HOME HELP FEEDBACK SUBSCRIPTIONS ARCHIVE SEARCH TABLE OF CONTENTS		QUICK SEARCH:   [advanced] Author: Keyword(s): Year:  Vol:  Page:

This Article Abstract Full Text (PDF) All Versions of this Article: 290/6/L1052    most recent 00122.2005v1 Alert me when this article is cited Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via ISI Web of Science (4) Citing Articles via Google Scholar Google Scholar Articles by Pini, L. Articles by Ludwig, M. S. Search for Related Content PubMed PubMed Citation Articles by Pini, L. Articles by Ludwig, M. S.

Airway remodeling in allergen-challenged Brown Norway rats: distribution of proteoglycans

Meakins-Christie Laboratories, McGill University, Montreal, Quebec, Canada

Submitted 18 March 2005 ; accepted in final form 21 December 2005

	ABSTRACT

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Proteoglycans (PG) have important effects on the mechanical properties of tissues and the phenotype of various structural cells. Little is known about changes in PG deposition in the airways in animal models of asthma. We studied changes in PG in the airway wall of Brown Norway rats sensitized to ovalbumin (OA) and exposed to repeated OA challenge. Control (Sal) animals were sensitized and challenged with saline. After the 3rd challenge, animals were killed and lungs fixed in formalin. Tissue sections were incubated with antibodies to the small, leucine-rich PG, decorin, and biglycan and collagen type I. Airways were classified according to basement membrane perimeter length (0.99, 1–2.99, and 3 mm). Decorin, biglycan, and collagen type I were increased in the airways of OA vs. Sal rats. Remodeling was most prominent in central airways. The distribution of PG differed with respect to the subepithelial vs. airway smooth muscle (ASM) vs. adventitial layer. Whereas biglycan was readily detected within the ASM, decorin and collagen were detected outside the ASM and especially in the adventitial layer. Differences in the distribution of these molecules within the layers of the airway wall may reflect their specific functional roles.

decorin; biglycan; collagen

The majority of studies of airway remodeling have focused on changes in matrix proteins in the subepithelium and reticular basement membrane. Changes in matrix deposition in the airway smooth muscle (ASM) and adventitial layer have not been as well defined, although Palmans et al. (22) reported, in chronically ovalbumin (OA-)challenged Brown Norway (BN) rats, that fibronectin was deposited primarily in the outer airway wall adjacent to the ASM. Alterations in ECM deposition in the ASM and adventitial layers could have important functional consequences, because of altered impedance to ASM shortening (4), effects on smooth muscle proliferation (14), and/or possible unlinking of airways and surrounding parenchymal attachments (17). Previous work from this laboratory in the BN rat model has shown that, after multiple OA challenges, both ASM mass and airway hyperresponsiveness are increased (6, 32); alterations in PG could contribute to these changes.

Although many studies have investigated remodeling in larger airways utilizing endobronchial biopsy (20, 25, 27), there is less information available on changes in the distal airways. Kraft (16) showed inflammation within the alveolar wall in human asthma, whereas Minshall et al. (19) showed evidence of increased cytokine expression in the peripheral airways. Palmans et al. (22), in their investigation of the BN rat model of chronic OA challenge, reported increases in fibronectin and collagen deposition in airways of all sizes. Whether PG are altered in this model is not known.

A number of studies using endobronchial biopsy to sample the large airways have reported increases in the PG, lumican, decorin, biglycan, and versican, in the airway subepithelial layer in atopic, mild asthmatic patients (9, 12, 25). Roberts (26), in autopsy studies of patients dying of fatal asthma, showed deposition of versican within the ASM layer. However, no studies have systematically compared the deposition of these molecules within the different layers of the airway wall or in central vs. more peripheral airways. To investigate these questions, we utilized the BN rat model of repeated OA exposure (29, 32).

