Introduction

Obesity is caused by energy intake in excess of energy expenditure, and is associated with an increased number and/or size of white adipocytes, which store the excessive energy in the form of triacylglycerol. The association between increased fat mass, insulin resistance and type 2 diabetes mellitus is well known. Yet, regional body fat distribution may influence the occurrence of insulin resistance associated with obesity. Increased accumulation of visceral (intra-abdominal) fat seems to be particularly associated with an increased risk of insulin resistance and type 2 diabetes. Two major lines of observations suggest a causative role for intra-abdominal fat in this association. First, subjects with normal body weight, but with increased visceral adiposity (e.g. elderly people or patients with certain forms of lipodystrophy) are prone to develop insulin resistance [1, 2]. Second, removal of intra-abdominal fat improved insulin sensitivity [3, 4], whereas the removal of subcutaneous fat tissue by liposuction in obese humans did not improve insulin action [5]. Thus, the pattern of body fat distribution, especially abdominal fat accumulation, determines insulin sensitivity.

One remaining question to define in this process is the relative contributions of: (1) the mere increase in intra-abdominal fat mass; and (2) the role of alterations in fat tissue biology that accompany obesity. Increase in fat mass as such has been suggested to increase the delivery of non-esterified fatty acids through the portal circulation, resulting in increased hepatic and muscular triacylglycerol accumulation [6]. Similarly, altered adipose tissue biology can change inter-organ cross-talk mechanisms through alterations in its metabolic and/or endocrine function. For example, a recent study demonstrated that the degree of macrophage infiltration into omental fat of obese patients correlated with histopathological findings in liver biopsies [7].

To investigate the isolated role of a mere increase in intra-abdominal fat in mice, we used intra-abdominal fat transplantation to increase the intra-abdominal mass of ‘normal’ fat. We reasoned that if the mere increase in fat mass is the predominant process occurring in obesity, increasing intra-abdominal fat mass by surgical transplantation of fat tissue from a normal, non-obese littermate would induce metabolic consequences in the recipient mice that resemble those occurring in obesity. If, on the other hand, the predominating effect is obesity-induced alterations in the endocrine function of fat tissue, the addition of such fat mass would not impair metabolic regulation.

Materials and methods

Animals

Male C57BL6JOlaHsd mice were purchased from Harlan Netherlands (Horst, the Netherlands). All mice were housed in a pathogen-free environment on a 12-h light-dark cycle, with free access to standard rodent diet (Provimi Kliba, Kaiseraugst, Switzerland). All protocols conformed to the Swiss animal protection laws and were approved by the Cantonal Veterinary Office in Zurich, Switzerland.

Surgical procedure

Transplantation procedure was performed at 6 weeks of age. Mice were anaesthetised with isoflurane (Abbott, Baar, Switzerland). Both epididymal fat pads were removed from the donor mouse, rinsed with 0.9% saline and thereafter stitched to the visceral side of the peritoneum of the recipient mouse using Vicryl 5.0 (Johnson-Johnson, Spreitenbach, Switzerland). Except for a small piece of fat tissue fixed in 4% buffered formalin, the entire two fat pads were weighed and then transplanted. Sham-operated control mice received the same treatment, but instead of the fat pad transplantation, an artificial suture was performed with Vicryl. Subcutaneous injection of buprenorphine every 12 h for 2 days was used for analgesia. In order to prevent transplant rejection, donor and recipient mice were littermates.

Glucose and insulin tolerance tests

For fasting intraperitoneal glucose tolerance test (ipGTT), either prolonged fasting (overnight, i.e. 12 h food withdrawal) or 7 h food withdrawal were used, as indicated. For intraperitoneal insulin tolerance test (ipITT) in the post-absorptive state, mice were fed and then fasted for 3 h. Either glucose (2 g/kg body weight) or human normal insulin (0.75 U/kg body weight) were injected intraperitoneally and blood was collected from the tail vein at different time points, as indicated [8]. Plasma glucose was measured using a glucose meter (Ascensia Contour; Bayer, Zurich, Switzerland).

