Abstract
Excess caloric intake results in increased fat accumulation and an increase in energy expenditure via diet-induced adaptive thermogenesis; however, the underlying mechanisms controlling these processes are unclear. Here we identify the neuropeptide FF receptor-2 (NPFFR2) as a critical regulator of diet-induced thermogenesis and bone homoeostasis. Npffr2−/− mice exhibit a stronger bone phenotype and when fed a HFD display exacerbated obesity associated with a failure in activating brown adipose tissue (BAT) thermogenic response to energy excess, whereas the activation of cold-induced BAT thermogenesis is unaffected. NPFFR2 signalling is required to maintain basal arcuate nucleus NPY mRNA expression. Lack of NPFFR2 signalling leads to a decrease in BAT thermogenesis under HFD conditions with significantly lower UCP-1 and PGC-1α levels in the BAT. Together, these data demonstrate that NPFFR2 signalling promotes diet-induced thermogenesis via a novel hypothalamic NPY-dependent circuitry thereby coupling energy homoeostasis with energy partitioning to adipose and bone tissue.
Similar content being viewed by others
Introduction
Energy homoeostasis is fundamental for survival and there are adaptive mechanisms in place to counteract energy imbalances1,2. In particular, under a positive-energy balance induced by excessive caloric intake, energy expenditure is increased to limit weight gain3,4,5. This capacity to increase energy expenditure in response to caloric excess is commonly referred to as diet-induced thermogenesis and consistently observed in humans4,6 and rodents3,5. One of the most critical tissues facilitating this process is brown adipose tissue (BAT), which, through an uncoupling protein-1 (UCP-1)-dependent mechanism, activates diet-induced thermogenesis7,8. Recent studies also revealed a creatine-futile-cycle pathway in white adipose tissue contributing to this thermogenetic response9. However, in comparison with the research advances made in this area in the periphery, far less is known about the central mechanisms.
The brain receives a variety of peripheral signals conveying nutrient status, thereby detecting perturbations in energy balance and allowing for the activation of adaptive mechanisms. The hypothalamus and brain stem are two key regions where peripheral circulating factors and sensory afferent fibres integrate with the central circuitry with a variety of different neuropeptide-expressing neuronal populations involved10,11,12. Among them is a group of neuropeptides belonging to the RF-amide peptide family including the neuropeptide FF group (NPFF and neuropeptide AF), the RFamide-related peptides group (RFRP-1 and -3, also named NPSF and NPVF), the prolactin-releasing peptide (PrRP) group, the pyroglutamylated RFamide peptide group (26RF and QRFP) and the kisspeptin group13. Interestingly, physiological studies have linked them to the regulation of feeding and energy homoeostasis14. For example, NPFF, which is expressed by neurons in the brain stem15,16, has been shown to reduce short-term feeding in rats and in pre-fasted and ad libitum-fed mice17,18. PrRP-expressing neurons expressed in the brain stem have been suggested to relay signals that mediate satiety17, whereas PrRP-expressing neurons in the dorsal medial hypothalamus are thought to mediate the thermogenic effect of leptin19. The kisspeptin system — best known for its role in stimulating the reproductive axis — is also increasingly recognized as an important factor in the energy metabolism and glucose regulation20,21.
RFamide peptides exert their functions via Gi/o associated G-protein-coupled receptors of which five have been identified in mammals, i.e., NPFFR1, NPFFR2, GPR10, GPR103 and KISS1R13. Pharmacological studies have revealed that the endogenous ligands NPFF and RFRPs are recognized by more than one receptor adding to the complexity of this system22. NPFFR2, which can be activated by NPFF, NPVF, PrRP and kisspeptin22,23,24, has the highest levels of expression in the hypothalamic nuclei that are linked to the regulation of energy homoeostasis25. Thus, it is likely to be that NPFF, NPVF, PrRP and kisspeptin influence aspects of energy homoeostasis predominantly via signalling at the NPFFR2.
Multi-ligand/multi-receptor systems with their susceptibility to cross-reactions impose great challenges on investigations into the specificities of the peptide and receptor functions. This is further complicated by the lack of selective agonist or antagonist suitable for in vivo investigation. Thus, we generated a variety of NPFFR2 mouse models and systematically examined the impact of altering NPFFR2 signalling on parameters of energy balance and its potential involvement in the regulation of diet-induced thermogenesis. Our results show that NPFFR2 signalling in the arcuate nucleus of the hypothalamus is crucial in maintaining a basal tone of neuropeptide Y (NPY), lack of which renders downstream pathways that control adaptive thermogenesis in the BAT unresponsive to caloric excess and consequently leads to exacerbated diet-induced obesity.
Results
Energy status regulates the expression of NPFFR2 ligands
The expression of the main ligands of NPFFR2 (NPFF, NPVF and PrRP) are altered depending on energy status with Npff mRNA being significantly reduced in response to 8 weeks of high-fat diet (HFD) feeding (Fig. 1a–c) and significantly increased after 24 h fasting (Fig. 1c). The hypothalamic expression of Npvf was significantly reduced in response to HFD (Fig. 1d) but unaltered by fasting (Fig. 1d). PrRP (Prlh) mRNA levels were significantly increased in the nucleus tractus solitarius (NTS; Fig. 1e, f) but were unaltered in the hypothalamus in response to HFD feeding (Fig. 1g), whereas hypothalamic Prlh mRNA expression was strongly reduced in response to fasting (Fig. 1g).
To test whether the expression of these ligands is under the control of leptin, we examined subpostrema area (SubP) Npff and NTS Prlh mRNA expression in Lep−/− mice. Consistent with the downregulation of SubP Npff and upregulation of NTS Prlh expression under HFD feeding (high leptin), Lep−/− mice exhibited significantly increased and decreased expression of SubP Npff and NTS Prlh, respectively (Fig. 1h–j). To examine whether leptin has a direct action on Npff expression, we conducted dual in situ hybridization (ISH) for Npff and Lepr. Although Npff staining is elevated in Lep−/− mice (Fig. 1k) — consistent with Fig. 1h — little or no colocalization of Lepr and Npff was evident (Fig. 1k), suggesting an indirect action of leptin, if any, in the regulation of Npff mRNA expression.
Generation and behavioural examination of Npffr2 −/− mice
To investigate the role of NPFFR2 signalling in the regulation of energy homoeostasis, we generated germline Npffr2−/− and conditional Npffr2lox/lox mouse models (Supplementary Fig. 1). Breeding of heterozygous Npffr2+/− mice resulted in live offspring with a frequency of genotypes that was not significantly different from the expected Mendelian ratio (Supplementary Fig. 2a) and with litter sizes actually being larger than those from wild-type (WT) breeding pairs (Supplementary Fig. 2b). Importantly, homozygous Npffr2−/− breeding pairs produced litters of a similar size to those of WT breeding pairs (Supplementary Fig. 2b), indicating that deletion of the Npffr2 does not affect fertility. Mortality rate and gender ratio of pups born from heterozygous and homozygous breeding pairs were not significantly different from those of WT (Supplementary Fig. 2c–d), suggesting that disruption of Npffr2 expression does not impact upon reproductive fitness.
Npffr2−/− and littermate control mice were further tested in behavioural test paradigms to identify potential abnormalities that could influence energy homoeostasis. Npffr2−/− mice of both genders did not differ from controls with regard to motor function or sensorimotor gating (Supplementary Table 1). In addition, neither the open-field test nor the elevated plus maze test revealed an anxiety-related phenotype (Supplementary Table 1). Finally in a hot water tail-flick test, the latency to flick the tail was comparable between Npffr2−/− and WT mice (Supplementary Table 1), indicating an unaltered responsiveness of Npffr2−/− mice to a thermal stimulus.
Enhanced diet-induced obesity in Npffr2 −/− mice
On a standard chow diet, male Npffr2−/− mice displayed a similar growth curve as WT mice (Fig. 2a). However, weight gain over a 10-week monitoring period (i.e., between 10 and 20 weeks of age) showed a small but significant reduction in the Npffr2−/− mice (Fig. 2b). Whole-body lean and fat masses assessed by dual-energy X-ray absorptiometry (DEXA) (Supplementary Fig. 3a, b) and adiposity assessed by the weights of dissected white adipose tissue depots (Fig. 2c, d) were unaltered in male Npffr2−/− mice. Female Npffr2−/− mice showed comparable body weight and weight gain to WT mice (Fig. 2e, f), but displayed a lean phenotype with significantly reduced individual and summed fat depots (Fig. 2g, h) (Supplementary Fig. 3c, d). Food intake in Npffr2−/− mice showed a significant reduction in males but not in females (Fig. 2i, j), suggesting that reduced feeding may contribute to the reduced body weight gain in the male Npffr2−/− mice (Fig. 2b).
When fed on a HFD, Npffr2−/− mice of both genders showed significantly greater gains in body weight (Fig. 2k, l) and adiposity (Fig. 2c, d, g, h). Serum leptin levels were significantly elevated in both HFD-fed WT and Npffr2−/− mice vs. their chow-fed counterparts with a greater increase in Npffr2−/− mice (Fig. 2m). In addition, HFD feeding led to increased serum insulin levels in both WT and Npffr2−/− mice, significantly so in female mice (Fig. 2n). Mice on HFD had higher calorie intake than their gender- and genotype-matched chow-fed counterparts (Fig. 2i, j); however, caloric intake on HFD was lower in the Npffr2−/− than WT mice, significantly so in male mice (Fig. 2i, j). This reduced energy intake in Npffr2−/− mice on HFD is in contrast to their exacerbated obesity suggesting mechanisms other than feeding are critical for this phenotype to occur.
Impaired diet-induced thermogenesis in Npffr2 −/− mice
Male Npffr2−/− mice on chow showed comparable energy expenditure (normalized to metabolically active tissue (MAT) weight26,27) and physical activity to male WT mice (Fig. 3a, c, i, k), whereas female Npffr2−/− mice displayed a significant increase in light-phase energy expenditure and overall physical activity (Fig. 3b, d, j, l). Respiratory exchange ratio (RER) was unaltered in Npffr2−/− compared with WT mice in both genders (Fig. 3m, n).
Interestingly, when fed a HFD for 7 weeks, Npffr2−/− mice of both sexes had significantly reduced energy expenditure compared with gender-matched WT mice (Fig. 3e, f, i, j), with female but not male Npffr2−/− mice also exhibiting a reduction in overall activity (Fig. 3g, h). When energy expenditure under chow and HFD conditions was compared, both Npffr2−/− and WT mice on HFD showed significantly higher energy expenditure (Fig. 3i, j), consistent with an elevation in diet-induced thermogenesis. However, this increase in energy expenditure on HFD was significantly diminished in both male and female Npffr2−/− compared with gender-matched WT mice (Fig. 3i, j). Physical activity was significantly increased in female HFD-fed WT mice, but this was not observed in female or male Npffr2−/− mice (Fig. 3k, l). RER was lower under HFD conditions compared with chow conditions for both WT and Npffr2−/− mice (Fig. 3m, n), indicating a greater use of lipids as oxidative fuel during HFD feeding. Moreover, under HFD, female but not male Npffr2−/− mice had significantly lower RER than gender-matched WT mice (Fig. 3m, n). However, as obesity itself is known to decrease RER by enhancing lipid supply28, the decreased RER in Npffr2−/− mice on HFD may be secondary to the increased obesity in these mice.
