GLP-1R–positive neurons in the lateral septum mediate the anorectic and weight-lowering effects of liraglutide in mice

We initiated our examination by performing immunostaining to define the distribution of endogenous GLP-1Rs within the mouse brain (; supplemental material available online with this article;). The specificity of the anti–GLP-1R antibodies was validated in wild-type and GLP-1R–knockout mice (, B and C). We found densely clustered GLP-1R–positive neurons prominently located in the dorsal portion of the LS (dLS) (), a region implicated in energy control according to previous work from our group and other groups (,). A large number of GLP-1R–positive cells were also detected throughout various hypothalamic nuclei, mainly in the PVN, dorsomedial hypothalamic nucleus (DMH), and Arc, and among scattered neurons in the lateral hypothalamus. A considerable GLP-1R–positive presence was also noted in the hindbrain, including the AP and the external cuneate nucleus. Other brain regions that exhibited considerable GLP-1R expression included the ventral pallidum, anterior pretectal nucleus, pontine nuclei, dentate gyrus, and lateral reticular nucleus (). Supplemental Figure 1A Supplemental Figure 1 Supplemental Figure 1A ^{32 33} Supplemental Figure 1A https://doi.org/10.1172/JCI178239DS1↗

If a brain region mediates the anorectic effect of GLP-1R agonists, its activity should be modulated by liraglutide. Thus, we systematically mapped brain activation induced by intraperitoneal (i.p.) administration of liraglutide with immunohistochemistry for c-Fos, an early marker of neuronal activity. Liraglutide induced a substantial elevation of c-Fos expression compared with saline controls in the LS, the PVN, and the AP, whereas there was no elevation in other GLP-1R–rich regions (, and). As previously noted, ablating GLP-1Rs in the PVN or the AP does not diminish the anorectic or weight-lowering effects of liraglutide (,). This led us to ask whether GLP-1Rs in the LS contribute to the pharmacological effects of liraglutide. Figure 1, A and B Supplemental Figure 1D ^{17 26}

Then we labeled GLP-1R–positive neurons in the LS by crossingmice withreporter mice. Specific expression of red fluorescent protein tdTomato in GLP-1R–positive neurons was observed in the LS (, A–C). Systematic administration of liraglutide (i.p.) markedly upregulated c-Fos expression in LSneurons (, D–F), suggesting activation of these neurons. To exclude potential influences of network effects caused by systematic administration, we cannulated above the dLS for localized infusion (). This local infusion of liraglutide into the LS also markedly upregulated c-Fos expression in LSneurons but not in GLP-1R–negative neurons (). Concurrently, a substantial reduction in food intake and body weight was also observed in mice with local liraglutide infusion (, G–K). GLP-1R-ires-Cre Ai14 Supplemental Figure 2 Supplemental Figure 2 Figure 1C Figure 1, D and E Supplemental Figure 2 GLP-1R GLP-1R

To probe the potential mechanism underlying the activation of LSfollowing liraglutide infusion, we then performed targeted whole-cell patch clamp recording from LSneurons (). Liraglutide dramatically increased the amplitude but not the frequency of excitatory postsynaptic currents in GLP-1–positive neurons. This result is in accordance with a previous report that a GLP-1 analog (exendin-4) enhanced excitatory synaptic transmission through AMPA receptors trafficking in the PVNneurons () (). GLP-1R GLP-1R CRH Figure 1F ¹⁶ Figure 1, G and H

Together, these findings demonstrate that LSneurons can be effectively activated by liraglutide, possibly through the enhancement of excitatory synaptic transmission. GLP-1R

To elucidate the role of GLP-1Rs in the LS in mediating the anorexigenic effects of liraglutide, we used CRISPR/Cas9 technology to specifically knock down GLP-1R expression in LSneurons. We injected an adeno-associated virus (AAV) containing–targeting single-guide RNA (sgRNA) and Cre-inducible mCherry into the dLS ofmice bred with Cre-inducible Cas9 knockin mice () (). Through this approach, we achieved an approximately 90% reduction in GLP-1R expression in sg–targeted neurons compared with controls (). GLP-1R GLP-1R GLP-1R-ires-Cre GLP-1R ³⁴ Figure 2A Figure 2B

