Impact of sputum bacteria on airway inflammation and health status in clinical stable COPD

D. Banerjee, O.A. Khair, D. Honeybourne
European Respiratory Journal 2004 23: 685-691; DOI: 10.1183/09031936.04.00056804

Abstract

Chronic obstructive pulmonary disease (COPD) is characterised by sputum production, bacterial colonisation, neutrophilic bronchial airway inflammation and poor health status. The aim of this study was to determine the impact of sputum potentially pathogenic microorganisms (PPMs) on bronchial airway inflammation, health status and plasma fibrinogen levels in subjects with moderate-to-severe COPD during the clinical stable state.

Sputum total cell and neutrophil counts, supernatant interleukin‐8, leukotriene B4, tumour necrosis factor‐α and neutrophil elastase levels, neutrophil chemotaxis and plasma fibrinogen levels were estimated. Health status was determined using the St George's Respiratory Questionnaire and the 36‐item Short-Form Health Survey questionnaire.

Twenty-seven (40%) subjects had PPMs and 40 (60%) non‐PPMs in their sputum. Both groups were of similar age, body mass index, smoking history and lung function. The PPMs group showed significantly higher levels of interleukin‐8, leukotriene B4, tumour necrosis factor‐α, neutrophil elastase and increased neutrophil chemotaxis. They also exhibited worse health status and raised plasma fibrinogen levels compared to the non‐PPMs group.

In conclusion, subjects with clinically stable moderate-to-severe chronic obstructive pulmonary disease who had potentially pathogenic microorganisms in their sputum demonstrated an exaggerated airway inflammatory response, poorer health status and increased plasma fibrinogen levels than those who had nonpotentially pathogenic microorganisms.

The presence of bacteria in the lower bronchial airways of patients with stable chronic obstructive pulmonary disease (COPD) has been labelled as colonisation. There is ongoing debate as to whether bronchial inflammation in the presence of bacteria is truly colonisation. The presence of bacteria is abnormal as the lower respiratory tract, in the absence of lung disease, is normally sterile. Bronchoscopic techniques for the study of infections in COPD have confirmed that stable patients often carry bacteria in the lower respiratory tract, and multiple strains, such as nontypeable Haemophilus influenzae, Streptococcus pneumoniae and Moraxella catarrhalis, may be present 14.

A relationship between the intensity of sputum bacterial load and sputum inflammatory markers has been shown in stable patients with COPD 5. Another study using bronchoalveolar lavage (BAL) found that patients with potentially pathogenic microorganisms (PPMs) had more neutrophils in BAL samples compared to those who had non‐PPMs 6. These studies, therefore, provide evidence that patients with stable COPD who show bacterial colonisation may have a more intense inflammatory response. How an exaggerated inflammatory response, as a result of bronchial airway PPMs colonisation, in the clinical stable state leads to the worsening of health status remains unclear.

A number of studies in COPD have suggested the possibility of a hypercoagulable state, with increased abnormalities of haemostasis. Raised fibrinogen and d‐dimer levels have been reported in patients with COPD 7. Fibrinogen levels have also been shown to be raised in patients with exacerbations of COPD, and there is some evidence that this may be associated with interleukin (IL)‐6 production 8. The effect of sputum PPMs colonisation on plasma fibrinogen levels in stable patients with moderate-to-severe COPD remains uncertain. The aim of the present study was to determine whether patients with COPD harbouring PPMs in their sputum during the clinical stable state have different degrees of airway inflammation, health status and plasma fibrinogen level compared to those stable patients with non‐PPMs.