Taken together, these results demonstrate that NPFFR2 signalling regulates energy balance under basal chow conditions in a gender-dependent manner. However, when energy homoeostasis is challenged by an obesogenic diet, NPFFR2 signalling has a key role in mediating diet-induced adaptive thermogenesis uniformly in both genders.
Impaired diet-induced brown fat thermogenesis in Npffr2 − /− mice
As diet-induced adaptive thermogenesis primarily takes place in BAT7,8, we investigated BAT thermogenesis by measuring temperatures at the BAT (TBAT) and lumbar back (TBack) regions of freely moving mice using infrared imaging. We also calculated the temperature difference between the BAT and lumbar back regions (ΔTBAT-Back) as an indicator of BAT thermogenesis, since during increased BAT thermogenesis ΔTBAT-Back would be expected to increase due to a direct contribution of heat arising from the BAT depot. TBAT and TBack in group-housed male or female mice on either chow or HFD were measured at baseline (14 weeks of age) and 6 weeks later (20 weeks of age). As results were consistent between the two genders, for clarity only data from female mice are presented here and male data are presented in Supplementary Fig. 4c-g. At baseline, WT and Npffr2−/− mice had comparable TBAT, TBack and ΔTBAT-Back (Fig. 4a, b). After 6 weeks of HFD, WT mice showed a significant increase in TBAT and a trend towards an increase in TBack, which resulted in an increase in ΔTBAT-Back (p = 0.07 HFD-fed vs. chow-fed WT mice by t-test) (Fig. 4c). These increases induced by HFD in WT mice were not seen in Npffr2−/− mice (Fig. 4d), indicating an impaired BAT thermogenic response to HFD in the absence of NPFFR2 signalling. Of note, TBAT and TBack in chow-fed Npffr2−/− mice at 20 weeks of age were higher compared with WT mice (Supplementary Fig. 4a), which could be due to a differential response between Npffr2−/− and WT mice to handling stress. Importantly however, ΔTBAT-Back was not significantly different between chow-fed Npffr2−/− and WT mice either at baseline or at the 6 weeks later time point (Supplementary Fig. 4b), suggesting comparable BAT thermogenesis between WT and Npffr2−/− mice under chow conditions. Male Npffr2−/− mice exhibited a similar thermogenic profile (Supplementary Fig 4c) and most importantly also exhibited the lack of increase in ΔTBAT-Back in response to HFD (Supplementary Fig 4f,g) consistent with a gender-independent mechanism to control diet-induced thermogenesis in the absence of NPFFR2 signalling.
We examined BAT protein levels for UCP-1 and peroxisome proliferator-activated receptor-γ coactivator (PGC)-1α, the two key molecules involved in BAT adaptive thermogenesis7,8,29. BAT weight was significantly higher in Npffr2−/− mice (Fig. 4e) in association with a trend towards increased protein content in the BAT tissue (Fig. 4f). Under HFD, WT and Npffr2−/− mice significantly increased their BAT weights (Fig. 4e) that was attributable at least in part to an increase in protein content (Fig. 4f). The basal expression of BAT UCP-1 and PGC-1α per mg protein was unaltered in Npffr2−/− mice (Fig. 4g–i). When fed on HFD, WT but not Npffr2−/− mice showed marked increases in UCP-1 and PGC-1α levels per mg protein (Fig. 4g–i). When increases in BAT mass under HFD were taken into account, UCP-1 expression per BAT depot showed a significant increase in WT and Npffr2−/− mice on HFD; however, this increase was significantly smaller in Npffr2−/− compared with WT mice (Fig. 4j). Similarly, the PGC-1α expression per BAT depot was significantly increased in HFD-fed WT but not in Npffr2−/− mice (Fig. 4k).
To investigate whether cold-induced BAT thermogenesis is affected in Npffr2−/− mice we used single housing as a mild cold challenge compared with group housing at standard (22 °C) temperature30. Singly housed WT mice showed significantly higher TBAT but a comparable TBack to group-housed animals, which led to a significantly higher ΔTBAT-Back in the single-housed mice (Fig. 4l). Npffr2−/− mice exhibited similar thermogenic responses to single housing as those seen in WT mice (Fig. 4m), indicating normal BAT thermogenic function in response to mild cold stress in the absence of NPFFR2 signalling. We further examined BAT thermogenesis at thermoneutrality (TN, 28 °C), using room temperature (RT) as the cold challenge. The ΔTBAT-Back was significantly higher under RT compared with that under TN in both WT and Npffr2−/− mice, and this increase in ΔTBAT-Back was similar in magnitude between WT and Npffr2−/− mice (Fig. 4n). Together, these results demonstrate that cold-induced thermogenesis is not controlled by NPFFR2 signalling.
We next examined BAT thermogenesis in WT and Npffr2−/− mice fed a HFD under TN condition. Npffr2−/− mice fed a HFD under TN exhibited significantly greater weight and fat gain compared to WT mice (Fig. 4o–q). Importantly, WT mice on HFD showed significant increases in TBAT and ΔTBAT-Back compared with chow-fed animals (Fig. 4r), whereas no such increases were seen in Npffr2−/− mice (Fig. 4s).
As leptin has been shown to have a role in diet-induced BAT thermogenesis31, we investigated the influence of leptin action in the absence of NPFFR2 signalling by examining pSTAT3 expression using immunohistochemistry in WT and Npffr2−/− mice in response to leptin stimulation. Chow-fed WT and Npffr2−/− mice had comparable basal pSTAT3 levels in the Arc of the hypothalamus and showed a more than twofold increase in pSTAT3 activation in response to leptin—administered either intraperitoneal (i.p.) (2 µg/g body weight) or intracerebroventricular (i.c.v.) (1.25 µg)—(Fig. 5a, b). WT and Npffr2−/− fed on HFD showed similar pSTAT3 in the Arc at baseline (Fig. 5a, b) and marked increases in pSTAT3 activation in response to i.p. leptin which was significantly greater in Npffr2−/− mice (Fig. 5a, b). These results demonstrate that leptin-induced pSTAT3 activation is not impaired in Npffr2−/− mice, suggesting that defective leptin signalling is unlikely to contribute to the impaired BAT thermogenesis and exacerbated diet-induced obesity seen in Npffr2−/− mice.
NPFFR2 signalling controls BAT function via an Arc NPY circuit
Consistent with a predominantly central action of NPFFR2, the Npffr2 mRNA is highly expressed in the hypothalamus with only minute levels in subcutaneous white adipose tissue and not detectable in BAT (Fig. 5c). Moreover, hypothalamic Npffr2 mRNA expression was significantly decreased in HFD versus Chow-fed mice (Fig. 5d), demonstrating the responsiveness of the hypothalamic NPFFR2 signalling to changes in energy status. ISH using RNAscope identified the most abundant expression of Npffr2 in the Arc (Fig. 5e) with high concentration at the ventral medial region (Fig. 5e–(i)) and little expression at the dorsal lateral part (Fig. 5e-(ii)). The accessibility of the Arc by RFamide peptides is supported by studies showing direct projections and actions of RFamide peptide-expressing neurons (e.g., Npvf- and Kiss1-expressing neurons) towards the Arc20,32,33 and hormone-like action of NPFF via secretion into the blood stream and cerebrospinal fluid34,35. Using retrograde tracing we show that projections from the SubP, where NPFF is predominantly expressed, exist that connect to the Arc (Supplementary Fig. 5a–e). Thus, red fluorescent beads were injected into the Arc and the fluorescent signal was examined 2 weeks later in the brain stem. Strong red fluorescence was seen at the injection site, which had some ‘crossover’ to the green channel due to the brightness of the tracer36. Importantly, specific red fluorescence-labelled cells and fibres were observed in the area postrema (AP) and SubP without any crossover to the green channel (Supplementary Fig. 5c–e). Specific red fluorescence-labelled cells and fibres were also seen in the NTS (Supplementary Fig. 5f–h), although appear to be fewer than those in the AP and SubP (Supplementary Fig. 5e).
To examine whether a lack of NPFFR2 alters the expression of related receptors of cross-reacting ligands, we determined the hypothalamic expression of Kiss1r and Npffr1—the cognate receptor for Kisspeptin and NPVF, respectively20,32,33,37 — in Npffr2−/− and WT mice. Although the expression of Npffr1 was not detectable in either WT or Npffr2−/− hypothalamic tissue (data not shown), the hypothalamic expression of Kiss1r was not significantly different between WT and Npffr2−/− mice (Supplementary Fig. 6a) and was not altered by HFD (Supplementary Fig. 6b), arguing against a compensatory action from related receptor signalling due to NPFFR2 deletion and contrasting the responsiveness of hypothalamic Npffr2 to the changed energy status (Fig. 5d).
As NPY signalling pathways originating from the Arc are known to have a key role in the regulation of energy homoeostasis38, we investigated whether its expression is influenced by lack of NPFFR2 signalling. Interestingly, Npffr2−/− mice under chow conditions exhibited significantly lower Npy mRNA levels in the Arc compared with WT mice (Fig. 5f, i). Six weeks of HFD feeding resulted in an approximately 30% reduction in Arc Npy mRNA expression in WT but not in Npffr2−/− mice compared with their chow counterparts (Fig. 5f, i). In contrast, expression of pro-opiomelanocortin (Pomc) mRNA was significantly increased in Npffr2−/− compared with WT mice under both chow and HFD conditions without significant effect of diet in either genotype (Fig. 5g).
To test whether NPFFR2 signalling uses a known NPY-dependent relay via tyrosine hydroxylase (TH)-positive neurons in the paraventricular nucleus (PVN)38, we investigated the expression levels of PVN-Th mRNA by ISH. Under chow PVN-Th mRNA was unaltered in Npffr2−/− mice (Fig. 5h, j); however, when fed a HFD for 6 weeks, PVN-Th mRNA levels were significantly increased in WT but not in Npffr2−/− mice (Fig. 5h,j). Thyrotropin-releasing hormone (Trh) mRNA showed a strong trend towards increasing in WT but not Npffr2−/− mice in response to HFD (Supplementary Fig. 6c). Oxt mRNA levels were significantly reduced in response to HFD in both WT and Npffr2−/− mice without significant differences between genotypes (Supplementary Fig. 6d). Together, these results indicate that the responsiveness of PVN-TH neurons to a HFD in terms of Th expression level is dependent on NPFFR2 signalling.
