Altered peripheral taste function in a mouse model of inflammatory bowel disease

Increased sugar intake and taste dysfunction have been reported in patients with inflammatory bowel disease (IBD), a chronic disorder characterized by diarrhea, pain, weight loss and fatigue. It was previously unknown whether taste function changes in mouse models of IBD. Mice consumed dextran sodium sulfate (DSS) during three 7-day cycles to induce chronic colitis. DSS-treated mice displayed signs of disease, including significant weight loss, diarrhea, loss of colon architecture, and inflammation of the colon. After the last DSS cycle we assessed taste function by recording electrophysiological responses from the chorda tympani (CT) nerve, which transmits activity from lingual taste buds to the brain. DSS treatment significantly reduced neural taste responses to natural and artificial sweeteners. Responses to carbohydrate, salt, sour or bitter tastants were unaffected in mice with colitis, but umami responses were modestly elevated. DSS treatment modulated the expression of receptor subunits that transduce sweet and umami stimuli in oral taste buds as a substrate for functional changes. Dysregulated systemic cytokine responses, or dysbiosis that occurs during chronic colitis may be upstream from changes in oral taste buds. We demonstrate for the first time that colitis alters taste input to the brain, which could exacerbate malnutrition in IBD patients.


INTRODUCTION
In ammatory bowel disease (IBD), a term that includes Crohn's disease and ulcerative colitis, causes diarrhea, pain, weight loss, fatigue, and potentially lethal complications from intestinal in ammation 1,2 .
While symptoms are similar in these two conditions, in ammation is continuous and limited to the large intestine in ulcerative colitis, but interspersed with healthy tissue throughout the gastrointestinal (GI) tract in Crohn's disease 1 .IBD is a chronic condition, with symptoms typically cycling between are-ups and remission.More than 85% of IBD patients are malnourished due to changes in food intake and absorption [3][4][5] .
The taste system plays a critical role in food selection and nutrition 6 , so gustatory dysfunction could exacerbate changes in body weight.The increased sweet consumption reported in Crohn's patients could also result from changes in taste function [7][8][9] .Multiple studies have shown decreased sensitivity to one or more taste qualities in at least a subset of IBD patients [7][8][9][10][11][12] , though taste was unaltered in other reports 9,13 .In a recent study, sensitivity to sweet, salty, bitter, and umami stimuli was reduced and sour sensitivity increased in IBD patients 12 .Well-established mouse models of IBD have been critical in identifying in ammatory mechanisms in colitis 2,14-16 , but have not been used to study the functional underpinnings of psychophysical taste changes.
The chorda tympani (CT) nerve transmits signals encoding taste quality from anterior lingual taste buds to the brain.Taste buds are composed of a heterogeneous population of receptor cells, including type I glial-like cells, type II cells responsive to sweet, bitter, and umami stimuli, and type III cells responsive to sour stimuli 17 .G-protein coupled receptors expressed by type II taste cells transduce complex taste stimuli.These include T1R2 + T1R3 heterodimers that bind sweet tastants, T1R1 + T1R3 receptors for umami stimuli, and T2Rs that transduce bitter stimuli 18 .Canonical taste receptors and downstream signaling molecules are also expressed in extraoral tissues including the gut [18][19][20] .
Communication between the gut and oral taste buds is well established.For example, peptides that regulate metabolism signal oral taste receptor cells in addition to hypothalamic neurons [21][22][23] .GI in ammation can also affect the taste system.Peripheral taste function is dysregulated by ingestion or enteral delivery of the in ammatory stimulus, lipopolysaccharide (LPS), derived from gram-negative bacteria 24,25 .LPS ingested during a single overnight period transiently reduced CT nerve responses to sucrose in mice 25 .Both acute and chronic LPS gavage, which bypasses oral taste buds, altered taste more extensively.Behavioral and neurophysiological responses to natural and arti cial sweeteners and NaCl were reduced in mice gavaged with LPS once or weekly 24 .Though chronic LPS gavage increased neutrophils in the small intestine and colon, mice did not display sickness behavior, weight loss or gut leakiness.Thus, peripheral taste sensitivity to sweet and salt stimuli was impaired by relatively mild in ammation localized to the GI tract 24 .These studies, together with reports of altered taste in IBD patients [7][8][9][10][11][12] , provide a rationale for testing taste function and potential mechanisms underlying changes in mice with colitis.