	METHODS

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Animal Model

Male BN rats, 8–10 weeks old, weighing 200 g, were sensitized by a single subcutaneous injection of 1 mg of OA (Sigma, Oakville, Ontario, Canada) and 100 µg of aluminum hydroxide; Bordetella pertussis (5 x 10⁸ heat-killed bacilli) was given intraperitoneally (ip) as an adjuvant. Challenged rats (n = 6) received aerosols of OA at 5-day intervals, on days 14, 19, and 24 after sensitization. Controls rats (n = 5) were challenged with saline (Sal). Rats were sedated with xylazine (7 mg/kg ip) and anesthetized with pentobarbital sodium (30 mg/kg ip). Orotracheal intubation was performed with polyethylene tubing (PE 240, 6 cm in length). The tip of the tracheal tube was inserted into a Plexiglas box into which aerosols of OA (5% wt/vol) were delivered via a micromist nebulizer (Hudson RCI; Teleflex Medical, Temecula, CA), which delivers particles with a mean aerosol diameter of 2.05 µm. OA or Sal was administrated for 5 min. All animals received humane care in compliance with the Guide to the Care and Use of Experimental Animals formulated by the Canadian Council of Animal Care, and an institutional animal ethics committee approved the protocol.

Immunohistochemistry

Tissue preparation and immunostaining. Two days after the last challenge, animals were killed by exsanguination, and lungs were removed. Lungs were fixed by intratracheal perfusion of 10% formalin at a constant pressure of 25 cmH₂O for 24 h. Lungs were embedded in paraffin, and sagittal sections (5 µm thick) were cut. Sections were incubated overnight with primary antibodies: rabbit polyclonal anti-mouse antibody for decorin (8) (1:1,000 dilution), rabbit polyclonal anti-human antibody for biglycan (28) (1:500 dilution) (both have been shown to cross-react with rat PG and were generous gifts of P. Roughley, Shriners Hospital, McGill University), or rabbit polyclonal anti-rat antibody for collagen type I (1:500 dilution, Cedarlane Laboratories, Hornby, Ontario, Canada). The secondary antibody applied was swine antibody to rabbit immunoglobulin (1:100 dilution; DAKO, Mississauga, Ontario, Canada). Streptavidin-alkaline phosphatase (1:200 dilution, DAKO) was used for detection. All immunostaining was developed with Fast Red (Sigma, Montreal, QC, Canada). Slides were counterstained with Gill II hematoxylin. Slides were examined under an Olympus light microscope (model BX50; Carson Group, Markham, Ontario, Canada). Positive staining appeared red under bright-field illumination. Control sections were processed in the absence of primary antibody.

PG immunolocalization by fluorescent microscopy. Excised lungs were fixed at a transpulmonary pressure of 25 cmH₂O with optimal cutting temperature medium and snap frozen in isopentane cooled in liquid nitrogen. Frozen sections were cut in 5-µm-thick sections with a cryostat and fixed in acetone-methanol. Sections were blocked by incubation with universal blocking solution for 30 min, followed by incubation with 10% normal goat serum. Slides were then rinsed with Tris-buffered saline (TBS) and incubated overnight at 4°C with mouse anti-human antibody for -smooth muscle actin (-SMA) (1:1,000 dilution, Sigma) and antibodies for biglycan or decorin. After being washed with TBS, sections were incubated with secondary antibody (1:000), 488 Alexa Fluor goat antibody to mouse immunoglobulin (-SMA) (Molecular Probes, Burlington, Ontario, Canada), and 546 Alexa Fluor goat antibody to rabbit immunoglobulin, (PG) (Molecular Probes). After being washed with TBS, sections were sealed with crystal mount and viewed under an Olympus florescence microscope (model BX51).