Remarkably, we found that the knockdown of dLS GLP-1Rs did not influence food intake or body weight in mice at the baseline, regardless of dietary conditions (, A–E). As expected, acute i.p. injection of various liraglutide dosages markedly reduced food intake in control mice (, and, F–I). However, the reduction in food intake was dramatically diminished in the GLP-1R–knockdown group (, and, F–I). Furthermore, GLP-1R knockdown in the LS attenuated body weight reduction induced by liraglutide (, and, F–I). A prolonged treatment experiment spanning 3 weeks further substantiated these findings. While liraglutide effectively reduced body weight in wild-type mice, the effect was dramatically blunted in mice with GLP-1R knockdown in the LS (). Supplemental Figure 3 Figure 2, C–H Supplemental Figure 3 Figure 2, C–H Supplemental Figure 3 Figure 2, C–H Supplemental Figure 3 Figure 2, I–K

We also examined the role of GLP-1Rs in other brain regions, such as PVN and Arc, with the same CRISPR/Cas9–mediated knockdown approach. However, neither the targeted knockdown of GLP-1Rs in the PVN nor the Arc altered the anorectic properties following liraglutide (). Collectively, these findings demonstrate that GLP-1Rs in the LS contribute to the anorectic effects of liraglutide. Supplemental Figure 4

To elucidate the influence of GLP-1R upregulation in LSneurons on food intake, we used a specific AAV vector encoding Cre-inducible mouse GLP-1Rs, complemented with a hemagglutinin (HA) epitope tag, for targeted injection into the dLS ofmice (). Subsequent immunohistochemical analyses confirmed the overexpression of GLP-1R (, B and C). This overexpression in the LS led to a substantial decrease in food consumption under sated conditions, but not in fasted mice (, D–G). The absence of effect in fasted mice may be due to negligible endogenous GLP-1 release in fasted animals (,). Thus, overexpression of GLP-1R in the LS is sufficient to lower food consumption in sated mice. GLP-1R GLP-1R-ires-Cre Supplemental Figure 5A Supplemental Figure 5 Supplemental Figure 5 ^{4 7}

Next, we assessed the effect of GLP-1R overexpression in the LS on chronic body weight and metabolic parameters. Overexpression of GLP-1Rs did not change chronic body weight compared with that of EYFP-expressing control mice (). Overexpression of GLP-1Rs in the LS also did not change oxygen uptake (VO), carbon dioxide discharge (VCO), respiratory exchange ratio, and average energy expenditure (, I–P). Supplemental Figure 5H Supplemental Figure 5 2 2

Having identified the vital role of LS GLP-1Rs in mediating the anorectic and weight-reducing effects of liraglutide, we sought to elucidate the specific function of LSneurons in the regulation of energy and body weight homeostasis by conducting loss-of-function experiments. GLP-1R

RNA hybridization has shown that all LS GLP-1R neurons express the vesicular GABA transporter (vGAT), indicative of inhibitory neurons, and none express the excitatory marker vesicular glutamate transporter 2 (vGluT2). Furthermore, among these LSneurons, 39% exhibited somatostatin (Sst) expression, and 23% showed neurotensin (Nts) expression (, A and B). We then used tetanus neurotoxin (TeNT), a specialized protease known to cleave synaptobrevin-2, thereby blocking neurotransmitter release, as a molecular tool for synaptic silencing (). To inactivate LSneurons, we injected AAV expressing double-floxed EGFP and TeNT (AAV-DIO-EGFP-2A-TeNT) into the bilateral LS ofmice to achieve specific expression of EGFP-2A-TeNT in LSneurons (and). On an ad libitum high-fat diet, TeNT mice exhibited greater body weight gain in comparison with EYFP control mice (); however, this difference was not observed under chow-fed condition (). Consistent with this, TeNT-mediated silencing of LSneurons markedly increased the consumption of palatable food but not standard chow (). GLP-1R GLP-1R GLP-1R GLP-1R Supplemental Figure 6 ³⁵ Figure 3A Supplemental Figure 6C Figure 3B Supplemental Figure 7A Figure 3, C and D GLP-1R-ires-Cre

Considering that several studies have associated the inhibition of central GLP-1R with aggravated glucose tolerance (), we conducted oral glucose tolerance tests to investigate the role of LSneurons. Interestingly, there was no difference between TeNT and control mice in glucose tolerance (). ³⁶ Figure 3E GLP-1R