Materials and methods

Study subjects

An observational study was undertaken. Sixty-seven subjects with clinically stable moderate-to-severe COPD, in accordance with British Thoracic Society/Association of Respiratory Technicians and Physiologists guidelines 9, were recruited from City Hospital and Birmingham Heartlands Hospital (both Birmingham, UK) clinics and lung function units. All subjects had a forced expiratory volume in one second (FEV1)/forced vital capacity (FVC) ratio of <70%, an FEV1 of <60% of the predicted value and FEV1 reversibility of <200 mL or <15% (of baseline) to a β2‐agonist bronchodilator. Current smokers were regarded as those who had smoked regularly for ≥6 months before the recruitment date and exsmokers as those who had stopped smoking regularly for >6 months before recruitment. Subjects with a recent infective exacerbation within the last 6 weeks or a clinical history of asthma, bronchiectasis, lung cancer and uncontrolled ischaemic heart disease or diabetes mellitus were excluded. Based on observations that many moderate-to-severe patients in clinical practice are on inhaled corticosteroids and the growing evidence that withdrawal of these may have a detrimental effect on clinical state 10, 11, it was decided that only those subjects taking inhaled corticosteroids should be recruited. Informed consent was obtained from all subjects and the study was approved by the City Hospital and Birmingham Heartlands Hospital ethics committees.

Study design

The present observational study assessed the impact of PPMs in the sputum of subjects with clinically stable moderate-to-severe COPD on bronchial airway inflammation, health status and plasma fibrinogen levels compared to subjects with non‐PPMs.

Clinical measurements

Spirometry (FEV1, FVC and FEV1/FVC) was performed using a MIR Spirobank (Medical International Research, Rome, Italy; accuracy ±3%; flow range ±16 L·s−1). Reversibility of FEV1 was assessed by repeating spirometric tests 20 min after inhalation of salbutamol (400 µg), given through a volume spacer by a trained member of the lung function department. Static lung volumes were measured at the City Hospital lung function unit by body box and gas transfer using the single-breath carbon monoxide method (V6200 Autobox; Sensormedics, Bilthoven, the Netherlands). Health status was measured using the St George's Respiratory Questionnaire (SGRQ) for disease-specific assessment of symptoms, activity and impact. The 36‐item Short-Form Health Survey questionnaire (SF‐36) was also used as a general health measure, covering eight health concepts: physical functioning, social functioning, physical role limitation, emotional role limitation, mental health, pain index, vitality, and general health perception. Fibrinogen levels (Klauss method), plasma viscosity using a Beckman Coulter Viscometer (Beckman Coulter, Inc., Fullerton, CA, USA) and C‐reactive protein (CRP) levels were measured by the local hospital haematology and biochemistry departments respectively.

Airway inflammation markers

All subjects underwent hypertonic (3%) saline sputum induction using a DeVilbiss ultrasonic nebuliser (DeVilbiss, Somerset, PA, USA; output 2.2 mL·min−1) as described previously 12. All samples had a squamous cell count of <30% of total and were therefore regarded as being adequate for cellular assessment. A portion of this sample was separated at this stage and saved for bacteriological assessment. Sputum plugs were separated from contaminating saliva by macroscopic examination using a pair of disposable plastic forceps with the aid of a hand-held lens. Processing the sputum for inflammatory markers included the use of 0.1% dithiothreitol solution as a mucolytic agent. From the resulting cell pellet, the total cell count was determined with a Neubauer haemocytometer, using the trypan blue exclusion method to determine cell viability. The cell pellet was rediluted in phosphate-buffered saline (pH 7.4) to give a final concentration ∼1×106 cells·mL−1. Cytospin preparations were performed using a Cyto-tek centrifuge (Cyto-tek, Sakura-Finetek Europe, Zoeterwoude, the Netherlands). Cell suspension (75 µL) was placed in the chamber holder and centrifuged for 5 min at 28.2×g. An even spread of cell suspension on the slide was obtained. The slide was left to air dry for 1 h and then stained using May-Grünwald-Giemsa. Once dried, the slide was mounted with distyrene/plasticiser/xylene glue using a coverslip. In order to obtain a differential cell count, 400 cells were counted at a magnification of ×40 using a multiple counter device, and the percentages of neutrophils, macrophages, eosinophils and lymphocytes (i.e. excluding squamous and epithelial cells) were obtained.

