Ferulic Acid Suppresses Amyloid <i>β</i> Production in the Human Lens Epithelial Cell Stimulated with Hydrogen Peroxide

Nagai, Noriaki; Kotani, Sachiyo; Mano, Yu; Ueno, Akina; Ito, Yoshimasa; Kitaba, Toshio; Takata, Takumi; Fujii, Noriko

doi:https://doi.org/10.1155/2017/5343010

BioMed Research International

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Abstract Introduction Materials and Methods Results Discussion Conclusions Conflicts of Interest Acknowledgments References Copyright Related Articles

Research Article | Open Access

Volume 2017 | Article ID 5343010 | https://doi.org/10.1155/2017/5343010

Ferulic Acid Suppresses Amyloid β Production in the Human Lens Epithelial Cell Stimulated with Hydrogen Peroxide

Noriaki Nagai,¹Sachiyo Kotani,¹Yu Mano,¹Akina Ueno,¹Yoshimasa Ito,¹Toshio Kitaba,²Takumi Takata,³and Noriko Fujii³

Academic Editor: Cheng-Xin Gong

Received21 Nov 2016

Revised13 Feb 2017

Accepted26 Feb 2017

Published20 Mar 2017

Abstract

It is well known that oxidative stresses induce the production of amyloid β (Aβ) in the brain, lens, and retina, leading to age-related diseases. In the present study, we investigated the effects of ferulic acid on the Aβ levels in H₂O₂-stimulated human lens epithelial (HLE) SRA 01/04 cells. Three types of Aβ peptides (Aβ_1-40, Aβ_1-42, and Aβ_1-43) were measured by ELISA, and the levels of mRNA for the expressed proteins related to Aβ production (APP, BACE1, and PS proteins) and degradation (ADAM10, NEP, and ECE1 proteins) were determined by quantitative real-time RT-PCR. H₂O₂ stimulation augmented gene expression of the proteins related to Aβ production, resulting in the production of three types of Aβ peptides. Treatment with 0.1 μM ferulic acid attenuated the augmentations of gene expression and production of the proteins related to the secretion of three types of Aβ peptides in the H₂O₂-stimulated HLE cells. These results provided evidence of antioxidative functions of ferulic acid for lens epithelial cells.

1. Introduction

A sequential proteolytic processing of amyloid precursor protein (APP) cleaved by β-secretase (β site APP cleaving enzyme, BACE1) [1] and γ-secretase [a presenilin complex (PS)] [2] leads to the production of amyloid β (Aβ) peptides. The cleavage of APP at different positions by γ-secretase mainly produces three Aβ peptides, Aβ_1–40, Aβ_1–42, and Aβ_1–43 peptides [3–7]. The most abundant variant of Aβ is Aβ_1–40, but Aβ_1–42 and Aβ_1–43, the longer forms, are more neurotoxic than Aβ_1–40. In addition, the neurotoxicity of Aβ_1–43 is higher than that of Aβ_1–42, although the accumulation of Aβ_1–43 is lower than that of Aβ_1–42 [7]. However, the APP cleaved by α-secretase (a disintegrin and metalloprotease domain protease 10, ADAM10) generates nonamyloidogenic soluble APPα [8–10]. Neprilysin (NEP) [11] and endothelin converting enzyme (ECE) [12] degrade the Aβ peptide. The production of Aβ is a normal process; however, the overproduction of Aβ, or an increased proportion of Aβ_1–42 and Aβ_1–43, appears to cause an early onset of cataract and Alzheimer’s disease [13, 14].

Cataract represents a disease of increasing lens opacity, and it has been reported that Aβ accumulation in the human lens causes lens opacification [15–18]. In addition, there have been several reports that oxidative stress can increase the accumulation and toxicity of Aβ peptides in the lens, retina, and brain and that enhanced Aβ accumulation leads to oxidative stress [14, 19–24]. Therefore, it is expected that drugs that inhibit the effect of Aβ peptides and lower oxidative stress can be used as anticataract eye drops.

