Animals

Experiments were carried out on young adult (2 months) male Wistar rats born in our local animal care facilities (Unité Expérimentale d'Infectiologie Expérimentale des Rongeurs et Poissons (UEIERP), Jouy-en-Josas, France). All animal experiments were conducted in accordance with the European Communities Council Directive of November 24, 1986 (86/609/EEC). P.C. and C.B. hold the Individual Authorization for Performing Experiments in Animals, including the animals experiments conducted in the present study, provided by Préfecture des Yvelines (France), according to French and European laws (agreements #78–154 and #78–65). All surgery was performed under sodium pentobarbital anesthesia, and all efforts were made to minimize the number and suffering of used rats.

They were kept under controlled conditions of light (12 h light and 12 h dark, lights on at 07∶00) and temperature (22°C) with free access to pellet food (M25, Dietex, Saint-Gratien, France) and tap water. To determine the effect of fasting, food but not water was withheld for 14 h before tests. For all experiments, rats were killed at the beginning of the light phase (09∶00–10∶00) by decapitation.

Electro-olfactogram (EOG) recording

EOG recordings were made from the OM in an opened nasal cavity configuration, on rat hemi-heads. Immediately after decapitation, the head was cut longitudinally and the nasal septum was removed from one hemi-head to expose the endoturbinates from which EOG recordings were performed at room temperature (Fig. 1A). The OM tissue was simultaneously dissected from the contralateral hemi-head and stored at −80°C for subsequent western blot analysis (see below).

The EOG recordings were done using an experimental design described earlier [14]. The hemi-head was placed in a recording chamber on a custom-designed platform (Siskiyou, Inc., Grants Pass, OR, USA) of an upright Olympus BX51WI microscope (Olympus, Rungis, FRANCE) equipped with a low magnification objective (4x) and MPC-325 motorized micromanipulators (Sutter Instruments, Novato, CA, USA). The odor stimulation device was modified from Scott and Brierley [46]. The hemi-head was kept under a constant flow of humidified filtered air (∼1200 ml/min) delivered close to the endoturbinates through a 9 mm glass tube (Fig. 1A (a)). This tube was positioned 2 cm from the epithelial surface and was centered on the recorded endoturbinates. Odor stimulations were performed by blowing air puffs (100 ms, 300 ml/min) through an exchangeable Pasteur pipette (Fig. 1A (b)) enclosed in the glass tube and containing a filter paper impregnated with 20 µl of the odorant, isoamyl acetate (IA; Sigma Aldrich (Saint-Quentin Fallavier, France)), diluted 1: 100 in DMSO. To prevent variable accumulations of the odorant in the pipette, an air flush was applied to the Pasteur pipette before it was placed in the glass tube and before each subsequent odorant application.

EOG voltage signals were recorded using an Multiclamp 700B patch-clamp amplifier (Axon Instruments, Molecular Devices, Union City, CA, USA) used in a DC current-clamp configuration (I = 0), low-pass bessel filtered at 1 KHz and digitized at a rate of 2 kHz using an Digidata 1322a A/D converter (Axon Instruments, Molecular Devices, Union City, CA, USA) interfaced to a Pentium PC and Pclamp 9.2 software (Axon Instruments). A reference Ag/AgCl electrode was placed on the frontal bone overlaying the olfactory bulb. Recordings were made with glass micropipettes of 4–5MΩ filled with a mucosal saline (MS) solution (45 mM KCl, 20 mM KC₂H₃O₂, 55 mM NaCH₃SO₄, 1 mM MgSO₄, 5 mM CaCl₂, 10 mM HEPES, 11 mM glucose, 50 mM mannitol, pH 7.4, 350 mOsm adjusted with mannitol). The composition of this solution was chosen to match the composition of mucus as closely as possible, according to previous studies [47]. Simultaneous EOG recordings of the responses evoked by isoamyl acetate, were recorded from the neighboring endoturbinates II_b and III. The recording electrodes were placed in the center of these endoturbinates (Fig. 1A). This position gave robust, reproducible and long-lasting EOG recordings ranging from 10 to 30 mV in response to IA. Odorant-free air stimulation, or stimulation with DMSO alone, always produced signals of less than 1 mV amplitude.

