Abstract
Chronic consumption of hyperpalatable and hypercaloric foods has been pointed out as a factor associated with cognitive decline and memory impairment in obesity. In this context, the integration between peripheral and central inflammation may play a significant role in the negative effects of an obesogenic environment on memory. However, little is known about how obesity-related peripheral inflammation affects specific neurotransmission systems involved with memory regulation. Here, we test the hypothesis that chronic exposure to a highly palatable diet may cause neuroinflammation, glutamatergic dysfunction, and memory impairment. For that, we exposed C57BL/6J mice to a high sugar and butter diet (HSB) for 12 weeks, and we investigated its effects on behavior, glial reactivity, blood–brain barrier permeability, pro-inflammatory features, glutamatergic alterations, plasticity, and fractalkine-CX3CR1 axis. Our results revealed that HSB diet induced a decrease in memory reconsolidation and extinction, as well as an increase in hippocampal glutamate levels. Although our data indicated a peripheral pro-inflammatory profile, we did not observe hippocampal neuroinflammatory features. Furthermore, we also observed that the HSB diet increased hippocampal fractalkine levels, a key chemokine associated with neuroprotection and inflammatory regulation. Then, we hypothesized that the elevation on glutamate levels may saturate synaptic communication, partially limiting plasticity, whereas fractalkine levels increase as a strategy to decrease glutamatergic damage.
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Introduction
Excessive consumption of highly palatable and energy-dense foods in Westernized societies is pointed out as a main environmental contributor to obesity, a pathological condition characterized by excessive accumulation of adipose tissue, as well by the imbalance between homeostatic caloric intake and energy expenditure1. Obesity may predispose to several harmful effects on human health, including not only metabolic and cardiovascular dysfunction, but also alterations in the central nervous system (CNS), which may affect mood, cognition, and memory2,3,4,5. Indeed, studies have demonstrated a negative relationship between highly palatable/energy-dense foods and obesity on different types of memory, such as episodic, aversive, and working memory3,4,6,7,8. Moreover, memory dysfunction associated with chronic consumption of highly palatable/energy-dense foods is linked to damages in decision-making, attention, executive skills, and social behavior, which may lead to a positive feedback of the obesogenic environment by maintaining food choices3,4. However, it is important to highlight that the complete underlying mechanism connecting the chronic consumption of highly palatable/energy-dense foods, obesity and memory deficits needs to be better addressed.
Pathological neuroinflammation is associated with negative impact on memory and cognitive function, and is closely related to metabolic alterations and peripheral inflammation9,10. Importantly, neuroinflammation associated with the consumption of highly palatable and energy-dense foods may be driven by peripheral low-grade inflammation through upregulation of pro-inflammatory serum levels of cytokines (IL-1β, IL-6, TNF-α, IFNγ), leptin, free fatty acids, and the reduction of blood–brain barrier permeability (BBB) tight junctions, as claudin-5 (CLDN5), occludin and zonula occludens-1 (ZO-1)11,12,13. In addition, it has been hypothesized that these mechanisms may increase the influx of peripheral immunomodulators into susceptible CNS areas, such as hypothalamus and hippocampus, intermediating the production of pro-inflammatory cytokines by glial cells, including astrocytes and microglia, which might contributes to obesity memory decline12,13,14,15. In this context, in chronic models of diet-induced obesity (DIO), the release of pro-inflammatory mediators by microglia, such as IL-1β, IL-6, TNF-α and nitric oxide, is associated with a decrease in neurotrophic factors production, synaptic proteins, and abnormal synaptic engulfment6,16,17,18,19. Furthermore, neuroinflammatory features are also associated with disruptions in neuron-glial cross-talk systems, such as the fractalkine/CX3CR1 pathway, which could lead to alterations in the number and complexity of hippocampal dendritic spines, impairment in long-term potential (LTP) formation, and cognitive decline in DIO models16,18. However, while data suggest a strong association between chronic consumption of highly palatable food, inflammation, and memory impairment in the context of obesity, the precise implications of this interaction on specific neurotransmitter systems remain elusive.
Glutamatergic neurotransmission has a crucial role in hippocampal memory and learning, a key area associated with the maintenance of several memory processes, such as acquisition, consolidation, memory retrieval, re-consolidation, and extinction20,21,22. In this context, glutamatergic signaling depends on the action of ionotropic (iGluR) and metabotropic receptors (mGluR), as I GluR-α-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid receptors (AMPA-R), N-methyl-d-aspartate receptors (NMDA-R), Kainate receptors (GluK1–GluK5) and mGluR1–mGluR823,24. Moreover, dysfunctions in the regulation of glutamate levels or glutamatergic signaling are associated with disturbances in neuroplasticity mechanisms, such as the production of neurotrophic factors, memory decline, cognitive deficits, and neurotoxic events23,24,25,26. Although it is poorly understood, evidence pointed out that immunomodulatory event may be involved in the regulation of central glutamatergic dynamics27,28,29. For instance, data from murine hippocampal slices showed that high levels of INF-ɣ, TNF, and IL-1β are able to increase the expression, activity, and recruitment of postsynaptic AMPA and NMDA subunits (GluR1, NR2A/NR2B, respectively), suggesting some part of these cytokines in the physiopathology of glutamatergic transmission28,29,30. Moreover, a pro-inflammatory environment could induce the production of glutamate by glial cells, increasing its concentration in the synaptic cleft27,31. Furthermore, increased glial fibrillary acidic protein (GFAP) expression in DIO models is associated with decreased expression of astrocytic glutamatergic transporters, such as glutamate transporter-1 (GLT-1), which may be associated with neurotoxicity and neuronal plasticity damage32. Thus, taking into consideration that few studies have investigated the role of glutamatergic signaling in an obesogenic environment generated by highly palatable diets, regarding memory impairment32,33,34, we decided to test the hypothesis that a chronic exposure to a highly palatable/ energy-dense diet may induce hippocampal neuroinflammation, triggered by peripheral inflammation, which in turn, may lead to abnormal regulation of glutamatergic neurotransmission and memory deficits.