Ferulic acid (4-hydroxy-3-methoxycinnamic acid) is a widely distributed constituent of plants and is used as an antioxidant to prevent the oxidation of substrates such as lipids, proteins, DNA, and carbohydrates [25, 26]. Ferulic acid has been shown to possess some scavenging activity toward hydroxyl radicals and peroxynitrite [27, 28]. Recently, several studies have shown that ferulic acid has beneficial effects against Alzheimer’s disease [29–31], diabetes [32], and cancer [33]. Alzheimer’s disease is a neurodegenerative disorder, and it had been shown that one of the main pathophysiological features of Alzheimer’s disease was the presence of extracellular senile plaques consisting essentially of Aβ, a peptide thought to be a leading cause of neurotoxicity [34]. It was reported that ferulic acid could be a suitable molecule to specifically bind to Aβ and inhibit fibril formation [35]. Furthermore, its compact structure could also be used for specific interactions with Aβ mature fibrils, thereby possibly promoting their destabilization [35]. Ferulic acid inhibits Aβ aggregation, destabilizes preformed Aβ fibrils in vitro [36], and protects cultured neuronal cells against Aβ-induced cytotoxicity [29]. Moreover, long-term administration of ferulic acid protects mice against Aβ-induced learning and memory deficits in vivo [30, 31]. Therefore, ferulic acid may be a useful molecule for the inhibition of Aβ production and accumulation.

In this study, we investigated the changes in Aβ production and accumulation in human lens epithelial (HLE) SRA 01/04 cells stimulated with hydrogen peroxide (H₂O₂). In addition, we demonstrated the preventive effects of ferulic acid on Aβ production and accumulation in HLE cells.

2. Materials and Methods

2.1. Cell Culture and Treatment

The HLE cell line SRA 01/04 was incubated in Dulbecco’s Modified Eagle’s Medium (DMEM) containing 10 μg/L gentamicin and 10% (v/v) fetal bovine serum (FBS) under humidified air containing 5% CO₂, at 37°C. Each treatment was usually carried out on the third day after seeding of 0.4 × 10⁴ cells/cm² (at approximately 80% confluency), and the culture medium was changed to non-FBS medium 1 hour before each experiment. The experiment was initiated by changing the medium to fresh medium containing 0–100 μM of H₂O₂ and the HLE cells were cultured for 24 hours to produce Aβ_1–40, Aβ_1–42, and Aβ_1–43 (H₂O₂-stimulated HLE cells). Ten μM of H₂O₂ and 0–30 μM of ferulic acid included in the medium were used for 24-hour cultures to observe the effect of ferulic acid on Aβ production (H₂O₂-stimulated HLE cells in the presence of ferulic acid).

2.2. Quantitative Real-Time RT-PCR

The experiment was performed as described previously [14, 37]. Briefly, extraction and purification of the total RNA from HLE cells were performed using an RNase-Free DNase kit and an RNeasy Mini kit (Qiagen, Tokyo, Japan), and an RNA PCR kit (AMV Ver. 3.0, Takara Bio Inc., Shiga, Japan) was used for the reaction according to the manufacturer’s instructions. Total RNA (1 μg, OD₂₆₀/OD₂₈₀ values > 1.8) was used for the reverse transcription (RT) reaction, and the reaction was performed at 42°C for 15 min, followed by 5 min at 95°C. The PCR reactions were performed using LightCycler® FastStart DNA Master SYBR Green I according to the manufacturer’s instructions (Roche Diagnostics Applied Science, Mannheim, Germany), and the quantities of the PCR products were measured fluorometrically in a real-time manner using a LightCycler® DX 400 (Roche Diagnostics Applied Science). In this study, the specific primers (10 pmol) for APP, BACE1, PS1, PS2, ADAM10, NEP, ECE1, or glyceraldehyde-3-phosphate dehydrogenase (GAPDH) were as follows: 5′-TGGTGGGCGGTGTTGTCATA-3′ (forward; FOR) and 5′-TGGATTTTCGTAGCCGTTCTGC-3′ (reverse; REV) for APP; 5′-GCAAGGAGTACAACTATGAC-3′ (FOR) and 5′-AGCTTCAAACACTTTCTTGG-3′ (REV) for BACE1; 5′-ATCATCTGCATAGTCCTCTC-3′ (FOR) and 5′-AGACAGCTTTGATGTTCAAG-3′ (REV) for PS1; 5′-TACAAGTACCGCTGCTACAAGTTC-3′ (FOR) and 5′-GCACTTCCCCAAGGTAGATATAGG-3′ (REV) for PS2; 5′-CACATGATTCTGGAACAGAG-3′ (FOR) and 5′-GTTGTTAAGTTTGTCCCCAG-3′ (REV) for ADAM10; 5′-CTGATATCAACACTCCAAAGC-3′ (FOR) and 5′-TCATCGTAGGTTGCATAGAG-3′ (REV) for NEP; 5′-AGAATGAGATTGTGTTTCCG-3′ (FOR) and 5′-CTATGCCACCAAAGTTTAAGG-3′ (REV) for ECE1; and 5′-TGCACCACCAACTGCTTAGC-3′ (FOR) and 5′-GGCATGGACTGTGGTCATGAG-3′ (REV) for GAPDH. The conditions for PCR were 95°C for 10 min (hot start), 60 cycles of 95°C for 10 s (denaturing), 63°C for 10 s (annealing), and 72°C for 5 s (extension). The differences in the threshold cycles for target groups (APP, BACE1, PS1, PS2 ADAM10, NEP, and ECE1) and GAPDH were used to calculate the levels of mRNA expression in HLE cells.

