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Gene Expression Profiling Reveals Cross-talk between Melanoma
and Fibroblasts: Implications for Host-Tumor
Interactions in Metastasis
Paul G. Gallagher,1Yongde Bao,
1Alyson Prorock,
1Paola Zigrino,
2Roswitha Nischt,
2
Vincenzo Politi,3Cornelia Mauch,
2Bojan Dragulev,
1and Jay William Fox
1
1Department of Microbiology, University of Virginia, Charlottesville, Virginia; 2Department of Dermatology, University of Cologne,Cologne, Germany; and 3Polifarma SpA, Rome, Italy
Abstract
Host-tumor interaction is considered critical in carcinogen-esis, tumor invasion, and metastasis. To explore the recipro-cal effects of host-tumor interaction, we developed a systemto assess the gene expression patterns of A2058 humanmelanoma cells cocultured in fibrillar collagen with HS-68primary human fibroblasts. The gene expression pattern ofthe cocultured A2058 cells was only modestly affected,whereas the HS-68 fibroblast gene expression pattern wassignificantly altered. Interleukin-11 and inhibitor of DNA-binding domain-1 gene expression in the cocultured A2058cells was down-regulated, indicative of a proinflammatoryresponse and resistance to apoptosis, respectively. The overallpattern of up-regulated genes indicated triggering of theproinflammatory process. In addition, the melanoma growthand migration stimulatory chemokines CXCL1 and CXCL2were significantly up-regulated in the cocultured fibroblasts.These results were corroborated by additional cocultureexperiments with the melanoma cell lines WM-164, BLM,and SK-Mel-28 and immunohistochemistry on invasive hu-man melanoma sections. Taken together, these resultsindicate that tumor cells cause a proinflammatory andmelanoma growth-promoting response in stromal fibroblasts.The role of inflammation in carcinogenesis, tumor promo-tion, invasion, and metastasis is viewed as being increasinglyimportant and the results of these studies underscore this aswell as identify certain key proteins that are expressed as aresult of the complex interactive processes in the host-tumormicroenvironment. (Cancer Res 2005; 65(10): 4134-46)
Introduction
Increasing attention is being focused on the interaction of tumorcells with the host in terms of exploring how that interaction isconducive to the induction, selection, and expansion of the tumorultimately leading to the malignant progression of the tumor (1–5).For example, studies on human breast carcinomas have shown thatvascular stroma formation occurs before invasion by tumor cells.In situ hybridization of breast carcinomas at various stagesdetected expression of vascular permeability factor and vascularendothelial growth factor, whereas the stromal cells were shown to
express thrombospondin-1, collagen type I, fibronectin, versican,and decorin, suggesting that the tumor induces vascularization inregions where they invade and host stroma promotes thisvascularization (6).The microenvironment in which host-tumor interaction occurs
has also been implicated in malignancy. The extracellular matrix(ECM) of the microenvironment is well known to regulate a varietyof cellular phenomena. Perturbation of the matrix by eitherproteolysis or alteration of its architecture due to changes inmolecular composition and/or stoichiometry resulting from host-tumor interaction can disrupt the homeostasis of the microenvi-ronment (7–9). For example, Thomasset et al. (10) have shown thatlow-level expression of the transgene matrix metalloproteinase(MMP) stromelysin-1 in mouse mammary epithelia causes an up-regulation of endogenous stromelysin-1 in fibroblasts. Thesechanges resulted in the development of preneoplastic andneoplastic lesions in mice that were associated with the up-regulation of other MMPs, ECM components, and mammary glandvascularization.The concept that inflammation plays a central role in tumor
progression has received increasing attention, particularly in thecontext of host-tumor interaction (1, 11). For example, macrophageinfiltrates of malignant melanoma have been associated withtumor stage and angiogenesis. Production of transforming growthfactor-h, tumor necrosis factor-a (TNF-a), interleukin (IL)-1a,arachidonate metabolites, and extracellular proteinases by themacrophages elicited the expression of IL-8 and vascularendothelial growth factor-A in melanocytes, thereby promotinginflammation and angiogenesis (12). Several studies have shownthat host-tumor interaction results in the production of proin-flammatory cytokines and chemokines, thereby promoting therecruitment of host leukocytes in the microenvironment of thetumor (13). However, in these investigations and most others, thereis always some question as to the cell source of the chemokinesand cytokines involved in the development of the proinflammatorypathway within the tumor microenvironment.Unlike melanocytes, melanoma cells constitutively produce a
large number of growth factors and cytokines and their respectivereceptors that enable the cells to progress to a more aggressivephenotype. Autocrine growth factors (e.g., basic fibroblast growthfactor, IL-8, and hepatocyte growth factor) stimulate proliferationand migration of melanoma cells themselves, whereas paracrinefactors (e.g., platelet-derived growth factor, transforming growthfactor-h, basic fibroblast growth factor, vascular endothelial growthfactor, and monocyte chemoattractant protein-1) are believed tomodulate the microenvironment to the benefit of melanomagrowth, invasion, and metastasis (14). On the other hand,fibroblasts are also a rich source of growth factors but only after
Note: Supplementary data for this article are available at Cancer Research Online(http://cancerres.aacrjournals.org/).