Methods
Animals and ethical aspect
C57BL/6J male mice (3–4 weeks) were purchased from the animal facility of Universidade Federal de Minas Gerais (UFMG). Animals were housed five per cage under the following environmental conditions: 12 h light/12 h dark cycle, temperature at 24 ± 2 °C with food and water provided ad libitum. The sample size for the animal experiments was determined through a rigorous calculation, considering the variance observed in specific assays, and was approved by the institutional animal use ethics committee (CEUA-UFMG no. 217/2020). All experiments were carried out in accordance with ARRIVE guidelines (https://arriveguidelines.org). All methods were performed in accordance with the relevant guidelines and regulations.
Diets and experimental design
After 1 week of habituation, mice were divided into two groups, and fed for 12 weeks with an isocaloric diet (American Institute of Nutrition 93-Growth diet (AIN93G, (carbohydrates: 64%, proteins: 20%; lipids: 16%; 3.9 kcal/g) or a highly palatable/energy-dense diet [high butter and sugar diet (HSB), (carbohydrate: 36%, proteins: 16%; lipids: 48%; 4.9 kcal/g)]11 (Supplementary data, Fig. S1A). Mice were weighed once a week. In addition, the cumulative energy intake was calculated by summing weekly values of the food amount eaten per cage multiplied by the caloric value of each diet35. Between the 11th and 12th week of the diet-induced obesity protocol, behavioral analyses were performed to evaluate memory and learning deficits (n = 10 per group) (Supplementary data, Fig. S1B). In parallel, a separate cohort of animals was submitted to the oral glucose tolerance test (n = 10 per group) (Supplementary data, Fig. S1A). At the end of week 12th euthanasia was performed in order to obtain tissues for biochemical, molecular and histological assays (n = 5–10 per group) (Supplementary data, Fig. S1B). Importantly, with the exception of histological analyses, all euthanasia was performed by decapitation to avoid interference with basal glutamatergic signaling. Immediately after euthanasia, the brain was isolated and the hippocampus was dissected for molecular measurements. Regarding serum analyses, cervical blood samples were collected in heparinized tubes, centrifuged at 1500×g, 4 °C, for 15 min, and stocked at − 70 °C until use. In addition, topics 2.6 and 2.9 contain information on the euthanasia and tissue preparation for histological and hippocampal synaptosome assays, respectively.
Behavioral assessment
All behavioral tests were performed during the light cycle, under controlled conditions of temperature and brightness (24 ± 2 °C, 70–80 lx). Furthermore, 30 min acclimation period was given to mice before starting the experiments. All apparatus were cleaned with 70% ethanol between the experimental sessions to avoid olfactory bias. None of mice cohorts used were subjected to more than two different behavioral tests (Supplementary data, Fig. S1B). Experimental tasks were designed to consider the most stressful behavioral experiment to be performed at last. In addition, one to four days of interval between experimental tasks were applied (Supplementary data, Fig. S1B). Also, mice were not deprived of food or water during experimentation. All behavioral memory tasks were manually analyzed with the support of the software X-Plot-Rat ®2005 (developed by the research team of Dr. Morato, Faculdade de Filosofia, Ciências e Letras de Ribeirão Preto, USP, Brazil).
Open field
To evaluate locomotor and exploratory behavior, the open field test was performed. Mice were randomly placed in a cylindrical and circular acrylic apparatus (30 cm × 40 cm), where free exploration was allowed for 30 min. Total distance traveled (cm), the average speed (m/s), as well as the time spent in the center of the arena (s) were recorded and analyzed by Any-maze Video Tracking System Software (version 5.26, Stoelting®).
Y maze test
The evaluation of short-term memory was performed by using the Y- maze test. For that, a grey plastic maze with three arms (A, B, C) (30 cm length, 6 cm width, 20 cm height) arranged at a 60° angle was used. In addition, different visual clues were used in each arm to help the mice to recognize them. Mice were placed individually at the distal part of A-arm and free to explore the apparatus for 8 min. An arm entry was considered only when both hind paws were placed completely inside. Percent alternation was calculated using the following formula:
Object location test (OLT) and object recognition test (ORT)
A white square acrylic open field (38 × 38 × 15 cm) was utilized for both tests. At the first day, mice were habituated to the apparatus for 5 min. 24 and 48 h after habituation, mice were re-exposed to the open field containing two identical objects, two identical plastic bottles (20.5 cm high, 6 cm wide), colored red and filled with 11 cm of water. In addition, these objects were located symmetrically at 80 mm of the apparatus wall and vertically separated from each other by 6 cm. Free exploration was measured for 10 and 5 min, in these respective days. To the OLT and ORT test (72 h after habituation), one of the objects was displaced 6 cm away from the original position (novel position) or one of the objects was replaced by a new object, without altering the original localization. In addition, the new object consisted of multi-colored lego blocks, stacked vertically to have the same dimensions as the familiar object. In both tests, mice were allowed to freely explore for 5 min. Interaction with the objects was defined as sniffing until 2 cm of distance from the object, as well as touching the objects with the nose or forepaws. The percent of total investigated time of the new object or moved object was calculated according to the following formulas36:
Contextual fear conditioning
A conditioning chamber (330 × 200 × 300 mm3) with a grid floor, and transparent acrylic board customized with black vertical lines was used for mice contextual fear conditioning37. The first day of the experimental procedure consisted of an induction of aversive conditioning to the context. For this, mice were individually habituated within 120 s to the apparatus and subsequently subjected to a foot shock (Unconditioned stimulus (US): 0.7 mA per 2 s). After the first shock, an interval of 60 s was given before a new US was applied. In total, three US were performed with a 60 s interval between them. At the end of the session, animals were removed from the apparatus and returned to their cages. 24 h after the aversive conditioning, the evocation memory test was executed in order to evaluate the memory retrieval. For this, mice were re-exposed to conditioning context, without receiving new shocks, for 5 min. Furthermore, in order to check for possible alternations in memory extinction process, we induced fear memory extinction by prolonging the exposition of the mice to the context for more than 15 min (totaling a 20 min of test). Finally, on the third day, mice were re-exposed to context, for 5 min, for the evaluation of memory extinction (memory extinction test). For analyses, freezing was considered as the entire absence of movement, excluding breathing periods. The computation of freezing was performed every minute during the entire memory evocation and extinction test session. All results were expressed in percent of freezing.
