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Role of neonatal hyperleptinaemia on serum adiponectin and suppressor of cytokine signalling-3 expression in young rats

Published online by Cambridge University Press:  05 August 2008

Magna Cottini Fonseca Passos ,
Fabiane Pereira Toste ,
Sheila Cristina Potente Dutra ,
Paula Affonso Trotta ,
Fernanda Pereira Toste ,
Patrícia Cristina Lisboa  and
Egberto Gaspar de Moura
Magna Cottini Fonseca Passos*
Affiliation:
Department of Physiological Sciences, Institute of Biology, State University of Rio de Janeiro, Rio de Janeiro20550-030, RJ, Brazil Department of Applied Nutrition, Nutrition Institute, State University of Rio de Janeiro, Av. 28 de Setembro 87, Rio de Janeiro20550-030, RJ, Brazil
Fabiane Pereira Toste
Affiliation:
Department of Physiological Sciences, Institute of Biology, State University of Rio de Janeiro, Rio de Janeiro20550-030, RJ, Brazil
Sheila Cristina Potente Dutra
Affiliation:
Department of Physiological Sciences, Institute of Biology, State University of Rio de Janeiro, Rio de Janeiro20550-030, RJ, Brazil
Paula Affonso Trotta
Affiliation:
Department of Applied Nutrition, Nutrition Institute, State University of Rio de Janeiro, Av. 28 de Setembro 87, Rio de Janeiro20550-030, RJ, Brazil
Fernanda Pereira Toste
Affiliation:
Department of Physiological Sciences, Institute of Biology, State University of Rio de Janeiro, Rio de Janeiro20550-030, RJ, Brazil
Patrícia Cristina Lisboa
Affiliation:
Department of Physiological Sciences, Institute of Biology, State University of Rio de Janeiro, Rio de Janeiro20550-030, RJ, Brazil
Egberto Gaspar de Moura
Affiliation:
Department of Physiological Sciences, Institute of Biology, State University of Rio de Janeiro, Rio de Janeiro20550-030, RJ, Brazil
*
*Corresponding author: Professor Magna Cottini Fonseca Passos, fax +55 21 25876129, email magna.cottini@pq.cnpq.br
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Abstract

Previously we had shown that neonatal leptin treatment programmes for both hyperleptinaemia and hyperinsulinaemia, which lead to leptin resistance and low expression of the hypothalamic leptin receptor (OB-Rb) of rats aged 150 d. Here we investigated in young post-weaned rats (age 30 d) if leptin treatment during lactation induces leptin and insulin resistance and if those changes are accompanied by changes in the suppressor of cytokine signalling-3 (SOCS-3) expression and serum adiponectin concentration. After delivery, the pups were divided into two groups: (1) a leptin group (Lep) that were injected with leptin daily (8 μg/100 g body weight subcutaneously) for the first 10 d of lactation; (2) a control (C) group, receiving saline. After weaning (day 21), body weight was monitored until the animals were age 30 d. They were tested for food intake in response to either leptin (0·5 mg/kg body weight intraperitoneally) (CL, LepL) or saline (CSal, LepSal) when they were aged 30 d. The CL group showed lower food intake, but no response was observed in the LepL group, suggesting leptin resistance. The Lep group had hyperleptinaemia (five-fold), hyperinsulinaemia (+42·5 %) and lower levels of serum adiponectin ( − 43·2 %). The hypothalamic expression of OB-Rb was lower ( − 22 %) and SOCS-3 was higher (+52·8 %) in the Lep group. We conclude that neonatal leptin treatment programmes for leptin resistance as soon as 30 d and suggests that SOCS-3 appears to be of particular importance in this event. In the Lep group, the lower serum adiponectin levels were accompanied by higher serum insulin, indicating a probable insulin resistance.

Keywords

HyperleptinaemiaAdiponectinSuppressor of cytokine signalling-3Leptin resistance
Type
Full Papers
Information
British Journal of Nutrition , Volume 101 , Issue 2 , January 2009 , pp. 250 - 256
Copyright
Copyright © The Authors 2008

Recently, epidemiological and experimental evidence has suggested that intra-uterine undernutrition is closely associated with adulthood obesity related to detrimental metabolic sequelae(Reference Breier, Vickers, Ikenasio, Chan and Wong1Reference Ravelli, Stein and Susser3), giving rise to the concept of ‘developmental origins of health and disease’(Reference Breier, Vickers, Ikenasio, Chan and Wong1, Reference Gluckman and Hanson4).

