Chronic noise exposure exacerbates AD-like neuropathology in SAMP8 mice in relation to Wnt signaling in the PFC and hippocampus

Non-genetic environmental hazards are thought to be associated with genetic susceptibility factors that increase Alzheimer’s disease (AD) pathogenesis. Aging and chronic noise exposure have been considered important factors in the AD. Here, we investigated the impact of chronic noise exposure on the AD-like neuropathology in the senescence-accelerated prone mouse (SAMP8) and the underlying mechanisms of such effects. We examined the consequences of AD-like neuropathology in 3-month-old SAMP8 mice using low- and high-intensity noise exposure and 8-month-old SAMP8 mice as aging positive controls. Immunoblotting and immunohistochemistry were conducted to examine AD-like pathological changes and potential mechanisms. Chronic noise exposure led to progressive overproduction of Aβ and increased the hyperphosphorylation of tau at Ser396, Thr205, and Thr231 sites in the hippocampus and the prefrontal cortex (PFC) in young SAMP8 mice, similar to that observed in aging SAMP8 mice. Both noise exposure and aging could cause a significant downregulation in Wnt signaling expression. These findings demonstrate that chronic noise stress exacerbated AD-like neuropathology, possibly by disrupting Wnt signaling and triggering aberrant tau hyperphosphorylation and Aβ in the PFC and hippocampus.

Noise exposure set-up. All noise exposures were performed as described in the previous study 14 . Briefly, the noise was generated using a noise generator and amplified with a power amplifier and delivered through a loudspeaker. A B & K 3560 C-size front end and 4938 1/4" pressure-field microphone were used to record the exposure conditions (Brüel and Kjaer Instruments, Denmark). The main spectrum of the noise emitted from the speaker had a range of 400-6300 Hz (1/3 octave bands). Animals were exposed to noise in a reverberation chamber where wire-mesh cages were placed at the center of the sound field. A loudspeaker was suspended directly above the cages. The noise level variation was less than 2 dB within the space available to the animal. The background noise level in the chamber was below 40 dB SPL.

Determination of protein concentration by ELISA. Frozen mice hippocampi were homogenized in
ice-cold 1 x phosphate buffered saline (0.02 mol/L, pH 7.0-7.2). Total protein concentrations were determined by the bicinchoninic acid method (Boster, Wuhan, China). Protein levels for Aβ 1-40 and Aβ 1-42 were determined in hippocampal homogenates using ELISA kits (BlueGene Biotech, Shanghai, China), according to the manufacturer's recommendations (www.bluegene.cc). Concentration values of Aβ 1-40 and Aβ 1-42 were normalized to total hippocampal protein levels. All concentrations were expressed in nanograms per gram of total protein and were defined as the average of duplicates for given mice.

Detection of Aβ by thioflavin T staining.
After cardiac perfusion with 4% paraformaldehyde, brain tissues were post-fixed in 4% paraformaldehyde for 72 h, paraffin embedded, and sectioned at 5 μm. The paraffin sections were placed in GENMED reagent A for 45 min then GENMED reagent B for 9 min. Slices were placed in a dye solution (GMS 80100.1, GenMed Scientifics Lnc, USA) for 10 min then subsequently washed. Sections were coverslipped with Antifade Mounting Medium (Cat No.S2110, Solarbio) and imaged on a fluorescence microscope (Olympus DP71, Japan).
Western Blot analysis. The hippocampus preparation and Western Blot was performed as described previously 15 . Briefly, the tissue was dissected and homogenized in ice-cold radioimmunoprecipitation assay buffer (Cat No.R0020, Solarbio). Homogenates were spun at 14,000 × g for 15 min at 4 °C, and the supernatants were collected. Later, 10 μg/lane of the sample was run on 10% sodium dodecyl sulfate-polyacrylamide gels (Cat No. M00657, GenScript, USA) and transferred to microporous polyvinylidene fluoride membranes (0.45 μm, F. Hoffmann-La Roche Ltd., Germany). Immunoblots were probed with specific antibodies, as described in section 4.5, and incubated with peroxidase-conjugated species-specific anti-IgG secondary antibodies. After visualizing by enhanced chemiluminescence (EMD Millipore Co., USA), the intensity values of the immunoreactive signals were quantified by using Gel-Pro 3.1 software (Media Cybernetics Inc., USA). Statistics. Data were analyzed using SPSS v. 19.0 software (SPSS Inc., Chicago, IL, USA). To determine statistical significance in noise exposure group with the control group, we performed a one-way analysis of variance followed by an LSD-test where P < 0.05 was considered statistically significant. Then, Student's t-test was performed to determine statistical significance compared with the aging group where P < 0.05 was considered statistically significant. The data presented in the graphs indicate group means ± standard deviation.

