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Transcriptional profiling of mesenchymal stromal cells from young and old rats in response to Dexamethasone

Abstract

Background

Marrow-derived stromal cells (MSCs) maintain the capability of self-renewal and differentiation into multiple lineages in adult life. Age-related changes are recognized by a decline in the stemness potential that result in reduced regeneration potential of the skeleton. To explore the molecular events that underline skeletal physiology during aging we catalogued the profile of gene expression in ex vivo cultured MSCs derived from 3 and 15 month old rats. The ex vivo cultured cells were analyzed following challenge with or without Dexamethasone (Dex). RNA retrieved from these cells was analyzed using Affymetrix Gene Chips to compare the effect of Dex on gene expression in both age groups.

Results

The molecular mechanisms that underline skeletal senescence were studied by gene expression analysis of RNA harvested from MSCs. The analysis resulted in complex profiles of gene expression of various differentiation pathways. We revealed changes of lineage-specific gene expression; in general the pattern of expression included repression of proliferation and induction of differentiation. The functional analysis of genes clustered were related to major pathways; an increase in bone remodeling, osteogenesis and muscle formation, coupled with a decrease in adipogenesis. We demonstrated a Dex-related decrease in immune response and in genes that regulate bone resorption and an increase in osteoblastic differentiation. Myogenic-related genes and genes that regulate cell cycle were induced by Dex. While Dex repressed genes related to adipogenesis and catabolism, this decrease was complementary to an increase in expression of genes related to osteogenesis.

Conclusion

This study summarizes the genes expressed in the ex vivo cultured mesenchymal cells and their response to Dex. Functional clustering highlights the complexity of gene expression in MSCs and will advance the understanding of major pathways that trigger the natural changes underlining physiological aging. The high throughput analysis shed light on the anabolic effect of Dex and the relationship between osteogenesis, myogenesis and adipogenesis in the bone marrow cells.

Background

The stromal compartment of the bone marrow contains mesenchymal stem and progenitor cells with high proliferating capacity in addition to cells at different stages of maturation. The mesenchymal cells are at the front of cell research today which differentiate in vitro and in vivo to multiple lineages including fibroblasts, adipocytes, cartilage, myogenic, and osteogenic cells [1–7]. MSCs also harbor the potential of trans-differentiation to many different lineages, thus providing a possible source of progenitors for cell therapy and tissue repair including bone, cartilage, cardiac, pancreas regeneration and neural injury repair [8]. Cell differentiation through distinct maturational stages involves coordination and activation of different sets of genes. Progenitor cells derived from the stroma compartment of the bone marrow differentiate under the control of transcription factors, which serve as lineage specific master genes for discrete differentiation steps. Definition of the key differentiation signals is important in order to induce the desired ex vivo lineage-specific maturation pathways.

Age related hormonal changes, for example a decline in sex hormones levels, are associated with a decrease in the number and activity of osteogenic cells and an increase in numbers of adipocytes [9–15]. It is generally accepted that these changes arise from a decrease in the stemness potential accompanied by a decrease in the proliferative ability and osteogenic capacity of the bone marrow cells [11, 15–18]. The changes in stemness with age result in reduced osteogenesis and increased adipogenesis, affecting the skeletal structure and the immune system. Age-related changes associated with osteoporosis were previously studied by us in animal models [15, 19] and in ex vivo cultures of stromal cells [20]. It is clear that the physiological status of the body affects the skeleton at the cellular level, but the underlying molecular mechanism remains unresolved.

The action of native or pharmacological glucocorticoid hormones, such as Dexamethasone (Dex), is mediated via glucocorticoid receptors (GRs). Dex is recognized by multiple effects on a wide range of tissues and physiological conditions in the body [21]. Dexamethasone promotes osteogenesis in vitro [22], and induces the expression of osteogenic markers in MSCs [20, 23–25].

