Anti-Amyloidogenic Effects of Metasequoia glyptostroboides Fruits and Its Active Constituents

Alzheimer’s disease (AD) is a serious neurodegenerative brain disease that interferes with daily life. The accumulation of beta-amyloid (Aβ), along with oxidative stress-inducing neurocellular apoptosis, has been considered one of the causes of AD. Thus, the purpose of this study is to find natural products that can reduce Aβ accumulation. The ethanol extract of Metasequoia glyptostroboides Hu & Cheng fruits (Cupressaceae) significantly reduced the aggregation of Aβ into oligomers and fibrils determined by Thioflavin T (ThT) assay. The solvent-partitioned ethyl acetate layer was further separated based on the bioassay-guided isolation method combined with the ThT assay. As a result, five compounds were isolated and elucidated as taxoquinone (1), sugiol (2), suginal (3), sandaracopimarinol (4), and sandaracopimaradien-19-ol (5) by comparing NMR data with references. All the compounds significantly reduced the aggregation of Aβ and enhanced the disaggregation of pre-formed Aβ aggregates in a dose-dependent manner. Furthermore, the inhibition of Aβ aggregation by the compounds protected PC12 cells from Aβ aggregate-induced toxicity. Among the five compounds, sandaracopimarinol (4) and sandaracopimaradien-19-ol (5) were the most effective. These results suggest that M. glyptostroboides and isolated five compounds have a potential for further study to be developed as anti-AD agents.


Introduction
As the proportion of the elderly population increases, dementia, which exhibits various cognitive impairments, becomes an important social and economic problem. It is predicted that 1 out of 85 people will develop dementia by the year 2050 [1]. Alzheimer's disease (AD), which accounts for 60-70% of dementia in the elderly, is one type of neurodegenerative disease, and the representative symptom of AD is cognitive decline. Although the pathologic mechanisms of AD are not clearly elucidated, the pathologic hallmarks of AD are considered as the accumulation of beta-amyloid (Aβ) proteins in the form of senile plaques, the entanglement of hyperphosphorylated tau proteins in the form of neurofibrillary tangles, and loss of specific neurons [2][3][4]. Among them, the accumulation of Aβ protein into senile plaques is reported to impair cognitive function by disrupting the endoplasmic reticulum, insulin signaling, and mitochondrial functions, which are key signaling systems in cells [5][6][7].
Aβ is a protein produced by the proteolytic cleavage of amyloid precursor protein (APP) by the proteases called βand γ-secretases. The cleavage of APP by β-secretase produces the large N-terminal ectodomain of APP (sAPPβ) and the membrane-bound Cterminal fragment, C99. The subsequent cleavage of C99 by γ-secretase eventually produces

Inhibitory Effect of M. glyptostroboides Ethanol Extract and Solvent-Partitioned Fractions on Aβ Aggregation
In order to determine the inhibitory effects of M. glyptostroboides extract on Aβ aggregation, the level of Aβ aggregation was measured by ThT assay. As shown in Figure 1A, ethanol extract of M. glyptostroboides significantly reduced the aggregation of Aβ in a dosedependent manner. Particularly, 50 µg/mL of the extract inhibited the aggregation of Aβ close to the control level. Then, the ethanol extract was partitioned based on solvent polarity, and four fractions including n-hexane, dichloromethane, ethyl acetate, and water fractions were obtained. These four fractions (50 µg/mL) were also tested to measure the inhibitory effect on the aggregation of Aβ. As a result, n-hexane, dichloromethane, ethyl acetate, and water fractions at 50 µg/mL significantly reduced the aggregation of Aβ down to 45.9, 28.4, 8.8, and 55.7%, respectively, compared to the Aβ only control group. Among the four fractions, the ethyl acetate fraction was the most active and was used for further experiments.

Isolation and Structure Elucidation of Compounds from M. glyptostroboides
To isolate the active compounds that inhibit the aggregation of Aβ, the ethyl acetate fraction was fractionated into various open CCs and a Medium-Pressure Liquid Chromatography (MPLC) using silica gel as a stationary phase based on the bioassay-guided isolation method. As a result, five compounds were isolated from M. glyptostroboides. The structures of five compounds (compounds 1-5) were elucidated based on the 1 H and 13 C-NMR data, and comparison with relevant references [16][17][18][19][20]. The isolated compounds were identified as taxoquinone (1), sugiol (2), suginal (3), sandaracopimarinol (4), and sandaracopimaradien-19-ol (5) (Figure 2).