Determination of plasma insulin, adipokines and NEFA levels

Plasma was collected from the tail vein after 7 h of fasting. Insulin was determined using an ELISA kit (Ultra Sensitive Rat Insulin ELISA; Crystal Chem, Downers Grove, IL, USA). NEFA levels were measured using the ACS-ACOD-MEHA method (Wako Chemicals GmbH, Neuss, Germany). Plasma leptin and adiponectin were determined with commercially available mouse endocrine and single plex adiponectin kits (MENDO-75K and MADPK-71K-ADPN; Linco Research, distributed by Labodia, Yens, Switzerland) that are capable of simultaneously measuring different adipokines in mouse serum or plasma. The two kits are based on Luminex xMAP technology (Linco Research, St Charles, MI, USA) and use microsphere bead sets that are uniquely labelled with a mixture of two fluorescent dyes. The captured antibodies specific for each analyte are covalently coupled to individual bead sets. At the time of the assay, a mixture of beads is incubated overnight at 4°C with 10 μl of standards or mouse plasma samples in a 96-well filter-bottom plate. On the next day, the beads are washed, and biotinylated detection antibody cocktail is added and incubated for 30 min at room temperature, followed by the addition of streptavidin-phycoerythrin and incubation for another 30 min. After a final wash, the resuspended beads are read on a Luminex 100 reader (Bio-Rad Laboratories, Hercules, CA, USA) and the concentration of each analyte in the samples to be tested is determined on the basis of individual standard curves.

Determination of homeostasis model assessment of insulin resistance

The homeostasis model assessment of insulin resistance (HOMA-IR) was calculated using glucose and insulin determinations obtained after 7 h of food withdrawal, using the following formula: fasting glucose (mmol/l)×fasting insulin (mU/ml)/22.5 [9, 10].

Histology

Epididymal fat tissues were fixed in 4% buffered formalin and imbedded in paraffin. Sections were obtained either at the time of transplantation or 8 weeks after transplantation and stained with haematoxylin-eosin. For each mouse at least four fields (representing a total of 350 to 550 adipocytes) were analysed. Images were analysed using ImageJ software for quantification (National Institutes of Health, Bethesda, MD, USA).

Data analysis

Statistical analyses of the obtained data were performed using Student’s t test or ANOVA (Fisher’s multiple comparisons test), as indicated. We performed Pearson correlations between the continuous variables and estimated the independent effect of fat transplantation by further adjustment for total body weight using a linear regression model (SPSS package software, version 14).

Results

Intraperitoneal fat transplantation increases intra-abdominal fat mass without significantly altering circulating adipokine levels

To increase the intra-abdominal mass of ‘normal’ fat tissue, epididymal fat pads were removed from a littermate donor and transplanted into the peritoneal cavity of the recipient. At the time mice were killed (10 weeks post-transplantation), transplanted fat pads were adherent to the peritoneum and were vascularised (Fig. 1a,b). Sham operations were performed in control littermates. Recipient mice tolerated the surgical procedure and the fat transplantation well, with no adverse events noted, and weight gain during the ensuing 10 weeks comparable to that of sham-operated littermate mice (Fig. 1c).

Fig. 1
figure 1

Intra-abdominal transplanted fat is viable and weight gain is similar in sham-operated and recipient mice. a, b Six-week-old mice received intraperitoneal transplantation of two epididymal fat pads (approximately 175 mg) removed from a littermate donor, as detailed in the Materials and methods. Sham-operated mice served as controls. At 10 weeks post-surgery, the abdominal cavity was opened, and transplanted (T) or endogenous (E) fat pads were visualised. a, sham; b, recipient. c Weight gain in recipient (open circles) and sham-operated littermate mice (closed squares). Results represent the mean±SEM of eight or nine animals per group

Recipient mice had a 50% increase in their combined (endogenous + transplanted) intra-abdominal perigonadal fat depot mass (p < 0.005, Table 1). Fat tissue morphometry was performed on histological sections stained with haematoxylin-eosin (Fig. 2a). Adipocyte cell perimeter in the transplanted and endogenous fat pads did not differ at the time of transplantation (transplanted fat pad: 4,853 ± 976 [arbitrary units], recipient endogenous fat pad: 4,056 ± 785, sham-operated fat pad: 4,170 ± 798; p = 0.72 ANOVA). However, adipocytes of endogenous epididymal fat pads in both sham-operated and recipient mice hypertrophied from transplantation to time of killing (adipocyte perimeter increase 1.64 ± 0.28-fold, p < 0.05 and 1.73 ± 0.31-fold, p < 0.05, in sham-operated and recipient mice, respectively), whereas adipocyte size of the transplanted fat pad did not increase (0.91 ± 0.14-fold, p = 0.47)(Fig. 2b). The combined intra-abdominal fat depot (endogenous + transplanted) did not result in a significant difference in total body weight between the recipient and control groups (Table 1). Consistent with this observation, circulating levels of adiponectin, leptin, resistin and NEFA (Table 1) in recipients compared with sham-operated controls were not statistically different (p = 0.12, 0.15, 0.59 and 0.16, respectively). Thus, transplanted fat increased intra-abdominal mass of adipose tissue while retaining adipocyte size of the transplanted fat, but it did not alter total body weight or circulating levels of secreted adipose tissue products.