The mother's undernutrition during lactation can programme the higher body weight of their offspring in the adult life(Reference Passos, Vicente, Lisboa and Moura5) and this can be mainly associated with the neonatal leptin surge. Intra-uterine undernutrition is also closely associated with obesity in adulthood. Yura et al. (Reference Yura, Itoh, Sagawa, Yamamoto, Masuzaki, Kawamura, Takemura, Kakui, Ogawa and Fujii6) report a mouse model in which undernutrition was applied during gestation; after birth the offspring was fed a high-fat diet and developed higher adiposity. In the neonatal period, undernourished offspring exhibited a premature onset of the neonatal leptin surge compared with offspring with normal intra-uterine nutrition. A premature leptin surge generated in control offspring by exogenous leptin administration led to accelerated weight gain with a high-fat diet. Both undernourished offspring and neonatal leptin-treated control offspring exhibited an impaired response to acute peripheral leptin administration with impaired leptin transport to the brain as well as an increased density of hypothalamic nerve terminals. The present study suggests that the premature leptin surge alters energy regulation by the hypothalamus and contributes to ‘developmental origins of health and disease’.

We have shown that leptin treatment in the first 10 d of lactation programmes for higher food intake and body weight, hyperleptinaemia(Reference Oliveira Cravo, Teixeira, Passos, Dutra, Moura and Ramos7), higher thyroid hormone serum concentration(Reference Teixeira, Ramos, Mouco, Passos and Moura8), hypothalamic leptin resistance, lower expression of hypothalamic leptin receptor (OB-Rb)(Reference Toste, Moura, Lisboa, Fagundes, Oliveira and Passos9) and higher medullar catecholamine content and secretion(Reference Trevenzoli, Valle, Machado, Garcia, Passos, Lisboa and Moura10) in adulthood (aged 150 d).

Leptin is a cytokine-like peptide that is produced primarily by adipose tissue and inhibits food intake and increases energy expenditure in rodents(Reference Schwartz, Seeley, Campfield, Burn and Baskin11). Leptin and insulin are key hormones involved in the regulation of energy balance and glucose homeostasis. Specific members of the suppressor of cytokine signalling (SOCS) family of proteins are now thought to have a role in the development of leptin and insulin resistance, owing to their ability to inhibit leptin- and insulin-signalling pathways(Reference Howard and Flier12).

SOCS proteins are induced by a variety of cytokines and act as a negative regulator of cytokine signalling. Among eight SOCS proteins(Reference Nicholson and Hilton13, Reference Krebs and Hilton14), leptin specifically induces SOCS-3 mRNA levels at the hypothalamus(Reference Bjørbaek, El-Haschimi, Frantz and Flier15, Reference Baskin, Hahn and Schwartz16) and activates SOCS-3 expression in neuropeptide Y (NPY) and pro-opiomelanocortin neurons(Reference Baskin, Hahn and Schwartz16). Thus, an increase in SOCS-3 mRNA levels could lead to a leptin resistance, by inhibition of the Janus kinase 2–signal transducer and activator of transcription 3 (JAK2–STAT3) pathway or phosphatidylinositol 3-kinase–phosphodiesterase 3B–cyclic AMP (PI3K–PDE3B–cAMP), an alternative pathway of leptin signalling(Reference Bjørbaek, El-Haschimi, Frantz and Flier15, Reference Bjørbaek, Elmquist, Frantz, Shoelson and Flier17).

Although the SOCS proteins were initially thought to be primarily involved in the attenuation of cytokine signalling through classical negative feedback, there is now a growing appreciation of a role for SOCS proteins in the negative regulation of receptor tyrosine kinase signalling, such as the inhibition of insulin signalling(Reference Pessin and Saltier18).

