Importance of Proteolytic Events, Time Course, and Role in Mediating Mitogenesis |
||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
 |
Abstract |
|---|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
We previously reported that mast cell tryptase is a potent mitogen for cultured airway smooth-muscle cells, but the early intracellular signals mediating this response are not known. In many cells, proliferative effects are mediated by a mitogen-activated protein kinase signaling pathway involving Raf-1, MAP kinase kinases (MEKs), and extracellular signal-regulated protein kinases (ERKs) 1 and 2. Therefore, we tested for tryptase-induced activation of ERK1 and 2 in cultured dog tracheal smooth-muscle cells. Tryptase, in nanomolar concentrations which potently stimulated DNA synthesis, increased dual phosphorylation of ERKs in cellular lysates as well as ERK2 kinase activity in immunoprecipitates. Pretreatment of cells with the MEK inhibitor PD098059 abolished tryptase-induced increases in DNA synthesis and attenuated increases in ERK2 activity. Irreversible inhibition of tryptase's proteolytic activity, using p-amidino phenylmethanesulfonyl fluoride, attenuated tryptase-induced increases in DNA synthesis and dual phosphorylation of ERKs by 76% and 40 to 60%, respectively. Tryptase also increased c-fos transcription as quantified in polymerase chain reactions. In concentrations that caused similar increases in DNA synthesis, tryptase and platelet-derived growth factor (PDGF-BB) increased ERK activity (and c-fos transcription) with markedly different kinetics, the tryptase-induced responses being slower in onset and more sustained. We conclude that tryptase-induced mitogenesis in airway smooth-muscle cells requires activation of ERK1 and 2; that these responses depend partially, but not completely, upon tryptase's properties as a protease; and that they are slower in onset and more sustained than those induced by PDGF-BB.
| |
Introduction |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
Tryptases are trypsin-like neutral serine-class proteases which
are selectively expressed in mast cells and basophils (for review, see Reference 1). In human mast cells, tryptases are
present in extremely high concentrations, accounting for
25% of the total intracellular protein (1). 
-Tryptase is the
major member of this family that is stored in mast-cell granules, and it also is the predominant tryptase in lung tissue
(1). Tryptase is released from mast cells by both immunoglobulin E-dependent and -independent mechanisms (1).
Once released, it has several potential effects on neighboring cells. One such effect is the ability to stimulate growth
(2). In isolated cells in culture, tryptase is a potent mitogen for human and rodent lung fibroblasts (2, 3), airway
smooth-muscle (4) and epithelial cells (5), and vascular endothelial cells (6). Therefore, tryptase's properties as a
growth factor may contribute to pathologic processes in
the lung, such as fibroblast proliferation in interstitial lung
diseases, airway smooth-muscle and glandular hyperplasia in asthma and chronic bronchitis (7), and abnormal new-vessel formation in pulmonary vascular disorders.
Little is known about the cellular mechanisms for tryptase-induced mitogenesis and about the early intracellular signals which mediate it. In its heparin-stabilized tetrameric form tryptase has potent catalytic activity (1), and some have assumed that its extracellular actions depend entirely upon its ability to cleave proteins. Of potential relevance are the findings that tryptase-induced mitogenesis in some cells (8) may be mediated via activation of protease-activated receptor (PAR)-2, one member of a new class of G protein-coupled PARs (9). It is not known whether PAR-2 activation accounts for all of tryptase's growth stimulatory effects. There is evidence that it may not. For example, PAR-2 activation has uniformly been associated with brisk increases in phosphoinositide hydrolysis and intracellular calcium concentrations (9). Tryptase did not induce either of these changes in lung fibroblasts in which it had potent mitogenic effects, even under conditions where increases in phosphoinositide hydrolysis and calcium concentrations were easily detectable in response to other mitogenic serine proteases (2). Further, it is increasingly apparent that some mitogenic serine proteases have the capacity to induce growth via nonproteolytic mechanisms (10), and PAR-2 activation by serine proteases is thought to proceed solely via proteolytic mechanisms (9). On the basis of these considerations, it is clear that more information is needed about the proteolytic versus nonproteolytic mechanisms through which tryptase stimulates growth in cells from airways and lung.
With respect to early intracellular signals, an important and unanswered issue is the potential role of mitogen-activated protein (MAP) kinases in mediating tryptase-induced mitogenesis. This family of proteins serves as second messengers for a variety of cellular effects, including proliferation, differentiation, and the responses to stresses such as irradiation, osmotic imbalances, or heat shock (11). MAP kinases include extracellular signal-regulated protein kinases (ERKs), p38 isoforms, and Jun amino-terminal kinase/stress-activated protein kinase proteins, all of which are serine/threonine kinases with extensive sequence homology. In most cells, growth and differentiation factors induce early activation of ERKs via sequential phosphorylation of the protein kinases Raf-1, MAP kinase kinase (MEK) 1 and 2, and ERK1 and 2 (also known as p44 and p42) (11). Whether tryptase activates MAP kinases to induce its growth-stimulatory effects in airway or lung cells is not known.
The major goal of our experiments was to determine whether tryptase activates ERK1 and 2 in cultured dog tracheal smooth-muscle cells, for which tryptase is a potent mitogen (4). Other goals were: (1) to assess the importance of tryptase's enzymatic activity in the mediation of its responses in our cells; (2) to establish the time course of tryptase's effects on ERK1 and 2, because the duration of ERK activation is known to be an important determinant of proliferative responses in airway smooth-muscle cells (12); and (3) to use PD098059, the cell-permeable MEK1 and 2 inhibitor (13), to determine whether activation of ERKs is vital for increased DNA synthesis in response to tryptase. Throughout these experiments, we compared the effects of tryptase with those of platelet-derived growth factor (PDGF), a member of the receptor tyrosine kinase class of growth factors that is a well established stimulator of both ERK activity and mitogenesis in airway smooth-muscle cells (14). Also, because we found significant differences in the time course of tryptase- versus PDGF-mediated activation of ERKs, we examined whether these differences are also apparent in induction of c-fos transcripts, inasmuch as c-fos is an immediate early response gene that is activated after translocation of activated ERK to the nucleus (15).
