Folate, one of the B vitamins, plays an important role in the normal functioning of the central nervous system(Reference Reynolds1). Folate deficiency, partially due to a poor diet, is associated with cognitive decline, dementia and increased risks of Alzheimer's disease (AD)(Reference Engelborghs, Vloeberghs and Maertens2–Reference Ramos, Allen and Mungas4). Although the causal effects of folate insufficiency on AD-associated cognition impairment are not well understood, studies have demonstrated that increased folate intake was correlated with a lower risk of AD(Reference Luchsinger, Tang and Miller5). Among cognitively impaired subjects with low folate levels, folate supplementation was associated with improving memory deficits and performance(Reference Fioravanti, Ferrario and Massaia6, Reference Bryan, Calvaresi and Hughes7). The 3-year randomised controlled Folic Acid and Carotid Intimamedia Thickness (FACIT) trial confirmed significant effects of folic acid supplementation in improving memory(Reference Durga, van Boxtel and Schouten8). This contrast with a negative trend in specific test scores of a folate-supplemented group was observed in dementia subjects(Reference Sommer, Hoff and Costa9). In a prospective study with 3718 residents, a faster rate of cognitive decline was associated with high folate intake(Reference Morris, Evans and Bienias10). The inconsistent results from epidemiological and folate intervention studies underscore a need to investigate how changes in dietary folate intake mechanistically affect the brain's integrity during the development of neurodegenerative diseases such as AD.
Oxidative damage was widely implicated in the pathogenesis of AD, occurring early in the AD brain, before the onset of plaque pathology and after the deposition of brain fibrillar β-amyloid (Aβ) peptide(Reference Duyckaerts11–Reference Velliquete, O'Connor and Vassar13). In brain tissues of AD patients, oxidative insults are frequently observed based on increased levels of lipid peroxidation, proteins and nucleic acids(Reference Behl and Moosmann14). Nucleic acids, particularly mitochondrial DNA (mtDNA), are the primary target of free radical damage due to a low level of DNA repair and the proximity of reactive oxygen species generated by respiratory chains. Human mtDNA is a double-stranded, circular, 16·5 kb molecule containing genes necessary for the synthesis of the catalytic components of oxidative phosphorylation. Elevated mtDNA oxidative damage was associated with mitochondrial (mt) respiratory dysfunction and vicious reactive oxygen species cycles, which may result in apoptotic cell death(Reference Chinnery, Samuels and Elson15, Reference Ravagnan, Roumier and Kroemer16). Accumulating evidence suggests that AD may be associated with mtDNA aberrations, elevated oxidative stress and mt respiratory dysfunction(Reference Reddy and Beal17, Reference Maruszak, Gaweda-Walerych and Soltyszewski18). Impaired energy metabolism and mt abnormalities are observed as a feature of peripheral cells and brain from patients with AD(Reference Bosetti, Brizzi and Barogi19, Reference Mancuso, Filosto and Bosetti20). In AD brain specimens, mtDNA of the frontal, parietal and temporal lobes had tenfold higher levels of oxidised bases than nuclear DNA(Reference Wang, Xiong and Xie21). Increased mtDNA defects and mt dysfunction are considered part of the spectrum of chronic oxidative stress during AD development(Reference Markesbery and Lovell22).
Several studies have recently reported that dietary folate may modulate the accumulation of large mtDNA deletions(Reference Branda, Brooks and Chen23–Reference Chou, Yu and Huang25) – a 4977 bp deletion in humans and a 4834 bp large deletion in rodents. The large mtDNA deletions are commonly found to accumulate in a variety of ageing tissues(Reference Cortopassi, Shibata and Soong26–Reference Lee, Pang and Hsu28). In particular, such large mtDNA deletions are present at high levels in the brain and heart of ageing human tissues, and are associated with elevated oxidative stress(Reference Cortopassi, Shibata and Soong26, Reference Lee, Pang and Hsu28, Reference Lee and Wei29). We previously demonstrated that dietary folate deprivation (FD) promotes the accumulation of large mtDNA deletions in whole-brain homogenates of rats(Reference Chou, Yu and Huang25). Such ageing-associated large mtDNA deletions, however, have not been characterised in various AD-susceptible brain regions in response to different dietary folate levels. We hypothesised that various dietary folate levels may modulate brain folate, thus affecting oxidative lesions and the frequencies of large mtDNA deletions in AD-susceptible brain regions before or after Aβ peptide challenge. The 11-amino acid fragment of the Aβ peptide, Aβ(25–35), located at the C-terminal end of Aβ(1–42) in the hydrophobic domain, was shown to mimic some of the pathological processes in the AD brain(Reference Sun and Alkon30). Using an animal model with an experimental design of an intracerebroventricular (icv) injection of Aβ(25–35) peptide to rats fed various levels of dietary folate, changes in brain folate, neuronal death and oxidative modification in lipids as well as mtDNA deletions of various brain tissues were measured to investigate the mechanisms by which dietary folate may affect brain oxidative damage in the absence/presence of Aβ(25–35) peptide challenge.
