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Gene Induction during Differentiation of Human Pulmonary Type II Cells In Vitro

Department of Pediatrics, Division of Neonatology, the Children's Hospital of Philadelphia; and Section of Thoracic Surgery, Department of Surgery, University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania

Correspondence and requests for reprints should be addressed to Philip L. Ballard, M.D., Ph.D., Children's Hospital of Philadelphia, 416 Abramson Research Center, 3516 Civic Center Boulevard, Philadelphia, PA. E-mail: ballardp{at}email.chop.edu

	Abstract

Top Abstract Introduction MATERIALS AND METHODS RESULTS DISCUSSION References

 
Mature alveolar type II cells that produce pulmonary surfactant are essential for adaptation to extrauterine life. We profiled gene expression in human fetal lung epithelial cells cultured in serum-free medium containing dexamethasone and cyclic AMP, a treatment that induces differentiation of type II cells. Microarray analysis identified 388 genes that were induced > 1.5-fold by 72 h of hormone treatment. Induced genes represented all categories of molecular function and subcellular location, with increased frequency in the categories of ionic channel, cell adhesion, surface film, lysosome, extracellular matrix, and basement membrane. In time-course experiments, self-organizing map analysis identified a cluster of 17 genes that were slowly but highly induced (5- to 190-fold) and represented four functional categories: surfactant-related (SFTPC, SFTPA, PGC, SFTPB, LAMP3, LPL), regulatory (WIF2, IGF2, IL1RL1, NR4A2, HIF3A), metabolic (MAOA, ADH1B, SEPP1), and transport (SCNN1A, CLDN18, AQP4). Induction of both mRNA and protein for these genes, which included nine newly identified regulated genes, was confirmed, and cellular localization was determined in both fetal and postnatal tissue. Induction of lysosomal-associated membrane protein 3 required both hormones, and expression was localized to limiting membranes of lamellar bodies. Hormone-induced differentiation of human type II cells is associated with genome-wide increased expression of genes with diverse functions.

Key Words: cyclic AMP • epithelial differentiation • glucocorticoid • human fetal lung • type II cell

	Introduction

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Pulmonary type II cells have a number of known physiologic functions. During lung development, they are the progenitor cell for type I cells that constitute the gas exchange surface in alveoli. After lung injury, type II cells proliferate to repopulate the pulmonary epithelium. These cells participate in transepithelial movement of sodium and water to clear fetal lung fluid at birth and to maintain alveolar fluid homeostasis with air breathing. Type II cells produce a variety of cytokines, chemokines, and other proteins involved in the inflammatory response, as well as proteins that have either immunomodulary or antioxidant roles. The most specialized function of type II cells is the production and secretion of surfactant, the complex mixture of lipid and surfactant proteins (SPs) that maintains alveolar stability and is required for successful adaptation to extrauterine life (1–3).

Differentiation of type II cells from undifferentiated precursor epithelial cells is marked by the disappearance of glycogen, which serves as a substrate for surfactant phospholipid synthesis, the formation of lamellar bodies, which are the intracellular storage sites for secreted surfactant, and expansion of the apical cell surface in the form of microvilli (4–7). A number of classes of proteins are developmentally increased during type II cell differentiation, including SPs, lipogenic enzymes, selected water and ion transporter/channels, metabolic enzymes, and structural proteins (8).

Studies of alveolar type II cell differentiation in cultured fetal lung explants and in vivo indicate that both glucocorticoids and cyclic AMP (cAMP) are important agents in the maturational process (5–9). Hormone treatment of explants or epithelial cells from second trimester human fetal lung results in differentiation of type II cells that contain lamellar bodies and secrete surface-active surfactant. A limited number of glucocorticoid-regulated genes have been identified (7, 8). In general, hormonally induced genes are also developmentally regulated, consistent with the view that glucocorticoid treatment causes precocious maturation and mimics the role of endogenous corticosteroids in lung development. In a survey of hormonal responses in fetal lung epithelial cells, most ( 90%) induced genes responded to both glucocorticoid and cAMP in either an additive or synergistic manner (7). Although many of the recognized inductive responses to glucocorticoid/cAMP exposure occur in lung epithelial cells, mesenchymal fibroblasts are also target cells for these hormones, and mesenchymal–epithelial interactions are important in lung development (10). Other reported regulators of lung development include thyroid hormones, epidermal growth factor, gastrin-releasing peptide, IL-1, and parathyroid hormone-related peptide; however, there is limited information regarding target genes for these agents (11).

Primary culture of fetal lung epithelial cells is a useful model system for examining changes in gene expression during type II cell differentiation. In this experimental approach, an enriched population of epithelial cells, isolated from second trimester human fetal lung tissue, is cultured in serum-free medium containing dexamethasone and 8-bromoadenosine 3',5'-cAMP (8-Br-cAMP) (7). Within 4 d, many of the hormone-treated cells develop intracellular lamellar bodies and secrete surface-active surfactant in response to secretagogues; cells cultured without hormones do not undergo differentiation. We previously used DNA microarray analysis to generate an initial, limited survey of regulated genes after 3 d of hormone-induced type II cell differentiation in vitro (7). In the present study, we have expanded the survey and analysis of induced genes and profiled gene expression at time points during the process of type II cell differentiation. We have analyzed the chromosomal distribution of induced genes and determined categories of the encoded proteins with regard to their molecular function and subcellular location. A cluster of 17 known genes that were highly induced contained 9 newly identified, hormonally responsive genes. Preliminary results have been published as an abstract (12).