Requests for reprints: Jay William Fox, Department of Microbiology, University ofVirginia, P.O. Box 800734, Charlottesville, VA 22908-0734. Phone: 434-924-0050; Fax:434-924-2514; E-mail: [email protected].
I2005 American Association for Cancer Research.
Cancer Res 2005; 65: (10). May 15, 2005 4134 www.aacrjournals.org
activation. When stimulated by melanoma cell–released factors,they can produce growth factors (e.g., insulin-like growth factor-I,hepatocyte growth factor, and ET-3) that in turn contribute to theorchestra of virtual modulation of cellular activities (15).Several investigators have shown that host-tumor interactions
also play a crucial role in the regulation of connective tissuebreakdown in different tumors. Tumor cell–derived factors, such asextracellular MMP inducer, have been shown to be expressed byvarious tumor cells, including melanoma, and to induce productionof MMP-1, MMP-2, and MMP-3 in normal fibroblasts (16). Recently,we could show in human primary melanoma and in lymph nodemetastases that the activity of MMPs (e.g., MMP-2 and MMP-9) waslocated primarily in those areas where tumor cells lay adjacent tothe ECM or within connective tissue septa among the aggregates ofmelanoma cells (17). This observation stresses the importance ofhost-tumor interactions with structural and cellular componentsof the surrounding ECM.
In this investigation, we report the results of assays designed toassess the reciprocal effect of soluble cofactors resulting from thecoculture of human melanoma cell lines A2058, BLM, WM-164, andSK-Mel-28 with human HS-68 fibroblasts on their respective geneexpression profiles using oligonucleotide microarrays. Interestingly,the gene expression profile of the fibroblasts was dramaticallyaltered under coculture conditions, whereas the effect on themelanoma A2058 cell gene expression profile was more modest.Overall, the fibroblasts responded to coculture by up-regulation ofa variety of genes associated with the proinflammatory pathwayand cellular proliferation and this up-regulation was confirmed byquantitative real-time PCR (qRT-PCR). Several transcripts of ECMcomponents were observed to be down-regulated in coculturedfibroblasts suggesting a potential alteration of the extracellularenvironment. Furthermore, the presence of several of theseproteins was detected by immunohistochemistry of invasivehuman melanoma.
Table 1. Genes with altered expression levels in A2058 melanoma cells when grown in coculture with HS-68 fibroblasts
In summary, we observed a profound effect on the geneexpression profile of fibroblasts when in coculture with melanomacells. Analysis of the gene expression profiles indicates theinitiation of the proinflammatory pathway and an altered ECM,conditions that have been implicated in tumor progression,invasion, and metastasis. However, the response to coculture withfibroblasts by the melanoma cell line is modest. Therefore, weconclude based on this study that the stroma, due to signalsoriginating from the tumor, is primarily responsible for thegeneration of a microenvironment that is proinflammatory,proproliferation, proinvasion, and prometastatic.
Materials and Methods
HS-68 fibroblast and melanoma cell culture and RNA isolation.Human primary foreskin fibroblasts (HS-68, American Type Culture
Collection, Manassas, VA) were grown in DMEM/10% FCS, and the
melanoma cell lines A2058, BLM, WM-164, and SK-Mel-28 were grown inDMEM/10% FCS and 1 Amol/L sodium pyruvate. Fibroblasts and melanoma
cells were seeded individually during polymerization of the collagen type Ilattice and cultured on opposite sides of a 1 Am pore, six-well cell culture
by biotin-labeled cRNA synthesis using BioArray High-Yield RNA Transcript
Labeling kit (Enzo, New York, NY). cRNA was fragmented according toAffymetrix standard protocol, and fragmented cRNA (10 Ag) was hybridizedto Affymetrix Hg-U95A probe arrays for 16 hours. The arrays were washed
and stained in an Affymetrix Automated Fluidics Station 400 and scannedwith a HP GeneArray scanner.
Gene expression analysis. Scanned gene array images were first
examined for visible defects and then checked for the fitness of the
gridding. When passed, the image file was analyzed to generate compositedata files (‘‘cell files’’). From this point on, a coordination of two paths of
analysis was carried on using the Affymetrix Microarray Analysis Suite
version 5.0 and the Dchip software version 1.1 (18). The detection of a
particular gene, called ‘‘present’’, ‘‘absent’’, or ‘‘marginal’’, was made usingthe nonparametric Wilcoxon ranked score algorithm in Microarray Analysis
Suite version 5.0. Those detection calls were later imported into and used
by the Dchip program. Scatter plots were also generated using this software
to inspect the reproducibility of the replicates as well as the degree ofchanges of the samples under comparison. Quantification of gene
expression was obtained using Dchip, which applied a model-based
approach to derive the probe sensitivity index and expression index. Thetwo indices were used in a linear regression to quantify a particular gene.
