Naringenin and lipopolysaccharide (LPS) were purchased from Sigma-Aldrich (St. Louis, MO, USA). MTT assay kit was obtained from Beijing Solarbio science and Technology Co., Ltd (Beijing, China). Enzyme-linked Immunosorbant assay (ELISA) kits for TNF-α, IL-1β, and IL-18 were bought from Elabscience Biotechnology Co., Ltd (Wuhan, China). Dulbecco's modified Eagle medium (DMEM) and OPTI-MEM were obtained from Gibco-BRL (Invitrogen Life Technologies, Carlsbad, USA). Anti-tyrosine hydroxylase (TH, Catalog No. Ab41528) and OX-42 (Catalog No. Ab1211) antibodies were purchased from Abcam (Cambridge, MA, USA). Anti-caspase-1 (Catalog. No. 22915-1-AP), ionized calcium-binding adapter molecule-1 (Iba-1, Catalog. No. 10904-1-AP), β-actin (Catalog. No. 20536-1-AP), Rabbit IgG (Catalog. No. SA00001-2), and mouse IgG (Catalog. No. SA00001-1) antibodies were purchased from Proteintech Group (Chicago, IL, USA). Anti-NLRP3 (Catalog. No. orb101128) antibody was purchased from Biorbyt (Cambridge, United Kingdom). Anti-ASC (Catalog. No. 67824) antibody was obtained from Cell Signaling Technology, Inc. (Beverly, MA, USA). The small interfering RNA (siRNA) against NLRP3 was purchased from GenePharma (Shanghai, China).

Adult male Sprague-Dawley rats (220–260 g) were purchased from the Experimental Animal Center of the Third Military Medical University (Chongqing, China; Specific pathogen-free Grade II; Certificate No. SCXK 2012-0011). All animal experiments were performed in accordance with Chinese Guidelines of Animal Care and Welfare and the present study was approved by the Animal Care and Use Committee of Zunyi Medical University (Zunyi, China). All the animals were housed in a temperature (25 ± 2°C) and humidity (60 ± 4%) environment, and given access to food and water ad libitum. Rats were acclimated to their environment for 1 week before the experiments. All the animals were randomly allocated to five experimental groups with six rats in each group: control (0.9% NaCl), NAR alone (100 mg/kg), LPS, LPS + NAR (50 mg/kg), and LPS + NAR (100 mg/kg). With anesthetized by 7% chloral hydrate (0.5 ml/100 g, v/w), rats received a single LPS (5 μg in 5 μl PBS) unilateral injection into the SN pars compacts followed by the coordinates 4.8 mm posterior to bregma, 1.7 mm lateral to the midline, and 8.2 mm ventral to the surface of the skull (20, 21). After seven daily intragastric administration of NAR, rat behavior was analyzed by rotarod test and then animals were sacrificed.

After rat motor performance was finished, rats were deeply anesthetized by 7% chloral hydrate, and transcardially perfused with cold PBS before 4% formaldehyde was used to fix. Then, brains were removed and post fixed with 4% formaldehyde for 48 h. Next, formaldehyde (4%) was replaced by 30% sucrose solution at 4°C until tissues sank. Brains were cut into 35-mm using a horizontal sliding microtome. A total of 36 consecutive brain slices through the entire SN was collected and used for the immunohistochemistry staining by every sixth section (22). DA neurons were recognized with an anti-TH antibody and microglia with OX-42. In brief, the brain slices were first treated with 0.3% Triton X-100 for 30 min and blocked with goat serum. Then, the slices were incubated overnight at 4°C with the following primary antibodies: TH (1: 800), OX-42 (1:800), and NLRP3 (1:800). Afterwards, brain tissues were incubated in fluorescent-conjugated secondary antibody for 1 h. Digital images of TH-positive neurons, OX-42-positive microglia and NLRP3-positive inflammasome in the SN were acquired by an Olympus microscope (Olympus, Tokyo, Japan) via an attached Polaroid digital microscope camera (Polaroid, Cambridge, MA, USA). Quantification of TH-positive neurons was determined by visually counting the number of TH-positive neuronal cell bodies. Activation of microglia and NLRP3 inflammasome was detected by the fluorescence intensity analysis of OX-42-positive microglia and NLRP3-positive inflammasome, respectively. The results were obtained from the average. The mean value was deduced by averaging the counts of six sections for each rat.

BV-2 cells (microglia cell lines) were purchased from the Cell Culture Center in the Institute of Basic Medical Sciences of Chinese Academy of Medical Sciences (Wuhan, China). MN9D cells (DA neuron cell line) were purchased from the Cell Culture Center in the Institute of Basic Medical Sciences of Chinese Academy of Medical Sciences (Beijing, China). BV-2 cells were cultured in MEM medium with 10% fetal bovine serum (FBS) and 1% penicillin-streptomycin on an atmosphere with 5% CO₂ at 37°C, while MN9D cells were cultured in DMEM medium. BV-2 cells were treated with different concentrations of NAR for 1 h followed by LPS treatment for an additional 24 h. Then, cells and culture medium were collected for the later indexes detection.

