Apoptotic mechanisms in the pathogenesis of COPD.

COPD is a leading cause of morbidity and mortality, characterized by a chronic abnormal inflammatory response to noxious agents. Apoptosis is a physiologic process, critical to cellular homeostasis, in which cell death follows a programmed sequence of events. Apoptosis has been recognized to play an important role in clinical and experimental models of lung diseases. Abnormal apoptotic events in smokers' and in emphysematous lungs have been shown in epithelial and endotheliallung cells, neutrophils, lymphocytes, and myocytes. Many factors associated with COPD, including cigarette smoke, have the potential to cause apoptosis of alveolar epithelial cells, the main sites of vascular endothelial growth factor (VEGF) production. The decreased expression of VEGF, a known survival factor for endothelial cells, and its receptor, results in lung septal endothelial cell death, leading perhaps to the emphysema observed in COPD. In smokers who develop COPD there is an activation of adaptive immunity, with an infiltration of CD4+ and, especially, CD8 + cells. CD8 + cells are cytotoxic to epithelial cells through the release of granzymes and perforin, which can further induce apoptosis of alveolar cells. Moreover, any reduction in neutrophil apoptosis or dysregulation of macrophage uptake of apoptotic neutrophils could lead to chronic inflammation and tissue injury. Increased rates of T-cell apoptosis may lead to a defective immune response to infective organisms, contributing to the high frequency of infections seen in COPD. Increased apoptosis of skeletal muscle could be responsible for the skeletal muscle atrophy, the main cause of unexplained weight loss in patients with COPD. This paper is a review of the current knowledge on the apoptotic pathways involved in COPD pathogenesis and their interaction with other known contributing factors.

Introduction

COPD is a leading cause of chronic morbidity and mortality worldwide, with a substantial economic and social burden (Siafakas et al 1995; Celli et al 2004; Pauwels and Rabe 2004). The 2002 WHO World Health Report listed COPD as the fifth leading cause of death in the world and further increases in its prevalence and mortality are expected in the coming decades (WHO 2002; Pauwels and Rabe 2004). Recently, the ATS–ERS Task Force has published a document on the pathogenesis, diagnosis, monitoring, and management of COPD (Celli et al 2004). The latest definition of COPD according to this document notes that COPD is “characterised by airflow limitation that is not fully reversible... is usually progressive and is associated with an abnormal inflammatory response of the lungs to noxious particles or gases, primarily caused by cigarette smoking ... it also produces significant systemic consequences.” (Celli et al 2004). Although significant progress has been made on the pathogenesis of COPD, the overall picture remains unclear.

Apoptosis, programmed cell death, is a highly ordered physiologic process by which useless, irreparably damaged or unwanted cells are eliminated throughout life. This process has attracted great attention in recent years, though the lung has been relatively little investigated. Elucidating the regulating mechanisms of apoptosis in lung cells should contribute to the understanding of the pathophysiology of lung disorders and allow identification of specific therapeutic targets (Plataki et al 2005).

This review focuses on the existing literature on apoptosis in COPD, and the potential role of apoptosis on COPD pathogenesis. A synopsis of the relevant literature is presented in Table 1.

Table 1

Studies of apoptosis in COPD

Cell type		Reference
Epithelial and endothelial cells
Human studies	↑apoptosis	Segura-Valdez (2000); Majo (2001)
	↓ VEGF, ↓ VEGF R2, ↓ VEGF KDR ↑ bax	Kasahara, Tuder, Cool (2000); Kasahara et al (2001)
	sFRP-1 gene expression	Yokohori (2004); Imai et al (2005)
	↑ bad	Imai and D’Armiento (2002)
	↑ Fas	Imai et al (2005)
	↑ p53	Hodge et al (2005)
	↑ activated caspases	Hodge et al (2005)
	↑ 4-HNE-modified proteins	Hodge et al (2005)Rahman et al (2002)
Animal and in vitro studies	VEGF R blockade → ↑ apoptosis injection of caspase 3 or Chariot → ↑ apoptosis	Kasahara, Tuder, Taraseviciene-Stewart, et al (2000); Tuder, Zhen, et al (2003)
	PIGF transgenic mice → ↑ apoptosis, ↓ VEGF	Aoshiba et al (2003)
	↓ ingestion of apoptotic cells by macrophages	Tsao et al (2004)Hodge, Hodge, Scicchitano, et al (2003)
Neutrophils
Human and animal studies	No difference in PBN apoptosis in stable COPD	Pletz et al (2004); Noguera et al (2004)
	↓ PBN apoptosis in acute exacerbations	Pletz et al (2004)
	↑ Mac-1, ↓ L-selectin of PBN	Noguera et al (2004)
	apoptosis of BALF granulocytes (horses)	Turlej et al (2001)
Lymphocytes
Human studies	↑apoptosis, ↑Fas, ↑TNF-a, ↑TNFR1, ↓bcl2 in PBT	Hodge, Hodge, Reynolds, et al (2003); Hodge et al (2005)
	↑ apoptosis, ↑p53, ↑ activated caspases in BALFT	Hodge et al (2005)
Skeletal myocytes
Human studies	No difference in apoptosis between COPD-controls	Gosker et al (2003)
	↓ apoptosis in COPD with low BMI	Agusti et al (2002)
Soluble apoptotic markers
Human studies	↑ plasma sFas in severe COPD	Yasuda et al (1998)
	No difference in plasma sFasL	Yasuda et al (1998); Takabatake et al (2000)

