The APP/PS1 transgenic AD model mice were provided by the Model Animal Research Center of Nanjing University. The mice were bred in the animal center of Anhui Province. Male APP/PS1 mice were used in the present study, and age- and gender-matched WT littermates were utilized as control. Mice were housed in standard laboratory conditions with free access to standard food and water (temperature, 22–25°C; atmosphere, ~50–60%; 12-h light/dark cycle). The mice were raised in a standard laboratory with free food and water and were allowed to adapt to the laboratory conditions before testing. The experiment was performed (approval no. LLSC20211172) according to the protocol of Animal Ethics Committee of Anhui Medical University (Hefei, China).

To study the protective effects of Rg1 on APP/PS1 male mice, six-month old (WT) or APP/PS1 male mice were divided randomly into 6 groups (n=10 in each group; weight, 25–35 g): WT-9M group, APP/PS1-6M group, APP/PS1-9M model group, APP/PS1 + apocynin (50 mg/kg), APP/PS1 + Rg1 (5 mg/kg) and APP/PS1 + Rg1 (10 mg/kg) groups. Rg1 (Chengdu Desite Biotechnology Co.; Content >98%) and apocynin (Merck Millipore) were dissolved with water and were administered orally (0.1 ml/10 g) for 12 weeks. The doses of Rg1 and apocynin were reported in previous studies (26,27). The WT-9M and APP/PS1-9M groups were given equal volume of solvent for 12 weeks.

Previously, olfactory dysfunction has been reported in AD patients even in the early stages of AD (28). Therefore, the changes of olfactory dysfunction were examined using a previously described method (29). Briefly, mice were subjected to restricted diet for 24 h prior to the test. All mice were acclimated to the test chamber for 1 h prior to testing. A small piece of food was randomly placed in a corner of a clean test cage 1 cm below the bedding. The mouse was then placed in the test cage at a constant distance from the hidden food. ANY-maze behavioral tracking software was used to record the latency of the mouse to find food. If the mouse failed to find the buried food within 5 min, the latency period was recorded as 300 sec. A total of 9 h after the aforementioned experiment, surface pellet tests were performed using the same protocol, but with the pellets placed on the surface to exclude possible motor impairment.

MWM is an important method to evaluate learning and memory impairments (30). The MWM consists of a circular pool (120 cm in diameter and 60 cm in height) filled with water and a video tracking system on top. MWM test includes four training trials from first day (day 1) to day 4 and the exploration trials on day 5 as previously described (31). During the training trials, the animals were placed in the water from each of the 4 quadrants in turn and ensured that their heads were to the wall of the pool. The animals were given 60 sec to find a platform hidden underwater. If animals did not find the platform within 60 sec, they were guided to the platform and were allowed to stay on the platform for 30 sec to familiarize and memorize the location of the platform. The mean escape latency (MEL, sec) of the four trials each day was recorded to indicate the learning performance. On day 5, the platform was removed, and each mouse was detected a swimming probe trial for 60 sec from the first quadrant. The latency first to the platform (LFP, sec), the swimming time in the platform quadrant (STP, sec), and the number crossing platform (NCP) were recorded to indicate the memory results.

After behavior test, the mouse was euthanized by cervical dislocation, and the brain tissues (n=4) were removed and fixed with 4% paraformaldehyde at 4°C for 24 h. The tissues were sectioned into 5-µm after paraffin-embedded using a slicer (Leica Microsystems GmbH). The pathological changes were examined by using intelligent tissue slice imaging system (3DHISTECH) after the slice was stained with hematoxylin for 4 min and eosin for 40 sec at room temperature (RT).

The sections (n=4) were deparaffinized by xylene and were hydrated by graded alcohol. Then the slices were stained with Thioflavin-S (1%, MedChemExpress USA, HY-D0972) at 37°C for 5 min, then were hydrated with 70% ethanol. After being washed twice with PBS, the slices were stained with Hoechst 33258 at RT for 5 min. Then the slices were sealed and examined with an intelligent slice imaging system (3DHISTECH). The green density was double-blindly analyzed from 3 regions (magnification, ×400) respectively in the cortex and hippocampal CA1 by using an Image-Pro Plus 6.0 analysis system (Media Cybernetics, Inc.) to evaluate the deposition of Aβ.