	MATERIALS AND METHODS

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Cell Culture
We isolated enriched populations of epithelial cells from second trimester human fetal lung tissue under institutional review board–approved protocols, as previously described (6). After overnight culture (Day 1), we cultured the cells for an additional 3 d in serum-free Waymouth's medium alone (control), or with dexamethasone (10 nM)/8-Br-cAMP (0.1 mM)/isobutylmethylxanthine (0.1 mM) (DCI), or with dexamethasone or 8-Br-cAMP/isobutylmethylxanthine separately. These concentrations maximally induce surfactant components in human lung explant cultures (9). For time-course experiments, cells were collected at 4, 8, 24, 48, and 72 h after addition of DCI or diluent (control). Epithelial cell purity by this procedure was 86 ± 2% (n = 6), with fibroblasts as the primary contaminating cell type (6, 7).

DNA Microarray Analysis
Total RNA was extracted from control and DCI-treated cells and converted to biotin-labeled cRNA using Affymetrix reagents (Affymetrix, Santa Clara, CA) and protocol. Biotin-labeled cRNA was hybridized to U133A Affymetrix microarray chips that contain 16–20 unique 25 mer oligonucleotide probes for 14,500 human genes plus corresponding 12–16 probes with a single nucleotide change (mismatch control). U133A hybridization, washing, staining, and scanning were performed by the Stokes Research Institute Nucleic Acid Core Facility using procedures described in the Affymetrix GeneChip Expression Analysis technical manual. A total of 18 chips were analyzed with cells cultured from 13 individual lungs. Gender was known for seven lungs (four female and three male). For studies of DCI effects at 72 h, a total of 10 chips (5 control and 5 DCI-treated) were used. In the first two experiments (4 chips) RNA was prepared from cells isolated from individual specimens of lung tissue (13- and 14-wk gestation) that were cultured in the presence or absence of DCI. In an additional three experiments (6 chips), equal amounts of RNA from 72-h control and DCI-treated cells (derived from 3–4 different lungs for each pool, 16- to 20-wk gestation) were pooled for analysis. To study the time course of gene induction, cells from 4 individual lung specimens (all 18-wk gestation) were cultured in the presence of DCI or Waymouth's media for 4, 8, 24, 48, and 72 h, and equal amounts of RNA from each experiment were pooled for analysis with 2 chips (DCI and control) used at each time point; data from the 72-h point in this experiment represent 1 of the 3 RNA pools noted previously here. RNA from all 13 cell preparations was analyzed by dot-blot hybridization, as previously described (7), to confirm induction of SP-B mRNA after 72 h DCI treatment. The strategy of pooling of RNA samples from separate experiments for microarray analysis has been found not to affect the inference for most genes (13).

Affymetrix Microarray Suite 5.0 was used to quantitate and analyze mRNA content for expressed genes. Default values provided by Affymetrix were applied to all analysis parameters. Probes for 70 control genes on each chip were used to normalize fluorescence intensity between chips, and arrays were scaled to an average intensity of 1,500 fluorescence units and analyzed independently. For very-low-abundance mRNAs in control cells (< 20 fluorescence units), a value of 20 units was assigned. The Microarray Suite software uses Wilcoxon's signed rank tests to evaluate whether a transcript is detectable on the array (present, marginal, absent), and the probability of a significant change between arrays (i.e., DCI-treated versus control), assigning P values and a change call (increase, decrease, no change) for each probe. For the current analysis, induced genes were defined as those that were detected as present and increased (DCI-treated for 72 h versus control) in all 5 experiments, with P < 0.003 for at least four experiments and a mean fold induction > 1.5-fold. We also determined q values for the entire data set using QVALUE software (available online at http://genomine.org/qvalue). This analysis indicated that induced genes met a false discovery rate of < 0.025 (14). When more than one probe set was present for the same gene, data were combined to provide a mean value. Fold-stimulation results are expressed as mean ± SE.

Database Analyses
We used databases and software in the public domain to compare various properties of induced genes of fetal epithelial cells with human genomic data. Distribution of induced genes among chromosomes (as % of chromosomal genes represented on the chip) and close clustering of induced genes was determined using data extracted from the NCBI website (available online at www.ncbi.nlm.nih.gov/mapview/maps.cgi?ORG=humandMAPS=ideogr,cntg,ugHs,genesandCHR=1).

The molecular function and subcellular location of induced genes was determined from the Swiss-Prot database (available online at http://us.expasy.org/sprot/sp-docu.html), and the relative distribution of genes between categories was compared with data for all human entries in this database (10,125 at the time of analysis). Subcellular location was primarily a single designation in this database, whereas multiple terms were generally assigned for gene molecular function.

Clustering Analysis for Self-Organizing Maps
GeneCluster 1.0 from the Whitehead Institute/Massachusetts Institute of Technology Center for Genome Research (available online at: http://www.genome.wi.mit.edu/cancer/software.html) was used to cluster differentially expressed genes in the time course by self-organizing maps (SOM). Cluster analysis was restricted to the 5,570 probes on U133A that met the following two criteria by Microarray Suite 5.0 analysis: (1) the probe was designated as "present" on at least one chip in the time course studies; and (2) in comparative analysis between control and DCI-treated cells, the probe was designated either "increased" or "decreased" for at least one time point. For our SOM analysis, we used a 6 x 4 matrix and the default settings of the software to create 24 patterns of gene expression.