Adiponectin acts predominantly in muscle and liver affecting fatty acids and glucose metabolism. Adiponectin has been shown to have insulin-sensitising, anti-atherogenic and anti-inflammatory properties(Reference Dyck, Heigenhauser and Bruce19). A low serum concentration of adiponectin(Reference Bacha, Saad, Gungor and Arslanian20, Reference Cote, Mauriege, Bergeron, Almeras, Tremblay, Lemieux and Despree21) is associated with higher insulinaemia and leptinaemia. Insulin and leptin are proposed to function as adiposity signals in the feedback regulation of food intake(Reference Schwartz, Woods, Porte, Seeley and Baskin22). Both hormones circulate in the bloodstream in proportion to body fat mass and regulate the activity of neurons found in regions of the brain associated with body-weight regulation(Reference Schwartz, Seeley, Campfield, Burn and Baskin11, Reference Marks, Porte, Stahl and Baskin23). Development of resistance to the action of these hormones appears to have an important role in the pathogenesis of obesity and type 2 diabetes.

Here, we demonstrate whether neonatal hyperleptinaemia changes serum adiponectin levels and expression of SOCS-3 protein in rats aged 30 d and if these factors could be associated with the development of leptin and insulin resistance.

Methods

Animals and treatment

Animal experimental protocols were approved by the Animal Care and Use Committee of the Biology Institute of the State University of Rio de Janeiro, which based their analysis on the principles described in the Guide for the Care and Use of Laboratory Animals(Reference Bayne24). Wistar rats were kept in a room with controlled temperature (25 ± 1°C) and with artificial dark–light cycles (lights on from 07.00 to 19.00 hours).

Pups were divided, within 24 h of birth, into two groups: daily subcutaneously injected with 8 μg/100 g body weight(Reference Oliveira Cravo, Teixeira, Passos, Dutra, Moura and Ramos7, Reference Toste, Moura, Lisboa, Fagundes, Oliveira and Passos9, Reference Malendowicz, Macchi, Nussdorfer and Nowak25) of recombinant mouse leptin (PeproTech Inc., London, UK) (Lep group) for the first 10 d of lactation and the control group (C group) that received instead the same volume of saline (NaCl; 0·9 %). Leptin was dissolved in saline and all the injections were made at 16.00 hours.

Within 24 h of birth, excess pups were removed, so that only six male pups were kept per dam (six dams), because it has been shown that this procedure maximises lactation performance(Reference Fishbeck and Rasmussen26).

At 2 h after leptin injection, two pups of each litter (Lep and C; six rats) were randomly chosen and blood samples were obtained by decapitation and trunk blood was collected for determination of serum leptin.

The pups were weaned at age 21 d. After weaning, two animals of each litter (six litters of each experimental group) were randomly chosen and placed together in the cage with free access to water and food until they were aged 30 d, when they were killed (twelve animals per group) with a lethal dose of pentobarbital (0·15 ml/100 g bodyweight, intraperitoneally) and blood was obtained by cardiac puncture.

Body composition analysis

Body composition (fat and protein mass) was determined at 30 d by carcass analysis as reported previously(Reference Toste, Moura, Lisboa, Fagundes, Oliveira and Passos9, Reference Fagundes, Moura, Passos, Oliveira, Toste, Bonomo, Trevenzoli, Garcia and Lisboa27). After killing, the animals were eviscerated, the carcasses were weighed, autoclaved for 1 h and homogenised in distilled water (1:1). Samples of the homogenate were stored at 4°C before analysis. Then 3 g of the homogenate were used for determining fat mass gravimetrically. The samples were hydrolysed in a shaking water-bath at 70°C for 2 h with 30 % KOH and ethanol. The total fatty acids and non-esterified cholesterol were removed with three successive washings with petroleum ether. After drying overnight in a vacuum all tubes were weighed and the results were expressed as g fat/100 g carcass. Protein mass was determined in 1 g of homogenate. The tubes were centrifuged at 2000 g for 10 min. The total protein concentrations were determined by the method of Lowry et al. (Reference Lowry, Rosebrough, Farr and Randall28). The results are expressed as g protein/100 g carcass.

