Mouse strains and genotyping

Using the chemical random mutagenesis technique with the germline supermutagen N-ethyl-N-nitrosourea (ENU), a mouse model for mutant Mc4r was generated by Ingenium Pharmaceuticals AG, Martinsried, Germany. Functional in vitro analysis of the mouse Mc4r containing the mutation Ile¹⁹⁴Phe revealed a partial loss of receptor function (~40-fold reduced agonist potency). At the in vivo level, this mutant causes the same full obese phenotype as observed in a mouse strain containing a Mc4r mutation (Tyr³⁰²Cys) with a complete loss-of-function in in vitro assays [21]. We used the Ile¹⁹⁴Phe mouse strain (referred to as Mc4r^mut) to closely mimic the Mc4r dysfunction most frequently found in humans with inhered obesity [23]. Mice were bred and maintained under specific-pathogen-free conditions at the centralised animal care facility, where lights were automatically controlled (12 h light/12 h dark). All animal experiments were conducted in accordance with the European Directive 2010/63/EU on the protection of animals used for scientific purposes and were performed with permission of the Animal Care and Use Committee (ACUC #TVV 43/07) and the Government of the State of Saxony, Germany.

The initial Ile¹⁹⁴Phe C3HeB/FeJ (C3H) mouse strain [21] was crossed into the C57BL/6J (B6) background over more than 12 generations. Breeding for experiments was performed with heterozygous breeding pairs. Genotyping of the littermates was performed by polymerase chain reaction (PCR) followed by BspHI (New England Biolabs, Frankfurt, Germany) restriction analysis. The following primers and PCR conditions were used: 5’- taccctgttaaacagtacggatac-3’ (sense) and 5’- gaacatggaaatgaggcagatca-3’ (antisense) creating a BspHI-site in Mc4r^+/+ sequence, conditions: 94°C 3 min; 35 cycles of 94°C 30 sec, 58°C 30 sec and 72°C 1 min. Products were digested with BspHI and fragments were separated in a 3% agarose gel.

We analyzed groups of Mc4r^+/+ and Mc4r^mut mice of both genders on standard chow diet and a semisynthetic diet containing 0.02% cholesterol (Ssniff GmbH, Soest, Germany) [24] (S1 Table). Furthermore, Mc4r^mut mice were crossed onto a homozygous B6.Ldlr^-/- background (The Jackson Laboratory, Bar Harbor, Maine, stock no. 002207) to generate double-deficient mice. These (Mc4r^mut;Ldlr^-/-) and the respective control (Ldlr^-/-) of both genders were weaned at 3 weeks of age and fed standard chow or semisynthetic diet until they were euthanized after 180 days of age. For euthanasia, mice were deeply narcotized by i.p. injection with a 100 μl mixture of 100 mg/kg body weight ketamine and 5 mg/kg body weight xylazine. Blood was collected post-euthanasia by heart puncture into syringes containing EDTA and the circulatory system was flushed with PBS (20 ml). Tissues (heart and brachiocephalic artery (BCA)) were collected from sacrificed mice and snap-frozen in Tissue-tek OCT compound (Sakura Finetek).

Blood chemistry and histology

Enzymes, lipids and glucose were analyzed in serum and whole blood, according to the guidelines of the German Society of Clinical Chemistry and Laboratory Medicine, using a Hitachi PPEModular analyzer and an Accu-Check^® blood glucose measurement device (both Roche Diagnostics, Mannheim, Germany), respectively. Lipoproteins were isolated by sequential ultracentrifugation from 60 μl of plasma at densities (d) < 1.006 g/ml (very low–density lipoprotein), 1.006 ≤ d ≤ 1.063 g/ml (intermediate-density lipoprotein and low-density lipoprotein), and d > 1.063 g/ml (high-density lipoprotein) in an LE-80K ultracentrifuge (Beckman) as described [25].

Atherosclerosis quantification in the aortic root and the BCA was performed as previously described [26]. In brief, the OCT-embedded BCA was sectioned from distal to proximal at 10 μm thickness. Atherosclerotic lesions luminal to the internal elastic lamina were quantified in three equidistant oil red O-stained sections 200, 400, and 600 μm from the branching point of the BCA into the carotid and subclavian arteries. Histomorphological characterization and computerized morphometric quantification (Zeiss KS300) of the lesions was performed by two investigators, blinded to the protocol. The mean of the lesion size of the three sections was used to represent individual atherosclerosis development in the BCA. The aortic root was sectioned from proximal to distal collecting and evaluating 5 sections (each in 50 μm distance).