Real-Time RT-PCR
RNA was prepared using RNA STAT (Tel-Test, Inc., Friendswood, TX) per the manufacturer's instructions. Samples were then treated with RQ1 RNase-free DNase (Promega, Madison, WI) and ethanol precipitated after phenol-chloroform extraction. Integrity, purity, and concentration were confirmed using an Agilent 2,100 bioanalyzer (Agilent Technologies, Palo Alto, CA) in the Nucleic Acid Core Facility at Children's Hospital of Philadelphia. cDNA was synthesized from 2 µg RNA samples using the SuperScript First-Strand RT-PCR kit (Invitrogen, Carlsbad, CA), according to the manufacturer's instructions. Real-time PCR reactions using a singleplex format were performed with an ABI Prism 7,000 (Applied Biosystems, Foster City, CA) in the Real-Time PCR Core Facility of the Children's Hospital of Philadelphia. We used the standard PCR protocol recommended by the manufacturer of Assay-on-Demand kits (Applied Biosystems, Foster City, CA). The specific primer and probe sequences are available from the authors on request. The assays were determined to be in the linear amplification range in each experiment using cDNA standards derived from RNA of cells treated for 5 d with DCI.

Antibodies
Antibodies were obtained from the following sources and used for immunofluorescence staining (dilutions shown) and Western analysis: lipoprotein lipase (LPL; 1:100, monoclonal clone 5D2; gift of J. Brunzell, University of Washington, Seattle); alcohol dehydrogenase (ADH; 1:250, monoclonal; Research Diagnostics, Inc., Flanders, NJ); Wingless-Int (Wnt) inhibitory factor-1 (WIF-1; 1:100, goat polyclonal; R&D Systems, Minneapolis, MN); epithelial sodium channel (ENaC; 1:200, rabbit polyclonal; Alpha Diagnostic International, San Antonio, TX); IL-1 receptor-like (IL1RL1, IL-1R4, ST2; 1:200, goat polyclonal; R&D Systems); monoamine oxidase (MAO; 1:500, chicken polyclonal; US Biological, Swampscott, MA); Aquaporin 4 (AQP4; 1:1000, rabbit polyclonal; US Biological); hypoxia-inducible factor 3 (HIF3; 1:100; Novus Biologicals Inc., Littleton, CO); lysosomal-associated membrane protein 3 (LAMP3, dendritic cell (DC)-LAMP, CD208; 1:250, monoclonal; Immunotech, Marseille, France); insulin-like growth factor (IGF)-II (1:100, goat polyclonal; R&D Systems); nuclear-related receptor 1 (Nurr-1, NR4A2; 1:1000, rabbit polyclonal; Santa Cruz Biotechnology, Santa Cruz, CA). Antibodies that failed to give positive immunostaining results with cultured lung cells were as follows: IGF-II (rabbit polyclonal; Chemicon International, Inc, Temecula, CA); WIF-1 (polyclonal; Santa Cruz Biotechnology); selenoprotein P (monoclonal; BD Transduction Laboratories, San Diego, CA).

Western Analysis
We performed immunoblotting using previously described procedures (7) and NuPAGE Bis-Tris gels with MES (2-[morpholino] ethane sulfonic acid) SDS Running Buffer, per the manufacturer's protocol (Invitrogen, Carlsbad, CA). Proteins were transferred to Duralose membrane (Stratagene, La Jolla, CA) and probed with primary antibodies and appropriate horseradish peroxidase–tagged secondary antibody. Signal was detected using the enhanced chemiluminescence kit (SuperSignal West PICO kit; Pierce, Rockford, IL) and blots exposed to Kodak Biomax MS film (Eastman Kodak Co., Rochester, NY). Films were scanned with an Agfa Argus II scanner and FotoLook SA scanning software on a Macintosh G4 computer (Apple Computer, Inc., Cupertino, CA). Semiquantitative densitometric analysis was done using MacBAS version 4.2, after background subtraction.

Immunofluorescence
Lung tissue (fetal uncultured or after explant culture, or normal human infant 1–3 mo of age) was fixed in cold 1% paraformaldehyde, washed in 1 mM NH₄Cl in PBS followed by cold PBS, then cryoprotected by 5% sucrose in PBS, and embedded in Tissue Freezing Medium (Triangle Biomedical Sciences, Durham, NC); 5 µm frozen sections were prepared for immunostaining. Isolated epithelial cells were cultured on glass coverslips for cell culture (Fisher Scientific, Pittsburgh, PA), then fixed with cold methanol (–20°C) and permeabilized with 0.3% Triton X-100 before immunostaining, as previously described (7). Secondary antibodies for immunofluorescence detection were tagged with Alexa 488 or Cy3 and used at 1:200 or 1:300. After immunostaining, some sections were exposed to 4', 6-diamidino-2-phenylindole (0.1 µg/ml, Molecular Probes, Eugene, OR) for 10 min to stain nuclei.