NPFFR2 signalling regulates bone metabolism
As Arc NPY neurons are also involved in the regulation of bone homoeostasis39, we used micro-computed tomography (μCT) analysis on isolated femora. Male Npffr2−/− mice, while having slightly reduced femoral length (Fig. 6a), have a significant increase in cancellous bone mass (bone volume over total volume, BV/TV) compared with WT mice (Fig. 6b), associated with a significant increase in trabecular thickness and trabecular number (Fig. 6c, d). Cortical bone volume and cortical thickness also showed a trend towards increasing in male Npffr2−/− mice (Fig. 6i,j). In contrast, female Npffr2−/− mice had unaltered femoral length and significant increases in cortical volume and cortical thickness compared with WT mice (Fig. 6k, l) without significant changes in cancellous bone parameters including cancellous bone volume (Fig. 6f), trabecular thickness (Fig. 6g) and trabecular number (Fig. 6h).
NPFFR2 signalling directly acts on Arc NPY neurons
To investigate whether NPFFR2 signalling directly regulates NPY-expressing neurons, a translating ribosome affinity purification (TRAP) approach was employed. Thus, GFP-L10a fusion protein encoding Rosa26CAG-EGFP (TRAP) mice40 were crossed onto our Npycre/+ mice to generate the Npycre/+; TRAPlox/lox mice (NPY-TRAP), where the ribosomal L10a-GFP fusion protein is only produced in NPY neurons (Fig. 7a). As a control we used InsCre/+; TRAPlox/lox mice (Ins-TRAP) in which the L10a-GFP fusion protein is expressed ubiquitously in the hypothalamus, as well as TRAPlox/lox (WT-TRAP) mice without any cre (Supplementary Fig. 7a). Quantitative PCR (qPCR) performed on mRNA isolated by immunoprecipitation with an anti-green fluorescent protein (GFP) antibody against the GFP-tagged ribosomal unit confirmed a significant enrichment of GFP and Npy transcripts in the immunoprecipitated RNA relative to the corresponding unprocessed RNA (Input) sample (Supplementary Fig. 7b) with no Npy enrichment in mice without the activation of TRAP (WT-TRAP) (Fig. 7b). Importantly, Npffr2 mRNA was also highly enriched indicating that Npffr2 is expressed on the NPY neurons in the Arc (Fig. 7c). Interestingly, Npffr2 enrichment was not observed in a NPY neuronal population from the amygdala where Npffr2 mRNA was actually deriched (Supplementary Fig. 7c).
Consistent with the TRAP results, dual ISH using RNAscope shows that a subset of NPY neurons in the Arc express Npffr2 (Fig. 7d-(i))—results also confirmed by recent studies employing a single-cell sequencing approach on Arc neurons41,42. Of note, there are Arc NPY neurons that do not express Npffr2 (Fig. 7d-(ii)), as well as non-NPY neurons that do express Npffr2 (Fig. 7d-(iii)), suggesting that NPFFR2 signalling could also affect other Arc neurons, allowing for the possibility of an indirect action of NPFFR2 signalling on NPY neurons. A similar distribution of Npffr2 expression with an overlap with NPY neurons can also be found in the DMH (dorsomedial hypothalamic nucleus; Supplementary Fig. 7e), a hypothalamic nuclei also known to have influences on BAT function43.
It is worth noting that although the neurochemical identities of these Arc Npffr2-expressing non-NPY neurons remains to be determined, they are unlikely to be the Pomc-expressing neurons, as little colocalization of Pomc and Npffr2 mRNA was observed (Supplementary Fig 7e), consistent with single-cell sequencing findings41.
As NPFFR2 has been shown to couple to the activation of the class of G-proteins that inhibit cAMP accumulation44,45, we examined the effect of NPFF-induced NPFFR2 signalling on the phosphorylation of the cAMP-responsive element binding protein (CREB) — a downstream responder to forskoline-induced increases in cAMP levels — using NPY-GFP mice46,47. I.c.v. injection of forskoline produced a marked increase in pCREB immunoreactivity in approximately 60% of Arc NPY neurons compared with saline-injected controls (Fig. 7e). Although NPFF alone had no apparent effect on cAMP/CREB activation (Fig. 7e), co-administration of NPFF with forskolin significantly reduced the number of Arc NPY neurons colocalized with pCREB-ir (approximately 20%) (Fig. 7f, Supplementary Table 2), demonstrating a direct action of NPFFR2 signalling on NPY neurons in the Arc.
NPFFR2 signalling on NPY neurons regulates diet-induced thermogenesis
The direct role of NPFFR2 signalling on NPY neurons in the control of energy homoeostasis in vivo was tested by an inducible conditional NPFFR2 knockout (KO) mouse model (NpycreER2/+,Npffr2lox/lox) where Npffr2 deletion occurs specifically in NPY neurons upon induction by tamoxifen. As controls, NpycreER2/+,Npffr2lox/lox mice without tamoxifen treatment and NpycreER2/+,Npffr2lox/+ mice treated with tamoxifen were used. Tamoxifen-induced NPY neuron-specific Npffr2 gene deletion was confirmed by PCR in NPY-expressing tissues including the hypothalamus, olfactory bulb and adrenal gland, but was absent in tissues with no NPY expression (e.g., the liver) or in tissues of mice that were not treated with tamoxifen (Supplementary Fig. 8).
Conditional NpycreER2/+,Npffr2lox/lox KO (referred as ‘conditional KO’ hereinafter) mice and control mice on chow diet were not significantly different with regard to body weight (Fig. 8a) or adiposity (Fig. 8b, c). Five weeks of HFD led to the development of obesity in both conditional KO and control mice with a trend of higher body weight (Fig. 8d) and significant greater increases in fat mass in the conditional KO mice (Fig. 8b, c), consistent with the results from the global Npffr2−/− mice.
Both control and conditional KO mice had greater energy intake on HFD than on chow with no significant difference between genotypes under either diet (Fig. 8e). Energy expenditure did not significantly differ between control and conditional KO mice under chow (Fig. 8f, l) or after 4 weeks of HFD (Fig. 8i, l); however, a strong trend towards a decrease in energy expenditure in the HFD conditional KO mice in the early period of the dark phase was observed (Fig. 8i). Physical activity was not significantly altered by genotype or diet (Fig. 8g, j, m). Interestingly, RER, although not significantly different between control and conditional KO mice under chow (Fig. 8h, n), was markedly higher in conditional KO mice when fed on HFD (Fig. 8k, n), suggesting a reduced reliance on lipids as oxidative fuel when there is an increased dietary lipid influx likely contributing to the greater fat gain in the conditional KO mice under HFD (Fig. 8b, c).
We also examined BAT thermogenesis in an additional cohort of mice at an earlier time point, i.e., 10 days after starting HFD. Both control and conditional KO mice showed significantly increased TBAT and an unaltered TBack (Fig. 9a, b), leading to a significant increase in ΔTBAT-Back (Fig., 9c). The increase in ΔTBAT-Back by HFD was significantly less in the conditional KO mice compared with controls (Fig. 9c), suggesting that diet-induced BAT activation is impaired in mice lacking NPFFR2 in NPY neurons in the early phase of HFD exposure. We further conducted indirect calorimetry during the transition period from chow to HFD where mice were monitored for the first 5 days of HFD feeding. Both control and conditional KO mice showed increased caloric intake once the diet was switched from chow to HFD (Fig. 9d). Importantly, although energy expenditure was increased on HFD compared with chow in both conditional KO and control mice, this increase was lower in the conditional KO mice with significant effects most evident during the light phase (Fig. 9e, f). These data show a key role of NPFFR2 signalling in NPY neurons in the quick implementation of HFD diet-induced thermogenesis in BAT.
NPFFR2 signalling on NPY neurons controls bone formation
Conditional KO mice displayed an increase in femur length, femur bone mineral density and a trend towards an increase in femur bone mineral content (Fig. 9g–i), demonstrating that specific signalling of NPFFR2 in NPY neurons is important for the control of bone formation. Further μCT analysis revealed that the conditional KO mice had significant increases in both trabecular and cortical bone mass, i.e., significant increases in cancellous bone volume, trabecular thickness, trabecular number, cortical bone volume and cortical thickness (Fig. 9j–o). These results are consistent with the findings in the global Npffr2−/− mice and confirm that NPFFR2 signalling also has a major role in the central regulation of bone homoeostasis via direct actions on NPY neurons.
Discussion
This study demonstrates that HFD-induced adaptive thermogenesis is dependent on functional signalling through NPFFR2 receptors. Loss of NPFFR2 results in significantly greater diet-induced increases in body weight and adiposity, predominantly due to a lack of BAT activation and a subsequent reduction in energy expenditure. One of the critical relay points for this thermogenic control is the Arc, where NPFFR2 signalling provides the tone for maintaining a baseline level of NPY expression necessary to exert homoeostatic control, via direct and possibly also indirect actions. Lack of this NPFFR2-induced tone on NPY neurons reduces the capacity of these neurons to control TH-positive neurons in the PVN, with a consequent reduction in BAT function38.
Our results show that NPFFR2 signalling regulates energy metabolism and bone mass in a gender-dependent manner under basal chow-fed conditions. However, under obesogenic conditions, NPFFR2 signalling exerts a uniform action in both genders to regulate diet-induced thermogenesis. It is interesting to note that there is a gender difference in the response of physical activity to energy excess, in that female but not male mice increased their activity in response to HFD. This increase in physical activity during HFD in female mice is consistent with observations in humans suggesting that increased physical activity can be an adaptive response to overfeeding48. Our study further shows that this increase in physical activity associated with HFD is absent in female Npffr2−/− mice, suggesting a gender-specific role for NPFFR2 signalling in the regulation of physical activity during a positive-energy balance that may at least partially contribute to altering energy expenditure in female mice.
We demonstrated that BAT is the critical tissue that acts to reduce energy excess, evidenced by the increased ΔTBAT-Back under HFD conditions compared with chow. Importantly, our study demonstrates that the full development of a BAT thermogenic response under caloric excess requires NPFFR2 signalling, as a lack of it results in an impaired BAT response accompanied with reduced UCP-1 and PGC-1α expression. In addition to diet-induced thermogenesis, BAT is critical for heat production during cold exposure49. Interestingly, our results show that NPFFR2 signalling is not involved in this aspect of BAT function, as mice that lack NPFFR2 signalling maintain a normal BAT thermogenic response to cold exposure. In contrast, NPFFR2 signalling maintains its influence on diet-induced thermogenesis while under altered thermal conditions. This suggests that diet or caloric excess and coldness may induce BAT thermogenesis via different pathways, with NPFFR2 signalling influencing the former but not the later.