| |
Materials and Methods |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
Materials
Porcine heparin (4 to 6 kD), N-p-tosyl-Gly-Pro-Lys p-nitroanilide (GPK), p-amidino phenylmethanesulfonyl fluoride (p-APMSF), and Triton X-100 were purchased from Sigma Chemical (St. Louis, MO). Other reagents and their sources were PD098059 (CalBiochem, La Jolla, CA); recombinant human PDGF-BB homodimer, protein G-agarose, P-81 phosphocellulose paper, Taq DNA polymerase, and Maloney murine leukemia virus (MMLV) reverse transcriptase (RT) (Life Technologies, Gaithersburg, MD); and serum-free media (cellgro COMPLETE; Mediatech, Inc., Herndon, VA). Antibodies used in these experiments, and their sources, were: phosphospecific anti-ERK antibody kit (New England BioLabs, Beverly, MA), anti-ERK2 antibody for immunoprecipitation (C-14; Santa Cruz Biotechnologies, Santa Cruz, CA), anti-phosphotyrosine antibody 4G10 (Upstate Biotechnologies, Lake Placid, NY), and anti-ERK1 and 2 polyclonal antibody (Zymed Labs, South San Francisco, CA). Goat antimouse horseradish peroxidase (HRP) conjugate was purchased from Dako (Carpinteria, CA), goat antirabbit HRP conjugate from Bio-Rad (Hercules, CA), and reagents for enhanced chemiluminescence (ECL) from Pierce (Rockford, IL). RNAzol B was purchased from Biotecx Inc. (Houston, TX) and RNAsin from Promega (Madison, WI). Sequenase T7 DNA polymerase was from United States Biochemical (Cleveland, OH).
Cell Culture
Primary cultures of dog tracheal smooth-muscle cells were established and maintained as previously described (16). Cells were
fed on alternate days and were passaged enzymatically when they
approached confluence. We used these preparations of cells because they fulfill established criteria for identification of smooth-muscle cells in culture, including intense and uniform staining for
smooth-muscle actin (at antibody concentrations no more than
2 µg/ml) and a contoured "hill-and-valley" morphology at confluence. Also, these cells possess morphologic features that distinguish them from dog tracheal fibroblasts in culture (16).
Tryptase
Tryptase was isolated from postmortem human lung tissue, as described previously (3). Purity of the tryptase in these isolates has been established using chromatographic, electrophoretic, and immunologic criteria (3).
Catalytic activity of tryptase was measured by assessing its ability to cleave GPK (4). Tryptase, in 1- to 5-µL aliquots, was added to 50 mM Tris buffer, pH 7.7, containing 120 mM NaCl, 20 µg/ml heparin, and 100 µM GPK (final volume: 100 µL). Rates of GPK hydrolysis were determined by measuring the change in absorbance at 405 nm and calculating the amount of cleaved substrate, assuming a molar extinction coefficient of 8,800.
To inhibit catalytic activity, we preincubated tryptase with p-APMSF (17). This compound is a specific, irreversible inhibitor of the class of serine proteases which cleaves substrates after lysine or arginine (17), and tryptase falls into this class (1). In our experiments, tryptase (final concentrations: 10.5 to 27 nM) was incubated with p-APMSF (final concentration: 10 µM) for 100 to 120 min at 4°C in 10 mM BisTris buffer, pH 6.1. As a control, tryptase was also incubated with p-APMSF diluent alone (1:1 acetonitrile/dimethylformamide). Incubates were then diluted 1:5 in serum-free cellgro COMPLETE media, pH 7.4, and incubated on ice for 3 to 5 h before application to cells in 96-well plates. To test for its possible cytotoxic effects, p-APMSF that had been incubated alone was added to wells containing serum-free media, PDGF-BB, and 10% fetal calf serum (FCS), and the effects on DNA synthesis (see the following section) were determined. Before application on cells, p-APMSF-treated tryptase was assayed for completeness of catalytic inhibition using the GPK assay, as described earlier.
DNA Synthesis
To quantify DNA synthesis in the cells, we measured the incorporation of bromodeoxyuridine (BrdU) into cellular DNA using an enzyme-linked immunosorbent assay (ELISA), as we described previously (4). Passages 1-5 were seeded at densities of 10,000 cells/well in 96-well formats. After 24 h in M199 media containing 10% FCS, cells were washed once with phosphate-buffered saline (PBS) and then starved for 24 h in cellgro COMPLETE serum-free media. Mitogens were introduced into the cultures and the BrdU (10 µM) was added 24 to 48 h later. PD098059 is a cell-permeant inhibitor of MEK1 and 2, kinases that activate ERK1 and 2 (13). Therefore, to test the effects of inhibiting this pathway on tryptase-induced increases in DNA synthesis, we added PD098059 40 to 60 min before mitogens in some experiments.
Western Analysis of Phosphorylated ERK1 and 2
After exposing cells to mitogens, we tested for increases in phosphorylation of ERK1 and 2 in lysates prepared from the cells. Different antibodies were used to detect either protein tyrosine phosphorylation in general in the lysates or to detect specific, doubly phosphorylated (on threonine 202 and tyrosine 204)
ERK1 and 2 only (18). Cells were grown to confluence in six-well plates, washed once with PBS, and then starved for 24 h in M199 media containing 0.5% FCS. After the indicated times of stimulation, media were removed and cells were washed twice with ice-cold PBS and lysed with 40 µL of Triton X-100 lysis buffer (50 mM
N-2-hydroxyethylpiperazine-N'-ethane sulfonic acid [pH 7.5],
100 mM NaCl, 1% Triton X-100, 1.5 mM MgCl2, 50 mM NaF,
10 mM sodium pyrophosphate, 1 mM ethylenediaminetetraactic acid [EDTA], 10% glycerol, 1 mM sodium vanadate, 1 mM PMSF,
10 µg/ml leupeptin, and 10 µg/ml aprotinin) augmented with 10 mM -glycerophosphate and 0.1% 2-mercaptoethanol. Plates were
rocked for 15 min, and the collected lysates were cleared by centrifugation for 15 min at 12,000 rpm. Proteins were separated using 10% polyacrylamide gels and sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE). They were then
transferred to nitrocellulose for immunoblotting. Nitrocellulose
blots were blocked in PBS/0.5% Tween-20/4% nonfat dry milk
for 1 h. Tyrosine phosphorylated proteins were detected using
4G10 monoclonal antibody, goat antimouse HRP conjugate, and
ECL. Dual phosphorylation of ERK1 and 2 was detected by exposing blots to phospho-ERK1 and 2 polyclonal antibody for 2 h,
followed by goat anti-HRP-conjugated antibody for 30 min, and
then reagents for ECL. To assess total amounts of ERK1 and 2, regardless of their phosphorylation states, we stripped the same
blots and then probed them a second time using an anti-ERK1
and 2 polyclonal antibody, followed by goat antirabbit HRP conjugate and reagents for ECL. The intensity of protein bands on
autoradiograms was quantitated using NIH-Image 1.61 software
(National Institutes of Health, Bethesda, MD).