The supernatant recovered from the sputum processing was decanted and stored at −70°C and later analysed for IL‐8, leukotriene (LT) B4, tumour necrosis factor‐α (TNF‐α) and neutrophil elastase (NE). IL‐8 and TNF‐α were measured by enzyme-linked immunosorbent assay (ELISA) using a commercially available kit (R&D Systems Europe, Abingdon, UK). LTB4 was also measured using a commercially available ELISA kit (Amersham International, Amersham, UK). NE activity was measured spectrophotometrically using the synthetic substrate N‐succinyl-Ala-Ala-Ala‐p‐nitroanilide as previously described by McGillivray et al. 13. The intra- and interassay coefficient of variation (CV) for these assays have previously been shown to be <10% 14. In the current study, the lower limits of detection were as follows: IL‐8 0.0125 nM; LTB4 0.137 nM; TNF‐α 0.1 pM; and NE 0.01 µM; all values below these limits were regarded as zero. The intra- and inter-assay CVs were: IL‐8 <9%; LTB4 <10%; TNF‐α <10 and <15% respectively; and NE <5%.

Neutrophil chemotaxis was assessed using modified techniques described previously by Falk et al. 15 and Harvath et al. 16. In brief, this technique required a 48‐well chamber unit (Neuro Probe® 48 Well Chemotaxis chamber; Neuro Probe, Inc., Cabin John, MD, USA) consisting of a top and bottom acrylic plate, a sealing silicone gasket and assembly hardware. The lower plate comprised 48 wells, each 25 µL in volume. Corresponding holes in the top plate formed the upper wells of 50 µL in volume. A single filter membrane sheet (polyvinylpyrrolidone-free Nucleopore® polycarbonate filter; Costar, High Wycombe, UK) containing 2‐µm pores was used to separate the two plates. Neutrophils were initially purified from peripheral blood by means of discontinuous Percoll density gradients using the method described by Jepsen and Skottun 17. The neutrophil chemotaxis assay was carried out in triplicate; 27.5 µL chemoattractant was pipetted into the lower chamber to obtain a meniscus and 50 µL neutrophils into the upper chamber, and the chamber unit incubated for 20 min at 37°C. The assay kit was disassembled and the membrane sheet carefully removed, air dried for 1 h and then stained using DiffQuik dyes (methanol fixative, eosin G and thiazine). Neutrophils were counted at a magnification of ×40. For each well (of the triplicate), cells wholly contained within five random half-pitch fields were counted and the mean taken. Neutrophil migration was expressed as a percentage of that in response to a positive control of 1×10−8 M N‐formyl-methionyl-leucyl-phenylalanine. The intra-assay CV was 8%.

Quantitative bacterial load assay

Quantitative bacterial culture measurements on the sputum were carried out as previously described by Pye et al. 18. All samples were processed for bacteriology within 4 h of expectoration. Viable bacterial numbers were expressed as the number of colony-forming units (cfu) per millilitre of original sputum. Bacterial pathogens recovered were classified as PPMs and nonpathogens as non‐PPMs, as previously described by Soler et al. 6. PPMs included respiratory bacterial pathogens, e.g. H. influenzae, S. pneumoniae, M. catarrhalis, H. parainfluenzae, Staphylococcus aureus, Pseudomonas aeruginosa and Klebsiella pneumoniae, and the following were regarded as non‐PPMs: Streptococcus viridans, Neisseria spp., Corynebacterium spp., Candida spp., Enterococcus spp., and coagulase-negative Staphylococcus. The impact of sputum PPMs and non‐PPMs on airway inflammation, health status and plasma fibrinogen levels were compared as groups rather than as individual bacterial species. Bacterial colonisation studies were performed by technical staff blind to the clinical characteristics of the subjects in the study.

