, whether anti-IL-5 has clinical benefits, e.g. in reducing asthma exacerbations, is uncertain. In animal models of asthma, CCR3 antagonists reduce the clustering of eosinophils along cholinergic nerves and AHR secondary to M2R dysfunction 152. In COPD, strategies to block CXCR2 and CXCR3 are in development and may offer novel approaches to reducing the inflammatory profile in COPD, which is currently not affected by pharmacotherapy. The potential efficacy of such an approach is supported by a recent safety study that used a monoclonal antibody to IL-8 in COPD, which resulted in small improvements in dyspnoea score 176. Alternative strategies that target events in cellular activation involved in migration may offer novel therapies. For example, the mast cell calcium-activated potassium channel modulates the retraction of the cell body during migration. Specific inhibition of this ion channel by TRAM-34 attenuated CXCL10-mediated mast cell migration 177.
Whether inflammatory cell localisation to structural cells can be modulated by current and future treatments needs to be examined further and the functional consequences of this inhibition need to be fully determined.
CONCLUSION
Emerging evidence suggests that inflammatory cell microlocalisation to structural cells has important functional consequences. Understanding the fundamental steps that are involved in the migration of inflammatory cells towards structural cells, such as the airway smooth muscle bundle and the interactions between these cells, may provide novel targets for the future treatment of asthma and chronic obstructive pulmonary disease. Therefore, researchers interested in the immunopathology of airway diseases need to be mindful of the importance of inflammatory cell localisation and consider how this may be modulated in the future.
Statement of interest
None declared.
- Received December 12, 2006.
- Accepted July 30, 2007.
- © ERS Journals Ltd
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