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Neuroprotection of soyabean isoflavone co-administration with folic acid against β-amyloid 1-40-induced neurotoxicity in rats

Published online by Cambridge University Press:  19 February 2009

Wei-wei Ma
Affiliation:
School of Public Health and Family Medicine, Capital Medical University, No. 10 Xitoutiao, You An Men, Beijing100069, China
Li Xiang
Affiliation:
School of Public Health and Family Medicine, Capital Medical University, No. 10 Xitoutiao, You An Men, Beijing100069, China
Huan-Ling Yu
Affiliation:
School of Public Health and Family Medicine, Capital Medical University, No. 10 Xitoutiao, You An Men, Beijing100069, China
Lin-Hong Yuan
Affiliation:
School of Public Health and Family Medicine, Capital Medical University, No. 10 Xitoutiao, You An Men, Beijing100069, China
Ai-Min Guo
Affiliation:
School of Public Health and Family Medicine, Capital Medical University, No. 10 Xitoutiao, You An Men, Beijing100069, China
Yi-Xiu Xiao
Affiliation:
School of Public Health and Family Medicine, Capital Medical University, No. 10 Xitoutiao, You An Men, Beijing100069, China
Li Li
Affiliation:
School of Public Health and Family Medicine, Capital Medical University, No. 10 Xitoutiao, You An Men, Beijing100069, China
Rong Xiao*
Affiliation:
School of Public Health and Family Medicine, Capital Medical University, No. 10 Xitoutiao, You An Men, Beijing100069, China
*
*Corresponding author: Dr R Xiao, fax +86 10 83911512, email xiaor22@ccmu.edu.cn
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Abstract

Soya isoflavones (SIF) and folic acid (FA) both confer the biological properties of antioxidation; however, the mechanism of their antioxidant effect on nervous system development is unclear. Our purpose is to investigate the neuroprotective effects of SIF, FA or co-administration of SIF with FA against β-amyloid 1-40 (Aβ1-40)-induced learning and memory impairment in rats. In the present study, the learning and memory ability of rats and the amount of amyloid-positive neurons in the cerebral cortex and hippocampal CA1 area were measured. The levels of total antioxidant capacity (T-AOC), glutathione (GSH) and glutathione peroxidase (GSH-Px) in serum and brain tissue were also measured. The results showed that intracerebroventricular administration of Aβ1-40 resulted in a dramatic prolongation of the escape latency; however, in the SIF, FA and SIF+FA treatment groups, the functional deficits of learning and memory were significantly improved. Moreover, after Aβ1-40 injection, the levels of T-AOC and GSH were profoundly decreased, suggesting a decline of antioxidant activity in the rats. However, intragastric pre-treatment with SIF, or FA, or SIF+FA resulted in a significant increase of antioxidative activity. SIF, or FA, or SIF+FA treatments also reversed the Aβ1-40-induced increase in the amount of amyloid-positive neurons. These results suggest that: (1) learning or memory impairment in experimental rats was caused by Aβ1-40, which is probably attributed to Aβ-induced oxidative damage and deposition of β-amyloid peptides in the brain; (2) pre-administration of SIF and/or FA may prevent the pathological alterations caused by Aβ1-40 treatment and the neuroprotective effects of SIF and/or FA are indicated.

Type
Short Communication
Copyright
Copyright © The Authors 2009

β-Amyloid-peptide (Aβ) has long been considered as the chief constituent of senile plaques observed in the brain of patients with Alzheimer's disease(Reference Li, Chen and Lee1). It has been reported that Aβ25-35 injection can cause mild learning and memory deficits in animals(Reference Klementiev, Novikova and Novitskaya2). This assertion has also been supported by other experiments in vivo (Reference Huang, Liang and Chen3).