When certain probes or transcripts deviated from the model to a set extent,
they were excluded from the quantification process. Normalization of the
arrays was done using the invariant set approach. Comparative analysis ofthe samples was done based on Dchip-generated fold changes and unpaired
sample t test. Typically, we considered a P of less than 0.05, a fold change
greater than 1.5 or less than �1.5, and a signal intensity difference of greater
than 100 or less than �100 as indications of significant change in geneexpression.
To aid in discovery of the potential biological processes represented by
the differentially expressed genes identified from the microarray data, theMAPPFinder program (19) was used in conjunction with GenMAPP
program (20). These programs were developed to reveal global gene
expression profiles across all areas of biology by integrating the annotation
of the Gene Ontology Project (The Gene Ontology Consortium, 2000).Briefly, the GeneChip data were reformatted to use Genbank accession
numbers as the gene identification to query the GenMAPP database. Search
terms included the possible pathways and the gene ontology terms. A Z
score is generated with each hit to indicate the strength of the associationof the cluster of genes to the gene ontology terms or pathways discovered.
For our data, we reported the genes with of a Z score equal to or greater
than 1.
Quantitative real-time PCR. Total RNA samples used in qRT-PCR werefrom the same preparations as described for the Affymetrix GeneChip
experiments. Reverse transcription was done with MultiScribe reverse
transcriptase (Applied Biosystems, Foster City, CA) and random hexamers
as per the manufacturer’s instruction. The resulting cDNA was thensubjected to qRT-PCR. For each of the transcripts of interest identified from
the GeneChip, primers were designed from the target sequences retrieved
from the Affymetrix Probe Sequence Database using the Primer Express 2.0software (Applied Biosystems). Quantitative PCRs were carried out in
triplicates using equal amounts of each cDNA sample equivalent to 50 ng of
starting total RNA. Each reaction contained the fluorescent indicator
SYBR Green I dye and 6 AL of each respective forward and reverse primer(5 Amol/L) in a total volume of 50 AL. Amplification PCR and monitoring of
the fluorescent emission in real-time were done in an ABI Prism 7900HT
Sequence Detection System (Applied Biosystems) as recommended by the
manufacturer (ABI SYBR Green Protocol). The data collected from thesequantitative PCRs defined a threshold cycle (Ct) of detection for the target
or the housekeeping genes in each cDNA sample.
To convert the Ct value into a relative abundance of target and
housekeeping gene per sample, a standard curve was generated for thehousekeeping gene using serial dilutions of cDNA sample: an arbitrary value
of template was first assigned to the highest standard and then
corresponding values were assigned to the subsequent dilutions, and theserelative values were plotted against the Ct value determined for each
dilution, resulting in the generation of the standard curve. The relative
amount of target and housekeeping genes in each sample was then
determined using the comparative Ct method (Applied Biosystems). Therelative quantity of target, normalized to an endogenous reference (usually a
housekeeping gene) and relative to a calibrator (the Rox reference dye), is
given by: relative quantity = 2� DDCt, where DDCt represents the difference
in Ct between the transcript and the housekeeping gene for the same RNAsample. The ratio of the relative quantities for the treated sample and the
experiment sample was used to derive the fold change. ANOVA was then
used to determine the mean and SE for each comparison.Immunohistochemistry. Cryosections (8 Am thick) were fixed with cold
acetone for 5 minutes and rinsed for 10 minutes in TBS. Paraffin sections
used for CD68 detection were first deparaffinized by xylol and ethanol
incubations and washed in TBS. Sections were blocked for 1 hour with 10%FCS in TBS before applying the primary antibodies diluted in TBS-FCS for
16 hours at 4jC. The sections incubated with a primary goat antibody were
also incubated with a bridging mouse anti-goat antibody (1:100, DAKO
Envision, Hamburg, Germany) for 30 minutes. After 3 � 15–minute washes,bound antibodies were detected with alkaline phosphatase–labeled anti-
mouse/anti-rabbit polymer (DAKO Envision) and neofuchsin as substrate.