Adiponectin, insulin and leptin serum quantification

All assays were performed using RIA kits (Linco Research, Inc., St Charles, MO, USA). The adiponectin kit had a lower detection limit of 0·78 ng/ml and the inter-assay and intra-assay CV were 7·31 and 4·09 %, respectively. The insulin kit had an assay sensitivity of 0·1 ng/ml and a range of detection from 0·1 to 10 ng/ml. The inter-assay and intra-assay CV were 4·2 and 8·47 %, respectively. The leptin kit measures both rat and mouse leptin with an assay sensitivity of 0·5 ng/ml and a range of detection from 0·5 to 50 ng/ml. The inter-assay and intra-assay CV were 6·9 and 7·3 %, respectively.

Glucose measurement

Glycaemia was determined in blood sample from the tail vein of fasting rats using a glucometer (ACCU-CHEK® Advantage; Roche Diagnostics, Mannheim, Germany).

Insulin resistance evaluation

We evaluated insulin resistance by the product of insulin and glucose:

Leptin resistance test

Peptide

Recombinant mouse leptin (PeproTech, Rocky Hill, NJ, USA) was dissolved in saline vehicle (0·9 %, w/v) and was given as a bolus injection at a dose of 0·5 mg/kg body weight intraperitoneally.

Feeding study

At 30 d, the rats of each experimental group (Lep and C) were randomly assigned to one of the following groups: leptin (CL, LepL) or saline (CSal, LepSal) group. The animals were food-deprived for 24 h while maintaining free access to water before the test. After an intraperitoneal injection of leptin or saline, they were returned to their home cages and provided with a supplementary amount of a standard diet. They were housed singly and food intake was measured by weighing the food cups 2, 4, 6 and 24 h after leptin or saline injections(Reference Passos, Vicente, Lisboa and Moura5, Reference Toste, Moura, Lisboa, Fagundes, Oliveira and Passos9, Reference Martin, Perez, He, Dawson and Millard29).

Western blotting analysis

The hypothalamus, collected under basal conditions, was homogenised in ice-cold lysis buffer (50 mm-HEPES (pH 6·4), 1 mm-MgCl2, 10 mm-EDTA, Triton X-100 (1 %), plus aprotinin, leupeptin and soyabean trypsin inhibitor, each one at 1 mg/ml). The homogenates were stored at − 20°C. The protein concentration was determined by the method of Bradford(Reference Bradford30).

The proteins (60 μg) were separated by SDS-PAGE (12 %) and transferred to a nitrocellulose membrane (Hybond™ ECL™; Amersham Pharmacia Biotech, Little Chalfont, Bucks, UK). The membrane was blocked for 30 min with 2 % bovine serum albumin in Tris-buffered saline Tween 20 (TBS-T) buffer (20 mm-2-amino-2-hydroxymethyl-propane-1,3-diol (Tris) (pH 7·5), 0·5 m-NaCl with 0·1 % Tween 20), incubated with OB-R-goat polyclonal IgG primary antibody (1:1000)/SOCS-3-goat polyclonal IgG primary antibody (Santa Cruz Biotechnology, Santa Cruz, CA, USA) in TBS-T overnight, washed three times with TBS-T, and incubated with secondary antibody (peroxidase-conjugated donkey IgG, 1:1000), for 1 h. After the membrane was washed three times with TBS-T, the antibody binding was visualised using diaminobenzidine (5 mg in 10 ml 0·1 m-Tris buffer, pH 7·4). Actin antibody (I-19, SC-1616; Santa Cruz Biotechnology) was used as an internal control. Densitometry analyses of the immunoreactive bands were determined by Image-Pro® Plus software (Media Cybernetics, Inc., Bethesda, MD, USA).

Statistical analysis

The data are reported as mean values with their standard errors. Two-way ANOVA followed by the Newman–Keuls multiple comparisons test were used to analyse body-weight evolution and food intake in response to the acute leptin treatment. Other experimental observations were determined by Student's t test with the significance level set at P < 0·05.

Results

Body composition

Body weight from birth until age 30 d is shown in Fig. 1. During that time, the Lep group had a lower body weight than the C group, from the third day of leptin injection to the 21st day (approximately − 5 %; P < 0·04). After day 21, these animals regained body weight, and reached the same weight of the C group at the end of the experimental period. Despite their normal body-weight gain, their fat mass was lower ( − 22·2 %; P < 0·004) and protein mass was higher (+100 %; P < 0·0002) compared with controls (Table 1).