Social interaction and social memory test
The evaluation of social interaction and social memory was conducted in a transparent and rectangular acrylic box (60 × 40 cm) divided into three compartments (20 × 40 × 22 cm) separated by two interior doors. Adult mice were individually habituated for 5 min in the central compartment. Subsequently, for the evaluation of social interaction, a plastic transparent cylinder (10 cm diameter with distributed holes) containing an unfamiliar male juvenile mouse (Stranger 1) was introduced into one of the chambers and an identical empty plastic cylinder was introduced in the remaining chamber. After, inner doors were opened and mice were free to explore the social apparatus for 10 min. Additionally, the location chamber with the juvenile mouse or the empty cylinder was alternated between experimental sessions. Then, a second unfamiliar mouse (Stranger 2) was placed in the empty cylinder for the evaluation of social memory. Thus, the adult mouse was free to explore the apparatus for another 10 min. Furthermore, in order to assess short- and long-term social memory, an additional single-chamber protocol was performed38. In summary, the training session consisted of habituating of mice for 15 min in a standard cage. After, a plastic transparent cylinder containing an unfamiliar male juvenile mouse was presented to an adult mouse for 5 min. For the evaluation of short-term memory (STM) and long-term memory (LTM), the same experimental procedures, and the same juvenile mouse, were re-exposed to the adults’ mice after an hour and a half and 24 h after the training session, respectively. Importantly, in three and one chamber paradigms, none of the juvenile mice were used more than four times. Moreover, in both protocols the social investigation was computed at the time that the resident mice introduced their nose or whiskers inside any of the cylinder's holes38. The social interaction and social memory index were calculated according to the following formulas:
STM and LTM were expressed by the raw interaction time with juvenile mice as compared to training, as well by the percentage of time of interaction with the juvenile mice considering the total time tested38.
Oral glucose tolerance test
The oral glucose tolerance test (oGTT) was adapted from Pedro et al. (2020)39. At 12th week, a separated cohort of mice was submitted to fast for 6 h (07 AM to 01 PM). Glucose (30%) was administered by gavage (2 g/kg). Blood sampling was obtained by the tip of the tail, using a scissor, and glucose concentration (mg/dL) was measured with a glucometer (On call plus II®), before glucose gavage, and 15, 30, 60, 90, and 120 min thereafter. The area under the curve (AUC) was calculated to assess differences in glucose metabolism between the groups of interest40.
Cholesterol measurement, adiposity and lee index
The total cholesterol levels were measured in the serum of mice by a commercial colorimetric enzymatic test in accordance with manufacturer instructions (Bioclin, MG, Brazil). A spectrophotometer with wavelength of 500 nm was used to acquire data. The following formula was utilized for final concentration determination: total cholesterol (mg/dL): [sample absorbance × 200]/standard absorbance. Alterations in body composition caused by HSB diet and cardiometabolic risk were evaluated through adiposity measurements and Lee Indexes. The sum of the weight of visceral adipose tissue fat pads (VAT) compounds from the epididymal (EAT), mesenteric (MAT), and retroperitoneal (RPAT) fat pad was used for the calculation of visceral adipose tissue index: [VAT (g)/body weight (g)] × 100. Lee index was calculated by the following formula:
Intracardiac perfusion and brain slices
At 12th week, animals were anesthetized with ketamine (80 mg/kg, i.p) and xylazine (8 mg/kg, i.p), and then submitted to a thoracotomy for heart exposition. A needle coupled to a peristaltic pump infusion system was inserted in the left ventricle and a small incision was made in the right atrium, allowing the withdrawal of blood by infusion of phosphate saline buffer (pH 7.4; 5 ml/min; 30–100 ml per animal). After animals were perfused with a paraformaldehyde solution (PFA 4%, pH 7.4, 20–30 ml per animal), decapitated, and their brains were stored overnight in PFA 4%. Subsequently, brains were cryoprotected, before being frozen in ice isopentane (99%, 20 s), by gradual dehydration in a 15% sucrose buffer (pH 7.4), and then in a 30% sucrose buffer (pH 7.4,) until complete precipitation. Brains were sliced into 30 µm sections in a cryostat at −25 °C (Leica Biosystems, Buffalo Grove, USA).
Evaluation of microglial density and morphology
Microglial morphological features may provide information about cellular functional phenotypes41. Thus, in order to evaluate whether an obesogenic diet affects the microglial densitometry and morphological parameters, immunohistochemistry analyses were performed. Slices were incubated with citrate buffer (pH 6.0, 70 °C, 1 h), washed with TBS (3×, 5 min), pretreated with 1% of H2O2 (15 min), washed (TBS, 3×, 5 min) and blocked with BSA 4% in TBS triton 0.5% for 1 h at room temperature followed by primary antibody incubation (rabbit anti-Iba-1 (1:500; Wako Chemicals, Osaka, Japan) for 48 h at 4 °C. After washing (TBS, 3×, 5 min), slices were incubated with biotinylated secondary antibody (goat anti-rabbit (1:500 in TBS; Vector Laboratories, Burlingame, USA; overnight at 4 °C). Posteriorly, slices were incubated with Avidin–Biotin solution (ABC) (VECTASTAIN ABC kit, Vector Laboratories, Burlingame, USA) for 1 h. For revealing the staining, DAB (Sigma-Aldrich, St. Louis, USA) diluted in TBS and activated with H2O2 0.04% was utilized in accordance with manufactured instructions. Sections were washed (TBS, 3×, 5 min) and mounted in histological slices. After drying, slices were sequentially dehydrated in ethanol 70, 80, 95% (3 min), and 100% (two twice, 4 min), and cleaned in xylene (two times, 5 min) before mount cover slices with DPX (Sigma-Aldrich, St. Louis, USA). The images of DG, CA1, CA2-CA3 were acquired in a light microscopy (APOTOME.2, Carl Zeiss, Jena, Germany) in 20× and 40× magnification, for densitometry and morphological analysis, respectively. The quantification of optical density and measurement of cell body to cell size ratio was performed using FIJI software (NIH, Bethesda MD, USA) in accordance with previously published methods41,42. For this, three brain slices per animal (technical replicates), six photos for DG, CA1 and 3 pictures for CA2–3 were used for analysis.