In the most widely used mouse model of relapsing IBD, dextran sodium sulfate (DSS)-treated drinking water is cycled on and off to allow intermittent recovery periods.While the mechanisms underlying DSSinduced colitis are incompletely understood, this treatment breaks down the epithelium in the colon, causing bacterial entry to the lumen and in ammation 14,16,26,27 .The DSS-induced colitis model is straightforward, reproducible, targets the distal colon, and has provided insight to innate immune responses and the in uence of the microbiome in IBD 14,16,26,27 .Intriguingly, DSS-induced colitis is more severe in mice lacking α-gustducin, a G-protein subunit expressed by a subset of intestinal epithelial cells 28,29 .This supports growing evidence for the immunoregulatory role of taste signaling molecules in in tissues outside of the oral cavity 20 .Taste transduction components in oral taste buds may also be targets of in ammatory changes in the GI tract 30 .
We hypothesized that DSS-induced colitis alters peripheral taste function.To test this, we recorded electrophysiological taste responses from the CT nerve of mice given three cycles of DSS, which elicited in ammation of the colon and symptomatic disease as expected.DSS treatment had striking effects on sweet taste function, reducing taste responses to all natural and arti cial sweet stimuli tested.CT responses to the umami stimulus, monosodium glutamate (MSG), were modestly increased.Tas1r2 was downregulated and Tas1r1 expression elevated in lingual taste buds of DSS-treated compared to control mice, as a molecular substrate for neural changes in sweet and umami responses, respectively.These results demonstrate major changes in sweet taste sensing in a mouse model of IBD, and provide a basis for further mechanistic studies linking gut in ammation and the regulation of taste transduction genes in lingual taste buds.

Results
Chronic DSS treatment induces body weight loss, diarrhea, and in ammation of the colon.We initially provided male and female mice with 3% DSS in drinking water or water alone from day 1-7, removed DSS, then recorded CT nerve responses 21-25 days after the start of the experiment.This treatment did not alter neural responses to any taste quality (Fig. S1a-c).DSS-treated males lost signi cantly more weight than control males on day 2, 3, and 5-8 (Fig. S1d; statistical test results in Table S1), while body weights were similar in treated and control females (p < 0.05).Since males exhibited signi cant weight loss in acute experiments as previously reported 31 , we continued using males to test taste function in chronic studies.As shown in Fig. 1a, mice lost signi cantly more body weight on days during and immediately following 2% DSS treatment cycles compared to controls.Actual p values are shown in Table 1.Recovery of body weight between DSS treatment mimicked remissions characteristic of IBD 26 .The disease activity index was signi cantly elevated during and after DSS treatment, compared with control scores that remained at baseline throughout the study (Fig. 1b; Table 1).This measure sums individual scores for body weight loss, stool consistency, and blood in stool 32 .Hemotoxylin and eosin stained sections of colon were also scored according to standard methods 32,33 .Colons from DSS-treated mice displayed in ammatory cell in ltrates, loss of tissue architecture (Fig. 2a) and signi cantly elevated disease scores (Fig. 2b) compared to water-treated controls (p = 0.024) 32,33 .Myeloperoxidase + neutrophils were also more abundant in colons from DSS-treated mice (Fig. 2c, d)(p = 0.029) Together, these results verify that DSS treatment induced in ammation, colon damage, diarrhea, and body weight loss typical of the model 14,26,29,32 ..75; p = 0.004] were similarly observed in decreased responsivity to the higher concentration of the arti cial sweetener, acesulfame potassium (aceK; p = 0.0044)(Fig.4c).Neural responses to 1.0M glucose were also reduced (p = 0.0054) in DSS-treated compared to control mice (Fig. 4d).In contrast, neural response magnitudes to the polysaccharide starch, polycose (Fig. 4d), HCl, quinine (QHCl)(Fig.4e) and NaCl (Fig. 4f) were similar in the two groups.There were signi cant main effects of stimulus concentration [F(1, 7) = 260.1;p < 0.0001] and the interaction with DSS treatment [F(1, 7) = 18.85; p = 0.0034], but not treatment alone on MSG responses.Post-tests demonstrated increased responsiveness to 0.3M MSG in the DSS group (Fig. 4g).Together, neurophysiological results demonstrate that chronic colitis inhibits responses to at least one concentration of each sweet-tasting stimulus tested while modestly elevating umami responses.
