Animal care and use

Animal experiments were approved by the University of Pittsburgh Institutional Animal Care and Use Committee. Male C57BL/6J low‐fat diet (LFD) control (stock #380056) and diet‐induced obese mice (stock #380050) were obtained from The Jackson Laboratory aged 22–23 weeks, maintained on low‐fat diet (LFD; 70% carbohydrate, 20% protein, 10% fat; Research Diets D12450B) or high‐fat diet (HFD; 20% carbohydrate, 20% protein, 60% fat; Research Diets D12492) for 3–4 weeks while acclimating to their new environment, and used at 26 weeks of age (20 weeks total on HFD where appropriate).

Animal surgery and in vivo procedures

Mice received i.p. injections (b.i.d.) of vehicle (PBS) or adropin (450 nmol/kg) for 2 days, followed by a single i.p. injection on the morning of the third day prior to in vivo procedures (Fig. A).

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Adropin reduces fasting blood glucose and improves glucose tolerance in obese mice. (A) Injection schedule for adropin treatment prior to in vivo metabolism experiments. (B) Body weight was significantly increased in vehicle‐ and adropin (Adr)‐treated high‐fat diet (HFD) mice relative to low‐fat diet (LFD) controls. (C–E) Plasma glucose and insulin levels, along with HOMA‐IR, were significantly increased in vehicle‐treated HFD mice following an overnight fast. This increase was significantly attenuated in obese mice treated with adropin for 3 days. (F, G) Glucose tolerance was significantly improved in adropin‐treated HFD mice relative to vehicle‐treated obese controls. N = 6; *P < 0.05 versus LFD fed.

Hyperinsulinemic‐euglycemic clamps were performed as previously described, with minor modifications (Costa et al. ). Mice recovered for 1 week prior to clamp experiments following surgical implantation of an indwelling catheter in the right jugular vein. Mice were fasted 6 h prior to infusion with [3‐³H] glucose at a rate of 0.05 μCi/min for 120 min to determine basal glucose turnover. A primed infusion of insulin and [3‐³H] glucose was administered at 10.7 mU/kg/min and 0.24 μCi/min, respectively, for 4 min, after which rates were reduced to 4.5 mU/kg/min insulin and 0.1 μCi/min [3‐³H] glucose. Blood was collected by tail massage for plasma measurements at set time points, and a variable infusion of 20% dextrose was given to maintain euglycemia. A bolus injection of [1‐¹⁴C] 2‐deoxyglucose (10 μCi) was given at 55 min during steady state to determine tissue‐specific rates of glucose transport. Glucose turnover was calculated as the ratio of the [3‐³H] glucose infusion rate to the specific activity of plasma glucose at the end of the basal infusion and during the last 40 min of the hyperinsulinemic infusion. Endogenous or hepatic glucose output represents the difference between the glucose infusion rate and the rate of glucose appearance. The plasma decay curve and tissue levels of the [1‐¹⁴C] 2‐deoxyglucose tracer were used to calculate tissue‐specific glucose transport rates. After the final blood sample, mice were euthanized with an intravenous injection of 150 mg/kg pentobarbital sodium.

Glucose tolerance tests (GTTs) were performed after an overnight fast as previously described (Jurczak et al. ) with minor modifications. After collecting a basal plasma sample (t = 0), mice were injected intraperitoneally with a 2 g/kg glucose bolus and blood glucose was measured by tail bleed at set time points using a Bayer Contour Next EZ handheld glucometer (t = 15, 30, 45, 60, and 120 min). HOMA‐IR was calculated using the standard equation (fasting insulin x fasting glucose/22.5) (Kumar et al. ; Gao et al. ).