Staining for eosinophils with major basic protein. Frozen sections from OA- and Sal-challenged rats were stained with major basic protein (MBP) to identify eosinophils in the airway wall. In brief, frozen slides were blocked with universal blocking solution and then incubated overnight at 4°C with primary antibody to MBP (anti-human, 1:30 dilution; a generous gift of Dr. R. Moqbel). After being washed with TBS, slides were incubated with secondary antibody (polyclonal rabbit, anti-mouse 1:60, DAKO). Slides were again washed with TBS and then incubated with mouse APAAP (1:60, DAKO), and the reaction was visualized via addition of Fast Red (Sigma). Slides were counterstained with Gill II hematoxylin, washed, dipped in lithium carbonate, rinsed again, and then sealed in crystal mount. Sections were dried overnight at 37°C. Slides were examined with an Olympus microscope (model BX51); positive cells appeared red under bright-field illumination.

Morphometric Analysis

Microscopic images at a magnification of x200 were captured with commercial software (Image-Pro Plus, Silver Spring, MD). Only airways cut in transverse section, defined as a minimum to maximum internal diameter >0.33, were examined (29). All airways from all animals that met these criteria were included in the analysis. The following measurements were made: basement membrane perimeter (Pbm); internal airway lumen (LuB) defined by the inner border of the epithelium; external area of the airway wall (Ae) defined by the external border of the adventitial layer; and total area of the airway wall [airway wall thickness (WA_T)] calculated as the difference between Ae and LuB. Lines were drawn with a digital pen (Wacom), and values were calculated with SigmaScan (Jandel Scientific, Corte Madera, CA). Airways were divided into three groups according to Pbm, small: Pbm 0.99 mm; medium: 1.0–2.99 mm; and large: 3 mm. We quantified the amount of each ECM protein by tracing the area of positive staining established by determining a color threshold. The area of positive staining was standardized for airway size using Pbm², as this scaled an area with an area.

Data Analysis

Comparison between OA and Sal within different-sized airway groups was performed by unpaired t-tests. ANOVA was used to perform comparisons among different-sized airways within OA and Sal groups. Linear regression was used to examine the correlation between staining for decorin and collagen in those airways in which staining was done in serial sections for the respective molecules. Linear regression by the least-squares technique was also applied to determine the relationship between WA_T and Pbm² in both OA and Sal groups. t-Test was used to determine differences in the slopes of the regression lines between OA and Sal for the three different-sized airway groups. Values of P < 0.05 were considered statistically significant. Values are means ± SE.

	RESULTS

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Biglycan, decorin, and collagen I immunoreactivity was readily identified in the airways of the rats sensitized and repeatedly challenged with OA as well as those sensitized and repeatedly challenged with Sal (Fig. 1, A–F). Staining for all proteins was more prominent in OA-challenged rats. Decorin and biglycan showed a different pattern of distribution. Biglycan was distributed within the ASM layer in both OA and Sal airways; decorin spared the smooth muscle bundles (see insets Fig. 1, A and C). Collagen seemed to be distributed in a similar manner to decorin. All proteins were detected in the subepithelial and adventitial layer; minimal positive staining was observed within the epithelium. Staining for eosinophils was carried out in frozen sections (Fig. 1, G and H). (The MBP antibody used required frozen tissue; lung morphology is not as well preserved as in formalin-fixed tissue.) Airway and peri-vascular eosinophilia was more prominent in OA-challenged rats compared with Sal control rats.

View larger version (123K): [in this window] [in a new window]   Fig. 1. Representative photomicrographs of immunostaining in the airway wall of ovalbumin (OA)-challenged (A, C, E, G) and saline (Sal) control rats (B, D, F, H). Staining of large airways with primary antibody for biglycan (A, B), decorin (C, D), and collagen type I (E, F). Positive staining for biglycan was present within the smooth muscle layer (A, see inset), whereas decorin staining occurred around the smooth muscle bundles (C, see inset). G and H show staining of small airways with antibody to major basic protein. Eosinophils (indicated by arrowheads) are more prominent in the airway wall of the OA-challenged rat. ASM, airway smooth muscle; VSM, vascular smooth muscle.