Abbreviations: BALF, bronchoalveolar lavage fluid; BALFT, BALF T-cells; BMI, body mass index; sFRP-1, frizzled-related protein; 4-HNE, 4-Hydroxy-2-nonenal; KDR, kinase insert domain-containing receptor; PBN, peripheral blood neutrophils; PBT, peripheral blood T-cells; PIGF, placenta growth factor; R, receptor; sFas, soluble Fas receptor; sFasL; soluble Fas ligand; TNF-α, tumor necrosis factor-α; VEGF, vascular endothelial growth factor.

Apoptosis

Apoptosis, “normal” or “programmed” cell death, is an evolutionarily conserved, innate process by which cells systematically inactivate, disassemble, and degrade their own structural and functional components. The term “apoptosis” was first introduced by Kerr et al in 1972 (Kerr et al 1972). It is a key mechanism allowing multicellular animals to tightly regulate cell growth (Baetu and Hiscott 2002). Necrosis, “accidental” cell death, is a pathological process which occurs when cells are exposed to a serious physical or chemical insult. During necrosis loss of membrane integrity leads to the influx of water and extracellular ions. Intracellular organelles, most notably the mitochondria, and the entire cell swell and rupture and the cytoplasmic contents are released into the extracellular fluid. During apoptosis coordinated morphological and biochemical changes occur within the nucleus, cytoplasm, organelles, and plasma membrane (Cohen 1993). Chromatin condenses and aggregates along the nuclear periphery and fragmentation of the nucleus occurs into chromatin containing fragments. Other cytoplasmic organelles remain structurally intact, although pore formation in the mitochondrial membrane is associated with apoptosis. The cell rounds up, dissociates itself from its neighbors, and shrinks, throwing out protuberances that separate into membrane-bound “apoptotic bodies”, containing cytoplasmic organelles and nuclear material. Within tissues apoptotic bodies are rapidly phagocytosed by neighboring cells (Cohen 1993).

Apoptosis can be triggered through two major pathways, one implicating death receptor ligation and the other the release of cytochrome c from mitochondria (Baetu and Hiscott 2002) (Table 2). The death receptor pathway is initiated by the ligation of members of the tumor necrosis factor (TNF) family, such as TNF-α and Fasligand, to their respective ligands, TNF receptor 1, and Fas (Baetu and Hiscott 2002). These “death-inducing” receptors recruit the death-inducing signaling complex through interaction with adaptor proteins such as Fas associated death domain protein (FADD). In turn, FADD recruits caspase-8. Caspase-8 activation leads to either direct activation of caspase-3, or to cleaving of Bid, a member of the bcl-2 family, which in turn targets mitochondria for cytochrome c release (Baetu and Hiscott 2002). The mitochondrial pathway can be triggered by both external and internal stimuli. Members of the bcl-2 family of proteins, like bcl-2, bax, and bad, gather at the surface of mitochondria, where they compete to regulate cytochrome c release, which leads to caspase-9 activation. Bcl-2 is an antiapoptotic and bad and bax are proapoptotic members of this family (Baetu and Hiscott 2002). Akt is a serine–threonine kinase that phospholylates and thereby inactivates the proapoptotic proteins bad and caspase 9, and elevates the expression of the antiapoptotic protein bcl-2 (Datta et al 1999). Both pathways converge at the level of caspase-3 activation. Caspases are proteolytic enzymes, the executioners of apoptosis. Caspase activation results in DNA laddering, characteristic of apoptotic cells, and to the cleavage of cytoskeletal proteins. p53 is a critical mediator of two different cellular responses following exposure to DNA damage: growth arrest in the G1 phase of the cell cycle or apoptosis in the case of irreparable damage (Canman and Kastan 1997). 4-Hydroxy-2-nonenal (4-HNE) is an end-product of lipid peroxidation, which is involved in provoking the toxic effects of oxidative stress to cells, promoting apoptosis (Rabacchi et al 2004). The frizzled-related protein sFRP-1 plays a part in the disruption of the normal Wnt signaling status and may also promote the apoptotic process (Jones and Jomary 2002).