Antioxidant Effect of Compounds Isolated from M. glyptostroboides
2,2-Diphenyl-1-picryl-hydrazyl (DPPH) free radical scavenging activity of compounds 1-5 was measured at various concentrations (25,50 and 150 µg/mL) to evaluate the Molecules 2023, 28, 1017 3 of 11 antioxidant activity. As shown in Figure 3, all compounds showed the antioxidant activity, but their activities were not statistically different. dependent manner. Particularly, 50 μg/mL of the extract inhibited the aggregation of Aβ close to the control level. Then, the ethanol extract was partitioned based on solvent polarity, and four fractions including n-hexane, dichloromethane, ethyl acetate, and water fractions were obtained. These four fractions (50 μg/mL) were also tested to measure the inhibitory effect on the aggregation of Aβ. As a result, n-hexane, dichloromethane, ethyl acetate, and water fractions at 50 μg/mL significantly reduced the aggregation of Aβ down to 45.9, 28.4, 8.8, and 55.7%, respectively, compared to the Aβ only control group. Among the four fractions, the ethyl acetate fraction was the most active and was used for further experiments.

Antioxidant Effect of Compounds Isolated from M. glyptostroboides
2,2-Diphenyl-1-picryl-hydrazyl (DPPH) free radical scavenging activity of com pounds 1-5 was measured at various concentrations (25, 50 and 150 μg/mL) to evalua the antioxidant activity. As shown in Figure 3, all compounds showed the antioxida activity, but their activities were not statistically different.

Inhibitory Effect of Compounds 1-5 on Aβ Aggregation
To determine the inhibitory effects of compounds 1-5 isolated from M. glyptostroboides on the aggregation of Aβ, ThT assay was performed. As shown in Figure 4, all of the compounds significantly inhibited the aggregation of Aβ. In particular, compounds 4 and 5 at 100 µg/mL reduced Aβ aggregation down to 26.9 and 25.4% compared to Aβ only group, which was close to the control group without Aβ. In addition, Aβ aggregations were reduced to 37.4 and 43.9% by the treatment with compounds 4 and 5 at 4 µg/mL. The inhibitory activities of compounds 4 and 5 at 4 µg/mL on Aβ aggregation were higher than compounds 1, 2, and 3 at 100 µg/mL which were 47.9, 66.8, and 54.8%, respectively.

Inhibitory Effect of Compounds 1-5 on Aβ aggregation
To determine the inhibitory effects of compounds 1-5 isolated from M. glyptostroboi des on the aggregation of Aβ, ThT assay was performed. As shown in Figure 4, all of th compounds significantly inhibited the aggregation of Aβ. In particular, compounds 4 and 5 at 100 μg/mL reduced Aβ aggregation down to 26.9 and 25.4% compared to Aβ onl group, which was close to the control group without Aβ. In addition, Aβ aggregation were reduced to 37.4 and 43.9% by the treatment with compounds 4 and 5 at 4 μg/mL The inhibitory activities of compounds 4 and 5 at 4 μg/mL on Aβ aggregation were highe than compounds 1, 2, and 3 at 100 μg/mL which were 47.9, 66.8, and 54.8%, respectively In case of control group, DMSO was adde instead of test samples. After 24 h, the aggregation of Aβ was determined by ThT assay. All dat represents the mean ± SD of three different experiments. * p < 0.05, significantly different from A only group.

Enhancement of Aβ Disaggregation by Compounds 1-5
To test the effects of the isolated compounds on the disaggregation of pre-aggregated Aβ, pre-aggregated Aβ in advance was incubated for 1 day with compounds 1-5, and then the level of Aβ aggregation was detected by ThT assay. All of the compounds exhibited positive effect on Aβ disaggregation in a dose-dependent manner. In particular, com