Nuclei were counterstained with hematoxylin solution for 1 minute
(Shandon, Pittsburgh, PA).The following antibodies were used: monoclonal antibody directed
against human fibroblasts (anti-Thy-1, 1:50, Dianova, Hamburg, Germany),
Table 4. Comparisons of expression levels measured for selected genes from HS-68 fibroblasts grown in coculture withA2058, BLM, WM-164, and SK-Mel-28 melanoma cells
Gene expression analysis. Within the 16 HGU95AV2 arraysused for the study, the percentage of genes determined to bepresent ranged from 49.6% to 55.4% with a median of 54.3%. Theaverage correlation coefficient between biological duplicates was>0.99. In a global view, the two different cell lines display quitedifferent expression profiles as evidenced by the correlationcoefficients extracted from the individual expression values forthe f12,000 genes for each sample under various conditions (seeSupplementary Data for details). The correlation coefficients withinthe A2058 cells have a mean of 0.985152 and a SD of 0.007936, andthose within the human fibroblast HS-68 cells have a mean of0.9763 and a SD of 0.01493. The correlation coefficients between thetwo cell lines have a mean of 0.876462 and a SD of 0.008629.Effect of coculture on the gene expression profiles of
melanoma A2058 cells. The change in the gene expression profileof the melanoma A2058 cells grown in coculture with the humanHS-68 fibroblasts compared with growth as a monoculture alonewas relativity modest. About 21 genes were determined to havesignificant fold changes compared with the gene expression profileof the melanoma A2058 cells cultured alone (Table 1).Dopachrome tautomerase , an enzyme involved in melanin
synthesis and melanocyte cell proliferation (21), was observed tobe up-regulated in A2058 cells cocultured with fibroblasts,indicating a growth stimulatory effect of fibroblast coculture onthe A2058 cells.The gene showing the greatest down-regulation in A2058
melanoma cells when cocultured with fibroblasts was IL-11 . Thiscytokine has been shown to be anti-inflammatory, functioning byinhibiting the secretion of proinflammatory cytokines by macro-phages (22, 23). Another gene that was down-regulated in thecocultured A2058 cells is the inhibitor of DNA-binding domain-1 .In mammary epithelial cell culture, inhibitor of DNA-bindingdomain-1 expression induces apoptosis (24); hence, in coculturewith fibroblasts, the A2058 cells with a decreased level of inhibitorof DNA-binding domain-1 may gain some resistance to apoptosis.
The results of analysis of the gene expression data by theMAPPFinder and GenMAPP programs to detect expression patternsassociated with biological ontology and pathways, respectively, areshown in Table 2. These data identified nine ontology classes and sixpathways as being significantly populated with up-regulated genesin the cocultured melanoma cells. Interestingly, two pathwaysassociated with chemokine signal transduction, the G13 signalingpathway (guanine nucleotide-binding protein) and small ligand Gprotein-coupled receptors (GPCR), were identified. The inflamma-tory response pathway was also identified as being active. Thissuggests involvement of the proinflammatory process as a result ofcoculture of A2058 melanoma cells with fibroblasts. In the up-regulated biological process class, melanin biosynthesis had thegreatest Z score. Up-regulation of this process class suggests anenhanced growth of the melanoma cells grown in coculture with thefibroblasts possibly due to a response to GROa (CXCL1) productionby cocultured HS-68 fibroblasts (see below). In addition, the defenseresponse biological process class was up-regulated.As seen in Table 2, eight pathway classifications and five
biological process classes were identified to be populated by asignificant number of down-regulated genes in the cocultured cells.Effect of coculture on the gene expression profiles of human
HS-68 fibroblasts. Quantitatively and qualitatively, the change inthe gene expression profile of the HS-68 fibroblast cells grown incoculture with the human A2058 melanoma cells was in sharp con-trast to that observed for the cocultured melanoma cells. From thegene expression data of cocultured HS-68 fibroblasts, 85 genes weredetermined to have significant fold changes compared with the geneexpression profile of the HS-68 fibroblasts cultured alone (Table 3).From the literature, 23 of the 85 genes that were altered have beenimplicated in processes associated with proinflammatory response,cell growth, proteolysis of ECM, and tumor invasion and metastasis.The GenMAPP and MAPPFinder programs identified 8 biological
pathways and 11 biological process classes up-regulated. In the up-regulated pathways, the blood clotting cascade had the greatestZ score (5.770). Eighteen genes were identified in that pathwayfrom the data set representing 90% of members of the pathway.The inflammatory response biological process class had the
greatest Z score (9.996) in the up-regulated group, with 132 genesin the class being identified from the data set (82% of the classmembers).