Briefly, the slides (n=4) were deparaffinized and hydrated as aforementioned. Then the slides were treated with 0.25% Triton X-100 (cat. no. ST797-100 ml; Beyotime Institute of Biotechnology) at RT for 30 min, and were blocked with 1%BSA (cat. no. ST2249-5g; Beyotime Institute of Biotechnology) at RT for 60 min. Next the slides were incubated with polyclonal Aβ_1–42 (1:150; cat. no. bs-0076R; BIOSS) and post-synaptic density scaffolding protein 95 (PSD95) (1:100; cat. no. GB11277; Wuhan Servicebio Technology Co., Ltd.) antibodies overnight at 4°C. The second day, the slides were treated with a secondary antibody conjugated to Rhodamine (1:200; cat. no. ZF-0317; OriGene Technologies, Inc.) at RT for 60 min. Lastly, the slides were sealed with anti-fade medium and were imaged by an intelligent slice imaging system (3DHISTECH). The red fluorescence density was analyzed from 3 regions (magnification, ×400) respectively in the cortex and hippocampal CA1 by using an Image-Pro Plus 6.0 analysis system to evaluate the changes of PSD95 and Aβ_1-42 expression.

The slides (n=4) were deparaffinized and were hydrated as aforementioned. Then, the slides were treated with H₂O₂ (3%) at RT for 10 min to eliminate endogenous peroxidase. Afterward, the slides were treated with boiling sodium citrate buffer (3.23 g/l, pH 6.0; OriGene Technologies, Inc.) to restore antigen. Next, the slides were blocked with 10% goat serum (cat. no. C0265; Beyotime Institute of Biotechnology) for 30 min at RT and were then incubated with specific primary antibodies against Beclin1 (1:100; cat. no. 11306-1-AP) and LC3 (1:100; cat. no. 14600-1-AP; both from ProteinTech Group, Inc.) overnight at 4°C. The next day, the slides were washed with PBS three times 5 min per time and were incubated with a rabbit-general secondary antibody (1:500; cat. no. S0001; Affinity Biosciences) at RT for 1 h. The slides were stained by a DAB kit (OriGene Technologies, Inc.) to produce brownish staining. Then the slides were mounted and examined by an intelligent tissue slice imaging system (3DHISTECH). The quantification of Beclin1 and LC3 was detected blindly by using Image-Pro Plus 6.0 software from 3 fields (magnification, ×400) respectively in the cortex and hippocampal CA1.