2.3. Measurement of Aβ

The measurements of Aβ_1–40, Aβ_1–42, and Aβ_1–43 levels were performed as previously described [14, 38]. Approximately 2.5 × 10⁶ HLE cells were collected with a cell scraper (Asahi Glass, Tokyo, Japan), homogenized in 250 μL of 70% formic acid, and then centrifuged at 9,100 ×g for 15 min at 4°C. The supernatants were added to 4.75 mL of 1 M Tris base, and the mixtures were used for the measurements of the Aβ_1–40, Aβ_1–42, and Aβ_1–43 peptides. The Aβ_1–40, Aβ_1–42, and Aβ_1–43 levels were measured using the human β amyloid (40) ELISA kit (dynamic range, 1–100 pM, Wako, Osaka, Japan), the human β amyloid (42) ELISA kit (dynamic range, 0.1–20 pM, Wako), and the human amyloid β (1–43) (FL) ELISA kit (dynamic range, 0.51–32.5 pM, IBL, Gunma, Japan) according to the manufacturer’s instructions, respectively. The Aβ levels were expressed as pmol/g of protein according to our previous reports. The protein levels in the samples used to determine Aβ_1–40, Aβ_1–42, and Aβ_1–43 were assessed using a Bio-Rad Protein Assay kit (Bio-Rad, Hercules, CA, USA).

2.4. Measurement of Cell Viability

HLE cells with or without added H₂O₂ and ferulic acid treatments were incubated in 96-well microplates (Iwaki, Chiba, Japan). The viability of the HLE cells was calculated by the Cell Count Reagent SF kit (Nacalai Tesque, Kyoto, Japan) according to the manufacturer’s instructions. The absorbance at 450 nm was measured, and the cell viability (%) was represented as the percentage of the absorbance measured for unstimulated HLE cells for each point (normal cells).

2.5. Statistical Analyses

All values were presented as mean ± standard error (SE), and statistical differences were evaluated by one-way analysis of variance followed by Dunnett’s multiple comparisons. P values of less than 0.05 were considered significant.