Inhibitory Effect of Compounds 1-5 on Aβ aggregation
To determine the inhibitory effects of compounds 1-5 isolated from M. glyptostroboides on the aggregation of Aβ, ThT assay was performed. As shown in Figure 4, all of the compounds significantly inhibited the aggregation of Aβ. In particular, compounds 4 and 5 at 100 μg/mL reduced Aβ aggregation down to 26.9 and 25.4% compared to Aβ only group, which was close to the control group without Aβ. In addition, Aβ aggregations were reduced to 37.4 and 43.9% by the treatment with compounds 4 and 5 at 4 μg/mL. The inhibitory activities of compounds 4 and 5 at 4 μg/mL on Aβ aggregation were higher than compounds 1, 2, and 3 at 100 μg/mL which were 47.9, 66.8, and 54.8%, respectively. In case of control group, DMSO was added instead of test samples. After 24 h, the aggregation of Aβ was determined by ThT assay. All data represents the mean ± SD of three different experiments. * p < 0.05, significantly different from Aβ only group.

Enhancement of Aβ Disaggregation by Compounds 1-5
To test the effects of the isolated compounds on the disaggregation of pre-aggregated Aβ, pre-aggregated Aβ in advance was incubated for 1 day with compounds 1-5, and then the level of Aβ aggregation was detected by ThT assay. All of the compounds exhibited a positive effect on Aβ disaggregation in a dose-dependent manner. In particular, com- In case of control group, DMSO was added instead of test samples. After 24 h, the aggregation of Aβ was determined by ThT assay. All data represents the mean ± SD of three different experiments. * p < 0.05, significantly different from Aβ only group.

Enhancement of Aβ Disaggregation by Compounds 1-5
To test the effects of the isolated compounds on the disaggregation of pre-aggregated Aβ, pre-aggregated Aβ in advance was incubated for 1 day with compounds 1-5, and then the level of Aβ aggregation was detected by ThT assay. All of the compounds exhibited a positive effect on Aβ disaggregation in a dose-dependent manner. In particular, compounds 4 and 5 efficiently disaggregated the pre-aggregated Aβ and the level of aggregated Aβ was down to 50.0 and 53.2%, respectively, at 100 µg/mL compared to Aβ only group ( Figure 5).

Inhibition of Aβ Aggregation by Compounds 1-5 Rescued the PC12 Cells from Aβ Aggregate-Induced Toxicity
The possible cytotoxicity of compounds 1-5 on PC12 cells was determined by MTT assay. Compounds 1-5 were not cytotoxic to PC12 cells up to 100 µg/mL except compound 3 ( Figure 6A). Compound 3 reduced the viability of PC12 cells only at 100 µg/mL. Thus, compound 3 at 100 µg/mL was excluded from the further study.
Molecules 2023, 28, x FOR PEER REVIEW 5 o pounds 4 and 5 efficiently disaggregated the pre-aggregated Aβ and the level of ag gated Aβ was down to 50.0 and 53.2%, respectively, at 100 μg/mL compared to Aβ o group ( Figure 5).

Inhibition of Aβ Aggregation by Compounds 1-5 Rescued the PC12 Cells from Aβ Aggre gate-Induced Toxicity
The possible cytotoxicity of compounds 1-5 on PC12 cells was determined by M assay. Compounds 1-5 were not cytotoxic to PC12 cells up to 100 μg/mL except compo 3 ( Figure 6A). Compound 3 reduced the viability of PC12 cells only at 100 μg/mL. Th compound 3 at 100 μg/mL was excluded from the further study.
Then, an MTT assay was performed to observe whether the inhibition of Aβ ag gation by compounds 1-5 could rescue PC12 cells from Aβ aggregate-induced toxicity shown in Figure 6B, compounds 4 and 5, which exhibited efficient inhibitory effects Aβ aggregation in Figure 5, significantly increased the viability of cells from Aβ ag gate-induced toxicity at all concentrations. In addition, compound 1 at 100 μg/mL protected the cells from Aβ aggregate-induced toxicity.

Discussion
Aβ, which is produced by proteolytic fragmentation of APP by β-and γ-secretases is considered one of the major causes of AD. In particular, over-produced Aβ aggregates into oligomers and fibrils, and Aβ aggregates are known to cause neurotoxicity and neu- Then, an MTT assay was performed to observe whether the inhibition of Aβ aggregation by compounds 1-5 could rescue PC12 cells from Aβ aggregate-induced toxicity. As shown in Figure 6B, compounds 4 and 5, which exhibited efficient inhibitory effects on Aβ aggregation in Figure 5, significantly increased the viability of cells from Aβ aggregateinduced toxicity at all concentrations. In addition, compound 1 at 100 µg/mL also protected the cells from Aβ aggregate-induced toxicity.