Total protein in the hippocampus and cortex tissues (n=4) were extracted with RIPA lysis buffer (Beyotime Institute of Biotechnology) containing protease and phosphatase inhibitors by using a cryogenic tissue grinder (Shanghai Jingxin Industrial Development Co., Ltd.) 60 Hz for 50 sec, at 4°C. The protein concentration was detected by using a BCA Protein Assay kit (Beyotime Institute of Biotechnology). The proteins (20 µg) were separated by 12% SDS-PAGE and were transferred onto a PVDF membrane (MilliporeSigma). Then, the membrane was treated with 5% non-fat milk dissolved in TBS-0.05% Tween-20 (TBST) buffer at RT for 1 h and then incubated with corresponding primary antibodies overnight at 4°C: PSD95 (1:1,000), NLRP1 (1:2,000; cat. no. ab3683; Abcam), ASC (1:500; cat. no. bs-6741R; BIOSS), Caspase-1 (1:1,000; cat. no. ab1872; Abcam), IL-1β (1:1,000; cat. no. ab9722; Abcam), IL-6 (1:1,000; cat. no. 21865-1-AP; ProteinTech Group, Inc.), TNF-α (1:1,000; cat. no. WL01581; Wanleibio Co., Ltd.), AMPK (1:1,000; cat. no. AF6423; Affinity Biosciences), p-AMPK (1:1,000; cat. no. bs-4010; Bioworld Technology, Inc.), mTOR (1:1,000; cat. no. 66888-1-lg; ProteinTech Group, Inc.), p-mTOR (1:1,000; cat. no. bs-4706; Bioworld Technology, Inc.), Beclin1 (1:1,000), LC3 (1:1,000), P62 (1:500; cat. no. WL02385; Wanleibio Co., Ltd.) and β-actin (1:2,000; cat. no. GB12001; Wuhan Servicebio Technology Co., Ltd.). The second day, the membrane was washed with TBST and was incubated in secondary antibody conjugated horseradish peroxidase (1:10,000; cat. no. ZF-2301; OriGene Technologies, Inc.) at RT for 1 h. After washed with TBST, the bands were visualized by an ECL reagent (Amersham; Cytiva) and were imaged with a Chemi mini imaging system (Q4600 Mini; Shanghai Bioshine Technology; URL, http://bioshine.bioon.com.cn/). The band density of protein was examined using an ImageJ 6.0 software (National Institutes of Health). The target band density was normalized to β-actin.

The total RNAs were extracted from hippocampus and cortex tissues (n=4) by using a TRIzol^® reagent (Invitrogen; Thermo Fisher Scientific, Inc.) as previously described (32). Firstly, the cDNA was synthesized with PrimeScript™ Reverse Transcriptase buffers with dNTP (cat. no. RR037A; Takara Bio, Inc.) from total RNA. The thermocycling conditions were at 37°C for 15 min, then at 85°C for 5 sec followed by cooling to 4°C. The qPCR analyses for mRNAs of ASC, NLRP1, IL-1β, Caspase-1 and β-actin were examined with a SYBR^®Premix Ex Taq II RTPCR kit (cat. no. RR820A; Takara Bio). The level of β-actin mRNA was used as internal control. The primer sequences (TsingKe Biological Technology) were as follows: NLRP1 forward, 5′-TGGCACATCCTAGGGAAATC-3′ and reverse, 5′-TCCTCACGTGACAGCAGAAC-3′; ASC forward, 5′-GTCACAGAAGTGGACGGAGTG-3′ and reverse, 5′-CTCATCTTGTCTTGGCTGGTG-3′; Caspase-1 forward, 5′-CGTGGAGAGAAACAAGGAGTG-3′ and reverse, 5′-AATGAAAAGTGAGCCCCTGAC-3′; IL-1β forward, 5′-CTGCTTCCAAACCTTTGACC-3′ and reverse, 5′-AGCTTCTCCACAGCCACAAT-3′; and β-actin forward, 5′-GATTACTGCTCTGGCTCCTAGC-3′ and reverse, 5′-GACTCATCGTACTCCTGCTTGC-3′. The PCR protocol was at 95°C for 30 sec, followed by amplification at 95°C for 5 sec (40 cycles), then at 60°C for 30 sec. The qPCR was performed with a Real-time PCR System (cat. no. CFX96; Bio-Rad Laboratories, Inc.). The CT values of the samples were calculated, and the 2^−ΔΔCq method was used to analyze transcript levels of the target mRNAs as previously described (33).

To verify whether there is an association between Rg1 and target protein, the molecular docking between ginsenoside Rg1 and NLRP1 was monitored. Firstly, the 3D Protein Data Bank (PDB) format file of NLRP1 (PDB ID: 6XKK) was obtained from the RCSB PDB, the 2D SDF of Rg1 was downloaded (PubChem CID: 441923) from the PubChem database, and the 2D structure was imported into ChemBio3D14.0 software for structural optimization, revealing the 3D mol2 structure. Then, the drug molecules and proteins were imported into AutoDock Tool to perform hydrogenation, charge calculation, atom addition and ROOT docking. The lower binding energy indicates the improvement of the docking result. Pymol 2.5.2 software (Schrödinger, Inc.) was used to analyze the docking results.