ERK2 Activity Assay
To confirm that the newly phosphorylated ERK proteins also
possessed increased kinase activity after exposure to mitogens, we immunoprecipitated them from cellular lysates and measured their ability to phosphorylate myelin basic protein (MBP), as described previously (19). The antibody we identified as suitable for
immunoprecipitation of dog ERK (C-14; Santa Cruz Biotechnologies) appeared to capture only ERK2 from our lysates (see RESULTS). For these experiments, cells were grown to confluence in
12- or 24-well plates, washed once with PBS, and then starved for
24 h in M199 media containing 0.5% FCS. After stimulation, media were removed and cells were washed twice with ice-cold PBS,
then lysed in Triton X-100 lysis buffer. Lysates were cleared by
centrifugation at 12,000 rpm to remove insoluble material. Aliquots of cleared lysates, each containing 100 to 150 µg protein,
were incubated overnight at 4°C with 3 µg polyclonal goat anti-ERK2 antibody followed by a 2-h incubation with 10 µl of a 50%
slurry of protein G-agarose. Immune complexes were washed
four times and assayed for kinase activity in 25 mM Tris (pH
7.0) containing 0.7 mM ethyleneglycol-bis-(-aminoethyl ether)-
N,N'-tetraacetic acid and 0.33 mg/ml MBP. Reactions were initiated by the addition of 35 mM magnesium acetate and 35 µM adenosine triphosphate (ATP) (1 µCi 
-32P ATP). After a 30-min
incubation at 30°C, the assay was terminated by pipetting 40 µL
of the reaction mixture onto circles of P81 phosphocellulose paper and immersing the papers in 0.5% phosphoric acid. Papers
were washed four times with phosphoric acid and once with acetone before drying and counting using liquid scintillation photometry.
Measurement of c-fos Transcript
We used polymerase chain reaction (PCR) to identify and quantify c-fos transcript in our cells. After exposure of the cells to mitogens, we isolated RNA from them, and synthesized complementary DNAs (cDNAs) for use as templates in PCR. For these experiments, subconfluent cells in six-well plates were exposed to mitogens, and media were removed by gentle aspiration before addition of 0.5 ml RNazol B per well. Total (nuclear and cytoplasmic) RNA was isolated as described previously (20) except that the chloroform concentration was increased 3-fold. RNA concentration was determined by absorption at 260 nm. Single-stranded cDNAs were synthesized from the RNA using MMLV-RT. Each reaction was carried out in 20 µl containing 2 µg RNA as template, deoxynucleotide triphosphates (dNTPs) (0.6 mM each per reaction), random hexamers (50 ng per reaction), RNAsin (20 U per reaction), 50 mM Tris (pH 8.3), 3 mM MgCl2, 75 mM KCl, and 10 mM dithiothreitol. Reverse transcription was at room temperature for 10 min, followed by 42°C for 45 min, with 200 U of MMLV-RT. Subsequent heat inactivation of the transcriptase was for 5 min at 95°C.
The sequences of oligonucleotides used for PCR were obtained from published gene sequences for human fos (21) and rat
-actin (22) genes. The c-fos primers were as follows: the 5'
primer, complementary to nucleotides 1910 to 1939, lying within
exon 3 of the human c-fos gene, was 5'-GAATAAGATGGCTGCAGCCAAATGCCGCAA; and the 3' primer, corresponding
to nucleotides 2230 to 2259 of exon 4 was 5'-CAGTCAGATCAAGGGAAGCCACAGACATCT. The predicted amplimer sizes
for human cDNA and DNA, respectively, were 236 and 352 base pairs (bp). -Actin primers were as follows: the 5' primer, complementary to nucleotides 3119 to 3136, was 5'-CCGCAAATGCTTCTAGGC; and the 3' primer, corresponding to nucleotides 3774 to 3754, was 5'-GGTCTCACGTCAGTGTACAGG.
The predicted product size for rat cDNA was 656 bp.
In preliminary PCR experiments, reactions were optimized for primer pair concentrations, annealing temperatures, and Mg2+ concentrations to produce the greatest yield of product with the least loss of specificity. In other preliminary experiments, concentrations of input cDNA were decreased by serial dilution to define a linear range of product amplification. Similarly, reactions were subjected to 20 to 40 cycles of amplification to determine a linear range, which occurred for both primer pairs between 25 and 28 cycles. Therefore, we employed 26 cycles for all subsequent experiments. A total of 15% of the reverse-transcribed cDNA was added to a reaction mixture containing 10 mM Tris (pH 8.0), 50 mM KCl, 1 to 4 mM MgCl2, dNTPs (0.2 mM each), 5' and 3' primers (0.2 to 0.6 µM each, 10 to 30 pmols per reaction), and 2.5 units Taq DNA polymerase (final volume, adjusted with distilled water: 50 µl). Reaction mixtures were heated to 94°C for 5 min before the addition of Taq DNA polymerase, and then were overlaid with light mineral oil. Incubations in a DNA thermal cycler for 26 cycles of PCR amplification were as follows: denaturation for 100 s at 95°C, annealing for 70 s at 56°C, and extension for 100 s at 72°C. PCR-generated DNA bands were detected by electrophoresis on a 2% agarose gel in 0.04 M Tris acetate containing 1 mM EDTA. Gels were electrophoresed at 10 V/cm for approximately 60 min, then stained with ethidium bromide.
The identity of the c-fos PCR amplimer was confirmed by sequence analysis. The amplified c-fos cDNA was ligated into pCR2.1, which was used to transform Escherichia coli. Several clones were sequenced using the dideoxy chain termination method and Sequenase T7 DNA polymerase.