In Situ Hybridization
Nonisotopic in situ hybridization on frozen sections was performed with fetal lung tissue (uncultured or after explant culture) that was fixed in cold 1% paraformaldehyde and embedded in tissue freezing medium. Sections (10 µm) were fixed in 4% paraformaldehyde, treated with proteinase K, and then refixed in paraformaldehyde, acetylated, and dehydrated. Antisense probes (2.5 µg), prepared using the Dig RNA Labeling kit (Roche, Indianapolis, IN) were diluted in 1 ml hybridization solution, placed on each slide, and incubated overnight at 70°C. After hybridization, slides were washed briefly in 5x SSC and high-stringency wash solution and then treated with RNase A. Slides were blocked with 1% Blocking Reagent (Roche) and incubated overnight at 4°C with alkaline phosphatase–coupled sheep anti-digoxigenin Fab fragments (Roche) diluted 1:5,000 in 1% Blocking Reagent in 1x PBS-0.1% Tween. Alkaline phosphatase activity was detected by incubation in 5-bromo-4-chloro-3-indolyl phosphate/nitro blue tetrazolium mixture for 24–72 h. The slides were counterstained with Nuclear Fast Red (Sigma, St. Louis, MO), allowed to air-dry, and mounted with VectaMount (Vector Laboratories, Burlingame, CA). Slides were examined with an Olympus 1X70 microscope (Olympus, Melville, NY) and Metamorph imaging system (Universal Imaging, West Chester, PA).

	RESULTS

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Number of Induced Genes
To assess the overall profile of gene expression in differentiated fetal lung epithelial cells, we identified those transcripts that were scored as "present" in cells treated with DCI for 72 h using the U133A Affymetrix microarray chip, which contains 22,500 probes for 14,500 human genes (available online at www.affymetrix.com). There were 8,453 mRNAs that were identified as present in each of five experiments. Because of redundancy in probe sets, the 8,453 mRNAs likely represent 5,450 separate gene transcripts. Assuming that the gene probes on this chip are representative of all the named human genes, we estimate that 38% of the human genome is expressed at detectable levels in fetal lung epithelial cells after 72 h of DCI treatment.

Analysis of microarray data for 5 experiments, representing 13 different fetal lungs between 13- and 20-wk gestation, revealed that 388 mRNAs were reproducibly induced > 1.5-fold by 72 h of DCI treatment compared with control cells. This represents 2.7% of the genes that are probed by the chip and 7.1% of the genes that are expressed at a detectable level in these cells. Of the 388 induced genes, 350 encode for proteins of currently known or putative function, and the remaining 38 genes are currently described as expressed sequence tags (ESTs) or encoding unknown proteins. The list contains 78 genes that we previously identified using a first-generation microarray chip (Affymetrix HuFL) containing probes for 5,500 human genes (7). The full list of induced genes is provided online at http://stokes.chop.edu/web/neoresearch, and original data for gene expression profiling after 72-h hormone exposure are deposited at the Gene Expression Omnibus (accession number GSE3306) at the National Center for Biotechnology Information (available online at www.ncbi.nih.gov). Downregulated genes, which are not a focus of this report, are included at the Gene Expression Omnibus website.

Chromosomal Locus of Induced Genes
The chromosomal locus was known for 377 genes induced by 72-h DCI exposure. Induced genes were localized to each of the chromosomes, except for chromosome Y, at a mean frequency of 1.1% (range 0.4–2.1%). The U133A chip has 42 probes for Y chromosome genes, representing 19% of genes currently assigned to the Y chromosome. It is possible that the failure to detect reproducibly induced genes of the Y chromosome reflects a relative scarcity of male lungs in the specimens studied.

Induced Genes Related to Phospholipid Biosynthesis
Hormone treatment of fetal lung cells increases the synthetic rate and content of phosphatidylcholine (PC) and alters the molecular composition of both PC and phosphatidylinositol (7). Accordingly, we examined induced genes of known protein function for those involved in phospholipid biosynthesis. A total of 13 genes were identified that participated in uptake of lipids (4 genes), biosynthesis (7 genes), or remodeling (2 genes) of phospholipids (Figure 1). Highly induced genes included lipoprotein lipase (LPL, 13-fold), fatty acid synthase (FAS, 6-fold), glycerol kinase (GK, 5-fold), and phosphatidylglycerophosphate synthase (PGS1, 3-fold); the other genes were all induced 1.6- to 2.5-fold. In addition, there were induced genes encoding a putative membrane phospholipid transporter (ABCA3), a putative acyltransferase (FLJ12443), and five induced genes related to cholesterol uptake or synthesis (LDLR, LSS, DHCR7, DHCR24, ACAT1).

View larger version (26K): [in this window] [in a new window]   Figure 1. Induced genes in phospholipid biosynthesis. A simplified pathway of lipid uptake and biosynthesis of phosphatidylcholine and phosphatidylglycerol (PG) with induced genes is shown. Mean induction in five microarray experiments was 2-fold except for genes where the fold induction is noted. ADFP, adipose differentiation-related protein; EC, extracellular; FA, fatty acid; MGLL, monoglyceride lipoprotein lipase; PAP, phosphatidic acid phosphatase; PG-P, phosphatidylglycerol phosphate.

Time Course of Gene Expression in Response to DCI
To evaluate kinetics of gene induction, we performed an initial microarray study for control and DCI-treated cells at 4, 8, 24, 48, and 72 h. We then used GeneCluster 1.0 software to perform SOM analysis, which categorizes genes by their temporal pattern of hormone response (induced, repressed, or no change) and has been used to identify groups of regulated genes that share regulatory elements or functional relationships (15, 16). Figure 2 shows the time course for four clusters of genes with mean induction values > 1.5-fold for at least one time point. Cluster 1 contained 18 highly induced genes, including SP-A, SP-B, and SP-C, and was selected for further study and confirmation of hormonal responsiveness. Real-time RT-PCR analysis (n = 3) confirmed the time-course data obtained by microarray (Figure 2). The expression pattern of this gene cluster was distinct from other induced clusters with regard to the level of induction and the continuing increase in expression between 48 and 72 h.

