Abstract
Aims/hypothesis
Insulin resistance in skeletal muscle is a hallmark of type 2 diabetes. Therefore, we sought to identify and validate genes involved in the development of insulin resistance in skeletal muscle.
Materials
Differentially regulated genes in skeletal muscle of male obese insulin-resistant, and lean insulin-sensitive Zucker diabetic fatty (ZDF) rats were determined using Affymetrix microarrays. Based on these data, various aspects of glucose disposal, insulin signalling and fatty acid composition were analysed in a muscle cell line overexpressing stearoyl-CoA desaturase 1 (SCD1).
Results
Gene expression profiling in insulin-resistant skeletal muscle revealed the most pronounced changes in gene expression for genes involved in lipid metabolism. Among these, Scd1 showed increased expression in insulin-resistant animals, correlating with increased amounts of palmitoleoyl-CoA. This was further investigated in a muscle cell line that overexpressed SCD1 and accumulated lipids, revealing impairments of glucose uptake and of different steps of the insulin signalling cascade. We also observed differential effects of high-glucose and fatty acid treatment on glucose uptake and long-chain fatty acyl-CoA profiles, and in particular an accumulation of palmitoleoyl-CoA in cells overexpressing SCD1.
Conclusions/interpretation
Insulin-resistant skeletal muscle of ZDF rats is characterised by a specific gene expression profile with increased levels of Scd1. An insulin-resistant phenotype similar to that obtained by treatment with palmitate and high glucose can be induced in vitro by overexpression of SCD1 in muscle cells. This supports the hypothesis that elevated SCD1 expression is a possible cause of insulin resistance and type 2 diabetes.
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Introduction
Skeletal muscle is the major site of glucose utilisation and peripheral insulin action in response to nutritional challenges. It has long been known that dysregulation of fatty acid and lipid metabolism influences insulin signalling on various levels, leading to impaired glucose tolerance, decreased fatty acid oxidation and glycogen synthesis, and eventually resulting in insulin resistance and type 2 diabetes (reviewed in [1, 2]). In particular, increased lipid accumulation in muscle, determined as intramyocellular lipid content, is frequently associated with insulin resistance [3–6]. Recently, it has also been implied that the degree of saturation of body lipids affects metabolic actions such as insulin signalling [7]. Stearoyl-CoA desaturase-1 (SCD1) is involved in the biosynthesis of mono-unsaturated fatty acids and catalyses the introduction of a double-bond at the Δ9 position of stearoyl (C18:0) and palmitoyl-CoA (C16:0). The products of SCD1 activity, oleic (C18:1 N9) and palmitoleic acids (C16:1 N7), constitute the majority of the mono-unsaturated fatty acids found in phospholipids, cholesterol esters and triglycerides. SCD1 expression is triggered by sterol regulatory element binding protein 1c [8] and is therefore highly regulated by a variety of stimuli, including leptin [9], insulin [10], glucose [11], cholesterol [12], iron [13], peroxisome proliferators [14] and polyunsaturated fatty acids [15].
Male Zucker diabetic fatty (ZDF) rats are a well-established animal model of insulin resistance and type 2 diabetes. Although experiments addressing changes in the transcriptional regulation of distinct genes in the development of insulin resistance or upon different treatments have been published [16, 17], to our knowledge a genome-wide, tissue-specific scan of differentially expressed genes in skeletal muscle of young ZDF rats has not yet been reported. Here, we describe a genome-scale Affymetrix gene expression study of genes differentially expressed in skeletal muscle of male ZDF rats with developing insulin resistance and type 2 diabetes compared with lean insulin-sensitive controls. Since we observed highly elevated Scd1 expression in insulin-resistant and diabetic muscle of the obese ZDF rats, the impact of SCD1 on insulin signalling and glucose disposal in skeletal muscle was further investigated in a cellular model.