Table 2

Markers upregulating (↑) or downregulating (↓) apoptosis in COPD

Apoptotic markers	Apoptosis
bcl-2	↓
bax	↑
bad	↑
Akt	↓
TNF-α	↑
Fas–Fas ligand	↑
p53	↑
4-Hydroxy-2-nonenal	↑
sFRP-1	↑

Abbreviations: sFRP-1, frizzled-related protein; TNF-α, tumor necrosis factor-α.

A number of methods are used for the detection of apoptosis. These assays try to measure one of the following apoptotic parameters: a) DNA fragmentation (eg, TdT-mediated dUTP nick end labeling, TUNEL); b) membrane alterations, such as phosphatidylserine translocation (eg, annexinV-propidium iodide staining); c) activation of caspases (eg, anti-active caspase 3 antibody); and d) detection of proteolytic cleavage products found in apoptotic cells (eg, anti-poly-ADP-ribose polymerase antibody, anti-fractin antibody). Apoptotic cells are also recognized by electron microscopy due to the characteristic morphological changes. Moreover, the expression of a number of genes and proteins involved in the regulation of apoptosis can also be studied by reverse transcription polymerase chain reaction (RT-PCR) or immunohistochemistry.

Apoptosis of epithelial and endothelial cells

Recently many reports have been published highlighting the presence of apoptosis in human COPD lungs and its role in the pathogenesis of emphysema (Shapiro 2000b). Pulmonary emphysema, defined as abnormal, permanent enlargement of airspaces distal to terminal bronchioles, accompanied by destruction of their walls, with or without obvious fibrosis, is a major component of COPD (Snider et al 1985). On the other hand, relatively little attention has been paid to the significance of epithelial or endothelial apoptosis in chronic bronchitis.

Animal and in vitro studies

The importance of apoptosis in the pathogenesis of emphysema stems from animal studies. Kasahara, Tuder, Taraseviciene-Stewart, et al (2000) suggested that chronic blockade of vascular endothelial growth factor (VEGF) receptors induces alveolar cell apoptosis and emphysema. Indeed, treatment of rats with a VEGF receptor blocker induced alveolar septal cell apoptosis, a pruning of the pulmonary arterial tree and enlargement of the air spaces, indicative of emphysema. Treatment with a caspase inhibitor prevented the septal cell apoptosis and emphysema caused by the VEGF receptor inhibitor. Aoshiba et al (2003) described the induction of emphysematous changes, including airspace enlargement, alveolar wall cell apoptosis (mainly epithelial cells), in mice treated with an intratracheal injection of active caspase-3 and Chariot, a protein transfection reagent, or nodularin, a proapoptotic serine–threonine kinase inhibitor. In addition, epithelial apoptosis and enhanced elastolytic activity were noted in bronchoalveolar lavage (BAL). In vitro findings showed the destruction of the elastin layer beneath the type II cells that were undergoing apoptosis. In both of these studies, fibrosis or increased infiltration of inflammatory cells was absent. Oxidative stress has been shown to have a critical role in alveolar septal cell apoptosis and emphysema caused by VEGF receptor blockade (Tuder, Zhen, et al 2003). Rats treated with a VEGF receptor blocker showed increased alveolar septal cell apoptosis, airspace enlargement, and expression of markers of oxidative stress, all of which were prevented by a superoxide dismutase mimetic. Apoptosis predominated in areas of oxidative stress, and treatment with a broad-spectrum caspase inhibitor markedly reduced the expression of markers of oxidative stress. In lungs treated with both the VEGF receptor blocker and the superoxide dismutase mimetic, the preservation of lung structure was associated with enhanced phosphorylation of the prosurvival and antiapoptotic Akt. Moreover it has been reported that i.v. injection of alpha-1 antitrypsin prevents VEGF receptor blockade-induced emphysema in rats (Choe et al 2003). Increased alveolar septal cell apoptosis and pulmonary emphysema, with enlarged air spaces and enhanced pulmonary compliance, were also noted in placenta growth factor (PIGF)–transgenic mice, with constitutive overexpression of PIGF (Tsao et al 2004). PIGF is a VEGF homolog, which may function by modulating VEGF activity or by triggering its own intracellular signals, involving proliferation, apoptosis, or angiogenesis (Cao et al 1996; Autiero et al 2003). In these mice, apoptotic septal cells were type II pneumocytes. At the same time, the messenger RNA of VEGF and platelet–endothelial cell adhesion molecule-1, an endothelial cell marker, were downregulated indicating a reduced number of endothelial cells and their survival factor VEGF. An inflammatory or fibrotic response was absent in these mice. In addition to an absolute increase in proapoptotic mechanisms, Hodge, Hodge, Scicchitano, et al (2003) suggested that impaired capacity for phagocytic clearance of apoptotic material may be a factor further contributing to emphysema pathogenesis. When incubating apoptotic airway epithelial cells with alveolar macrophages from BAL from COPD patients and control subjects, a significantly reduced proportion of alveolar macrophages from COPD subjects ingested apoptotic airway epithelial cells compared with controls.

