Tissue Samples

Gut specimens were derived from individuals undergoing resection for localized colon cancer or benign colonic diseases (e.g. diverticular disease). Microscopically normal colonic mucosa was dissected from the surgical specimen near the resection margin and immediately subjected to the experimental procedures.

For analysis of DUSP2 gene expression in normal and inflamed intestinal tissue, transmural gut specimens (snap frozen in liquid nitrogen immediately after surgical resection) were provided by the Institute of Pathology, University Hospital Heidelberg. Inflamed gut specimens were derived from patients suffering from ulcerative colitis (UC) or Crohn’s disease (CD). The diagnosis was confirmed by histopathological and clinical criteria prior to qRT-PCR analysis. Specifically, samples considered to be inflamed were characterized by dense mononuclear cell infiltrations, crypt abscesses/cryptitis, erosions or ulcerations. Normal control tissue was obtained from individuals suffering from localised colon cancer or benign colonic disease.

Antibodies

For immunoflourescent staining of tissue sections the following primary antibodies were employed: CD68, 1 µg/ml (clone: PGM-1, Dako Cytomation, Hamburg, Germany); CD14, 1 µg/ml (clone: TÜK4, Dako); CD86, 10 µg/ml (clone: FUN-1, BD Pharmingen, Heidelberg, Germany). Isotype- and concentration-matched control antibodies (Dako) served as negative controls.

For flow cytometric analysis the following mAb were purchased from BD Bioscience (Heidelberg, Germany): CD3 V450, CD14 FITC, CD33 PE-Cy7, CD86 AF700, HLA-DR V500, CD117 APC.

“Loss of Epithelial Layer” (LEL) Organ Culture

Mucosal specimens were washed extensively in RPMI 1640 (Life Technologies, Paisley, UK) containing antibiotics prior to removing the mucus layer by dithiothreitol (DTT) treatment (1 mM, 10 min; Sigma, St. Louis, MO, Germany). Subsequently, punches of defined surface area were prepared and denuded of epithelial cells by exposure to 0.7 mM EDTA (Sigma) in HBSS (without Ca²⁺ and Mg²⁺; Life Technologies) at 37°C in a shaking water bath for 30 min (50 ml EDTA/HBSS per punch) [14]. This incubation was repeated three times with two washing steps (10 min in HBSS/antibiotics) after each incubation period.

Where indicated, total mucosa specimens of the same surface area were cultured under identical conditions.

Isolation of Lamina Propria and Peripheral Blood Leukocytes

Lamina propria leukocytes (LPL) were isolated by enzymatic tissue digestion according to a modified method of Bull and Bookman [14]. Briefly, after depletion of the epithelial layer (see above) mucosal tissue was cut into 2–4 mm pieces and digested in a shaking waterbath at 37°C for 1.5 h using collagenase IV (70 µg/ml; Sigma) and deoxyribonuclease I (100 µg/ml; Sigma) in RPMI 1640 containing 2% fetal calf serum (Sigma), 2% L-glutamine (Life Technologies), and antibiotics. The resulting cell suspension was separated from undigested tissue by filtration through a 70 µm nylon mesh (BD Bioscience, Heidelberg, Germany). For further purification, the cell suspension was subjected to Percoll (GE Healthcare, Munich, Germany) and Ficoll-Hypaque (GE Healthcare) density gradient centrifugation.

Peripheral blood was taken during the operation. Peripheral blood mononuclear cells (PBL) were obtained by Ficoll-Hypaque (GE Healthcare) density gradient centrifugation.