3. Results

3.1. The Effect of H₂O₂ Stimulation on Aβ Production and Accumulation in HLE Cells

Figures 1(a)–1(c) shows the levels of Aβ accumulation in the H₂O₂-stimulated HLE cells. The Aβ_1–40 and Aβ_1–42 levels were enhanced with increasing H₂O₂ concentration. Although the Aβ_1–43 was not detected in the unstimulated HLE cells, an accumulation of Aβ_1–43 was observed with stimulation by 10–100 μM H₂O₂. Figure 1(d) shows the cell viability in the H₂O₂-stimulated HLE cells. The cell viability in the 1 μM and 10 μM H₂O₂-stimulated HLE cells was similar to that of the unstimulated HLE cells (None). However, the HLE cell viabilities in the presence of 50 μM and 100 μM H₂O₂ were decreased, and the cell viability at 100 μM H₂O₂ was significantly lower than that of the untreated cells (None). Figure 2 shows the mRNA levels for proteins related to Aβ production (APP, BACE1, PS1, and PS2) and to degradation (ADAM10, NEP, and ECE1) in the H₂O₂-stimulated HLE cells. APP, BACE1, and PS1 mRNAs were increased with increasing concentrations of H₂O₂, while PS2 mRNA levels were not altered. The H₂O₂ stimulation did not change the mRNA levels of proteins related to Aβ degradation (ADAM10, NEP, and ECE1).

(a) Aβ1–40 levels

(b) Aβ1–42 levels

(c) Aβ1–43 levels

(d) Cell viability

(a) APP mRNA

(b) BACE1 mRNA

(c) PS1 mRNA

(d) PS2 mRNA

(e) ADAM10 mRNA

(f) NEP mRNA

(g) ECE1 mRNA

3.2. The Preventive Effects of Ferulic Acid on Enhanced Aβ Production and Accumulation in H₂O₂-Stimulated HLE Cells

Figures 3(a)–3(c) show the effects of ferulic acid on the specific Aβ levels in the 10 μM H₂O₂-stimulated HLE cells. At 0.01–0.1 μM of ferulic acid, Aβ levels were relatively decreased in the H₂O₂-stimulated HLE cells. However, at 30 μM of ferulic acid, the Aβ levels were higher than those at 0.1 μM of ferulic acid; thus, the preventive effects of the Aβ level increase peaked at 0.1 μM of ferulic acid. Figure 3(d) shows the effect of ferulic acid on cell viability in the H₂O₂-stimulated HLE cells. A decrease in cell viability was not observed at 0.01–30 μM of ferulic acid. Figure 4 shows the effects of ferulic acid on the mRNA levels for proteins related to Aβ production (APP, BACE1, PS1, and PS2) and degradation (ADAM10, NEP, and ECE1) in the H₂O₂-stimulated HLE cells. Ferulic acid decreased the mRNA levels of APP, BACE1, and PS1. However, the mRNA levels of PS2 and the mRNA levels for proteins related to Aβ degradation (ADAM10, NEP, and ECE1) in HLE cells treated with ferulic acid were similar to the HLE cells without ferulic acid treatment.

(a) Aβ1–40 levels

(b) Aβ1–42 levels

(c) Aβ1–43 levels

(d) Cell viability

Figure 3

The effect of ferulic acid on Aβ_1–40 (a), Aβ_1–42 (b), Aβ_1–43 (c), and cell viability (d) in 10 μM H₂O₂-stimulated HLE cells. The 10 μM H₂O₂ and 0–30 μM ferulic acid were added simultaneously to the medium, and the HLE cells were incubated for 24 h. Open columns = H₂O₂-stimulated HLE cells. Closed columns = H₂O₂-stimulated HLE cells with ferulic acid treatment. The data are presented as the means ± SE of 5–8 experiments. , versus H₂O₂-stimulated HLE cells in the absence of ferulic acid (open columns) for each category.

(a) APP mRNA

(b) BACE1 mRNA

(c) PS1 mRNA

(d) PS2 mRNA

(e) ADAM10 mRNA

(f) NEP mRNA

(g) ECE1 mRNA

Figure 4

The effect of ferulic acid on mRNA levels of APP (a), BACE1 (b), PS1 (c), PS2 (d), ADAM10 (e), NEP (f), and ECE1 (g) in H₂O₂-stimulated HLE cells. The 10 μM H₂O₂ and 0–30 μM ferulic acid were added simultaneously to the medium, and the HLE cells were incubated for 24 h. Open columns = H₂O₂-stimulated HLE cells. Closed columns = H₂O₂-stimulated HLE cells with ferulic acid treatment. The data are presented as the means ± SE of 5–8 experiments. , versus H₂O₂-stimulated HLE cells in the absence of ferulic acid (open columns) for each category.