Human studies

Segura-Valdez et al (2000) were the first to show increased apoptosis in the lungs of COPD patients. In their study, endothelial cells from capillaries and arterioles, and occasionally alveolar epithelial, interstitial, and inflammatory cells, exhibited prominent intranuclear staining by in situ end labeling of fragmented DNA. In a report by Kasahara et al (2001), there was increased apoptosis of alveolar epithelial and endothelial cells in lung tissue samples obtained from patients with emphysema compared with lung samples from either nonsmokers or smokers without emphysema. Moreover, VEGF, VEGF receptor 2 (VEGF R2) protein, and mRNA expression were significantly reduced in emphysema (Kasahara et al 2001). The authors proposed that epithelial and endothelial alveolar septal death due to a decrease of endothelial cell maintenance factors may be part of the pathogenesis of emphysema. It must be noted that in this study the septal structures in the emphysematous areas examined for the presence of apoptotic cells did not show clear signs of acute or chronic inflammation. The same group has reported significantly reduced expression of the VEGF receptor, kinase insert domain-containing receptor (KDR), in emphysematous lungs (Kasahara, Tuder, Cool, et al 2000). Yokohori et al (2004) also found that the fraction of the total alveolar wall cells undergoing apoptosis and proliferation was significantly higher in patients with emphysema than in asymptomatic smokers and nonsmokers. Patients with emphysema also showed a significant increase in the bax index, suggesting that the overexpression of bax protein may be involved in the apoptosis of the alveolar wall cells in these patients. Most of the apoptotic cells in this study were epithelial type-II cells. A study on tissue from the emphysematous lung areas of human patients by Imai et al (2005) showed that the apoptotic index was closely correlated with the severity of disease. They have also identified the expression of the frizzled-related protein sFRP-1 gene, an inducer of apoptosis, in emphysema. In a recent study, Imai et al (2005) identified extensive cell death by apoptosis, confirmed with several different techniques, in the lung tissue of patients with emphysema. Apoptosis was inversely correlated with surface area. Bcl-2 expression was not detected in emphysematous lung, whereas bax and bad expression was. Bax staining was localized to alveolar epithelial cells and bad staining to both epithelial and mesenchymal cells (Imai et al 2005). Rahman et al (2002) investigated the presence of 4-HNE, a highly reactive diffusible product of lipid peroxidation which mediates oxidant-induced cell signaling and apoptosis, in lung tissue from subjects with and without COPD. The 4-HNE-modified protein levels were elevated in airway and alveolar epithelial cells, endothelial cells, and neutrophils in COPD patients, compared with those in subjects without COPD. Moreover, there was a significant inverse correlation between the levels of 4-HNE adducts in alveolar epithelium, airway endothelium, and neutrophils, and FEV1. TNF-α is also considered to play an important role in the induction of apoptosis, and allele 2 of the polymorphism at position −308 in the promoter of the TNF-α gene has been associated with increased TNF-α secretion in vitro (Sakao et al 2002). Sakao et al (2002) reported that the TNF-α-308*1/2 allele frequency was higher, though not significantly, in COPD patients with more extensive emphysema changes, as assessed by computed tomography (CT). Majo et al (2001) investigated the presence of apoptotic alveolar epithelial cells in the lung, as indirect evidence of T-cell-mediated cytotoxicity, through the cytolytic effect of CD8 + cells by perforin-mediated lysis and apoptosis (Chrysofakis et al 2004). It was found that apoptosis of alveolar wall cells in active smokers with emphysema increased together with the amount smoked and the number of CD8 + T-cells after a certain dose of smoking was reached, suggesting that cytotoxicity may play a role in the pathogenesis of emphysema (Majo et al 2001). Recently, in a study by Hodge et al (2005) using flow cytometric assays on cell populations obtained from bronchial brushing, both the percentage and absolute number of apoptotic bronchial epithelial cells was significantly higher for patients with COPD than controls. They also noted increased expression of Fas, p53, and activated caspases by brushing-derived bronchial epithelial cells in COPD (Hodge et al 2005). Most of the above studies, however, were performed in lung tissue, whereas apoptotic cells lose their attachments with surrounding matrix and might therefore accumulate in airway lumen. Future studies, combining tissue and cytological (induced sputum and BAL) samples could reveal increased number of detached apoptotic cells.