Gene Expression Analysis by qRT-PCR

Tissue samples were disrupted with the aid of a RiboLyser device (ThermoHYBAID, Heidelberg, Germany) in lysing matrix “D” tubes (Q-BIOgen, Heidelberg, Germany) containing 400 µl lysis buffer from the MagnaPure mRNA Isolation Kit II (ROCHE Diagnostics, Mannheim, Germany). 300 µl of the lysate was collected and mixed with 600 µl capture buffer containing oligo-dT. After centrifugation at 13000 rpm for 5 min, 880 µl of this mix was transferred into a MagnaPure sample cartridge and mRNA was isolated with the MagnaPure-LC device using the mRNA-II standard protocol. MRNA was reverse transcribed using AMV-RT and oligo- (dT) as primer (First Strand cDNA synthesis kit, Roche) according to the manufactures protocol. Primer sets optimized for the LightCycler (RAS, Mannheim, Germany) were developed and provided by SEARCH-LC GmbH (Heidelberg, Germany). The qRT-PCR was performed with the LightCycler FastStart DNA Syber Green I kit (RAS) according to the protocol provided in the parameter specific kits. To correct for differences in the content of mRNA, the calculated transcript numbers were normalized according to the expression of the housekeeping gene peptidylprolyl isomerase B (PPIB). Values were thus given as transcripts per 1000 transcripts of PPIB.

Double Immunofluorescence Staining of Tissue Sections

Staining was performed on 2 µm sections of formalin fixed, paraffin embedded human colon tissue. After deparaffinization in graded alcohols, heat induced antigen-retrieval was achieved by incubating the slides in a pressure cooker for 5 min in citrate buffer, pH 6.0. Double immunofluorescence staining was performed using a combination of CD68 (mouse mAb, IgG3) and either CD14 (mouse mAb, IgG2a) or CD86 (mouse mAb, IgG1κ). Incubations were performed overnight at 4°C in antibody diluent (DCS, Hamburg, Germany). Biotinylated rabbit anti-mouse IgG1, (2 µg/ml; Zymed, San Francisco, CA, USA), biotinylated rabbit anti-mouse IgG2a (4 µg/ml; Zymed) and sheep anti-mouse IgG3 (1∶100, lot number AAM05; AbDserotec, Oxford, UK) served as secondary antibodies (30 min at room temperature). DyLight488-conjugated donkey anti-sheep antibody (green fluorescence; 8 µg/ml; Dianova), and Cy3-conjugated streptavidin (red fluorescence; 2 µg/ml; Dianova) were used as secondary reagents (30 min at room temperature). Slides were mounted and viewed with a TCS SL confocal microscope (Leica Microsystems, Wetzlar, Germany).

For quantification, CD14⁺ and CD86⁺ cells were counted in an area (lamina propria) defined by 100 CD68⁺ cells. Three different areas were evaluated per experiment. In order to allow for consistent and comparable results within/between the different experimental conditions areas densely populated by CD68⁺ subepithelial macrophages were excluded from the analysis.

Flow Cytometry

1×10⁵ to 1×10⁶ cells were incubated with a cocktail of up to six antibodies labelled with different fluorochromes. Peripheral blood monocytes (PBMO) were identified as CD33⁺ CD3⁻ cells. CD33⁺ CD3⁻ lamina propria myeloid cells (LPMO) [15] were further distinguished from mast cells by lack of or low CD117 expression. Flow cytometric analysis was performed using an LSR II (BD Biosciences) and FACSDiva v6 software (BD Bioscience). Doublets were identified by plotting FSC-A versus FSC-H and excluded from the analysis. As negative controls the (auto)fluorescence of the myeloid cell populations (stained with CD33PE-Cy7/CD3 V450, and CD117 APC (LPMO), respectively) was determined.

Laser-Capture Microdissection (LMD)

12 µm thick cryosections were prepared from flash frozen colonic tissue samples collected prior to culturing as well as after loss of the epithelial layer (LEL-M 5 h). After transfer to NF 1.0 PEN membrane coated slides (Carl Zeiss MicroImaging, Munich, Germany) sections were treated with DTT (1 mg/ml) for 5 min and stored in 100% EtOH at −20°C. Immediately before laser-capture microdissection, sections were stained with Cresyl Violet (0.1% in 100% EtOH; Sigma) and subsequently dehydrated by immersion in 100% EtOH and Xylene (Roth, Karlsruhe, Germany). LMD was performed for 1 h each using the PALM MicroBeam (Carl Zeiss MicroImaging). Microdissected tissue was collected using opaque AdhesiveCaps (Carl Zeiss MicroImaging).