In this study, we analyze the molecular changes in aged rats that influence the cellular potential and the response to Dex. We used GeneChip technology to explore the molecular changes regulating the processes that govern the commitment and differentiation of the MSCs in young and aged animals. This approach enables us to analyze genome-wide patterns of mRNA expression and to provide an efficient access to genetic information. We compared gene profiling between MSCs cultured ex vivo from young and old rats (3 and 15 month old). The cells were maintained in vitro and maintained in presence or absence of Dex. The RNA extracted was analyzed to assess the transcriptome profile of MSCs. From the microarrays we further analyzed the lineage-specific gene expression in the MSCs enabling us to reveal genome-wide patterns of mRNA expression and to sort the gene profiles that govern various cell activities.

Results

The GeneChip analysis

Primary marrow stromal cells (MSCs) derived from the bone marrow include stem and progenitor cells with high proliferating capacity. We have earlier studied MSC in rat [19] and mouse [4, 15] models and demonstrated that the decline in stemness with aging is associated with bone atrophy, increase of adipocytes and augmentation of T-lymphopoiesis.

The present study aimed to compare the profile of genes expressed by cultured MSCs derived from 3 and 15 month old rats, expanded in vitro and treated or untreated with Dex. We used microarray technology to compare the transcriptome profile between cultured MSCs from 4 experimental groups: young Y (3 month) and old O (15 month) rats that were treated (YT, OT) or untreated (YU, OU) with Dex. The molecular analysis represents snapshot of cellular states from these rats and reflects their potential for tissue differentiation. The analysis resulted with 10290 Probe Sets (PS) that changed with fold change of two or higher. The PS clustering attempts to elucidate the pattern of gene expression which is unique to MSCs.

Genes differentially expressed between experimental groups

The gene expression was studied for RNA from each age group, and the overlap between them was calculated. RNA was retrieved from four groups of cells according to treatment and animal age: untreated cells from 3 month old rats (young untreated – YU – 1), 15 month old rats (old untreated – OU – 2) and treated cells from young and old rats (YT – 3, OT – 4). Differentially expressed PS were marked either as increasing or decreasing according to expression ratios between Dex-treated and untreated cells. In cells derived from young rats, the analysis resulted in 3318 differentially expressed PS, 1604 increasing (YI) and 1714 decreasing (YD). In cells derived from old rats, 2725 PS were differentially expressed – 1314 increasing (OI), 1411 decreasing (OD) following treatment.

A total of 888 PS increased and 1077 PS decreased in cells derived from both young and old rats due to the Dex treatment. The analysis of differentially expressed PS was repeated for fold change of 3, 4 and 5 and resulted in smaller numbers of differentially expressed PS. The number of PS differentially expressed at fold change higher then 2 decreased, but the ratio of expressed PS in both ages versus PS expressed in cells derived from young or old rats did not change much, indicating a common response to Dex in both ages (Figure 1).

Figure 1
figure 1

Ratio of PS differentially expressed in both age groups vs. each age group. BI – PS that increased in cells derived in both age groups, YI – PS that increased in cells derived from young rats, OI – PS that increased in cells from old rats. BD, YD, OD – PS that decreased in cells from both age groups, in cells from young and old rats respectively. The graph presents ratios for multiple fold changes: 2,3,4,5. BI/YI and BD/YD (white bar), BI/OI and BD/OD (grey bar).

The ratio of PS changed in both groups relative to PS changed in cells from old rats remained constant. The ratio of PS increased in both groups (BI) relative to PS increased in old (OI) and the ratio of decreasing PS (BD/OD) remained at about 60% and 70%, respectively. The PS increased in both groups (BI) relative to PS increased in young (YI) lowered from 55% to 32% as the number of differentially expressed PS decreased (due to increasing fold change). The ratio of PS decreased in both groups (BD) relative to PS that decreased in young (YD) lowered from 63% to 48% as the number of PS in general decreased.