Table 4. Comparisons of expression levels measured for selected genes from HS-68 fibroblasts grown in coculture withA2058, BLM, WM-164, and SK-Mel-28 melanoma cells (Cont’d)
Nine biological pathways and 25 biological process ontologyclasses were associated with the down-regulated gene expressiondata. Interestingly, the inflammatory response pathway wasidentified from the down-regulated gene set as having the greatestZ score (3.975) populated by 29 genes representing 94% of thepathway members, whereas the humoral immune responsebiological process class had the greatest Z score (5.075) of thiscategory with 23 genes (85% of the members) identified in this class.Based on the data, it seems that there is a significant response in
HS-68 fibroblasts to coculture with A2058 melanoma cells, muchmore so than that observed with the A2058 cells cocultured withfibroblasts. As noted from the list of genes whose expression wassignificantly altered in the HS-68 fibroblasts and the results fromthe pathway and biological process class surveys, the fibroblastsrespond to coculture with a proinflammatory response accompa-nied by other changes that have typically been associated withpromotion of tumor invasion and metastasis.Quantitative real-time PCR. Table 4 shows the results of qRT-
PCR on six genes based on identification from the gene analysisdata of cocultured HS-68 fibroblasts, which we determined to be ofparticular interest due to their role in the proinflammatorypathways and matrix degradation. These results, in terms of foldchanges, show relatively good concordance with the microarraydata in terms of fold change of gene expression.qRT-PCR results are also shown in Table 4 for HS-68 fibroblasts
cocultured with three additional human melanoma cell lines: BLM,WM-164, and SK-Mel-28. The human melanoma cell line BLM is ahighly invasive melanoma that readily forms metastases in nudemice (25). The human melanoma lines WM-164 and SK-Mel-28 areonly modestly invasive (26, 27). The BLM melanoma cells exhibitedsignificant fold changes for the six genes analyzed, whereas the foldchanges for the WM-164 and SK-Mel-28 cell lines were modestcompared with the BLM and A2058 cells.Immunohistochemistry. To corroborate the in vitro gene
expression results, immunohistochemical studies on invasive humanmelanoma specimens were done. Nevus and melanoma biopsies ofprimary tumors were analyzed for the presence of selected genes(e.g., GROa, IL-1h, and IL-8) that were surprisingly up-regulated infibroblasts in cocultures. Antibodies against CD68 and fibroblast-specific antigen (Thy-1) were used to identify macrophages andfibroblasts in the tissue, respectively. Figure 1 is a representative ofseveral biopsies that were examined. In a nodular melanoma with amaximal tumor thickness of 2.3 mm, CD68-positive macrophageswere detected between the tumor cells, whereas Thy-1-positive,spindle-shaped fibroblasts embedded in a spare stroma surroundedthe melanoma cell nests. GROa staining was mainly associatedwith the stromal fibroblasts located close to the tumor cells. IL-8 andIL-1h staining was detected in the stromal fibroblasts adjacent to thetumor cells but also in somemelanoma cells. In the congenital nevus,some macrophages were depicted in the vicinity to the nevus cellnests at the junctional zone. Thy-1-positive fibroblasts, however,were not stained for IL-8, IL-1h, and GROa.Table 5 presents a summary of an immunohistochemical survey
for the expression of GROa, IL-1h, and IL-8 in biopsies from ninehuman malignant melanomas. In all sections, strong positivestaining associated with fibroblasts was observed for IL-1h and IL-8,with modest staining observed for GROa. These data corroboratethe representative immunohistochemistry shown in Fig. 1.Interestingly, there did not seem to be any significant correlationof staining intensity to whether the biopsies were from nodularmalignant melanomas or superficial spreading melanomas.
Discussion
The relationship between host and tumor has recently beenappreciated to be a dynamic one, whereby the environment of hostas represented by the stroma, tissues, organs, and ECM affects thebehavior of the tumor and similarly the presence of the tumor has areciprocal effect on the host. This interplay between the host andthe tumor may in fact be a critical factor in terms of whether thehost eliminates the tumor or the tumor continues to progress andmetastasize (28). As early as 1863, cancer was noted to often beassociated with chronic inflammation and subsequent cell prolif-eration, and over the years, anti-inflammatory therapies have beensuggested as an approach for cancer prevention and treatment(13, 29). Thus, the host-tumor interaction can result in a variety ofproinflammatory processes that may lead to the successfulimmunologic abatement of the tumor by the host (13). However,if the proinflammatory response resulting from host-tumorinteraction is blunted, such that a full, effective immune responsedoes not occur, then an environment may occur that could promotetumorigenesis, tumor progression, and metastasis (1).Effect of coculture of A2058 melanoma cells and HS-68
fibroblasts. The design of the experimental system for thecoculture of melanoma cells with fibroblasts in the context offibrillar collagen allowed for the exchange of soluble mediators inthe culture medium yet segregated the cells. The pore size of themembrane separating the two cell lines was such that physicalinteraction of invadopods from the cells could occur but not cellularpassage through the membrane. As seen from Table 1, there isrelatively little change in the gene expression profile of A2058 cellsgrown in coculture with fibroblasts compared with growth alone infibrillar collagen. However, there seems to be a significant effect ofcoculture on the gene expression profile of HS-68 fibroblasts in thepresence of A2058 cells (Table 3). This suggests the possibility thatthe fibroblasts are more responsive to the pool of soluble mediatorsproduced by the two cell lines than the melanoma cells. It could alsobe interpreted that the melanoma cells are constitutively activatedand not responsive to factors released by fibroblasts.Proinflammatory environment in cocultured A2058 cells