Table 1 Total body weight, perigonadal fat pad weight and circulating plasma levels of adipokines and NEFA
Fig. 2
figure 2

Adipocyte size of transplanted fat pads remains stable over time. a Representative, haematoxylin- and eosin-stained histological sections of endogenous or transplanted fat pads from recipient or sham-operated mice at the time of transplantation or after killing (10 weeks later). Adipocyte cell perimeter was measured using ImageJ. b Up to 470 cells for each fat pad were analysed. The mean ± SEM of four different mice is depicted here. All values are expressed relative to the adipocyte cell perimeter of transplanted epididymal fat pad at the time of transplantation. Black bar, endogenous fat pad of sham-operated mice; white bar, transplanted fat pad of recipient mice; grey bar, endogenous fat pad of recipient mice

Recipient mice with transplantation-mediated increase in intra-abdominal fat mass exhibit improved glucose tolerance in the fasting state

We first assessed whether intra-abdominal fat transplantation altered insulin sensitivity in the non-fasting state. For this, insulin sensitivity was measured 4 weeks after transplantation, after overnight feeding followed by 3 h of food withdrawal. Glucose lowering during post-absorptive ipITT was identical between recipient and sham-operated littermate mice (Fig. 3). To evaluate the effect of fat transplantation on glucose homeostasis in the fasting state, ipGTTs were performed. At 4 weeks post-transplantation, overnight-fasted mice exhibited improved glucose tolerance, as manifested by lower plasma glucose levels at 15, 30, 45, 60, 90 and 120 min after glucose administration, resulting in a 20% decrease in the AUC for glucose (recipient: 999 ± 46, sham-operated: 1267 ± 66; p < 0.001, Fig. 4a,b). To test whether this effect was observable after a shorter fasting period, mice were fasted for 7 h prior to ipGTT. Glucose levels during ipGTT during these conditions were somewhat more variable (as evidenced by larger SEMs), but overall, recipient mice had lower glucose levels and lower mean glucose AUCs than sham-operated controls (Fig. 4c,d). Circulating insulin levels were also measured during ipGTT (7 h of fasting) and tended to be lower in the transplanted mice than in controls, particularly in the basal fasting state (baseline: 79.8 ± 8.2 vs 113.9 ± 20.9 pmol/l, p = 0.13; 15 min: 134.6 ± 13.5 vs 150.2 ± 7.6 pmol/l, p = 0.41; 30 min: 126.7 ± 18.3 vs 139.8 ± 19.3 pmol/l, p = 0.62). These results suggest that the post-challenge insulin secretory response was maintained (and not exaggerated) in mice receiving intra-peritoneal fat transplantation, while insulin sensitivity in the fasting state was improved.

Fig. 3
figure 3

Intra-abdominal transplantation of fat tissue does not alter post-absorptive insulin tolerance. Intraperitoneal ITT (0.75 U/kg body weight) was performed 4 weeks after surgery in recipient (open circles) and sham-operated mice (filled squares) that had fasted for 3 h. Blood was collected from the tail vein at the indicated time points. Results are the mean±SEM of nine or ten different animals in each group

Fig. 4
figure 4

Lean mice with transplantation-mediated increase in intra-abdominal fat mass exhibit improved fasting glucose tolerance. Intraperitoneal GTT (2 g glucose/kg body weight) was performed 4 weeks after surgical procedure in recipient (open circles) and sham-operated mice (filled squares) that had fasted overnight (a, b) or for only 7 h (c, d). Results are expressed as mean plasma glucose concentration or AUC±SEM from 15 (sham) or 16 (recipient) animals (a, b) or from six (sham) or seven (recipient) animals (c, d). *p < 0.05, **p < 0.01, ***p < 0.001 (Student’s t test)

To further assess fasting insulin sensitivity, HOMA-IR was calculated. Fasting glucose levels were significantly (p = 0.03) lower in recipient mice (Fig. 5a), while insulin levels tended to be lower, although this difference did not reach statistical significance (p = 0.13, Fig. 5b). Nevertheless, HOMA-IR was found to be statistically (p = 0.02) lower in recipient mice than in sham-operated controls (Fig. 5c), suggesting that an increase of intra-abdominal fat mass by transplantation of normal fat in fact improved fasting insulin sensitivity. To further verify this observation, we assessed whether there was a ‘dose-effect’ between the amount of transplanted fat and HOMA-IR. Consistent with the expected relationship between body mass and insulin sensitivity, total body weight at the time mice were killed positively correlated with HOMA-IR (r = 0.672, p = 0.024) by simple correlation analysis, whereas correlation between the transplanted fat weight and HOMA-IR tended to be negative (r = −0.42, p = 0.19) (Fig. 5d). Therefore, to evaluate the effect of fat transplantation independently of total body weight, we assessed the association between the transplanted fat weight and HOMA-IR, while adjusting for total body weight at time of death. Using a linear regression model, we found that the beta coefficient between the transplanted fat weight and HOMA-IR was −0.505, p = 0.031, while the β coefficient in the same model for total body weight was 0.728, p = 0.006. This suggests that, independently of the positive relationship between HOMA-IR and total body weight, increasing the amount of transplanted fat predicts increased fasting insulin sensitivity.