All results were showed as the mean ± SD. The GraphPad Prism 8.0 software (GraphPad Software, Inc.) was used for statistical analysis. The results of four-day training in MWM were analyzed by repeated-measure two-way analysis of variance (ANOVA) and other data were analyzed by one-way ANOVA. Tukey's post hoc test was performed to compare the significance between groups. P<0.05 was considered to indicate a statistically significant difference.

Firstly, BFT was used to observe the effects of Rg1 on olfactory function in APP/PS mice. The buried pellet results showed that there were no differences in the latency to find the food between the WT-9M and APP/PS1-6M group mice, while in the APP/PS1-9M group mice the latency to find the food was significantly increased compared with the WT-9M group mice. Meanwhile, it was revealed that Rg1 and apocynin treatment significantly reduced the latency to find the food compared with the APP/PS1-9M group mice (Fig. 1A and B, P<0.05). Additionally, the surface pellet test showed similar results to the buried pellet test (Fig. 1C, P<0.01), suggesting that there was no motor dysfunction in the experimental mice. These results suggested that Rg1 treatment can improve olfactory dysfunction in APP/PS1 mice.

Then, MWM was conducted to examine the learning and memory ability of mice. On the first day (day 1), there was no significant difference in escape latency among the groups. With the progress of the experiment, the escape latency became increasingly shorter in the WT-9M and administration groups. While in APP/PS1-9M group, the escape latency was significantly longer than that of the WT-9M mice in days 2–4 (Fig. 2A, P<0.05 or P<0.01). Meanwhile, it was identified that the escape latency was significantly reduced by apocynin treatment in days 2–4, by Rg1 (5 mg/kg) in day 4 and Rg1 (10 mg/kg) in days 3–4 compared with APP/PS1-9M group (Fig. 2A, P<0.05 or P<0.01). On the fifth day of the probe test, the results showed that the LFP was significantly increased, the NCP and the STP were significantly decreased in APP/PS1-9M mice compared with the WT-9M group (Fig. 2B-E, P<0.05 or P<0.01). While compared with the APP/PS1-9M group, treatment with apocynin and Rg1 (5 and 10 mg/kg) could significantly reduce the LFP and increase the NCP (Fig. 2B-E, P<0.05 or P<0.01). The results indicated that Rg1 treatment can significantly improve the learning and memory impairments in APP/PS1 mice.

The H&E staining results revealed that, compared with WT-9M, there were few pathological changes in the cortex and hippocampal CA1 areas in APP/PS1-6M mice, while in APP/PS1-9M mice, neuronal damages, such as pyknosis and nucleoli inconspicuous (black arrows) and Aβ plaques (yellow arrows), were increased in the cortex and hippocampal CA1 (Fig. 3). Compared with APP/PS1-9M, treatment with apocynin and Rg1 (5 and 10 mg/kg) could alleviate the neuronal damages in the cortex and hippocampal CA1 (Fig. 3). The results indicated that Rg1 treatment could improve neuronal damages in APP/PS1 mice.

To confirm the effect of Aβ deposition, the Thioflavin-S staining and immunofluorescence were conducted to detect the Aβ deposition and Aβ_1–42 level. The Thioflavin-S staining results demonstrated that there was a small amount of Aβ deposition in the cortex and hippocampal CA1 in APP/PS1-6M mice, while in APP/PS1-9M mice, the Aβ depositions (yellow arrows) were significantly increased compared with WT-9M (Fig. 4A-C, P<0.05 or P<0.01). Compared with APP/PS1-9M, treatment with apocynin and Rg1 could significantly reduce Aβ depositions in the cortex and hippocampal CA1 (Fig. 4A-C, P<0.05 or P<0.01). The immunofluorescence results of Aβ_1–42 were similar to that of Thioflavin-S staining, suggesting that Aβ_1–42 expression was significantly increased in APP/PS1-9M mice, and was significantly downregulated by apocynin and Rg1 treatment in the cortex and hippocampal CA1 (Fig. 4D-F, P<0.05 or P<0.01). The results indicated that Rg1 treatment decreases Aβ generation and deposition in APP/PS1 mice.