Clustering analysis

PS were clustered to profile distinct Dex effect for both age groups; 4060 PS were differentially expressed, up or down regulated more than 2-fold, due to the Dex treatment in cells derived from young and old rats. The analysis resulted in six clusters that were divided into PS that increased (A-C) or decreased (D-F) (Figure 2). Cluster A (704 PS) represents PS that increased in cells derived from young rats, Cluster B, represents 420 PS increased in old rats, and PS that increased in cells from both age groups are included in Cluster C (888 PS). PS that decreased in cells derived from young rats are put in Cluster D (631 PS), PS that decreased in cells from old rats – in Cluster E (322 PS), and Cluster F (1071 PS) presents PS that decreased in cells from both age groups. A small number of PS increased in cells from young rats and decreased in cells from old rats (12 PS) or the opposite pattern of expression (6 PS) (data not shown). PS who had a known Gene ID were analyzed for functional properties of the genes.

Figure 2
figure 2

Illustration of the clusters A to E. Four groups of analyzed samples are presented: 1 – young untreated (YU), 2 – old untreated (OU), 3 – young treated (YT), 4 – old treated (OT). The mean of each PS was standardized to 0, and the standard deviation was 1. The clusters included PS increased in cells from young rats (A), increased in cells from old rats(B), increased in cells from both age groups (C), decreased in cells from young rats(D), decreased in cells from old rats (E), decreased in cells from both age groups (F). Expression patterns of all clusters are presented with error bars. PS at levels lower than zero indicates the repressed expression and PS at levels above zero indicates the induced expression.

Functional pathways involved in mesenchymal cells differentiation

Comparing gene expression profiles between Dex-treated or untreated cultured cells obtained from young and old rats results with clustering of 6 groups (Figure 2) analyzed for statistically significant functions, using the GOTM. This analysis shows functions affecting response to Dex and differentiation of skeletal and bone marrow cells. Tables 1 and 2 describe the major functions that have a high fold change and highlight various differentiation pathways of mesenchymal cells affected by Dex treatment.

Table 1 Genes induced by Dexamethasone in MSCs

Series of genes increased following Dex treatment of MSCs are represented in clusters A-C (Figure 2): genes increased in cells derived from young rats (A), in cells derived from old rats (B) and genes increased in cells derived from both age groups (C) (Table 1). The overall gene expression reflects the Dex-related shift of cellular metabolism, which results in a decrease in proliferation, coupled with differentiation of MSCs to osteogenic and myogenic directions and a repression of the adipogenic pathway.

Cluster A (genes that increased only in cells derived from young rats) includes VEGF, Id1, Madh5 and beta-catenin which are related to angiogenesis (p = 0.00125), implying that neovascularization is linked to osteoblast maturation and bone remodeling (p = 0.00448), which included the genes PTHr1, IBSP, Madh5 and bone ECM protein Mepe. These genes are related to osteogenesis and indicate an osteogenic differentiation of these cells. Human and mouse orthologs disclosed components of ECM structural constituent such as collagens IV, V, VI and laminin (p = 0.00287). Dex has an anabolic effect on cells from young rats that increases osteogenesis-related markers, while such an effect was undetected in cells derived from old rats and is possibly related to the decrease in bone formation associated with aging.

Cluster C presents genes that increased due to Dex treatment in cells derived from both young and old rats (Table 1) which are related to cell growth (p = 2.36E-06), regulation of cell cycle (p = 0.00418), muscle differentiation and contraction (p = 0.00555, p = 0.00157), cytoskeletal components (p = 0.00868) including structural constituents of the cytoskeleton and actins (p = 0.00533, p = 0.00803). A reciprocal relationship of proliferation and differentiation is recognized by a decrease in genes that activate proliferation as cells differentiate. Human and mouse orthologs of the rat genes are related to the dystrophin complex (p = 0.00311) which plays a role in development of skeletal muscle. An increase in muscle related genes due to Dex indicates the potential of mesenchymal stem cells to differentiate into myotubes.