View larger version (19K): [in this window] [in a new window]   Figure 2. Time course of induced gene clusters. Cells were exposed to DCI or diluent for 4, 8, 24, 48, or 72 h. Time-course data by microarray, examined by SOM analysis, revealed 4 clusters of induced genes with mean induction > 1.5-fold for at least 1 time point (dashed lines). mRNA content for the 17 genes of Cluster 1 was also determined by real-time RT-PCR analysis (solid line) and mean ± SE values (n = 3) are shown. The time-course patterns by microarray and RT-PCR were comparable for both mean values and for individual genes (not shown), with all genes demonstrating continued induction between 48 and 72 h.

Western analysis confirmed that DCI treatment increased protein expression for 5 of the 11 newly identified genes of Cluster 1 (Figure 3). The increases were in the 2- to 4-fold range for LPL, ENaC, WIF-1, and ADH, and higher (22-fold) for IL1RL1 (ST2), which was faintly detected in control tissue and strongly present after DCI treatment. IL1RL1 (ST2) protein was only detected in DCI-treated lung explants (row 2) and not in epithelial monolayer cultures, perhaps reflecting protein abundance and stability to enzymatic digestion of lung tissue. WIF-1 from DCI-treated cells migrated slightly slower than for control, perhaps reflecting a hormone effect on posttranslational modification as well as gene expression. One or more available antibodies for MAO, HIF3, AQP4, LAMP3 (DC-LAMP), IGF-II, and NR4A2 were tested, but failed to detect specific bands at the expected locations on protein blots.

View larger version (94K): [in this window] [in a new window]   Figure 3. Western blot analysis of LPL, IL1RL1, ENaC, WIF-1, and ADH. Undifferentiated epithelial cells were isolated from individual fetal lung specimens and cultured in control media or DCI to promote differentiation. Equal amounts of protein from total cell extracts of control and DCI-treated cells were run on SDS-PAGE gels, blotted to Duralose, and incubated with primary antibodies. For IL1RL1 (row 2), hormone treatment was performed with fetal lung explants due to lack of immunoreactivity with sonicates of monolayer cells. Representative blots from two experiments are shown. Bands of the expected molecular size were detected for LPL (58 kD), IL1RL1 (72 kD), ENaC (74 kD), WIF-1 (42 kD), and ADH-1 (39 kD). In 3–5 experiments, mean ± SE values for fold-induction by densitometric scanning were: LPL, 2.3 ± 0.5; IL1RL1, 21.6 ± 2.4; ENaC, 3.3 ± 0.4; WIF-1, 4.3 ± 1.1; and ADH, 1 2.3 ± 0.2.

View larger version (88K): [in this window] [in a new window]   Figure 4. Immunostaining of highly induced proteins in fetal lung explants. Human fetal lung (16- to 19-wk gestation) was cultured as explants for 5 d in control or DCI media, fixed, and frozen sections of each group (uncultured, control, DCI-treated) were placed on the same slide for processing with each antibody as described in MATERIALS AND METHODS. Uncultured tissue is in the left panel of each row (a, d, g, j, m, p, s, v, y), control tissue at 5-d culture is in the middle panel (b, e, h, k, n, q, t, w, z), and DCI-treated tissue is shown in the right panel (c, f, i, l, o, r, u, x, aa). Results were similar with three separate lung specimens, and representative staining is shown. For each of the proteins, uncultured tissue showed low to absent immunostaining. Fluorescence signal was also low for control tissue, except for somewhat increased signal with AQP4, IL1RL1, HIF3, MAO, and ADH; HIF3 staining in control explants was restricted to the mesenchyme. For all antibodies, staining was most intense for tissue cultured in DCI and was localized to epithelial cells, except for ADH (primarily mesenchymal) and HIF3 (epithelial and mesenchymal). Different patterns of epithelial cell staining are evident: cytoplasmic (LAMP3, HIF3, MAO), basal (LPL), basolateral (ENaC, AQP4), apical (IL1RL1, NR4A2). Arrows indicate epithelial cells. A, alveolar space; m = mesenchyme.

View larger version (103K): [in this window] [in a new window]   Figure 5. Immunofluorescence staining of postnatal lung for proteins of Cluster 1. Frozen sections of postnatal lung (1–3 mo normal infant) were immunostained as described for fetal lung explants (Figure 4). The staining patterns for most genes were similar to those observed in the explants. LPL and AQP4 staining localized to epithelial cell membranes with areas of stronger intensity; the pattern of DC-LAMP was consistent with restricted type II cell expression; NR4A2, ENaC, and weak punctate HIF3 staining appeared to be cytoplasmic in epithelial cells; and ADH staining occurred primarily in mesenchymal cells. Staining of postnatal tissue was not detected for MAO and IL1RL1 under the conditions used. Nonspecific staining (not shown) was consistently low for postnatal tissue.