Discussion
Aβ, which is produced by proteolytic fragmentation of APP by βand γ-secretases is considered one of the major causes of AD. In particular, over-produced Aβ aggregates into oligomers and fibrils, and Aβ aggregates are known to cause neurotoxicity and neuronal loss because of the increased mitochondrial dysfunction and ER stress [4,5,8]. In this study, the extract of M. glyptostroboides fruits significantly decreased the production of neurotoxic Aβ aggregates. In addition, five diterpenoids were isolated as active constituents. Among them, sandaracopimarinol (4) and andaracopimaradien-19-ol (5) efficiently decreased the aggregation of Aβ and enhanced the disaggregation of Aβ aggregates. Furthermore, sandaracopimarinol (4) and andaracopimaradien-19-ol (5) rescued the PC12 cells from Aβ aggregate-induced toxicity by inhibiting Aβ aggregation.
The ethanol extract of M. glyptostroboides fruits was selected for further study because it efficiently inhibited Aβ aggregation determined by ThT assay. Then, the bioassay-guided isolation of ethanol extract of M. glyptostroboides fruits allowed to isolate five pure compounds. The structures of these compounds were elucidated based on 1 H-and 13 C-NMR data by comparison with references [16][17][18][19][20]. As a result, compounds 1-3 were identified as taxoquinone, sugiol, and suginal, respectively, which are abietane-type diterpenoids. The aromatic abietane structure is the most abundant naturally occurring abietane-type diterpenoid. Aromatic abietane-type diterpenoids, such as ferruginol, sclareol, isorosmanol, and carnorol have been reported to possess various biological properties, including anti-bacterial, anti-cancer, anti-fungal, anti-tumor, anti-viral, and anti-inflammatory activities [24][25][26][27]. However, the inhibitory effect of aromatic abietane-type diterpenoids on Aβ aggregation has not been reported, yet.
Taxoquinone (1) is known to be a natural anti-bacterial agent against a wide range of bacteria with little or no toxicity for centuries [28]. In addition, taxoquinone (1) has potent anti-diabetic and anti-melanin potential due to the inhibition of α-glucosidase and tyrosinase inhibition [16,28]. Sugiol (2) is also reported to efficiently inhibit α-glucosidase and tyrosinase and have potential anti-diabetic and anti-menalin effects [29]. Suginal (3) has been reported to have anti-bacterial activity [30]. It has a structure very similar to that of sugiol and has an additional carbonyl group.
Even though diterpenoids with a pimarane structure such as pimaradienoic acid and continentalic acid have been reported to have anti-Alzheimer's activities by inhibiting Aβ aggregation [33], the inhibitory effects of sandaracopimarinol (4) and sandaracopimaradien-19-ol (5) against Aβ aggregation were first reported in this study.
Taken together, these results suggest that the extract of M. glyptostroboides fruits and five diterpenoids isolated from M. glyptostroboides including taxoquinone (1), sugiol (2), suginal (3), sandaracopimarinol (4), and sandaracopimaradien-19-ol (5) significantly reduced the aggregation of Aβ and enhanced the disaggregation of Aβ aggregates from oligomers and fibrils to monomers. Furthermore, sandaracopimarinol (4), and sandaracopimaradien-19ol (5) protected the neuronal cells from Aβ aggregate-induced toxicity by reducing Aβ aggregation. Therefore, the extract of M. glyptostroboides fruits and active constituents has the potential to prevent AD by inhibiting Aβ aggregation and protecting the neuronal cells.

Plant Material and Extraction
The fruits of M. glyptostroboides were collected from Dankook University (Cheonan, Republic of Korea) in January 2020. A voucher specimen has been deposited in the Pharmacognosy Laboratory of College of Pharmacy, Dankook University, Republic of Korea. The dried and pulverized M. glyptostroboids fruits (4 kg) were extracted three times with ethanol (30 L) under reflux for 24 h at room temperature. The ethanol filtrate was evaporated under vacuum to yield the ethanol extract (310 g). The extract was suspended in distilled water and then partitioned sequentially into n-hexane, dichloromethane, ethyl acetate, and water. Four fractions including n-hexane (115.2 g), dichloromethane (46.0 g), ethyl acetate (30.9 g), and water (115.8 g) fractions were obtained.