We further explored the effect of TeNT expression on liquid food intake during fixed-interval food delivery and operational food self-administration tasks. TeNT expression markedly increased the number of licks and Ensure intake, and the TeNT mice also showed markedly more active poking to obtain Ensure compared with controls (, and). Silencing LSneurons, on the other hand, did not increase water consumption (, C–E), implying that the higher intake of Ensure was not due to the increased need for water. Figure 3, F–H Supplemental Figure 7B Supplemental Figure 7 GLP-1R

We also assessed the effects of LSneuronal silencing on metabolic parameters. Both VOand VCOwere markedly higher in the TeNT mice compared with controls, particularly during the active phase (i.e., the dark cycle) of the day (, F–I). Despite these differences, the respiratory exchange ratio — the ratio of VCOproduced to VOconsumed — remained unchanged (, J and K), indicating no substantial differences in the metabolic utilization of carbohydrates and fats between the TeNT mice and the controls. Interestingly, energy expenditure (EE) was also markedly higher in the TeNT mice (, L and M), possibly because of an increased basal metabolic rate. GLP-1R 2 2 2 2 Supplemental Figure 7 Supplemental Figure 7 Supplemental Figure 7

Mindful of studies implying an anxiogenic role for the LS (–), we explored whether the altered consumption could be attributed to changes in anxiety levels and found that LS:TeNT mice exhibited similar anxiety levels and locomotor activity in an open-field test compared with control mice (, N and O). This suggests that the altered consumption was unlikely to result from changes in anxiety level or locomotion. Together, these data demonstrate that inactivation of LSneurons increases food consumption and promotes obesity induced by high-fat food. ^{37 39} Supplemental Figure 7 GLP-1R GLP-1R

To investigate the role of LSneurons in the anorexigenic and weight-reducing effects of liraglutide, we measured the effects of liraglutide on the reduction of food intake and body weight in mice with active (control: AAV-DIO-EYFP) and inactive (TeNT: AAV-DIO-EGFP-2A-TeNT) LSneurons. Liraglutide treatment markedly decreased food consumption and body weight in the control group under both chow-fed and high-sucrose-fed conditions. However, silencing of LSneurons markedly reduced these effects at various doses of liraglutide (, and). GLP-1R GLP-1R GLP-1R Figure 3, I–L Supplemental Figure 8

Nausea is one of the most common adverse side effects reported with GLP-1R agonists, such as liraglutide (–). To investigate whether liraglutide-induced nausea requires the action of LSneurons, we used the standard conditioned taste avoidance (CTA) model () (). Intraperitoneal administration of liraglutide consistently induced a robust CTA across both the TeNT and control groups, with no substantial differences observed between the two (, Q and R). These findings indicated that the LSneurons were not involved in the liraglutide-induced nausea. ^{40 42 40} Supplemental Figure 7P Supplemental Figure 7 GLP-1R GLP-1R

In summary, these results support the notion that LSneurons play an essential role in mediating the anorexigenic and body weight–reducing effects of liraglutide. GLP-1R

Next, to explore the intrinsic activity of LSneurons during naturalistic feeding, we recorded Casignals using fiber photometry under freely moving conditions (). We observed a pronounced decrease in Casignal at the initiation of food consumption in food-deprived mice, and this reduction persisted throughout the eating episode, returning to baseline levels once feeding ceased (and). Interestingly, when mice were exposed to more palatable food sources, such as high-sucrose or high-fat items, rather than standard chow, the decrease in neuronal activity was more pronounced (). This result indicates that the dynamics of LSactivity were modulated by food palatability. GLP-1R 2+ 2+ GLP-1R Figure 4A Figure 4B Supplemental Video 1 Figure 4, C–F

To test whether the activity of LSneurons is modulated by energy homeostasis, we presented a pellet of high-fat food to satiated mice. Compared with fasted mice, satiated mice exhibited a markedly smaller inhibitory response during consumption (). To examine this phenomenon more closely, we divided the feeding behavior into 3 stages (initial, middle, and final) and observed a gradually diminishing inhibitory response from the initial to the final stage (). These results demonstrate that the current energy state can actively modulate LSneuronal activity during feeding. GLP-1R GLP-1R Figure 4, G–J Figure 4, K and L

We extended our observation to the food-seeking phase by allowing fasted mice to visually perceive but not physically access a caged food pellet, thus triggering typical seeking behaviors. Despite these actions, no discernible alteration in the Casignal was detected (), demonstrating that food seeking does not modulate dLSneuronal activity. 2+ GLP-1R Figure 4M