Lipid extraction

Lipid extraction was conducted according to Folch et al. [27]. Frozen liver tissue (n = 5 per group, 6-month-old male) was transferred into chloroform/methanol (2:1, v/v) and vortexed for at least 1 minute. Afterwards, the tissue was sonicated on ice for 1 minute and shaken for 2 h at room temperature and 90 rpm. After shaking, 600 μl 0.9% NaCl solution was added and samples were vortexed for 1 minute. Phase separation was achieved by 10 minutes of centrifugation at 2,500 rpm. The organic phase was transferred into a new tube and vaporized by vacuum centrifugation. Complete cholesterol was determined using the enzymatic Amplex^® Red Cholesterol Assay Kit (Invitrogen). To determine the amount of extracted cholesterol, the pellet was solubilized in 500 μl 1× reaction buffer. A volume of 20 μl of this solution was further diluted 1:10 in 1× reaction buffer. The reaction was started by adding 50 μl of the diluted extract to 50 μl master mix which was prepared according to the assay protocol. The solution was incubated at 37°C for 30 minutes. Afterwards the samples were excited at 560 nm and fluorescence intensity was measured with an Infinite^® M200 TECAN Reader at 590 nm. Intensities were compared to a standard curve and the amount of cholesterol was calculated per gram of liver tissue.

RNA sequencing of liver transcripts

Total RNA from liver (10 male mice per genotype) was extracted by using the RNeasy Micro Kit^™ (Qiagen, Hilden, Germany) as described in the manufacturer’s instructions. The quantity of the RNA was measured using a spectrophotometer (Nanodrop ND 1000) and RNA quality of all samples was examined on the Agilent 2100 bioanalyzer using the RNA 6000 Nano Chip (Agilent Technologies, Santa Clara, CA). We only included RNA samples with a RIN value above 8.

Indexed cDNA libraries were generated using TruSeq RNA Sample Preparation Kits v2 (Illumina, San Diego, CA, USA) according to the manufacturer’s protocol, constructing libraries with an average size of 300 bp as evaluated on the Agilent 2100 bioanalyzer with DNA 1000 Chips.

Libraries were sequenced on Illumina HiScanSQ (Core Unit Sequencing, University of Leipzig), performing ten biological replicates for each genotype. 101 bp raw paired-end reads were generated on 8 flow cell lanes. Briefly, after quantification of the libraries using the Library Quantification Kit—Illumina/Universal (KAPABiosystems) according to the instructions of the manufacturer, products were used for cluster generation. Library DNA at a concentration of 10 pM was clustered using an Illumina cBot according to the PE_Amp_Lin_Block_Hybv8.0 protocol of the manufacturer. Sequencing was performed using version 3 chemistry and the version 3 flow cell according to the manufacturer’s instructions. Median cluster density was usually about 600,000 clusters per mm² or 80–100 million raw clusters per lane.

After intensities call, raw reads were separated according to library indexes allowing up to one mismatch in the index sequence, but requiring that all bases have a quality score above 15 (PHRED-scale). After assigning reads to samples we used an in-house-sequencing pipeline to trim the adapters and to remove low quality reads [28]. Reads were mapped to the reference mouse genome (July 2007 NCBI37/mm9) with Ensembl v66 annotations using Tophat 2.0.6. [29, 30] which aligns reads using Bowtie2 (version 2.1.0). Mitochondrial reads and reads which did not map uniquely to a genome position were excluded. The transcription level for each gene was obtained by intersecting mapping results with gene annotations using BEDTools IntersectBed [31]. Using the DESeq software package [32], differential expression of wt and KO genes was examined. Only genes that were expressed at least in 10 animals among the groups were included for analyses. Differentially expressed genes with a nominal p-value < 0.05 were considered as statistically significant.

Statistical analyses

For analyses of significant differences between the genotypes an unpaired two-tailed Student’s t-test was used, p-values of < 0.05 were marked *, < 0.01 **, and < 0.001 with ***. To correlate gender difference in weight gain and body length dependent on the genotypes and diets a 3-way ANOVA was used (S2 Table).

To assess the relationship between the plaque sizes (aortic root, BCA) and the total cholesterol serum levels a Pearson product-moment correlation coefficient was computed. The results were summarized in scatterplots and tested for significance.

To test for influence of different parameters on the atherosclerotic plaque size, we run a multiple regression analysis. We included the serum cholesterol levels, sex, diets, and the Mc4r deficiency as potential predictors and used the plaque size as response variable. The overall model including all predictors was highly significant for both, the plaque size in heart and the BCA (BCA: F_{(4, 94)} = 37.44, p-value < 2.2e^-16 r² = 0.60; heart: F_{(4, 81)} = 65.09, p-value < 2.2e^-16, r² = 0.75).

