Abstract
Visceral white adipose tissue (vWAT) expands and undergoes extensive remodeling during diet-induced obesity. Much is known about the contribution of various stromal vascular cells to the remodeling process, but less is known of the changes that occur within the adipocyte as it becomes progressively dysfunctional. Here, we performed a transcriptome analysis of isolated vWAT adipocytes to assess global pathway changes occurring in response to a chronic high fat diet (HFD). The data demonstrate that the adipocyte responds to the HFD by adopting a fibroblast-like phenotype, characterized by enhanced expression of ECM, focal adhesion and cytoskeletal genes and suppression of many adipocyte programs most notably those associated with mitochondria. This study reveals that during obesity the adipocyte progressively becomes metabolically dysfunctional due to its acquisition of fibrogenic functions. We propose that mechano-responsive transcription factors such as MRTFA and SRF contribute to both upregulation of morphological genes as well as suppression of mitochondrial programs.
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Introduction
Obesity continues to be a global health issue with the prevalence rising in not only adults but also children1. Weight gain due to excess nutrition leads to expansion and remodeling of the adipose tissue2. Healthy adipocytes maintain a remarkably high degree of plasticity; quickly responding to whole body energy demands either through the release of fatty acids and glycerol, storage of excess calories as triglycerides and/or secretion of adipokines. The unique ability of the adipocyte to regulate its size through dynamic expansion or shrinkage requires continual remodeling of the tissue environment, specifically the extracellular matrix (ECM)3,4,5,6. The ECM is an important component of adipose tissue as it provides adipocytes with structural support and protection from mechanical stresses as well as serving as a reservoir of growth factors and cytokines7,8,9. Remodeling in healthy adipose tissue involves the continuous turnover of ECM proteins by a cycle of matrix deposition and degradation by enzymes such as metalloproteinases (MMPs)10. The maintenance of a pliable ECM is necessary to maintain the homeostasis of the tissue through the unrestricted expansion and contraction of adipocytes3,4. In addition to ECM turnover, angiogenesis within the fat pad keeps up with the expansion rate during healthy remodeling, ensuring that the tissue remains well oxygenated11. Maintenance of a flexible ECM is also necessary to allow for adipocyte progenitor cells to traverse to areas where new adipocytes are required5.
Unhealthy remodeling of adipose tissue due to over feeding involves enhanced deposition and decreased degradation or turnover of ECM, combined with an increase in crosslinking and stiffening of ECM fibers ultimately leading to adipocyte dysfunction, reduced adipogenic capacity and fibrosis with all contributing to whole body metabolic dysfunction, including type 2 diabetes and cardiovascular complications12,13. Indeed, deletion of collagen 6 (col6), a component of the ECM that has enriched expression in adipose tissue, resulted in improved glucose tolerance and decreased liver triglycerides when challenged with an ob/ob background or a high fat diet14. Obesity-related remodeling also includes a change in various cell populations of the stromal vascular compartment. In lean individuals, adipose tissue is primarily composed of M2 macrophages, eosinophils, Tregs and ILCs that suppress inflammation. Whereas obesity is accompanied by an infiltration of B cells and various T cells (i.e. NK and Th1 cells) and polarization of M1 macrophages as well as a reduction in Tregs and ILCs leading to inflammation and associated insulin resistance. Secretion of proinflammatory cytokines also lead to expansion of profibrotic cells (ECM producing cells such as myofibroblasts) in addition to the inflammatory immune cells15.
In contrast to our extensive understanding of the many changes occurring in the stromal cell compartment of adipose tissue with obesity, less is known about the adipocyte-specific processes leading to an unhealthy adipocyte. The goal of this study was to evaluate the transcriptional response to HFD in isolated adipocytes. Our data demonstrate that adipocytes respond to a HFD by adopting a more fibroblast-like phenotype characterized by enhanced expression of ECM, cell adhesion and cytoskeletal genes along with suppression of adipocyte programs most importantly mitochondrial-related and lipolytic genes. Eventually, with prolonged high fat diet the transcriptional signature of the adipocyte is extensively altered from that of a healthy functional fat cell. We discuss the potential role of the morphological changes and associated transcriptional regulators in not only upregulating fibroblast-like genes but also in suppressing normal adipocyte functions.
Methods
Animal studies
C57BL/6J male mice were purchased from Jackson Laboratories (stock number 000664) and fed either a high fat diet (HFD) containing 60% kcal from fat (D12492; Research Diets) or control chow diet (D12450B or D12450K; Research Diets) starting from 6 weeks of age for 8, 20 or 34 weeks. Mice were maintained on a standard 12 hr light/dark cycle with ad libitum access to food and water. Bodyweights were measured prior to study and at the end of the study under fed conditions. On the final day of each study timepoint, mice were fasted for 6 hours (4:00–10:00am) by the removal of food but with free access to water. Mice were euthanized using carbon dioxide asphyxiation followed by cervical dislocation. All harvested tissues were weighed, and then either wrapped in foil and immediately snap-frozen in liquid nitrogen (LN2) or fixed in 10% neutral-buffered formalin for histological analysis. Subcutaneous adipose tissue was harvested from the inguinal region by carefully pulling the skin back from the flanks to reveal the triangular fad pads. Perigonadal adipose tissue, also known as epididymal adipose tissue, was harvested from the region surrounding the testes. With both adipose depots, careful attention was made to exclude lymph nodes during dissection At the completion of the study, tissues were stored at −80 °C.