Subjects, materials and methods
Reagents
Chemicals were purchased from Sigma (Deisenhofen, Germany) and cell culture reagents from Invitrogen (Karlsruhe, Germany). Rat anti-haemagglutin (HA) 3F10 and anti-MYC 9E10 antibodies were purchased from Roche (Mannheim, Germany), rabbit anti-(phospho-)AKT and anti-IRS1 antibodies from Biosource (Solingen, Germany) or Upstate/Biomol (Hamburg, Germany), anti-phosphotyrosine antibody was from Santa Cruz (Heidelberg, Germany), anti-protein–tyrosine phosphatase b (PTPN1) antibody from Merck Bioscience (Schwalbach, Germany) and anti-beta-actin antibody from Sigma. Horseradish peroxidase-coupled secondary antibodies were from Amersham (Freiburg, Germany), Alexa Fluor 488-labelled anti-rat secondary antibody was from Molecular Probes (Karlsruhe, Germany).
Animals and sample preparation
Age-matched groups of obese male ZDF rats (Genetic Models Incorporated [GMI] fa/fa) and their lean littermates (GMI+/?) were purchased from Charles River (Sulzfeld, Germany). The rats were housed in pairs at 20°C on a 12-h light/12-h dark cycle with free access to water and standard rat diet (ssniff R/M-H; ssniff Spezialdiaeten, Soest, Germany) for 1 week upon arrival to allow recovery from transport. All experimental procedures were conducted according to the German Animal Protection Law. After 2 h of starvation (24 h for the group studied at 8 weeks of age), blood samples were drawn under terminal isoflurane. Tissue probes were excised rapidly and snap-frozen in liquid nitrogen. Determination of blood metabolic parameters was performed as described previously [18].
Affymetrix microarray analysis
Skeletal muscle probes (gluteus maximus, 150 mg) were lysed in RLT buffer (Qiagen, Hilden, Germany) with a homogeniser (UtraTurrax; Janke and Kunkel IKA Labortechnik, Staufen, Germany). Total RNA from the tissue lysates was isolated with the Qiagen RNeasy kit, including proteinase K digestion, DNase digestion and an additional RNeasy cleanup step, as recommended by the manufacturer. First- and second-strand cDNA syntheses were performed with 10 μg of each total RNA using SuperScript SSII RT polymerase system (Invitrogen) and a T7(dT)24 primer. Double strand cDNA was extracted with phenol–chloroform then precipitated with ethanol. Biotin-UPT- and -CTP-labelled cRNA was transcribed in vitro using the Enzo BioArray High Yield RNA Transcript Labeling Kit (Enzo Diagnostics, Farmingdale, NY, USA) and purified by RNeasy cleanup and ethanol precipitation. Aliquots of each total RNA and cRNA were monitored before and after the purification steps by UV spectrophotometry, agarose gel electrophoresis and BioAnalyzer RNA chips (Agilent, Boeblingen, Germany). cRNA samples (15 μg) were fragmented at 94°C for 35 min, added to hybridisation buffer and hybridised to RG-U34 A, B and C microarrays (Affymetrix, High Wycombe, UK) for 16 h at 45°C and 60 rev/min. Microarrays were washed and double-stained with streptavidin–phycoerythrin conjugate (Molecular Probes) and anti-streptavidin antibody, using methods described by Affymetrix. After washing, the microarrays were analysed in a confocal GeneArray Scanner (HP, Boeblingen, Germany) with Microarray Suite Version 4.0 software (Affymetrix). Quality control of each chip was performed according to the Affymetrix quality criteria, including mean average difference, raw intensity and 3′/5′ ratio of the housekeeping genes beta-actin and glyceraldehyde-3-phosphate dehydrogenase. Expression profiling data were analysed using the in-house software GECKO 2 [19]. Briefly, this software performed a global normalisation on all microarrays using a reference chip for each group of biological replicates and the 75th percentile of the median of all transcribed genes. Biological replicates were subsequently agglomerated and a new matrix containing ratios and p-values was generated by crosswise element-by-element concatenation of all chips in one age-group, and significance was assessed with Student’s t-test. Merging of the respective biological replicates of each age (6, 7 and 12 weeks) and phenotypic group (lean and obese) and subsequent filtering for p-values lower than 0.05 and changes in expression levels between the lean and obese groups higher than twofold resulted in the sets of differentially expressed genes reported here. The procedure we describe and the choice of a ratio of changes of at least twofold have been shown to ensure limitation of false positives and good reproducibility by alternative methods, e.g. quantitative RT-PCR (qRT-PCR) and Northern blotting [19, 20].