Effects of cholesterol diet and Ldlr deficiency on increases in body weight and length in Mc4r-deficient mice

Mc4r deficiency led to a significant increase in body weight in male (45%) and female (50%) mice fed on standard chow and in male (30%) and female (62%) mice on a semisynthetic diet (Table 1). The body weight differences between Mc4r^mut and the other mouse strains were already obvious after one month after birth (S1 Fig). The difference of weight due to Mc4r deficiency was also found on the Ldlr^-/- background (standard chow: male 36%, female 83%; semisynthetic diet: male 37%, female 89%). Here, the weight difference between wt female mice and Mc4r^mut;Ldlr^-/- females (standard chow: 83%; semisynthetic diet: 89%) was significantly higher as in Mc4r-deficient females mice (standard chow: 50%; semisynthetic diet 62%). The Ldlr^-/- alone did not significantly influence the body weight in both genders and under the different diets.

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Table 1. Body weight and length under standard and cholesterol-containing diets.

Body weights and length of the different genotypes were determined after 184 ± 3 (range 172–194) days after birth. Animals were kept on standard chow or semisynthetic diet containing 0.02% cholesterol. Data are given as means ± SD. Number of animals are given in parenthesis, and results between groups were tested for significance to the respective Mc4r^+/+: *p < 0.05, ** p < 0.01; *** p < 0.001.

https://doi.org/10.1371/journal.pone.0167888.t001

In our mouse strain male and female Mc4r^mut animals showed a slightly increased body length of 6% compared to wild-type controls (Table 1). The difference of length between wt and Mc4r^mut was also found on the semisynthetic diet in male (4%) and female (8%) mice. The difference of length due to Mc4r deficiency was also found on the Ldlr^-/- background (standard chow: male 5%, female 8%; cholesterol diet: male 7%, female 10%).

The gender differences in weight gain and body length depending on the genotypes and diet were tested using a 3-way ANOVA. It revealed a significant interaction between genotype and sex (F_{3, 182} = 5.6579, p < 0.001) which was mainly driven by the differences of females and males on the Mc4r^mut background. In all cases the differences of body weight and length in female Mc4r^mut were higher than in male Mc4r^mut (S2 Table, S2 and S3 Figs).

In summary, Mc4r-deficient mice showed the expected obese phenotype with gender-specific characteristics. The combination of Mc4r and Ldlr deficiencies had no major impact on the development of obesity in the Mc4r^mut mouse strains.

Dyslipidemia in mice lacking both receptors Mc4r and Ldlr

Next, we addressed the question whether Mc4r deficiency contributes to increases in plasma lipids in Ldlr^-/- mice and, therefore, can be considered as a risk factor of atherosclerosis. As shown in Fig 1 and Table 2, Mc4r deficiency alone caused small and moderate increases in plasma cholesterol levels under standard chow and semisynthetic cholesterol-containing diet, respectively, in both genders. The increase in cholesterol was most pronounced in the LDL fraction (Table 2). The triglyceride levels remained normal in Mc4r^mut on both diets. Essentially similar results were found in a Mc4r gene-deletion mouse strain but the cholesterol content of the diet was not stated [33].

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Table 2. Plasma lipids and lipoproteins and liver cholesterol on standard chow and semisynthetic diets.

Plasma lipids and liver cholesterol content of the different genotypes were determined after 184 ± 3 days after birth. Animals were kept on standard chow and semisynthetic diet. Data are given as means ± SD and tested for significance to the respective Mc4r^+/+: *p < 0.05, ** p < 0.01; *** p < 0.001. The number of animals per group was between 10 and 14 (plasma lipids) and 5 (liver cholesterol). n.d., not determined.

https://doi.org/10.1371/journal.pone.0167888.t002

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Fig 1. Severe hypercholesterolemia and hypertriglyceridemia in mice lacking both MC4 and LDL receptors.

Serum cholesterol (A) and serum triglycerides (B) were determined in the indicated mouse strains (n = 10–14 male mice). Female mice show essentially similar results (see Table 2). The statistic evaluation is given in Table 2.

https://doi.org/10.1371/journal.pone.0167888.g001

As shown in Fig 1 and Table 2, the combination of both receptor defects caused massive increases in plasma cholesterol and triglyceride levels. Importantly, this effect was already seen under standard chow which did not contain detectable amounts of cholesterol. The cholesterol and triglyceride levels were higher in male compared to female mice. Significant increases in lipids were found in all lipoprotein fractions (Table 2).