Microarray Analysis

RNA was isolated with the RNeasy Micro Kit (Qiagen, Hilden, Germany) according to the manufacturer’s instructions for microdissected samples, using glycogen (Sigma) as a carrier. RNA quantity and integrity was determined using the Agilent 2100 Bioanalyzer (Agilent Technologies, Waldbronn, Germany). All samples had a RNA integrity number (RIN) between 3.1 and 6.6. The mean RIN of RNA samples directly sampled by LMD (t = 0 h) was 5.1±1.67 compared to 3.9±0.75 after 5 h (t = 5 h) incubation. Samples were stored at −80°C until microarray analysis.

Microarray analysis was performed using the whole genome cDNA-mediated Annealing, Selection, extension and Ligation (WG-DASL) Assay (Illumina, San Diego, CA, USA) employing a minimum of 200 ng of total RNA per sample (≥40 ng/µl; input 5 µl). Four replicates were measured for each time point. The analysis was conducted at the Genomics and Proteomics Core facility of the German Cancer Research Center (DKFZ), Heidelberg, Germany. Complete microarray data have been submitted to the GEO repository and are available under the accession number GSE56448.

Analysis of Microarray Data

Microarray data were normalized by variance stabilizing normalization (vsn) [16]. Differential expression has been calculated by the test implemented in the limma package [17], and P values adjusted for multiple testing by the method of Benjamini and Hochberg [18]. Over-representation analysis of GeneOntology (GO) terms ('biological process' branch only) was calculated by GOstats [19] using the hypergeometric test conditional on the GO structure. Heatmaps were calculated on gene-wise z-transformed data by hierarchical clustering (complete linkage method, Euclidean distance) on rows. All calculations were performed in R v.3.0.0 [20] with the following extension packages: lumi v.2.12.0 [21], limma v.3.16.8 [17], GOstats v.2.26.0 [19], and GO.db v.2.9.0. For comparison with published data [22], we took the list of limma results for all probes from the microarray and selected those genes that had a corrected P value of less than 0.01 and absolute log2-fold change of at least one. This resulted in 439 up-regulated and 297 down-regulated genes, respectively. To calculate significance of overlap, 1000 random lists of length 439 were drawn from all microarray probes in [22] and overlap calculated with genes found to be differentially expressed in the LEL model. The distribution of sizes of intersection sets was used to calculate empirical P values (given as “<0.001” if the observed size was never exceeded by data from any random list).

TUNEL Assay

Apoptosis was analysed using the TACS 2 TdT-DAB In Situ Apoptosis Detection Kit (Trevigen, Gaithersburg, MD, USA). The assay was performed according to the manufacturer’s instructions.

Ethics Statement

All human studies were approved by the ethics committee of the University of Heidelberg and performed in accordance with the principles laid down in the Declaration of Helsinki. Written informed consent was obtained from the patients.

Induction of Inflammatory Gene Expression in Resident Lamina Propria Cells following EDTA-mediated Loss of the Epithelial Layer

Healthy colonic mucosa of defined size was prepared from freshly obtained human surgical specimens and depleted of epithelial cells by exposure to EDTA under standardized conditions. Mucosal tissue was harvested prior to culturing (total mucosa (TM) t = 0 h), during or immediately after loss of the epithelial layer (“loss of the epithelial layer” mucosa (LEL-M) t = 3/4/5 h); Fig. 1A). As a control, total mucosa (including the epithelial layer) was cultured for 5 h prior to harvesting (TM t = 5 h).

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Figure 1. Induction of inflammatory gene expression in resident lamina propria cells following loss of the epithelial layer.