DSS-induced colitis alters lingual taste bud expression of taste transduction genes.We next tested whether colitis modulates alters taste function by modulating taste transduction genes.We used quantitative real-time PCR (qPCR) to analyze the expression of keratin (K)8, a marker of mature taste receptor cells, and taste receptor genes for sweet and umami stimuli (Fig. 5).K8 expression was similar between groups, indicating that changes in neural taste responses in mice with colitis are not mediated by taste receptor cell gain or loss (Fig. 5a).Comparable CT responses to polycose, salty, acid and bitter stimuli between groups support that conclusion (Fig. 4d-f).However, the umami receptor subunit, Tas1r1, was signi cantly upregulated in DSS-treated mice compared to controls (Fig. 5b)(p = 0.0149), in parallel with enhanced neural responses to MSG (Fig. 4g).Expression of the sweet taste subunit, Tas1r2, was signi cantly reduced by DSS (Fig. 5c)(p < 0.0001) along with reduced neural responses to sweet stimuli (Fig. 4a-d).Expression of Tas1r3, which forms a sweet receptor heterodimer with Tas1r2 and a umami receptor with Tas1r1, was not signi cantly different between groups.These results indicate that colitis alters the expression of sweet and umami taste transduction genes as a substrate for neural changes.
In ammation in the anterior tongue.We examined tongue sections stained with hematoxylin and eosin to determine if DSS treatment compromised the integrity of the lingual epithelium and elicited in ammation in the tongue (Fig. 6a) similar to colon (Fig. 2a).However, the lingual epithelium, fungiform papillae, and taste buds were intact and appeared similar in DSS-treated and control groups.We also tested whether in ammation near taste buds could be responsible for changes in neural responses and receptor genes for sweet and umami stimuli.As shown in Fig. 6b-d, however, macrophage density in the epithelium and mucosa was similar between groups.Thus, while DSS drinking damaged the colon as expected, the lingual epithelium was intact indicating that oral in ammation was not the proximate cause of taste changes.

DISCUSSION
We demonstrate, for the rst time that we are aware of, that taste function is altered in an animal model of IBD.Chronic colitis reduced sweet taste transmission to the brain, in parallel with the downregulation of the Tas1r2 sweet receptor subunit in oral taste receptor cells.DSS treatment suppressed neural responses to a wide range of natural and arti cial sweeteners.Only the two lowest concentrations of sucrose and aceK were unaffected by DSS (Fig. 4a, c), likely because responses were near zero creating a " oor effect".Chronic DSS also modestly elevated responses to 0.3M MSG and upregulated expression of the Tas1r1 subunit that transduces umami stimuli in taste cells.While we did not perform behavioral taste testing, we previously showed that milder, chronic gut in ammation suppressed brief-access licking and 23-hr licking in addition to CT responses to sweet stimuli 24 .Thus, reduced neural responsiveness could potentially impair behavioral sensitivity to sweet tastants.
Several studies indicate that sweet taste may also be dysregulated in IBD patients.Patients with Crohn's disease exhibit higher taste thresholds for sucrose compared to control subjects, which may lead to overconsumption of sugar 7,34 .In other studies, however, IBD patients exhibited lower sensitivity to multiple taste modalities 11 , reduced sensitivity to bitter, salty, umami and fat but increased sour sensitivity 12 , or reduced sensitivity to multiple modalities except sour 10 .Others report no taste changes in patients 13 .Studies on IBD-induced taste dysfunction may lack consensus because of the inclusion of patients with both Crohn's disease and ulcerative colitis, patients in different stages of are-up and remission, varied dietary and environmental conditions, sex differences and the use of different methods to test taste sensitivity 1,2,7,8,10-13 .In the current chronic study, we used male mice because acute disease symptoms were more pronounced, likely due to more robust in ammatory responses and protective effects of estrogen in the DSS model 31,35 .Additional studies will determine whether female mice with colitis exhibit similar changes in sweet and umami taste function.Nonetheless, these results highlight the value of DSS-induced colitis in revealing mechanisms underlying taste changes in animals with de ned environmental conditions and genetic backgrounds.