Pathophysiologic implications

The above studies suggest that apoptosis plays a significant role in emphysema development. The lung is unique because of its exposure to the external environment and high oxygen tension (Tuder, Petrache, et al 2003). Many factors associated with COPD are potential causes of apoptosis of alveolar epithelial cells (Hodge, Hodge, Scicchitano, et al 2003). These include the 5000-plus chemical compounds and free radical molecules present in cigarette smoke, increased production of cytokines, neutrophil activity, and disruptions of epithelial cell–matrix interactions (Hodge, Hodge, Scicchitano, et al 2003; Tuder, Petrache, et al 2003). It is possible that lung cell apoptosis, excessive proteolysis, and oxidative stress interact, leading to the destruction seen in emphysema (Tuder, Petrache, et al 2003) (Figure 1). Increased apoptosis of the epithelial cells, which are the main sites of VEGF production, may account for decreased VEGF expression. Gerber, Dixit, et al (1998) and Gerber, McMurtrey, et al (1998) reported that VEGF induces the expression of anti-apoptotic proteins and Alon et al (1995) that VEGF acts as a survival factor for endothelial cells. If the amount of VEGF is sufficiently reduced and the signal transduction via VEGF R2 is impaired, then alveolar endothelial cells could die as a consequence of a failing VEGF-dependent endothelial cell maintenance program. The compromised microcirculation resulting from endothelial cell damage may further promote pneumocyte cell death, perpetuating a vicious circle (Tsao et al 2004). However, it is still unclear whether pneumocytes and endothelial cells use this kind of cell communication. Furthermore, the presence of elevated markers of oxidative stress in smokers’ lung is well documented, especially during exacerbations (Tsoumakidou et al 2005). Apoptotic death due to growth factor withdrawal is mediated by oxidative stress (Tuder, Zhen, et al 2003). The findings of Tuder, Zhen, et al (2003), that apoptosis predominated in areas of oxidative stress, and that apoptosis blockade by a broad-spectrum caspase inhibitor markedly reduced the expression of markers of oxidative stress, suggest that there is a bidirectional relationship and a positive feedback loop between lung alveolar cell apoptosis and oxidative stress (Tuder, Zhen, et al 2003). Aoshiba et al (2003) provided evidence of detection of increased elastolytic activity in apoptotic lung epithelial cells, which may amplify the destruction of alveolar elastin. The subsequent destruction of the basement membrane and loss of cell–extracellular matrix attachments may lead to further apoptosis of the surrounding cells. This dynamic feedback mechanism could play a pivotal role in the regulation of local tissue proteolysis (Tuder, Petrache, et al 2003). Finally, the damaging effects of apoptosis could be amplified by reduced clearance of these cells and persistence of apoptotic cell products, as suggested by Hodge, Hodge, Scicchitano et al (2003). Proteases derived from the inflammatory reaction present in COPD can hinder apoptotic cell recognition and proper uptake (Vandivier et al 2002; Tuder, Petrache, et al 2003). Although cigarette smoking has been shown to induce apoptosis of bronchial epithelial cells in vitro, in a study by Hodge et al (2005) cessation of smoking did not reduce the increased percentage of apoptotic cells in COPD. The increased apoptosis that persists after smoking cessation suggests that this might be a reflection of ongoing abnormalities remaining after smoking cessation, once COPD has been established.