(A) Time scheme of the LEL model. Arrows indicate time points of tissue collection. Tissue samples were collected prior to culturing (TM t = 0 h), after washing (TM t = 2 h), as well during and after completion of epithelial cell release by EDTA treatment (LEL-M t = 3/4/5 h). As a control, tissue samples were collected from TM cultured for 5 h (TM t = 5 h). (B) LEL induces gene expression of IL1B, IL6, IL8, IL23A, TNFA, IFNG, and CCL2 in resident lamina propria cells. Transcript levels of cytokines/chemokines were determined by qRT-PCR in tissue samples collected as described in (A). Shown are the mean normalized transcript numbers ± SEM of at least 4 independent experiments. Gray bars represent transcript levels of TM (t = 0/2/5 h), black bars represent transcript levels of LEL-M (t = 3/4/5h). (C) EDTA treatment does not induce inflammatory cytokines in PBMC or LPMC. PBMC and LPMC, respectively, were exposed to 0.7 mM EDTA/HBSS or medium (RPMI/2% FCS) for 3 h. Subsequently, transcript levels of IL6, IL8, IL1B, and IL23A were determined by qRT-PCR (IL8 and IL23A not tested for LPMC). The results of two independent experiments are shown.

https://doi.org/10.1371/journal.pone.0097780.g001

We chose to employ qRT-PCR in order to evaluate the tissue expression of a selected number of “conventional” inflammatory genes. As shown in Fig. 1B, expression of the cytokine genes IL6, IL8, IL1B, IL23A, TNFA, IFNG as well as the chemokine gene CCL2 was markedly upregulated in LEL-M (t = 3/4/5 h) when compared to mucosa prior to culturing, which contained only low numbers of these transcripts. Transcript levels of all inflammatory mediators analysed were also higher in LEL-M at t = 5 h when compared to total mucosa cultured for the same period of time (TM t = 5 h). IL12B mRNA was not consistently detected in EDTA treated mucosa (data not shown). Note that treatment of peripheral blood (PBMC) and lamina propria (LPMC) mononuclear cells (isolated by enzymatic digestion), respectively, with EDTA using similar conditions as employed for epithelial cell detachment from mucosal tissue did not cause upregulation of IL6, IL8, IL1B and IL23A transcript numbers (CCL2, IFNG, TNFA not tested) (Fig. 1C).

Induction of Co-stimulatory Molecules and Pattern Recognition Receptors in Resident Lamina Propria Cells Following EDTA-mediated Loss of the Epithelial Layer

Pattern recognition receptors and co-stimulatory molecules are critically involved in innate and adaptive immune responses [23], [24]. Under homeostatic conditions, their expression has been described to be detectable only at low levels in the intestinal lamina propria [10]–[12]. We therefore examined the effect of EDTA-mediated loss of the epithelial layer on the expression of the genes encoding the PRR CD14, TLR2, as well as the co-stimulatory molecules CD86 and CD54 in mucosa cells. As shown in Fig. 2A, transcript levels of these genes were upregulated in mucosal tissue within 3 h after starting to inflict LEL (5 h LEL-M versus 0 h TM) while being not or marginally altered in total mucosa cultured for the same period of time (5 h TM versus 0 h TM).

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Figure 2. Expression of surface receptors in resident lamina propria cells following loss of the epithelial layer.

(A) LEL induces gene expression of CD14, CD86, TLR2, and CD54 in resident lamina propria cells in situ. Tissue samples of total mucosa (TM) were collected prior to culturing (0 h TM) and simultaneously from both TM and LEL mucosa after completion of epithelial cell release by EDTA treatment (5 h TM, 5 h LEL-M) (see Fig. 1a). Subsequently, transcript levels of CD14, TLR2, CD54, and CD86 were determined by qRT-PCR. Transcript numbers (normalized to 1000 transcripts PPIB) of “5 h LEL-M” were set to 1, and those of all other conditions were calculated as a fraction/multiple of 1. Shown are the mean normalized transcript numbers ± SEM of three or four independent experiments. Numbers in brackets indicate the absolute transcript numbers normalized to 1000 transcripts PPIB. Gray bars represent transcript levels of TM (0 h, 5 h), black bars represent transcript levels of LEL-M (5 h). (B) LEL induces protein expression of CD14 and CD86 in resident lamina propria cells in situ. Double immunofluorescence staining of CD68 (green) and CD14 or CD86 (red) in healthy total mucosa prior to culturing (TM t = 0 h) and after 5 h of culture (TM t = 5 h) as well as in mucosa immediately after LEL (LEL-M t = 5 h). Colocalization of both antigens is shown by yellow signals in the overlay. Magnification: x40. LEL enhances the expression of CD14 and CD86 on some CD68⁺ and a large pool of CD68⁻ cells. The results represent one of three independent experiments. (C) Quantification of CD14⁺ and CD86⁺ cells in TM 5 h and LEL-M 5 h, respectively. The mean numbers (± SEM) of CD14⁺ and CD86⁺ cells, respectively, per area of 100 CD68⁺ cells were determined with three areas/experimental condition being evaluated. Shown are the results of two independent experiments.