Quantitative real-time PCR
Total RNA (1 μg) was reverse-transcribed with the AMV-RT first-strand cDNA synthesis kit (Roche) in a 20 μl reaction volume. Reverse-transcribed single strand cDNA (2 μl) was used as a template for amplification in a Lightcycler using FastStart DNA Master Sybr Green according to the instructions of the manufacturer (Roche). Primers used were 5′-TGCTATGTTATCCTTTCTCTTG-3′ and 5′-GGACACTTAATACACGATGTT G-3′ (rat SCD1), 5′-CTTCTTCATCTTCACCTTCTTA-3′, 5′-GCCCTAAGTATTCAAGTTCTGT-3′ (rat solute carrier family 2, member 4 [SLC2A4, also known as glucose transporter 4, GLUT4]), 5′-AAGTCCCTCACCCTCCCAAAAG-3′ and 5′-CCTCAACACCTCAAACCACTCC-3′ (rat beta-actin). The correct sizes of the resulting fragments (121, 136 and 268 base pairs, respectively) were monitored by agarose gel electrophoresis. Total RNA contents were calculated using a concentration standard curve of the respective amplified fragments and normalised to expression levels of the housekeeping gene beta-actin. Confidence of the microarray data was assessed by TaqMan qRT-PCR of selected genes (covering a range of fold changes between +10.63 and −2.19), using the Applera TaqMan Universal PCR Master Mix and Pre-Developed TaqMan Assay Reagents on an ABI Prism 7900 device according to the instructions of the manufacturer (Applera, Norwalk, CT, USA). Endogenous RNA control 18S rRNA (Applera; 4310893E) was used for normalisation as an internal control. Table S1 of the Electronic Supplementary Material (ESM) summarises the design of primer and probe sequences and sequence identifiers of the commercially available primer and probe sets from Applera.
HPLC analysis of long-chain acyl-CoA species
HPLC analysis from freshly prepared KH2PO4 cell lysates was performed using a Waters Alliance 2690 system (2487 detector; Millennium 2010 chromatographic manager; Waters, Eschborn, Germany) as described elsewhere [18].
Cloning and plasmids
The complete open reading frame of human SCD1 was amplified from human skeletal muscle cDNA (Invitrogen) by PCR using primers 5′-CGGGATCCCGCCACCATGCCGGCCCACTTGCTGCAG-3′ and 5′-CCGCTCGAGCGGTCAAGCGTAGTCTGGGACGTCGTATGGGTACATGCCACTCTTGTAGTTTCC-3′. The 3′ primer introduced a sequence encoding a carboxy-terminal in-frame HA epitope tag. The resulting fragment and pcDNA3.1(+) hygro vector (Invitrogen) were digested with BamHI/XhoI and ligated to obtain pcDNA3.1(+) hygro-SCD1-HA. The identity of the construct was confirmed by sequencing.