Results
Chronic noise-induced aggregation of Aβ in the hippocampus and PFC. In order to evaluate the effect of chronic noise exposure on the production of Aβ, we performed ELISA and immunoblotting assays to determine the relative levels of Aβ 1-40, Aβ 1-42 and Aβ in hippocampus tissue. The amount of Aβ 1-40 (F (3,19) = 5.016, P = 0.012) was significantly higher both in noise exposure group and aging group (Fig. 1A). And the assessment of the Aβ 1-42 (F (3,19) = 9.007, P = 0.001) content revealed a similar trend (Fig. 1B). Expression levels of Aβ were analyzed by quantitative immunoblot analysis in hippocampal and PFC extracts in RIPA buffer from individual mice sacrificed after the end of noise exposure ( Fig. 1C and D). Expression of Aβ both in hippocampal (F (2, 11) = 13.053, P = 0.002) and PFC (F (2,17) = 67.741, P < 0.001) significantly increased after exposure to both 88 dB and 98 dB white noise for 30 days, with a more significant trend in the high-intensity noise exposure (HN) group which was close to the levels found in the aging group ( Fig. 1E and F). This indicates that chronic noise exposure accelerated senescence-related AD-like pathological alterations.
To determine the distribution patterns of Aβ in the different regions of the hippocampus and PFC, we analyzed brain paraffin sections stained with thioflavin T. Expression of Aβ was observed in Cornu Ammonis (CA) 1, Cornu Ammonis (CA) 3, and Dentate Gyrus (DG), but at low levels in the hippocampus and PFC of control mice (Fig. 1G). To a certain extent, the result of the distribution patterns of Aβ by thioflavin T well-reflected the results of our immunoblot.
Chronic noise-induced tau phosphorylation in the hippocampus and PFC. To assess the influence of chronic noise exposure on the phosphorylation of tau, western blot analysis was used to detect T-tau and phosphorylated tau (p-tau) at Ser396, Thr205, and Thr231 sites in hippocampus and PFC extracts ( Fig. 2A and F). Similar expression patterns of T-tau and p-tau were also observed in the hippocampus and PFC of noise-exposed and aging groups, with significantly increased levels at the Ser396 (hippocampus, F (  and Thr231(hippocampus, F (2,17) = 8.131, P = 0.001; PFC, F (2,17) = 620.429, P < 0.001) sites ( Fig. 2B-E,G-J). These findings indicate that chronic noise exposure aggravated tau phosphorylation in SAMP8 mice.
To determine the distribution patterns of p-tau in the hippocampus and the prefrontal cortex, we analyzed brain paraffin sections by immunofluorescence. P-tau (Thr231) immunoreactivity was observed in the CA3, DG, and cortex both in noise exposure group and aging group, but at low levels in the control group hippocampi (Fig. 3A). In noise-exposed mice, however, p-tau immunoreactivity was substantially higher in CA3 and DG pyramidal cell layers, and in the cortex cell layer compared to the control group ( Fig. 3B and C). Furthermore, we found the same results in the aging group (Fig. 3D). Thus, our immunohistochemical staining results mirrored our immunoblot results.
Next, we examined the protein levels of Dickkopf-related protein 1 (Dkk-1) and tumor protein 53 (p53). Dkk-1 inhibits Wnt signaling and is induced by p53. Statistical analysis indicated that chronic noise exposure and age significantly correlated with Dkk-1 (hippocampus, F (2,17) = 52.864, P < 0.001; PFC, F (2,17) = 53.640, P < 0.001) protein levels, manifested by a significant increase in the noise-exposure and aging groups in both the hippocampus and PFC, as well as an increase in p53 levels (hippocampus, F (2,17) = 12.542, P = 0.001; PFC, F (2,17) = 204.120, P < 0.001) (Fig. 5A-F). Taken together, these results point to a downregulation of Wnt signaling induced by chronic noise exposure and aging in the hippocampus and PFC of SAMP8 mice (Fig. 6). These results suggest that chronic noise exposure is likely to promote the adverse aging effects through the inhibition of Wnt signaling.