EOG responses were recorded until their amplitudes stabilized, (i.e. at least 3 successive responses displaying the same amplitude), and the last response was taken as the reference. One endoturbinate was treated by a local application of the mucosal saline solution (MS), while the other endoturbinate received the same MS containing the tested peptide (1 µM NPY or NPY-receptor agonist). Droplets of approximately 1 µl of the solution were delivered by capillarity onto the recorded area of endoturbinates II_b or III (respectively white and grey circles in Fig. 1A) using glass micropipettes (∼5 µm in diameter). One droplet covered about 1–2 mm diameter of the olfactory mucosa on a given endoturbinate, as checked under the microscope. MS and peptide-containing-MS treatments were systematically shifted between the two endoturbinates (II_b and III) from one rat hemi-head to the other. Responses to IA were then recorded on each endoturbinate every 5 min, for 30 min following local treatment (Fig. 1A). The effect of NPY was compared between fed (n = 10 rats) and fasted (n = 10 rats) rat hemi-heads, whereas the effects of NPY-receptor agonists were studied in overnight-fasted rat hemi-heads (n = 10, 5 and 10 rats, respectively for Y₁, Y₂ and Y₅ receptor agonist). Analysis were performed off-line using Clampfit 9.2 (Axon Instruments). Peak amplitude, rise time (from 10% to 90%), fast (from 100% to 50%) and slow (from 40% to 10%) decay slopes of EOG responses were measured. Since the EOG response decay kinetics highly correlate with the amplitude, the two decay slopes were normalized to the corresponding response peak amplitude prior to statistical analysis. The amplitude and kinetics of the olfactory signals recorded following the local peptide applications were normalized to those of the control responses prior to this treatment.

Y₁R Western blotting

In order to quantify Y₁R protein, the OM tissue dissected from fed (n = 5) and fasted (n = 11) rat hemi-heads was homogenized in a volume of extraction buffer (25% glycerol, 0.42 M NaCl, 1.5 mM MgCl₂, 0.2 M EDTA, 20 mM Hepes; pH = 7.5) containing 1∶100 of phenyl-methylsulphonyl fluoride (PMSF), 1% Nonidet-P-40 and 1∶25 of a cocktail of anti-proteases (Complete; Roche Diagnostics, Meylan, France). These tissue extracts were then centrifuged at 16000 g for 20 min, the supernatants were collected and protein levels quantified using BCA protein assay (Pierce, Perbio Science, Brébières, France). To test for the presence of Y₁R, we performed an 8% SDS-PAGE analysis of boiled aliquots (75 µg of total proteins) from each extracts. Following electrotransfer, membranes were blocked with 4.5% nonfat milk and then incubated overnight at 4°C with a rabbit polyclonal Y₁R antibody (ab 73897; 1∶500; Abcam, Cambridge, UK) or a mouse monoclonal β-actin antibody (chosen as the reference protein) (A5441; 1∶3000; Sigma Aldrich, Saint-Quentin Fallavier, France). After extensive washing in PBS-0.5% milk (4×15 min each), the membranes were incubated with horseradish peroxidase-conjugated anti-rabbit secondary antibody (1∶5000; Sigma Aldrich, Saint-Quentin Fallavier, France). The targeted proteins were detected using an ECL western blotting detection kit (Amersham Biosciences, Orsay, France). The integrated density of protein level of each band on the blots was determined by densitometry using ImageJ software (free Java port of NIH image, http://rsb.info.go/ij/).

Immunohistochemistry (IHC)