Photographs of PCR amplimers in agarose gels were made
and video images were obtained and stored using a OneScanner
gel documentation system and Ofoto software (Apple Computer,
Inc., Cupertino, CA). The bands of interest were scanned and peak
areas and mean intensities were determined using NIH-Image
1.55 software (Wayne Rasband, National Institutes of Health).
Total pixel intensity for each band was determined as the mean
intensity multiplied by the area. Background pixel intensity was
subtracted from signal-associated total pixel intensity, giving the
background-corrected pixel intensity. Background-corrected pixel
intensity for c-fos was normalized to the background-corrected
pixel intensity for -actin in the analysis of the results of each
experiment. The normalized relative intensities are plotted as
means ± standard error of the mean (SEM) (n = 3 or more per
treatment group). The data were analyzed using an unpaired t test
of Sigma STAT (Jandel Scientific, San Rafael, CA).
| |
Results |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
Concentration Dependence of Mitogen-Induced Increases in DNA Synthesis
Tryptase and PDGF caused potent, concentration-dependent effects on DNA synthesis in our cells (Figure 1). In all subsequent experiments comparing effects of tryptase with those of PDGF, we used concentrations of the two mitogens that were approximately equipotent and induced 30 to 60% increases in DNA synthesis relative to those produced by 10% FCS. The concentrations of the two mitogens inducing these degrees of DNA synthesis differed somewhat in different preparations of cells.
|
Attenuation of Tryptase-Induced DNA Synthesis by Irreversible Serine Protease Inhibition
In 10 experiments, pretreatment with p-APMSF (final concentration: 10 µM) always inhibited the amidolytic activity of tryptase (final concentrations: 2.1 to 5.4 nM) for GPK substrate by 99% or more (data not shown). Using the same assay, we demonstrated that this degree of inhibition persisted for at least 24 h under the conditions of the DNA synthesis assay. Treatment with p-APMSF attenuated tryptase-induced increases in DNA synthesis by 76.8 ± 6.4% but did not significantly alter responses to PDGF (Figure 2).
|
Mitogen-Induced Increases in ERK1 and 2 Phosphorylation
Antiphosphotyrosine immunoblots. Exposure to tryptase for 5 or 10 min increased the phosphorylation of two protein bands on immunoblots probed with an antiphosphotyrosine-specific antibody (Figure 3A). These phosphorylated proteins ranged in size from 46 to 48 kD and 42 to 44 kD and comigrated with ERK1 and 2 as identified on the same immunoblots using a polyclonal anti-ERK1 and 2 antibody (data not shown). PDGF treatment increased tyrosine phosphorylation of the same two proteins. PDGF increased tyrosine phosphorylation of many other proteins, as expected, and equipotent concentrations of tryptase had much more limited effects (Figure 3A). Intensities of the ERK1 and 2 bands, expressed as percent increases over controls, are shown in Figure 3B. Concentrations of tryptase and PDGF that were approximately equipotent in terms of their effects on DNA synthesis caused increases in ERK tyrosine phosphorylation which differed in two respects, depending on the mitogen. First, tryptase caused much smaller increases than PDGF. Second, there was a suggestion that the intensity of the bands induced by tryptase was increased at 10 compared with 5 min, whereas the intensity of PDGF-induced bands were either unchanged or decreased at 10 compared with 5 min (Figure 3B).
|
Anti-phospho-ERK immunoblots. MEK maximally activates ERK1 and 2 by phosphorylating both threonine and tyrosine in a TEY sequence of the ERK proteins (11). Using an anti-phospho-ERK antibody developed to detect these phosphorylated residues, we identified two bands corresponding to phospho-ERK1 and 2 in cellular lysates. Tryptase-induced threonine and tyrosine phosphorylation of ERK1 and 2 was reduced after pretreatment of the tryptase with p-APMSF (Figure 4). In five separate experiments, the reduction in phospho-ERK by pretreatment with p-APMSF was 57.6 ± 9.8% for ERK1 and 37.6 ± 6.9% for ERK2 (mean ± SEM).
|
Figure 5 shows the results of time-course experiments in which cells were exposed to tryptase or PDGF for 0 to 120 min before lysis and immunoblotting as shown in Figure 4. At baseline (time 0), ERK2 phosphorylation (Figure 5, bottom) was present even before mitogen addition but ERK1 phosphorylation was not (Figure 5, top). The kinetics of responses to the two mitogens were quite different. For PDGF, responses were near maximal at 5 min. This maximal level of stimulation persisted for 10 to 15 min and then decreased promptly to near control levels by 60 min. For tryptase, the onset of phosphorylation was delayed and did not reach a maximum until 15 min. For the remainder of the 120-min period, responses to tryptase were sustained and remained significantly above control levels, even at 120 min.
|
Mitogen-Induced Increases in ERK2 Activity and Their Attenuation by MEK1 Inhibition
ERK activity was assessed directly in immunoprecipitates prepared from cell lysates using an antibody recognizing a carboxy terminal epitope of rat ERK2. In several species, this antibody also cross-reacts with ERK1. However, no ERK1 was detected in our immunoprecipitates on blots probed with the anti-ERK1 and -ERK2 polyclonal antibody. Therefore, the precipitating rat ERK2 antibody appeared selective for canine ERK2 and our assay provides a selective measure of ERK2 activity. Treatment of cells with 50 to 100 ng/ml PDGF (approximately 2 to 4 nM) induced 8.1 ± 2.3- and 7.5 ± 2.3-fold increases in ERK2 activity at 5 and 10 min, respectively (Figure 6A). In other experiments, we found that tryptase-induced increases in ERK2 kinase activity were sustained at 30 and 60 min when compared with 15 min (Figure 6B). By contrast, responses to PDGF at 30 and 60 min clearly were decreased compared with 15 min (Figure 6B). Tryptase (3 to 10 nM) increased ERK2 activity by 2.3 ± 0.6- and 3.8 ± 0.7-fold above basal values at 5 and 10 min, respectively (Figure 6A). Because ERK1 and 2 are activated by the dual-specificity kinases MEK1/2 (11), the perturbation of MEKs by PD098059, a specific inhibitor (13) of MEK1 and 2, should attenuate ERK activity in this assay. As shown in Figure 7, pretreatment of cells with PD098059 before their exposure to tryptase or PDGF significantly inhibited basal and mitogen-induced ERK2 activities in lysates prepared from these cells.