Evaluation of astrocyte reactivity
Immunofluorescence analyses were performed to evaluate astrocyte reactivity. Hippocampal brain slices were incubated with citrate buffer (pH 6.0) at 70 °C for 60 min, washed with TBS (3×, 5 min), and blocked overnight with 4% BSA in 0.5% TBS triton (TBSt), before incubation with primary antibody (mouse anti-GFAP (1:500; Millipore, Darmstadt, Germany) for 48 h at 4 °C. Afterwards, slices were washed with TBS (3×, 5 min) and incubated, at dark, with secondary antibodies (120 min), (goat anti-mouse, 1:1000; Alexa Fluor 488, Life Technologies, Carlsbad, USA). Finally, after the washing (TBS, 3×, 5 min), 1 µg/ml of DAPI was added (30 min). Sections were washed (TBS, 3×, 5 min), mounted in histological slices, and after drying, mounted cover with Fluoromount (Sigma-Aldrich, St. Louis, USA). Images were acquired with a fluorescence microscopy (AxioCam M2, Carl Zeiss, Jena, Germany) in 20× magnification. The quantification of cell bodies was performed in the dentate gyrus (DG), CA1, CA2–CA3 using FIJI software (NIH, Bethesda MD, USA). For this, two brain slices per animal (technical replicates), four photos for DG, CA1 and two pictures for CA2–3 were used for analysis. All results were represented as percent of the area stained for GFAP and the mean fluorescence intensity of the cells.
Measurement of cortical and hippocampal glutamate release
Purification of synaptosomes
The hippocampal pools of synaptosomes (3 mice per pool) were obtained in accordance with Dunkley et al. (1986)43. After decapitation and dissection, tissues were immediately homogenized in an ice gradient solution (320 mM sucrose, 0.25 mM dithiothreitol, 1 mM EDTA), centrifuged (1000g, 10 min, 4 °C) and the resultant supernatant was purified by separation in a discontinuous percoll gradient (Sigma Aldrich®) at concentrations of 23%, 15%, 10%, and 3% (pH 7.4). After centrifugation (6000g, 15 min, 4 °C), the isolated synaptosome was re-suspended in a Krebs–Ringer–HEPES solution (KRH) without CaCl2 (124 mM NaCl, 4 mM KCl, 1.2 mM MgSO4, 10 mM glucose, 25 mM HEPES, pH 7.4, 10 mg/ml), and centrifuged (6000g, 15 min, 4 °C). The Pellet was obtained, centrifuged (3.333g, 60 s), re-suspended in KRH, and incubated at 37 °C per 30 min. This process was repeated once more and synaptosome aliquots were immediately led for reading and quantification.
Measurements of glutamate release
Glutamate release was indirectly quantified by a fluorescent method44. Fluorescence quantification was measured using a fluorimeter (Synergy TM2, Biotek®). Excitation and emission wavelengths were recorded at 360 nm and 450 nm, respectively. Isolated nerve terminals were incubated with CaCl2 (1 mM), and NADP+ (1 mM) in KRH medium (2 min). Glutamate dehydrogenase (Sigma Aldrich®; 50 units per well) was added to each well, and readings were performed until the fluorescence reached balance (5 min). KCL 33 mM was used as a depolarizing stimulus (10 min). Finally, calibration curves were obtained after standard amount of glutamate (Sigma Aldrich®; 5 nM/μL) was added to the medium (5 min). Glutamate levels were normalized to the total amount of synaptosomal protein that was obtained through Bradford assay.
Real-time PCR
RNA was isolated from the hippocampal samples with TRIZOL reagent® (Invitrogen, Burlington, EUA) in accordance with manufacturer instructions. The RNA concentration and quality were determined by spectrophotometer lecture (NanoDropTM (Thermo Scientific, Wilmington, USA). cDNA was prepared from 500 ng of the isolate RNA through reverse transcriptase reaction using 300 ng of random primers. Quantitative PCR was performed with specifc primers and Power SYBR® Green PCR Master Mix kit (Thermo Scientific, Wilmington, USA) in accordance with manufacturer instructions and QuantStudio™ 7 Flex Real-Time PCR System were employed for execution of the qPCR, as well as data analysis. Specific primers sequence of the target genes (AMPA: GLUR2; NMDA: NR1, NR2A, NR2B; mGluR5: Grim5, GLT-1:SCLA2), BBB proteins [Claudin-5, Occludin, Zoocludin-1(ZO-1)], cytokines and chemokines (IL-1β, IL-6, TNF-α, INF-ɣ, CX3CL1, and CX3CR1), as well synaptic plasticity factors [Synaptophysin: SYP, postsynaptic density protein 95 (PSD-95): DLG4, and activity-regulated cytoskeleton-associated protein (ARC)] were designed with Primer3plus software and validated with NCBI Primer-BLAST (Supplementary data, Table S1). Samples were prepared in triplicate and gene expression variations were determined by the ΔCt method using the RPL32, as a constitutive normalizing gene. In the case of cytokines, the mean of two normalizing genes was used by the ΔCt calculation: GAPDH and HPRT.
Evaluation of neurotrophic factors, fractalkine, and cytokine levels
In order to measure the levels of neurotrophic factors (BDNF, NGF, GDNF), fractalkine (CX3CL1), serum leptin, and inflammatory cytokines (IL-1β, IL-6, TNF-α, INF-ɣ), in the serum and hippocampus, an ELISA assay was performed. An cold extraction solution (100 mg of tissue per milliliter), containing Tris–HCl (20 mM); NaCl (137 mM); NP40 (1%); Glycerol (10%); phenyl methyl sulfonylfluoride (1 mM) or aprotinin A (0.5 µg/mL), Pesptatin A (1 μM), EDTA (10 mM), E-64 (10 μM), sodium vanadate (0.5 mM), and deionized water was added to hippocampus samples. Samples were mechanically processed, and centrifuged (14,000 rpm, 4 °C, 20 min). The hippocampal supernatant and serum samples were stocked at −80 °C until use. The levels of all interesting targets were measured using commercial kits from R&D system (DuoSet, Minneapolis, MN) in accordance with manufacturer instructions. Results were acquired on a spectrophotometer and expressed as pg/mL or pg/100 mg of tissue.