Fig. 5
figure 5

The effect of fat transplantation on fasting glucose, insulin and HOMA-IR. Fasting plasma glucose (a) and insulin (b) were measured in recipient and sham-operated mice after 7 h of food withdrawal, and HOMA-IR (c) was calculated as detailed in the Methods section. Results represent the mean±SEM of 11 to 12 different animals per group. d Pearson correlation between HOMA-IR and total body weight (stars, continuous line) (r = 0.672, p = 0.024) or transplanted fat pad weight (open circles, dotted line) (r = −0.42, p = 0.19) was performed. * p < 0.05; # p = 0.13

Discussion

It is unclear whether increased intra-abdominal fat mass as such or altered fat tissue biology contributes to the metabolic derangement associated with obesity. The first notion is supported by findings that intra-abdominal fat mass reduction improves insulin sensitivity in rats [4], whereas implantation of cultured adipocytes into the peritoneal cavity of mice induces insulin resistance [11]. Here we used intra-abdominal fat tissue transplantation to increase fat mass. Surprisingly, lean recipients of epididymal fat transplant from lean littermates exhibited improved fasting glucose tolerance and increased insulin sensitivity. Thus, increasing intra-abdominal fat mass by transplantation of normal adipose tissue did not mimic the effects of increased fat mass in obesity.

In this model, fat mass of transplanted fat tissue was inversely correlated with HOMA-IR, independently of the expected positive association between total body weight and HOMA-IR. Histological examination of the transplanted adipose tissue revealed that after 10 weeks of observation (transplantation to scarification) adipocyte cell size increased significantly in endogenous fat pads, whereas it remained unchanged in the transplanted fat pads (Fig. 2b). Insulin action was previously shown to be dependent on fat cell size: large adipocytes correlate well with insulin resistance [1214] and show decreased insulin-stimulated glucose uptake [15]. Interestingly, the transplanted fat depot exhibited features reminiscent of those induced in adipose tissue by thiazolidinediones. These drugs were shown to increase cellularity in adipose tissue by promoting fat cell differentiation and inducing apoptosis of large adipocytes, resulting in smaller, more insulin-sensitive adipocytes that secrete higher levels of adiponectin [16, 17]. It is thus possible that the insulin-sensitising effects of the transplant are secondary to similar alterations in the transplanted adipose tissue. We therefore assessed whether alterations in circulating levels of secretory products of fat tissue mediated the improved glucose tolerance and increased insulin sensitivity in mice receiving fat transplantation. However, we did not observe any significant increases in the circulating levels of potential insulin-sensitising adipokines like leptin or adiponectin [18] or any significant decreases in factors associated with reduced insulin sensitivity (resistin and NEFA, Table 1).

Although potentially informative, such analysis is limited in at least two major aspects. First, we measured total adiponectin levels, but recent studies suggest that the circulating high-molecular-mass complex of adiponectin correlates better with insulin sensitivity than total serum adiponectin levels [19, 20]. Second, with regard to the unaltered circulating levels of adipokines and NEFA observed by us, it should be noted that venous drainage of intra-abdominal fat is to the portal system. It therefore remains possible that intra-portal levels of secreted products were affected, thereby predominantly influencing liver glucose homeostasis. Such a scenario, in which the greatest effect of intra-abdominal fat tissue transplantation is seen in the liver, is also supported by the fact that the insulin-sensitising effects of intra-abdominal fat transplantation was largely observed in the fasting state, conditions in which glycaemia is largely controlled by hepatic glucose production and insulin sensitivity.

In conclusion, our findings suggest that in addition to increased fat mass, altered adipose tissue function is required to reproduce obesity-related metabolic changes such as insulin resistance. These changes may include impaired metabolic function of adipocytes, changes in cellular composition of adipose tissue (e.g. macrophage infiltration) [21] and/or alterations in the secretory function of adipose tissue (inflammatory cytokines, adipokines, NEFA). The second possible conclusion is that augmentation of normally functioning adipose tissue appears to result in a new metabolic steady state with increased insulin sensitivity. Such compensation and adaptation mechanisms may be unable to counterbalance larger degrees of fat tissue expansion. Yet, the results suggest that multiple factors in the cross-talk mechanisms between different insulin-sensitive tissues need to be affected in order to impair glucose homeostasis in obesity. The notion that adipose tissue function (rather than mass) and its inter-organ cross-talk are key determinants of obesity-induced metabolic derangement further defines this disorder as an endocrinopathy, and adipose tissue as an endocrine organ.