All experimental protocols performed on animals were in accordance with regulations and established guidelines and were reviewed and approved by Institutional Animal Care and Use Committee (IACUC) at Pfizer Inc, Cambridge, MA.
Adipose tissue fractionation
Dissociation media was prepared by adding 2 grams of bovine serum albumin (BSA) to 100 mL of 4.5 g/L glucose DMEM media (Invitrogen) and warmed in a 37 °C water bath to dissolve. Adipose tissue was dissected at the termination of the study. The fat pad was rinsed with PBS before being gently minced in dissociation media with scissors and a razor blade. The minced tissue was then digested by transferring to a 50 mL falcon tube containing 25 mL of 1 mg/mL type I collagenase (Worthington) dissolved in dissociation media and placed in a 37 °C water bath with gentle shaking for approximately 40 minutes. The dispersed tissue was then passed through a 100 µm mesh filter and centrifuged at 200xg for 10 minutes. The floating adipocytes were carefully removed and added to a tube containing approximately 5 volumes of trizol (Qiagen) and immediately snap frozen in a bath of LN2. The pelleted SVF was resuspended in erythrocyte lysing buffer (155 mM NH4Cl, 10 mM KHCO3, 1 mM EDTA), incubated at room temperature for 3 minutes and then centrifuged at 200xg for 10 minutes. Pelleted SVF was resuspended in 2 mL trizol (Qiagen) and immediately snap frozen in a bath of LN2. Cell fractions were stored at −80 °C.
Body composition analysis
After 34 weeks of HFD, the relative total body fat mass and lean mass of mice was assessed by MRI scanning with an EchoMRI 700 instrument.
Plasma collection and analysis of circulating plasma parameters
Whole blood was collected by cardiac puncture using a 26 G needle immediately following euthanasia by carbon dioxide and cervical dislocation. Whole blood was added to K2EDTA-containing collection tubes, gently inverted to mix and stored on ice before being centrifuged at 13,800xg for 10 minutes at 4 °C. Plasma was carefully removed and transferred to clean, pre-chilled microcentrifuge tubes on ice and analyzed immediately or stored at −80 °C for analysis at a later time. Glucose, ALT, AST, cholesterol, NEFA, glycerol, triglycerides and lactate were measured using a Siemens Advia 1800 Chemistry Analyzer (Siemens). Insulin was measured using Stellux Chemi Rodent Insulin ELISA kits (Alpco). Leptin was measured using Luminex magnetic bead assay kit (Thermofisher) according to manufacturer instructions.
Histology and staining
Perigonadal adipose and liver tissues were processed with a standard paraffin-embedding protocol after fixation in 10% neutral-buffered formalin (Fisher Scientific), cut into 5 µm sections and mounted onto slides (Charles River). H&E staining was done by Charles River laboratories using their in-house protocols. Elastin staining was performed using an Elastica van Gieson staining kit (Millipore) according to manufacturer instructions. Picrosirius red staining was performed as previously described16,17. Bright field images for all stained tissue sections were captured with an Axio scan Z1 imager (Zeiss) with a 20x/0.8 objective. Digital zoom was used to select regions of interest and zoomed regions were cropped.
Immunofluorescence of paraffin-embedded tissue sections
5 µm slices of paraffin-embedded perigonadal adipose tissue were mounted onto slides, deparaffinized and rehydrated before performing antigen retrieval. A Decloaking Chamber NxGen (Biocare Medical) was used for antigen retrieval according to manufacturer instructions. Briefly, slides were submerged in citrate buffer (10 mM sodium citrate, 0.05% tween-20, pH 6.0) and incubated for 15 minutes at 90 °C in the decloaking chamber. The slides were then cooled by submerging in room temperature water for 5 minutes and then rinsed twice with cold 0.1% tween-20 in tris-buffered saline (TBS) for 5 minutes. After the slides were rinsed, they were transferred to blocking solution (10% normal goat serum, Thermofisher) supplemented with 0.3 M glycine and 0.1% tween-20 and incubated at room temperature for 1 hour. After blocking, slides were rinsed twice with 0.1% tween-20 in TBS at room temperature. Wax circles were then drawn around the tissues and primary antibodies that had been diluted in 0.1% tween-20 TBS + 5% BSA as in Table 1 were applied and incubated overnight at 4 °C. The next day, slides were washed three times with 0.1% tween-20 TBS at room temperature. Secondary antibodies were diluted in 0.1% tween-20 TBS + 5% BSA along with DAPI as in Table 1. Slides were incubated with secondary antibodies in the dark for 1 hour. Slides were then washed three times with 0.1% tween-20 TBS at room temperature in the dark. Coverslips were mounted using Prolong gold antifade (Thermofisher). Fluorescent images for all stained adipose tissue sections were captured with an Axio scan Z1 imager (Zeiss) at 20x magnification. All chemicals were purchased from Sigma Aldrich.