In addition to DSS, dietary and gut manipulations can alter peripheral taste function in rodents.Acute or chronic oral LPS gavage increased neutrophils in the colon, as shown here, and suppressed neural and behavioral responses to sweet stimuli 24,25 .LPS also reduced CT nerve and behavioral responses to NaCl, but treated mice did not exhibit weight loss or sickness behavior unlike DSS suggesting divergent mechanisms 24 .Dietary manipulations with and without changes in body weight can also affect taste.
Rats chronically consuming 30% sucrose solution did not gain signi cantly more weight compared to groups fed solid high-sucrose or control food, but CT nerve taste responses to sweet and salty stimuli decreased 36 .Fewer taste receptor cells responded to sweet stimuli and behavioral detection of sucrose and aceK was impaired in obese mice fed a high-fat diet 37 .The same investigators showed that a highfat diet, with and without weight gain, reduced the expression of gustducin and PLCβ2 downstream from sweet, umami and bitter receptor signaling as a mechanism for dampened taste responses 38 .The regulation of downstream taste transduction molecules in colitis, in addition to the decrease in sweet subunit expression identi ed here, will be of interest in future studies.
Mechanisms by which the in amed colon affect taste buds remain to be determined.DSS is unlikely to damage taste buds directly since the lingual tissue structure is intact.The taste cell marker gene, K8, was also expressed at similar levels in DSS and control groups, indicating that taste buds do not undergo signi cant degeneration in mice with colitis.Though in ammation can regulate taste function 39,40 , we found no evidence of increased immune cell responses near taste buds in DSS-treated vs. control mice.
IBD can cause zinc de ciency 41,42 , which impairs behavioral and neural taste responsiveness in rodents [43][44][45] .In previous studies, however, zinc de ciency suppressed CT responses to multiple taste qualities (i.e.NaCl, QHCl, HCl, NH 4 Cl, and glutamic acid) 44 .We did not measure serum zinc levels here, but found more restricted changes in neural responses to sweet stimuli and MSG.Malnourishment is a common symptom of IBD, and DSS-treated mice lost weight in the current study.Yet, CT responses to sodium were speci cally impaired in rats maintained on a protein-de cient diet prenatally through adulthood 46 .Thus, there are mismatches in the taste modalities affected by dietary zinc and protein de ciency compared to mice with colitis.
DSS-induced colitis alters cytokine levels in serum as well as colon, providing a potential route of communication between the in amed gut and taste buds.Circulating Th1-Th17 responses (i.e.TNF-α, IL-6, IL-17, CXCL-1) dominate in the acute phase after DSS treatment, while Th2 cytokines (i.e.IL-4 and IL-10) are chronically upregulated in mice with colitis 47,48 .Oral taste bud cells express receptors for cytokines including TNF, IL-1, IL-6, and IL-10, which can also affect their function and life span [49][50][51][52][53][54] .Yet, the speci c changes in sweet and umami taste observed in mice with chronic colitis limit potential upstream mechanisms.The Th2 cytokine, IL-10, is important for mucosal homeostasis 55 , and IL-10Rα (IL-10R1), the ligand-binding subunit of the IL-10 receptor, is co-localized to T1R3 + sweet-and umamisensing taste cells 50 .However, serum IL-10 levels are elevated in mice with chronic DSS-induced colitis, while taste bud number and size decreased in the absence of IL-10 47,48,50 .The microbiota of the tongue, saliva and the GI tract is dysregulated in mice with colitis and patients with IBD [56][57][58] , which also could alter taste function.Type II taste cells express a genetic signature and possibly functions similar to microfold (M) cells that surveil mucosal-associated lymphoid tissues (MALT) 59 .Mice de cient in Spib, a transcription factor critical for M cell development, displayed increased licking responses to sucrose and MPG 59,60 .While the parallels are imperfect, since neural responses to sweet and umami stimuli were inversely altered here, taste changes in colitis could depend on in ammatory or microbial dysregulation 60,61 .
In conclusion, we report novel taste changes in male mice with chronic colitis.Tas1r2 expression is suppressed and Tas1r1 elevated in taste buds, mediating decreased sweet and heightened umami neural inputs to the brain.Chemosensory cells and receptor proteins in the gut and airway act as sentinels for microbes and coordinate in ammatory and neural responses 20,[62][63][64][65] .These results, together with previous studies 24,25 , indicate that taste buds are also modulated by gut in ammation, which may in turn affect diet and nutrition.Changes in taste function could lead to excess consumption of palatable foods or nutritional de cits further exacerbating IBD, warranting further investigation 66-69 .

