Characterization of pulmonary vascular remodelling in smokers and patients with mild COPD

Tissue

Resected lung specimens were obtained from 15 patients, all male, who underwent lobectomy or pneumonectomy because of lung carcinoma. Pulmonary function tests were performed in the days preceding surgery. All patients were heavy smokers. Patients were divided into two groups: one with airflow obstruction (COPD, n=8) and the other with lung function within the normal range (smokers, n=7). The clinical and functional characteristics of the two groups are shown in table 1⇓. For control purposes, specimens from three nonsmokers who also underwent lung resection for carcinoma, were subjected to the same protocol (age: 69±8 yrs; forced expiratory volume in one second (FEV₁): 102±4% predicted; forced vital capacity: 95±10% pred; total lung capacity: 97±12% pred; carbon monoxide diffusing capacity: 90±12 % pred).

Following surgical resection, lung tissue sections were fixed by overnight immersion in 4% buffered formaldehyde at 4°C and embedded in paraffin. Two blocks of parenchyma, sampled in areas of normal appearance far from the neoplasic lesion, were selected in each case for serial sectioning (3 µm thick).

Histological stains for extracellular matrix protein identification

One tissue section was stained with haematoxylin and eosin for artery location purposes. Serial sections were stained with orcein to localize elastin fibres, Masson's trichrome to identify collagen, and alcian blue to localize proteoglycans 14. After staining, sections were examined by light microscopy.

Morphometric studies

The morphometric characteristics of pulmonary muscular arteries were analysed in lung tissue sections stained with orcein. Arteries with an external diameter between 100–500 µm and complete elastic laminas, were evaluated using a computerized image-analysis system (Microm S.A., Barcelona, Spain), as previously described 3. External and internal elastic laminas and the inner aspect of the intima were outlined, the areas occupied by the muscular layer, the intimal layer and the lumen were computed, and all were expressed as a percentage of the measured total area (area encompassed by the external elastic lamina). Because vascular contraction during surgical manipulation and tissue shrinkage during fixation could induce changes in vessel morphometry, a theoretical diameter of the fully distended artery was calculated by dividing the length of the external elastic lamina by pi (π) 15. In order to evaluate the effect of these potential artifacts, an index of “narrowing” was then estimated in each artery as the ratio between the measured total area and that extrapolated from the theoretical distended diameter.

Immunohistochemistry

Tissue sections were immunostained with monoclonal antibodies to identify intrinsic cells of the vascular wall using the avidin-biotin complex/horseradish peroxidase (ABC/HRP) method (Vector Laboratories, Burlingame, CA, USA). Briefly, in order to inhibit endogenous peroxidase activity, sections were incubated with 0.3% H₂O₂ in methanol. After two washouts with phosphate-buffered saline (PBS), nonspecific binding was suppressed by incubation with 3% normal horse serum. One of the following optimally diluted primary monoclonal mouse antibodies was used overnight at 4°C: antihuman factor VIII‐related antigen (factor VIII; M 0616) was used to identify endothelial cells; both anti‐α‐smooth muscle actin (α‐SMA; M 0851) and anti-desmin (M 0760) were used to characterize smooth muscle cells (SMCs); and anti-vimentin (M 0725), which is present in all mesenchymal cells, was used to localize fibroblasts (all antibodies were obtained from Dako, Glostrup, Denmark). Species-matched normal serums served as negative controls. After two washouts in PBS, sections were incubated with biotinylated horse antimouse immunoglobulin (Ig)‐G (1:400 dilution) (Vector Laboratories), washed, and finally incubated with the ABC/HRP. Ig complexes were visualized by immersing sections in a solution of diaminobenzidine and hydrogen peroxide. Sections were then washed again, counterstained with Gill's haematoxylin, dehydrated and cover slipped.

Data analysis

For each patient, 11±2 pulmonary muscular arteries with evident intimal thickening at microscopical examination were studied. Histochemical and immunohistochemical stains were performed in serial sections, in such a way that the same arteries were analysed with the different stains in adjacent sections.

In each arterial intima, the amount of elastin, collagen and proteoglycan deposition, as well as the density of the cell infiltrate, was assessed semiquantitatively using a visual scale ranging from 0–3 (0=absent; 1=scarce; 2=moderate; and 3=abundant), in a way similar to that reported by Tuder et al. 16. Furthermore, the number of SMCs containing desmin or vimentin in the intima was estimated as a per cent rank of positive actin cells using the following ranges: 1) <25%; 2) from 25–75%; and 3) >75%.

Autopsy material from a case with primary pulmonary hypertension and prominent concentric obliterative arteriopathy, subjected to the same histological protocol, was used for control purposes.

Statistical analysis

Data are expressed as mean±sd. Measurements from the two groups were compared using an unpaired t‐test. The relationship between morphometric measurements and the scoring of histological stains was assessed by one-way analysis of variance (ANOVA). The extracellular matrix determinants of intimal thickness were assessed by multiple linear regression analysis, with intimal thickness as the dependent variable, and the amount of elastin, collagen and proteoglycans as the independent variables. A p‐value <0.05 was considered statistically significant in all cases.