Cells were cultured in 1 × 10⁵/well in 96-well plates for 24 h. Subsequently, the conditioned medium was replaced by a new medium with 2% FBS and then cells were exposed to LPS with or without NAR for another 24 h. Afterwards, 3-(4, 5-dimethylthiazol-2-yl)- 2,5-diphenyltetrazoliumbromide (MTT) was applied to determine cell viability. The absorbance was detected by an automated microplate (Sunnyvale, CA, USA) reader within 550 nm wavelength.

The levels of TNF-α, IL-1β, and IL-18 were measured by ELISA according to the manufacturer's instructions. The microplate reader was used to measure the absorbance at 450 nm.

BV-2 cells were transfected with siRNA oligos against NLRP3. Cells were seeded on 24-well plates for 24 h. GP-siRNA-Mate plus was used to transfect with siRNAs. After 6 h of transfection, the transfection solution was removed and cells were rinsed with PBS and then replaced with MEM medium containing 2% FBS followed by treatment of NAR and/or LPS.

Rotarod test was assessed by studying the muscular coordination with cylindrical arrangement of thin steel rods contained. First, rats were trained to adapt at a speed of 10 rpm/min before the experiment start. After intragastric administration of NAR for 7 days, the rods were divided into two parts with compartmentalization. With speed accelerating from 10 to 30 rpm over a period of 5 min, two rats were detected at the same time and the duration time each rat stayed on the rod was recorded and calculated for analyzing the behavior changes of rats.

The total protein content was extracted from rat midbrain tissue and BV-2 cells using a lysis buffer containing protease inhibitors. The protein concentration was measured by the BCA protein assay. Equal amounts of protein were separated by sodium dodecyl sulfate/polyacrylamide gel electrophoresis and transferred to a polyvinylidene fluoride membrane. The membrane was blocked in TBS with Tween 20 containing 5% non-fat dry milk for 4 h and probed with primary antibodies overnight at 4°C and incubated with the following primary antibodies: TH (1:1,000), Iba-1 (1:800), NLRP3 (1:1,000), ASC (1:400), caspase-1 (1:800), β-actin (1: 2,000), and then incubated for 1 h with a horseradish-peroxidase-conjugated anti-mouse IgG antibody or anti-rabbit IgG at 1:2,000 dilution. Protein bands were visualized on X-ray film by utilizing an enhance chemiluminescence system before the enhanced ECL reagent used.

Data were indicated as mean ± standard error of the mean (SEM). Statistical significance was analyzed by one-way analysis of variance (ANOVA) using GraphPad Prism software (GraphPad Software Inc., San Diego, CA, USA). With ANOVA demonstrating the significant differences, pairwise comparison between means was evaluated by Bonferroni's post-hoc test with correction. A value of p < 0.05 was considered statistically significant.

After seven daily intragastric administration of NAR, rat behavior changes were analyzed by rotarod test. As shown in Figure 1A, LPS decreased the time rat stayed on the rod (54.86 ± 5.72%; t = 5.683, p < 0.05) and NAR attenuated LPS-induced decrease in the time rat remained on the rod (164.14 ± 8.48%; t = 3.935, p < 0.05). Results from DA neuronal counting and densitometric analysis as indicated in Figures 1B,C, LPS reduced DA neuronal loss compared with control group (52.64 ± 6.27%; t = 5.811, p < 0.05) and this reduction was inhibited by NAR treatment in a dose-dependent manner (170.62 ± 11.35%; t = 3.937, p < 0.05). To further confirm NAR-mediated DA neuroprotection, the effects of NAR on TH protein expression after LPS treatment were determined. As shown in Figure 1D, NAR ameliorated LPS-induced decrease in TH protein expression (145.93 ± 20.72%; t = 3.110, p < 0.05).

Next, we investigated the effects of NAR on microglia-induced neuroinflammation. Double-Immunofluorescence analysis was performed to determine the co-location of microglia and NLRP3 inflammasome. As shown in Figure 2A, in parallel with DA neuronal loss, LPS induced microglia activation and the activated state of microglia was suppressed by NAR. Since the activation of NLRP3 inflammasome was involved in the modulation of neuroinflammatory responses, the effects of NAR on LPS-elicited NLRP3 inflammasome activation were detected. As shown in Figure 2B, the activation of NLRP3 inflammasome was located in activated microglia and NAR could inhibit LPS-induced microglial (63.11 ± 3.78%; t = 11.01, p < 0.05) and NLRP3 inflammasome activation (63.41 ± 3.85%; t = 11.47, p < 0.05). Also, as shown in Figure 2C, NAR decreased LPS-induced protein expressions of Iba-1 (19.18 ± 5.59%; t = 7.982, p < 0.05), NLRP3 (59.36 ± 3.72%; t = 3.295, p < 0.05), and caspase-1 (62.78 ± 3.13%; t = 6.802, p < 0.05). As shown in Supplementary Figure 2, NAR decreased LPS-induced protein expressions of pro-IL-1β (p < 0.05) and IL-1β mRNA (p < 0.05).