View larger version (10K): [in this window] [in a new window]   Fig. 2. Area of immunostaining for biglycan (A), decorin (B), and collagen I (C) in OA (solid bars) and Sal (open bars) rats in the 3 groups of airways. A, area; Pbm, basement membrane perimeter. Thin lines represent comparisons between airways from OA- and Sal-challenged rats; thick lines represent comparisons among small, medium, and large airways in OA-challenged animals. n, Total number of airways examined in each group. **P < 0.01; *P < 0.05.

View larger version (7K): [in this window] [in a new window]   Fig. 3. Relationship between positive staining for decorin and collagen I in airways from OA ()- and Sal-challenged () rats. Linear regression was not significant (r = 0.37). Only those airways in which both proteins were stained on serial sections were included in the analysis.

View larger version (9K): [in this window] [in a new window]   Fig. 4. Relationship between total wall area (WAT) and basement membrane perimeter squared (Pbm2) in airways from OA ()- and Sal-challenged () rats. Linear regressions were significant for each group (r = 0.85 and 0.71 for OA and Sal, respectively. P < 0.05); the slopes of the 2 regression lines for the large and medium airway subgroups were significantly different from each other (P < 0.05).

View larger version (108K): [in this window] [in a new window]   Fig. 5. Representative photomicrographs of double immunofluorescent staining. A, C, and E show staining of a medium-sized airway for biglycan (A, fluorescent red), -smooth muscle actin (SMA) (C, fluorescent green) and the composite image (E). Biglycan was mainly localized in the smooth muscle layer. B, D, and F show staining of a small airway for decorin (B, fluorescent red), -SMA (D, fluorescent green) and the composite image (F). Decorin staining occurred around the smooth muscle bundles, primarily in the adventitial layer. Staining of serial sections of the same airway with -SMA and biglycan (G) and -SMA and decorin (H) underscores the different patterns of PG deposition relative to the smooth muscle layer, even within the same airway.

	DISCUSSION

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

Remodeling and changes in collagen and glycoproteins have been well described in the asthmatic airway wall in both humans and animal models (20, 22, 27). The absolute amount of collagen is increased in the subepithelial layer (20, 22); the specific subtypes of collagen upregulated include collagen types I and III (5, 27). Characterization of alterations in PG is more recent. Using endoscopic techniques to sample large airways, we have shown increases in versican, lumican, and biglycan in the subepithelial layer of the airway wall in patients with mild asthma (9, 12). Redington and coworkers (25) have reported substantial deposition of decorin in the reticular basement membrane. Roberts (26) reported prominent deposition of versican, biglycan, and decorin in the airway wall of patients dying from asthma or in whom asthma was a major contributor to death. In the current study, we extend these observations to an animal model of asthma, which permits a more careful characterization of the precise distribution of these molecules vis-à-vis the entire airway wall and the entire airway tree.

Significant increases in biglycan deposition were observed in both small and large airways, and significant increases in decorin deposition were observed in medium-sized airways in OA vs. Sal control animals (Fig. 2). We also characterized changes in collagen type I. Like Palmans et al. (22), who used a similar approach in chronically OA-challenged BN rats to characterize collagen deposition, collagen was increased in large airways in BN vs. control rats at 4 wk postsensitization and challenge. In our study, however, the increases in collagen were generally less substantial than the increases in PG. The relatively greater changes in PG in this repeated challenge model may reflect the tendency of PG to be upregulated at an earlier time point in the remodeling process, establishing a "provisional matrix" into which collagen and elastic fibers may be subsequently laid down. This temporal sequence has been described for pulmonary fibrosis in both humans and animal models (2, 31). Moreover, in this study, airway eosinophilia was more prominent in the OA-challenged rats, as has been shown previously in this repeated challenge BN rat model (22). This suggests that acute inflammation was ongoing.

We also examined whether matrix protein deposition within the airways of OA-challenged animals differed as a function of airway size. Although large airways showed the greatest deposition of biglycan, the amount of collagen deposition was greatest in the smaller airways. These latter data are different from those reported by Palmans et al. (22) in their OA-challenged animals examined at 4 wk, although their animals received six challenges over the 4-wk period compared with the three challenges delivered to the animals in the current protocol.