Genes decreased following Dex treatment are clustered in D-F (Figure 2) for cells derived from young rats (D), old rats (E) and from both age groups (F) (Table 2). Genes repressed following Dex treatment in cells derived from young rats are related to adipocyte differentiation, regulation and function (Table 2, Cluster D). PPARγ and CEBPα are TFs essential for adipocyte differentiation (p = 0.0056). PPARγ maintains adipogenesis affecting early differentiation and survival of mature adipocytes and CEBPα is activated later than PPARγ. An inhibition of PPARγ and CEBPα in response to Dex results with a decrease of adipogenesis. The effect of Dex in lowering the adipogenesis (Table 2, cluster D) is complementary to increasing the osteogenesis (Table 1, cluster A).

Table 2 Genes repressed by Dexamethasone in MSCs

Cluster F (Table 2) summarizes genes repressed by Dex treatment in cells derived from both age groups and includes genes related to defense response (p = 0.0006). We noticed a decrease in RAS signaling genes (p = 0.00016), such as Nras, Kras2, Grb2 and Aps, which is complimentary to the proliferation and differentiation genes induced by Dex (Table 1, Cluster C). Dex repressed genes related to catabolism (p = 0.00027) and proteolysis (p = 0.00312), including mainly lysosomal (p = 1.4E-07) hydrolases (p = 0.00019). The suppression of adipogenic differentiation is monitored by the decrease of genes related to lipid binding (p = 0.00024), lipid transport (p = 0.0096) and diacylglycerol binding (p = 0.00474) including genes such as FABP-4 (aP-2) and lipoprotein lipase (Lpl). Protein Kinase C isoforms comprised some of the genes identified as lipid binding cluster. The variants of this gene have a role in muscle differentiation and mediate PTH receptor action in repressing adipogenesis and inducing osteogenesis.

The functional analysis of the clusters resulted in major pathways – an increase in osteogenesis and muscle formation, coupled with a decrease in adipogenesis. We selected the genes representing these differentiation pathways (Table 3) and divided them into clusters and functional groups. Genes which increased only in cells from young rats belong to the functional group of bone remodeling and angiogenesis. Genes that increased in both cells derived from young and old rats are related to muscle development and cell cycle. Other genes that decreased only in cells derived from young rats are related to adipocyte differentiation and genes that decreased in both groups are related to lipid binding, catabolic peptidases, immune response and RAS signaling. To validate the results from the gene array we employed RT-PCR analysis summarized in Figure 3 (p values are specified in the legend). Analyses were performed for the expression of BSP, Biglycan and BMP4 to follow osteogenic pathway; desmin and actin γ2 – to follow the effect of age and Dex on the cell potential to differentiate to myoblasts. AP-2, LPL and Adipsin were used to follow adipogenesis. Analyzed markers showed age and Dex related changes detected with a similar fold change levels for both RT-PCR and array analysis. The expression of GR was analyzed to verify that the response to Dex resulted with down regulation of the receptor. The expression level of GR decreased in cells from both age groups – the ratios were 0.4 and 0.54 on the chip, and 0.44 and 0.42 by RT-PCR. The fold change for desmin on the chip array was 2.4 for cells derived from young rats and 2.36 for cells derived from old rats and 1.9 and 2.05 by RT-PCR, respectively. AP-2 expression decreased on the chip (0.04 and 0.01), and by RT-PCR (0.2 and 0.12). Dex triggered an increase in the osteogenic related genes that was more prominent in young animals. An increase was noted in muscle-related genes in cells from both age groups; and a decrease in genes related to the lipid metabolism. The expression level of these genes behaved in a similar manner on the chip and when checked by RT-PCR. The comparison between the two methods confirmed the biological effect of Dex on cells from young and old rats.