Materials and methods
Experimental diets and animals
The FD diet was specially formulated by Harlan Teklad (Madison, WI, USA) using an l-amino acid-defined regimen (see Table S1 of the supplementary material, available at http://www.journals.cambridge.org/bjn). The FD diet replenished with a moderate level of folate at 8 mg/kg diet was designated the moderate folate (MF) diet(Reference Walzem and Clifford31). The MF diet supplemented with folate in drinking-water (0·003 %) was designated the folate-supplemented (FS) diet. All diets contained succinylsulphathiazole (1/100 g) to suppress intestinal microfloral folate production.
Male weaning Wistar rats (n 35) were obtained from the Animal Center of the National Science Council (Taipei, Taiwan, ROC). Rats were housed in stainless-steel wire cages in an air-conditioned room maintained at 25°C and 70 % humidity with a 12 h dark–12 h light cycle. After a 3 d acclimatisation period during which rats were fed a non-purified diet, they were randomly assigned to the FD, MF and FS diets (n 14, 14 and 7 in each respective group) using a pair-fed model as previously described(Reference Chou, Yu and Huang25). Access to food and tap water was available ad libitum, and rats were weighed twice a week. The single aggregated Aβ(25–35) peptide (1 mg/ml) or vehicle solution (sterile distilled water) was icv administrated to rats fed the various folate diets 1 week before killing. Rats fed with the MF diet in the absence of Aβ injection were designated as the control group. All experimental procedures and protocols were approved by the Institutional Animal Care and Use Committee of Fu-Jen University. Institutional and national guidelines for the care and use of animals were followed.
β-Amyloid(25–35) peptide preparation and surgery
Aβ(25–35) peptides were aggregated as previously described(Reference Wilkinson, Koenigsknecht-Talboo and Grommes32). In brief, the peptide was dissolved in sterile distilled water at a concentration of 1 mg/ml, divided into aliquots in tubes and stored at − 20°C. These were ‘aged’ before the administration by incubation at 37°C for 7 d. Light microscopic observation showed the existence of both birefringent fibril-like structures and globular aggregates.
An icv injection of Aβ(25–35) peptide was given according to operating protocols with some modifications(Reference Stepanichev, Moiseeva and Lazareva33). After 3 weeks of feeding the experimental diets, rats were anaesthetised and positioned in a stereotaxic frame, and a midline sagittal incision was made in the scalp. Holes were drilled in the skull over the lateral ventricles using the following coordinates: anterior-posterior (AP), − 0·1 cm; medial-lateral (ML), − 0·15 cm; dorsal-ventral (DV), − 0·35 cm. All injections were made using a 10 μl Hamilton syringe equipped with a 30S gauge needle. Animals were injected with sterile distilled water (the vehicle group) or the aggregated Aβ(25–35) peptide at a volume of 8 μl into each cerebral lateral ventricle at a rate of 1 μl/min. The needle was left at the site of the injection for an additional 2 min. At 7 d after a single injection, the animals were decapitated. The cortical, hippocampal and medullary tissues were immediately dissected over ice frozen in liquid N2 and stored at − 180°C. The frontal cortical tissues were removed and postfixed in the same fixative solution for 48 h and then embedded in paraffin.
Brain and liver folate assay
Tissue samples for the folate analysis were prepared as previously described(Reference Varela-Moreiras and Selhub34). Using a Polytron homogeniser (OMNI 2000; OMNI, Inc., Waterburg, CT, USA), liver and brain samples were homogenised in an extraction solution containing 5 mm-2-mercaptoethanol, 0·1 m-sodium ascorbate, 50 mm-HEPES and 50 mm-2-(N-cyclohexylamino) ethanesulphonic acid/l (pH 7·85). The homogenate was centrifuged at 20 000 g for 10 min. The supernatant extract was stored at − 180°C in N2 for later analysis. After incubation of the thawed sample extracts with chicken pancreatic conjugate (4:1, v/v) at 37°C for 6 h, a microbiologic assay was performed using cryoprotected Lactobacillus casei in ninety-six-well microtitre plates(Reference Horne and Patterson35). The absorbance was detected at 600 nm in an MRX model ELISA reader (Dynatech Laboratories, Billingshurst, West Sussex, UK).