View larger version (74K): [in this window] [in a new window]   Figure 6. Fluorescence immunostaining of fetal lung cells in monolayer culture. Control Day 5 cells are in the left panel of each pair (a, c, e, g, i, k, m) and DCI-treated cells are in the right panel of each pair (b, d, f, h, j, l, n). Control and treated cells for each antibody were photographed under identical exposures to allow direct comparison of staining intensities, and representative images from three or more lungs are shown. LPL immunostaining was greater in DCI-treated cells (b) compared with control cells (a), and was detected as punctate cytoplasmic staining. AQP4 stained minimally in control cells (c) and intensely stained the epithelial plasma membrane (pm) in treated cells (d). LAMP3 showed minimal staining of control cells (e) and intense perinuclear, punctate staining in treated cells (f). (g and h) HIF3 staining overlayed with 4', 6-diamidino-2-phenylindole staining (blue) of nuclei. Staining occurred in intranuclear loci, consistent with nucleoli, in both control (g) and DCI-treated cells (h), as well as diffuse cytoplasmic staining, especially in DCI-treated cells. ADH showed intense generalized cytoplasmic staining in mesenchymal cells in both control (i) and DCI-treated (j) epithelial cells, with some staining of epithelial cells. IGF2 showed a modest increase in staining of DCI-treated cells (l) with a perinuclear vesicular pattern. NR4A2 staining was weak in control cells (m), with increased intensity in the cytoplasm of DCI-treated cells (n). N, nucleus; LB, lamellar bodies; FB, fibroblast; E, epithelial cell.

View larger version (122K): [in this window] [in a new window]   Figure 7. In situ hybridization for WIF1, MAO, and IGF2 expression. Human fetal lung (16- to 19-wk gestation; n = 3) was cultured as explants for 5 d in control or DCI media. Explant tissue was fixed, and frozen sections from each group (uncultured, control, DCI-treated) were placed on the same slide for processing with each probe. Uncultured tissue is in the left panel of each row (a, d, g), control tissue at 5 d culture is in the middle panel (b, e, h) and DCI-treated is in the right panel (c, f, i). WIF1, MAOA, and IGF2 were all expressed to the highest degree in epithelial cells of DCI-treated explants (c, f, i). IGF2 was the only one of these messages expressed in the cells prior to culture, whereas MAOA showed some expression after culture in the absence of DCI, and WIF1 was expressed only in DCI-treated explants.

View larger version (15K): [in this window] [in a new window]   Figure 8. Properties of hormone-induced DC-LAMP gene expression. (A) Exposure of cells to DCI increased DC-LAMP mRNA in a linear fashion between 8 and 72 h of exposure, as assessed by both cDNA microarray (RNA pooled from cells of 4 lungs) and qPCR in a separate representative experiment. (B) DC-LAMP protein increased progressively between 12 and 72 h of DCI exposure compared with control cells. Values are mean ± SEM (n = 5). The inset shows a representative Western blot for DCI exposure plus lanes for control cells ("C") at 12 and 72 h. (C) Exposure to DCI, but not to dexamethasone or cAMP alone, induced DC-LAMP protein. The inset shows a blot from a representative experiment. Detection of DC-LAMP staining was performed with the Supersignal West Femto-ECL detection reagent. Values are mean ± SE for three experiments. *P < 0.05 versus control; **P < 0.05 versus 24 h DCI.

View larger version (51K): [in this window] [in a new window]   Figure 9. Induction of DC-LAMP in epithelial cells by confocal immunofluorescence microscopy. Isolated cells were cultured from Days 1 to 5 in the absence (control, lower panels) or presence of DCI (upper panels) and stained for DC-LAMP (left panels; 1:100 dilution) and SP-B (center panels; 1:100 dilution), and the images were overlayed (right panels). The yellow color of the overlayed image shows colocalization of the DC-LAMP and SP-B in vesicles (e.g., lamellar bodies) surrounding the nuclei (dark). A higher power confocal microscopy (6,300x) image of lamellar bodies (LB, far-right panel) shows localization of DC-LAMP (red) in lamellar body membranes surrounding SP-B (green) staining within lamellar bodies.

	DISCUSSION

Top Abstract Introduction MATERIALS AND METHODS RESULTS DISCUSSION References

DNA microarray approaches have been used in other studies to assess differential gene expression in lung tissue and cells under various conditions. Recent reports describe changes in gene expression in response to transforming growth factor- treatment of lung fibroblasts (20), effects of treatment of newborn mice with dexamethasone and retinoic acid (21), changes in gene expression during development of mouse lung (22), and effects of phosphorylation status of TTF-1 (23). In the dexamethasone study (21), a significant difference in gene expression was detected for 499 genes of 12,000 queried—a percentage comparable to that for induced plus repressed genes in our study.

There are some limitations to both the experimental model and microarray methodology used in this study. Hormonal treatment of fetal lung cells in primary culture may not completely replicate type II cell differentiation as occurs in vivo. However, several lines of evidence support the appropriateness of this culture system as a model for in vivo lung development. Key lipogenic enzymes are induced, PC synthesis increases with a shift in composition toward that of mature surfactant, content of SPs increases many-fold, the cells develop lamellar bodies, and surface-active surfactant is secreted in response to secretagogue treatment (6, 7). Collectively, these responses represent a coordinated, precocious expression of the surfactant system. In addition, there is induction of a number of other nonsurfactant-related genes (e.g., SCNN1A, ATP1B1, ATP1A1, FASN) whose expression is known to increase during type II cell differentiation in vivo (8). A more definitive assessment of the cultured cell model and profile of induced genes will be provided by a future study comparing gene expression in cultured fetal versus mature type II cells obtained from postnatal lung specimens. The study is also limited by conditions inherent to microarray analysis (e.g., false discovery rate) and by the number of lungs and chips used, which suggests caution in interpreting global expression results (e.g., enrichment of functional categories).