Statistical analysis

In order to determine whether the distributions of all continuous data were normal, a Kolmogorov-Smirnov test was performed. In cases in which such an assumption could not be met for bacterial cfus and airway inflammatory cell counts, data were logarithmically transformed and presented as mean±sem. Nonparametric health status data are presented as median and interquartile range (IQR). Continuous variables with normal distributions were compared using the parametric unpaired two-independent-group t‐test, whereas those data not normally distributed were compared using the nonparametric Mann-Whitney U‐test. Correlations between parametric data were undertaken using Pearson's correlation and nonparametric data using Spearman's rank correlation. Two-tailed tests were used and the level of significance was taken as p<0.05.

Results

Twenty-seven (40%) subjects had PPMs in their sputum as opposed to 40 (60%) who had non‐PPMs. Fourteen (52%) and 13 (32%) subjects from the PPMs and non‐PPMs groups respectively were current smokers (p=0.47) The demographics of the PPMs and non‐PPMs groups are shown in table 1. There were no significant differences between the two groups with regard to age, body mass index, smoking history, lung function or C‐reactive protein levels.

View this table:
Table 1

Clinical demographic data for subjects with sputum potentially pathogenic microorganisms (PPMs) and non‐PPMs

Sputum bacteriology

There were a total of 38 bacterial isolates from the PPMs group. Ten subjects in this group yielded more than one bacterial isolate in their sputum. The PPM species isolated are shown in table 2. H. influenzae, M. catarrhalis and S. pneumoniae made up 91% of all bacterial isolates.

View this table:
Table 2

Potentially pathogenic microorganisms#

Sputum airway inflammatory mediators

Subjects with PPMs in their sputum exhibited higher neutrophil numbers (although this did not quite reach significance), a higher neutrophil differential, higher supernatant levels of IL‐8 (fig. 1a), LTB4 (fig. 1b), TNF‐α (fig. 1c) and NE (fig. 1d), and a more exaggerated neutrophil chemotactic response than those subjects who had non‐PPMs in their sputum. These results are summarised in table 3. Inflammatory parameters were logarithmically transformed for sputum total cell count and absolute neutrophil count. In the PPM group, correlation studies between log total cfus (i.e. bacterial load) for each subject sputum sample and sputum inflammatory markers revealed significant relationships for IL‐8 (r=0.51, p=0.007), LTB4 (r=0.49, p=0.01) and TNF‐α (r=0.57, p=0.002). No significant relationship existed between bacterial load and sputum neutrophil count or neutrophil chemotaxis.

Fig. 1.—
Fig. 1.—

Supernatant a) interleukin (IL)‐8, b) leukotriene (LT) B4, c) tumour necrosis factor‐α (TNF‐α) and d) neutrophil elastase (NE) in the potentially pathogenic microorganism (PPMs) and non‐PPMs groups. Horizontal bars indicate medians (……: lower limit of detection). #: p=0.006; : p=0.005; ***: p=0.001.

View this table:
Table 3

Comparison of sputum airway inflammatory parameters between subjects with potentially pathogenic microorganisms (PPMs) and non‐PPMs

Health status, fibrinogen level and plasma viscosity

Subjects with PPMs in their sputum demonstrated worse health status than subjects with non‐PPMs in the following scores: SGRQ total (p=0.004), SGRQ impact (p=0.005), SGRQ symptoms (p=0.03), SGRQ activity (p=0.004), SF‐36 vitality (p=0.02) and SF‐36 physical role limitation (p=0.03) (table 4). Bacterial load did not correlate with any health status parameter.

View this table:
Table 4

Comparison of health status scores and plasma fibrinogen levels and viscosity between subjects with potentially pathogenic microorganisms (PPMs) and non‐PPMs

There was no difference in plasma viscosity between the PPMs and non‐PPMs groups. Those with PPMs, however, showed a significantly increased level of plasma fibrinogen (p=0.05) (table 4). There was no significant correlation between bacterial load and plasma fibrinogen levels in the PPMs group.

Discussion

The present study has shown that subjects with moderate-to-severe COPD who have PPMs in their sputum have an exaggerated airway inflammatory response, worse health status and higher levels of plasma fibrinogen compared to subjects who have non‐PPMs in their sputum, even in the clinical stable state.