|
|
MEK1/2 Inhibition Reduces Tryptase-Stimulated DNA Synthesis
PDGF-BB and tryptase-induced increases in BrdU incorporation were largely abolished by pretreatment of cells with the MEK1/2 inhibitor PD098059 (Figure 8). Pretreatment of cells with 50 µM PD098059 inhibited BrdU incorporation induced by tryptase (2.3 to 9.9 nM) or PDGF (100 ng/ml) by 102.4 ± 6.1 and 89.8 ± 7.3%, respectively (means ± SEM, n = 6 and 9 experiments for the two mitogens, each performed in triplicate). Responses to 10% FCS were not affected (Figure 8).
|
Mitogen-Induced Increases in c-fos Transcript
Figure 9 shows the electrophoresis of the DNA generated
by RT-PCR which produced bands of sizes predicted from
the published c-fos and -actin gene sequences (21, 22).
Cloning and sequencing of DNA in the band generated
with the c-fos primers indicated that, in the 236-bp amplified region of this gene, the dog c-fos product was 98 and
100% identical to human c-fos in nucleotide and amino acid
sequence, respectively. To test for differences in RNA integrity and efficiency of the RT reactions, RT-PCR for -actin also was carried out. Assuming that -actin was
equally expressed under all conditions and time points, we
normalized the RT-PCR-amplified c-fos signal to the -actin
signal. PDGF increased the normalized c-fos transcript by
greater than 12-fold after 30 min, nearly equivalent to the
increases induced by 10% fetal bovine serum (FBS) (data
not shown). By comparison, tryptase increased c-fos transcript by only about 2-fold. Further, the peak response to
PDGF occurred at 30 min and declined sharply by 75 min
(Figure 9B), whereas the response to tryptase was highest at 75 min, remained high at 180 min, and declined toward
baseline at 360 min (Figure 9A).
|
| |
Discussion |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
Thickening of the airway wall is a characteristic finding in asthma that relates in part to hyperplasia of airway smooth-muscle cells (7). This change in the airway wall contributes importantly to the development of bronchial hyperresponsiveness because the thickening gives rise to exaggerated decreases in airway caliber when the smooth muscle shortens (7). Tryptase is released in airways during allergen challenge in atopic subjects (1) and is present in increased concentrations in induced sputum samples obtained from patients with asthma (1). Approximations of in vivo tryptase concentrations in bronchi are possible, based on estimates of mast cell numbers in the smooth-muscle layer and of tryptase concentrations per mast cell (4). Over this range of estimated nanomolar concentrations, we have previously demonstrated that tryptase is a mitogen in cultured dog (4) and human (23) airway smooth-muscle cells. The major new finding of the current study is that tryptase activates the ERK class of MAP kinases in these cells and that these proteins likely are important second messengers for tryptase-induced mitogenesis. In addition, our time-course experiments demonstrated striking differences between tryptase and PDGF in both the early and sustained phases of ERK activation (Figure 5). Tryptase's effects on ERK activation depended in part upon its properties as a protease, but our experiments demonstrated a substantial proportion (40 to 60%) mediated via nonproteolytic mechanisms. Although prior studies have not always shown complete inhibition of tryptase's effects by protease inhibitors (2, 6), our findings constitute the first clear demonstration, to our knowledge, that nonproteolytic actions may contribute importantly to tryptase's activation of cells.
Our experiments provide several different lines of evidence for tryptase-induced activation of ERK1 and 2, including increased tyrosine phosphorylation (Figure 3), specific dual phosphorylation of threonine 202 and tyrosine 204 in ERK1 and 2 (Figure 4), and ERK2 activity in immunoprecipitates (Figure 6). The findings add tryptase to the
growing list of airway smooth-muscle mitogens for which
ERK activation has been demonstrated, and these include PDGF (14), insulin-like growth factor-1 (12), epidermal
growth factor (12), endothelin (24), thrombin (25), and -hexosaminidase (26). Thus, ERKs are likely a part of a pathway shared by multiple smooth-muscle mitogens acting via
different receptors.
Despite the relatively similar increases in DNA synthesis ultimately induced by tryptase and PDGF, the time courses of ERK activation in response to tryptase and PDGF differed from one another in several respects over the 2 h they were assessed in our study (Figure 5). The response to tryptase was slower in onset, reaching a peak at about 15 min, as compared with 5 min for PDGF (Figure 5). Similar differences in the onset kinetics were suggested in our analysis of the antiphosphotyrosine immunoblots (Figure 3) and measured ERK2 activities (Figure 6A). In addition, increases in c-fos transcripts were delayed in onset in response to tryptase compared with PDGF (Figure 9), indicating that the differences in ERK1 and ERK2 kinetics were also reflected in the downstream activation of an important early response gene (15).
To our knowledge, few other investigators have reported differences in the time to achieve maximum ERK
activation under different experimental conditions in other
cells. However, in one study, trypsin induced brisk increases
in ERK activity (peaking at 5 min) in rat aortic smooth
muscle cells, and this effect of trypsin was mediated via direct activation of PAR-2 (27). In the same study, in bovine
pulmonary arterial fibroblasts, peak ERK activation by
trypsin was delayed and did not occur until 15 min; the
mechanism for trypsin-induced ERK activation in these
cells is unknown but was independent of PAR-2. In our
experiments, the delay in tryptase-induced ERK activation
may be evidence against direct activation of a cell-surface
receptor and may reflect, instead, a multiple-step requirement for cellular activation. Examples of such multiple-step processes include proteolytic cleavage of factors in the media, releasing their growth-promoting activity for the smooth-muscle cells, or proteolytic liberation from extracellular
matrix of factors, such as transforming growth factor- or
fibroblast growth factors, which in turn may activate their
own receptors on the smooth-muscle cells. Our findings indicate the need for more information about the earliest
events that occur during tryptase's activation of cells in
airways and lung.