and HS-68 fibroblasts. From the gene expression profile of thecocultured fibroblasts, there are a variety of changes in geneexpression that could be considered to be of a proinflammatorynature (Tables 3 and 6). For example, the proinflammatorychemokine IL-8 (CXCL8) and the inflammatory cytokine IL-1bwere observed to increase 6.8- and 2.4-fold, respectively. The up-regulation of these genes is indicative of the development of aproinflammatory/inflammatory environment resulting from thecoculture of melanoma cells and fibroblasts. IL-8 is produced bymany cell types, and in addition to being a neutrophil chemo-attractant, it has been shown to have other activities that can beconsidered prometastatic (30, 31). However, in a recent report, Liet al. (32) showed a direct role of IL-8 in angiogenesis by inducingMMP-2 synthesis, inhibiting endothelial cell apoptosis, andenhancing antiapoptotic gene expression. It is well establishedthat melanoma cells constitutively express increased amounts ofIL-8. Melanoma cell–induced expression of this cytokine byadjacent stromal fibroblast therefore would amplify enhancedneovascularization of the tumor.IL-1 receptor antagonist (IL-1RA) was observed to be modestly
up-regulated (1.6-fold) in cocultured fibroblasts (Table 3). IL-1RAbinds to the IL-1 receptor, thereby inhibiting interaction with IL-1.IL-1 is a key, pleiotropic inflammatory cytokine that promotes
Melanoma-Fibroblast Cross-talk
www.aacrjournals.org 4141 Cancer Res 2005; 65: (10). May 15, 2005
angiogenesis, tumor growth, and metastasis (33). IL-1RA is oftencoexpressed with IL-1, and depending on the ratio betweencytokine and its antagonist, there is diminution of the biologicaleffects of IL-1. For example, IL-1 is constitutively expressed at highlevels in the metastatic melanoma cell line SMEL (34). When thiscell line is transduced with IL-1RA, tumor growth resulting fromthe transduced cells was significantly reduced in athymic nudemice, as was metastasis to the lung, clearly indicating a role for IL-
1RA in modulating IL-1 activities. In addition, IL-1 is required forangiogenesis by stimulating the proliferation of endothelial cellsand the synthesis of adhesion molecules and proteolytic enzymeson endothelial cells (35). Using IL-1a and IL-1h knockout mice,these authors were able to show that local tumor or lungmetastases of B16 melanoma cells were not observed comparedwith wild-type animals. In addition, vascularization of melanomacell–populated Matrigel plugs by endothelial cells was observed in
Figure 1. Immunohistologic staining of Thy-1(fibroblast-specific antigen), CD68 (macrophageantigen), IL-8, GROa, and IL-1h in specimens of arepresentative sample of human congenital nevusand a primary nodular melanoma. Serial sections(8 Am) of paraffin-embedded tissue were stainedusing monoclonal or polyclonal antibodies raisedagainst Thy-1, CD68, IL-8, GROa, and IL-1h.Bound antibodies were detected by alkalinephosphatase and neofuchsin as a substrate andcounterstained with hematoxylin. Magnification,�20. Bar , 50 Am.
Cancer Research
Cancer Res 2005; 65: (10). May 15, 2005 4142 www.aacrjournals.org
wild-type and inhibited by the addition of IL-1RA, whereas in-growth of endothelial cells was absent in IL-1h knockout mice,suggesting that host-derived IL-1 has an important impact ontumor growth and metastasis.In our studies of the cocultured fibroblasts, we have not examined
the protein levels of either IL-1h or IL-1RA and hence have no realunderstanding of the relative amounts of these proteins; however,from the perspective of the gene expression data, both the inten-sities and the fold changes were greater for IL-1b than IL-1RA .Therefore, we would expect that the net result is that the IL-1RAexpression in this system may serve to attenuate the inflammatoryresponse due to IL-1h, but it is not likely to completely ablate it.The down-regulation of IL-11 represents another interesting
change in the gene expression profile of the cocultured A2058 cellsthat could play a role in an inflammatory environment. As seen inTable 1, gene expression of IL-11 was down-regulated. IL-11 isinvolved in the regulation of type I cytokine proinflammatorypathways and has been shown to decrease keratinocyte prolifer-ation and cutaneous inflammation by attenuating the expressionof a variety of critical genes associated with inflammation anddisease. Therefore, it is reasonable that the down-regulationobserved for IL-11 in cocultured A2058 cells could contribute toa proinflammatory state.From the MAPPFinder and GenMAPP analyses of the gene
expression data for pathways and biological process classes thatare altered due to the coculture of melanoma cells and fibroblasts,it was seen that the inflammatory response pathway was identifiedas being up-regulated in the cocultured melanoma cells (Table 2).However, closer consideration of this suggests that this pathwaymay not be fully engaged. Of the 31 genes associated with thepathway, 28 were detected as ‘‘present,’’ although only 2 of thesegenes were actually changed due to the coculture conditions. TheZ score for this pathway was 1.9, and although significant, it isrelatively low; hence, it is probable that the up-regulation of thispathway under these conditions is rather modest and does notrepresent a fully effective inflammatory response.