Isolation of Active Compounds
The ethyl acetate fraction was fractionated by open CC using silica gel as stationary phase with solvent mixture of n-hexane and acetone (100:1), and 10 subfractions (MGE1~MGE10) were obtained. The subfraction 8 (MGE8) was further fractionated by open silica CC with solvent mixture of n-hexane and acetone (100:5), and compound 1 (89.5 mg) and compound 2 (222.5 mg) were obtained as pure compounds.

ThT Assay
To quantify the aggregation of Aβ to oligomers and fibrils, ThT assay was performed. The Aβ 1-42 was dissolved in DMSO at 1 mg/mL concentration and test samples were also dissolved in DMSO. To monitor the effects of test samples on the Aβ aggregation, 20 µM of Aβ 1-42 was incubated with various concentrations of test samples at 37 • C for 24 h. For the control group, DMSO was used instead of test samples. Then, 3 µM of ThT was added, and fluorescence was measured after 30 min using an Emax precision microplate reader (Molecular Devices, CA, USA) with excitation at 442 nm and emission at 485 nm. The Aβ only was used as a control, and each assay was repeated 3 times.
To monitor the disaggregation effects of test samples on the pre-aggregated Aβ, the ThT assay was performed. Briefly, 20 µM of Aβ 1-42 was pre-incubated at 37 • C for 24 h. After that, various concentrations of test samples or DMSO were added and incubated at 37 • C for additional 24 h. Then, 3 µM of ThT was added and fluorescence was measured after 30 min using an Emax precision microplate reader (Molecular Devices) with excitation at 442 nm and emission at 485 nm. The Aβ only was used as a control and each assay was performed in triplicate.

DPPH Assay
Antioxidant activity was measured using DPPH. The sample (10 µL) was mixed with 0.2 mM DPPH reagent (190 µL). The mixture was vortexed and kept in a dark place at 37 • C for 30 min. The change in absorbance was measured with an E-max precision microplate reader (Molecular Devices) at 540 nm. Ascorbic acid was used as a positive control. The inhibition rate was converted into a percentage of the difference between the absorbance values of a negative control treated with DMSO and the test samples. All experiments were repeated three times. Percent inhibition was calculated as (%) = (A control − A test )/A control * 100.

Cell Cultures
PC12 cells (rat pheochromocytoma cells) were obtained from Korea Cell Line Bank (Seoul, Republic of Korea) and grown in RPMI 1640 with 15% heat-inactivated horse serum and 5% heat-inactivated FBS. The cells were incubated in a humidified 5% CO 2 at 37 • C.

MTT Assay
In order to determine the cytotoxicity of test samples, MTT assay was performed. PC12 cells were harvested from flasks and plated in 96-well plates with 6 × 10 4 cells per well. Plates were incubated at 37 • C for 3 h to allow the cells to attach to the plates. Test samples were diluted with DMSO and added to individual wells. DMSO was added in case of control group. The plates were then incubated for an additional 24 h at 37 • C. The cell viability was determined using an MTT toxicity assay by adding 10 µL of 5 mg/mL MTT to each well. After 3 h incubation at 37 • C, 70 µL of the medium was gently removed, and then 70 µL of DMSO was added to each well. Plates were incubated at room temperature for 30 min to dissolve the MTT formazan crystals, and then the absorbance was measured at 540 nm using an E-max precision microplate reader (Molecular Devices). An average from 3 replicate wells was used for each sample, and each assay was performed in triplicate.
To investigate whether the inhibition of Aβ aggregation by test samples could rescue the cells from Aβ aggregate-induced toxicity, test samples (4, 20, and 100 µg/mL) and Aβ 1-42 (10 µM) were mixed together in 96-well plates and incubated at 37 • C for 24 h to inhibit the formation of Aβ aggregates. For the control group, DMSO was added instead of test samples. The mixture was added to PC12 cells and incubated at 37 • C for an additional 24 h. The cell viability was determined using MTT assay. An average from 3 replicate wells was used for each sample, and each assay was performed in triplicate.

Statistical Analysis
All data in figures are expressed as mean ± SD of three different experiments. Data were analyzed using a two-tailed Student's t-test in Microsoft Excel ver. 2016. Differences with a p-value smaller than 0.05 were considered statistically significant.