Fluorescent images for all stained adipose tissue sections were captured with an Axio scan Z1 imager (Zeiss) with a 20x/0.8 objective. All images were compared against background control slides containing secondary fluorophore-conjugated antibodies only. Histogram display adjustments were made for each fluorophore and were kept the same across samples. Digital zoom was used to select regions of interest and zoomed regions were cropped.
Frozen tissue preparation
Frozen adipose tissue was powdered by gently hammering in foil on a metal pedestal partially submerged in LN2. Frozen pieces of tissue were hammered until pulverized to a fine, uniform powder and then transferred to a vial, pre-chilled in LN2. Powdered tissues were then returned to −80 °C for storage or prepared for further analysis.
Protein isolation and western blot analysis
Total adipose tissue lysates were made by scooping approximately 200 mg powdered adipose tissue (prepared as described above) into a microcentrifuge tube on ice containing 400 µL RIPA buffer (ThermoFisher) supplemented with 1% triton X-100 (Sigma) and 1x protease and phosphatase inhibitor cocktail (Cell Signaling Technologies). After vortexing to ensure thorough mixing, samples were sonicated for 2 rounds of 3 seconds at 30 mHz with a brief pause in between rounds. Careful attention was paid to ensure the samples did not warm during sonication. After sonication, the samples were cleared by centrifugation at 18,800xg for 15 minutes at 4 °C. The supernatant was careful removed, avoiding the lipid cake at the surface as well as particulates at the bottom of the tube. The supernatant was transferred to a clean, pre-chilled microcentrifuge tube and cleared again as described above. After clearing, protein concentrations were determined by BCA assay (Pierce). For western blot analysis, equal amounts of protein from cleared tissue lysates were prepared with 4x Nupage LDS loading buffer (ThermoFisher) and 1x reducing agent (DTT; ThermoFisher) before being heated for 10 minutes at 70 °C. After a brief cooling period until no longer warm to the touch, the samples were loaded into 26 lane 4–20% Tris-Glycine midi gels (Biorad) and separated by SDS-PAGE according to manufacturer instructions (Biorad). After SDS-PAGE was complete, the proteins were then transferred to a pre-activated and transfer buffer equilibrated polyvinylidene difluoride (PVDF) membrane (Biorad) by wet tank transfer. The wet transfer conditions were 90 minutes at 85 V keeping the transfer chamber cold with an internal ice pack and surrounding the chamber with ice. Transfer buffer was 1x Tris/Glycine transfer buffer (Biorad) supplemented with 20% methanol (Fisher). Following transfer, PVDF membranes were blocked with 5% non-fat milk (Biorad) in tris-buffered saline supplemented with 0.2% tween-20 (TBS-T; 50 mM Tris-Cl, pH 7.5, 150 mM NaCl, 0.2% tween-20) for 1 hour at room temperature with gentle rocking. Membranes were then rinsed with TBS-T before being incubated overnight at 4 °C with gentle rocking. Primary antibodies prepared in 5% BSA/TBS-T with dilutions specified in Table 1. The following day, primary antibodies were removed and the membranes were washed 3 × 5 minutes with TBS-T buffer. After washing, membranes were incubated with appropriate HRP-linked secondary antibodies diluted in 5% non-fat milk in TBS-T for 1 hour at room temperature with gentle rocking. Membranes were then washed 3 × 5 minutes with TBS-T buffer. Proteins were detected using SuperSignal West Femto Maximum Sensitivity Substrate kit (ThermoFisher). Membranes were exposed and images were captured using a ChemiDoc XRS + system (Biorad) with careful monitoring of exposure time to avoid saturation of signal. All antibodies and dilutions used are listed in Table 1. Densitometry analysis was done using Image Lab 5.2.1 software (BioRad).
RNA and cDNA preparation
Isolated adipocytes and stromal vascular cells snap frozen in trizol were thawed on ice and then transferred to Fastprep matrix D lysing tubes (Mp Biomedicals) for homogenization using a Qialyzer instrument (Qiagen). Cells were homogenized with 2 cycles of 2 minutes at 20 1/s frequency, rotating tubes within holders (outside to inside and vice-versa) between rounds. RNA was extracted from the tissue homogenates using the RNeasy Lipid Tissue Mini kit and the Qiagen user-developed protocol titled Purification of total RNA from fatty tissues using the RNeasy Lipid Tissue Mini Kit and MaXtract High Density (Qiagen). On-column DNA digest was performed for all samples according to manufacturer protocol (Qiagen). RNA was quantified using a Nanodrop 8000 spectrophotometer and quality was assessed using an Agilent 4100 Bioanalyzer (Agilent). cDNA was synthesized from RNA using High-capacity cDNA reverse transcription kits (Applied Biosystems).
Gene expression
Real-time quantitative PCR (qPCR) was performed with a Quantstudio 7 flex instrument (Applied Biosystems) using Taqman Fast advanced mastermix (Applied Biosystems) and appropriate taqman probes for the genes of interest. Relative expression was normalized to housekeeping genes (Ppia and Tbp). All taqman probes were purchased from ThermoFisher and are listed in Table 2.