AD models not only have Aβ deposition, but also are accompanied by synaptic dysfunction (34). Therefore, the expression of PSD95 was detected by immunofluorescence and immunoblot analysis. The immunofluorescence results showed that the expression of PSD95 was significantly decreased in the cortex and hippocampal CA1 in both APP/PS-6M and APP/PS1-9M mice compared with WT-9M mice, particularly in APP/PS1-9M mice (Fig. 5A-C, P<0.01). After Apocynin and Rg1 treatment, the expression of PSD95 was significantly increased in the cortex and hippocampal CA1 (Fig. 5A-C, P<0.01). The immunoblot results of PSD95 were similar to that of immunofluorescence results, suggesting that the expression of PSD95 was significantly decreased in APP/PS-6M and APP/PS1-9M mice, and was significantly increased after Apocynin and Rg1 treatment (Fig. 5D, P<0.05 or P<0.01). These results indicated that Rg1 treatment can improve synaptic dysfunction in APP/PS1 mice.

It has been reported that NLRP1 inflammasome is involved in learning and memory impairments and neuronal damages during the aging process in mice (19). Therefore, the effect of Rg1 treatment on the expression of NLRP1 inflammasome proteins was further examined through immunoblot and RT-qPCR. The results showed that, compared with WT-9M, there was no significant increase in the expression of NLRP1 inflammasome-related proteins in the APP/PS1-6M group. While in the APP/PS1-9M group, the expression levels of NLRP1, ASC, caspase-1, IL-1β, IL-6 and TNF-α were significantly increased. Compared with the APP/PS1-9M group, after apocynin and Rg1 treatment, the expression levels of these proteins were significantly downregulated (Fig. 6A-H, P<0.05 or P<0.01). Similar results were observed using qPCR; the levels of NLRP1, ASC, caspase-1 and IL-1β mRNA were significantly increased in the APP/PS1-9M mice and were significantly decreased after apocynin and Rg1 treatment (Fig. 7A-D, P<0.05 or P<0.01). These results suggested that Rg1 treatment can inhibit NLRP1 inflammasome in APP/PS1 mice.

Autophagy also plays important roles in Aβ generation and metabolism, and its malfunction is involved in the progress of AD (35). Therefore, the effect of Rg1 on autophagy function in APP/PS mice was further studied. The results showed that there were no significant differences in the expression levels of p-AMPK/AMPK, p-mTOR/mTOR, Beclin1, LC3 II/LC3 I and P62 in APP/PS1-6M mice compared with WT-9M. While in APP/PS1-9M mice, the levels of p-AMPK/AMPK, Beclin1 and LC3 II/LC3 I were significantly increased, and the levels of p-mTOR/mTOR and P62 were significantly decreased (Fig. 8A-G, P<0.05 or P<0.01). Moreover, apocynin and Rg1 treatment could significantly reverse the changes of these proteins in APP/PS1 mice (Fig. 8A-G, P<0.05 or P<0.01). Furthermore, the expression levels of Beclin1 and LC3 were detected by immunohistochemistry. There were similar results that the expression levels of Beclin1 and LC3 were increased in APP/PS1-9M mice and were significantly decreased after Rg1 treatment in cortex and hippocampus CA1 (Figs. S1 and S2, P<0.05 or P<0.01). These results indicated that Rg1 treatment can improve autophagy dysfunction in APP/PS1 mice.

Molecular docking was used to further verify the interaction between Rg1 and NLRP1. The results showed that several hydrogen bonds may form between Rg1 and NLRP1 (Fig. S3A and B). Meanwhile, the binding energy (affinity: −5.31 kcal/mol) in the docking analysis showed favorable binding results between Rg1 and NLRP1 (Fig. S3C).