Overall, our data demonstrated a relatively greater increase in matrix deposition in the larger airways in the OA-challenged animals. This can perhaps be explained by the method of OA challenge employed in the current protocol. Antigen was administered by aerosol inhalation. The aerosol particles were most likely to be deposited on the mucosa of the larger-sized airways (3). As this is the type of antigen challenge that typically occurs in asthmatic patients, we believe it is the most pertinent to study.

We also investigated the deposition of PG molecules within the various layers of the airway wall. Immunohistochemical studies showed that there were different patterns of PG distribution; biglycan seemed to be prominent within the subepithelial and smooth muscle layer, whereas decorin spared the smooth muscle layer and was most evident in the adventitial layer. To further clarify the distribution of PG in relationship to ASM, we performed double immunostaining studies using -SMA antibody to identify ASM. We observed localization of biglycan and -SMA within the same layer of the airway wall; decorin was prominent outside the -SMA-positive layer, especially in the airway adventitia (Fig. 5). The data describing the distribution of decorin are similar to those reported by Roberts (26) in airway walls of patients dying of asthma, in whom they describe decorin prominence in the airway adventitia and septal structures. This pattern of distribution in patients with longstanding disease may reflect the importance of decorin as a regulator of collagen fibril formation. In areas where collagen deposition is prominent, decorin should be present. However, we were unable to document a significant correlation between decorin and collagen deposition in airways in which staining for both ECM molecules was performed (Fig. 3). This may reflect that, in this model, the airway remodeling process was in a relatively early stage.

The close association of biglycan with the smooth muscle layer is perhaps more surprising. Potter-Perigo et al. (24) have recently reported in human cell culture studies that biglycan was preferentially produced by vascular smooth muscle cells, whereas decorin was produced by bronchial smooth muscle cells. The pattern of distribution we observed suggests that cell secretion and accumulation of PG within the airway wall may be altered in asthmatic disease.

These data also raise the question of the functional impact of PG molecules on the surrounding cellular environment. PG are ECM proteins that subserve a number of important biological functions. They interact with various cytokines and growth factors, influence biomechanical behavior of the tissues, and affect cell adhesion and migration (13). Decorin and biglycan interact with TGF-, a cytokine known to play an important role in the airway fibrosis observed in asthma (20, 25). A recent study by Tufvesson and Westergren-Thorsson (30) describes the effects of biglycan and decorin on lung fibroblast phenotype. Both PG induced comparable changes in fibroblast morphology and stress fiber formation. However, important differences were noted in the amount of -SMA induced, a finding that could have potential implications for differential effects of decorin and biglycan on ASM phenotype. Moreover, decorin and biglycan differentially upregulated mRNA for proteins involved in cell-matrix interactions, cell-cell interactions, and intracellular signaling. In vascular smooth muscle, the large PG, versican, is required for normal cell proliferation (7). A recent study by Johnson et al. (14) reported that ECM proteins secreted by asthmatic ASM cells enhanced ASM cell proliferation. Excess biglycan within the smooth muscle layer in the airway wall of OA-challenged animals may have the capacity to augment the smooth muscle hypertrophy previously reported in this model (6, 32).