Western blotting

Liver tissue was rapidly harvested following sacrifice, washed in ice‐cold PBS, and flash‐frozen in liquid nitrogen. Tissues were homogenized using CHAPS lysis buffer using a bead mill, then incubated on ice for 60 min. Whole cell lysates were recovered by centrifugation at 4°C/13,000g for 5 min. Protein lysates were prepared in LDS sample buffer, separated using Bolt SDS/PAGE 4–12% or 12% Bis‐Tris gels, and transferred to nitrocellulose membranes (Life Technologies). Protein expression was analyzed using the following primary antibodies: rabbit GAPDH (2118S) from Cell Signaling Technologies; rabbit PDK4 (PA5‐13776) from ThermoFisher; goat PGC‐1α (ab106814) from Abcam; rabbit CD36 (18836‐1‐AP), rabbit CPT1a (15184‐1‐AP), rabbit PEPCK1 (16754‐1‐AP), and rabbit G‐6‐Pase (22169‐1‐AP) from ProteinTech. Protein loading was confirmed using GAPDH as a loading control. Images were obtained and quantified using the LiCor Odyssey system.

Peptide synthesis

The adropin (34–76) peptide was synthesized by the solid‐phase on Liberty Microwave Synthesizer using a FMOC synthesis protocol as previously reported (Thapa et al. ). The final product was re‐purified by HPLC and confirmed by mass spectrometry.

Statistics

Means ± SEM were calculated for all data sets. Data were analyzed using two‐tailed student's t‐tests or one‐way ANOVA (with Dunnett's post hoc tests) as appropriate. P < 0.05 was considered significant.

Adropin reduces fasting blood glucose and improves glucose tolerance in obese mice

Previous studies have shown that acute adropin treatment improves glucose homeostasis in diet‐induced obese mice fed a HFD for 18–20 weeks (Kumar et al. ; Gao et al. ). We first sought to replicate these studies under our experimental conditions to ensure technical fidelity. LFD and HFD mice were given serial i.p. injections of vehicle or adropin over 3 days, followed by a 16‐h fast (Fig. A). Both the HFD mouse groups showed significantly increased body weight compared to LFD‐fed controls after 20 weeks (Fig. B). Fasting blood glucose and insulin (along with HOMA‐IR) were significantly elevated in vehicle‐treated HFD mice, which was reversed by adropin treatment (Fig. C–E). Mice were then given a bolus i.p. injection of glucose, and their plasma glucose levels measured over the next 120 min. Whole‐body glucose clearance was significantly decreased in vehicle‐treated HFD mice relative to LFD‐fed controls, while adropin‐treated HFD mice showed no change relative to LFD‐fed controls (Fig. F,G). Overall, these data support and extend upon previous studies showing that exogenous adropin treatment improves glucose tolerance in obese mice.

Adropin treatment has negligible effects on whole‐body insulin sensitivity, while reducing whole‐body glucose uptake, in obese mice

Previous studies demonstrated improved glucose tolerance in adropin‐treated obese mice, but could not account for tissue‐specific contributions to the observed improvements in whole‐body glucose homeostasis in vivo (Kumar et al. ; Gao et al. ). To better understand the action of adropin on glucose metabolism in obesity, we next examined insulin sensitivity, as well as whole‐body and tissue‐specific glucose metabolism in vehicle‐ and adropin‐treated mice using hyperinsulinemic‐euglycemic clamps. Body weights in both the HFD mouse groups were matched (Fig. A), and adropin treatment did not significantly affect insulin levels under basal or clamp conditions (Fig. B). Glucose infusion rates required to maintain euglycemia (Fig. C) in adropin‐treated HFD mice were 10% higher than in vehicle‐treated HFD controls during the clamp; however, this trend did not reach statistical significance (Fig. D,E). This suggests that adropin has only a moderate positive effect on whole‐body insulin sensitivity under hyperinsulinemic conditions.

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Adropin has minimal beneficial effects on whole‐body insulin sensitivity in obese mice. (A) Body weights were matched between vehicle‐ and adropin (Adr)‐treated high‐fat diet (HFD) mice groups. (B) There was no significant difference in plasma insulin levels under basal or hyperinsulinemic‐euglycemic clamp conditions. (C, D, E) Treatment with adropin led to a small, but nonsignificant improvement in whole‐body insulin sensitivity as shown by an increased glucose infusion rate required to maintain and match euglycemia between the groups over the course of the clamp. N = 6–8.