3.3. The Effects of Ferulic Acid on Aβ Production and Accumulation in HLE Cells

Because 0.1 μM of ferulic acid showed the greatest suppression of the production of Aβ, we further determined the impact of 0.1 μM of ferulic acid on the HLE cells without H₂O₂ stimulation (Figure 5). As shown in Figure 5, the Aβ_1–43 level was not detected by the HLE cells treated with or without 0.1 μM ferulic acid, and Aβ_1–40 levels and the mRNA levels of proteins related to Aβ production (APP, BACE1, PS1, and PS2) and degradation (ADAM10, NEP, and ECE1) were similar to those of the naïve HLE cells. On the other hand, the Aβ_1–42 levels in HLE cells, treated with 0.1 μM ferulic acid, were significantly lower than that without ferulic acid.

(a) Aβ1–40 levels

(b) Aβ1–42 levels

(c) Aβ1–43 levels

(d) APP mRNA

(e) BACE1 mRNA

(f) PS1 mRNA

(g) PS2 mRNA

(h) ADAM10 mRNA

(i) NEP mRNA

(j) ECE1 mRNA

Figure 5

The effect of 0.1 μM of ferulic acid on the production of Aβ_1–40 (a), Aβ_1–42 (b), Aβ_1–43 (c) levels, and mRNA levels of APP (d), BACE1 (e), PS1 (f), PS2 (g), ADAM10 (h), NEP (i), and ECE1 (j) in HLE cells. The 0.1 μM of ferulic acid was added simultaneously to the medium, and the HLE cells were incubated for 24 h. Open columns = the naïve HLE cells. Closed columns = HLE cells in the presence of 0.1 μM ferulic acid. N.D. = not detectable. The data are presented as the means ± SE of five experiments. , versus naïve HLE cells (open columns) for each category.

4. Discussion

In the cataractous lens, an accumulation of Aβ peptide was observed, and lens opacification occurred via oxidative stress [14, 15]. Therefore, the prevention of Aβ accumulation in the lens is important for cataract therapy. In this study, we investigated whether treatments with ferulic acid prevented the Aβ production and accumulation in the human lens and showed that ferulic acid attenuated the increase in the mRNA levels of proteins related to Aβ production (APP, BACE1, and PS1) and prevented the accumulation of Aβ_1–40, Aβ_1–42, and Aβ_1–43 in H₂O₂-stimulated HLE cells.

Previous reports showed that the Aβ levels in the retina and brain were enhanced by oxidative stress [19–24]. In addition, we also reported that H₂O₂ in the rat lens induced lipid peroxidation and led to the accumulation of Aβ_1–42 in the lens epithelium [14]. Therefore, in our current study, the HLE cells were exposed to H₂O₂ to enhance the Aβ production. The results clearly suggested that 10 μM of H₂O₂ induced Aβ production, whereas 0.01–0.1 μM of ferulic acid significantly decreased the mRNAs (APP, BACE1, and PS1) related to Aβ production (Figure 4) and the Aβ production in H₂O₂-stimulated HLE cells (Figure 3). It was previously reported that oxidative stress increased the accumulation of Aβ in the lens, retina, and brain [14, 19–24]. In addition, ferulic acid has been shown to possess some scavenging activity for hydroxyl radicals and peroxynitrite [27, 28] and to inhibit the oxidation of substrates. Taken together, our results suggested that 0.1 μM and 1 μM of ferulic acid may prevent H₂O₂ effects, resulting in a decrease of specific mRNAs and in Aβ accumulation. However, the mRNA levels of proteins related to Aβ production (APP, BACE1, and PS) in HLE cells incubated with 30 μM of ferulic acid were similar to that of the H₂O₂-stimulated HLE cells incubated with 0.1 μM of ferulic acid (Figure 4). However, the Aβ_1–40, Aβ_1–42, and Aβ_1–43 levels in the HLE cells stimulated with 30 μM of ferulic acid were elevated when compared with those of the H₂O₂-stimulated HLE cells incubated with 0.1 μM of ferulic acid (Figure 3). It was reported that ferulic acid undergoes specific interactions with Aβ mature fibrils, possibly promoting their destabilization [35]. Moreover, ferulic acid inhibited Aβ aggregation and destabilized preformed Aβ fibrils [36]. From these findings, the destabilization of Aβ fibrils by ferulic acid may be related to the difference in the levels of Aβ in the HLE cells treated with 0.1 μM and 30 μM of ferulic acid. In this study, the Aβ monomer in/on the cells would be measured, since the HLE cells were collected, and all protein fractions were precipitated with 70% formic acid. We tried to measure the Aβ levels in medium; however the Aβ levels were not detected by using ELISA method. We hypothesize that both the fibrils and monomeric Aβ are present in the medium but were below the detection level of the ELISA assay. For the certification of this hypothesis, there is a need to measure the levels of Aβ in the medium by using high resolution mass spectrometry in future studies.