RNAseq library preparation
cDNA libraries for RNA-seq analysis were prepared from total RNA (isolated as described above) according to Illumina TruSeq stranded mRNA sample prep LS protocol. Pooled sample libraries were sequenced on Nextseq. 500 instrument with Nextseq. 500/550 High output kit, 150 cycles (Illumina).
Gene expression profiling (read mapping, quantification and differential expression)
Stromal vascular fraction analysis
Raw sequencing reads were subjected to quality control analysis via FastQC18 and reports aggregated via MultiQC19. Reads were then trimmed based on a sliding window and presence of adapter sequences using Trimmomatic20 set to the following parameters: ILLUMINACLIP::2:30:10 LEADING:3 TRAILING:3 SLIDINGWINDOW:4:15 MINLEN:50. Salmon21 was used to quantify the expression of transcripts to a reference transcriptome containing protein coding and long non-coding RNAs from the gencode M10 annotation before aggregation to the gene level. Only genes with a raw count of greater than 5 and present in at least half of the replicates were used for downstream analysis. Normalization and differential expression were performed using DESeq222 set to default parameters. All raw sequencing data has been deposited to Gene Expression Omnibus record number GSE138242.
Isolated adipocytes analysis
The raw RNA-seq fastq files were processed using the count-based differential expression analysis best practice protocol23 to quantify for gene expression. Accordingly, sequencing reads were aligned to the mouse genome mm10 using the STAR aligner24. FeatureCounts was used to count the number of reads unambiguously overlapping each gene, where each gene was considered to be the union of its exons25 with GENCODE annotation (vM2 for mouse). Sample normalization factors were computed using the EdgeR TMM method26. Unless otherwise stated, all counts per million (CPM) and log2CPM values are computed using these normalization factors. We converted the gene symbols to Entrez IDs using the annotations in the mygene.info package27. Of the 38924 genes, 9690 gene symbols did not have an associated Entrez ID and were discarded from this study. Only genes with gene-expression data above log2CPM of 2.0 were considered expressed, filtering the rest, resulting in a gene list of 11600 informative genes. The resulting genes with Entrez IDs correspond to the set of ‘background or detected genes’ consisting of 11600 genes. The biological replicates for each condition were pooled for differential expression analysis. Genes with a q-value of < 0.05 were considered significantly differentially expressed. All raw sequencing data has been deposited to Gene Expression Omnibus record number GSE142187.
Transcriptional pathway analysis of RNAseq data
Differentially expressed genes were selected based on padj < 0.05. GSEA pathway enrichment analysis was conducted on differentially expressed gene lists that were ranked by logFC28,29. Lists of differentially expressed genes were also analyzed for enriched GO terms30,31 using the online EnrichR tool32,33 and Revigo34. Differentially regulated genes associated with mitochondria were identified by comparing gene lists to the MitoCarta35,36.
Statistical analysis
Data were analyzed using GraphPad Prism 7 software (GraphPad) and are presented as mean ± standard error of mean (SEM). Group comparisons were analyzed using either two-tailed unpaired student t test or a two-way ANOVA followed by multiple comparisons correction method stated in figure legend. Differences were deemed statistically significant with p < 0.05.
Results
Diet-induced obesity leads to progressive metabolic impairment over 34 weeks
To begin to evaluate adipose tissue remodeling in the context of weight gain and progression of obesity, we fed C57/Bl6J mice either chow diet (CD) or 60% high fat diet (HFD) over a time course of 8, 20 and 34 weeks starting from 6 weeks of age. Most HFD diets studies have analyzed the effect of the diet on overall metabolism for relatively short periods (8–20 weeks). Here, we were interested in determining what effect a chronic diet (34 weeks) would have on the mice compared to their normal weight gain with age. As anticipated, mice fed either CD or HFD gained weight as time progressed and mice fed HFD gained significantly more weight compared to CD groups at all time points (Fig. 1A). Body composition analysis revealed that after 34 weeks of HFD, total lean mass was modestly increased, and total fat mass increased approximately 2-fold compared to CD group (Fig. 1A). In agreement with weight gain, both subcutaneous and perigonadal adipose depots expanded in mass. Subcutaneous fat pads were larger and continued to increase in weight with time compared to perigonadal fat pads that had reached a plateau from the 8 weeks of HFD timepoint (Fig. 1B). Examination of perigonadal adipose tissue cross sections stained with Hematoxylin and Eosin (H&E) revealed that HFD led to larger adipocytes but also enhanced staining intensity surrounding the adipocytes compared to CD at all times (Fig. 1C). Next to gain insight into the metabolic health of the mice, we measured fasting insulin, cholesterol, NEFA and leptin in the plasma. Fasting insulin and circulating cholesterol were elevated with HFD at all times (Fig. 1D) compared to CD. Circulating NEFAs were transiently increased in the CD with time and were decreased in the HFD group at all times (Fig. 1D). Circulating leptin rose in a similar pattern to the expansion of subcutaneous fat pads (Fig. 1B,D) in response to HFD compared to CD. Liver weight and circulating enzymes associated with liver damage, alanine aminotransferase (ALT) and aspartate transferase (AST), were significantly elevated after 34 weeks of HFD (Supplementary Fig. 1A,C) compared to CD. Progressive lipid accumulation in the liver in the HFD groups was also evident by H&E staining of tissue sections (Supplementary Fig. 1C). Thus, collectively confirming that HFD-fed mice were becoming increasingly metabolically impaired over time. Moreover, the age-associated changes in mice fed chow seem to recapitulate some of the HFD phenotypes at earlier time points. Immunofluorescent staining of the perigonadal adipose tissue sections with a macrophage marker, F4/80, confirmed that the clustering around adipocytes was populated with macrophages (Fig. 1E). Assessment of CHOP expression, a marker of ER stress37, by immunofluorescent staining after 34 weeks of HFD revealed elevated expression within the crown-like structures surrounding the adipocytes (Fig. 1E). Furthermore, CHOP expression colocalized more frequently with F4/80 expression in the HFD-fed group (Fig. 1E) compared to CD group.