The distribution of PG molecules within the various layers of the airway wall in the asthmatic model could also have implications for airway function from a more mechanical perspective. It has consistently been shown in the OA-challenged, BN rat model that multiple OA challenges lead to enhanced airways responsiveness (22, 32). Data from our laboratory demonstrate that PG influence both airway mechanics and the viscoelastic behavior of the lung tissues (1, 10). Specific enzymatic degradation of glycosaminoglycan side chains altered lung parenchymal strip viscoelastic properties (1). Both airway resistance and tissue compliance measured in vivo were altered in mice deficient in the small PG, decorin (10). Hence, excess deposition of PG within the airway wall could potentially affect airway mechanical properties and airway responsiveness (21). The distribution of PG deposition within the smooth muscle layer of the airway wall could also have an impact on the impedance to ASM shortening during induced constriction (4, 23). Finally, changes in PG deposition in the adventitial layer could have an effect on airway parenchymal interdependence. The airway wall could become unlinked from the modulating effects of the surrounding parenchymal attachments, permitting airways to constrict relatively unimpeded (18). Alternately, excess deposition of PG could affect the tethering between the airways and parenchyma in such as a way as to augment the impedance offered by the surrounding parenchymal attachments. Palmans and coworkers (22) reported excess fibronectin deposition in the outer wall layer of chronically OA-challenged BN rats and similarly postulated an impact on airway parenchymal interdependence and bronchial reactivity, although less is known about the biomechanical characteristics of fibronectin.

In conclusion, we have found that decorin, biglycan, and collagen type I are upregulated in the airway wall of sensitized BN rats exposed to repeated OA challenge; the greatest changes occurred in the larger airways. The pattern of distribution in the ASM and adventitial layer, of the two small PG studied, biglycan and decorin, differed. To better understand how changes in these molecules affect cell phenotype, studies on the effects of PG on the functional behavior of the adjacent structural cells are warranted. The BN rat model of allergic asthma provides a ready source of cells to further pursue these questions.

	GRANTS

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Supported by the Canadian Institutes of Health Research and the J. T. Costello Memorial Research Fund.

	ACKNOWLEDGMENTS

 
The authors thank Meiyo Tamaoka for help with the BN rat model and Pierre Fiset for help with the figures.

	FOOTNOTES

 

Address for reprint requests and other correspondence: M. Ludwig, Meakins Christie Labs, 3626 St. Urbain St., Montreal, QC Canada (e-mail: mara.ludwig{at}mcgill.ca)