On the other hand, 0.1 μM of ferulic acid shows different effects between Aβ_1–40 and Aβ_1–42 levels (Figure 5). It was known that the Aβ_1–42 was easy to aggregate in comparison with Aβ_1–40; however, the amount of Aβ_1–42 production was lower than that of Aβ_1–40 [7]. Therefore, the destabilization of Aβ aggregation by ferulic acid may strongly affect the Aβ_1–42 in comparison with Aβ_1–40. Further studies are needed to elucidate the precise mechanisms for the prevention of Aβ production and the accumulation by ferulic acid in the lens. In addition, it is important to measure the ratio of Aβ fibrils and Aβ monomers to clarify the molecular mechanism involved in the downregulation of APP, BACE1, and PS1 mRNAs in ferulic acid treated cells. Therefore, we are now investigating the protein expression and aggregation of Aβ in H₂O₂-stimulated HLE cells incubated with 0.1 μM and 30 μM of ferulic acid by using western blotting and immunostaining methods. Moreover, we are developing a drug delivery system for ferulic acid to the lens. In the future, we will determine the in vivo effects of a ferulic acid ophthalmic formulation on lens opacification and Aβ accumulation in the UPL rat model.

5. Conclusions

We have shown that stimulation with H₂O₂ leads to increased mRNA levels of proteins related to Aβ production (APP, BACE1, and PS) and to an enhanced accumulation of Aβ_1–40, Aβ_1–42, and Aβ_1–43 in HLE cells. In addition, we showed that treatments with ferulic acid attenuated the increases in the mRNA levels of proteins related to Aβ production and prevented Aβ_1–40, Aβ_1–42, and Aβ_1–43 accumulation in H₂O₂-stimulated HLE cells. An ophthalmic eye drop formulation containing ferulic acid could prevent both oxidative stress and Aβ accumulation in HLE cells, resulting in the suppression of lens opacification during cataract. This study provides significant information that can therefore be used to design further studies aimed at developing anticataract drugs.

Conflicts of Interest

The authors declare no conflicts of interest. The authors alone are responsible for the content and writing of the paper.

Acknowledgments

This work was supported in part by Grant 25288075, from the Ministry of Education, Culture, Sports, Science, and Technology of Japan.

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Copyright

Copyright © 2017 Noriaki Nagai et al. This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

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BioMed Research International

Ferulic Acid Suppresses Amyloid β Production in the Human Lens Epithelial Cell Stimulated with Hydrogen Peroxide

Abstract

1. Introduction

2. Materials and Methods

2.1. Cell Culture and Treatment

2.2. Quantitative Real-Time RT-PCR

2.3. Measurement of Aβ

2.4. Measurement of Cell Viability

2.5. Statistical Analyses

3. Results

3.1. The Effect of H2O2 Stimulation on Aβ Production and Accumulation in HLE Cells

3.2. The Preventive Effects of Ferulic Acid on Enhanced Aβ Production and Accumulation in H2O2-Stimulated HLE Cells

3.3. The Effects of Ferulic Acid on Aβ Production and Accumulation in HLE Cells

4. Discussion

5. Conclusions

Conflicts of Interest

Acknowledgments

References

Copyright

3.1. The Effect of H₂O₂ Stimulation on Aβ Production and Accumulation in HLE Cells

3.2. The Preventive Effects of Ferulic Acid on Enhanced Aβ Production and Accumulation in H₂O₂-Stimulated HLE Cells