MATERIALS & METHODS
Animals and DSS treatment.C57BL/6J mice (#000664, Jackson Laboratory) were 9-10 weeks old at the beginning of treatment (day 0) after acclimatizing to the vivarium for at least 6 days.Mice were housed in a barrier facility with lights on a 12:12 light:dark cycle.All groups had free access to rodent chow (#2918; Envigo Teklad) throughout the study and ltered tap water between treatment periods.Mice were provided with 2% DSS (#160110, 36-50 KDa, MP Biomedicals) dissolved in distilled water or distilled water alone in 15 ml tubes tted with lixit valves.Mice were randomly assigned to the DSS or water control groups using the GraphPad Prism online randomisation tool.We focused chronic studies on males since their weight loss was greater in preliminary acute studies (Fig. S1).DSS was provided in three cycles at day 1-7, 22-29 and 42-49.This treatment induces chronic, relapsing and remitting colitis mimicking IBD 33,70 .Mice were weighed, uid intakes recorded to con rm DSS ingestion, and stool samples collected daily during treatment and every 1-3 days between treatment periods.Sample sizes were based on previous work on gut-taste interactions, and are provided in gure legends 24,25 .Animal procedures followed National Institutes of Health guidelines and were approved by the Augusta University Institutional Animal Care and Use Committee.Mice losing more than 25% of their original body weight were removed from the study and euthanized (n = 2) in compliance with a priori humane endpoints in our approved animal use protocol.
Neurophysiology.We recorded CT nerve responses to tastants at day 56-61 following the rst treatment period at day 0. Mice were anesthetized with ketamine (80 mg/kg) plus xylazine (10 mg/kg) i.p. and body temperature maintained at 36-39 o C. We injected supplemental anesthetic as needed.We tracheotomized mice, approached the CT nerve laterally and dissected it free of surrounding tissues, then placed it on a platinum electrode 24,52 .Neural activity was ampli ed (Grass Instruments), integrated with a time constant of 1.5 sec, and the summated signal recorded with PowerLab hardware and software (AD Instruments).Taste stimuli, applied to the tongue at room temperature with a syringe, included 0.10 and 0.50M NaCl; monosodium glutamate (MSG; 0.3M); 0.1, 0.5 and 1.0 M sucrose; 0.05 and 0.10M saccharin; 0.025 and 0.05M acesulfame (AceK); 1.0M glucose; 16% polycose; 0.01 M quinine (QHCl), and 0.01N HCl mixed in distilled water.Chemical stimuli were purchased from Sigma with the exception of polycose (#00746, Abbott Labs).CT nerve response magnitudes were calculated by subtracting the baseline from the height of the summated, integrated responses 20 sec after stimulus application 24 .We normalized relative responses to mean 0.5M NH 4 Cl responses recorded at the beginning and end of the stimulus series, and only analyzed bracketed series if 0.5M NH 4 Cl responses deviated by ≤ 10%.At the end of recordings anesthetized mice were overdosed with iso uorane without awakening, followed by tissue harvest and bilateral thoracotomy or cervical dislocation, which was also the method of euthanasia for all experiments below unless otherwise noted.Euthanasia methods comply with American Veterinary Medical Association (AVMA) standards.