Cell culture, transfections and immunofluorescence
Rat L6GLUT4myc myoblasts expressing MYC epitope-tagged SLC2A4 (GLUT4) [21] were kindly provided by A. Klip (Hospital for Sick Children, Toronto, ON, Canada). Cells were maintained in alpha-MEM supplemented with 10% FCS, antibiotics (penicillin–streptomycin) and 2 μg/ml blasticidin at 37°C in 5% CO2 and 95% humidity and were subcultured twice weekly. Transfections were carried out with L6GLUT4myc cells grown in six-well plates to 60% confluence, 2.5 μg plasmid DNA and Fugene 6 reagent (Roche), as recommended by the manufacturer. For all transient transfections and for stably selected cell clones, empty pcDNA3.1(+) hygro vector served as negative control (subsequently referred to as ‘wild-type’ [WT]). Stable single-cell clones were selected with 500 μg/ml hygromycin B, picked manually and expanded. SCD1-HA expression levels were determined by SDS-PAGE and Western blotting (NuPAGE; Invitrogen) using anti-HA 3F10 monoclonal (Roche), anti-rat horseradish peroxidase secondary antibodies and chemiluminescence detection (Amersham). For fatty acid treatment, palmitate was dissolved in ethanol at 70°C to obtain a 20 mmol/l stock solution and coupled at a concentration of 200 μmol/l to 0.75% (w/v) fatty-acid free BSA in cell culture medium for 1 h at 37°C to obtain a molar ratio of 2:1. Immunofluorescence assays were performed as described [22], using stable L6GLUT4myc SCD1-HA cells or L6GLUT4myc cells transiently transfected with pcDNA3.1(+) hygro SCD1-HA grown on coverslips to 70% confluence. SCD1-HA expression was detected using anti-HA 3F10 antibody (Roche) and anti-rat Alexa Fluor 488 antibody (Molecular Probes). Neutral lipid staining was performed with 1 μg/ml Nile Red (Sigma) in PBS for 10 min after fixation and permeabilisation of the cells. Nuclei were visualised using 1 μmol/l ToPro iodide in PBS (Molecular Probes). Confocal images were taken with a Leica TCS SP2 confocal laser scanning microscope.
2-Deoxyglucose uptake assay and analysis of insulin signalling
Stably transfected L6GLUT4myc cells were plated in 96-well Cytostar-T scintillating microplates (Amersham) at 3.0×104 viable cells per well. After 32 h the cells were serum-starved with alpha-MEM supplemented with 2% newborn bovine serum and antibiotics (penicillin–streptomycin) for 16 h. To analyse glucose uptake, the cells were washed twice in KRB, pH 7.3 (KRB), and incubated for 25 min with the given insulin concentrations in KRB. [14C] 2-deoxyglucose (0.01 MBq per well; Amersham) was added and the cells were incubated for another 25 min in a total volume of 150 μl per well. Reactions were stopped by adding 10 μmol/l cytochalasin B; plates were sealed and scintillation was measured in a Wallac Microbeta counter (Perkin Elmer, Rodgau-Juegesheim, Germany). Unspecific uptake was determined by incubating control wells with 20 μmol/l cytochalasin B and subtracted from each value. Insulin signalling was monitored in stably transfected L6GLUT4myc cells plated in 12-well plates upon direct stimulation with 10 nmol/l insulin for 15 min and subsequent lysis in 1-TBS, 1% NP-40, 2 mmol/l sodium vanadate, 2 mmol/l Pefabloc and 1 μg/ml leupeptin. Levels of IRS1 tyrosine phosphorylation were quantified after immunoprecipitation of the proteins with anti-IRS1 antibody (Cell Signaling, Frankfurt, Germany) and immunoblotting using a phosphotyrosine antibody (Santa Cruz) and anti-IRS1 antibody for normalisation. AKT1 phosphorylation levels were determined with anti-phospho-S473 AKT1 (Biosource) and anti-AKT1 (Upstate) antibodies and direct immunoblotting of the lysates. Protein concentrations were determined with BCA protein assay (Pierce, Bonn, Germany).
Statistical analysis
Data are means±SEM of at least three independent experiments or show a representative graph of several independently performed experiments with similar results, as appropriate. Statistical significance was determined with Student’s t-test (p-values below 0.05 were considered significant) using the SigmaStat 2.03 program (SPSS, Chicago, IL, USA). Quantitative RT-PCR gene expression and phosphorylation data were calculated as fold change compared with controls and are given in arbitrary units (mean set to 1.0).