The intake of soyabean isoflavones (SIF) has been proved to be associated with decreased risk of some kinds of diseases. However, there is a paucity of basic research exploring the mechanism of their actions in the mammal central nervous system. Although there is solid evidence from models of familial amyotrophic lateral sclerosis and ischaemia, supporting the idea that SIF may produce some extent of neuroprotection(Reference Trieu and Uckun4, Reference Liang, Qiu and Shen5), there remains less understanding whether they have similar neuroprotective effects against Aβ-induced neurotoxicity. Additionally, it has been well established that folic acid (FA) deficiency may lead to many neurological and psychological disorders including impaired memory function(Reference Eussen, de Groot and Joosten6) and Alzheimer's disease(Reference Luchsinger, Noble and Scarmeas7), whereas FA supplementation can improve cognitive function(Reference Das8). The exact principles of neuroprotective actions exhibited by FA are intangible.

Recently, a growing number of reports have indicated the involvement of oxidative stress in the occurrence of Aβ-induced neurotoxicity(Reference Cetin and Dincer9, Reference Crouch, Harding and White10). Given the previously reported notion that dietary sources of sufficient antioxidants are critical for preventing oxidative damage(Reference Fritz, Seppanen and Kurzer11), it seems that the antioxidant ability of FA and SIF is, at least partially, responsible for its neuroprotective roles. Nevertheless, whether SIF or FA can diminish oxidative damage during the development of learning and memory impairment and the neuroprotection of SIF co-administered with FA in vivo were not mentioned.

In the present study, we first investigated the negative influences exerted by intracerebroventricular administration of Aβ1-40 upon the learning ability and memory function of adult rats using the water maze test. Thereafter, neuroprotective effects of intragastric administration of SIF, FA or co-administration of SIF with FA were systemically evaluated using immunohistochemistry. In addition, the antioxidant activity changes in the serum and brain tissues of rats were further investigated to elucidate the possible neuroprotective mechanisms of SIF, FA or co-administration of SIF and FA in rats.

Materials and methods

Animals

The experiments were performed on seventy-five adult male Wistar rats (250 ± 30 g at the beginning of the experiment). The animals were provided by the Laboratory Animal Centre of Capital Medical University and handled in accordance with the guidelines established by the Chinese Committee on Experimental Animal Supervision.

All the rats were randomly divided into five groups: (1) control group (intracerebroventricular administration of physiological saline); (2) Aβ1-40 group (intracerebroventricular administration of Aβ1-40 (10 μg) alone); (3) SIF group (intragastric pre-administration of SIF (160 mg/kg body weight per d) for 2 weeks before Aβ1-40 treatment); (4) FA group (intragastric pre-administration of FA (0·7 mg/kg body weight per d) for 2 weeks before Aβ1-40 treatment); (5) SIF and FA group (co-administration of SIF (160 mg/kg body weight per d) and FA (0·7 mg/kg body weight per d) for 2 weeks before Aβ1-40 treatment).

Surgery

All experimental rats were first anaesthetised by intraperitoneal injection of sodium pentobarbital (50 mg/kg body weight). Then physiological saline (10 μl) or Aβ1-40 (10 μg/10 μl) was injected, respectively, into the targeted cerebral ventricle (anteroposterior − 1·2 mm from Bregma, mediolateral 2·0 mm, dorsoventral − 4·0 mm) according to the rats' solid localisation spectrum of a graph.

Morris water maze-learning and memory ability

On the eighth day after the injection of Aβ1-40, the learning and memory ability of the rats was tested by an assessment of the rats' behaviour in a Morris water maze. These animals were released from four randomly assigned start positions respectively. Each rat was given training each day for four consecutive days to find the hidden platform and the full acquisition time course was recorded. The data on day 5 were recorded. The final readout included the escape latency, the distance to arrive at the hidden platform, and the frequency of the rat spanning the quadrant where the platform laid.

Immunohistochemistry

The SABC (streptavidin-biotin complex) immunocytochemical method was used to measure the amount of amyloid-positive cells in the cerebral cortex and hippocampal CA1 area. Leica Qwin Standard V2.8 image analysis software (Leica, Cambridge, UK) was applied to calculate the amount of Aβ1-40-positive expressed neurons.