Fed (n = 4) and fasted (n = 5) rats were deeply anaesthetized with sodium pentobarbital (CEAV, Libourne, France; 100 mg/kg) and perfused transcardially with 200 ml saline and then with 300 ml of a freshly prepared fixative solution of 4% paraformaldehyde in 0.1 M phosphate-buffered saline (PBS). The skull was opened and the brain was carefully dissected. The bones of the skull were discarded from the lateral and dorsal walls of the nose and the olfactory mucosa (septum and turbinates) with the olfactory bulb were removed as a block. Tissues were post-fixed in the same fixative for 3 h at room temperature, cryoprotected with saccharose (30%) and cut using a cryostat into 14 μm thick serial horizontal sections. The slide-mounted sections were stored at −80°C until use. Upon request, tissue sections were rehydrated with three PBS washes. In order to block endogen peroxidase, the sections were treated at room temperature with 1% H₂O₂ for 30 min. The non-specific binding sites were blocked for 30 min at room temperature with a non-immune serum issued from the host species of the secondary antibody (usually 1∶10 normal goat serum in PBS containing 0.25% Triton X-100, and 2% bovine serum albumin). Sections were then incubated with the primary antibody in Triton (0.05%) – BSA (0.2%) –1∶10 normal goat serum – PBS for 48–72 h at 4°C. A polyclonal antibody raised in rabbit was used to localize Y₁R in the OM (ab 73897, 1∶250, Abcam, Cambridge, UK). A monoclonal antibody raised in mouse was used to localize β-tubulin isotype III (clone SDL.3D10, 1∶200, Sigma Aldrich, Saint-Quentin Fallavier, France). Controls were performed using incubation with non-immune serum in place of the primary antibody; no immunostaining was observed when the primary antibodies were omitted. After washes in PBS, labeling was visualized using secondary antibodies conjugated either with fluorochrome (Alexa-Fluor-488- and Alexa-Fluor-546-conjugated secondary antibodies, raised in goat, Molecular Probes, Invitrogen, Cergy Pontoise, France, 1: 1000, 1 h at room temperature) or biotin revealed with a biotin–avidin–peroxidase kit (Vectastain ABC Kit, Vector Laboratories, AbCys, Paris) using diaminobenzidine (DAB) as a chromogen in presence of H₂O₂ and nickel ammonium sulfate (DAB substrate kit for peroxydase, Vector Laboratories, AbCys, Paris). For immunofluorescence detection, preparations were washed in PBS and mounted in DAPI-containing Vectashield (AbCys, Paris, France). For DAB detection, sections were air dried, dehydrated in ethanol, cleared in xylene and mounted in DePeX (GURR, Labonord, Villeneuve d'Ascq, France).

Images processing

IHC images were acquired either on a DMBR Leica microscope equipped with an Olympus DP-50 CCD camera using Cell^F software (Olympus Soft Imaging Solutions GmbH, OSIS, Münster, Germany), or on an AxioObserver.Z1 microscope equipped with a structured illumination system (Zeiss Apotome, Oberkochen, Germany) using Axio Vision 4.8 (Zeiss). Apotome observations were made at the Mima2 facilities in Jouy-en-Josas (France). Images were cropped, resized, rotated, merged, and adjusted for contrast and brightness, for presentation purposes, using ImageJ, but their content was not altered in any case.

Chemicals

All chemicals were dissolved in distilled water or DMSO when required. Concentrated stock solutions were kept frozen at −20°C, and diluted extemporaneously to their final concentrations in the appropriate saline solutions. Neuropeptide Y (Human, Rat) Trifluoracetate Salt was purchased from Bachem (Weil am Rhein, Germany). Selective agonists of Y₁ ([Phe7, Pro34] pNPY), Y₂ (Ahx [5]–[24] pNPY) and Y₅ ([Ala31, Aib32] pNPY) NPY receptors subtypes were generously donated by Prof. Dr. Beck-Sickinger from the Institut of Biochemistry in Germany (Leipzig University). A commercial Y₁-receptor agonist ([Leu 31, Pro 34] Neuropeptide Y; NeoMPS, Strasbourg, France) was alternately used to confirm the results obtained with EOG recordings. The rabbit polyclonal anti-Y₁R antibody (ab73897) and the Y₁R immunogen peptide (ab82262) were both purchased from Abcam (Cambridge, UK). All other chemicals were purchased from Sigma Aldrich (Saint-Quentin Fallavier, France).

Statistical analysis

Group data presented in the text and figures are expressed as mean ± standard error of the mean (SEM). For EOG data analysis, we first used a 2-way analysis of variance (ANOVA) to determine the overall significance of the effects of time, MS, NPY or agonist treatments. When the ANOVA indicated a significant effect, post hoc Bonferroni multiple comparison of mean tests was used to determine individual differences between responses at each time considered, and differences over time for each treatment. For western blot analysis, statistical comparisons were performed using the Welch's t-test (intended for use with two samples having unequal variances). A probability value of p<0.05 was used as an indication of significant differences (p<0.05 (*); p<0.01 (**); p<0.001 (***)).