Fig. 1 (a) Body weight from birth until age 30 d of animals treated with saline (–●–) or with leptin () on the first 10 d of lactation. Values are means of twelve animals per group. ( ← ), Significant differences between the treated and control groups from the third day of leptin injection to day 21: *P < 0·05. (b) Values from day 0 to day 10 for the control (–○–) and leptin-treated (–▲–) rats. * Mean value for the leptin-treated group was significantly different from that of the control group (P < 0·05).

Table 1 Body composition and serum hormone concentrations of animals at age 30 d that were given daily injections of leptin for the first 10 d of lactation and control animals

(Mean values with their standard errors for ten animals per group)

* Mean value was significantly different from that of the control group (P < 0·05).

Serum leptin, insulin, adiponectin, blood glucose and insulin resistance index

The Lep group had a higher serum leptin (+136 %; P < 0·05) concentration 2 h after the last leptin injection, which confirmed the hyperleptinaemia. Table 1 shows serum hormone concentrations for offspring aged 30 d. The Lep group had higher serum leptin (5-fold; P < 0·0001), higher glycaemia (+8 %; P < 0·05) and hyperinsulinaemia (+43 %; P < 0·05), but lower serum adiponectin ( − 43·2 %; P < 0·05) compared with the control group. The Lep group showed a significantly higher (+65 %; P < 0·05) insulin resistance index, which may indicate insulin resistance (Table 1).

Leptin resistance test

Fig. 2 shows the leptin resistance test for animals aged 30 d. The effectiveness of the test is demonstrated by the result of the control group, where leptin treatment significantly suppressed food intake at 2 h ( − 26·3 %; P < 0·05), 4 h ( − 21 %; P < 0·02) and 6 h ( − 17·6 %; P < 0·05) after leptin injection compared with the group that received saline (Fig. 2 (a)). However, the LepL group did not show a similar decrease, in all periods studied, suggesting a resistance to the anorexigenic effect of leptin (Fig. 2 (b)).

Fig. 2 Effect of acute leptin treatment () compared with saline treatment alone (■; control) on food intake of rats aged 30 d that were treated with saline (a) or leptin (b) for the first 10 d of lactation. Values are the means of cumulative intake for five animals per group, with standard errors represented by vertical bars. * Mean value was significantly different from that of the respective saline control group (P < 0·05).

Western blotting of the hypothalamic leptin receptor and suppressor of cytokine signalling-3

Western blotting of total protein lysates from the hypothalamus of rats aged 30 d is shown in Fig. 3. The level of OB-Rb was lower ( − 21·6 %; P < 0·05), while SOCS-3 expression was higher (+52·8 %; P < 0·002) when compared with the control group.

Fig. 3 Western blots of leptin receptor (OB-Rb) (a) and suppressor of cytokine signalling-3 (SOCS-3) (b) in the hypothalamus of rats at age 30 d that were given daily injections of leptin (Lep) for the first 10 d of lactation and controls (C) that received the same volume of saline. Shown below the plots are densitometric analyses of the immunoreactive bands for OB-Rb and SOCS-3. A representative experiment is shown from three independent experiments. Data are means of four animals in each group, with standard errors represented by vertical bars. * Mean value was significantly different from that of the control group (P < 0·05).

Discussion

The findings of the present study confirms in young (age 30 d) rats similar changes observed in adult ones (age 150 d) caused by leptin neonatal programming. At both ages, the rats were programmed for hyperinsulinaemia, hyperleptinaemia and leptin resistance probably due to lower hypothalamic OB-Rb expression(Reference Toste, Moura, Lisboa, Fagundes, Oliveira and Passos9). Here we evaluated other parameters, showing lower adiponectinaemia and higher SOCS-3 expression. The major finding of the present study is that this programming occurs as soon as 1 week after weaning.