One interesting consideration whether the conditions for acomplete inflammatory response could be developed under theseconditions stem from the MAPPFinder and GenMAPP analyses ofthe gene expression data of cocultured HS-68 fibroblasts. Fromthese data, the inflammatory response biological process class wasidentified as being up-regulated (Table 6) with a highly significantZ score, yet the inflammatory response pathway was identified asbeing down-regulated. We interpret these superficially conflictingdata to be due to the fact that a sufficient variety of genesassociated with proinflammation and inflammation are presentand up-regulated and hence identified as an up-regulated biologicalprocess class. However, they are not sufficient in number or foldchange to be considered as an up-regulated pathway. This, inconjunction with the down-regulation of IL-11 in the A2058 cells,leads us to conclude that it is likely that only a partial, incompleteproinflammatory/inflammatory response is being developed due tothe coculture of the A2058 cells with the fibroblasts.Effect of coculture on cell growth, proliferation, matrix
degradation, and angiogenesis. There is a close relationshipbetween cell growth, proliferation, matrix degradation, andangiogenesis and the proinflammatory pathway is considered tobe central to these processes in melanoma (36). Although we didnot assay for cellular growth and proliferation in these studies, it islikely that these events were occurring in the coculture systembased on the results from the gene expression profiles. Epiregulinwas observed to be up-regulated in the cocultured fibroblasts(Table 3). Epiregulin is a member of the epidermal growth factorfamily, and in addition to its abilities to stimulate cell growth, it hasbeen implicated in the pathobiology of pancreatic ductaladenocarcinoma (37). The gene for immediate-early response wasalso seen to be up-regulated in the cocultured fibroblasts. This genehas been shown to function to protect cells from Fas ligand orTNF-a-induced apoptosis and its up-regulation in fibroblaststherefore may serve to protect these cells from apoptosis underthe conditions of inflammation during tumor invasion (38).Matrix degradation has been shown to play a crucial role during
tumor invasion and to involve various classes of proteases,including MMPs. Genes of MMP-1 and MMP-3 were found to beup-regulated in fibroblasts cocultured with melanoma cells. Bothproteases play a key role in the degradation of fibrillar collagensand have been immunolocalized at the host-tumor junction at adermal invasion zone (39).The primary driver of cell growth, proliferation, matrix
degradation, and angiogenesis in invasive melanoma is likely IL-1h (40). Stimulation of melanoma cells by IL-1h causes theexpression of the chemokine IL-8, which can result in a widevariety of biological responses, including proliferation of keratino-cytes and melanoma cells, haptotatic migration of the melanomacells, and induction of angiogenesis (41–44). Interestingly, theseactivities seem to have some dependence on the environment ofthe tumor cells. IL-8 production in A375 melanoma cells is highwhen these cells are cocultured with human keratinocytes thatproduce IL-1, whereas when A375 cells are cocultured withhepatocytes that do not produce IL-1 their IL-8 level of expressionwas decreased (45). These studies indicate the role of the tumorenvironment in terms of promoting processes associated withtumor progression and metastasis. In our studies of the cocultureof A2058 human melanoma cells with HS-68 primary humanfibroblasts in fibrillar collagen, no up-regulation of chemokine orcytokine expression was observed in the A2058 cells; however, inthe cocultured fibroblasts, IL-1b , IL-8 , GROb , GROa , and CCL2
Table 5. Expression of GROa, IL-1h, and IL-8 in humanmalignant melanomas
Specimen Depth
(mm)
Melanoma
type
GROa IL-1h IL-8
1 1.61 SSM ++ ++ ++
2 4.5 NMM ++ +++ +++
3 2.25 NMM +++ +++ ++4 4.05 SSM + +++ +++
5 8 SSM + +++ +++
6 3.51 SSM ++ +++ +++
7 2.8 SSM + +++ +++8 3.6 NMM + +++ +++
9 3.15 SSM + +++ +++
NOTE: Expression of cytokines and chemokines was analyzed by
immunohistochemistry on cryosections of melanomas from ninedifferent patients. Intensities of specific stainings were arbitrarily set
as the following: +, modest expression; ++, moderate expression; +++,
(monocyte chemoattractant protein-1) were observed to be up-regulated (Table 3). Overexpression of CXCL1-3 by stimulatedmelanoma cells has been shown to function in an autocrine fashionto promote melanoma cell growth and proliferation (46, 47). Basedon our data, it is quite possible that host stroma, in this caserepresented by melanoma-stimulated fibroblasts, can also expressthese chemokines to promote melanoma growth and proliferation.As noted above, the chemokine CCL2 was also up-regulated in
fibroblasts in coculture with melanoma cells. This chemokine has
been shown to be important in attracting macrophage infiltrates totumors, a process that has been linked to tumor progression,invasion, and angiogenesis (48, 49). As observed in our experi-ments, the stimulation of cocultured fibroblasts by the A2058 cellspromotes an environment rich in chemokines known to stimulatemelanoma proliferation, synthesis of proteolytic enzymes, tumorcell invasion, and angiogenesis associated with macrophageinvasion, underscoring the potential for a central role of hoststroma in melanoma metastasis.