Energy homoeostasis regulatory pathways to BAT have been identified to relay from the Arc via the PVN directly projecting to the intermediolateral cell column of the spinal cord50,51, with another one relaying from the PVN to the locus coeruleus and brain stem to control BAT function38. In particular, the later one is a key factor where Arc NPY neurons exert an inhibitory tone on PVN TH neurons subsequently reducing sympathetic outflow to BAT38. Considering that NPFFR2 expression is minimal in the PVN but abundant at the Arc25,32, Arc NPY is likely the key loci in the Arc NPY-PVN-TH pathway for NPFFR2’s action. Importantly, NPFFR2 signalling has a crucial influence on Arc NPY expression as a lack of NPFFR2 signalling results in a strong downregulation of Arc Npy mRNA rendering this regulatory pathway unresponsive to HFD. As such, this suggests that NPFFR2 signalling is necessary for maintaining levels of NPY required for a balanced energy homoeostatic state and that it also allows for the initiation of an adaptive response when energy balance is challenged such as by caloric excess.
Our results and those from others41,42 demonstrate the colocalization of NPFFR2 receptors on NPY neurons, suggesting a direct action of NPFFR2 signalling on NPY levels. The effects of NPFF and related peptides on neurons have been demonstrated in electrophysiology studies using various neuronal preparations such as isolated spinal cord tissue52, dorsal raphe nucleus neurons53,54 and hypothalamic slice preparations55. As NPFFR2 is predominantly coupled to Gi proteins as demonstrated by studies using electrophysiological and in vitro assay approaches56,57, using pCREB as a marker for forskolin-induced cAMP activation, we demonstrated that NPFF co-administered with forskolin significantly reduced forskolin-activated NPY neuronal number in the Arc, providing the first evidence for a direct action of NPFFR2 signalling on hypothalamic NPY neurons. However, Npffr2 single-labelled Arc neurons were also identified by our RNAscope experiments and the co-administration of NPFF with forskolin reduced forskolin-activated Arc NPY neuronal number by approximately 20%. These results leave room for an additional indirect mechanism whereby NPFFR2 signalling controls Arc NPY neurons. Interestingly, Kisspeptin, which has been suggested to act on NPFF receptors33, was shown to exert an indirect action on Arc NPY neurons that is primarily dependent on GABAergic input to NPY cells20. In line with an action of NPFF system through GABAergic transmission, NPFF has been shown to have a dis-inhibitory role via an attenuation of GABAergic inhibitory input to the parvocellular neurons of the PVN in the hypothalamic slice preparation55. Furthermore, an indirect action of NPFFR2 signalling on Arc NPY neuronal activity via GABAergic input is also in line with single-cell transcriptome data showing abundant Npffr2 expression in hypothalamic GABA-expressing non-NPY cells42. Thus, it is conceivable that NPFFR2 signalling has dual actions, i.e., direct and indirect, on Arc NPY neurons to regulate diet-induced thermogenesis and BAT function.
Analysis of our conditional KO mouse model with NPFFR2 specifically deleted in NPY neurons demonstrates that specific functions of NPFFR2 signalling depend on a direct action of NPFFR2 signalling on NPY neurons. Specifically, lack of NPFFR2 in NPY neurons shows a transient impairment in diet-induced thermogenesis and BAT thermogenic activity, suggesting that the direct action of NPFFR2 signalling on NPY neurons is especially important in the initiation of diet-induced thermogenesis, but may contribute less to the maintenance of these effects during prolonged energy excess. In addition, our conditional NPFFR2 KO model revealed an important role for direct NPFFR2 signalling on NPY neurons in the control of oxidative fuel selection under obesogenic conditions, which may be counter-acted by indirect actions of NPFFR2 signalling on NPY neurons, as these effects were not observed in our germline NPFFR2 KO mice. Moreover, the unaltered food intake observed in conditional NPFFR2 KO mice—in contrast to the reduced food intake in germline NPFFR2 KO—suggests that NPFFR2 signalling does not regulate feeding through direct activity on NPY neurons. Finally, results from the conditional NPFFR2 KO mice demonstrate a critical role for direct NPFFR2 signalling on NPY neurons in the control of bone homoeostasis making this an important control centre for determining energy partitioning.
NPFFR2 receptors can be activated by several ligands and we show here that they have distinct distribution patterns and that their mRNA expression levels are differentially regulated by energy status. The strong NPFFR2 expression in the Arc shown in our study is in line with anatomical and biological evidence that suggests direct actions of various RFamide peptides towards NPFFR2 in the Arc. Thus, NPVF fibres from the DMH have been shown to have direct projections to Arc32. Kiss1 mRNA and kisspeptin fibres are present in the Arc and can activate Arc neurons via NPFFR2 signalling20,33. Moreover, the main NPFFR2 endogenous ligand, NPFF, has been suggested to act on NPFFR2 in a hormone-like fashion due to its existence in the cerebrospinal fluid and plasma, and thus has easy access to the Arc34,35. Our study extends these previous reports demonstrating a direct neuronal input from the brain stem neurons to the Arc by showing specific labelling of neurons and fibres in the AP, SubP and NTS upon the delivery of retro beads into the Arc, in support of a possible direct action of NPFF at Arc NPFFR2.
Our results showing that Npff expression in the SubP area is upregulated in Lep-/- mice are consistent with the observed downregulation of NPFF in HFD-fed animals where leptin levels are increased. Although this suggests a role for leptin in the regulation of Npff expression in the SubP area, this action is likely to be indirect since little colocalization between Lepr and Npff was identified. These data also suggest that in addition to the well-known direct action of leptin on Arc NPY neurons, leptin may impact on brain stem NPFF and, in turn, Arc NPFFR2 signalling to regulate Arc NPY neurons that control energy homoeostasis. Possibilities also exist for other factors to control NPFF levels and subsequent NPFFR2 signalling. This is supported by our finding that impaired leptin signalling may not contribute to the exacerbated diet-induced obesity and impaired diet-induced BAT thermogenesis in Npffr2−/− mice, as HFD did not impair pSTAT3 activation in response to exogenous leptin in these mice.
The location of NPY neurons in the Arc of the hypothalamus, which has been shown to be accessible to circulating factors due to a semi-permeable blood–brain barrier, makes them the ideal coordination centre for receiving signals that communicate energy levels, as seen with factors such as leptin, ghrelin and satiety hormones such as GLP-1 or PYY. However, results from this study showing that NPFFR2 signalling also controls these NPY neurons highlights that additional central neuronal pathways are also important in the control of energy homoeostasis, particularly those that influence energy expenditure and energy partitioning by promoting increased thermogenesis and formation of bone. This seems to be especially critical in the situation of negative energy balance where the levels of peripheral signals are generally low and no longer able to influence NPY levels. The consequence of such a rise in NPY being a strong reduction in both thermogenesis and bone formation, while fat accumulation is promoted. The greater bone mass observed in Npffr2−/− mice is consistent with the low Arc Npy mRNA level, which reflects a positive-energy balance and has been shown to enhance osteoblast activity and bone mass39. These results therefore suggest that NPFFR2 signalling controls neuronal NPY populations that influence both the control of thermogenesis as well as bone homoeostasis, two processes that are highly energy consuming. Thus, it may be postulated that NPFFR2 signalling channels excess energy between thermogenesis and bone formation with a lack of the NPFFR2 signalling shifting the balance towards bone anabolism with reduced effects on thermogenesis. As such, NPFFR2 signalling in NPY neurons seems to be critical to switch between these anabolic and catabolic stages by controlling the level of NPY expression and thereby influencing the development of an obese phenotype. As such, targeting this pathway could be a novel and powerful way to control thermogenesis and energy partitioning, thereby providing a potential new treatment option for obesity.
Methods
Animals
All research and animal care procedures were approved by the Garvan Institute/St. Vincent’s Hospital Animal Ethics Committee and the University of New South Wales Animal Care and Ethics Committee in accordance with the Australian Code of Practice for the Care and Use of Animals for Scientific Purpose. Mice were housed under conditions of controlled temperature (22 °C for standard laboratory temperature; 28 °C for thermoneutrality) and illumination (12 h light cycle, lights on at 07:00 h). Mice had free access to water and were fed either a normal chow diet (8% calories from fat, 21% calories from protein, 71% calories from carbohydrate, 2.6 kcal/g; Gordon’s Speciality Stock Feeds, Yanderra, NSW, Australia) or a HFD (23% calories from fat, 19.4% calories from protein, 4.7% calories from crude fibre, 4.7% calories from acid detergent fibre and 20 MJ/kg; Specialty Feeds, Glen Forrest, WA, Australia).
The generation of Npffr2−/− mice is detailed in Supplementary Fig. 1. Briefly, a 129/SvJ mouse genomic BAC library (Genome Systems, St Louis, USA) was screened using a mouse Npffr2 cDNA probe. Positively hybridizing clones were isolated and mapped. Three BamHI fragments covering Exon 2 and 3, as well as surrounding areas, were subcloned and used to generate the targeting construct. A cassette containing the neomycin resistance gene (Neo) flanked on one side by a 34 bp-long Cre-recombinase recognition (loxP) site was placed downstream of exon 2 of the Npffr2 gene. A second loxP sequence was inserted upstream of exon 2 by cloning two complementary 46 mer oligonucleotides into unique NheI site 2.5 kb upstream of Exon 2. Exon 2 contains the translational start of the Npffr2 gene, which when deleted by Cre-recombinase action results in a non-functional Npffr2 gene. The linearized targeting vector was transfected into ES cell line Bruce4 (C57BL/6-Thy1.1 background, Ozgene) and positive clones screened by Southern blotting. Two positive clones were injected into C57BL/6 blastocysts and chimeric mice were bred with C57BL/6 mice to generate heterozygous and subsequently homozygous NPFFR2 conditional mice. Crossing of the homozygous NPFFR2 conditional mice with an oocyte-specific Cre-transgenic line was used to generate the germline deleted NPFFR2 KO mice.
To generate an inducible and conditional NPFFR2 KO mouse model where NPFFR2 is specifically deleted from NPY neurons upon tamoxifen induction, Npffr2lox/lox mice were crossed with NpyCreERT2/+ mice38 on a C57BL/6 background to generate NpyCreERT2/+;Npffr2lox/+ mice and a breeding colony was maintained by mating NpyCreERT2/+;Npffr2lox/+and Npffr2lox/lox mice. Genotyping was performed by PCR using genomic DNA isolated from tail tips. Induction of NPFFR2 deletion from NPY neurons was induced by feeding the NpyCreERT2/+;Npffr2lox/+ mice with tamoxifen diet (500 mg tamoxifen/kg chow, Specialty Feeds, Glen Forrest, WA, Australia) (referred as ‘conditional KO’ herein) at 6 weeks of age for 3 weeks after which mice were put back on normal diet for 2 weeks before phenotyping. NpyCreERT2/+;Npffr2lox/lox mice not receiving tamoxifen diet and NpyCreERT2/+;Npffr2lox/+ receiving tamoxifen were used as controls. Male mice were used for this study due to possible profound impacts of tamoxifen—a selective oestrogen-receptor modulator—on female mice.