Statistical analysis
Statistical analyses were performed using the graphpad prism software 8 (San Diego, USA). The normality and homoscedasticity of the data were tested using Shapiro–Wilk and Levene's test, respectively. Outliers were detected via the box-plot interpolation method. Data were expressed by mean ± SEM. Furthermore, as appropriated, unpaired test-t, Mann–Whitney test, repeated measures ANOVA, two-way ANOVA, and mixed effect model, followed by Tukey post hoc test were employed. In addition, in ORT and OLT we also used a one-sample T-test for comparing the experimental control means with a hypothetical mean of 0.5 (different from random)45. The level of statistical significance adopted was p < 0.05.
Results
HSB diet induces obesogenic phenotype and metabolic abnormalities
Our results showed a significant time × diet interaction effect, associated with a gradual increase of body weight in our DIO model (two-way ANOVA, F11, 456 = 15, 42, p < 0.0001) (Supplementary data, Fig. S2A, B). Furthermore, the HSB group presented a higher adiposity index (unpaired T student-test, t18 = 5.832, p < 0.0001), increased lee index (unpaired T student-test, t18 = 2.330, p = 0.0316), and elevated cumulative energy intake (unpaired T student-test, t10 = 7.639, p < 0.0001) (Supplementary data, Fig. S2C–F), all pointing out to a possible alteration in body composition caused by the increase of palatable diet consumption. Regarding metabolic dysfunction, a chronic exposure to HSB diet induced higher fasting glucose levels (unpaired T student-test, t18 = 3.548, p = 0.0023) (Supplementary data, Fig. S2G), and increased oral glucose intolerance (unpaired T student-test, area under curve (AUC) t18 = 3.117, p = 0.0052) (Supplementary data, Fig. S2H–I). Additionally, elevated levels of total cholesterol were observed (Mann–Whitney test, total cholesterol, p = 0.0002) (Supplementary data, Fig. S2J). Taken together, these data suggest that the HSB diet was effective in inducing obesity features, which is in accordance with previous literature11.
HSB diet impairs the process of memory reconsolidation and extinction
To investigate possible memory impairment in our DIO model, we first assessed whether the chronic exposure to an obesogenic diet was able to induce changes in the exploratory behavior, and short-term memory. For that, the open field and Y maze test were performed, respectively (Supplementary data, Fig. S3 and Fig. 1A). We observed that in both behavioral tests, none of the investigated parameters were affected by the HSB diet (Open field: unpaired T student-test, Total traveled distance t16 = 0.4205, p = 0.6797, mean speed t16 = 0.4873, p = 0.6327; Mann–Whitney test, time in center, p = 0.1359. Y maze: unpaired T student-test, alternation index t18 = 0.06189, p = 0.9513) (Supplementary data, Fig. S3, and Fig. 1B). Next, in order to evaluate the impact of HSB diet in events associated with hippocampus-dependent long-term memories, mice were subjected to the ORT, OLT, or contextual fear conditioning (Fig. 1C, F). Notably, HSB diet was able to reduce the total investigation time in ORT and OLT, which may suggest a decline in episodic memory (Unpaired t-test, Total investigation time: ORT t18 = 2.731, p = 0.0137; and OLT t16 = 2.315, p = 0.0342) (Fig. 1D, E). Although memory retrieval was similar in both groups (unpaired t-test: memory evocation test, t14 = 1.612, p = 0.1292) (Fig. 1G), we observed that the obese group presented an abnormal extinction curve, besides an increased freezing percentage in the extinction test as compared to the lean group (two-way ANOVA, memory extinction curve: F1, 56 = 30.06, p < 0.0001; unpaired t-test: memory extinction test, t15 = 4.417, p = 0.005) (Fig. 1H, I). Therefore, this dataset may suggest that HSB diet is able to impact specific memory events, such as extinction. Finally, to determine whether the long-term memory impairment promoted by the HSB diet may impact social skills, we conducted some assays to verify social interaction and social memory (Supplementary data, Fig. S4A, D). First, our preliminary data showed that HSB diet was not able to decrease social interaction and social memory index (Mann–Whitney test, social interaction index, p = 0.1481; unpaired t-test, social memory index t18 = 0.3997, p = 0.6941) (Supplementary data, Fig. S4B, C). Furthermore, in the single chamber social interaction test, we observed that similarly to the lean group, the HSB group showed a decrease in the raw interaction time with familiar juvenile rats in the STM, and a tendency to decrease the interaction in the LTM assessment tests (one-way repeated measure, STM, p = 0.0094; LTM, p = 0.0678) (Supplementary data, Fig. S4E). Interestingly, this pattern was also corroborated with the percentage of STM and LTM, that remained unchanged in the HSB group, suggesting that social skills and social memory were not affected by the obesogenic environment (unpaired t-test, STM index t16 = 0.08577, p = 0.9327; LTM index t16 = 1.378, p = 0.1872) (Supplementary data, Fig. S4F, G).