Table 6. Pathways and biological process classes associated with differentially expressed genes in cocultured HS-68fibroblasts
Taken together, there appears from our gene expression data tobe an activation of a pathway(s) initiated with IL-1h. IL-1 has beenshown to activate nuclear factor-kB, which in turn can up-regulatethe expression of MMPs, urokinase-type plasminogen activator,CXCL1-3, chemokines, and TNF-a (49). TNF-a has also been shownto up-regulate IL-8 and CCL2 (50). In the cocultured fibroblasts, weobserved the up-regulation of IL-1b , nuclear factor-kB , MMP-1 ,MMP-3 , tissue plasminogen activator, CXCL1 , and CXCL2 . Further-more, we also saw IL-8 and CCL2 up-regulated, but not TNF-a .Nevertheless, it could be that TNF-a protein levels, but not geneexpression, was increased in the coculture system because the genefor TNF-a-induced protein 6 was up-regulated, suggesting an effectof TNF-a on the system.Relevance of gene expression data to invasive human
melanoma. Over the years, many experimental and clinical effortshave aimed to improve the criteria for melanoma diagnosis andtreatment. To improve the knowledge in molecular pathology ofmelanoma, particularly in discriminating between very earlymelanoma lesions and benign nevi, cDNA/oligonucleotide arraytechnology is increasingly being used to identify new biologicalmarkers for malignancy or for invasive potential. However, analysisof tumor tissue alone may not identify small changes in geneexpression occurring in the microenvironment of tumor-stroma.Identification of regulated genes resulting from cross-talk andactivation due to coculture of melanoma cells and fibroblasts fromour studies have provided insight into the molecular mechanismsinvolved in tumor-stroma interactions.Our studies have shown that coculture of melanoma cells and
fibroblasts has a profound reciprocal effect on gene expressionprofiles, with dramatic alterations in fibroblasts compared with amore modest effect on the melanoma cells. The fibroblasts werefound to be more easily activated and responded to coculture byup-regulation of a large number of genes associated with theproinflammatory pathway, matrix proteolysis, and cellular prolif-eration. Interestingly, cytokines and chemokines (e.g., IL-1a,
CXCL1/GROa, and CXCL8/IL-8) that were thought to be producedby inflammatory cells or by melanoma cells were identified to beup-regulated in fibroblasts, suggesting that these cells are likely toalso contribute to the inflammatory reaction.In this study, we extended the coculture experiments of A2058
cells, a modestly invasive human melanoma cell line with HS-68fibroblasts to other human melanoma cell lines. The humanmelanoma BLM cell line has been shown to be highly metastaticwith early and frequent formation of metastasis in nude mice afters.c. inoculation (25). SK-Mel-28 and WM-164 melanoma cells are alow invasive cell lines (26) and WM-164 melanoma cells show noorgan metastasis unless injected i.v. in mice (29). Interestingly, weobserved that the fibroblasts grown in coculture with the highlymetastatic BLM melanoma cell lines showed the significantlygreater fold changes in the six relevant gene transcripts comparedwith the low invasive A2058, SK-Mel-28, and WM-164 melanomacell lines. It is interesting to speculate that melanoma with agreater invasive potential may elicit a greater ‘‘proinvasion’’ effecton the gene expression profiles of stromal cells.Therefore, we conclude that stroma, due to signals originating
from the tumor, by responding to the presence of transformed cellsis primarily responsible for the generation of a microenvironmentthat is proinflammatory, proproliferation, proinvasion, and prom-etastatic. Studies directed at disrupting the cross-talk between hostand tumor may define new strategies for therapeutic intervention.
Acknowledgments
Received 2/6/2004; revised 1/6/2005; accepted 3/1/2005.Grant support: Polifarma S.p.A (J.W. Fox), University of Virginia Cancer Center
(J.W. Fox), Alexander von Humboldt Stiftung (J.W. Fox), Wilhelm Sander Foundationgrant 1999.093.2 (R. Nischt and C. Mauch), Koeln Fortune Program of the Faculty ofMedicine grant 10/2004 (P. Zigrino), Deutsche Forschungsgemeinschaft through theSFB 587 at the University of Cologne (C. Mauch), and German Research Foundationgrant Ni 304/9-1 (R. Nischt).
The costs of publication of this article were defrayed in part by the payment of pagecharges. This article must therefore be hereby marked advertisement in accordancewith 18 U.S.C. Section 1734 solely to indicate this fact.
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