Discussion
Previous studies have demonstrated that acute or chronic noise exposure could induce various indicators of AD-like pathological changes 11,[16][17][18][19] that increase the risk of AD development. In this study, we evaluated the effects of chronic noise exposure in AD-like neuropathological alterations in SAMP8 mice. The present study delivers new insights into the link between noise exposure and AD. Our results represent a comprehensive description of the in vivo after-effects of noise exposure on both Aβ accumulation and tau phosphorylation in spontaneous mice of accelerated aging. Our study also implicates Wnt signaling in noise-induced augmentation of AD-like pathology in accelerated aging mice.
It was established that chronic noise exposure could induce AD-like pathology. Following noise stress, we detected significantly higher levels of Aβ protein expression in the hippocampi and PFC. According to the amyloid-cascade hypothesis of the AD, production of the more aggregate-prone Aβ42 is considered to be the key event in AD pathology 20,21 . Aβ peptides originate from proteolysis of the β-Amyloid precursor protein (APP) by the sequential enzymatic actions of β-secretase and γ-secretase 22,23 . Our previous results demonstrated that a persistent increase in Aβ(1-40) and Aβ(1-42) peptide levels and the expression of APP and β-/γ-secretase occurs in the hippocampi of rats following chronic noise exposure 19 . Notably, we confirmed the overexpression of Aβ in the hippocampus and cortex of SAMP8 mice through immunoblot and immunofluorescence. When it comes to phosphorylation tau, we found an increase in the phosphorylation level of tau protein at Ser396, Thr205, and Thr231 sites in the hippocampus and PFC extracts in both the HN group and the aging group. Therefore, there is The SAMP8 mouse is an excellent model to study both aging changes and early AD changes in comparison to the transgenic mice 24 . It has been reported that SAMP8 mice present with the cognitive deficit and other AD-like neuropathological alterations from young ages (5-6 months) 25 . Therefore, we selected 3 months SAMP8 mice to investigate the relationship between chronic noise exposure and the progression of the AD. On the other hand, we chose 8 months SAMP8 mice as aging positive control group to study if there is a possibility that chronic noise-exposure would exacerbate age-related AD-like pathology. Our data of present study showed there is a series of the AD-like neuropathological alterations in chronic noise exposed mice, as well as or even worse than that in aging mice. All of these findings indicate that chronic noise may exacerbate age-related AD-like pathology.
The molecular mechanisms of chronic noise exposure and aging on AD-like pathology seem to be complex. Growing evidence has suggested that the Wnt canonical pathway could be involved in the pathogenesis of AD [26][27][28] . On one hand, in the absence of a Wnt ligand, GSK-3β facilitates β-catenin phosphorylation, which is degraded in the proteasome leading to loss of Wnt/β-catenin signaling function 29 . GSK3β also has been shown to phosphorylate tau and may have a role in the production of paired helical filaments (PHF) in the human brain 30 . The lasting increases in GSK3β in close correspondence with increases in tau hyperphosphorylation observed in this study suggest that GSK3β might play a causal role in the induction and persistence of tau hyperphosphorylation consistent with our previous studies 12,14 . On the other hand, the Wnt pathway is neuroprotective against Aβ toxicity 31 . Active Wnt/β-catenin signaling favors the generation of non-amyloidogenic forms of APP, thereby reducing the production of the Aβ42 peptide and its aggregates 32,33 . It is interesting that the Aβ peptide that has been reported could inhibit Wnt/β-catenin signaling 34 . Otherwise, Aβ neurotoxicity significantly enhances the expression of Dkk-1 as reported in both cultured cortical neurons and brain tissue samples of AD patients 35 . In the present study, we found down-regulation of Wnt signaling in both noise exposure and aging groups. Hence, there may be a synergy between chronic noise exposure and aging in AD by inhibiting Wnt signaling.

Conclusions
In summary, our results demonstrated that chronic noise can exacerbate AD-like neuropathology in spontaneous mice of accelerated aging, which may contribute to cognitive deficits that are characteristic of neurodegenerative diseases like AD. Additionally, our findings indicate that the accelerated abnormalities in AD-like neuropathology observed in mice of accelerated aging after chronic noise is likely to be the result of dysregulation of Wnt Figure 6. A simplified model of the relationship between Wnt signaling and AD pathology. Chronic noise exposure and aging could induce activation of Dkk-1, a Wnt pathway inhibitor. In the one hand, in absence of Wnt ligands, Dvl protein expression decreased and both β-catenin and tau are phosphorylated by GSK-3β, in the other hand, without the inhibition of Wnt, the expression of Aβ significantly increased, which further exacerbates the downregulation of wnt. All of this indicates that the AD-like neuropathology observed in mice of accelerated aging after chronic noise is likely to be the result of dysregulation of Wnt signaling. Dkk-1, Dickkopf-related protein 1; Dvl, disheveled; p, phosphorylation.
SCIEnTIfIC REPORtS | (2018) 8:14622 | DOI:10.1038/s41598-018-32948-4 signaling (Fig. 6). These data suggest that genetic and environmental influences could be one mechanism behind the wide variation in the onset and progression of the AD. Further detailed studies are required to clarify the molecular mechanisms underlying the regulation of Wnt signaling in noise-induced neuropathological changes in the AD.