Adipocytes upregulate expression of extracellular matrix genes in response to high fat diet
To specifically analyze the 2 main cell fractions of adipose tissue, adipocyte (AF) and stromal vascular fractions (SVF), the perigonadal depot (PGWAT) was digested with collagenase as briefly outlined in Fig. 2A. Gene expression was assessed in both PGWAT fractions by qPCR for a selected set of genes associated with extracellular matrix (ECM) and tissue remodeling (Fig. 2B). The gene expression of these remodeling markers in the SVF cells appeared to be influenced greater by age than by HFD as shown by similar fold increases and pattern of gene expression between the 2 diet groups (Fig. 2B, left panel). Expression of collagens (col1a1, col4a1, col6a3) and fibronectin (fn1) were similarly upregulated in SVF from CD and HFD groups at 34 weeks (Fig. 2B, left panel). Tissue remodeling enzymes mmp2, mmp9, mmp11 and timp1 expression was also similar between the groups (Fig. 2B, left panel). TGF-β1 (tgfb1), its receptors (tgfbr1, tgfbr2) as well as expression of its target genes (itga5, acta2, ctgf, serpine) were all similarly expressed in SVF cells in response to HFD and time (Fig. 2B, left panel). One marker that was more strongly upregulated in response to high fat compared to CD in SVF was tnc. Tnc is a pro-fibrotic glycoprotein that has been shown to contribute to tissue remodeling and fibrosis through its interaction with toll-like receptor 4 (TLR4), a receptor associated with pro-inflammatory responses38,39,40,41. In contrast to SVF cells, AF cells responded strongly to high fat stimulus compared to CD (Fig. 2B, right panel). Expression of collagens (col1a1 and col6a3), fibronectin (fn1) were strongly upregulated in the AF from HFD PGWAT starting at 8 weeks and progressing to 34 weeks compared to CD adipocytes (Fig. 2B, right panel). Expression of matrix metalloproteinases, mmp2 and mmp11, were elevated in response to HFD, and a tissue inhibitor of metalloproteinases, timp1, displayed a similar expression pattern for diet and time (Fig. 2B, left panel). Tgfb1, inhba, itga5 and ctgf were all strongly upregulated in response to HFD at 20 and 34 weeks compared to CD (Fig. 2B, left panel). In contrast to SVF, tnc was strongly downregulated in the AF by 34 weeks independent of high fat stimulus (Fig. 2B, left panel). Given the increased expression of multiple ECM and tissue remodeling genes, we next assessed PGWAT tissue cross sections with histological staining for collagen (Picro Sirius Red) and elastin (Elastica van Gieson). Pericellular collagen staining was particularly apparent after 20 and 34 weeks HFD compared to CD (Fig. 2C, top panel), and became localized around the larger adipocytes at 34 weeks in the PGWAT of both CD and HFD mice (Fig. 2C, top panel). Elastin staining was similar to that of collagen (Fig. 2C, bottom panel). Interestingly, both collagen and elastin staining displayed the highest intensity in the areas of the tissue in which there was obvious SVF remodeling, the macrophage-enriched crown-like structures surrounding the dying adipocytes42. It has been shown that adipose tissue macrophages associate with elastin fibers and that macrophages are the predominant producers of MMP-12, a degrading enzyme for elastin, suggesting that macrophages play an active role in elastin remodeling43. Curiously, there appeared to be a transient increase in overall elastin staining in the 20 week CD group (Fig. 2C, bottom panel). This is interesting because it occurred before the tissue went on to nearly triple in weight by the 34 week timepoint, perhaps suggesting a time of remodeling in response to an unknown stimulus. Alpha smooth muscle actin (α-SMA) immunofluorescent staining of perigonadal tissue sections revealed an interesting pattern in CD mice (Fig. 2D). At 8 weeks, the expression of α-SMA appeared to be confined to cells distributed throughout the tissue, which then became more ordered around adipocytes by 20 weeks (Fig. 2D). Intriguingly at 34 weeks, α-SMA expression was delicately outlining the adipocytes in addition to concentrating between them in areas of higher nuclei density (Fig. 2D). In comparison, α-SMA positive cells in the 34 week HFD group appeared to have concentrated localization (Fig. 2D). These cells could be myofibroblasts and/or blood vessel cells.