Measurements of antioxidative status

Brain tissue homogenates prepared from each group of rats were centrifuged at 4000 g for 15 min and the supernatant fraction of the homogenates was then used for the neurochemical assay. The serum was also collected from all experimental rats for the neurochemical assay. The levels and/or activities of total antioxidant capacity (T-AOC), glutathione (GSH) and GSH peroxidase (GSH-Px) in the serum and brain tissue were analysed using the measurement kit. T-AOC activity, GSH and GSH-Px levels in the serum and brain tissue were as determined according to the guidelines of the kit.

Statistical analysis

Data were expressed as mean values and standard deviations. Statistical comparisons were performed by one-way ANOVA. The acceptable level of significance was set at P < 0·05.

Results

Aβ1-40-treated rats exhibited significantly prolonged escape latency compared with that in the control group. However, the escape latency of rats in the FA, SIF, or SIF co-administered with FA groups was much shorter than that of the Aβ1-40-treated group with statistical significance. No significant differences were found in the distance and frequency of rats spanning the platform between the five groups. Furthermore, Aβ1-40-treated rats showed a substantial increase in the number of Aβ-positive cells in both the cerebral cortex and CA1 area of hippocampus formation. However, in the SIF-, FA- and SIF+FA-treated rats, a significant decrease was observed in the number of Aβ-positive cells in each tested region in comparison with that in the Aβ1-40-injected group. In the Aβ1-40-treated group, the level of T-AOC and the activity of GSH in the serum decreased dramatically compared with that in the control group. Pre-treatment of these animals with intragastric administration of SIF, FA or SIF co-administered with FA for 14 d before Aβ1-40 injection led to an apparent increase in T-AOC level and GSH activity in the serum. However, GSH-Px activity showed no significant difference. Aβ1-40 injection profoundly reduced T-AOC level and GSH activity in the brain tissues. Pre-treatment with FA, SIF or FA co-administered with SIF for 14 d before Aβ1-40 injection clearly increased T-AOC activity and GSH level. However, GSH-Px activity showed no significant difference (Table 1).

Table 1 Effects of soya isoflavone (SIF) co-administration with folic acid (FA) on the learning and memory impairments of rats damaged by β-amyloid peptide (Aβ)

(Mean values and standard deviations for fifteen rats)

T-AOC, total antioxidant capacity; GSH, glutathione; GSH-Px, GSH peroxidase.

Mean value was significantly different from that of the Aβ1-40 group: *P < 0·05, **P < 0·01.

Mean value was significantly different from that of the control group: †P < 0·05, ††P < 0·01.

Control group, intracerebroventricular administration of physiological saline treatment; Aβ1-40 group, intracerebroventricular administration of Aβ1-40 (10 μg) alone; SIF group, intragastric pre-administration of SIF (160 mg/kg body weight per d) for 2 weeks before Aβ1-40 treatment; FA group, intragastric pre-administration of FA (0·7 mg/kg body weight per d) for 2 weeks before Aβ1-40 treatment; SIF+FA group, co-administration of SIF (160 mg/kg body weight per d) and FA (0·7 mg/kg body weight per d) for 2 weeks before Aβ1-40 treatment.

Discussion

The present study suggests that intragastric administration of SIF and/or FA can prevent the neurotoxicity induced by Aβ1-40, and this neuroprotection may be achieved by increasing the antioxidant effect and decreasing the numbers of Aβ-positive neurons, and eventually improving the learning and memory ability of rats.

The Morris water maze is a classical method to evaluate learning and memory accurately with different treatments(Reference Snihur, Hampson and Cain12). The results of the Morris water maze showed that Aβ1-40-treated rats exhibited significantly prolonged escape latency compared with that of the control group. SIF and/or FA could alleviate the change induced by Aβ1-40, especially in the group injected with SIF alone. However, no significant differences in the total distance and the frequency of animals spanning the platform were found between the five groups. These results indicate that SIF and/or FA could alleviate Aβ1-40-induced impairment of spatial learning.

The cerebral cortex and hippocampus are important regions that process learning and memory. In the present study, Aβ-positive neurons in the cerebral cortex and hippocampus CA1 in rats were numbered to investigate the toxicity of Aβ1-40 and the neuroprotection of SIF and/or FA. The amount of Aβ-positive neurons reflects the toxicity of Aβ1-40. The present results showed that SIF and/or FA can reduce the number of Aβ-positive neurons both in the cerebral cortex and hippocampus CA1, which indicates that SIF and/or FA could alleviate the toxicity of Aβ1-40.