According to our fiber photometry data, we propose that this specific cluster of neurons functions analogously to a brake pad in the regulation of feeding behavior. In the reduced activity state, these neurons facilitate the continuation of feeding. Conversely, when activity is heightened, they play a crucial role in suppressing food intake. To examine whether activation of LSneurons is sufficient to suppress food intake independent of endogenous GLP-1R or exogenous liraglutide, we injected an AAV into the dLS ofmice expressing the excitatory Gq-coupled designer receptor exclusively activated by designer drugs (DREADD) hM3D-mCherry in a Cre-dependent fashion (). This method resulted in the selective expression of hM3D-mCherry in LSneurons (). Intraperitoneal injection of the DREADD agonist clozapine-oxide (CNO) induced robust c-Fos expression in LSneurons transduced with hM3D, indicating increased neuronal activity (). GLP-1R GLP-1R GLP-1R GLP-1R-ires-Cre N ⁴³ Figure 5A Figure 5B

Next, we performed feeding assays after i.p. injection of CNO or saline. Compared with saline, DREADD-based activation of LSneurons via CNO reduced a 2-hour consumption period of both standard chow and high-sucrose food during the dark period when mice normally consume food actively (). In an overnight fast condition, activation of LSneurons markedly reduced food intake for both standard chow and high-sucrose food (, A and B). This result suggests that the activity of these neurons can overcome the motivational hunger drive and suppress feeding. Considering prior evidence that GLP-1R activation augments glucose tolerance (,), we probed the potential of LSneurons to modulate glucose homeostasis. Activation of LSneurons did not affect glucose homeostasis (), supporting the role of these neurons in anorectic effects rather than glucose-lowering effects. GLP-1R GLP-1R GLP-1R GLP-1R Figure 5, C and D Supplemental Figure 9 ^{44 45} Figure 5E

We further investigated the long-term effects of chronic LSneuronal activation. CNO was administered bi-daily for 1 week continuously to mice expressing hM3D-mCherry. Chronic CNO administration effectively suppressed both food intake and body weight, which were recovered upon cessation of CNO. In control mice with mCherry expression, the same CNO injection failed to change food intake and body weight (). GLP-1R Figure 5, F–H

To explore whether LSneuronal activity acts as negative or positive valence, we implemented optogenetic activation by expressing channelrhodopsin (ChR2-mCherry) selectively in LSneurons (). In a real-time place preference/avoidance test, LS:ChR2 mice exhibited a substantial avoidance of the photostimulation-paired chamber (, C–E). To examine whether transient activation of LSneurons is sufficient to suppress feeding, we trained LS:ChR2 mice to consume Ensure on a fixed ratio 1 schedule, and photostimulation (20 Hz, 1.5 seconds) was synchronized with Ensure administration (). Photostimulation of LSneurons decreased the nose-poking and Ensure consumption (). Collectively, these experiments suggested that LSneurons encoded negative valence and suppressed appetite. GLP-1R GLP-1R GLP-1R GLP-1R GLP-1R GLP-1R GLP-1R Figure 5I Supplemental Figure 9 Figure 5J Figure 5K

Finally, we sought to elucidate the specific projection targets of LSneurons that are integral to food regulation. We injected AAV-FLEX-tdTomato-T2A-synaptophysin-EGFP into the LS ofmice (, A and B). With this tracing strategy, axonal fibers are labeled in red tdTomato, while synapses projecting from LSneurons are labeled in green EGFP (). We found that LSneurons made major synaptic connections with multiple brain regions (, C and D), including the nucleus of the horizontal limb of the diagonal band (HDB), the lateral and medial preoptic area (LPO/MPA), the lateroanterior hypothalamic nucleus (LA), the lateral hypothalamic area (LH), the medial tuberal nucleus (MTu), the lateral and medial habenular nucleus (LHb/MHb), the CA3 field of the hippocampus (CA3), and the pyramidal cell layer of the hippocampus (Py). Previous research has suggested that multiple hypothalamic brain areas, including the LH and MTu mentioned above (,), are involved in feeding regulation. Thus, LSneurons project to multiple brain areas that are implicated in feeding regulation. GLP-1R GLP-1R GLP-1R GLP-1R GLP-1R-ires-cre Supplemental Figure 10 ³⁵ Supplemental Figure 10 ^{46 47}

Our study examined male and female animals, and similar findings are reported for both sexes.