Results
Skeletal muscle-specific gene expression profiles of insulin-resistant ZDF rats
To investigate early tissue-specific events in the development of insulin resistance in skeletal muscle, we examined 34 obese male ZDF (GMI fa/fa) rats and lean controls (GMI+/?) of three ages (6, 7 and 12 weeks; n=5–6). All obese ZDF rats exhibited the expected phenotype of increased weight gain and altered metabolic parameters (Table 1) compared with the respective age-matched controls. The 6- and 7-week-old obese ZDF rats showed the typical features of insulin resistance, such as hyperinsulinaemia (increased by 615 and 607% for the two ages, respectively; p<0.01) and elevated triglyceride levels (increased by 190 and 282%; p=0.04), but were normoglycaemic. The 12-week-old obese animals were already diabetic with hyperinsulinaemia (increased by 527%; p=0.04), hyperglycaemia (glucose and HbA1c increased by 288 and 169%, respectively; p=0.02 and p=0.04, respectively) and elevated triglyceride levels (increased by 639%; p=0.006).
To identify differentially expressed genes in skeletal muscle of these animals, we performed Affymetrix gene expression profiling using total RNA from gluteus maximus muscle and RGU-34A, B and C microarrays, covering in total 26,256 transcripts. An average of 3,724±69 (lean) and 3,701±65 (obese) transcripts were expressed in muscle (3,621 vs. 3,605 [lean vs. obese, 6 weeks]; 3,793 vs. 3,790 [7 weeks]; 3,757 vs. 3,707 [12 weeks]). The total number of differentially expressed genes was 119 transcripts for the comparison between lean and obese ZDF rats in the 6-, 7- and 12-week age groups. A complete list of the differentially expressed genes in the respective age groups is presented in the ESM (Tables S2–S4). Among the differentially expressed genes, there was a prevalence of genes involved in lipid metabolism, all of which were expressed more highly in insulin-resistant muscle (e.g. Cd36 [previously known as Fat], 2,4-dienoyl-CoA reductase, carnitine o-palmitoyltransferase, lipoprotein lipase, carnitine o-octanoyltransferase and stearoyl-CoA desaturase 1).
To assess the quality of the microarray data, a subset of eight genes was selected and expression levels were determined by TaqMan qRT-PCR. Higher expression in the obese animals of the respective age groups could be confirmed by qRT-PCR analysis for all the lipid metabolism genes mentioned above (ESM Table S5a–c). In addition to the time-points reported for the microarray analyses, minimally but significantly elevated expression levels in the obese animals could be detected by qRT-PCR for dienoyl-CoA reductase (weeks 6 and 7), carnitine octanoyltransferase (week 7) and lipoprotein lipase (week 7). However, only carnitine octanoyltransferase expression in week 7 (2.39-fold higher) exceeded a twofold change, whereas in the microarray experiments this was only observed in week 12. The decreased expression of only one gene, creatine kinase in week 12, could not be reproduced by qRT-PCR: expression values for creatine kinase were extremely high in all groups and not regulated in the obese animals. In contrast, the opposite differential expression of metallothionein 2 between week 7 and 12 observed in microarrays could be confirmed by qRT-PCR.
Increased SCD1 expression and palmitoleoyl-CoA levels in insulin-resistant ZDF rats
Scd1 and Cd36 were the only genes that were consistently highly expressed in both Affymetrix and TaqMan qRT-PCR analyses in all obese insulin-resistant or diabetic muscle probes tested (the increase in SCD1 expression was 5.9-, 10.6- and 3.2-fold in the 6-, 7- and 12-week-old animals, respectively; p<0.01; Fig. 1a). This prompted us to further investigate the role of SCD1 in the pathogenesis of insulin resistance. For example, elevated Scd1 expression was further shown for the 6- and 7-week-old groups by Lightcycler quantitative real-time PCR using Scd1-specific primers, and normalising for beta-actin expression (7.55- and 7.25-fold increase; p=0.02 and p=0.008, respectively; Fig. 1b). In an independent set of experiments, we additionally found that skeletal muscle from 8-week-old obese ZDF rats, compared with their lean littermates, contained 3.72-fold (p<0.01) higher amounts of palmitoleoyl-CoA (C16:1 N7) in HPLC analysis (Fig. 1c). Furthermore, much higher Scd1 expression levels (173-fold; p<0.01) were observed by quantitative real-time PCR (Lightcycler; Fig. 1d).