For the ribosome translation affinity purification approach (TRAP), ROSA26CAGGFP-L10a mice were sourced from Jax laboratory (B6;129S4-Gt(ROSA)26Sortm9(EGFP/Rpl10a)Amc/J) and crossed onto our NPYcre line obtained from Jax laboratory (Tg(Npy-cre)RH26Gsat)40,58.
Mice monitoring and tissue analyses
Body weight of mice was monitored weekly. WT and Npffr2−/− mice of both genders at 12 weeks of age were examined for whole-body fat and lean masses using DEXA (Lunar PIXImus2 mouse densitometer; GE Healthcare, Waukesha, WI, USA) under light isoflurane anaesthesia. The head and the tail were excluded from DEXA analyses. Spontaneous daily food intake was examined at 15 weeks of age where mice were transferred from group housing on soft bedding to individual cages with paper towel bedding and allowed to acclimatize for two nights. Basal daily food intake was determined as the average of duplicate readings taken over 2 consecutive days. At 18 weeks of age, animals were investigated for energy metabolism using indirect calorimetry as described below. Mice were culled when 20 weeks old between 1200 and 1500 h by cervical dislocation followed by decapitation. White adipose tissue depots (inguinal, epididymal, mesenteric and retroperitoneal) were removed and weighed as published previously59. Brain and BAT were removed and frozen for further analysis by quantitative real-time PCR and western blotting, respectively, as described below. Femora were excised, fixed overnight in 4% paraformaldehyde (PFA) in phosphate-buffered saline (PBS) at 4 °C and then stored in 70% ethanol at 4 °C before undergoing processing as detailed below.
Conditional KO mice and control mice were monitored for weekly body weight and examined for spontaneous food intake, energy metabolism by indirect calorimetry with subsequent body composition by body composition by DEXA and adiposity by tissue dissection at 14, 15 and 16 weeks of age, respectively, following procedures described above or detailed below. Femora was collected at the tissue collection and processed as described above.
High-fat feeding study
A separate set of Npffr2−/− and WT mice at 8 weeks of age were fed with a HFD (23% calories from fat, 19.4% calories from protein, 4.7% calories from crude fibre, 4.7% calories from acid detergent fibre and 20 MJ/Kg; Specialty Feeds, Glen Forrest, WA, Australia) for 8 weeks. Body weight was monitored throughout the HFD feeding period. After 6 weeks on HFD, mice were examined for body composition by DEXA scan as described above. After 7 weeks on HFD, metabolic rate, RER ratio and physical activity were examined as described below with concomitant measurement of food intake. Tissue analysis was performed at the end of 8 weeks of HFD feeding as described above.
A subset of conditional KO and control mice at 12.5 weeks of age were fed with a HFD for 5 weeks, with weekly body weight being monitored. Spontaneous food intake, energy metabolism by indirect calorimetry with subsequent body composition analysis by DEXA and adiposity by tissue dissection was performed at 3, 4 and 5 weeks after the commencement of HFD feeding, respectively.
Indirect calorimetry and measurement of physical activity
Metabolic rate was measured by indirect calorimetry using an eight chamber open-circuit calorimeter (Oxymax Series; Columbus Instruments, Columbus, OH, USA) as described previously59. Briefly, mice were housed individually in specially built Plexiglas cages (20.1 × 10.1 × 12.7 cm). Temperature was maintained at 22 °C with airflow of 0.6 l/min. Mice were singly housed for at least 3 days before their transfer into plexiglass cages and were acclimatized to the cages for 24 h before recordings commenced. Mice were subsequently monitored in the system for 24 h. Oxygen consumption (VO2) and carbon dioxide production (VCO2) were measured every 27 min. The RER ratio was calculated as the quotient of VCO2/VO2, with 100% carbohydrate oxidation giving a value of 1 and 100% fat oxidation giving value of 0.760,61. Energy expenditure (kcal heat produced) was calculated as calorific value (CV) × VO2, where CV is 3.815 + 1.232 × RER62. Energy expenditure was normalized to MAT mass (lean body mass + (0.2) × fat mass)26. Data for the 24 h monitoring period was averaged for 1 h intervals for energy expenditure and RER. Ambulatory activity of individually housed mice was evaluated within the metabolic chambers using an OPTO-M3 sensor system (Columbus Instruments, Columbus, OH, USA), whereby ambulatory counts were a record of consecutive adjacent photobeam breaks. Cumulative ambulatory counts of X and Y directions were recorded every minute and summed for 1 h intervals.
Determination of body and BAT temperature
A subset of male and female WT and Npffr2−/− mice were studied for body and BAT temperatures by a non-invasive high-sensitivity infrared imaging63,64. Mice were group-housed throughout the study with two to three mice per cage, unless indicated otherwise, and fed on either chow or a HFD. Two days before infrared imaging, mice were shaved at interscapular and lumbar back regions under light isoflurane anaesthesia to expose the skin of these areas for temperature reading. Infrared imaging experiments were carried out on the following 2 consecutive days and readings from the two measurements were averaged. Briefly, a high-sensitivity infrared camera (ThermoCAM T640, FLIR, Danderyd, Sweden, sensitivity = 0.04 °C) fixed on a tripod was placed 90 cm above the freely moving mice to record the surface temperatures of the mice in a 30–60 s video. Thermo frames that had mouse body naturally extended with both shaved skin regions vertical to camera lenses were extracted from the video. The hottest pixels of the lumbar back and interscapular regions from each extracted frames were obtained simultaneously and used as indicators of body and BAT temperature, respectively.
Leptin injection and pSTAT3 immunohistochemistry studies
WT and Npffr2−/− mice at 15 weeks of age were examined for pSTAT3 activation in response to leptin. Leptin (Peprotech #450-31) was administered either via i.p. (2 µg/g body weight) or i.c.v. (1.25 µg, 1 µL) injections with saline-injected mice as control. The i.c.v. injection followed the procedures described previously65. Thirty minutes later, under ketamine/xylazine anaesthesia, mice were subjected to cardiac perfusion with saline and 4% formaldehyde in PBS. Brains were removed, post-fixed at 4 °C overnight in 4% formaldehyde in PBS and dehydrated in 30% glucose at 4 °C till sink. Subsequently, brains were stored at − 80 °C until they were sectioned coronally on a cryostat at 40 µm thickness. Free-floating sections were pretreated with citric buffer (pH 6.0) at 80 °C for 30 min, 3% H2O2 in 50% ethanol for 15 min and blocked in 5% normal goat serum in PBS/0.2% Triton X for 60 min at RT. Anti-pSTAT3 antibody (Cell Signalling #9145, 1:500) was added in antibody diluent containing 2.5% normal goat serum and 0.1% bovine serum albumin (BSA) in PBS/0.2% Triton X and incubated overnight at RT with gentle rocking. Sections were washed, incubated with goat anti-rabbit IgG-biotin secondary antibody (1:250, Sigma #B8895) in antibody diluent for 1 h. Sections was subsequently incubated with ExtrAVidin-Peroxidase (1:250, Sigma #E2886) in antibody diluent for 1 h and the signal was developed by liquid DAB substrate (Dako #K3468). Sections were mounted on Superfrost® slides (Menzel-Glaser, Braunschweig, Germany), coverslipped and photographed with a DM 6000 Power Mosaic microscope (Leica, Germany). To quantify cell numbers, in each mouse (n = 3–4), three to four sections between Bregma level − 1.58 mm and − 1.94 mm were chosen. All pSTAT3 immuno-positive cells with a clear profile at Arc were counted and then averaged for each mouse as the number per section.
A separate cohort of WT and Npffr2−/− mice were fed a HFD for 6 weeks and subsequently received i.p. injection of leptin (2 µg/g body weight) or saline (10 µL/g body weight). After 30 min, mice were killed for the immunohistochemical examination of pSTAT3 expression following the protocol described above.
Western blotting
Western blotting was performed on BAT samples following procedures described previously59, in order to determine the protein levels of UCP-1 and PGC-1α. Briefly, BAT samples were resuspended in radioimmunoprecipitation assay buffer (PBS, pH 7.5; 1% nonident NP-40; 0.5% sodium deoxy-cholate; and 0.1% SDS), supplemented with protease and phosphatase inhibitors (10 µg/ml phenylmethylsulfonyl fluoride, 10 µg/ml aprotinin, 10 µg/ml leupeptin, 1 mmol/l Na3VO4 and 10 mmol/l NaF) and solubilized for 2 h at 4 °C. Equal amounts of tissue lysate (20 µg protein) were resolved by SDS-polyacrylamide gel electrophoresis and immunoblotted with appropriate antibodies against PGC-1α (Millipore AB3242, 1:1000), UCP-1 (Alpha Diagnostics International, UCP11-A, 1:1000) and GAPDH (Cell Signalling #3683, 1:1000). Immunolabeled bands were imaged using Fusion Fx7 imaging system (Vilber Lourmat, France) and quantitated by densitometry using Fiji: an open-source platform for biological-image analysis. Image of the molecular size marker was overlayed with the image of immunolabeled bands of the same blot to identify specific bands on the blot. The uncropped gel image of the representative bands and the same uncropped gel image overlayed with molecular size marker are shown in Supplementary Figure 9. Protein levels of PGC-1α or UCP-1 were normalized to GAPDH and analysed for per mg protein and per BAT depot as described previously66, and presented as percentage of that of control group.