Table 3 Gene array analysis for adipogenesis, osteogenesis and myogenesis pathways
Table 4 Primers used for RT-PCR amplification
Figure 3
figure 3

RT-PCR analysis of genes related to bone remodeling, muscle development and lipid binding and metabolism. (A) – bone remodeling include BMP4, Biglycan, BSP, (B) – muscle development include Actin, Desmin and (C) – lipid binding and metabolism include AP-2, LPL, Adipsin. (A-C) – Y axis represents the gene expression level (normalized to G3PDH) of the YU (light blue bars), YT (blue bars), OU (pink bars), and OT (purple bars). T-test comparing expression level in treated and untreated age-matched samples was performed – * p value < 0.005, expression levels of all genes analyzed except Biglycan are significant with p value < 0.05. (D) – Y axis represents the ratio between treated and untreated cells from young (blue bars) and old (purple bars) rats.

Discussion

Mesenchymal stem cells have an ability to differentiate into multiple lineages including adipocytes, myocytes and bone forming cells [1–7]. Aging affects the bone marrow microenvironment in multiple ways, repressing the "stemness" of cells which results in a decrease in bone formation. The number of precursor cells of the hematopoietic and osteogenic cells as well as their proliferative ability decrease with aging [10, 11]. Although there are some contradictory findings in the literature related to proliferative and osteogenic potential, some of them rely on studies performed with total bone marrow population [17, 26]. Other experiments [9–15], including ones in our laboratory [15, 19], have focused on the mesenchymal stem cells and have shown a decrease in the stemness potential followed by a decline in the proliferative and osteogenic capacities. Consequently the molecular mechanism of the decrease in stemness associated with a decrease in bone formation with aging is yet unclear.

To better understand the molecular mechanisms governing the cellular changes we profiled the response of ex vivo cultured stromal cells challenged by Dex and compared cells derived from young and old rats. The gene expression profile revealed overlap of Dex action between the MSC derived from the two age groups. The functional analysis of the differentially expressed genes highlighted a general shift in the metabolism of the MSCs which included repression of proliferation and was complemented by induction of differentiation. Specifically, we monitored genes related to induction of myogenic and osteogenic differentiation coupled with a decrease in adipogenesis.

The results presented show a decrease in proliferation coupled with an increase in muscle related genes, observed in both age groups (Cluster C). The expression of muscle related genes indicates that the potential of mesenchymal stem cells to differentiate to myotubes is enhanced by Dex, which was reported earlier [27]. A reciprocal relationship of proliferation and differentiation is known – acquisition of differentiated phenotype is accompanied by a decrease in cells' proliferation potential, a relationship which is well documented for osteoblasts [28] and for myoblasts [29]. Dysfunction of tumor suppressor proteins results in attenuation of osteogenesis and myogenesis, in vivo [30, 31] and in vitro [32]. It was shown that myoblasts lacking Rb failed to differentiate into myotubes even when transfected with MyoD, an essential transcription factor for myogenesis [33]. In the MSCs analyzed in the present study, Dex decreased proliferation and triggered myogenesis. In addition, the genes induced are known to play a role in osteogenesis, which was also induced. Few examples are shown by the expression of PDGFa [34], TGFb3 and p53 [32], genes known to play a role in osteogenesis [35] in addition to myogenic differentiation.

Aging is accompanied by a reduced stemness potential of MSCs resulting in a decrease of osteogenesis and replacement of bone marrow with fat cells. This phenomena is associated with osteoporosis [36] and overall reduction of osteogenic stem cells with aging [12]. In agreement with this, in our study the cells derived from young rats, but not the ones derived from old rats, responded to Dex with an increase in genes involved in bone remodeling, angiogenesis and a decrease in genes related to adipocyte differentiation.

Genes increased in cells derived from young rats (Cluster A) were related to bone remodeling and included PTHr1, BSP, Madh5, Mepe, byglican and BMP4 which are expressed in osteoblasts during differentiation and bone regeneration [35, 37, 38], indicating an anabolic effect of Dex on the cells derived from young rats. The anabolic effect of Dex is known, as demonstrated by increases in the expression of bone related genes including BSP in rat osteoblastic cells [39, 40]. Such an effect was not observed on cells derived from old rats, which might be related to the decrease in bone formation potential recognized with aging. Neovascularization is linked to osteoblast maturation and bone deposition [41]. The angiogenesis functional group included VEGF, Id1, Madh5, beta-catenin and other genes. These genes are recognized in the literature for their role in osteoblastic differentiation in addition to their role in angiogenesis [42–45]. The expressed genes' function in angiogenesis implies that MSCs induce or attract formation of blood vessels. In addition, examining the human and mouse orthologs revealed ECM structural constituents including proteins that build up the basement membrane, like collagens IV, V, VI and laminin. Expression of these genes can indicate a potential for an endothelial differentiation.