The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

	REFERENCES

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 

1. Al Jamal R, Roughley PJ, and Ludwig MS. Effect of glycosaminoglycan degradation on lung tissue viscoelasticity. Am J Physiol Lung Cell Mol Physiol 280: L306–L315, 2001.[Abstract/Free Full Text]
2. Bensadoun ES, Burke AK, Hogg JC, and Roberts CR. Proteoglycan deposition in pulmonary fibrosis. Am J Respir Crit Care Med 154: 1819–1828, 1996.[Abstract]
3. Brain JD and Valberg PA. Deposition of aerosol in the respiratory tract. Am Rev Respir Dis 120: 1325–1373, 1979.[ISI][Medline]
4. Bramley AM, Roberts CR, and Schellenberg RR. Collagenase increases shortening of human bronchial smooth muscle in vitro. Am J Respir Crit Care Med 152: 1513–1517, 1995.[Abstract]
5. Chakir J, Shannon J, Molet S, Fukakusa M, Elias J, Laviolette M, Boulet LP, and Hamid Q. Airway remodeling-associated mediators in moderate to severe asthma: effect of steroids on TGF-beta, IL-11, IL-17, and type I and type III collagen expression. J Allergy Clin Immunol 111: 1293–1298, 2003.[CrossRef][ISI][Medline]
6. Du T, Sapienza S, Wang CG, Renzi PM, Pantano R, Rossi P, and Martin JG. Effect of nedocromil sodium on allergen-induced airway responses and changes in the quantity of airway smooth muscle in rats. J Allergy Clin Immunol 98: 400–407, 1996.[CrossRef][ISI][Medline]
7. Evanko SP, Angello JC, and Wight TN. Formation of hyaluronan- and versican-rich pericellular matrix is required for proliferation and migration of vascular smooth muscle cells. Arterioscler Thromb Vasc Biol 19: 1004–1013, 1999.[Abstract/Free Full Text]
8. Fisher LW, Stubbs JT III, and Young MF. Antisera and cDNA probes to human and certain animal model bone matrix noncollagenous proteins. Acta Orthop Scand Suppl 266: 61–65, 1995.[Medline]
9. Flood-Page P, Menzies-Gow A, Phipps S, Ying S, Wangoo A, Ludwig MS, Barnes N, Robinson D, and Kay AB. Anti-IL-5 treatment reduces deposition of ECM proteins in the bronchial subepithelial basement membrane of mild atopic asthmatics. J Clin Invest 112: 1029–1036, 2003.[CrossRef][ISI][Medline]
10. Fust A, LeBellego F, Iozzo RV, Roughley PJ, and Ludwig MS. Alterations in lung mechanics in decorin-deficient mice. Am J Physiol Lung Cell Mol Physiol 288: L159–L166, 2005.[Abstract/Free Full Text]
11. Hildebrand A, Romaris M, Rasmussen LM, Heinegard D, Twardzik DR, Border WA, and Ruoslahti E. Interaction of the small interstitial proteoglycans biglycan, decorin and fibromodulin with transforming growth factor beta. Biochem J 302: 527–534, 1994.
12. Huang J, Olivenstein R, Taha R, Hamid Q, and Ludwig MS. Enhanced proteoglycan deposition in the airway wall of atopic asthmatics. Am J Respir Crit Care Med 160: 725–729, 1999.[Abstract/Free Full Text]
13. Iozzo RV. Matrix proteoglycans: from molecular design to cellular function. Annu Rev Biochem 67: 609–652, 1998.[CrossRef][ISI][Medline]
14. Johnson PR, Burgess JK, Underwood PA, Au W, Poniris MH, Tamm M, Ge Q, Roth M, and Black JL. Extracellular matrix proteins modulate asthmatic airway smooth muscle cell proliferation via an autocrine mechanism. J Allergy Clin Immunol 113: 690–696, 2004.[CrossRef][ISI][Medline]
15. Kolb M, Margetts PJ, Sime PJ, and Gauldie J. Proteoglycans decorin and biglycan differentially modulate TGF--mediated fibrotic responses in the lung. Am J Physiol Lung Cell Mol Physiol 280: L1327–L1334, 2001.[Abstract/Free Full Text]
16. Kraft M. The distal airways: are they important in asthma? Eur Respir J 14: 1403–1417, 1999.[Abstract]
17. Macklem PT. A theoretical analysis of the effect of airway smooth muscle load on airway narrowing. Am J Respir Crit Care Med 153: 83–89, 1996.[Abstract]
18. Mead J, Takishima T, and Leith D. Stress distribution in lungs: a model of pulmonary elasticity. J Appl Physiol 28: 596–608, 1970.[Free Full Text]
19. Minshall EM, Hogg JC, and Hamid QA. Cytokine mRNA expression in asthma is not restricted to the large airways. J Allergy Clin Immunol 101: 386–390, 1998.[CrossRef][ISI][Medline]
20. Minshall EM, Leung DY, Martin RJ, Song YL, Cameron L, Ernst P, and Hamid Q. Eosinophil-associated TGF-beta1 mRNA expression and airways fibrosis in bronchial asthma. Am J Respir Cell Mol Biol 17: 326–333, 1997.[Abstract/Free Full Text]
21. Moreno RH, Hogg JC, and Pare PD. Mechanics of airway narrowing. Am Rev Respir Dis 133: 1171–1180, 1986.[ISI][Medline]
22. Palmans E, Kips JC, and Pauwels RA. Prolonged allergen exposure induces structural airway changes in sensitized rats. Am J Respir Crit Care Med 161: 627–635, 2000.[Abstract/Free Full Text]
23. Pare PD. Airway hyperresponsiveness in asthma: geometry is not everything! Am J Respir Crit Care Med 168: 913–914, 2003.[Free Full Text]
24. Potter-Perigo S, Baker C, Tsoi C, Braun KR, Isenhath S, Altman GM, Altman LC, and Wight TN. Regulation of proteoglycan synthesis by leukotriene d4 and epidermal growth factor in bronchial smooth muscle cells. Am J Respir Cell Mol Biol 30: 101–108, 2004.[Abstract/Free Full Text]
25. Redington AE, Roche WR, Holgate ST, and Howarth PH. Co-localization of immunoreactive transforming growth factor-beta 1 and decorin in bronchial biopsies from asthmatic and normal subjects. J Pathol 186: 410–415, 1998.[CrossRef][ISI][Medline]
26. Roberts CR. Is asthma a fibrotic disease? Chest 107: 111S–117S, 1995.[Medline]
27. Roche WR, Beasley R, Williams JH, and Holgate ST. Subepithelial fibrosis in the bronchi of asthmatics. Lancet 1: 520–524, 1989.[CrossRef][ISI][Medline]
28. Roughley PJ, White RJ, Magny MC, Liu J, Pearce RH, and Mort JS. Non-proteoglycan forms of biglycan increase with age in human articular cartilage. Biochem J 295: 421–426, 1993.
29. Sapienza S, Du T, Eidelman DH, Wang NS, and Martin JG. Structural changes in the airways of sensitized brown Norway rats after antigen challenge. Am Rev Respir Dis 144: 423–427, 1991.[ISI][Medline]
30. Tufvesson E and Westergren-Thorsson G. Biglycan and decorin induce morphological and cytoskeletal changes involving signalling by the small GTPases RhoA and Rac1 resulting in lung fibroblast migration. J Cell Sci 116: 4857–4864, 2003.[Abstract/Free Full Text]
31. Venkatesan N, Ebihara T, Roughley PJ, and Ludwig MS. Alterations in large and small proteoglycans in bleomycin-induced pulmonary fibrosis in rats. Am J Respir Crit Care Med 161: 2066–2073, 2000.[Abstract/Free Full Text]
32. Wang CG, Du T, Xu LJ, and Martin JG. Role of leukotriene D4 in allergen-induced increases in airway smooth muscle in the rat. Am Rev Respir Dis 148: 413–417, 1993.[ISI][Medline]