A cellular model of SCD1 function
To directly analyse the impact of SCD1 on insulin signalling and glucose disposal in muscle cells, we generated L6GLUT4myc cells that stably overexpressed human HA-tagged SCD1 (referred to as SCD1 cells), confirmed SCD1 expression by Western blot analysis (Fig. 2a), and found SCD1 to be localised in endoplasmic reticulum-like subcellular structures by confocal laser scanning microscopy (Fig. 2c). Furthermore, Nile Red staining after 4 h of treatment with 200 μmol/l palmitate showed increased accumulation of neutral lipids in L6GLUT4myc cells transiently overexpressing SCD1 (Fig. 2b). For all subsequent experiments, controls cells (WT cells), derived from L6GLUT4myc cells stably transfected with empty control vector, served as controls.
SCD1 overexpression impairs glucose uptake and insulin signalling in vitro
2-Deoxyglucose uptake assays revealed impaired basal and insulin-stimulated glucose uptake in SCD1 compared with WT cells (mean decrease in five cell clones tested, 2.3-fold; p<0.05; Fig. 3a). By immunoprecipitation and Western blotting, we further analysed insulin-stimulated IRS1 and AKT1/protein kinase B phosphorylation patterns. Compared with WT cells, SCD1 cells showed 43% (p<0.05) decreased tyrosine-phosphorylation of IRS1 (Fig. 3b) and 27% (p<0.05) decreased serine473 phosphorylation of AKT1/protein kinase B, indicating a negative impact of SCD1 expression on key points in insulin signalling.
SCD1 overexpression alters cellular gene expression levels
Screening for expression levels of genes known to be involved in or to be modulating insulin signalling revealed a 1.45-fold increased expression of PTPN1 protein in SCD1 cells (Fig. 4a) in Western blotting analysis. Upon differentiation, Lightcycler quantitative real-time PCR revealed that SCD1 cells contained 1.7-fold decreased transcript levels of the glucose transporter Slc2a4/Glut4 (Fig. 4b), whereas the protein level of the stably transfected MYC-tagged SLC2A4 remained unaltered in control experiments probing MYC-tag expression in immunoblot analysis (not shown).
SCD1 overexpression alters cellular long-chain acyl-CoA levels
To assess the impact of SCD1 overexpression on high-glucose- and fatty acid-induced insulin resistance, glucose uptake assays were performed upon treatment with high palmitate (200 μmol/l) and glucose (20 mmol/l). Glucose alone rendered SCD1 cells less insulin-sensitive, but did not alter basal glucose uptake (Fig. 4d). Additional treatment with 200 μmol/l palmitate decreased the insulin sensitivity of WT cells to the level of SCD1 cells (maximum insulin stimulation was reduced to 58%), whereas the latter did not exhibit any further impairment of insulin sensitivity (Fig. 4e).
To investigate whether the observed phenotype regarding insulin sensitivity is reflected in the products of SCD1 enzymatic activity and alterations in long-chain fatty acyl-CoA levels, HPLC analyses from KH2PO4 lysates of palmitate-treated SCD1 and WT cells were performed. Table 2 demonstrates that C16:0 levels were slightly increased in WT compared with SCD1 cells, but highly elevated in both cell lines after palmitate treatment (393 and 727%). C18:0 levels were below the detection limit in all probes tested, although more than 107 cells were analysed per data point. Treatment with palmitate at high glucose concentrations moderately diminished C18:1 N9 (176 and 125%), but increased C16:1 N7 levels (379 and 110%) in both WT and SCD1 cells. Interestingly, SCD1 cells per se contained slightly elevated levels of C18:1 N9 (150%) but significantly higher levels of C16:1 N7 (696%) than WT cells. Quantitative RT-PCR analysis further revealed that palmitate treatment increased Scd1 transcript levels in WT cells 19.1-fold (Fig. 5), but endogenous Scd1 levels in SCD1 cells remained mainly unaltered (1.13-fold decrease).