DNA microarray technology is a powerful tool for quantitative analysis of gene expression on a nearly genome-wide basis. Nevertheless, there are a number of caveats associated with this experimental approach that may lead to false-positive or false-negative results for changes in gene expression. Genes that are targeted by more than one probe set, which was 35% of the induced genes in this study, are less susceptible to errors for these reasons. Microarray data require confirmation by other measurements of mRNA content. Because protein levels do not always mimic changes in RNA levels, protein confirmation and immunohistochemistry are valuable. In our study, induction of all 17 genes of known function in Cluster 1 was confirmed by real-time RT-PCR. Induction was also found by Western analysis and/or immunostaining for 16 of 17 genes examined. The failure to confirm immunoreactive selenoprotein P, which has been previously detected in lung tissue (24), could reflect inappropriate specificity of the antibody used, low abundance of the protein, or induced transcription without increased translation.

We found 13 induced enzymes or transporters related to synthesis of PC and phosphatidylglycerol, key phospholipids of surfactant, with only one gene (LPL) included in Cluster 1. Hormonal induction of some of the biosynthetic proteins (fatty acid synthase, choline phophotransferase, stearoyl–coenzyme A desaturase) has been previously described (8, 25). It is noteworthy that molecules involved in lipid uptake (LPL, monglyceride lipoprotein lipase, LDL receptor, membrane phosphatidic acid phosphatases, and adipose differentiation-related protein) or with a putative transport function (ABCA3) are hormonally responsive, as determined by microarray analysis, suggesting that the increased production of surfactant phospholipids involves enhanced uptake of extracellular substrate as well as increased synthetic activity. Induction of LPL is consistent with a model in which fibroblasts store triglyceride that is then provided to epithelial cells (26).

When gene expression was analyzed over time, SOM analysis revealed a variety of kinetic patterns, likely reflecting, in part, both primary and secondary hormone responses. A cluster of 17 genes of known function, including the SP genes, was upregulated after 4- to 8-h lag period to relatively high levels of expression by 72 h. As coordinate regulation of genes can indicate regulatory or functional relationships, some of the newly identified genes of this cluster may have key roles in the type II cell. The cluster contains eight genes (SFTPA, SFTPB, SFTPC, PGC, IGF2, SCNN1A, AQP4, CLDN18) that are known to be hormonally responsive in fetal lung (6–9, 17, 18, 27, 28). Although SFTPD was also induced by DCI, the time course of expression and fold induction differed from the other SPs and, therefore, it clustered with another group of induced genes. PGC encodes pepsinogen C, also referred to as gastricsin, which is an aspartic protease and member of the pepsin family that is type II cell specific and may have a role in SP-B processing (17). The function of IGF-II in alveolar epithelial cells may relate to cell proliferation. SCNN1A and AQP4 both function in alveolar fluid homeostasis (27). DCI treatment also increased expression of SCCN1B, but expression of the subunit was not detected. Of the nine AQP genes probed by the chip, expression was detected for only AQP3 and AQP4. The tight-junction protein, claudin 18, is involved in paracellular ion permeability and epithelial cell barrier function, and induction of claudin 18 is associated with changes in transepithelial resistance of type II cell monolayers (18).

In addition, Cluster 1 contains 9 newly identified, regulated genes of fetal lung epithelial cells. Seven genes (LAMP3, LPL, MAOA, WIF1, HIF3A, SEP1, and ADH1B) have been detected in the lung, including three (LAMP3, LPL, MAOA) in type II cells; LAMP3 has been previously localized to lamellar bodies. Three of these genes (LPL, MAOA, ADH1B) are hormonally regulated in other tissues. In lung cells, we found that ADH1B was responsive only to dexamethasone, three genes (WIF1, NR4A2, HIF3A) were induced by cAMP but not by dexamethasone, and the other five genes were regulated by an interaction of glucocorticoid and cAMP. The pattern of hormonal responsiveness for gene induction emphasizes the physiologic importance of both glucocorticoid and cAMP in differentiation of type II cell function as well as ultrastructure (7). Mechanistically, the variety of hormone responses rules out the possibility that the genes of Cluster 1 are all regulated by a common pathway (e.g., hormonally induced transcription factor).

LPL, which hydrolyses serum lipoprotein triglycerides, has been detected previously in lung tissue, and its activity increases after birth in temporal association with increased numbers of lipofibroblasts (26, 29). We report the new observation that LPL is hormonally regulated in the lung similar to previous findings in selected other tissues, such as adipocytes (30). Immunostaining indicated localization of LPL to type II cells, with basolateral expression as required for hydrolysis of triglycerides derived from serum or adjacent fibroblasts.

LAMP account for about half of the total lysosomal membrane protein. The newest member of this family, LAMP3 (also referred to as DC-LAMP/CD208) (31), has been previously identified in lung tissue and localized to lamellar bodies of mouse type II cells (32). We found that DC-LAMP was highly induced by combined hormone treatment in differentiating human type II cells. Moreover, DC-LAMP was localized exclusively to limiting membranes of lamellar bodies in a pattern identical to that for ABCA3 (33). LAMP1 and LAMP2 were also expressed in the human fetal lung cells, but were not affected by hormone treatment. A role for DC-LAMP in surfactant modification and/or in secretion has been proposed (32).