Hippocampal neuroinflammation is not associated with chronic consumption of HSB diet
Considering the hypothesis that an increased peripheral inflammatory environment may impair BBB permeability, contributing to glial reactivity, and consequently to memory decline, through neuroinflammatory mechanisms12, we decided to investigate whether obesity induced by HSB diet could modulate serum leptin levels, likewise the pattern of peripheral and hippocampal pro-inflammatory cytokines, microglial and astrocyte reactivity, as well as the expression of proteins associated with BBB integrity (Figs. 3A and 6A). The results showed that in the periphery, HSB diet did not impairs the levels of IL-1β, IL-6, and TNF-α, but increased leptin levels, and INF-ɣ concentrations in the serum (Unpaired t-test test, IL-1β t15 = 0.9297, p = 0.3672; IL-6 t16 = 2.066, p = 0.0593; TNF-α t10 = 1.843, p = 0.0951; leptin t9 = 12.01, p < 0.0001; and INF-ɣ t18 = 2.334, p = 0.0314) (Fig. 2). Nonetheless, this fact was not observed in the hippocampus, where mRNA expression of inflammatory genes as well as protein levels of the cytokines evaluated remained unchanged in the HSB group (RT-PCR: Unpaired t-test test, IL-1β t11 = 0.007761, p = 0.9939; IL-6 t12 = 0.2917, p = 0.7755; TNF-α t12 = 0.8585, p = 0.4074; Mann–Whitney test, INF-ɣ, p = 0.2593; ELISA: IL-1β t8 = 0.0004175, p = 0.9997; IL-6 t8 = 0.4157, p = 0.6885; TNF-α t8 = 1.587, p = 0.1511; and INF-ɣ t8 = 1.985, p = 0.0824) (Fig. 3B–I). In accordance with these data, the comparison between Iba-1 optical densities, cell body to cell size ratio, as well as GFAP fluorescence intensity and percentage of GFAP stained area did not reveal significant differences between lean and obese groups (microglial optical density: unpaired t-test test, DG t14 = 0.1013, p = 0.9192; CA1 t14 = 0.1171, p = 0.9084; CA2–CA3 t13 = 0.6522, p = 0.5257; Microglial body to cell size ratio: Unpaired t-test test, DG t14 = 0.08705, p = 0.9319; Mann–Whitney test, CA1, p = 0.9329; CA2–CA3, p = 0.3282; GFAP fluorescence intensity: Mann–Whitney test, DG, p = 0.6991; unpaired t-test test, CA1 t10 = 0.3422, p = 0.7393; CA2–CA3 t10 = 0.7844, p = 0.4510; GFAP stained area: Mann–Whitney test, DG, p = 0.3095; unpaired t-test test, CA1 t10 = 0.3420, p = 0.7394; and CA2–CA3 t10 = 0.7843, p = 0.4510) (Figs. 4 and 5). Finally, HSB diet was not able to modulate the mRNA levels of Claudin-5, occludin, and ZO-1 levels, which suggest the regular maintenance of hippocampal BBB integrity in the obese mice group (unpaired t-test test, Claudin-5 t17 = 0.7456, p = 0.4661; Occludin t17 = 0.2230, p = 0.8262; and ZO-1 t18 = 0.9340, p = 0.3627) (Fig. 6B–D). Therefore, this dataset may suggest that the inflammatory features in our DIO model are present only in the periphery, and likely are not associated with the development of a hippocampal neuroinflammatory process.
Chronic consumption of HSB diet promotes an increase in hippocampal glutamate release
In order to verify the impact of the obesogenic environment on glutamatergic neurotransmission, we started our investigation by measuring hippocampal glutamate levels (Fig. 7). Notably, HSB diet increases hippocampal glutamate levels (Unpaired t-test test, hippocampal glutamate t17 = 4.003, p = 0.0009) (Fig. 7B). Considering this, we decided to evaluate whether the increase of glutamate levels in the obese group might be associated with dysfunctional expression of AMPA and NMDA receptors by the quantification of functional subunits, respectively, GluR2, NR1, and NR2A/NR2B, as well the mRNA expression for mGluR5. Interestingly, our findings did not show remarkable differences between the diet groups (Unpaired t-test test, GluR2 t18 = 0.9338, p = 0.3627; NR1 t17 = 0.3773, p = 0.7106; NR2A t17 = 0.8998, p = 0.3808; mGluR5 t18 = 1.102, p = 0.2851; Mann–Whitney test, NR2B, p = 0.6305) (Fig. 7C–G). Finally, in order to evaluate whether excess of glutamate promoted by HSB diet was able to impair glutamatergic clearance in the synaptic cleft, we also quantify the mRNA levels of astrocyte glutamate transporter (GLT-1). Interestingly, we did not find alterations in the comparison between groups (Unpaired t-test test, GLT-1 t17 = 0.01760, p = 0.9862) (Fig. 7H).
HSB diet up-regulates fractalkine but does not alter levels of neurotrophic factors and pre/post-synaptic plasticity proteins in the hippocampus
The Fractalkine/CX3CR1 axis is associated with microglia and neuronal crosstalk by regulating synaptic plasticity and glutamatergic neurotransmission, which provides implications in several pathological conditions of memory46. In addition, neurotrophic factors, pre/post synaptic proteins, as well as glutamate levels interact with each other to regulate neuroplasticity, providing a key role in memory regulation26,47. Thus, we decided to conduct a preliminary investigation, a posteriori, to elucidate whether the obesogenic environment associated with HSB diet might cause alterations in the Fractalkine/CX3CR1 axis, besides in the levels of neurotrophic factors, and pre/post synaptic proteins associated with memory regulation and plasticity (Fig. 8A). For this, we measured hippocampal levels of fractalkine, CX3CR1, BDNF, NGF, GDNF, synaptophysin, PDS-95 and ARC (Fig. 8B–J). Our results showed that mRNA levels of fractalkine and CX3CR1 were unaffected by HSB diet (Unpaired t-test test, Fractalkine t18 = 0.6510, p = 0.5233; Mann–Whitney test, CX3CR1, p = 0.6842) (Fig. 8B, C). However, we observed that hippocampal fractalkine protein levels were up-regulated in obese mice (unpaired t-test, t16 = 2.451, p = 0.0399) (Fig. 8D). Regarding neurotrophic factors, synaptophysin, PSD-95, and ARC, our preliminary data reveal no changes in any of the markers assessed (ELISA: unpaired t-test test, BDNF t8 = 0.7803, p = 0.4577; Mann–Whitney test, NGF, p = 0.5476; and GDNF, p = 0.4857; RT-PCR: unpaired t-test test, Synaptophysin t17 = 0.8716, p = 0.3956; PSD-95 t8 = 0.6794, p = 0.5060; ARC t17 = 0.7103, p = 0.4871) (Fig. 8E–J).