This article has been cited by other articles:

				M. L. D'Antoni, C. Torregiani, P. Ferraro, M.-C. Michoud, B. Mazer, J. G. Martin, and M. S. Ludwig Effects of decorin and biglycan on human airway smooth muscle cell proliferation and apoptosis Am J Physiol Lung Cell Mol Physiol, April 1, 2008; 294(4): L764 - L771. [Abstract] [Full Text] [PDF]

				F. G. Salerno, V. Pinelli, L. Pini, B. Tuma, R. V. Iozzo, and M. S. Ludwig Effect of PEEP on induced constriction is enhanced in decorin-deficient mice Am J Physiol Lung Cell Mol Physiol, November 1, 2007; 293(5): L1111 - L1117. [Abstract] [Full Text] [PDF]

				S. S. An, T. R. Bai, J. H. T. Bates, J. L. Black, R. H. Brown, V. Brusasco, P. Chitano, L. Deng, M. Dowell, D. H. Eidelman, et al. Airway smooth muscle dynamics: a common pathway of airway obstruction in asthma Eur. Respir. J., May 1, 2007; 29(5): 834 - 860. [Abstract] [Full Text] [PDF]

				B. Tigani, C. Cannet, H. Karmouty-Quintana, F.-X. Ble, S. Zurbruegg, E. Schaeublin, J. R. Fozard, and N. Beckmann Lung inflammation and vascular remodeling after repeated allergen challenge detected noninvasively by MRI Am J Physiol Lung Cell Mol Physiol, March 1, 2007; 292(3): L644 - L653. [Abstract] [Full Text] [PDF]

This Article Abstract Full Text (PDF) All Versions of this Article: 290/6/L1052    most recent 00122.2005v1 Alert me when this article is cited Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via ISI Web of Science (4) Citing Articles via Google Scholar Google Scholar Articles by Pini, L. Articles by Ludwig, M. S. Search for Related Content PubMed PubMed Citation Articles by Pini, L. Articles by Ludwig, M. S.