Genes repressed following Dex treatment in cells derived from young rats (Cluster D) are related to adipocyte differentiation, regulation and function. This function included the two transcription factors PPARγ and CEBPα, which are essential for adipocyte differentiation. PPARγ maintains adipogenesis and is necessary for early differentiation and survival of mature adipocytes [46]. CEBPα is activated later than PPARγ during adipogenesis [47] and lack of this TF results in non-functional adipocytes [48]. These factors are sufficient for adipogenic differentiation in non-adipogenic mesenchymal cells [49] including myoblasts [50]. Adipogenesis and osteogenesis represent two divergent pathways of differentiation from the mesenchymal stem cells. Genes up-regulated in osteogenesis, such as Msx2, repress adipogenesis by inhibition of PPARγ and CEBPα [49]. Alternatively, PPARγ inhibits osteogenesis suppressing the osteoblastic phenotype [51]. We have demonstrated an interchanging relationship between osteogenesis and adipogenesis affected by Dex. Dex increased beta-catenin in the cells derived from young rats that is concurrent with an increase in osteoblastic potential of these cells. Beta-catenin represses adipogenesis [52] and induces osteogenesis [45]. Thus, the Dex effect of suppressing the adipogenesis (Table 2, cluster D) and increasing the osteogenesis (Table 1, cluster A) suggests that beta-catenin plays a role in the Dex dependent modulation of the two lineages.

The genes repressed in both ages (Cluster F, Table 2) include proliferation related genes, which complement the genes induced in cells from both age groups. We also observed a decrease in adipogenesis related genes, and in catabolic peptidases, indicating an anabolic effect of Dex. In addition, Dex decreased the expression of genes related to defense and immune response (Table 2). Dex is known to decrease the expression of immune genes, mostly tested on lymphocytes [21]. Mesenchymal cells have been shown to express immune cell markers, known to produce supportive stroma that regulates the HIM in the differentiation of the immune cells [53, 54]. Thus, the decrease in immune-related genes may be related to the stromal function. This is strengthened by the fact that repressed genes also included sub-sets of membranous proteins and genes related to antigen processing and presentation (human and mouse orthologs). Hormonal modulation affects cells signaling. We identified repression of RAS pathway, which included the genes Nras, Kras2, Grb2 and Aps and also play a role in control of cell proliferation and can also repress differentiation in the myogenic [55] and osteogenic [56] pathways. Grb2 adaptor protein mediates the proliferative anti-myogenic differentiation action of Met (HGF Recptor) [57], FGFR [58] and is involved in signaling of Dystrophin complex [59]. The decrease in Ras signaling genes is complimentary to the proliferation and differentiation genes induced by Dex (Table 1, Cluster C) and indicates a decrease in cell proliferation, which is coupled with myoblastic or osteoblastic differentiation.

Suppression of adipogenic differentiation was noted by decrease of genes related to lipid binding, lipid transport and diacylglycerol binding including representative genes, such as FABP-4 (aP-2) [60, 61] and lipoprotein lipase (Lpl) [62]. Adipsin repression marked the catabolism function of adipocytes [63]. Protein Kinase C isoforms are associated with various differentiation pathways. PKC repression increases myogenesis [64] and as a mediator of PTH receptor actions this enzyme is known to increase osteogenesis and repress adipogenesis in mesenchymal cell lines [65]. PKC is also associated with inducing osteoblast production of IL-6 [66] which promotes bone resorption. Thus, the decrease in PKC induces mesenchymal differentiation to the myogenic pathway.