To further confirm the inhibitory actions of NAR on microglia-elicited neuroinflammation, BV-2 cells were employed to examine the effects of NAR on LPS-induced microglial activation. First, MTT assay showed that LPS (0.01–1 μg/ml) and NAR (1–100 μM) had no significant cytotoxicity (Figure 3A). Second, microglia in LPS-treated cultures presented an enlarged cell body and irregular status from resting round and small cells in control cultures to the highly activated amoeboid shapes. NAR attenuated LPS-induced microglial activation (Figure 3B). Moreover, NAR suppressed LPS-induced Iba-1 protein expression (50.22 ± 0.28%; t = 11.75, p < 0.05) (Figure 3C). Then, the inhibitory ability of NAR on the production of microglial pro-inflammatory factors was assessed. As shown in Figure 3D, NAR reduced LPS-induced production of NO (19.61 ± 4.82%; t = 14.40, p < 0.05), IL-1β (69.27 ± 3.88%; t = 6.365, p < 0.05), and IL-18 (42.71 ± 2.15; t = 9.588, p < 0.05) in the culture medium.

The effects of NAR on microglial NLRP3 inflammasome activation were further confirmed. As shown in Figure 4A, LPS induced NLRP3 inflammasome activation, and this activated state of NLRP3 inflammasome was attenuated by NAR treatment. Similarly, NAR inhibited LPS-induced activation of NLRP3 (74.58 ± 1.07%; t = 3.634, p < 0.05) and caspase-1 (62.97 ± 10.47%; t = 2.647, p < 0.05) (Figure 4B).

To investigate the role of NLRP3 inflammasome on NAR-mediated anti-inflammatory properties, NLRP3 siRNA (Nlrp3-Mus-727 siRNA oligo) was applied in the cell cultures. The successful transfection with NLRP3 siRNA was verified by NLRP3 protein level in cells (28.09 ± 4.84%, p < 0.05) (Figure 5A). Meanwhile, as shown in Figure 5B, LPS still induced NLRP3 activation after NLRP3 siRNA treatment compared with cells only treated with NLRP3 siRNA (264.03 ± 31.40%; t = 4.269, p < 0.05) but the lower NLRP3 activation was shown in LPS+NLRP3 siRNA than that in LPS alone treatment cultures (60.70 ± 7.23%; t = 4.741, p < 0.05). However, no significant difference of NLRP3 protein expression between LPS+NLRP3 siRNA and LPS+NAR+NLRP3 siRNA was detected. Furthermore, the effects of NAR on pro-inflammatory factors release after NLRP3 siRNA treatment were determined. As shown in Figure 5C, LPS also increased the production of NO (177.75 ± 13.48%; t = 1.906%, p < 0.05), IL-1β (144.18 ± 7.80%; t = 4.200, p < 0.05), and IL-18 (144.22 ± 7.58%; t = 3.733, p < 0.05) after NLRP3 siRNA treatment but this increase was not inhibited after NAR administration. Collectively, these results suggested that NLRP3 inflammasome was involved in NAR-exerted anti-neuroinflammatory actions.

To further observe the link of inhibition of microglial activation with NAR-mediated DA neuroprotection, microglia-conditioned medium (MCM) was prepared from BV-2 cell cultures and added back to MN9D cell cultures. First, cell viability assay (Figure 6A) indicated that direct application of LPS on MN9D cells had no significant neurotoxicity, whereas MCM (LPS) caused neuronal damage (67.10 ± 1.78 %; t = 9.251, p < 0.05). Additionally, compared with MCM (LPS) group, MCM (LPS+NAR) produced neuroprotection from MCM (LPS)-induced neurotoxicity (139.92 ± 3.62%; t = 7.482, p < 0.05). However, with MN9D cells treated with MCM (LPS) followed by NAR treatment, no neuroprotection was exhibited. Results from TH protein expression detection were consistent with cell viability assay (Figure 6B), which together implied that NAR-mediated DA neuroprotection was microglia-dependent.

Since microglia were the target of NAR-produced neuroprotection, we next examined whether NAR-mediated DA neuroprotection was attributable to inhibition of microglial NLRP3 inflammasome activation. As shown in Figure 7A, compared with MCM (LPS) group, MCM (LPS+NLRP3 siRNA) (136.79 ± 3.73%; t = 8.852, p < 0.05) and MCM (LPS+NAR) (138.42 ± 3.43%; t = 7.474, p < 0.05) protected against MCM (LPS)-induced neurotoxicity, while no significant difference of cell viability between these two groups was indicated. Compared with MCM (LPS + NLRP3 siRNA) and MCM (LPS + NAR) groups, MCM (LPS + NAR+NLRP3 siRNA) didn't produce more neuroprotection from MCM (LPS)-elicited neuronal damage. Similar observation was demonstrated in TH protein expression assessment (Figure 7B).

The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.