Analysis of glucose turnover showed that adropin treatment significantly reduced whole‐body glucose uptake (Fig. A). This correlated to a nonsignificant ~15% decrease (P = 0.23) in gastrocnemius glucose uptake (Fig. B). In contrast, uptake rates in the quadricep and heart remained unchanged (Fig. C, and data not shown). These data suggest that any moderate improvements in insulin sensitivity in adropin‐treated obese mice are not due to increased muscle glucose utilization under hyperinsulinemic conditions.

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Adropin reduces whole‐body insulin‐stimulated glucose uptake in obese mice. (A) Whole‐body glucose uptake was significantly decreased in adropin (Adr)‐treated obese mice relative to high‐fat diet (HFD) controls under hyperinsulinemic conditions. (B) There was a small, but nonsignificant decrease in glucose uptake in the gastrocnemius of adropin‐treated HFD mice. (C) Furthermore, there was no change in quadricep glucose transport between the HFD mouse groups. N = 6–8; *P < 0.05 versus vehicle‐treated HFD.

Adropin lowers fasting hepatic glucose production and improves hepatic insulin sensitivity during hyperinsulinemic conditions

Finally, we examined other pathways that may promote improved glucose homeostasis in obese mice treated with adropin. Under basal fasting conditions, we found that there was a trend (P = 0.06) toward reduced endogenous (hepatic) glucose production in adropin‐treated HFD mice relative to their vehicle‐treated controls (Fig. A). This trend was maintained under clamp conditions, and there was a significant reduction in hepatic glucose production in adropin‐treated mice relative to control animals (Fig. A). These data suggest that adropin reduces basal rates of hepatic glucose production and improves hepatic insulin sensitivity during hyperinsulinemia.

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Adropin improves hepatic insulin sensitivity in obese mice during hyperinsulinemia. (A) There was a decrease in hepatic glucose production under both basal and hyperinsulinemic conditions in adropin (Adr) mice. (B–H). Adropin treatment suppressed expression of hepatic fatty acid uptake (CD36 and CPT1a), PDH‐inhibitory (PDK4), and gluconeogenic (G‐6‐Pase) proteins in high‐fat diet (HFD) diet mice. N = 4–8; *P < 0.05 versus vehicle‐treated HFD.

Adropin treatment of obese mice has been shown to limit fatty acid oxidation in skeletal muscle homogenates by reducing the expression of fatty acid uptake proteins, leading to a concurrent increase in glucose utilization (Gao et al. ). As fatty acid oxidation contributes to the energy required for hepatic glucose production (Rui ), we examined whether adropin treatment impacted mediators of fatty acid uptake in the liver. As expected, in both the HFD mouse groups there was a significant elevation of PGC‐1α expression relative to LFD mice (Fig. B,C). Despite this, there was a significant decrease in the expression of the cell membrane fatty acid uptake protein CD36, and a trend toward a decrease (P = 0.12) in the expression of the mitochondrial fatty acid translocator CPT1a, in adropin‐treated HFD mice relative to vehicle‐treated obese controls (Fig. B,D,E). Additionally, while there was a significant upregulation of the pyruvate dehydrogenase inhibitory kinase PDK4 in HFD mice relative to LFD controls, this effect was lost following adropin treatment (Fig. B,F). Finally, while there was no change in the expression of the gluconeogenic enzyme PEPCK1, we found that there was a significant increase in G‐6‐Pase expression in HFD mice which was reversed by adropin treatment (Fig. B,G,H). Combined, these data point to a decrease in fatty acid utilization and reduced gluconeogenic activity as a potential mechanism for reduced hepatic glucose production in adropin‐treated obese mice.