Discussion
Skeletal muscle is the major site of glucose disposal in the body. Here we report the first genome-wide, tissue-specific screen for genes differentially expressed in skeletal muscle of insulin-resistant and diabetic ZDF rats. We observed a unique gene expression profile with a prevalence of lipid-metabolising enzymes among the differentially expressed genes, which was confirmed by TaqMan qRT-PCR. The striking and consistent overexpression of Scd1 in the obese animals of all ages tested supports the hypothesis that muscle reacts to a high fatty acid burden by regulating key enzymes in lipid metabolism, whereas most transcriptional changes probably occur in adipose tissue. Interestingly, in muscle of insulin-resistant animals (6 and 7 weeks of age), Scd1 and Cd36 were initially increased, whereas dienoyl-CoA reductase, a protein involved in beta-oxidation, first became increased at a later time-point in animals with established diabetes (12 weeks of age). Similar changes towards elevated lipid utilisation in already diabetic ZDF rats have been observed in the kinetic studies of Etgen and Oldham [23]. Cd36 transgenic and knock-out mice models further revealed a correlation of insulin resistance, increased fatty acid influx and increased Cd36 expression in muscle [24, 25]. However, in the qRT-PCR data slightly but significantly elevated dienoyl-CoA reductase expression was already observed in the 6- and 7-week-old insulin-resistant animals, implying that the direction of the observed changes was already defined at this stage.
The second largest group of genes dysregulated in our experiments was involved in protein trafficking, catabolism and cytoskeleton integrity (e.g. the cytosolic sorting protein Pacs1, ubiquitin-conjugating enzyme E2-3, alpha-tropomyosin, slow skeletal muscle troponin, alpha-actin and beta-myosin), supporting the notion that changes in membrane and cytoskeleton composition accompany insulin resistance in muscle. Increased expression of metallothionein 2 in week 12 could represent a response against beginning oxidative stress in the already diabetic state. From the GECKO analysis, we estimated a false-positive rate of 5%. Accordingly, we could not reproduce any differential expression of creatine kinase by qRT-PCR. As we observed extremely high expression levels of this mRNA in all probes, oversaturated signals could also have accounted for this discrepancy.
The prominent expression of Scd1 that we report in insulin resistance is in agreement with other rodent models of obesity and insulin resistance, such as ob/ob mice [9, 26, 9]. The differences in the absolute levels of Scd1 transcript overexpression in the different experiments reported for the 6-, 7- and 12-week-old (Fig. 1a,b) rats compared with the extremely high values for the 8-week-old ZDF rats (Fig. 1d) probably result from different times of starvation (2 vs. 24 h) before the analyses. Due to the high turnover and fast induction of SCD1, the transcript levels do not necessarily reflect SCD1 enzymatic activities or products in a linear manner.
In humans, an abundance of the SCD1 product C16:1 N7 palmitoleic acid has also been described in insulin resistance and obesity [7]. We further established a causative role for SCD1 in muscle insulin resistance in cell culture experiments: SCD1 protein stably overexpressed in recombinant muscle cells was functional regarding its subcellular localisation and increased neutral lipid accumulation upon palmitate treatment. Interestingly, these SCD1 cells exhibited impaired glucose uptake, decreased insulin sensitivity at various steps of the insulin signalling cascade and dysregulation of known key regulators of insulin action. This is consistent with and extends the phenotype of Scd1 −/− mice [27, 28], as our data indicate that the improved insulin sensitivity observed for Scd1 −/− mice is a direct result of the lack of Scd1 expression rather than that it is caused by adaptive changes during development of the mice, or is a simple result of ameliorated obesity in Scd1 −/− mice.