Another difference in the time courses of ERK phosphorylation by tryptase versus PDGF in our experiments was the more sustained response to tryptase. Thus, at 60 to 120 min after addition of the mitogens, ERK1 and 2 phosphorylation in response to PDGF had returned nearly to baseline levels, whereas responses to tryptase still were elevated well above those levels (Figure 5). Measurements of ERK2 kinase activity confirmed our observations that responses to tryptase were more sustained than to PDGF (Figure 6B). We can only speculate as to possible mechanisms contributing to these differences. The ERK activation state at any time is the net effect of activating kinases and inactivating protein phosphatases. Tyrosine- and threonine-phosphorylated sites on ERK1 and 2 are susceptible to the actions of phosphatases in cytosolic and nuclear compartments (28). Some immediate early genes encode dual specificity MAP kinase phosphatases (MKPs) that inactivate ERK by dephosphorylating both threonine and tyrosine residues. In fibroblasts, MKP-1 messenger RNA was induced in 15 min in response to serum (29). Thus, in our cells, it is possible that PDGF exposure leads to early increases in ERK phosphatase activity but that tryptase either fails to induce these effects or does so more slowly. Inhibitory feedback mechanisms may also modulate the kinetics of intracellular signaling, and activated ERK has been shown to phosphorylate Son of sevenless (SOS) and to disassociate the Grb2-SOS complex involved in Ras activation (30). In our experiments, differences in the importance of such feedback regulation of the Grb2-SOS complex and Ras activation during PDGF- and tryptase-induced ERK activation might account for the observed differences in kinetics. In a Chinese hamster ovarian fibroblast cell line, angiotensin II induced a sustained phase of ERK activity via 12-lipoxygenase activation (31). Whether such a mechanism accounts for tryptase's sustained activation is unknown.
In some previous studies, sustained ERK activation appeared vital for growth stimulation. For instance, in CCL39 cells, thrombin caused both peak and sustained activation of ERK1 (32) and the sustained activation correlated best with the degree of mitogenicity. However, in other cells, thrombin induced a brisk and only transient activation of ERK that was followed by potent mitogenic effects (33). The finding in our experiments that concentrations of tryptase and PDGF which induced comparable increases in DNA synthesis caused quite different degrees of late-phase ERK activation would suggest that sustained ERK activation was not a requirement for induction of potent mitogenic effects in our cells. However, the 2-h period of our observations is not sufficient to make firm conclusions about this issue. Also, the fact that PDGF-stimulated levels of ERK1 and 2 phosphorylation at 60- and 120-min time points still were slightly above basal (Figure 5) may have been an important determinant of growth responses to this mitogen.
Our conclusion that ERK activation is required for tryptase-induced mitogenesis rests on the observed inhibitory effects on tryptase-induced BrdU incorporation of PD098059 (Figure 8). This compound is a cell-permeable inhibitor of MEK1 and 2 (13), the kinases just upstream from ERKs that dually phosphorylate and activate them (11). The strength of this evidence depends on the specificity of PD098059 effects; and support for a high degree of specificity, in the concentrations employed in our experiments, is emerging on the basis of findings in both airway smooth-muscle cells (14) and other systems (13). However, the definitive demonstration of a requirement for ERK activation would necessitate using other experimental approaches, including transient transfections with cDNAs encoding dominant-negative MEK1 or ERKs (14). Also, our experiments provide no information about the degree to which ERK activation alone is sufficient in mediating tryptase's growth-stimulatory effects and no information about the potential importance of other pathways, such as activation of phosphatidylinositol 3-kinase, in mediating these effects. The failure of PD098059 to completely inhibit the mitogenesis induced by 10% FBS in our experiments (Figure 8) is consistent with the compound's reported inability to attenuate extremely potent degrees of MEK1 activation in intact cells (13, 24), perhaps because of its low solubility in aqueous solutions making it difficult to achieve high intracellular concentrations (13).
Our experiments with the irreversible serine protease inhibitor p-APMSF demonstrated that substantial portions of the responses to tryptase were mediated via proteolytic cleavage by its catalytic site. On the other hand, approximately 25% of tryptase-induced increases in DNA synthesis (Figure 2) and 40 to 60% of the peak increases (at 15 min) in ERK1 and 2 phosphorylation (Figure 5) persisted after treatment of the tryptase with p-APMSF. It is possible but unlikely that these latter effects related to the 1% or less residual catalytic activity in p-APMSF-treated tryptase. Also, it is important to note that although the majority of thrombin's mitogenic effects are mediated via proteolytic mechanisms (33), there is strong evidence that noncatalytic portions of the thrombin molecule also can induce mitogenesis (10). Similarly, it is possible that tryptase's effects in our cells related to both catalytic and noncatalytic effects of the molecule. An interaction of tryptase's glycosyl residues (34) with glycoprotein receptors on the smooth-muscle cell is one noncatalytic effect that might lead to growth stimulation, particularly because glycoprotein receptor activation clearly can induce mitogenesis in airway smooth-muscle cells (26). Also, we cannot exclude with absolute certainty the presence of a contaminant in our preparations of human lung tryptase that serves as an important cofactor with tryptase during ERK activation. However, the purity of the human lung tryptase preparations used in our experiments has been characterized extensively using chromatographic, electrophoretic, and immunologic criteria (3). Tryptase from another source, HMC-1 cells (35), also has potent mitogenic effects in our cells (current authors' unpublished observations), and it is somewhat unlikely that an important contaminating cofactor would be common to two preparations isolated by such different techniques.
In summary, our experiments demonstrate that tryptase activates MAP kinases of the ERK class in airway smooth-muscle cells and that this signaling pathway is likely important in stimulating DNA synthesis in these cells. We have developed a new technique for irreversible inhibition of tryptase's catalytic activity using p-APMSF. Our findings indicate that, although full degrees of ERK activation and increased DNA synthesis in response to tryptase require an intact catalytic activity, substantial portions of these responses likely are mediated via noncatalytic effects. Our experiments also demonstrated striking differences in the kinetics of tryptase- versus PDGF-induced ERK activation. These findings suggest the need for more information about the earliest events at the cell membrane which mediate tryptase's mitogenic effects and about the significance of transient versus sustained ERK activation in response to different mitogens.
| |
Footnotes |
|---|
Address correspondence to: James K. Brown, M. D., Pulmonary and Critical Care Medicine Section (111-D), Dept. of Veterans Affairs Medical Center, 4150 Clement St., San Francisco, CA 94121. E-mail: jkbrown{at}itsa.ucsf.edu
(Received in original form March 9, 2000 and in revised form October 19, 2000).