In agreement with other studies(Reference Ahima, Prabakaran and Flier31Reference Oates, Noodside and Walker33) and our previous findings(Reference Oliveira Cravo, Teixeira, Passos, Dutra, Moura and Ramos7Reference Toste, Moura, Lisboa, Fagundes, Oliveira and Passos9, Reference Dutra, Moura, Rodrigues, Lisboa, Bonomo, Toste and Passos34), leptin injected peripherally during the first 10 d of lactation did increase serum leptin in the neonatal period at age 10 d and it is still higher at age 30 d. Ahima et al. (Reference Ahima, Prabakaran and Flier31) demonstrated in normal lean mice that during the neonatal period leptin rises transiently, which was termed as the ‘neonatal leptin surge’. In their experiment, leptin increased 5- to 10-fold to a peak level of 50 (sd 10) ng/ml in mice aged 10 d.

In the neonatal period, leptin alters hypothalamic neuropeptide expression and the metabolic rate before exerting its anorectic effect(Reference Mistry, Swick and Romsos32, Reference Ahima and Hileman35). Bouret et al. (Reference Bouret, Draper and Simerly36) demonstrated that leptin treatment in ob/ob mice in the neonatal period (4–12 d of life) reverts the reduction in nervous fibres that express pro-opiomelanocortin; the contrary occurred with NPY neurons. However, the treatment during adulthood did not result in the formation of anorexigenic and orexigenic neurons, confirming the existence of a critical period, where the neurons are leptin-dependent for their development in mice.

Several groups reported that exogenous leptin does not significantly inhibit growth, food intake, or energy expenditure during the first 2–3 postnatal weeks(Reference Mistry, Swick and Romsos32, Reference Ahima and Hileman35). More specifically, Mistry et al. (Reference Mistry, Swick and Romsos32) have shown that leptin does not alter significantly O2 consumption (a marker of energy expenditure) or food intake in normal lean mice until postnatal day 17. So, this suggests that the neonatal brain is relatively insensitive to leptin and may present leptin resistance(Reference Mistry, Swick and Romsos32). However, leptin receptors are expressed in the arcuate nucleus of the hypothalamus (ARH) of rats(Reference Matsuda, Nakamura, Nakao, Arai, Katsuki, Heike and Yokota37) before the development of ARH pathways.

Leptin also acts as a trophic signal that directs key developmental events in the early hypothalamic pathways that convey leptin signals to brain regions regulating body weight. Events imposed by prenatal nutrition that alter leptin levels may have consequences for the formation and function of circuits that regulate food intake and body weight throughout the life of an animal(Reference Bouret, Draper and Simerly36).

Plagemann et al. (Reference Plagemann, Harder, Rake, Waas, Melchior, Ziska, Rohde and Dörner38) showed in the small-litter model that the offspring developed overweight, hyperleptinaemia and hyperinsulinaemia, and did not find the expected decrease in NPY content in the arcuate nucleus and paraventricular nucleus when the rats were age 21 d. Since the NPY system is functionally mature already at this age, these findings might indicate an acquired resistance of the hypothalamic NPY system to increased levels of leptin and insulin in early postnatal overfed rats. In another model studied by our group, the prolactin blockage caused a higher transfer of leptin through the milk(Reference Bonomo, Lisboa, Passos, Pazos-Moura, Reis and Moura39) and the offspring developed higher adiposity and leptin resistance at adulthood(Reference Bonomo, Lisboa, Pereira, Passos and de Moura40). Also leptin injection to the mothers during lactation caused similar effects at adulthood(Reference Lins, Moura, Lisboa, Bonomo and Passos41). Since the rat central nervous system is still developing on the first days postnatally, leptin could imprint the orexigenic and anorexigenic neurons, programming for the development of diseases later in life.

In respect to the programming effects of leptin on body-weight regulation, our data disagree with some reports(Reference Stocker, O'Dowd, Morton, Wargent, Senitt, Hislop, Glund, Seckl, Arch and Cawthorne42Reference Picó, Oliver, Sánchez, Miralles, Caimari, Priego and Palou44) and agree with others(Reference Yura, Itoh, Sagawa, Yamamoto, Masuzaki, Kawamura, Takemura, Kakui, Ogawa and Fujii6, Reference Vickers, Gluckman, Coveny, Hofman, Cutfield, Gertler, Breier and Harris45). In the study of Stocker et al. (Reference Stocker, O'Dowd, Morton, Wargent, Senitt, Hislop, Glund, Seckl, Arch and Cawthorne42) the administration of leptin from pregnancy and throughout lactation to rats fed on a low-protein diet reduces the susceptibility of a high-fat-diet to induce higher weight gain. However, in that study those authors did not study the effect of maternal leptin treatment in mothers fed a standard chow diet. Our model is a more physiological one, since the animals received a normal diet during all the study.