NPY enhances EOG responses in the OM of fasted rats

The potential neuromodulatory role of NPY in the OM was studied using EOG recordings of the responses evoked by an odorant, isoamyl acetate (IA), both in fed (n = 10) and overnight-fasted (n = 10) animals. We compared the effects of NPY and vehicle (mucosal saline solution (MS)) applications on the olfactory responses in each recorded rat hemi-head. Simultaneous EOG recordings of the responses evoked by IA were recorded from the neighboring endoturbinates IIb and III (Fig. 1A). One endoturbinate was treated by a local application of MS (white circle, Fig. 1A), while the other endoturbinate received the same MS containing the tested peptide (1 µM NPY or NPY-receptor agonist; grey circle, Fig. 1A). MS and peptide-containing-MS treatments were systematically shifted between the two endoturbinates (II_b and III) from one hemi-head to the other, in each condition (fed/fasted). Local treatment of the OM with MS did not significantly change the amplitude and the kinetics of IA-induced olfactory responses (Fig. 1B–C) recorded up to 30 min post-treatment. In both fed and fasted animals, the EOG responses amplitudes displayed slight and gradual decrease over time (about 15% within 30 to 45 min of recording), as previously reported [48]. In both fed and fasted animals, two-ways ANOVA analysis showed no significant effect of MS treatment, and no difference between the time-course of the EOG amplitudes observed in both conditions. In fed animals, the local treatment with NPY (1 µM) did not significantly change this slow temporal waning (n = 10; fig. 1B). In contrast, in fasted animals, local application of NPY raised the olfactory responses (n = 10; Fig. 1C). The two-ways ANOVA analysis revealed a significant effect of NPY (p<0.01), significantly different time-courses of the EOG amplitudes between MS and NPY treatments (p<0.01), and a significant treatment x time-course interaction (p<0.01). NPY induced a transient increase of the amplitude of IA-evoked EOG responses, reaching a maximum, around 30% above the corresponding MS-treated EOG amplitudes, 5 min after the application (118.1±3.1% and 86.6±6.4% of control EOG amplitude, respectively in NPY- and MS-treated groups; n = 10; p<0.01), and lasting for up to 15 min. The EOG-amplitudes then, followed the progressive decay observed in the MS treated animals, despite a small but significant rebound at 30 min (n = 10, fig. 1C). In contrast to its potentiating effect on the amplitude, NPY did not modify the kinetics of IA-evoked responses in fasted rats (not shown).

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Figure 3. Y₁ receptor is prominently located in OSNs.

(A) Bright field microscopy images of OM sections from endoturbinates of an overnight fasted rat showing the neuronal localization of Y₁R revealed with DAB (light microscope) at medium (40x) (a and b) and high (100x) (d and e) magnification. Stronger signal was detected in the lower half of the epithelium, corresponding to olfactory sensory neurons (OSNs) (white stars), and in few more basally situated cells (e, black arrowheads). No labeling was observed in control sections incubated with non-immune rabbit serum (c). The dashed line indicates the limit between the olfactory epithelium (OE) and the lamina propria (LP). (B) Immunofluorescence images of OM sections from endoturbinates of an overnight fasted rat showing the neuronal localization of Y₁R (B-a, green) with OSN marker, β tubulin III (B-b, red) by double labeling. Cell nuclei were counterstained with DAPI (B-c, blue). Y₁R expression was observed in β tubulin III-positive OSNs (B-d), more clearly seen at higher magnification (B–e).