Discussion
The main idea of this work was to understand how an obesogenic inflammatory environment associated with prolonged consumption of a highly palatable/ energy-dense diet, may impact central neurotransmission and its functionality. For that, we have demonstrated that chronic exposure to HSB diet promotes hippocampal-dependent memory impairment and increases glutamate levels in the hippocampus of obese mice. Although we observed elevated levels of peripheral inflammatory markers typical of obesity, such as leptin, and INF-ɣ, in the hippocampus we did not observe damage to the integrity of the BBB or neuroinflammatory features associated with exposure to an obesogenic diet, which overturned our hypothesis that increased glutamate levels in the hippocampus could be associated with hippocampal neuroinflammatory mechanisms triggered by obesogenic peripheral inflammation (Figs. 2, 3, 4, 5 and 6). In this milieu, highly palatable/ energy-dense foods are strongly associated with glucose metabolism impairment and diabetes mellitus type 2 (TDM2)11,48. An interesting study demonstrated that the co-association between obesity and TDM2 was able to reduce the molecular carbon labeling of glutamate in the hippocampus and cortex, which could be associated with decrease in glucose metabolism in the tricarboxylic acid (TCA) cycle, generating biochemical dysfunctions in glutamate production48. In accordance with that, exposure to a high-fat or high fat-sucrose diet may decrease glutamine synthase activity, glutamate/glutamine levels, and up-regulate GLT-1 expression and activity, which may suggest that these dietary components by themselves, could impact glutamate metabolism33,34. Considering that glutamatergic recycling is a process that requires a large energy input, it is possible that the increase of GLT-1 expression and/or activity acts as a compensatory mechanism in order to improve the glutamatergic recycling efficiency and also vesicular glutamate levels in a metabolic failure scenario33,34,49. However, it is important to note that it has been suggested that the GLT-1 clearance efficiency tends to decrease gradually after persistent metabolic dysfunctions or increased neuroinflammation, which may predispose to glutamatergic excitotoxicity and memory decline32,49. Therefore, considering that in similar DIO studies with a shorter diet exposure time, as well as the fact that the HSB diet induces a metabolic impairment without affecting GLT-1 expression (Fig. 7H and Fig. S2), we hypothesized that the increase in hippocampal glutamate levels may be a result of an earlier GLT-1 compensatory mechanism due to the persistence of metabolic failure (Fig. 9).
It has been reported that increased glutamate levels are associated with impairment in synaptic plasticity, including abnormal formation of LTP and long-term depression (LTD), in a mechanism involving overactivation of ionotropic and metabotropic receptors, increased Ca+2 signaling, decreased production of neurotrophic factors, synaptic proteins, among others25,26,50. Interestingly, in DIO models, LTP and LTD phenomena are decreased in CA1-CA3 region, which may be associated with acquisition and reconsolidation dysfunctions of aversive and episodic memory, suggesting that an obesogenic environment may increase the vulnerability to a poor synaptic plasticity regulation and cognitive impairment45,51. Although none of these studies evaluated whether decrease in synaptic plasticity and memory were associated with glutamatergic neurotransmission, it has been demonstrated that HFD promotes a downregulation of NMDA hippocampal NR2B subunit, which may lead to dysfunctions in synaptic plasticity dependent on LTD, likely contributing to plastic decline regulation in an obesity environment34. Here, we did not observe changes in the levels of expression of NMDA and AMPA subunits, as well as other classical receptors that also may contribute to the regulation of LTP and LTD, such as mGluR5 (Fig. 7C–G). However, we cannot rule out the possibility that the functional pattern of these receptors may be altered. In this context, it is well known that the saturation of iGluR activity, due to high glutamate levels, can disrupt the formation of new LTP and LTD patterns, contributing to the weakening of reinforcing traces of memories, new memory encoding, and learning52,53. Interestingly, our behavior dataset suggest that the main deleterious effects of the HSB diet is concentrated on processes associated with the reinforcement of consolidated memories, in the case of ORT and OLT, and new learning (memory extinction) (Fig. 1D–E, H, I). Thus, although we did not assess the hippocampal pattern of LTP/LTD, which is an important limitation of our work, we hypothesized that increased glutamate levels might induce the saturation of glutamatergic receptor activity, promoting an impairment of synaptic plasticity, as well as limiting the plastic capacity of the hippocampal network, which could impair signal transduction associated with refinement and extinction of an acquired memory. Nevertheless, the absence of behavioral changes observed in the Y maze test, aversive memory evocation, and social recognition suggests that possibly primary memory processes such as acquisition, consolidation, and retrieval could still be preserved (Fig. 1B, G, and Fig. S4). Although speculative, we believe that two alternatives might support this phenomenon: (I) Impairment of synaptic plasticity, promoted by the elevation of glutamate levels is not strong enough to saturate the signal transduction associated with acquisition and consolidation. However, increased glutamate levels can limit consolidated circuits and the full acquisition of new information relative to a familiar context. (II) Compensatory systems may be attempting to partially protect hippocampal circuitry from the potentially deleterious effects of increased glutamate levels on plasticity (Fig. 9).
Fractalkine, a chemokine abundantly produced by neurons, belonging to the CX3C chemokine family, acts in several synaptic plastic processes and also contributes to memory and learning in physiological conditions54,55. Furthermore, the effects of fractalkine-CX3CR1 signaling have been pointed out as a potential neuroprotective path in conditions associated with neurotoxicity and memory decline, such as Alzheimer´s and Parkinson´s disease56,57. In this sense, in vitro experiments showed that increased hippocampal fractalkine levels are associated with neuroprotective effects against glutamatergic excitotoxicity in a mechanism that involves the reduction of postsynaptic AMPA-evoked currents, increased expression of synaptic NR2A/NMDA, activation of survivor pathways, and production of neurotrophic factors, such as BDNF58,59,60. Moreover, it was demonstrated that CX3CR1 expression in hippocampal neurons mediated the neurotrophic effects of fractalkine in a viral neurotoxicity model61. Interestingly, in a murine model for Alzheimer's disease, it was reported that the overexpression of fractalkine reversed the decline in hippocampal synaptophysin62. Furthermore, lower levels of fractalkine-CX3CR1 signaling in the hippocampus of obese or lean mice treated with a CX3CR1 antagonist are associated with decreased levels of PSD-95 and cognitive deficits18. Importantly, we observed that HSB diet exposition can increase hippocampal fractalkine levels, but did not change the concentration of neurotrophic factors, as well as the mRNA expression of synaptophysin, PSD-95, and ARC (Fig. 8). Perhaps this fact is due to neuroprotective fractalkine effects in response to increased glutamate levels, which could be evidence in favor of the compensatory neuroprotective hypothesis previously raised. It is also important to point out that although we observed an increase in the protein levels of fractalkine, the expression of fractalkine mRNA remains unchanged in HSB group (Fig. 8). This is in accordance with in vitro reports, where glutamate-induced neurotoxicity did not affect fractalkine gene expression but increases soluble fractalkine levels, which may indicate that the neurotoxic environment may promote fractalkine cleavage from the neuronal membrane63. Interestingly, although fractalkine can signal as a membrane-bound protein or a soluble fragment, some studies suggest that the soluble form is more associated with neuroprotective effects57,64. Therefore, we hypothesize that the increased levels of fractalkine may be an attempt to limit a possible hippocampal synaptic damage promoted by glutamate (Fig. 9). However, further experiments including the molecular investigation of survival and cell growth pathways modulated by fractalkine may help to support this hypothesis.