All animal husbandry and experimental procedures were approved by the Animal Care and Use Committees at the Shenzhen Institute of Advanced Technology, Chinese Academy of Sciences (CAS). Adult male C57BL/6J mice (3–5 months old; Guangdong Medical Laboratory Animal Center),mice (Shanghai Model Organisms, NM-KI-200134), GLP-1R-KO mice (Shanghai Model Organisms, NM-KO-190803),mice (The Jackson Laboratory, 007908), andmice (The Jackson Laboratory, 024857) were used for this study. Mice were maintained at a constant temperature of 22°–25°C, following a 12-hour light/12-hour dark cycle. GLP-1R-ires-Cre Ai14:Rosa26-loxP-STOP-loxP-tdTomato Rosa26-LSL-Cas9

Fiber photometry recordings were initiated at least 3 weeks after surgery using the fiber photometry system ThinkerTech. A 470 nm blue LED light (30 μW) was channeled through a singular implanted ferrule. The resulting signals were analyzed using a custom MATLAB script. Thescore was determined as (− μ)/σ, where the mean and standard deviation were derived from the signal 5 seconds before stimulation. z x

For recordings during free-moving feeding, mice — either food-deprived for 24 hours or fed normally — were introduced to a transparent acrylic enclosure measuring 15 × 15 × 30 cm and then connected to the fiber photometry apparatus. A 5-minute habituation period was followed by the gentle placement of a food pellet (choices included chow or high-sucrose or high-fat content) in the center of the box. The system simultaneously captured the free-feeding behavior and the GLP-1R:GCaMP signals for 15 minutes. All obtained data were segmented and time-aligned according to individual behavioral bout onsets. Fluorescence signals were normalized usingscores, taking into account the mean and standard deviation from time windows of −5 to 0 seconds before the first bite and −10 to 0 seconds leading up to the last bite. Any behavioral bouts lasting fewer than 10 seconds were disregarded. z

Body weight was consistently measured manually at the same daily interval. In experiments involving TeNT-induced synaptic inactivation and GLP-1R overexpression, mice were provided with either standard chow or high-fat food. For experiments focused on the knockdown of LS GLP-1Rs, mice received daily i.p. injections of liraglutide at a dose of 200 μg/kg of body weight. For chemogenetic activation experiments, mice received semidiurnal i.p. injection of CNO at a dose of 2 mg/kg body weight.

Mice were individually housed and acclimated to metabolic cages (TOW-INT Tech.) for at least 3 days before testing under a 12-hour light/12-hour dark cycle. Energy expenditure, VO, VCO, respiratory exchange ratio, food intake, and water intake were measured continuously and simultaneously at a sampling frequency of 5 times per minute. Data were exported to Excel and analyzed using MATLAB (MathWorks). Light and dark cycles were indicated by white (6 am to 6 pm) and black (6 pm to 6 am), respectively. Food and water were freely available during testing. The gas sensors for COand Owere calibrated before each test. 2 2 2 2

Blood glucose was measured by making a small horizontal incision on the mouse's tail end using a razor blade. A drop of blood was gently massaged out, and its glucose concentration was determined using a Bayer blood glucose meter. Throughout this procedure, food was withheld. In the TeNT-induced synaptic inactivation experiments, blood glucose was gauged after an overnight fast of 16 hours. Subsequently, these fasting mice were given an oral dose of 1.5 g/kg 30%-glucose solution (Sigma-Aldrich, catalog G6125). Blood samples were taken at baseline, and then at intervals of 10, 30, 60, 90, and 120 minutes after glucose administration. For chemogenetic activation experiments, fasting blood glucose levels (the baseline at time zero) were measured 30 minutes after administration of CNO injections. d

Mice were euthanized using a pentobarbital sodium overdose and then transcardially perfused with phosphate-buffered saline (PBS; pH 7.4), followed by 4% paraformaldehyde (PFA). The brains underwent postfixation in 4% PFA for 8–12 hours and were subsequently dehydrated in 30% sucrose for 24–48 hours or until fully submerged. The tissue was then embedded in Tissue-Tek OCT compound (Sakura) and frozen with dry ice. Using a cryostat (Leica), 40-μm sections were prepared, with free-floating sections stored in PBS.