Adipocytes exert a robust transcriptional response to high fat diet
To take an in-depth look at the transcriptional changes occurring globally within the different fractions of the PGWAT, we conducted RNA-seq analysis on the isolated SVF and adipocytes of CD and HFD fed mice at 8, 20 and 34 weeks. After 8 weeks, the number of differentially expressed genes (DEGs) in the SVF in response to HFD was limited to a few hundred (Supplemental Fig. S2A,B). Interestingly after 20 weeks of HFD the number of DEGs substantially increased in the SVF before a subsequent overall decrease at 34 weeks (Supplemental Fig. S2A,B). Conversely, the adipocytes appeared to respond more strongly to HFD. After 8 weeks of HFD, the number of DEGs in adipocytes was approximately 5500 genes (Supplemental Fig. S2A,B). After 20 weeks, the number of DEGs in adipocytes reached a maximum, as was seen in the SVF, before modestly decreasing in total number by 34 weeks (Supplemental Fig. S2A,B).
Principal component analysis of the adipocytes revealed clustering of the diet groups and timepoints. This analysis facilitates a high level overview of similarities and differences between the samples and groups in relation to how they cluster44 (Fig. 3A). 8 and 20 week CD samples clustered closely together and the groups partially overlapped, suggesting similarities between them (Fig. 3A). 8, 20 and 34 week HFD samples clustered together within their respective groups and were near each other however there was no overlap between any of the groups (Fig. 3A). Thus suggesting that high fat was eliciting global transcriptional changes leading to high level differences between the groups at earlier timepoints compared to CD. Intriguingly, the 34 week CD samples clustered nearer the 8 and 20 week HFD groups than the 8 or 20 week CD groups (Fig. 3A). This is consistent with the data in Fig. 1, which showed that changes in metabolic parameters following 34 weeks of chow diet were similar to those resulting from 8 or 20 weeks of HFD. Hierarchical clustering analysis highlighted the directional changes occurring globally within the different diet groups and timepoints (Fig. 3B). To perform a more detailed transcriptional profiling of the adipocytes, we took a reductionist approach to correct for any carryover of the SVF into the adipocyte fraction. An overview of the workflow is detailed in (Fig. 3C). After selection of DEGs (both up and downregulated) from the SVF and adipocytes in response to HFD compared to CD based on padj < 0.05, the lists were overlaid at each timepoint to reveal genes that were differentially expressed only in the SVF (Fig. 3C, first row of Venn diagrams, green color), in the adipocyte fraction (Fig. 3C, first row of Venn diagrams, red color) or in both fractions (Fig. 3C, first row of Venn diagrams, brown color) at each of the times. Next, we took the lists of DEGs that were specifically changing in the adipocyte fraction from each of the timepoints (Fig. 3C, first row of Venn diagrams, orange color) and overlaid them using a final Venn diagram (Fig. 3C, lower Venn diagram with 3 circles). This final comparison allowed us to identify DEGs that were differentially expressed across all timepoints (Fig. 3C, lower Venn diagram, bright green color) or specifically at each timepoint (Fig. 3C, lower Venn diagram, blue, pink and yellow colors). Once these lists were made, GO term enrichment analysis was performed to determine the dominant pathways that were changing in the adipocytes in response to HFD at 8, 20 and 34 weeks as well as what pathways were in common over all timepoints.
Upregulation of ECM and remodeling-related genes and pathways in high fat diet adipocytes
641 DEGs were maintained upregulated over all timepoints in response to high fat stimulus in isolated adipocytes (Fig. 4A, green color). GO term analysis revealed enrichment of pathways related to extracellular matrix organization, cytoskeleton, focal adhesion and others (Fig. 4B, green color). GO terms and associated genes for Fig. 4B are listed in [Supplemental Fig. 3. Notably, pro-fibrotic cytokine TGF-β1 (Tgfb1) expression was found to be upregulated in adipocytes at all times. 8 weeks of HFD lead to upregulation of 889 genes which were surprisingly not significantly associated with any GO terms (Fig. 4A, blue color). By 20 weeks of HFD, adipocytes significantly upregulated 650 genes associated with Wnt signaling, negative regulation of cell growth, positive regulation of cell differentiation and microtubule polymerization (Fig. 4A,B, pink color). Genes associated with these GO terms, including other TGF-β ligands tgfb2 and tgfb3, are listed in Supplemental Fig. 3. Thirty four weeks of HFD lead to 992 genes uniquely upregulated (Fig. 4A, yellow color) which equated to the enrichment of GO terms associated predominantly with RNA metabolic process, lysosome, cadherin binding, cytoskeleton, focal adhesion and others (Fig. 4B, yellow color). 34 week upregulated GO terms and associated genes are listed in Supplemental Fig. 3.