Figure 1

Lung epithelial cell apoptosis. Increased apoptosis of epithelial cells may account for the decreased vascular endothelial growth factor (VEGF) expression, resulting in alveolar endothelial cells death. The compromised microcirculation resulting from endothelial cell damage may further promote pneumocyte cell death. Increased elastolytic activity in apoptotic lung epithelial cells amplifies the destruction of alveolar elastin. The subsequent destruction of the basement membrane and the loss of cell–extracellular matrix attachments lead to further apoptosis of the surrounding cells.

Abbreviations: BM, basement membrane; ECM, extracellular matrix.

Animal studies have proposed a model of emphysema related to increased apoptosis that excludes inflammation. Animal models, however, do not imitate human diseases and gross lung structure differences in the airways limit extrapolation of findings from animals to humans, eg, smoking mice are not coughing up sputum (Shapiro 2000a). Most human studies on epithelial–endothelial cell apoptosis also focus on emphysema. Taking into account that chronic bronchitis and emphysema overlap in COPD and that patients included in human studies had no a1-antitrypsin deficiency, it is difficult to ignore the chronic bronchitis component, although not clearly mentioned in those studies, and the possible implication of inflammation in emphysema. Further studies on COPD including chronic bronchitis are needed to examine the contribution of inflammation and apoptosis in the peripheral airways disease.

Neutrophil apoptosis in COPD

An abnormal inflammatory response, and particularly the persistent presence in tissue of granulocytes and other leukocytes that represent the cellular elements of inflammation, is considered a central process in the pathogenesis of COPD (Haslett 1999). Neutrophil accumulation in the lungs is a characteristic feature of COPD (Jeffery 1998; Saetta 1999; Cosio Piqueras and Cosio 2001). This could be explained by two mechanisms: 1) increased neutrophil recruitment and chemotaxis, and 2) delayed tissue clearance, due either to delayed apoptosis or defective clearance of these cells. Apoptosis provides an injury-limiting neutrophil clearance mechanism and promotes resolution, rather than persistence, of inflammation (Haslett 1999). The dysregulation of neutrophil apoptosis in the lungs of COPD patients has not been extensively studied.

Human and animal studies

Pletz et al (2004) assessed the apoptosis of peripheral blood neutrophils in COPD patients during acute exacerbation and found reduced apoptosis of neutrophils in hospitalized patients with an acute exacerbation of COPD. The apoptosis rate increased progressively during the recovery. The apoptosis rates in healthy volunteers were significantly higher than in COPD subjects at admission, but there was no significant difference in apoptosis rate between controls and COPD patients at discharge (Pletz et al 2004). Noguera et al (2004) found that peripheral blood neutrophil apoptosis in stable COPD patients occurred at a rate similar to that found in healthy individuals and smokers with normal lung function. Qualitatively, however, there was increased surface expression of Mac-1 and decreased surface expression of L-selectin in the apoptotic neutrophils of COPD patients (Noguera et al 2004). Using flow cytometric techniques, there was a nonsignificant trend for reduced apoptosis of neutrophils in COPD (Hodge et al 2005). In a study by Turlej et al (2001), broncoalveolar lavage fluid (BALF) granulocytes from heaves-affected horses demonstrated a significant delay in apoptosis compared with blood granulocytes from the same horses and blood and BALF granulocytes from healthy horses (Turlej et al 2001). Heaves is considered to be an animal model for COPD (Raulo et al 2001). The rate of apoptosis in blood granulocytes from healthy and heaves-affected horses was similar. The enhanced survival of BALF granulocytes from sick horses was suppressed in the presence of anti-GM-CSF receptor antibodies.

Apoptosis is an important mechanism controlling functional longevity of neutrophils at inflamed sites (Haslett 1999). During apoptosis the neutrophil surface membrane remains intact and neutrophils lose the ability to degranulate on deliberate external stimulation. Macrophages can clear large number of apoptotic neutrophils without leakage of potential injurious neutrophil contents into the surrounding milieu (Haslett 1999). The uptake of apoptotic neutrophils may not only suppress the release of proinflammatory agents, such as interleukin (IL)-1β, GM-CSF, IL-8, and TNF, but increase macrophage release of agents, such as transforming growth factor β (TGF-β), and prostaglandin E2, that have suppressive influences on the inflammatory response (Fadok et al 1998; Haslett 1999). It has been demonstrated in vitro that nicotine prolongs neutrophil survival in a dose-dependent manner by suppressing apoptosis (Aoshiba et al 1996). Several inflammatory agents known to be elevated in COPD, such as lipopolysaccharide (LPS) and GM-CSF, or hypoxic conditions inhibit neutrophil apoptosis. Thus, any reduction in neutrophil apoptosis or dysregulation of macrophage uptake of apoptotic neutrophils could lead to chronic inflammation and tissue injury, such as that observed in COPD. The observation by Noguera et al (2004) of higher surface expression of Mac-1 and lower expression of L-selectin in apoptotic neutrophils of COPD patients compared with controls is compatible with a higher activation status during the apoptosis process. This suggests that neutrophils may still contribute to tissue damage in COPD patients even during apoptosis (Noguera et al 2004). Moreover, increased surface expression of Mac-1 may alter the ability of macrophage recognition and removal of apoptotic neutrophils (Noguera et al 2004).