RNA extraction and quantitative real-time PCR
We measured the mRNA expression levels of Npvf and Prlh in the brain hypothalamic region, and Npff in the brain stem region following procedures described previously59. Thus, total RNA from the brain hypothalamic region and brain stem region was extracted using TRIzol® reagent (Sigma, St Louis, MO, USA) following the manufacturer’s protocol. The quality and concentration of RNA was determined by measuring the absorbance at 260 and 280 nm using a spectrophotometer (NanoDrop 1000, NanoDrop Technologies, LLC, USA). Two micrograms of total RNA was taken for DNase treatment (RQ1 RNase-Free DNase, Promega, Madison, WI USA) to remove genomic DNA contamination. Subsequently, cDNA was synthesized with oligo(dT)20 and random hexamers using Superscript III First-strand Synthesis System for reverse transcription-PCR (Invitrogen, Mount Waverley, VIC, Australia). Quantitative real-time PCR was then carried out on an ABI Prism 7900 HT instrument (Applied Biosystems Inc, Foster City, CA USA) using the TaqMan Universal PCR master mix (Applied Biosystems Inc., Foster City, CA USA) following the manufacturer’s instructions. Probes and primers for the target gene, the Npvf (Mm00452052_m1), Npff (Mm00450676_g1), Prlh (Mm01286067_m1) and the reference gene, Actb (Mm00607939_s1), were selected from TaqMan gene expression assay reagents (Applied Biosystems, Inc., Foster City, CA USA). Fluorescent signals generated during PCR amplifications were monitored and analysed with ABI Prism 7900 HT SDS software (Applied Biosystems, Inc., Foster City, CA USA). In order to determine the efficiency of each TaqMan gene expression assay, standard curves were generated by serial dilution of cDNA and quantitative evaluations of target and reference gene levels were obtained by measuring threshold cycle numbers (Ct). The relative expression of target mRNA was computed from the target gene Ct values and the reference gene Actb Ct value using the standard curve method (Sequence Detection Systems Chemistry Guide, Applied Biosystems, Inc). For measuring the expression level of Npffr2 and Kiss1r, LightCycle (LightCycler 480 Real-Time PCR system; Roche Applied Science, Mannhelm, Germany) was used. The primers 5′- AAGCAGCATGTGCAAGATCA-3′ and 5′- TGACAGTGAGCTTTGGCTTA-3′ were used for Npffr2, 5′- TGCTGGCTCTATATCTGCTG-3′ and 5′-CTTGAAGCACCAGGAACAGC-3′ were used for Kiss1r. The PCR condition used in measuring these genes were as following67: 94 °C for 30 s, 62 °C for 30 s, 72 °C for 20 s for 40 cycles. Expression of the gene was normalized to the expression of housekeeping gene Actb.
In situ hybridization
Coronal brain sections (25 µm) were cut on a cryostat and thaw-mounted on Superfrost® slides (Menzel-Glaser, Braunschweig, Germany). Matching sections from the same coronal brain level were assayed together using DNA oligonucleotides complementary to mouse Npy (5′-GAGGGTCAGTCCACACAGCCCCATTCGCTTGTTACCTAGCAT-3′), mouse pro-opiomelanocortin (Pomc) (5′-TGGCTGCTCTCCAGGCACCAGCTCCACACATCTATGGAGG-3′), mouse thyrotroppin-releasing hormone (Trh) (5′-AACCTTACTCCTCCAGAGGTTCCCT GACCCAGGCTTCCAGTTGTG-3′), mouse TH (Th) (5′-CTCTAAGGAGCGCCGGATGGTGTGAGGACTGTCCAGTACATCA-3′, mouse Npff (5′-GAGACTGAGGAAGGCACAGGCAAGCAAGGAGCCATGAACCACAGG-3′) and mouse Prlh (5′-GCTGTGAGAGAACTTGGCACTTCCATCCAGTGGGAAGCAGCTTAG-3′). Oligonucleotides were labelled with [α-35S] thio-dATP (PerkinElmer, Boston, MA, USA) using terminal deoxynucleotidyltransferase (Roche, Mannheim, Germany) following manufacturer’s instructions and purified through a G25 column. Fresh brain sections were fixed in 4% PFA, rinsed twice in PBS, pretreated with acetic anhydride (0.25% vol/vol), rinsed twice in PBS, delipidated in chloroform, dehydrated in ethanols, air dried and hybridized with radiolabelled probe (2.5–5.0 × 105 c.p.m. per section) overnight in a 42 °C humidified chamber. The slides were then washed in three times in 5xSSC with 0.5 mM DTT (1,4-Dithiothreitol, VWR International #APLA29480005), twice in 2 × SSC/formamide (50% vol/vol) with 50 mM DTT at 43 °C, cooled to RT, rinsed in 1 × SSC, dH2O and 70% ethanol, and air dried. Subsequently, hybridization signals on sections were visualized by exposure to BioMax MR film (Kodak, Rochester, NY, USA) and digitalized images from the scanned autoradiograms were acquired. For structural details, the brain sections were photoemulsion-dipped and superficially counterstained with haemotoxylin, with which regions of interest were visualized and captured into digital images acquired by bright-field microscope (DM 6000 Power Mosaic microscope, Leica, Germany). Quantification of the mRNA expression levels of respective genes were performed by densitometry for brain areas of interest outlined with consistent defined dimensions across corresponding sections on the photomicrographs using Fiji software for Mac OS.
We used RNAscope duplex chromogenic assay (Advanced Cell Diagnostics, Inc.)—a novel ISH technique to visualize multiple cellular mRNA targets in fresh frozen tissues68—to detect colocalisation of Npffr2 and Npy in the Arc, Npffr2 and Pomc in the Arc, Lepr and Npff in the brain stem. Coronal brain sections (25 µm) were cut on a cryostat and thaw-mounted on Superfrost® slides (Menzel-Glaser, Braunschweig, Germany), and dual labelled for the mRNA of Npy (ACD #313321-C2) and Npffr2 (ACD #410171), Pomc (ACD #314081-C2) and Npffr2, or Lepr (ACD #402731) and Npff (ACD #300031-C2), using RNAscope® 2.5 Duplex Detection Kit following manufacturer’s protocol (Advanced Cell Diagnostics, Inc.). Section staining was photographed using a DM 6000 Power Mosaic microscope (Leica, Germany).
pCREB immunohistochemistry and colocalization with NPY neurons
To investigate the signalling response of NPY neurons to NPFFR2 activation, we examined the effect of NPFFR2 signalling activation by NPFF on forksolin-induced phosphorylation of the CREB—a downstream responder to forskoline-induced increases in cAMP level—in NPY-GFP mice46,47. NPY-GFP mice at 15 weeks of age received i.c.v. injection of one of the following four solutions at 1 µL: Saline, forskolin (Sigma #F6886, 2.5 mM), NPFF (150 nM) or forskolin (2.5 mM) + NPFF (150 nM), under ketamine/xylazine anaesthesia. NPFF was kindly provided by Professor Annette G Beck-Sickinger (University Leipzig, Germany). Procedures for i.c.v. injection were as described previously65. Thirty minutes after the injection, mice were killed by cardiac perfusion with saline and 4% formaldehyde in PBS. Brains were removed, post-fixed at 4 °C overnight in 4% formaldehyde in PBS and dehydrated in 30% glucose at 4 °C till sink. Subsequently, brains were stored at − 80 °C till sectioned coronally on a cryostat at 40 µm thickness. Free-floating sections were blocked in 5% normal goat serum in PBS/0.2% Triton X for 60 min at RT and incubated with anti-pCREB antibody (Cell Signalling #9198, 1:800) in antibody diluent containing 2.5% normal goat serum and 0.1% BSA in PBS/0.2% Triton X overnight at RT with gentle rocking. Sections were washed, incubated with donkey-anti-rabbit Cy3 antibody (1:500, Jackson ImmunoResearch Laboratories, Inc. #711-165-152) in antibody diluent for 2 h. Sections then were washed, mounted on Superfrost® slides (Menzel-Glaser, Braunschweig, Germany), coverslipped and photographed using fluorescent microscope (Leica DM 5500, Germany) equipped with a colour camera (DFC310 Fx). For quantification, two to three sections between Bregma level − 1.70 mm and − 1.94 mm from each mouse (n = 5 and 4 for forskolin and forskolin + NPFF group, respectively) were chosen. GFP-labelled NPY neurons, Cy3-labelled pCREB-ir-positive neurons and NPY/pCREB colocalizing neurons in the arcuate nucleus were counted using Fiji software for macOS. The two sides of the arcuate nucleus were counted separately and counts per side of the arcuate nucleus from the same brain were averaged and presented.
Retrograde neuronal tracing
WT mice were stereotaxically injected into one side of Arc with 0.5 μl of red retrograde beads (Lumaflour, Inc.). Fourteen days after injection, mice were killed by cardiac perfusion with saline and 4% formaldehyde in PBS. Brains were removed, post-fixed at 4 °C overnight in 4% formaldehyde in PBS and dehydrated in 30% glucose at 4 °C till sink. Subsequently, brains were stored at − 80 °C till sectioned coronally on a cryostat at 40 µm thickness. Free-floating sections were collected and mounted on Superfrost® slides (Menzel-Glaser, Braunschweig, Germany), coverslipped and examined using a Leica DM 5500 fluorescent microscope. Tracer labelling was viewed under fluorescent filter set with 540–552 nm, 565 nm and 580–620 nm for excitation, beamsplitter and emission, respectively. Tracer signal was also examined for possible crossover to other channel. For this we used a green channel filter set with 460–500 nm, 505 nm and 512–542 nm for excitation, beamsplitter and emission, respectively. Sections were photographed using a colour camera (DFC310 Fx) equipped to the microscope.
TRAP reverse-transcriptase qPCR
TRAP experiment was performed based on the previously published protocol with some modifications40,69. Thus, the Arc was dissected out by careful manual dissection under the inverted microscope using the forth ventricle as the reference in chilled dissection buffer (1 × Hank’s balanced salt solution, 2.5 mM HEPES-KOH [pH 7.4], 35 mM Glucose and 4 mM NaHCO3) supplemented with fresh 100 μg/mL of cycloheximide (CHX; Sigma). The tissue was homogenized with a hand pestle mixer (Argos Technologies) in 500 μL of lysis buffer (20 mM HEPES-KOH [pH 7.4], 5 mM MgCl2, 150 mM KCl, 0.5 mM DTT) supplemented with fresh protease inhibitor (1 tablet/mL; Roche Mini Complete, EDTA-Free), 100 μg/μL CHX and 40 U/mL of RNAsin (Promega), and then incubated at 4 °C for 5 min. Homogenates were centrifuged for 10 min at 2000 × g at 4 °C to remove pellet nuclei and cell debris, and then 50 μL of NP-40 working solution (10% vol/vol; Biochemica) and DHPC (300 mM; Avanti Polar Lipids) were added to the supernatant and mixed gently by inverting the mixture 10 times. After incubation on ice for 5 min, the lysate was centrifuged for 10 min at 13,000 × g. 20% of the lysate was kept as input. Regarding the antibody-beads preparation step, 50 μL protein G Dynal magnetic beads (Invitrogen) were washed three times with 0.15 M KCl buffer (20 mM HEPES KOH [pH 7.4], 5 mM MgCl2, 150 mM KCl, 1% NP-40, 0.5 mM DTT, 100 μg/ml CHX) at RT and then 10 μL of anti-GFP antibodies (2 μg/μL; Invitrogen A11122) were added into the beads and incubated with beads suspended in 0.15 M KCl buffer (275 μL) for 1 h at RT with mild end-to-end rotation. Next, the antibody-bound beads were collected by using the magnetic rack and washed three times with 0.15 M KCl buffer before use. The beads were then mixed with the cell-lysate supernatant and the mixture was incubated at 4 °C with mild end-to-end rotation overnight. Beads were subsequently collected on a magnetic rack, washed three times with 0.35 M KCl buffer (20 mM HEPES KOH [pH 7.4], 5 mM MgCl2, 350 mM KCl, 1% NP-40, 0.5 mM DTT, 100 μg/ml CHX) at 4 °C and immediately placed in 350 μL of RNA lysis buffer (RLT) supplemented with 10% of 2-Mercaptoethanol at RT and incubated for 5 min. Next, the RLT-containing RNA was purified with the RNeasy microKit (Qiagen) following the manufacturer’s protocol. DNase digestion step was included in the purification. RNA quantitation and purity were confirmed by NanoDrop Spectrophotometers. Forty nanograms of RNA was used to synthesis cDNA by using the SuperScript III First-Strand Synthesis System (Thermo Fisher Scientific). RT-qPCR using primers for Npy, GFP and Npffr2 was carried out in samples prior (input) and after the immunoprecipitation in at least triplicates from 1:5 dilution cDNA from each sample using the LightCycler® (LightCycler® 480 Real-Time PCR system, Roche Applied Science, Germany), SYBR Green I (Molecular Probes) and Platinum Taq DNA Polymerase (Invitrogen). Primers 5′-AATCAGTGTCTCAGGGCTG-3′ and 5′-CTATCTCTGCTCGTGTGTTT-3′ were used for assaying Npy, 5′-CGGATCTTGAAGTTCACCTT-3′ and 5′-GAGCGCACCATCTTCTTCA-3′ were used for GFP, 5′-GTACGACCAGAGGCATACA-3′ and 5′-AGCACCCTGTGCTGCTCA-3′ were used for Actb. The primers used for Npffr2 have been described in RNA extraction and quantitative real-time PCR. The PCR condition used in all the TRAP RT-qPCR experiment were as following: 94 °C for 30 s, 62 °C for 30 s, 72 °C for 20 s for 40 cycles67. Expression of the gene was normalized to the expression of housekeeping gene Actb.