Upregulation of a subset of ECM and remodeling genes in the isolated adipocytes with HFD was evident after calculating the Log2FC from RNAseq TPM values (Fig. 4C). Collagens (col1a1, col6a3), elastin (eln), fibronectin (fn1), TGFB family members (tgfb1), and integrins (itga5) were all upregulated in adipocytes in response to a HFD. Next, we examined collagen 6 (COL6), an enriched collagen in adipose tissue14, and f-actin expression (using phalloidin45) by immunofluorescent staining of PGWAT tissue sections (Fig. 4D). We found that both proteins were more prominent with HFD, particularly at the later timepoints (Fig. 4D). Interestingly, by 34 weeks HFD the phalloidin staining was more punctate than in previous timepoints (Fig. 4D). COL6 signal appeared to decrease in CD mice over the time, suggesting active degradation and remodeling was occurring in response to the expanding adipocytes.
Downregulation of mitochondrial genes and GO terms in high fat diet adipocytes
Adipocytes had a similar number of downregulated genes at each timepoint as those being upregulated (Fig. 5A). Notably, 580 genes were downregulated at all times and of these genes the top GO term was mitochondrion (Fig. 5A,B, green color, Supplemental Fig. S4). After 8 weeks of HFD, 1087 genes were downregulated specifically at this time (Fig. 5A, blue color). These genes enriched for GO terms primarily related to RNA processing and transcription (Figs. 5B and S4). After 20 weeks of HFD 661 genes were downregulated, out of which 72 were associated to the top enriched GO term mitochondria (Fig. 5, pink color and Supplemental Fig. S4). Other downregulated GO terms were associated with the peroxisome and ubiquitination. After 34 weeks of HFD, 857 were found to be specifically downregulated and GO terms associated with the mitochondrion became more prevalent including mitochondrion inner membrane, mitochondrial translation and mitochondrion (Fig. 5, yellow color and Supplemental Fig. S4). Given the known concept of mitochondrial dysfunction occurring during obesity, we next examined proteins important for adipocyte function (lipolysis) and health (adiponectin)46. Western blot analysis of total PGWAT lysates showed a decrease in lipolytic enzymes, ATGL and phosphorylated ser563 HSL, a PKA site that leads to activation of HSL47, after 8 weeks of HFD (Fig. 5C). Total HSL and MAGL expression declined at the later 20 and 34 week times (Fig. 5C). Adiponectin also decreased after 20 weeks of HFD and continued to decrease during the remainder of the 34 weeks (Fig. 5D). Immunofluorescence of cleaved caspase-3 (a marker of autophagy48) appeared dispersed and relatively small in area in 8 week CD, becoming more scarce with time however larger in area. 8 week HFD treatment resembled the 34 week CD. HFD treatment lead to increasing cleaved caspase-3 activity during the 34 week period suggesting increased apoptosis with obesity (Fig. 5E).
Discussion
It is well documented that white adipose tissues particularly visceral depots undergo an extensive remodeling in response to high fat diet (HFD), which includes deposition of ECM and infiltration of proinflammatory immune cells. With time, HFD causes inflammation and fibrosis that results in dysfunctional adipose depots and disruption of metabolic homeostasis. Much is known about the contribution of the stromal cells (immune, vascular, fibroblasts etc) to the unhealthy remodeling, but little is known about the response or contribution of the adipocytes. In the present study, we performed a RNAseq analysis of isolated adipocytes to assess global pathway changes occurring in response to HFD. Our data reveal that adipocytes respond dramatically to the diet by enhancing expression of genes coding for ECM, focal adhesions and cytoskeleton, which is maintained throughout the entire 34 weeks of the diet. In fact, the transcriptional signature of the resultant pathological adipocytes resembles that expressed prior to their adipogenesis, i.e. more similar to fibroblastic-like cells. This is intriguing and somewhat controversial however there is precedence for adipocytes to revert to preadipocytes or fibroblast-like cells in other tissues undergoing remodeling in response to stress. Dermal adipocytes have the flexibility to transition to myofibroblasts49. In scleroderma, the skin undergoes extensive remodeling resulting in fibrosis of the tissue. Scleroderma myofibroblasts have been shown to originate from subdermal adipocytes49. The data further demonstrate that after 20 weeks of HFD, genes associated with Wnt signaling are significantly upregulated. Wnt signaling has been shown to be implicated in dermal fibrosis50. Furthermore, surgical-induced injury to subcutaneous fat pads in rats led to the dedifferentiation of mature adipocytes to cells with a fibroblast morphology51. Mammary adipocytes have been shown to dedifferentiate into PDGFRα + cells during lactation52. PDGFRα is an accepted marker of precursor cells53.
It is well accepted that adipose tissue becomes progressively fibrotic during diet-induced obesity due to the extensive deposition of ECM around adipocytes as well as blood vessels. In other organs, fibrosis is characterized by proliferation and differentiation of perivascular progenitors into myofibroblasts that reorganize and contract the ECM fibers providing mechanical stimulations within the tissues54,55,56,57. Recent studies suggest that similar mechanisms operate in adipose tissue and contribute to its unhealthy state58,59,60,61,62. Other studies have suggested that the adipocyte plays a central role in adipose fibrosis by expressing ECM genes in response to hypoxia63,64. Our data also support a role for the adipocyte but GO terms enrichment analysis of HFD upregulated genes suggests that pathways responsive to TGF-β are a principal regulator of adipocyte-specific production of ECM, focal adhesions and cytoskeleton. This does not exclude a role for hypoxia since its stimulation of collagen type VI and endotrophin could lead to release of TGF-β from immune cells65,66.