Acknowledgments: This work was supported by the Research Service of the Department of Veterans Affairs and NIH-NHLBI Grant HL-24136.
Abbreviations BrdU, bromodeoxyuridine; cDNA, complementary DNA; ECL, enhanced chemiluminescence; ERK, extracellular signal-regulated protein kinase; FBS, fetal bovine serum; FCS, fetal calf serum; GPK, N-p-tosyl-Gly-Pro-Lys p-nitroanilide; HRP, horseradish peroxidase; MAP, mitogen-activated protein; MEK, MAP kinase kinase; MMLV, Maloney murine leukemia virus; p-APMSF, p-amidino phenylmethanesulfonyl fluoride; PAR, protease-activated receptor; PBS, phosphate-buffered saline; PCR, polymerase chain reaction; PDGF, platelet-derived growth factor; RT, reverse transcriptase; SEM, standard error of the mean; SOS, Son of sevenless.
| |
References |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
1. Schwartz, L. B.. 1994. Tryptase: a mast cell serine protease. Methods Enzymol. 244: 88-100 [Medline].
2. Ruoss, S. J., T. Hartmann, and G. H. Caughey. 1991. Mast cell tryptase is a mitogen for cultured fibroblasts. J. Clin. Invest. 88: 493-499 .
3.
Hartmann, T.,
S. J. Ruoss,
W. W. Raymond,
K. Seuwen, and
G. H. Caughey.
1992.
Human tryptase as a potent, cell specific mitogen: role of signaling
pathways in synergistic responses.
Am. J. Physiol. (Lung Cell. Mol. Physiol.)
262:
L528-L534
4. Brown, J. K., C. L. Tyler, C. A. Jones, S. J. Ruoss, T. Hartmann, and G. H. Caughey. 1995. Tryptase, the dominant secretory granular protein in human mast cells, is a potent mitogen for cultured dog tracheal smooth muscle cells. Am. J. Respir. Cell Mol. Biol. 13: 227-236 [Abstract].
5. Cairns, J. A., and A. F. Walls. 1996. Mast cell tryptase is a mitogen for epithelial cells: stimulation of IL-8 production and intracellular adhesion molecule-1 expression. J. Immunol. 156: 275-283 [Abstract].
6. Blair, R. J., H. Meng, M. J. Marchese, S. Ren, L. B. Schwartz, M. G. Tonnesen, and B. L. Gruber. 1997. Human mast cells stimulate vascular tube formation. J. Clin. Invest. 99: 2691-2700 [Medline].
7. James, A. L., P. D. Pare, and J. C. Hogg. 1989. The mechanics of airway narrowing in asthma. Am. Rev. Respir. Dis. 139: 242-246 [Medline].
8.
Akers, I. A.,
M. Parsons,
M. R. Hill,
M. D. Hollenberg,
S. Sanjar,
G. J. Laurent, and
R. J. McAnulty.
2000.
Mast cell tryptase stimulates human lung
fibroblast proliferation via protease-activated receptor-2.
Am J. Physiol.
(Lung Cell. Mol. Physiol.)
278:
L193-L201
9.
Dery, O.,
C. U. Corvera,
M. Steinhoff, and
N. W. Bunnett.
1998.
Proteinase-activated receptors: novel mechanisms of signaling by serine proteases.
Am. J. Physiol.
274:
C1429-C1452
10. Schaeffer, P., E. Riera, E. Dupuy, and J. Herbert. 1997. Nonproteolytic activation of the thrombin receptor promotes human umbilical vein endothelial cell growth but not intracellular Ca2+, prostacyclin, or permeability. Biochem. Pharmacol. 53: 487-491 [Medline].
11. Garrington, T., and G. Johnson. 1999. Organization and regulation of mitogen-activated protein kinase signaling pathways. Curr. Opin. Cell Biol. 11: 211-218 [Medline].
12.
Kelleher, M.,
M. Abe,
T.-S. O. Chao,
M. Jain,
J. Green,
J. Solway,
M. Rosner, and
M. Hershenson.
1995.
Role of MAP kinase activation in bovine
tracheal smooth muscle mitogenesis.
Am. J. Physiol. (Lung Cell. Mol. Physiol.)
268:
L894-L901
13.
Alessi, D. R.,
A. Cuenda,
P. Cohen,
D. T. Dudley, and
A. R. Saltiel.
1995.
PD 098059 is a specific inhibitor of the activation of mitogen-activated
protein kinase in vitro and in vivo.
J. Biol. Chem.
270:
27489-27494
14.
Karpova, A.,
M. Abe,
J. Li,
P. Liu,
J. Rhee,
W.-L. Kuo, and
M. Hershenson.
1997.
MEK1 is required for PDGF-induced ERK activation and DNA synthesis in tracheal myocytes.
Am J. Physiol.
272:
L558-L565
15.
Chen, R.,
C. Abate, and
J. Blenis.
1993.
Phosphorylation of the c-fos transrepression domain by mitogen-activated protein kinase and 90-kDa ribosomal S6 kinase.
Proc. Natl. Acad. Sci. USA
90:
10952-10956
16. Tom-Moy, M., J. M. Madison, C. A. Jones, P. de Lanerolle, and J. K. Brown. 1987. Morphologic characterization of cultured smooth muscle cells isolated from the tracheas of adult dogs. Anat. Rec. 218: 313-328 [Medline].
17. Laura, R., D. J. Robison, and D. H. Bing. 1980. (p-Amidinophenyl)methanesulfonyl fluoride, an irreversible inhibitor of serine proteases. Biochemistry 19: 4859-4864 [Medline].
18. Yung, Y., Y. Dolginov, Z. Yao, H. Rubinfeld, D. Michael, T. Hanoch, E. Roubini, Z. Lando, D. Zharhary, and R. Seger. 1997. Detection of ERK activation by a novel monoclonal antibody. FEBS Lett. 408: 292-296 [Medline].
19. Alessi, D. R., P. Cohen, A. Ashworth, S. Cowley, S. J. Leevers, and C. J. Marshall. 1995. Assay and expression of mitogen-activated protein kinase, MAP kinase kinase, and Raf. Methods Enzymol. 255: 279-290 [Medline].