MC4R-deficient mice develop hepatic steatosis independent of plasma cholesterol levels

Because cholesterol and triglycerides are mainly produced in the liver, we focused our analysis on hepatic functional parameters. As shown in Table 3, Mc4r^mut mice present significantly elevated activities of ASAT, ALAT, GLDH, and CHE. Interestingly, enzyme activities were further increased by semisynthetic diet but not by Ldlr deficiency (see Table 3). Liver morphology and histology revealed a massive hepatic steatosis without histological signs of inflammation (see accompanied paper Lede et al.) as already described for Mc4r^mut [34, 35]. This non-alcoholic fatty liver disease (NAFLD) may slowly progress into non-alcoholic steatohepatitis (NASH), which is characterized by excessive liver inflammation. It has been shown that cholesterol is an important risk factor for the progression to hepatic inflammation in diet-induced NASH [36].

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Table 3. Blood glucose, serum urea levels, and liver enzymes on standard chow and semisynthetic diets.

Enzyme activities of the different genotypes were determined after 184 ± 3 days after birth. Animals were kept on standard chow and semisynthetic diet. Data are given as means ± SD and tested for significance to the respective Mc4r^+/+: * p < 0.05, ** p < 0.01; *** p < 0.001. The number of animals/group is between 10 and 14.

https://doi.org/10.1371/journal.pone.0167888.t003

Mc4r^mut mice develop a late-onset hyperglycemia [11] and normal basal blood glucose levels but increased insulin levels and hepatic insulin resistance have been reported [37, 38]. We found no significant effects on basal blood glucose levels in all genotypes under the two diets (Table 3). Interestingly, there were no significant differences in liver cholesterol between the mouse strains and both diets (Table 2) and no significant correlation between the liver cholesterol and the serum cholesterol concentrations.

Severe atherosclerosis in mice lacking both Mc4r and Ldlr

We analyzed atherosclerotic plaque formation in the aortic root and the BCA as pathomorphological readout for atherosclerosis in our mouse strains. No atheromata were found in mice with an Ldlr^+/+ genotype regardless of the diet. Although significantly elevated cholesterol levels (up to 4 mmol/L in Mc4r^mut on the semisynthetic diet) and obesity Mc4r^mut mice did not develop atherosclerotic plaques. However, the combination of both receptor defects significantly increased atheroma formation compared to the atherosclerosis found in Ldlr^-/- mice (Figs 2, 3 and S5). Strikingly, atherosclerotic plaque formation was already found in Mc4r^mut;Ldlr^-/- on standard chow as quantified in histological sections stained with Sudan red (Fig 3). Staining of aortic root sections with an anti-CD68 antibody, a marker expressed in macrophages, revealed macrophage-positive plaque formation in female Mc4r^+/+;Ldlr^-/- and Mc4r^mut;Ldlr^-/- mice of both gender (S6 Fig). Quantitative PCR analysis of the macrophage chemoattractant protein MCP1 (CCL2) showed detectable MCP1 expression in male mice on an Ldlr^-/- background, whereas MCP1 was detectable in all female groups (S7 Fig) with significant increases in atherosclerotic animals. TNF-α expression was found in aortic roots of semisynthetic fed mice (S7 Fig).

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Fig 2. Atherosclerosis in the aortic root in mice lacking Ldlr and Mc4r;Ldlr.

Representative sections of the aortic root prepared from the different mouse strains. Depicted are sections of the aortic root of female and male Mc4r^mut and Mc4r^mut;Ldlr^-/- mouse strains fed a chow and semisynthetic diet (0.02% cholesterol).

https://doi.org/10.1371/journal.pone.0167888.g002

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Fig 3. Quantification of atherosclerotic lesions at the aortic root and brachiocephalic artery (BCA).

Male and female mice (wt: +/+, Mc4r deficiency: mut), all on an Ldlr-deficient background, were fed with standard chow and semisynthetic diet. Atherosclerosis quantification in the BCA (A) and the aortic root (B) was performed after 6 months as previously described (14). Data of the indicated genotypes are given as a scatter and box plot showing the median (bold line) and the lower and the upper quartile (as box) (7–15 animals per group; from left to right: n = 11, 12, 11, 13, 13, 12, 15, 12, 10, 11, 7, 12, 13, 8, 14, 11).

https://doi.org/10.1371/journal.pone.0167888.g003

To examine the relationship between plasma cholesterol levels and the atherosclerotic plaque size, we run a multiple regression analysis. Thus, we included the serum cholesterol levels, sex, diets and the Mc4r deficiency as potential predictors and used the plaque size as response variable. The overall model including all predictors was highly significant for both, the plaque size in the aortic root and BCA (BCA: F(4, 94) = 37.44, p-value < 2.2e-16 r2 = 0.60; heart: F(4, 81) = 65.09, p-value < 2.2e-16, r2 = 0.75). Only cholesterol levels, diet and sex had a significant impact whereas the Mc4r deficiency did not reach significance (see S3 Table).