TGF-β regulates gene expression through several overlapping signaling/ transcription factor pathways including SMADs, JNK, ERKs and MRTFA/SRF. Our earlier studies have provided data implicating MRTFA as a factor contributing to diet-induced metabolic disruption of adipose tissue by regulating the fate of perivascular progenitors to favor fibrogenesis over adipogenesis60,67. The healthier phenotype of HFD fed MRTFA-deficient mice compared to controls could also be due to its absence in mature adipocytes thereby preventing conversion of healthy adipocytes to dysfunctional fibroblast-like cells. Similarly, absence of SMAD3 signaling protects mice from diet-induced obesity and insulin resistance in part by enhancing production of beige adipocytes in white adipose tissue68. SMAD3 might also have detrimental effects on obese adipocytes. Strategies to inhibit TGF-β signaling (SMADs and MRTFA) might limit the negative consequences of obesity by directly retaining the metabolic functions of adipocytes.
The dramatic acquisition of a more fibroblast-like program of gene expression will have a direct impact on the morphological integrity of the adipocyte. An important feature of a metabolically healthy adipocyte is its ability to expand and contract in response to lipid storage and release. The unique morphology of the fat cell facilitates these changes in volume due to formation of a cortical cytoskeleton surrounding the lipid droplet rather than an extensive network of filaments throughout the cytoplasm as in the case of fibroblastic cells. Such a filamentous network most likely forms in the obese adipocyte due not only to actin production but also expression of focal adhesions that anchor to ECM externally and cytoskeleton internally providing mechanical tension across the cell. A stiff ECM surrounding them but also an actin-cytoskeleton internally acting to constrain expansion of the adipocyte with accumulation of lipid. Early studies demonstrated the need to downregulate the cytoskeleton and ECM during adipogenesis in order to facilitate formation of a unilocular fat cell69,70.
Besides providing the adipocyte with its plasticity, the cortical cytoskeleton also contributes to the normal metabolic functions of the adipocyte such as glucose uptake71. It is also conceivable that adipocyte tubulins play a role in regulating mitochondrial activity72,73. Consequently, a dramatic rearrangement of actin and tubulin cytoskeleton could have a detrimental effect on normal adipocyte metabolic functions. In fact, our data show that in addition to upregulation of ECM and cytoskeletal genes, there is a corresponding down-regulation of other genes. Most notably, 580 genes were downregulated at all times and of these genes the top GO term was mitochondrion. Other programs down-regulated included those also playing central roles in normal healthy adipocyte functions including lipolysis and adiponectin production. Down-regulation of these programs could be related to changes in overall morphology but are more likely due to suppression of transcriptional factors and/or chromatin rearrangements by the same signaling pathways that upregulated ECM and cytoskeletal genes. As discussed earlier, MRTFA/MKL1 along with SRF respond to extracellular signals via the polymerization state of actin to enhance expression of the morphological genes74,75,76. These same factors however antagonize the activity of PPARγ67,77,78,79, which is a master regulator of genes controlling normal adipocyte functions including glucose uptake and mitochondrial activity. Therapies being developed for tissue fibrosis that target signaling pathways regulating TGFβ-associated transcription factors might be effective in preventing the decline in adipocyte-specific functions during obesity.
Change history
07 January 2021
The original version of this Article included references to Supplemental Files 1 and 2 with sequencing data. This data was deposited in GEO with accession number GSE142187, and therefore the supplemental files were removed in production. This has now been corrected in the HTML and PDF versions of the Article.
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Acknowledgements
We would like to thank David A. Beebe, Katherine Cialdea, Collin P. Crowley, Matthew Gorgoglione, Kenneth Kelly Jr. and Trenton Ross for their assistance during study take downs and tissue collection. Katherine Hales and the Pfizer WRDM Optical Microscopy Technology Center for helpful discussion and assistance. Angela Hadjipanayis and the Pfizer WRDM Next Generation Sequencing Technology Center for assistance with running RNAseq experiments. Evanthia E. Pashos for preliminary RNAseq analysis. Xaralabos Varelas and Matthew D. Layne for helpful discussion. This work was supported by NIH/NIDDK grants DK117161 and DK117163.
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J.E.C.J. contributed to study design, performing experiments, analysis of results, drawing schematic in Fig. 2 and manuscript preparation. N.R. aided in experiments and analysis of results. J.O. and R.G. contributed to analysis of results. V.P. and C.V. contributed to manuscript preparation. S.R.F. contributed to study design and oversight, analysis of results and manuscript preparation.
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During completion of these studies J.E.C.J., R.G., C.V. were employed by Pfizer Inc. Pfizer provided support in the form of salaries for these authors but did not have any additional role in the study design, data collection and analysis, decision to publish, or preparation of the manuscript. N.R., V.P. and S.R.F. declare no competing interests.
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Jones, J.E.C., Rabhi, N., Orofino, J. et al. The Adipocyte Acquires a Fibroblast-Like Transcriptional Signature in Response to a High Fat Diet. Sci Rep 10, 2380 (2020). https://doi.org/10.1038/s41598-020-59284-w
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