Bone μCT
Following fixation, left femora were cleaned of muscle and analysed using μCT with a Skyscan 1172 scanner and associated analysis software (Skyscan, Aartselaar, Blegium), as previously described70. Briefly, analyses of the cortical bone were carried out in 229 slices (1.0 mm) selected 572 slices (2.5 mm) proximally from the distal growth plate resulting in calculations of the following parameters: total tissue area, bone area, marrow area, periosteal perimeter, cortical thickness and polar moment of inertia (an index of strength). Analyses of the trabecular bone were carried out in 229 slices (1.0 mm) and selected 114 slices (0.5 mm) proximally from the distal growth plate resulting in calculations of the following parameters: total tissue volume, bone volume, trabecular number, trabecular thickness and trabecular separation.
Behavioural testing
WT and Npffr2−/− mice at 17 weeks of age were tested in a battery of behavioural tests with an inter-test interval of at least 48 h: elevated plus maze (EPM), open field (OF), prepulse inhibition, motor function tests (i.e., pole test and beam walking test) and hot water tail-flick test71. All tests were conducted during the first 5 h of the light phase to minimize effects of the circadian rhythm on the performance of test mice.
Elevated plus maze: The EPM assesses the natural conflict between the tendency of mice to explore a novel environment and avoidance of a brightly lit, elevated and open area. The grey plus maze was ‘+’ shaped as described previously72. Mice were placed at the centre of the ‘+’ (faced towards an enclosed arm) and were allowed to explore the maze for 5 min. The time spent in and number of entries into the open and enclosed arms were recorded using AnyMazeTM (Stoelting, Wood Dale, USA) tracking software (percentages calculated based on total arm entries/total are time excluding centre time).
Open field: The OF test provides measures of locomotion, exploration and anxiety-like behaviour. This test mimics the natural conflict in mice between the tendency to explore a novel environment and to avoid an exposed open area. Test mice were placed for 30 min into an infrared photobeam-controlled OF activity test chamber (43.2 × 43.2 cm—illumination level: 20 lx; MED Associates, Inc., Vermont, USA), which was divided into a central and a peripheral zone (MED software coordinates for central zone: 3/3, 3/13, 13/3, 13/13; box size: 3; ambulatory trigger: 2; resting delay: 1000 ms; resolution: 100 ms). Measures of locomotion included distance travelled and ambulatory time; vertical activity was taken as a measure of exploration (i.e., rearing).
Hot water tail-flick test: Pain sensitivity (i.e., nociception) was assessed using the hot water tail-flick test. Mice were gently wrapped in a soft tissue towel and the tail tip was placed in a 52 °C warm water bath and the latency to flick the tail was recorded. Each test consisted of three trials (intertrial interval of 3–4 min). In between trials, mice were returned to their home cage.
Statistical analyses
All data are expressed as means ± SEM. Energy expenditure, RER and physical activity over the continuous 24 h period were averaged for the whole 24 h period, as well as for the light and dark periods. Differences between different genotypes were assessed by two-sided analysis of variance (ANOVA) or repeated-measures ANOVA combined with Tukey’s honest significant difference post-hoc analysis where appropriate. Statistical analyses were performed with SPSS for Mac OS X, version 16.0.1 (SPSS, Inc., Chicago, IL, USA). Statistical significance was defined as p < 0.05.
Oligonucleotides
A list of the oligonucleotides used in this study is presented in Supplementary Table 3.
Data availability
The data supporting the findings of this study are available within the article and its Supplementary Information files, and from the corresponding author upon reasonable request.
References
Leibel, R. L., Rosenbaum, M. & Hirsch, J. Changes in energy expenditure resulting from altered body weight. N. Engl. J. Med. 332, 621–628 (1995).
Rosenbaum, M., Hirsch, J., Gallagher, D. A. & Leibel, R. L. Long-term persistence of adaptive thermogenesis in subjects who have maintained a reduced body weight. Am. J. Clin. Nutr. 88, 906–912 (2008).
Bachman, E. S. et al. betaAR signaling required for diet-induced thermogenesis and obesity resistance. Science 297, 843–845 (2002).
Bouchard, C. et al. The response to long-term overfeeding in identical twins. N. Engl. J. Med. 322, 1477–1482 (1990).
Rothwell, N. J. & Stock, M. J. A role for brown adipose tissue in diet-induced thermogenesis. Nature 281, 31–35 (1979).
Levine, J. A., Eberhardt, N. L. & Jensen, M. D. Role of nonexercise activity thermogenesis in resistance to fat gain in humans. Science 283, 212–214 (1999).
Nedergaard, J. & Cannon, B. UCP1 mRNA does not produce heat. Biochim. Biophys. Acta 1831, 943–949 (2013).
von Essen, G., Lindsund, E., Cannon, B. & Nedergaard, J. Adaptive facultative diet-induced thermogenesis in wild-type but not in UCP1-ablated mice. Am. J. Physiol. Endocrinol. Metab. 313, E515–E527 (2017).
Kazak, L. et al. Genetic depletion of adipocyte creatine metabolism inhibits diet-induced thermogenesis and drives obesity. Cell. Metab. 26, 660–671 (2017).
Riediger, T. The receptive function of hypothalamic and brainstem centres to hormonal and nutrient signals affecting energy balance. Proc. Nutr. Soc. 71, 463–477 (2012).
Hoyda, T. D., Smith, P. M. & Ferguson, A. V. Gastrointestinal hormone actions in the central regulation of energy metabolism: potential sensory roles for the circumventricular organs. Int. J. Obes. (Lond.). 33 Suppl 1, S16–S21 (2009).
Bartness, T. J. & Song, C. K. Brain-adipose tissue neural crosstalk. Physiol. Behav. 91, 343–351 (2007).
Findeisen, M., Rathmann, D. & Beck-Sickinger, A. G. RFamide peptides: structure, function, mechanisms and pharmaceutical potential. Pharmaceuticals 4, 1248 (2011).
Bechtold, D. A. & Luckman, S. M. The role of RFamide peptides in feeding. J. Endocrinol. 192, 3–15 (2007).
Nystedt, J. M., Brandt, A., Vilim, F. S., Ziff, E. B. & Panula, P. Identification of transcriptional regulators of neuropeptide FF gene expression. Peptides 27, 1020–1035 (2006).
Vilim, F. S. et al. Gene for pain modulatory neuropeptide NPFF: induction in spinal cord by noxious stimuli. Mol. Pharmacol. 55, 804–811 (1999).
Bechtold, D. A. & Luckman, S. M. Prolactin-releasing peptide mediates cholecystokinin-induced satiety in mice. Endocrinology 147, 4723–4729 (2006).
Murase, T., Arima, H., Kondo, K. & Oiso, Y. Neuropeptide FF reduces food intake in rats. Peptides 17, 353–354 (1996).
Dodd, G. T. et al. The thermogenic effect of leptin is dependent on a distinct population of prolactin-releasing peptide neurons in the dorsomedial hypothalamus. Cell. Metab. 20, 639–649 (2014).
Fu, L. Y. & van den Pol, A. N. Kisspeptin directly excites anorexigenic proopiomelanocortin neurons but inhibits orexigenic neuropeptide Y cells by an indirect synaptic mechanism. J. Neurosci. 30, 10205–10219 (2010).
Tolson, K. P. et al. Impaired kisspeptin signaling decreases metabolism and promotes glucose intolerance and obesity. J. Clin. Invest. 124, 3075–3079 (2014).
Liu, Q. et al. Identification and characterization of novel mammalian neuropeptide FF-like peptides that attenuate morphine-induced antinociception. J. Biol. Chem. 276, 36961–36969 (2001).
Elhabazi, K. et al. Endogenous mammalian RF-amide peptides, including PrRP, kisspeptin and 26RFa, modulate nociception and morphine analgesia via NPFF receptors. Neuropharmacology 75, 164–171 (2013).
Oishi, S. et al. Activation of neuropeptide FF receptors by kisspeptin receptor Ligands. ACS Med. Chem. Lett. 2, 53–57 (2011).
Gouarderes, C., Puget, A. & Zajac, J. M. Detailed distribution of neuropeptide FF receptors (NPFF1 and NPFF2) in the rat, mouse, octodon, rabbit, guinea pig, and marmoset monkey brains: a comparative autoradiographic study. Synapse 51, 249–269 (2004).
Even, P. C. & Nadkarni, N. A. Indirect calorimetry in laboratory mice and rats: principles, practical considerations, interpretation and perspectives. Am. J. Physiol. Regul. Integr. Comp. Physiol. 303, R459–R476 (2012).
Montgomery, M. K. et al. Mouse strain-dependent variation in obesity and glucose homeostasis in response to high-fat feeding. Diabetologia 56, 1129–1139 (2013).
Turner, N. et al. Excess lipid availability increases mitochondrial fatty acid oxidative capacity in muscle: evidence against a role for reduced fatty acid oxidation in lipid-induced insulin resistance in rodents. Diabetes 56, 2085–2092 (2007).
Lin, j, Handschin, C. & Spiegelman, B. M. Metabolic control through the PGC-1 family of transcription coactivators. Cell. Metab. 1, 361–370 (2005).