For staining, sections were initially rinsed with PBS 3 times, 10 minutes each. They were then blocked at room temperature using a solution of 10% normal goat serum and 0.3% Triton X-100, followed by an overnight incubation at 4°C with the primary antibody. After three 10-minute washes with PBST, sections were incubated with a fluorophore-linked secondary antibody for 2 hours and then counterstained with DAPI (1:3,000 dilution). Images were captured using an Olympus Virtual Slide Microscope (VS120-S6-W) and later analyzed by an evaluator unaware of the experimental group identities. Antibody information is summarized in. Supplemental Table 3

Mouse brains were sectioned into 18-μm slices using a Leica cryostat and affixed to SuperFrost Plus microscope slides. Probes targeting GLP-1R (catalog 418851-C3), vGAT (catalog 319191-C3), vGluT2 (catalog 319171), somatostatin (Sst; catalog 404631), and neurotensin (Nts; catalog 420441) were specifically designed and validated by Advanced Cell Diagnostics. All fluorescence in situ hybridization experiments were performed using the RNAscope v2 Assay (catalog 323100) following the manufacturer's guidelines. Briefly, brain slices were air-dried at 39°C for 2 hours, washed with 1× PBS, treated with 3% hydrogen peroxide in methanol and Target Retrieval buffer (Advanced Cell Diagnostics [ACD]) for 15 minutes, and subjected to RNAscope Proteinase III incubation at 40°C for 15 minutes. The brain slices were subsequently incubated with mRNA probes at 40°C for 2 hours. Specific signals were then amplified using a multiplexing amplification solution, and detection was carried out using the TSA Plus Fluorescence Kit (Advanced Cell Diagnostics, 322809). Subsequent quantitative analyses were performed using ImageJ software (NIH).

For cell counting of c-Fos, tdTomato, and GLP-1Rmarkers, we obtained 40 μm coronal sections from the target brain areas of each mouse. Images were captured using an Olympus Virtual Slide Microscope (VS120-S6-W). A custom MATLAB script was used for cell counting, while colocalization was visually determined. + + +

Coronal 250- to 300-μm slices containing the LS were prepared using a vibratome (Leica, VT-1000S) in an ice-cold choline-based solution containing (in mM) 110 choline chloride, 2.5 KCl, 0.5 CaCl, 7 MgCl, 1.3 NaHPO, 1.3 Na-ascorbate, 0.6 Na-pyruvate, 25 glucose, and 25 NaHCO, saturated with 95% Oand 5% CO. Slices were incubated in 32°C oxygenated artificial cerebrospinal fluid (in mM: 125 NaCl, 2.5 KCl, 2 CaCl, 1.3 MgCl, 1.3NaHPO, 1.3 Na-ascorbate, 0.6 Na-pyruvate, 25 glucose, and 25 NaHCO) for at least 1 hour before recording. Slices were transferred to a recording chamber and superfused with 2 mL/min artificial cerebrospinal fluid. Patch pipettes (2–5 MΩ) pulled from borosilicate glass (World Precision Instruments, PG10150-4) were filled with a Cs-based low-Clinternal solution containing (in mM) 135 CsMeSO, 10 HEPES, 1 EGTA, 3.3 QX-314, 4 Mg-ATP, 0.3 Na-GTP, 8 Na-phosphocreatine, 290 mOsm/kg, adjusted to pH 7.3 with CsOH. The whole-cell voltage-clamp recording was performed at room temperature with a Multiclamp 700B amplifier and a Digidata 1440A (Molecular Devices). Data were sampled at 10 kHz and analyzed with Clampfit (Molecular Devices) or MATLAB. The excitatory postsynaptic currents were recorded at a holding potential of –70 mV. 2 2 2 4 3 2 2 2 2 2 4 3 3 2 –

All experiments were conducted blinded. All statistical data can be found in the figure legends. Statistical significance was set at *< 0.05, **< 0.01, ***< 0.001, ****< 0.0001. Data are presented as means ± SEM. Sample sizes and sex distribution for figures are listed in. P P P P Supplemental Table 4

All procedures performed were approved by the Animal Care and Use Committees at the Shenzhen Institute of Advanced Technology, Chinese Academy of Sciences (CAS).

All data sets generated or analyzed during this study are included in the published article and its supplemental material. The supporting data values are available in thefile. Any additional information required to reanalyze the data reported in this paper is available upon request. Supporting Data Values