In addition to the knockout model, Houdali et al. triggered insulin resistance by prolonged glucose infusion into skeletal muscle of Wistar rats and correlated the resulting impairment in insulin signalling with increasing Scd1 expression levels and activities in vivo [29, 30]. In our cell culture model, stable overexpression of SCD1 alone was sufficient to impair glucose uptake and insulin signalling, indicating that SCD1 levels or enzyme activity determined the observed phenotypic changes and thus supporting the findings of Houdali et al. Analysis of functional glucose uptake data and HPLC LCACoA profiles upon palmitate treatment of SCD1-overexpressing vs. WT cells revealed that palmitate treatment in high-glucose conditions could lower the insulin sensitivity of WT cells to the level of SCD1 cells per se. Additionally, this treatment increased C16:1 N7 levels and endogenous Scd1 transcript levels in WT but not in SCD1 cells, which contained higher amounts of stably transfected SCD1. This implies that, in SCD1 cells, feedback mechanisms besides polyunsaturated fatty acids were limiting endogenous Scd1 expression at the level of transcription—probably the mono-unsaturated SCD1 product 16:1 N7 itself [31]. However, the underlying mechanisms remain unclear. As all samples were analysed at 20 mmol/l glucose, we cannot define any further the extent to which glucose itself increased endogenous Scd1 expression (e.g. compared with cells incubated at 5.5 mmol/l glucose), but we observed clear induction of Scd1 when WT cells were incubated with both 200 μmol/l palmitic acid and 20 mmol/l high-glucose solution.
Elevated LCACoAs levels have been proposed to account for insulin resistance [32, 33]. However, our data suggest that LCACoA composition, in particular the relative proportion of mono-unsaturated 16:1 N7, is probably the more important determinant. As our HPLC analysis addressed only changes in LCACoA, we cannot determine where C16:1 N7 mono-unsaturated fatty acids may further exert a negative impact on cellular insulin signalling: as a component of phospholipids on the level of membrane composition or as ceramide or di- or triglycerides, all of which are fractions known to be associated with insulin sensitivity and to have a composition known to be altered by SCD1 activity [31, 34]. Our observations point to the existence of direct effects of SCD1, or the products of its enzymatic activity (in particular C16:1 N7), on immediate signalling events, and of indirect downstream effects on the level of transcription or protein expression. In particular, treatment of WT cells with high glucose and high palmitate mimicked the phenotype of SCD1 overexpression. As SCD1 is highly regulated by nutritional challenges, it is tempting to speculate that nutritional oversupply of glucose and saturated fatty acid species could trigger insulin resistance by upregulating Scd1 expression, which in turn elevates C16:1 N7 levels. Further studies should elucidate the exact mechanisms underlying the negative effects of SCD1 and mono-unsaturated C16:1 N7 fatty acyl Co-A species on insulin signalling and (post-)transcriptional regulation.
Abbreviations
- ESM:
-
Electronic Supplementary Material
- GMI:
-
Genetic Models Incorporated
- HA:
-
haemagglutin
- LCACoA:
-
long chain acyl-CoA
- PTPN1:
-
protein–tyrosine phosphatase b
- qRT-PCR:
-
quantitative RT-PCR
- SCD1:
-
stearoyl-CoA desaturase 1
- WT:
-
wild-type
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Acknowledgements
We are grateful to Dr Amira Klip (Hospital for Sick Children, Toronto, ON, Canada) for kindly providing L6 cells overexpressing GLUT4myc. We thank Gertraud Jerabek-Sandow for help with qRT-PCR, Stefan Welte for help with analysing IRS1 and AKT1 phosphorylation, and Dr Guenter Mueller for helpful discussions (all at Sanofi-Aventis, TD Metabolism, Frankfurt, Germany).
Duality of interest
All authors are employees of Sanofi-Aventis Deutschland GmbH, Frankfurt, Germany.
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Voss, M.D., Beha, A., Tennagels, N. et al. Gene expression profiling in skeletal muscle of Zucker diabetic fatty rats: implications for a role of stearoyl-CoA desaturase 1 in insulin resistance. Diabetologia 48, 2622–2630 (2005). https://doi.org/10.1007/s00125-005-0025-2
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DOI: https://doi.org/10.1007/s00125-005-0025-2