https://doi.org/10.1371/journal.pone.0097780.g002

In parallel, protein expression of CD14 and CD86, respectively, was determined in formalin-fixed tissue samples collected prior to culturing and immediately after epithelial cell depletion by immunohistological analysis. As shown in Fig. 2B, expression of both surface receptors was not detectable in lamina propria cells in the presence of an intact epithelial layer (TM t = 0 h) - in accordance with a previous study [25]. After 5 h of culture of total mucosa (TM t = 5 h) some CD14⁺ and CD86⁺ cells, respectively, which were negative for the macrophage marker CD68 (green fluorescence) appeared in the lamina propria. Note that at this time point signs of epithelial layer disintegration were already detectable by Hematoxylin-Eosin staining (see Figure S1). Importantly, following detachment of epithelial cells (LEL-M t = 5 h) higher numbers of CD14⁺ as well as CD86⁺ CD68⁻ cells than in the medium control (TM t = 5 h) could be observed in the lamina propria (Fig. 2B and 2C). Notably, the expression pattern of CD86 and CD14 in mucosal cells as observed in the organ culture model resembles that in intestinal inflammation in vivo (ulcerative colitis) (see Figure S2).

In line with the in situ results, expression of CD14 and CD86 was detectable on lamina propria myeloid cells (LPMO; CD33⁺ CD3⁻ CD117⁻) rapidly isolated after epithelial cell detachment (by enzymatic digestion of the lamina propria) as determined by flow cytometry. Expression levels on LPMO were comparable to those on autologous peripheral blood monocytes (PBMO; CD33⁺ CD3⁻) (see Figure S3A). Both myeloid cell populations expressed HLA-DR with significantly higher levels being detectable on LPMO than on PBMO. Note that neither EDTA nor enzymatic treatment (as employed for the isolation of LPL) of PBL resulted in an upregulation of CD14 and CD86 surface expression on PBMO (see Figure S3B, C).

Early Inflammatory Gene Expression Profile of Resident Lamina Propria Cells

Given that our investigation so far contained the bias of arbitrary selection of inflammatory “markers”, we in addition decided to perform a global gene expression analysis. In order to focus on the features of immunocompetent cells in the intestine with regard to their phenotypic and functional changes over time, frozen tissue samples collected prior to culturing (TM t = 0 h) as well as immediately after EDTA treatment (LEL-M t = 5 h) were subjected to laser-capture microdissection (LMD) of the lamina propria (LP). Subsequently, mRNA was extracted for global gene expression analysis followed by bioinformatic evaluation. As shown in Fig. 3, microarray analysis of four individual experiments (replicates R1–R4 for each of the two experimental conditions (TM-LP t = 0 h and LEL-LP t = 5 h)) yielded reproducible results. Compared to microdissected lamina propria prior to culturing (t = 0 h), 1119 genes were differentially regulated in the lamina propria following EDTA treatment (t = 5 h) with 488 genes being significantly up-, and 631 genes significantly downregulated (cut-off: adjusted p value <0.01). Table 1 lists the top 40 upregulated genes, respectively, ranked by fold change (for a complete list of all differentially regulated genes see Table S1). Importantly, among these significantly upregulated genes were also some of those observed to be upregulated using qRT-PCR (see Fig. 1), namely IL6, IL8, IL1B, IL23A and CCL2. An increase in gene expression of IFNG as well as TNFA was also observed though not at a statistically significant level (data not shown). Given that a number of epithelial cell specific genes were included within the dataset of downregulated genes (likely due to some epithelial cell contamination of the microdissected lamina propria preparation), the subsequent functional analysis was at this point restricted to the dataset of significantly upregulated genes only.