Speakman, J. R. & Keijer, J. Not so hot: optimal housing temperatures for mice to mimic the thermal environment of humans. Mol. Metab. 2, 5–9 (2012).
Enriori, P. J., Sinnayah, P., Simonds, S. E., Garcia Rudaz, C. & Cowley, M. A. Leptin action in the dorsomedial hypothalamus increases sympathetic tone to brown adipose tissue in spite of systemic leptin resistance. J. Neurosci. 31, 12189–12197 (2011).
Poling, M. C., Quennell, J. H., Anderson, G. M. & Kauffman, A. S. Kisspeptin neurones do not directly signal to RFRP-3 neurones but RFRP-3 may directly modulate a subset of hypothalamic kisspeptin cells in mice. J. Neuroendocrinol. 25, 876–886 (2013).
Liu, X. & Herbison, A. Kisspeptin regulation of arcuate neuron excitability in kisspeptin receptor knockout mice. Endocrinology 156, 1815–1827 (2015).
Burlet-Schiltz, O. et al. Identification of neuropeptide FF-related peptides in human cerebrospinal fluid by mass spectrometry. FEBS Lett. 532, 313–318 (2002).
Sundblom, D. M. et al. Neuropeptide FF-like immunoreactivity in human cerebrospinal fluid of chronic pain patients and healthy controls. Peptides 18, 923–927 (1997).
Schofield, B. R. Retrograde axonal tracing with fluorescent markers. Curr. Protoc. Neurosci. Chapter 1, Unit 1 17 (2008).
Lyubimov, Y. et al. Human kisspeptins activate neuropeptide FF2 receptor. Neuroscience 170, 117–122 (2010).
Shi, Y. C. et al. Arcuate NPY controls sympathetic output and BAT function via a relay of tyrosine hydroxylase neurons in the PVN. Cell. Metab. 17, 236–248 (2013).
Baldock, P. A. et al. Neuropeptide Y knockout mice reveal a central role of NPY in the coordination of bone mass to body weight. PLoS ONE 4, e8415 (2009).
Zhou, P. et al. Interrogating translational efficiency and lineage-specific transcriptomes using ribosome affinity purification. Proc. Natl Acad. Sci. USA 110, 15395–15400 (2013).
Henry, F. E., Sugino, K., Tozer, A., Branco, T. & Sternson, S. M. Cell type-specific transcriptomics of hypothalamic energy-sensing neuron responses to weight-loss. eLife 4, 09800 (2015).
Romanov, R. A. et al. Molecular interrogation of hypothalamic organization reveals distinct dopamine neuronal subtypes. Nat. Neurosci. 20, 176–188 (2017).
Zhang, W. & Bi, S. Hypothalamic regulation of brown adipose tissue thermogenesis and energy homeostasis. Front Endocrinol. (Lausanne) 6, 136 (2015).
Gouarderes, C. et al. Functional differences between NPFF1 and NPFF2 receptor coupling: high intrinsic activities of RFamide-related peptides on stimulation of [35S]GTPgammaS binding. Neuropharmacology 52, 376–386 (2007).
Mollereau, C., Mazarguil, H., Zajac, J. M. & Roumy, M. Neuropeptide FF (NPFF) analogs functionally antagonize opioid activities in NPFF2 receptor-transfected SH-SY5Y neuroblastoma cells. Mol. Pharmacol. 67, 965–975 (2005).
Impey, S. et al. Cross talk between ERK and PKA is required for Ca2 + stimulation of CREB-dependent transcription and ERK nuclear translocation. Neuron 21, 869–883 (1998).
Mayr, B. & Montminy, M. Transcriptional regulation by the phosphorylation-dependent factor CREB. Nat. Rev. Mol. Cell Biol. 2, 599–609 (2001).
Apolzan, J. W. et al. Effects of weight gain induced by controlled overfeeding on physical activity. Am. J. Physiol. Endocrinol. Metab. 307, E1030–E1037 (2014).
Cannon, B. & Nedergaard, J. Brown adipose tissue: function and physiological significance. Physiol. Rev. 84, 277–359 (2004).
Zheng, J. Q., Seki, M., Hayakawa, T., Ito, H. & Zyo, K. Descending projections from the paraventricular hypothalamic nucleus to the spinal cord: anterograde tracing study in the rat. Okajimas Folia Anat. Jpn 72, 119–135 (1995).
Toth, Z. E., Gallatz, K., Fodor, M. & Palkovits, M. Decussations of the descending paraventricular pathways to the brainstem and spinal cord autonomic centers. J. Comp. Neurol. 414, 255–266 (1999).
Huang, E. Y., Bagust, J., Sharma, R. P. & Walker, R. J. The effect of FMRF-amide-like peptides on electrical activity in isolated mammalian spinal cord. Neurosci. Res. 30, 295–301 (1998).
Roumy, M. & Zajac, J. Neuropeptide FF selectively attenuates the effects of nociceptin on acutely dissociated neurons of the rat dorsal raphe nucleus. Brain Res. 845, 208–214 (1999).
Ding, Z. & Zajac, J. M. Neuropeptide FF receptors exhibit direct and anti-opioid effects on mice dorsal raphe nucleus neurons. Eur. J. Pharmacol. 740, 271–276 (2014).
Jhamandas, J. H., Simonin, F., Bourguignon, J. J. & Harris, K. H. Neuropeptide FF and neuropeptide VF inhibit GABAergic neurotransmission in parvocellular neurons of the rat hypothalamic paraventricular nucleus. Am. J. Physiol. Regul. Integr. Comp. Physiol. 292, R1872–R1880 (2007).
Bonini, J. A. et al. Identification and characterization of two G protein-coupled receptors for neuropeptide FF. J. Biol. Chem. 275, 39324–39331 (2000).
Elshourbagy, N. A. et al. Receptor for the pain modulatory neuropeptides FF and AF is an orphan G protein-coupled receptor. J. Biol. Chem. 275, 25965–25971 (2000).
Qi, Y. et al. Snord116 is critical in the regulation of food intake and body weight. Sci. Rep. 6, 18614 (2016).
Zhang, L. et al. Peripheral neuropeptide Y Y1 receptors regulate lipid oxidation and fat accretion. Int. J. Obes. (Lond.). 34, 357–373 (2010).
Ferrannini, E. The theoretical bases of indirect calorimetry: a review. Metabolism 37, 287–301 (1988).
Frayn, K. N. Calculation of substrate oxidation rates in vivo from gaseous exchange. J. Appl. Physiol. 55, 628–634 (1983).
McLean, J. A. & Tobin, G. Animal and Human Calorimetry (Cambridge Univ. Press, 1987).
Marks, A., Vianna, D. M. & Carrive, P. Nonshivering thermogenesis without interscapular brown adipose tissue involvement during conditioned fear in the rat. Am. J. Physiol. Regul. Integr. Comp. Physiol. 296, R1239–R1247 (2009).
Zhang, L. et al. Stress- and diet-induced fat gain is controlled by NPY in catecholaminergic neurons. Mol. Metab. 3, 581–591 (2014).
Loh, K. et al. Insulin controls food intake and energy balance via NPY neurons. Mol. Metab. 6, 574–584 (2017).
Fischer, A. W. et al. Leptin raises defended body temperature without activating thermogenesis. Cell Rep. 14, 1621–1631 (2016).
Ip, C. K., Fossat, N., Jones, V., Lamonerie, T. & Tam, P. P. Head formation: OTX2 regulates Dkk1 and Lhx1 activity in the anterior mesendoderm. Development 141, 3859–3867 (2014).
Wang, F. et al. RNAscope: a novel in situ RNA analysis platform for formalin-fixed, paraffin-embedded tissues. J. Mol. Diagn. 14, 22–29 (2012).
Heiman, M., Kulicke, R., Fenster, R. J., Greengard, P. & Heintz, N. Cell type-specific mRNA purification by translating ribosome affinity purification (TRAP). Nat. Protoc. 9, 1282–1291 (2014).
Lee, N. J. et al. NPY signalling in early osteoblasts controls glucose homeostasis. Mol. Metab. 4, 164–174 (2015).
Karl, T., Pabst, R. & von Horsten, S. Behavioral phenotyping of mice in pharmacological and toxicological research. Exp. Toxicol. Pathol. 55, 69–83 (2003).
Karl, T., Duffy, L. & Herzog, H. Behavioural profile of a new mouse model for NPY deficiency. Eur. J. Neurosci. 28, 173–180 (2008).
Acknowledgements
We thank the staff the staff of the Garvan Institute Biological Testing Facility, staff of the Australian BioResources and Adam Bryan at Neuroscience Research Australia for facilitation of these experiments and taking care of our test mice. We thank Jerry Tanda for critical comments on the manuscript. We thank Irene Kahr for technical assistance in generating the targeting construct for the Npffr2 gene. We thank Ananda Kalutantiri for the information technology support. This research was supported by the National Health and Medical Research Council of Australia (NHMRC) with project grants (#1102012), a Career Development Fellowship (#1045643) to T.K. and a Research Fellowship to H.H. (#1118775). T.K. was also supported by the NHMRC dementia research team initiative (#1095215) and the Rebecca L. Cooper Medical Research Foundation.
Author information
Authors and Affiliations
Contributions
L.Z. and H.H. designed and supervised the project. L.Z., C.K.I., I.J.L., F.R., Y.Q., T.K., J.K.L., N.J.L. and R.F. performed experiments and acquired the data. L.Z., T.K., P.A.B. and H.H. analysed and interpreted the results. L.Z. and H.H. wrote the manuscript.
Corresponding author
Ethics declarations
Competing interests
The authors declare no competing interests.
Additional information
Publisher's note: Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
Electronic supplementary material
Rights and permissions
Open Access This article is licensed under a Creative Commons Attribution 4.0 International License, which permits use, sharing, adaptation, distribution and reproduction in any medium or format, as long as you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons license, and indicate if changes were made. The images or other third party material in this article are included in the article’s Creative Commons license, unless indicated otherwise in a credit line to the material. If material is not included in the article’s Creative Commons license and your intended use is not permitted by statutory regulation or exceeds the permitted use, you will need to obtain permission directly from the copyright holder. To view a copy of this license, visit http://creativecommons.org/licenses/by/4.0/.
About this article
Cite this article
Zhang, L., Ip, C.K., Lee, IC.J. et al. Diet-induced adaptive thermogenesis requires neuropeptide FF receptor-2 signalling. Nat Commun 9, 4722 (2018). https://doi.org/10.1038/s41467-018-06462-0
Received:
Accepted:
Published:
DOI: https://doi.org/10.1038/s41467-018-06462-0
Comments
By submitting a comment you agree to abide by our Terms and Community Guidelines. If you find something abusive or that does not comply with our terms or guidelines please flag it as inappropriate.