Catabolic peptidases and lysosomal proteins decreased following Dex treatment. Matrix metalloproteinases 7,9,12 & 13, genes which play a role in collagen catabolism and bone remodeling [67] were included in this group. Additional genes were lysosomal proteases important in lympho-myeloid cells and cathepsins. Cathepsin K is the main protease in osteoclastic function that plays a role in bone resorption [68]. The decrease in expression of these genes indicates a lower rate of bone resorption, which consequently results in an increase in gene related to bone formation mediating the effects of Dex.

Conclusion

Aging affects the bone marrow microenvironment in multiple ways, including a decrease in the differentiation potential of cells associated with decrease in bone formation. To better understand molecular mechanisms governing the cellular changes we profiled the response of ex vivo cultured stromal cells to Dex and compared cells derived from young and old rats. The gene expression profiling highlights age-independent modes of Dex action which overlapped between the two age groups. While this study demonstrates the effect of Dex on in ex vivo cultured cells, it would be interesting to expand the scope to include the in vivo effects of Dexamethasone. In general, pattern of expression included repression of proliferation and induction of differentiation. The RNA analyzed was extracted from pooled samples from multiple animals, a method which has been proven to reduce variability, recommended when using a small number of microarrays [69]. It is possible that additional replicates would further refine these gene lists and may alter some of our conclusions. Continuing research and verification of this interesting subject are required in the future. Specifically, we catalogued genes related to induction of myogenic differentiation coupled with a decrease in adipogenesis. We demonstrated Dex-related decrease in immune response genes; Dex decreased genes that regulate bone resorption and induced osteoblastic differentiation. The high throughput analysis enlightens the effect of Dex and the relationship between osteogenesis and adipogenesis in the bone marrow due to aging. We have also demonstrated the plasticity of cells and the reciprocal relationship of the osteogenic, myogenic and adipogenic lineages in the bone marrow.

Methods

Ex vivo cultures of mesenchymal cells

Mesenchymal stromal cells (MSCs) were cultured from female Wistar rats. Cells were cultured in Dulbecco's modified essential Medium (DMEM) with 10% heat-inactivated fetal calf serum (FCS) (Gibco, USA) [4]. The bone marrow cells were harvested from young rats (3 months old) and old rats (15 months old). Cells were collected as previously described [15]. In brief, the bone marrow cells were flushed from the long bone collected and prepared for single cells suspension. Cells pooled from six rats in each group were cultured in 75 cm2 flasks (Falcon, USA) containing 20 ml of growth medium, Dulbecco's Modified Essential Medium (DMEM) containing 10% heat-inactivated fetal calf serum (FCS). Under these conditions, the hematopoietic cells died and the cultures finally remained only with cells forming the adherent stromal fibroblast-like layer. Cells were plated and after one week of culturing were trypsinized, single cell suspensions were re-cultured for 7 days and were grown in absence or presence of 10-8 M Dexamethasone (Dex). On day 14 cells were harvested for RNA extraction and created four samples – young untreated (1 – YU), old untreated (2 – OU), young treated (3 – YT) and old treated cells (4 – OT).

RNA analysis and microarrays

Total RNA were extracted from the design four experimental groups. Each group is composed from multiple animals, a method which has been proven to reduce variability, and is recommended when using a small number of microarrays [69]. RNA was extracted using the TRIzol and cRNA prepared according to Affymetrix protocols. Gene expression was measured by hybridization to Affymetrix RAE230A Gene Chip DNA microarrays (Affymetrix, Santa Clara, CA, USA), containing 15,766 probe sets (PS) (excluding controls), comprising 14,280 Unigene clusters (11,497 Gene IDs, 4,699 full-length transcripts). The data is available as accession GSE3339 of the Gene Expression Omnibus (GEO).