A significant limitation of the studies by Pletz et al (2004) and Noguera et al (2004) is that they studied neutrophil apoptosis in vitro and in circulating, not lung-derived, cells. Peripheral blood neutrophils are expected to exhibit different apoptotic behavior than the cells exposed to the complex inflammatory processes of the COPD lung, and in vivo neutrophils are under the dynamic influence of several pro-and anti-apoptotic factors simultaneously. The above-mentioned studies do not provide enough evidence to rule out delayed neutrophil apoptosis as a cause of neutrophil accumulation and chronic inflammation in COPD lungs.

Lymphocyte apoptosis in COPD

Studies quantifying the inflammation of the airways in smokers and defining their phenotype found that the predominant inflammatory cell present was the CD8 + T-cell and that their number correlated inversely with the degree of airflow limitation (Saetta etal 1993; Jeffery 1998; Hodge, Hodge, Reynolds, et al 2003; Hogg et al 2004; Chrysofakis et al 2004; Tsoumakidou et al 2004). These findings suggest an important role for activated T-cells in the pathogenesis of airway abnormalities in COPD. A possible mechanism in order to prevent permanent damage and remodeling in COPD could be removal of excess inflammatory cells, including T-cells, by apoptosis, as has been suggested in other disease models (Ponomarev and Dittel 2005).

Hodge, Hodge, Reynolds, et al (2003) assessed apoptosis of T lymphocytes isolated from peripheral blood in COPD patients, and found significantly increased apoptosis of stimulated T-cells, CD4, and CD8, compared with controls. There was no significant difference in levels of apoptosis between CD4 and CD8 T-cell subsets in COPD patients. An upregulation of Fas, TNF-α, TNF receptor 1, and TGF receptor (TGFR) was also observed. Monocyte production of TGF-β and release of active TGF-β in the peripheral blood were increased. There was a decrease in anti-apoptotic bcl2 and IL-7R expression in the peripheral blood T-cells in COPD (Hodge et al 2005). The authors concluded that the increased T-cell death may be associated with both an increase in pro-apoptotic and a decrease in anti-apoptotic mediators in the peripheral blood in COPD. The same group investigated apoptosis of lung-derived T-cells (Hodge et al 2005). They found an increased percentage and absolute number of apoptotic BAL-derived T-cells in COPD. In addition, there was no significant change in the percentage of T-cells expressing bcl2 or bax, although p53 expression and activated caspases by BAL-derived CD3 + T-cells were significantly increased in COPD (Hodge et al 2005).

Several observations can be made based on the findings by Hodge, Hodge, Reynolds, et al (2003). The increased numbers of T-cells in COPD lungs may result from local proliferation of T-cells in the lung or enhanced trafficking from the bloodstream. This trafficking also occurs from the airways to the bloodstream. Therefore, the authors think that it is possible that increased apoptosis of T-cells in the peripheral blood in COPD may result either from local apoptotic stimuli in the airways or from apoptotic stimuli in the peripheral blood (Hodge, Hodge, Reynolds, et al 2003; Hodge et al 2005). Increased numbers of apoptotic T-cells in the lung, if not effectively cleared, may lead to secondary necrosis, which has a pro-inflammatory effect. Furthermore, the increased secretion of TGF-β by monocytes may be attributed to ingestion of increased numbers of apoptotic cells (Fadok et al 1998). Increased rates of T-cell apoptosis may lead to a defective immune response to infective organisms, contributing to the high frequency of infections seen in COPD (Hodge et al 2005).