https://doi.org/10.1371/journal.pone.0045266.g003

We next aimed to determine the subtype of NPY receptor implicated in this positive modulation of the olfactory responses in fasted rats. While Y₁, Y₂ and Y₅ are the most prevalent NPY receptors in the mammalian brain, Y₁ receptors mediate most of the previously reported actions of NPY in the olfactory system. We thus compared the effects of selective agonists of Y₁, Y₂ and Y₅ receptors [49], [50] to the control MS application on the EOG responses recorded in overnight-fasted rats (Fig. 2). As with NPY, the selective application of Y₁ agonist [Phe7, Pro34] pNPY (1 µM; [51]) induced a significant transient increase of the amplitude of IA-induced EOG in overnight-fasted rats, reaching a maximum, around 25% above the corresponding MS-treated EOG amplitudes, 5 min after the application (108.7±6.3% and 85.5±2.8% of control EOG amplitude, respectively in Y₁ agonist- and MS-treated endoturbinates; n = 10; fig. 2A; p<0.01). Moreover, this Y₁-mediated increase appeared to be slightly more transient than the NPY effect, as the two-ways ANOVA analysis revealed a significant effect of Y₁ agonist (p<0.05), but no difference in the time-course of the EOG amplitudes between MS and Y1 agonist treatments (and no treatment x time-course interaction). In contrast, local treatment with the selective Y₂ receptor agonist Ahx [5]–[24] pNPY (1 µM; [52]) did not change the amplitude or time-course of the olfactory response amplitudes in fasted rats (n = 5, fig. 2B). Finally, local treatment with the selective Y₅ agonist [Ala31, Aib32] pNPY (1 µM; [53]) induced a slight and delayed increase of the amplitude of IA-induced EOG in overnight-fasted rats, slowly reaching a maximum, around 15% above the corresponding MS-treated EOG amplitudes, 25 min after the application (101.6±5.0% and 85.7±5.1% of control EOG amplitude, respectively in Y5 agonist- and MS-treated endoturbinates; n = 10; fig. 2C; p<0.01). The two ways ANOVA analysis revealed no difference in the time-course of the EOG amplitudes between MS and Y5 agonist treatments (and no treatment x time-course interaction). However, as expected from the NPY effect, none of the three selective agonists tested changed the kinetics of the IA-induced EOG responses (not shown).

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Figure 4. Y₁ receptor expression is up-regulated in the OM of fasted rats.

(A) Immunoblotting for Y₁R in OM extracts from fed and fasted rats reveals two main bands (55 and 70 kDa) on the western blot membranes. (B) Comparison of Y₁R protein expression level in the OM (endoturbinates II_b and III) of fed (n = 5) and fasted (n = 11) rats. The integrated density of each band on the western blots was determined by densitometry using ImageJ software, and normalized to β-actin signal. Each sample was measured on two independent gels. Results from both blots were pooled and are expressed as mean ± SEM; significant difference is denoted by * P<0.05 (Welch's t-test).

https://doi.org/10.1371/journal.pone.0045266.g004

Thus, on the basis of these electrophysiological data, NPY application significantly and transiently increased EOG amplitudes in fasted but not in fed rats. This increase of olfactory response amplitudes appeared to mainly imply a prominent fast-developing Y1-mediated effect, followed by a slight slowly-developing Y5-mediated component.

NPY-Y₁ receptors are localized in OSNs

Since the most prominent part of the NPY positive modulation was mediated via the activation of the Y₁ type receptor, we used immunohistochemical methods to identify the different cell types expressing Y₁R in the OM of fed (n = 4) and fasted rats (n = 5). We found Y₁R heterogeneously expressed in the OM. Most of the labeled cells were morphologically similar to olfactory sensory neurons (OSNs), with cell somas mostly located in the lower half of the epithelium, grouped in patches of various number of Y₁R immunoreactive cells (Fig. 3A–B). In addition to these cells, few labeled cells were localized close to the lamina propria, in the basal cell layer of the OM (Fig. 3B–b). When the Y1R primary antibody was replaced by non-immune rabbit serum, no immunostaining was observed (Fig. 3A–c). To confirm the Y₁R expression in OSNs, we performed double labeling with a neuronal marker, β tubulin III. Y₁R expression was observed in β tubulin III-positive OSNs (Fig. 3C). However, not all the β tubulin III-positive OSNs were positive for Y₁R, further suggesting an heterogeneity of the expression in the neuronal population. Therefore, we decided to quantify and compare the relative expression of Y₁R, using a western blot analysis of the endoturbinates II_b and III dissected from the fed and fasted rat hemi-heads contralateral to those used for EOGs.

Y₁R expression is upregulated in the OM of fasted rats

OM tissue from the II_b and III endoturbinates of fed (n = 5) and fasted (n = 11) rats were dissected from hemi-heads opposite to the EOG-recorded ones. The Y₁R protein expression level in the OM extracts was quantified on duplicated western blots. Two main bands of the same intensity, of roughly 55 and 70 kDa, were recognized by the Y₁R antibody on the western blot membranes (Fig. 4A). The application of the pre-absorbed antibody in the same conditions led to the distinct decrease of both the 55 kDa and the 70 kDa band (Fig. S1), thus indicating that the Y₁R is expressed as two different isoforms in the OM. The expression of these two isoforms was analyzed in fed and fasted animals. Both of them showed an enhanced expression in overnight fasted rat OM, which was significant for the 70 kDa band (+65%) (Fig. 4B).