Gene expression analysis

Total RNA extracted from cultured cells following ex vivo expansion was reverse transcribed using avian myeloblastosis virus reverse transcriptase (AMV-RT) and oligo-dT to generate cDNA that served as a template for the polymerase chain reaction (PCR) (Takara Shuzo Co. Ltd., Japan) with gene specific primers (Table 4). The integrity of the RNA, the efficiency of the RT reaction and the quality of cDNA subjected to the RT-PCR was controlled by amplification of Gluteraldehyde-3-Phosphate Dehydrogenase (G3PDH) (Clontech, Palo Alto, CA). The reaction products were separated by electrophoresis in 1% agarose gels (SeaKem GTG, FMC, USA) in Tris Borate EDTA (TBE) buffer. The amplified DNA fragments were stained by ethidium bromide, and their optical density was measured using Bio Imaging System, BIS 202D and analyzed using "TINA" software. PCR amplification was performed at least twice and subjected to semi-quantitative analyses by comparison of OD of gene-specific PCR products normalized to the OD of co-amplified G3PDH-PCR product in four groups YO, OU, YT and OT.

The computerized data analysis

We used the MAS 5.0 algorithm to provide a baseline expression level and detection for each PS. PS were filtered according to the following criteria: (a) at least one sample was detected as Present (P) when calculating MAS 5.0 detection call; and (b) at least one sample had an expression level higher than 20. The expression levels of 10290 retained PS normalized using the Quantile Normalization method, provided by the software package 'affy' (version 1.5.8) [70], available as part of the Bioconductor project. For every PS, the ratio between expression level of the treated and untreated samples was calculated. PS were analyzed when the expression ratio at least 2 fold, in either age group. Gene expression of cells cultured from young rats (young treated versus young untreated) was compared to cells from old rats (old treated versus old untreated). After filtering the PS were standardized by transforming each expression pattern to have a mean of 0 and a variance of 1.

Clustering analysis

We used a rule-based clustering method on the PS that were differentially expressed when the fold change was at least two and were analyzed for either increasing or decreasing expression between Dex-treated and untreated cells. For every PS, the ratio between expression level of the treated and untreated samples was calculated. Every PS was graded as increased, decreased or unchanged. The young grade (YT/YU) was compared to the old grade (OT/OU), and this determined the cluster. This method resulted in 4060 PS, clustered in 8 distinct clusters. This clustering method separated increased and decreased PS due to Dex, and highlighted difference between old and young rats. Partial data is discussed in this paper and complete lists of functions and genes are available upon request.

Gene Ontology analysis

The clusters were analyzed for Gene Ontology (GO) annotations appearing in a statistically significant manner in the cluster, when compared to a background. The background was comprised of all expressed genes – a list of all genes expressed in at least one of the four samples. For each GO term the number of genes with this term in a cluster was compared to the number of genes with this term in the background. Additionally the ratio between number of genes in the cluster and number of gene in the background was calculated. The two ratios served to calculate a p-value, and terms with a p-value lower than 0.01 were listed. The analysis was done using GO Tree Machine (GOTM) [71], the 08/09/04 version. For verification, the same functional analysis was done on Human and Mouse orthologs (provided by Affymetrix 29/07/04), using the EXPANDER software suite [72].

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Acknowledgements

This study is a partial fulfillment of Uri David Akavia's requirements towards his PhD thesis at Tel Aviv University, Israel. The study was supported by CellProM Grant from the EEC and a grant from Tel-Aviv University to DB.

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Correspondence to Dafna Benayahu.

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UDA carried out the computational analysis, IS carried out the molecular studies. DB conceived of the study, designed and coordinated it. The GeneChip hybridization was performed at the Functional Genomics unit, The Chaim Sheba Medical Center and Sackler School of Medicine headed by GR. All authors helped to draft the manuscript, read and approved the final manuscript.

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Akavia, U.D., Shur, I., Rechavi, G. et al. Transcriptional profiling of mesenchymal stromal cells from young and old rats in response to Dexamethasone. BMC Genomics 7, 95 (2006). https://doi.org/10.1186/1471-2164-7-95

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