The decrease in the CD4/CD8 ratio seen in COPD cannot be explained by a preferential increase in the apoptosis of CD4 cells. Recent studies in mice showed that cigarette smoke exposure specifically prevented the expansion and maximal activation of CD4 T-cells and reduced the number of both activated CD4 and CD8 T-cells. Consequently, smoke exposure decreased the activated CD4:CD8 T-cell ratio from 3 to 1.5 (Robbins et al 2004). The mutagenic effect of cigarette smoke on “susceptible” smokers could predispose dendritic cells to production of cytotoxic CD8 + cells, which in turn induce epithelial cell death and apoptosis by perforin (Chrysofakis et al 2004; Tzanakis et al 2004) (Figure 2).

Figure 2

Oxidative stress of cigarette smoke in “susceptible” smokers activates adaptive immunity, predisposing dendritic cells to clonal expansion of CD4 + and especially of cytotoxic CD8 + cells, inducing epithelial cell death by perforin.

In conclusion, the observation of increased peripheral blood and BAL T lymphocyte apoptosis is not sufficient to establish a causal relationship with the pathogenesis of COPD. Further studies investigating the apoptotic pathways in lymphocyte subsets in both airways (induced sputum) and peripheral blood in COPD are needed in order to draw safe conclusions.

Skeletal muscle wastage and apoptosis in COPD

COPD is considered to be a complex lung disease with systemic consequences, involving several organs (Oudijk et al 2003). Unexplained weight loss and peripheral muscle weakness is a major problem for patients with COPD, seriously affecting their quality of life. Whereas apoptosis in mononucleated cells leads to cell death, in multinucleated cells, like the myocyte, it causes cell atrophy (Allen et al 1997). Increased apoptosis of skeletal muscle could be responsible for the skeletal muscle atrophy, the main cause of unexplained weight loss in patients with COPD. Gosker et al (2003) reported absence of apoptosis of muscle fibers, at least not at a higher rate in stable COPD patients compared with controls (Gosker et al 2003). On the other hand, Agusti et al (2002) found that skeletal muscle apoptosis is increased in patients with COPD and low body mass index (BMI) compared with patients with COPD and normal BMI, healthy volunteers, and sedentary subjects undergoing orthopedic surgery. They also found that in patients with COPD, BMI is inversely related to skeletal muscle apoptosis and that this skeletal muscle apoptosis is associated with a lower exercise tolerance despite a similar degree of lung function impairment. A simple explanation for the different findings of these two studies is that COPD patients included in the study by Gosker et al were in a weight stable condition with a similar BMI to the control group. Increased skeletal muscle apoptosis could not be attributed to aging, inactivity, lung function impairment, smoking history, and oral steroids (Agusti et al 2002). Underweight patients with COPD were younger than those with normal BMI, they had similar lung function impairment (including arterial hypoxemia) and smoking history, and none had received oral steroids. Oxidative stress and systemic inflammation are both prominent features in COPD and have the potential to induce apoptosis (Boots et al 2003; Oudijk et al 2003). Moreover, mitochondria play a key role in apoptosis, and mitochondrial abnormalities have been reported in skeletal muscle in COPD. An increase in the activity of cytochrome oxidase (Sauleda et al 1998) and the presence of significant bioenergetic abnormalities (ATS-ERS 1999) have been demonstrated in skeletal muscle in COPD. A central cytokine in the loss of muscle mass could also be TNF-α by stimulating apoptosis via interaction with the TNF-α receptor present on the muscle cells (Oudijk et al 2003). The role of apoptosis in muscle wasting in COPD is an attractive concept that needs further investigation to confirm the presence of apoptosis in these cells and elucidate possible pathogenetic pathways.

Conclusion

Despite the now widely recognized harmful effects of tobacco, COPD remains a leading cause of morbidity and mortality worldwide. Apoptosis is a highly regulated process playing a protective role in physiologic conditions. The mechanisms controlling apoptosis act differently on different cell populations and different tissue settings. Dysregulation of apoptosis has been implicated in many lung diseases.

The reviewed studies indicate that apoptosis might play a significant role in COPD pathogenesis, together with oxidative stress, protease–antiprotease imbalance, and genetic susceptibility. COPD pathology deteriorates even after smoking cessation. This observation may be related to increased apoptosis in the airways of COPD patients even after smoking cessation. These studies provide evidence of activation of different apoptotic mechanisms in COPD compared with controls, which could also represent a protective reaction of the lung to deleterious stimuli. The link between apoptosis and COPD pathogenesis remains to be proven and extensive research, including also the chronic bronchitis component of COPD, is still needed in order to verify the above issues. Elucidating the pathogenetic mechanisms leading to this condition will help to develop new therapeutic strategies against this highly prevalent and often fatal disease.