Functional and morphometric measurements

Patients in the two groups were matched by age and smoking history. Patients with COPD showed a moderate degree of airflow obstruction and in all but one, the partial pressure of arterial oxygen (P_a,O2) was within the normal range (>80 mmHg) (table 1⇑). The morphometric measurements of pulmonary muscular arteries are summarized in table 2⇓. A similar number of arteries in each subset, with a similar diameter and degree of narrowing (index of narrowing; 17±13% and 11±13%, smokers and COPD patients, respectively) were measured. At the morphometric analysis the intimal layer occupied approximately one-third of the measured total area. There were no differences in the degree of intimal enlargement between the group of patients with COPD and the smokers. The thickness of the muscular layer and the size of the arterial lumen were also similar between the two groups. In comparison, control subjects showed thinner intimas and larger lumens, whereas the muscular area was similar (table 2⇓).

Immunohistochemistry

A single endothelial layer outlined the innermost portion of the pulmonary muscular arteries, as disclosed by staining with the factor VIII antibody. No proliferation of endothelial cells was detected within the intimal coat (fig. 1a⇓). In contrast, the majority of cells present in the thickened intimas showed positive immunoreactivity to α‐SMA antibody, with a mean score of 2.6±0.7 (possible maximal score, 3) (fig. 1b⇓). The intensity of staining of positive α‐SMA cells in the intima was similar to that in the muscle cells of the adjacent media. However, whereas medial SMCs were oriented circumferentially, SMCs infiltrating the intima were oriented longitudinally (fig. 1b⇓).

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Fig. 1.—

Serial sections of a pulmonary muscular artery from a patient in the smokers' group, with prominent intimal thickening and luminal narrowing. The following immunostainings are shown: a) factor VIII‐related antigen; b) α‐smooth muscle actin; c) vimentin; and d) desmin. Whereas factor VIII is expressed only in a single endothelial cell lining (as indicated by the arrow in a), note the intense muscle-specific actin expression by the intimal cells (b). Vimentin immunostaining is found in adventitial fibroblasts, endothelial cells and in the majority of smooth muscle cells in both the intima and the media (c). In contrast, desmin immunoreactivity is preserved in the medial layer but is negative in most of the intimal cells (d). A: adventitia; M: medial layer; I: intimal layer; L: lumen. Internal scale bar=50 µm.

Vimentin intermediate filaments were expressed in endothelial cells, adventitial fibroblasts and in the majority of SMCs in both the intima and the media (fig. 1c⇑). The majority of SMCs showed positive immunoreaction for desmin. However, whereas all the cells in the media expressed both desmin and vimentin filaments, in the intima the number of cells expressing desmin (mean score 1.9±1.1) was lower than that of cells expressing vimentin (mean score 2.5±0.7) (fig. 1d⇑). This finding is consistent with a phenotypically heterogeneous population of SMCs in the thickened arterial intimas.

Fibroblasts, which stained to vimentin antibody but not to α‐SMA and desmin antibodies, were localized in the adventitia but not in the intima.

No differences in the pattern of immunostaining were observed between patients with and without airflow obstruction (table 3⇓). In control subjects, only the intimas were inmunostained with the endothelial cell markers.

Extracellular matrix proteins

Elastin was the most abundant extracellular matrix protein in the intimal layer, with a mean score of 2.9±0.3 (possible maximal score 3) and was present in the majority of the muscular arteries, irrespective of the degree of intimal enlargement (table 4⇓). Elastic fibres had a concentric deposition pattern and occupied the whole intimal surface (fig. 2a⇓). In arteries with thick intimas, fibres at the abluminal side, adjacent to the internal elastic lamina, were more dense and thicker than those at the adluminal side.

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Fig. 2.—

Histological stains of serial sections of a pulmonary muscular artery from a patient in the smokers' group. a) orcein stain; b) Masson's trichrome stain; c) alcian blue stain. Observe the abundant amount of elastin (a) and collagen (b) within the intimal layer, with a scarce proportion of proteoglycans (c). Internal scale bar=100 µm.' group. a) orcein stain; b) Masson's trichrome stain; c) alcian blue stain. Observe the abundant amount of elastin (a) and collagen (b) within the intimal layer, with a scarce proportion of proteoglycans (c). Internal scale bar=100 µm.

Studies with the Masson's thricromic stain localized abundant collagen throughout the intimal layer (mean score 1.8±1.1), intermixed with elastin fibres (fig. 2b⇑). The pattern of collagen-fibre deposition was opposed to that of elastic fibres, as it was more prominent in the adluminal side of the intima. The amount of collagen deposition was related to the degree of intimal thickening. Intimal thickness was 30±10% in the arteries without collagen deposition, 30±13% in those with scarce deposition, 32±10% in those with moderate deposition, and 45±12% in those with abundant deposition (ANOVA: p<0.001) (fig. 3⇓). Multiple regression analysis showed a better estimate of the degree of intimal thickening when both elastin and collagen deposition were taken together as covariables (R²=0.26, p<0.001).

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Fig. 3.—

Relationship between the amount of collagen and the intimal thickness in pulmonary muscular arteries of patients with mild chronic obstructive pulmonary disease (COPD) and smokers. For each category of amount of collagen, the box represents the interquartile range (between the 25–75th percentiles), with the median shown as a horizontal bar within each box. The bars outside each box indicate the 95% range of all values. *: p<0.05 compared with the other categories.

Alcian blue staining revealed weak signals for proteoglycans in the majority of arterial intimas (mean score 0.7±0.8) (fig. 2c⇑). No differences were shown between smokers and COPD patients regarding the amount of elastin, collagen or proteoglycans (table 3⇑). The pulmonary arteries of nonsmoking controls did not show extracellular matrix deposition out of the internal elastic lamina.