WIF1 encodes an inhibitor of Wnt proteins, a large family of secreted signaling molecules that interact with the receptor Frizzled and regulate nuclear transcription through the action of -catenin (34). Targeted deletion of -cateninin in mouse lung epithelial cells at < E15 results in a more proximal epithelial cell phenotype and decreased branching of secondary bronchi (35). In murine fibroblasts, WIF1 is strongly induced during BMP-2-mediated osteoblast differentiation (19). Our data represent the first description of WIF1 expression in human fetal lung epithelial cells and its hormonal responsiveness. This finding is consistent with a role for Wnt signaling in lung development.

HIF3A was a highly induced gene in cAMP-treated lung cells. HIF1A was also induced (1.7-fold) by DCI treatment; however, transcripts for the HIF-associated proteins pVHL (von Hippel-Lindau tumor suppressor protein) and ARNT (aryl hydrocarbon receptor nuclear translocator) were expressed at low levels in the cells and were not induced. HIF-3 has been previously described in adult lung, where it is greatly increased by hypoxia, induces angiogenesis factors, and triggers proliferation of pulmonary vascular smooth muscle cells (36, 37). A possible role for HIF3 in the developing lung is to facilitate induction of angiogenesis coordinately with alveolization.

Novel IL-1 receptor–like genes, including IL1RL1 (T1/ST2), IL-1 receptor–related protein and IL-1 receptor–related protein 2, comprise a cytokine receptor gene cluster at chromosome locus 2q12 (38). We found synergistic induction of IL1RL1 during type II cell differentiation; in addition, IL1R1 was induced (2.2-fold), whereas IL1R2 and IL1RN (receptor antagonist) transcripts were not detected. Although there has been extensive study of IL1RL1 isoforms in hematopoietic cells, the precise role of IL1RL1/ST2 in human lung type II epithelial cells is unknown.

The NR4A2 gene encodes a member of the nuclear receptor superfamily known as nuclear-related receptor 1, a transcription factor that has been shown to regulate midbrain development, in particular dopaminergic neurons, and aldosterone synthesis in the adrenal cortex (39). Expression of NR4A2 has been described in rat lung (40), and we report responsiveness to cAMP, suggesting a possible role in cell differentiation.

ADH and monamine oxidases are nicotinamide adenine dinucleotide oxidoreductases that catalyze metabolism of alcohols and biogenic amines, respectively. Class I ADHs are expressed in a variety of tissues with epithelial localization (41). By contrast, we found that immunoreactivity localized predominantly to lung fibroblasts with the one antibody available for study. ADH is glucocorticoid responsive in hepatocytes (42); however, there are no previous reports of glucocorticoid regulation of ADH1B in the lung. Of the different ADH genes surveyed, only the isoform of Class I ADH was induced. Increased ADH activity could provide glycerol as substrate for phospholipid synthesis or promote production of retinoic acid from retinol (41). Retinoic acid has a number of effects in the developing lung, including coactivation of the SP-B gene, promotion of phospholipid synthesis, and enhancement of alveolization (43–45).

We found that the MAO-A, but not MAO-B (not detected), was induced in lung cells and was localized to epithelial cells by immunofluorescence. Both isozymes are expressed in a variety of tissues, including the adult lung, where MAO-A is the more abundant form and localizes to the alveolar wall and smooth muscle cells (46). Induction of both ADH and MAO-A are consistent with upregulated catecholamine metabolism at the airway surface and/or essential housekeeping oxidoreductase functions in lung cells preparatory to the availability of oxygen at birth.

The time-course study also identified a subset of induced genes that were maximally upregulated soon after hormone treatment. It is likely that transcription factors in this subset are primary hormonal targets (versus being induced secondarily by other induced factors) and potential mediators of hormonal effects on other genes. Current studies are investigating the role of two of these factors, TTF-1 and "homeodomain-only" protein (HOP), in type II cells. Our findings indicate that while TTF-1 is required for DCI-induction of many genes, an increase in TTF-1 alone induces only a small subset of genes, implicating a role for other hormone-induced regulatory factors. HOP is regulated by TTF-1 and appears to act as a negative regulator of SP gene expression (V.K., unpublished data). Future studies will focus on the role of other induced transcriptional regulators during type II cell differentiation.

	Acknowledgments

 
The authors thank S. Angampalli, P. Wang, and P. Zhang for technical assistance, E. Rapaport for assistance and advice in microarray hybridization and data analysis, and T. Ferguson and C. Dennis for editorial assistance.

	Footnotes

 
This work was supported by National Institutes of Health grants HL56401 (L.W.G., S.H.G., and P.L.B.), HL59959 (S.H.G.), HL19737 (P.L.B. and J.G.) and the Gisela and Dennis Alter Endowed Chair in Pediatrics (P.L.B.).

This article has an online supplement, which is accessible from this issue's table of contents at www.atsjournals.org

Originally Published in Press as DOI: 10.1165/rcmb.2004-0389OC on February 10, 2006

Conflict of Interest Statement: None of the authors has a financial relationship with a commercial entity that has an interest in the subject of this manuscript.

Received in original form December 7, 2004

Accepted in final form January 27, 2006

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