Immuno uorescence, histology and image analysis.Mice were euthanized as above and tongues removed on the mandible and xed in paraformaldehyde for 5-7 hours, then dissected free of the mandible, bisected longitudinally and cryoprotected overnight in 30% sucrose in PBS 52 .We used half of the tongue for qPCR (below) and half for immunostaining.Proximal and distal colons were dissected, ushed in PBS and mounted using the Swiss-roll technique 71 .Tongues and colons were ash-frozen in in O.C.T. (Sakura) and serially cryosectioned at 8 µm for immunostaining.Colon sections were incubated overnight at 4 0 C in anti-mouse myeloperoxidase (MPO; 1:100; #AF3667, R&D) to identify neutrophils 24 followed by Alexa Fluor secondary antibody for 1 hr at room temperature (1:1000; Jackson Immunoresearch).Nuclei were stained with DAPI (#D1306; Invitrogen / Thermo Fisher Scienti c) and slides coverslipped with Fluoromount-G (#0100-01; SouthernBiotech).We identi ed macrophages in anterior tongue sections with CD68 (1:200; ab53444, Abcam) using similar procedures 52 .Sections of colon and tongue were also cleared and stained with hematoxylin and eosin.MPO + neutrophils were analyzed in four distinct sections of colon using a microscope equipped with epi uorescence (Olympus BX51), a digital monochrome camera (Cool Snap, Roper Scientic) and MetaMorph software (MDS Analytical Technologies) 24 .A region of interest (12.9 mm 2 ) was placed in the area of greatest MPO + cellular density within a section of colon and the image captured.MPO staining was thresholded, the % positive pixels / region calculated for each section of colon and the four values summed for each animal (Metamorph Software, Universal Imaging) 24 .The investigator was blinded to DSS or water treatment.We also captured bright eld images of hematoxylin and eosin-stained distal colon to assess in ammation and tissue breakdown.Disease scores for colons were assigned by an investigator blinded to treatment: colon architecture (normal, 0 -severe crypt distortion with loss of crypts, 3); in ammatory in ltration (normal, 0 -dense in ammation, 3); muscle thickening (normal, 0marked muscle thickening, 3); goblet cell depletion (absent, 0 -present, 1) and crypt abscess (absent, 0present, 1).The individual scores were summed to determine the disease score for each animal 32,33 .
DSS induces colitis by breaking down the gastrointestinal barrier 14 .While DSS is only brie y present in the oral cavity, we stained sections of tongue with hematoxylin and eosin to assess epithelial integrity and lingual in ammation using methods described above.We also analyzed CD68 + macrophages (1:100; Abcam) in fungiform papillae and the dorsal mucosa of the anterior two-thirds of the tongue 52 .
Images were captured from four non-overlapping, standard-sized regions of interest (12.9 mm 2 ) in the lingual epithelium, and four regions from the dorsal lingual mucosa.Image montages were assembled for each region, and CD68 + pixels thresholded to calculate the percentage of staining per standard area.
Quantitative real-time polymerase chain reaction (qPCR).We performed qPCR using previously described methods 52 .Tongue halves were stored in RNAlater (Fisher Scienti c) at -80 o C until use.Primer sequences (Integrated DNA Technologies) are listed in Table 2.We performed qPCR using the QuantiTect SYBR Green PCR kit (Applied Biosystems) and the QuantStudio III Real-Time PCR Systems (Applied Biosystems).We normalized transcripts to gapdh1 and used the 2 -ΔΔCT method to analyze changes in mRNA expression in DSS-treated relative to water-treated tongues 72 .a The expression of the taste receptor cell marker gene, keratin (K)8, was similar between groups.b The umami taste receptor subunit, Tas1r1, was signi cantly increased in mice with colitis compared to controls.cExpression of the sweet taste receptor subunit, Tas1r2, was signi cantly reduced by DSS treatment.dExpression levels of Tas1r3, which forms heteromeric umami receptors with Tas1r1and sweet receptors with Tas1r2, were similar between groups.*p < 0.05; ***p < 0.0001.

Figures
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Table 1
a. Mice treated with DSS on shaded days.b.Not determined; small sample size (n < 2) or no data in at least one group (ND); c.All data are 0, so the p-value cannot be calculated.Conclusion is no difference between the two groups.

Table 2 Primers
52atistical analyses were performed with Prism 9.4.1 (GraphPad Software).Colon disease scores, the density of MPO + neutrophils in colon, mRNA expression in lingual epithelium, and the density of lingual CD68 + macrophages were compared between DSS-treated and control groups with two-tailed Student's t tests.One outlier was identi ed by Grubb's test (α = 0.05; G = 2.488) in the K8 mRNA data and not included in further analyses.To account for the repeated measurements on the same animal, we analyzed group differences in % body weight loss and disease index scores over time with linear mixed models tted using R package lme4 (version 1.1-29).For comparing % body weight loss, p values were calculated using t tests with the degrees of freedom approximated by Satterthwaite's method; for comparing disease index scores, p values were calculated using Wilcoxon rank-sum test.Neurophysiological responses were analyzed with two-way ANOVAs with treatment group and stimulus concentration as factors followed by Bonferroni post-tests52.We used Student's t tests to analyze neural responses when we only one stimulus concentration was tested.We considered P values ≤ 0.05 signi cant in all statistical analyses.
Con ict of interest statement: The authors declare no competing nancial interests.This study reports methods and results according to ARRIVE guidelines.