20. Chirgwin, J. M., A. E. Pryzbyla, R. J. MacDonald, and W. J. Rutter. 1979. Isolation of biologically active ribonucleic acid from sources enriched in nuclease. Biochemistry 18: 5294-5299 [Medline].
21. Irving, J., J. Feng, C. Einstrom, M. Pikaart, and B. Villeporteau. 1992. An altered repertoire of fos/jun (AP-1) at the onset of replicative senescence. Exp. Cell Res. 202: 161-166 [Medline].
22.
Mullhaupt, B.,
A. Feren,
E. Fodor, and
A. Jones.
1994.
Liver expression of
epidermal growth factor RNA.
J. Biol. Chem.
269:
19667-19670
23. Brown, J. K., C. A. Jones, G. H. Caughey, and I. P. Hall. 1997. Mast cell tryptase is the dominant mitogenic serine protease for human and dog airway smooth muscle cells. Am. J. Respir. Crit. Care Med. 155: A905 .
24. Whelchel, A., J. Evans, and J. Posada. 1997. Inhibition of ERK activation attenuates endothelin-stimulated airway smooth muscle cell proliferation. Am. J. Respir. Cell Mol. Biol. 16: 589-596 [Abstract].
25.
Shapiro, P.,
J. Evans,
R. Davis, and
J. Posada.
1996.
The seven-transmembrane-spanning receptors for endothelin and thrombin cause proliferation
of airway smooth muscle cells and activation of the extracellular regulated
kinase and c-jun NH2-terminal kinase groups of mitogen-activated protein
kinases.
J. Biol. Chem.
271:
5750-5754
26.
Lew, B.,
B. Dempsey,
Y. Zhao,
M. Muthalif,
S. Fatima, and
K. Malik.
1999.
-Hexosaminidase-induced activation of p44/p42 mitogen-activated protein kinase is dependent on p21 ras and protein kinase C and mediates bovine airway smooth-muscle proliferation.
Am. J. Respir. Cell Mol. Biol.
21:
111-118
27. Belham, C. M., R. J. Tate, P. H. Scott, A. D. Pemberton, H. R. P. Miller, R. M. Wadsworth, G. W. Gould, and R. Plevin. 1996. Trypsin stimulates proteinase-activated receptor-2-dependent and -independent activation of mitogen-activated protein kinase. Biochem. J. 320: 939-946 .
28. Keyse, S. M.. 1998. Protein phosphatases and the regulation of MAP kinase activity. Cell Dev. Biol. 9: 143-152 .
29.
Iyer, V. R.,
M. B. Eisen,
D. T. Ross,
G. Schuler,
T. Moore,
J. C. F. Lee,
J. M. Trent,
L. M. Staudt,
J. Hudson Jr.,
M. S. Boguski,
D. Lashkari,
D. Shalon,
D. Botstein, and
P. O. Brown.
1999.
The transcriptional program in the response of human fibroblasts to serum.
Science
283:
83-87
30.
Chen, D.,
S. B. Waters,
K. H. Holt, and
J. E. Pessin.
1996.
SOS phosphorylation and disassociation of the Grb2-SOS complex by the ERK and JNK
signaling pathways.
J. Biol. Chem.
271:
6328-6332
31.
Wen, Y.,
J. Nadler,
N. Gonzales,
S. Scott,
E. Clauser, and
R. Natarajan.
1996.
Mechanisms of ANG II-induced mitogenic responses: role of 12-lipoxygenase and biphasic MAP kinase.
Am. J. Physiol.
271:
C1212-C1220
32.
Meloche, S.,
K. Seuwen,
G. Pages, and
J. Pouysségur.
1992.
Biphasic and
synergistic activation of p44mapk (ERK1) by growth factors: correlation between late phase activation and mitogenicity.
Mol. Endocrinol.
6:
845-854
33.
Trejo, J.,
A. J. Connolly, and
S. R. Coughlin.
1996.
The cloned thrombin receptor is necessary and sufficient for activation of mitogen-activated protein kinase and mitogenesis in mouse lung fibroblasts.
J. Biol. Chem.
271:
21536-21541
34. Miller, J. S., G. Moxley, and L. B. Schwartz. 1990. Cloning and characterization of a second complementary DNA for human tryptase. J. Clin. Invest. 86: 864-870 .
35. Butterfield, J. H., D. A. Weiler, L. W. Hunt, S. R. Wynn, and P. E. Roche. 1990. Purification of tryptase from a human mast cell line. J. Leukoc. Biol. 47: 409-419 [Abstract].
This article has been cited by other articles:
 |
|
 |
|
  B. Riteau, C. de Vaureix, and F. Lefevre Trypsin increases pseudorabies virus production through activation of the ERK signalling pathway. J. Gen. Virol., May 1, 2006; 87(Pt 5): 1109 - 1112. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 J. K. Brown, M. D. Hollenberg, and C. A. Jones Tryptase activates phosphatidylinositol 3-kinases proteolytically independently from proteinase-activated receptor-2 in cultured dog airway smooth muscle cells Am J Physiol Lung Cell Mol Physiol, February 1, 2006; 290(2): L259 - L269. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
J. Hjoberg, L. Le, A. Imrich, V. Subramaniam, S. I. Mathew, J. Vallone, K. J. Haley, F. H. Y. Green, S. A. Shore, and E. S. Silverman Induction of early growth-response factor 1 by platelet-derived growth factor in human airway smooth muscle Am J Physiol Lung Cell Mol Physiol, April 1, 2004; 286(4): L817 - L825. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 A. L. Lazaar, M. I. Plotnick, U. Kucich, I. Crichton, S. Lotfi, S. K. P. Das, S. Kane, J. Rosenbloom, R. A. Panettieri Jr., N. M. Schechter, et al. Mast Cell Chymase Modifies Cell-Matrix Interactions and Inhibits Mitogen-Induced Proliferation of Human Airway Smooth Muscle Cells J. Immunol., July 15, 2002; 169(2): 1014 - 1020. [Abstract] [Full Text] [PDF]
|
|
| ||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
| Proc. Am. Thorac. Soc. | Am. J. Respir. Crit. Care Med. |