In the study of Picó et al. (Reference Picó, Oliver, Sánchez, Miralles, Caimari, Priego and Palou44) a daily oral dose of leptin (5-fold the leptin concentration of milk) was given to suckling male rats during lactation. After weaning the pups were fed with a normal-fat or a high-fat diet. Leptin-treated animals had, in adulthood, lower body weight, fat content, food intake and hypoleptinaemia. These data are similar to our previous study where the lactating rats were submitted to a protein-restricted diet(Reference Passos, Ramos and Moura46). Offspring with a protein-restricted diet had, in adulthood, lower body weight and this can be mainly associated with a lower milk concentration of protein. It is possible that in the study of Picó et al. (Reference Picó, Oliver, Sánchez, Miralles, Caimari, Priego and Palou44) that the animals present malnutrition, since oral doses of leptin could lead to an accentuated higher satiety and lower milk intake with consequent protein restriction and lower body weight in adulthood. However, it is also possible, that oral leptin could induce some gastrointestinal mediators that were bypassed by subcutaneous injection.

Vickers et al. (Reference Vickers, Gluckman, Coveny, Hofman, Cutfield, Gertler, Breier and Harris43) showed that leptin injection on the first days of lactation in female rats whose mothers were submitted to energy restriction during pregnancy normalises the body-weight gain, the food intake and body fat of the offspring in adulthood. However, in this study the neonatal leptin treatment did not cause changes in the female adult offspring from mothers with a normal diet during pregnancy. Moreover, our present findings confirm the recent data of Vickers et al. (Reference Vickers, Gluckman, Coveny, Hofman, Cutfield, Gertler, Breier and Harris45), which showed that the administration of leptin on the first days of lactation in male rats, whose mothers received a normal diet during pregnancy, programmed for higher body weight, hyperinsulinaemia and higher total adiposity. Our findings also corroborate the study of Yura et al. (Reference Yura, Itoh, Sagawa, Yamamoto, Masuzaki, Kawamura, Takemura, Kakui, Ogawa and Fujii6) where neonatal leptin-treated rats developed pronounced weight gain, adiposity and leptin resistance later in life.

It is possible that the differences in these studies occur mainly because of the dose, different periods of development (pregnancy and lactation), sex, undernutrition during the treatment and a higher-fat diet after weaning.

In the present study we showed the consequences of neonatal leptin treatment at an early age. The Lep animals presented higher serum leptin and insulin concentrations and, different from observed before in adult animals, the young Lep group had hyperglycaemia and a higher insulin resistance index, suggesting insulin resistance. The development of resistance to the action of these hormones appears to have an important role in the pathogenesis of obesity and type 2 diabetes. The serum adiponectin concentration has been considered an appropriate parameter for evaluation of insulin resistance(Reference Hara, Horikoshi, Yamauchi, Yago, Miyazaki, Ebinuma, Imai, Nagai and Kadowaki47). The Lep group presented, at age 30 and 150 d, lower serum adiponectin; this could be related to their insulin resistance at those ages.

Leptin resistance may occur for one of several reasons: leptin may fail to cross the blood–brain barrier, the hypothalamic receptors may be down-regulated or there may be abnormalities in the leptin receptor signalling pathway, such as SOCS-3 activation(Reference Jéquier48Reference Sahu50).

We demonstrated that leptin treatment during lactation increases serum leptin concentration in adulthood, which leads to leptin resistance by reducing the expression of the hypothalamic OB-Rb(Reference Toste, Moura, Lisboa, Fagundes, Oliveira and Passos9), since hyperleptinaemia can down-regulate its receptors. But here we add another level of complexity to this programming effect, showing the increase in SOCS-3 protein, that can be caused by both hyperleptinaemia or hyperinsulinaemia and may be one of the causes of both leptin and insulin resistance.

It is interesting that in this model the first thing to occur is leptin resistance, even with a lower adiposity. Thus, the primary defect seems to be hypothalamic and we suggest that higher SOCS-3 could have an important role blocking the leptin's signalling transduction.