It is critical to underscore the limitations of our work. Firstly, due to our focus on a single time point, our current dataset lacks the ability to establish definitive conclusions about the connection between glutamatergic dysfunction and neuroinflammation. While in this study we observed higher glutamate levels in the hippocampus, this elevation might be the outcome of a process not directly linked to neuroinflammation but rather related to metabolic dysfunction, as hypothesized earlier. However, due to the limitations of our experimental design, we cannot ascertain whether the absence of neuroinflammation was a result of a previous neuroinflammatory process or a subsequent response to increased glutamate levels in the hippocampus. It remains uncertain whether a potential neuroinflammatory process could be initiated independently of peripheral inflammation. Taking this into consideration, it is important to point out that the chronology of neuroinflammation in obesity is still poorly known, and that the initiation of this phenomenon appears to be related with a non-linear temporal dynamics based on a variety of circumstances, including the ingredients and centesimal composition of the diets, duration of diet exposure, as well as the age of onset of dietary exposure65,66,67,68. In this milieu, a study pointed out that a short-term exposure to a HFD 60%, from 2 to 7 days, was associated with a decrease in synaptophysin expression, increase in TNF-α, IL-6 levels, astrocyte reactivity and BBB permeability in the hippocampus, suggesting that this region may be quickly affected by damage induced by highly palatable and energy-dense foods69. Furthermore, emerging evidence suggests that post-weaning exposure to a HFD containing 60% of calories from fat, 20% from protein, and 20% from carbohydrates for duration of 6 weeks can induce neuroinflammatory features. Additionally, this HFD regimen has been associated with reduced levels of GLUA1 and GLUA2, which are important subunits of the AMPA receptors67. Moreover, the enduring impact of alterations in this setting may have long-term consequences, as it can lead to sustained high levels of glutamate, decrease the expression of vesicular glutamate transporter (vGLUT), trigger ongoing astrocyte reactivity in the hippocampus, and result in memory impairment70. Interestingly, in an intriguing study conducted over a span of eight weeks, researchers implemented a diet closely resembling to ours. Notably, the results revealed no significant alterations in dendritic spine density, neuroinflammation, or glutamate dysfunction within the hippocampus. Nevertheless, the authors reported that this HFD was able to induce cognitive decline along with all the aforementioned molecular dysfunctions in the prefrontal cortex6. Thus, while our findings are not conclusive, it is tempting to suggest that prolonged exposure to HSB diet might cause acute neuroinflammation in the hippocampus which may predispose to late changes in glutamatergic signaling. Nonetheless, the absence of studies examining the kinetics of hippocampal neuroinflammation associated with an obesogenic environment leaves us with insufficient concrete evidence to speculate on this possibility. Furthermore, it is essential to consider that several other brain structures implicated in memory processes, including the cortex, cerebellum, and amygdala, can also experience neuroinflammatory states as a result of both short-term and long-term exposure to a poor diet6,42,65. Also, we must recognize that other brain regions might indeed exhibit neuroinflammatory and glutamatergic signaling changes consistent with our initial hypothesis. However, it is important to emphasize that such possibilities extend beyond the limits supported by the data we have gathered in our study. Other important limitations of our study are the facts that we did not demonstrate whether the pattern activity of iGluR was affected by the obesogenic environment, and whether our DIO model presented damages in potential molecular pathways linked to neurotoxicity, which makes it difficult to understand potential changes associated with plastic mechanisms. Finally, we did not measure parameters such as sex-specific differences as well as molecular pathways associated with the neuroprotective effect of fractalkine. Thus, a deeper investigation of the plastic electrophysiological parameters, pathways associated to glutamate-fractalkine signaling, neuroinflammatory kinetics, and sex differences, is needed in order to elucidate the nature of these highlights.
Data availability
The datasets generated during and/or analyzed during the current study are available from the corresponding author on reasonable request. Drawings: All drawings were manually performed using the inkscape software (https://inkscape.org/about/overview/).
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Acknowledgements
The authors would like to thank the Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES) for the fellowship support. We also thank the staff of the Center for Image Acquisition and Processing (CAPI) for all their support and use of infrastructure for the microscopy and fluorimetric assay. We acknowledge Rinaldo do Nascimento, Webster Glayser Pimenta dos Reis, and Gislene Gomes da Rocha for the technical support.
Funding
This study was supported by the Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq), Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES), Programa de Apoio à Pós-graduação (PROAP-CAPES), Pró-reitora de Pesquisa da UFMG (PRPq), Fundação de Amparo à Pesquisa do Estado de Minas Gerais (FAPEMIG).
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R.R., L.B.V. and A.C.P.O. designed the study. R.R. performed most experiments. R.R., G.R.C., B.S.R.S., M.C.M.S., and L.O.G. executed the behavioral experiments. E.G.S. and F.C.M. performed and analyzed RT-PCRs. R.R., and H.B.F. performed Elisa. R.R., C.O.S., C.N.F., and V.L. performed the metabolical characterization. R.R., B.S.R.S., G.R.C., and C.S.O. performed imunofluoresce, and imunohistochemistry experiments. Microscopy analysis was performed by R.R. and G.F.G. R.R. and L.B.V. executed and analyzed synaptossome data. Statistical analysis was performed by R.R. The article was written by R.R. and L.B.V. The drawings, tables, schemes, and figures were made by R.R. G.F.G., F.M.R., G.S.P.M., A.M.C.F., T.U.M., A.S.M., and A.C.P.O. made substantial contributions to conception and design of the study and critically revised the manuscript for important intellectual content. All other authors revised the data and discussed the manuscript.
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Ribeiro, R., Silva, E.G., Moreira, F.C. et al. Chronic hyperpalatable diet induces impairment of hippocampal-dependent memories and alters glutamatergic and fractalkine axis signaling. Sci Rep 13, 16358 (2023). https://doi.org/10.1038/s41598-023-42955-9
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DOI: https://doi.org/10.1038/s41598-023-42955-9
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