The strong relationship between oxidative stress and Aβ prompted us to investigate the oxidative damage of neurons induced by Aβ1-40. We found that Aβ1-40 could lower T-AOC and GSH levels, indicating the oxidative damage induced by Aβ1-40 due to changes in redox homeostasis and reduction of antioxidant ability both in serum and brain tissue.

SIF and FA are both diet-derived antioxidants, which are critical in protection against oxidative damage(Reference Patel, Boersma and Crawford13). SIF have been described to decrease antioxidant enzyme activities in tissues and erythrocytes of experimental rats(Reference Breinholt, Lauridsen and Dragsted14). FA has also been proved to establish strong antioxidant activity(Reference Dhitavat, Ortiz and Rogers15).

The antioxidant enzyme system of cells plays an important role in oxidative stress. Antioxidant enzymes such as GSH, GSH-Px and superoxide dismutase are all antioxidant molecules that act as redox homeostasis keepers in vivo (Reference Yan, Yang and Li16). Therefore, the agent that exhibits a regulatory effect on these antioxidant molecules is suggested to be the promising prevention or treatment strategy for oxidative impairment. In the present study, we further investigated the neuroprotection of SIF and/or FA on Aβ1-40-damaged neurons, so the level of oxidative damage-related molecules was measured experimentally in rat serum and brain tissues. The present results demonstrated that SIF show neuroprotection by up-regulating the antioxidant level both in serum and brain tissues. Compared with the Aβ1-40 treatment group, the T-AOC activity and GSH level in the FA, SIF, and FA co-administered with SIF groups were all increased, which indicates that SIF and/or FA can alleviate oxidative damage by maintaining redox homeostasis and increasing antioxidant activity both in serum and brain tissues.

However, the protective effects of SIF and FA in combination in the Morris water maze test, the number of Aβ-positive cells and the antioxidative parameters were not significantly different from isolated effects. The reason may be related to the isolated protective effects of SIF and FA that were so strong that the combination effect was not prominent, while the protective effect was enhanced when the isolated effects were not sufficient.

In addition, previous studies have indicated that SIF exhibit antioxidant activity and modulate the enzymic antioxidant defence system by increasing resting erythrocyte superoxide dismutase activity and restoring the altered redox homeostasis(Reference Jiang, Wu and Jiang17). FA supplementation can improve the total plasma antioxidant capacity in haemodialysis patients(Reference Alvares Delfino, de Andrade Vianna and Mocelin18).

All together, these results were consistent with our findings that SIF, FA, or SIF co-administered with FA performed strong antioxidant activity in vivo, which may be the possible mechanism of the neuroprotective effect of these food-derived antioxidants.

Conclusions

Learning or memory impairment in experimental rats was caused by Aβ1-40, which can probably be attributed to Aβ-induced oxidative damage and deposition of Aβ in the brain. Pre-intragastric administration of SIF and/or FA can inhibit the neurotoxicity induced by Aβ1-40 via increasing the antioxidant effect in both serum and brain tissues and decreasing the number of Aβ-positive neurons, finally improving the learning and memory ability of rats.

Acknowledgements

The present study was supported by grants from the Beijing Municipal Commission of Education Science and Technology Developmental Plan Foundation (no. KM200610025010 and no. KZ200710025011) and the National Natural Science Foundation of China (no. 30771802 and no. 30571560). W.-W. M. contributed to the drafting of the paper and the data analysis; H.-L. Y., L.-H. Y., A.-M. G. and Y.-X. X. performed the data analysis; L. X. and L. L. contributed to the measurement of immunohistochemistry, neuroethology and antioxidative status; R. X. designed the study and was the final principal of the study.

The authors have no conflicts of interest to declare.

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Figure 0

Table 1 Effects of soya isoflavone (SIF) co-administration with folic acid (FA) on the learning and memory impairments of rats damaged by β-amyloid peptide (Aβ)(Mean values and standard deviations for fifteen rats)