Those animals had hyperleptinaemia even with lower adiposity. Leptin can be produced by other tissues, such as skeletal muscle(Reference Wang, Liu, Hawkins, Barzilai and Rossetti51), that is probably higher in those animals that presented higher protein mass. In fact, the hyperleptinaemia in this model seems to be not related to the mass of adipose tissue. Even though in most of the models leptin does correlate with adipose tissue mass, this relationship seems to be not so simple(Reference Mantzoros and Moschos52); in some cases the relationship is curvilinear, reflecting more the process of fat accumulation than the total fat mass. Since leptin is produced by other tissues, such as muscle(Reference Wang, Liu, Hawkins, Barzilai and Rossetti51), the increase of leptin production in those tissues could be the main explanation for these findings. Another explanation could be differences in the leptin clearance of these two groups.

In conclusion, the present results showed that neonatal hyperleptinaemia has a role as a neurotrophic factor that alters energy regulation by the hypothalamus and contributes to developmental programming of leptin and insulin resistance in rats as soon as 1 week after weaning. These effects may be explained by a higher expression of SOCS-3 protein and lower serum adiponectin. Our findings also suggested that the resistance to the anorexigenic effect of leptin at 30 d can be one of the ‘imprinting’ factors that associate the hyperleptinaemia during the first 10 d of lactation with the programming of higher risk to develop diabetes mellitus with ageing.

Acknowledgements

Research was supported by grants from the National Council for Scientific and Technological Development (Conselho Nacional de Desenvolvimento Científico e Tecnológico; CNPq), Coordination for the Enhancement of Higher Education Personnel (Coordenação de Aperfeiçoamento de Pessoal de Nível Superior; CAPES) and the State of Rio de Janeiro Carlos Chagas Filho Research Foundation (Fundação de Amparo à Pesquisa do Rio de Janeiro; FAPERJ). Fernanda P. T. and P. A.T. were recipients of a CNPq fellowship and Fabiane P. T. was a recipient of a CAPES fellowship. All authors are grateful to Ms Monica Gaspar de Moura, Tiago Gomes and Mr Carlos Roberto for their technical assistance.

M. C. F. P., P. C. L. and E. G. M. designed the study and wrote the protocol and manuscript. Fabiane P. T. managed the literature searches. Fabiane P. T., Fernanda P. T., S. C. P. D. and P. A. T. were responsible for animal programming, and biochemical and molecular procedures. All authors contributed to and approved the final manuscript.

The authors declare no conflict of interest.

References

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Figure 0

Fig. 1 (a) Body weight from birth until age 30 d of animals treated with saline (–●–) or with leptin () on the first 10 d of lactation. Values are means of twelve animals per group. ( ← ), Significant differences between the treated and control groups from the third day of leptin injection to day 21: *P < 0·05. (b) Values from day 0 to day 10 for the control (–○–) and leptin-treated (–▲–) rats. * Mean value for the leptin-treated group was significantly different from that of the control group (P < 0·05).

Figure 1

Table 1 Body composition and serum hormone concentrations of animals at age 30 d that were given daily injections of leptin for the first 10 d of lactation and control animals(Mean values with their standard errors for ten animals per group)

Figure 2

Fig. 2 Effect of acute leptin treatment () compared with saline treatment alone (■; control) on food intake of rats aged 30 d that were treated with saline (a) or leptin (b) for the first 10 d of lactation. Values are the means of cumulative intake for five animals per group, with standard errors represented by vertical bars. * Mean value was significantly different from that of the respective saline control group (P < 0·05).

Figure 3

Fig. 3 Western blots of leptin receptor (OB-Rb) (a) and suppressor of cytokine signalling-3 (SOCS-3) (b) in the hypothalamus of rats at age 30 d that were given daily injections of leptin (Lep) for the first 10 d of lactation and controls (C) that received the same volume of saline. Shown below the plots are densitometric analyses of the immunoreactive bands for OB-Rb and SOCS-3. A representative experiment is shown from three independent experiments. Data are means of four animals in each group, with standard errors represented by vertical bars. * Mean value was significantly different from that of the control group (P < 0·05).