The precise role of bacteria in COPD has been a source of controversy for many years. The current study found that 40% of subjects had PPMs in their sputum, and the commonest microorganisms isolated were H. influenzae, M. catarrhalis and S. pneumoniae. This compares favourably with previous findings 2, 6, 19. There were four Gram-negative isolates from three subjects in the current study: K. pneumoniae, P. aeruginosa, a coliform and Acinetobacter baumannii. These three subjects had an FEV1 of 33–41% pred. A previous study suggested that exacerbations in patients with COPD at the severe end of the spectrum (as assessed by FEV1 as a percentage of the predicted value) are more likely to be caused by such Gram-negative organisms 20. There was no relation, however, between pulmonary lung function and sputum PPMs colony-forming unit numbers in the present study.

Subjects who had non‐PPMs (such as S. viridans, Neisseria spp., Corynebacterium spp. and coagulase-negative Staphylococcus) in their sputum interestingly showed an inflammatory response, although levels of supernatant cytokines were lower than in those subjects with PPMs. There were fewer neutrophils in the sputum of subjects with non‐PPMs, but this did not quite reach significance. The perception of what is pathogenic can change. For example, M. catarrhalis was not regarded as a pathogen for many years and there is little information about the propensity of different non‐PPMs species to stimulate bronchial inflammation 21. In the current work, differentiation between non‐PPMs species and their relationship to airway inflammation and health status was not carried out; instead they were analysed as a group. It may also be possible that certain subjects with non‐PPMs had negative sputum cultures to PPMs which could have been detected by other methods, e.g. bronchoalveolar lavage (BAL). Sputum culture has been shown to be a reliable method of obtaining microbiological data 22. However, the present study seems to suggest that a chronic inflammatory response in moderate-to-severe COPD is present despite the absence of PPMs in the sputum. Indeed, Hill et al. 5 have shown that non‐PPMs generate similar levels of IL‐8 to 1×105 cfu·mL−1 PPMs in subjects with COPD.

In the current research, subjects with PPMs had worse health status scores than those with non‐PPMs. There was a significant difference between the two groups in all SGRQ components (p‐value 0.005–0.03) and SF‐36 physical role limitation and vitality (p=0.03 and 0.02 respectively). There was, however, no numerical difference between the SF‐36 physical role limitation medians and hence its biological significance is doubtful. The mean differences in SGRQ score ranged 9.9–13.6, illustrating that the differences were greater than the 4 scale points that are regarded as clinically meaningful. These particular data have not been shown before in the literature and illustrate that the presence of bacteria in sputum, even when subjects are in the clinical stable state, has a significant impact on health status.

The mechanism of this difference in health status cannot be explained solely on the basis of differences in lung function as both groups in this study were similar in this respect. However, it is possible that bacteria cause a worse health status by inducing an exaggerated inflammatory response. This was demonstrated by the current data in that there were more sputum neutrophils in those with PPMs (although this did not quite reach significant levels (p=0.058)) and also significantly higher levels of supernatant IL‐8, LTB4, TNF‐α, NE and neutrophil chemotaxis than in those with non‐PPMs. There is also some evidence from Angrill et al. 23 that patients with bronchiectasis colonised by such non‐PPMs exhibit a reduced inflammatory response in terms of reduced absolute neutrophil counts and IL‐8, IL‐6, TNF‐α and NE levels. Neutrophils in sputum may lead to activation of other inflammatory cells in the lung, leading to the release of systemic pro-inflammatory proteins/cytokines, which eventually lead to systemic ill-health, e.g. skeletal muscle dysfunction, abnormal nutrition and metabolism, etc., which would impact on symptoms. It may be argued that the presence of neutrophils in the sputum is a normal response to the original bacterial insult to the bronchial airways. In the present study, no difference was seen in the levels of CRP between both groups and mean levels were within the normal range. This indicates that there was probably no acute systemic clinical state present in the two groups, although a bronchial inflammatory response was detectable from sputum measurements. These results may reflect the “compartmentalised” nature of COPD airway inflammation in those subjects who are in the clinical stable state.