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Figure 3. Early inflammatory gene expression profile of resident lamina propria cells.

Frozen tissue samples collected prior to culturing (TM 0 h) and immediately after release of the epithelial layer (LEL-M 5 h) were subjected to laser-capture microdissection of the lamina propria. Following RNA extraction, global gene expression profiles of lamina propria cells were obtained by microarray analysis. Shown is a heatmap of significantly regulated genes in LEL-LP 5 h vs. TM-LP 0 h (four matched replicates (R1–R4) for each time point replicates representing four independent experiments). Colors show expression relative to the average (black), higher (yellow), or lower (blue) relative expression, respectively. Data have been transformed to gene-wise zero mean and unit variance (z transform). Rows have been re-ordered by hierarchical clustering (complete linkage, Euclidean distance metrics).

https://doi.org/10.1371/journal.pone.0097780.g003

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Table 1. Top 40 upregulated genes in the LEL model.

https://doi.org/10.1371/journal.pone.0097780.t001

In order to gain insight into biological processes occurring during the initiation of an inflammatory response in the organ culture model, an analysis of overrepresentation of gene ontology (GO) categories in our dataset of upregulated genes was performed (Table 2: top 30 significantly over-represented GO terms; for a complete list of all significantly over-represented GO terms see Table S2). Among the GO categories identified were many representing basic features of an inflammatory response, namely “regulation of response to stress” [26], “positive regulation of defense response” [27], “regulation of an inflammatory response”, “blood vessel development” [28], “(chemo)taxis” [26] and “interleukin-1 production” [29]. Furthermore, according to this analysis, NF-κB activation, cAMP and cytokine induced responses as well as the unfolded protein response seem to be important signaling events determining initial activation processes in lamina propria cells. In addition, several GO terms identified cover aspects of the innate response to bacteria suggesting that such microorganisms (or molecules derived from the latter) may contribute to the induction of the inflammatory response in the organ culture model. Alternatively, non-bacterial stimuli eliciting expression of similar gene sets may participate in this response. Of note, significant induction of apoptotic processes in lamina propria cells following LEL as proposed by the GO term analysis could not be substantiated experimentally by TUNEL assay (see Figure S4).

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Table 2. Over-representation of GO terms in dataset of upregulated genes in the LEL model.

https://doi.org/10.1371/journal.pone.0097780.t002

Inflammatory Events in the LEL Model Partially Reflect those Occurring in Intestinal Inflammation in vivo

To address (1) the in vivo relevance of the organ culture model and (2) the central point whether early activation processes occurring in the in vitro system differ from events that exist in symptomatic human colonic diseases, our data collected from the in vitro systems were subjected to a comparative analysis with published data from microarray analyses from inflamed colonic tissue (ulcerative colitis (UC)). In the absence of any published gene expression profiling studies using microdissected lamina propria cells, UC data sets generated based on the examination of total biopsy tissue were employed for this comparative analysis [22].

As illustrated in the Venn diagram (Fig. 4A), 57 of 488 significantly upregulated and 134 of 631 downregulated genes in our in vitro model were also found to be upregulated and downregulated, respectively, in active UC samples when compared to normal (non-inflamed) gut samples [22]. This corresponds to a significant enrichment of genes differentially expressed in UC (as identified by Granlund et al. [22]) in our dataset (p<0.001 for up- and downregulated genes, respectively, as determined by a permutation test with 1000 lists of random genes). Among the shared upregulated genes (see Table S3) were also biomarkers for clinical and/or endoscopic disease activity in UC, such as IL8, CXCL2, LCN2, and MMP9 [30]–[32]. In addition to IL8 (see Fig. 1), increased CXCL2 gene expression in LEL-M (t = 5 h) vs. TM (t = 0 h and t = 5 h) was confirmed by qRT-PCR (Fig. 4B; other markers not tested). As expected, S100A8 and S100A9 genes, IBD biomarkers preferentially expressed in peripheral blood myeloid cells (granulocytes, monocytes) [33] migrating into the tissue in response to inflammatory stimuli, were not observed to be upregulated in the LEL model. Notably, a comparison of our dataset with publicly available results (Top 200 differentially regulated genes) of a meta-analysis of IBD gene expression profiles [34] gave similar results (data not shown). These observations clearly demonstrate that key inflammatory events as observed in intestinal inflammation in vivo are at least partially reproduced by the organ culture model in vitro.