Transcriptional changes in cholesterol and bile acid syntheses

As stated above, no differences in liver cholesterol levels were observed between the mouse strains. To further substantiate this finding, we analyzed the transcript levels of components relevant for cholesterol and bile acid biosynthesis by RNA-Seq technology. Approximately 30 million reads per animal (10 animals per genotype) were analyzed. Interestingly, the number of Ldlr transcripts was significantly increased in all Ldlr^-/- strains (Table 4). Detailed analysis revealed that all transcripts mapped to exons 1–4 of the Ldlr whereas Ldlr transcripts of wt mice were almost equally distributed over all exons. Comparison of transcripts mapping only to exon 1–4 revealed an approximately 10-fold increase in Ldlr^-/- strains. The Ldlr^-/- mouse strain was generated by insertion of a neomycin resistance cassette into exon 4 [5]. The targeted allele would encode a truncated non-functional protein that will not bind LDL, and lacks a membrane spanning segment. Immunoblot analysis of liver membranes detected a truncated protein in homozygous mutant animals [5]. This nicely fits with the RNA-Seq data and upregulation can be interpreted as a compensatory regulation because of the lack of Ldlr function.

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Table 4. Transcriptional changes of selected components of the cholesterol and bile acid biosyntheses.

RNA sequencing was performed with RNA from livers of 10 animals of each genotype. Means of the expression ratio (KO/WT) for each gene are listed. For p-value calculations an unpaired two-tailed Student’s t-test was used.

https://doi.org/10.1371/journal.pone.0167888.t004

Several studies on mice with hepatic steatosis have shown that several transcription factors and components of the triacylglycerol metabolism such as PPARγ (Pparg), fatty acid synthetase (Fasn), SREBP-1c (Srebf1) and stearoyl-coenzyme A desaturase 1 (Scd1) are increasingly expressed in the liver. We confirmed some of them in our mouse strains where Mc4r^mut and Mc4r^mut;Ldlr^-/- showed significantly higher mRNA levels for PPARγ and stearoyl-coenzyme A desaturase 1 compared to wild-type animals (Table 4). The transcripts of fatty acid synthetase and SREBP-1c were higher in those mouse strains but values reached no significance. The detailed analysis of the complete liver transcriptome data under the different diets and changes in liver lipid compositions is presented in the accompanied manuscript Lede et. al.,).

In congruence with unchanged hepatic cholesterol we found no evidence for significant changes in components of the cholesterol biosynthesis (Table 4). Only the mevalonate kinase (Mvk), 3-ketosteroid reductase (Hsd17b7) and sterol-C4-methyl oxidase (Sc4mol) in double KO showed significant reduction in transcript expression levels. However, the transcript level of the rate-limiting enzyme of the cholesterol biosynthesis, the HMG-CoA reductase (Hmgcr), remained unchanged.

The synthesis of primary bile acids from cholesterol occurs via two pathways: the classic neutral pathway involving cholesterol 7-alpha-hydroxylase (Cyp7a1), and the acidic pathway involving a distinct microsomal oxysterol 7-alpha-hydroxylase (Cyp7b1). Transcriptome analysis revealed a significant reduction of Cyp7b1 in all mutant mice compared to wt mice (Table 4). Also, Cyp7a1 transcript was in general lower in all mutant mice livers but did not reach significance. Interestingly, the bile acid transporter Slco1a1 was significantly downregulated in all Mc4r^mut strains (Table 4). To evaluate if changes in transcript levels of these enzymes result in differences of bile acid production, we analysed the bile acid content of the liver and of bile collected from the gall bladder. We found reduced (but not significant) bile acid concentrations in the liver of the Mc4r^mut;Ldlr^-/- compared to WT animals (S4A Fig). As shown in S4B Fig, comparison between Mc4r^mut and Mc4r^+/+ groups, showed no significant differences in bile acids in the collected bile (p = 0.38, WT vs. Mc4r^mut; p = 0.28, Ldlr^-/- vs. Mc4r^mut;Ldlr^-/-). However, significant lower bile acid levels where found in the Ldlr^-/- and Mc4r^mut;Ldlr^-/- strains when compared to WT animals (p = 0.037; p = 0.012).