It is possible that the subjects in the PPMs group represent “frequent exacerbators” (as opposed to “infrequent exacerbators”). Subjects with frequent exacerbations have worse health status 24 and increased levels of sputum IL‐6 and IL‐8 compared to those subjects with infrequent exacerbations 25. Moreover, patients with frequent exacerbations also demonstrate a faster decline in FEV1 than infrequent exacerbators, with exacerbations contributing to ∼25% of the observed lung function decline in subjects with COPD 26. More recently, it has been demonstrated that there is a significant relationship between sputum bacterial load and disease progression in subjects with COPD, showing that the rate of decline in FEV1 is proportional to the rise in colonising bacterial load 27.

The exacerbation rate during the preceding year in subjects in the current study was determined by their recalling the number of times their symptoms worsened and resulted in a visit to their primary care physician for antibiotics and oral corticosteroids. Recall accuracy may be questioned as there was no objective evidence of symptoms in this preceding year, e.g. diary cards. In the present study, however, subjects with PPMs reported a higher median exacerbation rate (median 2, IQR 1–2) compared to subjects with non‐PPMs (median 1, IQR 0–2), although this just failed to achieve significance (p=0.09).

If the frequency of exacerbations between the PPMs and non‐PPMs groups in the current study is truly not different, it is possible that what determines inflammation and health status at any particular point in time is not the number of exacerbations in the preceding year but the current qualitative and quantitative PPMs colonisation state.

The interactions between inhaled corticosteroids, airway inflammation and infective exacerbations remain complex and have yet to be fully evaluated. The influence of inhaled corticosteroids on morbidity and mortality has been debated elsewhere 28, and previous studies assessing the effect of inhaled corticosteroids on airway inflammation have been mixed 2932. A more recent study, however, has shown that inhaled corticosteroids may attenuate the secretion of IL‐8 and IL‐6 from cultured bronchial epithelial cells when stimulated by TNF‐α 33. In the current study, all patients recruited were taking inhaled corticosteroids. The impact of inhaled corticosteroid therapy on airway inflammation generated by bacterial colonisation is unclear. Further sequential studies investigating the impact of bronchial airway colonisation on airway inflammatory markers, health status and FEV1 decline in patients receiving or not receiving inhaled corticosteroid therapy during the clinical stable state may be necessary.

The present study also found increased levels of plasma fibrinogen in subjects with PPMs compared to those with non‐PPMs. Raised fibrinogen levels have been found in stable patients and increase during an acute exacerbation 8. This increment in fibrinogen level was similar to the difference in level between the two groups in this current study, even during the stable state. The cohort of subjects in this previous study was also similar to the current study with regard to spirometric results. The exact mechanism of fibrinogen level increase in COPD is unclear, but it is hypothesised that it may be mediated through IL‐6 8. It is possible that airway bacterial colonisation leads to enhanced release of IL‐6, causing raised fibrinogen levels. Increased fibrinogen levels in the stable state, which theoretically translate into a prothrombotic state, raises the question of long-term anticoagulation in susceptible patients.

In summary, the current study showed that those subjects with potentially pathogenic microorganisms in their sputum exhibited a higher level of airway inflammation, poorer health status and increased levels of plasma fibrinogen than subjects with nonpotentially pathogenic microorganisms during the clinical stable state. Further studies are needed to explain the interactions between bacterial colonisation, airway inflammation and health status in chronic obstructive pulmonary disease.

Acknowledgments

The authors would like to thank R. Stockley, S. Hill and D. Bayley for their advice and technical supervision of the laboratory procedures.

  • Received May 21, 2003.
  • Accepted December 6, 2003.

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Impact of sputum bacteria on airway inflammation and health status in clinical stable COPD
D. Banerjee, O.A. Khair, D. Honeybourne
European Respiratory Journal May 2004, 23 (5) 685-691; DOI: 10.1183/09031936.04.00056804
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