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Figure 4. Inflammatory events in the LEL model partially reflect those occurring in intestinal inflammation in vivo.

(A) The overlap of differentially expressed genes in the LEL model in vitro and in inflamed tissue obtained from ulcerative colitis patients (vs. normal control tissue) as published in Granlund et al. [22] is depicted by a Venn diagram. (B) Upregulation of the IBD biomarker gene CXCL2 in the LEL model. Tissue samples of total mucosa (TM) were collected prior to culturing (0 h TM). Furthermore, tissue samples were collected simultaneously from both TM and LEL mucosa after completion of epithelial cell release by EDTA treatment (5 h TM, 5 h LEL-M) (see Fig. 1a). Subsequently, transcript levels of CXCL2 were determined by qRT-PCR. Shown are the mean normalized transcript numbers ± SEM of three to four independent experiments. Gray bars represent transcript levels of TM (0 h, 5 h), the black bar represents transcript levels of LEL-M (5 h). (C) Identification of DUSP2 as a novel gene upregulated in intestinal inflammation. Left panel: Tissue samples of total mucosa (TM) were collected prior to culturing (0 h TM). Furthermore, tissue samples were collected simultaneously from both TM and LEL mucosa after completion of epithelial cell release by EDTA treatment (5 h TM, 5 h LEL-M) (see Fig.1a). Subsequently, transcript levels of DUSP2 were determined by qRT-PCR. Shown are normalised transcript numbers (including mean) as determined in four independent experiments. Right panel: Transcript levels of DUSP2 were determined in transmural tissue samples of normal (NC) as well as of inflamed (UC, CD) gut by qRT-PCR. Shown are normalized transcript numbers (including mean) as determined in five different tissue samples of NC, UC, and CD, respectively.

https://doi.org/10.1371/journal.pone.0097780.g004

Not surprisingly, the majority of differentially regulated genes in the organ culture model differ from those differentially regulated in active UC (Fig. 4A) [22]. Their potential clinical relevance – in particular with respect to the initial phase of an intestinal inflammatory response- needs to be further evaluated. In this regard it is interesting to note that several of the genes detected to be solely upregulated in our organ culture model have been prioritized as key genes linked to gene loci identified to be associated with UC (or inflammatory bowel disease (IBD) in general) in genome wide association studies [35] (GWAS; see Table S4).

Furthermore, for one of the genes observed to be significantly upregulated in the LEL model, dual specific phosphatase 2 (DUSP2), we tried to confirm its differential expression in intestinal inflammation in vivo. DUSP2, a regulator of MAP kinases, is induced in human leucocytes following stimulation. It may potentially represent an important signaling module involved in the initiation of intestinal inflammation as it has been demonstrated to promote inflammatory responses in rheumatoid arthritis in mice [36], [37]. As shown in Fig. 4C, induction of DUSP2 expression in the LEL model as observed by global gene expression profiling was confirmed by qRT-PCR (left panel). Importantly, in agreement with this result in the LEL model in vitro, significantly higher expression levels of this gene were observed in inflamed tissue of UC vs. normal control tissue (NC) in vivo (p<0.05). Increased DUSP2 transcript numbers were also detected in inflamed CD tissue, however at a lower level. Note that the low induction of transcript levels of DUSP2 in UC and CD vs. NC tissue when compared to the LEL model may be due to the fact that different types of tissue were used for these analyses (UC/CD/NC: transmural tissue; LEL model: mucosa).