Lipid peroxidation
Lipid peroxidation was quantified by measuring thiobarbituric acid-reactive substance (TBARS) production(Reference Fraga, Leibovitz and Tappel36). The reaction reagents consisted of 3 g sodium dodecylsulphate, 0·1 m-HCl, 10 g phosphotungstic acid and 0·7 g 2-thiobarbituric acid/l. The sample mixture was incubated for 45 min at 95°C, and TBARS were extracted in 2·5 ml of 1-butanol. After centrifugation at 1000 g for 10 min, the fluorescence of the butanol layer was measured using a Hitachi F-3000 fluorospectrophotometer (Tokyo, Japan) at 555 nm emission and 515 nm excitation. The TBARS values were expressed as nanomoles of malondialdehyde equivalents per gram of protein using a standard curve of 1,1,3,3-tetraethoxypropane. The protein concentration was determined using a protein dye-binding standard curve(Reference Bradford37).
Analysis of the frequencies of accumulated large mitochondrial DNA4834 deletions
The breakpoints of mtDNA4834 deletion are at the deletion junction (8103, 12 937–12 952 bp) with two 16 bp repeats that normally flank the wild-type mtDNA. The primers for the detection of large mtDNA deletions were designed to detect PCR products when mtDNA were deleted at the particular junctions to join the flanking region(Reference Chou, Yu and Huang25). The quantity of mtDNA4834 deletion was determined by co-amplifying the mtDNA displacement loop and mtDNA4834 deletion in a real-time PCR assay. Primers for each have been previously described(Reference Chou, Yu and Huang25). The extent of mtDNA4834 deletions was quantified with a deletion probe (DYXL-5′-(12952) TCACTTTAATCGCCACATCCATAACTGCTGT (12982)-3′ BHQ1) and an mtDNA probe (6FAM (15795) 5′-TTGGTTCATCGTCCATACGTTCCCCTTA (15822)-3′ BHQ1). PCR amplification was carried out in a 20 μl reaction volume consisting of a TaqMan Universal Master Mix (4 μl), 200 nmol/l of each mtDNA4834 deletion primer, 50 nmol/l of each displacement loop primer and 100 nmol/l of each mtDNA4834 deletion and displacement loop probes. The cycling conditions included an initial phase of 2 min at 50°C and 10 min at 95°C, and then forty cycles of 15 s at 95°C and 0·5 min at 72°C. The fluorescence spectra were monitored by the LightCycler Detection System with Sequence Detection Software version 4 (LightCycler; Roche Diagnostics, Mannheim, Germany). The cycle at which a statistically significant increase in normalised fluorescence was first detected was designated the threshold cycle number (C t). The relative frequencies of mtDNA4834 deletions to mtDNA were calculated using ΔC t = mt C t del-mt C t D-loop, where D-loop represents the displacement loop. Fewer mtDNA deletions will give rise to a higher C t number to obtain a detectable fluorescence signal; thus, a smaller ΔC t value indicates more deletions. The ΔC t values were used to quantify the relative amount of large mtDNA deletions in percentage with the equation:
Neural cell death by haematoxylin and eosin histological examination
Whole-mount preparations of the frontal tip from rats were scanned using a digital slide system Aperio ScanScope CS (Aperio Technologies, Vista, CA, USA), and all images were analysed by Aperio's ImageScope Viewer software (Aperio Technologies). Morphological features of dead cells in the frontal cortical brain tissues of rats were identified by counting neurons with obviously condensed pyknotic nuclei surrounded by cytoplasmic eosinophilia using haematoxylin and eosin histochemistry as previously described(Reference Tocco, Musleh and Sakhi38). Damaged and viable neurons were quantified from several randomly selected fields, and the ratios were recorded.
Statistical analysis
Data are presented as means and standard deviations. The effects of dietary folate intake and an Aβ(25–35) injection on animal growth, folate status, lipid peroxidation, DNA oxidative injuries and neuronal death were analysed by one-way ANOVA and Duncan's multiple range test using the general linear model of SAS Institute (Cary, NC, USA). Differences were considered significant at P < 0·05. Pearson's correlation coefficients were used to measure the associations between folate levels, lipid peroxidation and mtDNA deletions in various brain tissues and the liver.
Results
Animal growth in response to dietary folate intakes and an intracerebroventricular β-amyloid peptide injection
Growth rates of rats in the experimental groups are presented in Table 1. Among the vehicle groups, the FD rats had a significantly lower weight gain and feed efficiency than did control rats (P < 0·05). An icv administration of Aβ(25–35) peptide did not affect the weight gain or feed efficiency of FD or control rats. Among the Aβ(25–35)-administered groups, the Aβ+MF and Aβ+FS groups showed higher weights and feed efficiencies than the Aβ-FD group. The FD and Aβ+FD groups exhibited abnormal increases in liver weight, whereas the Aβ+MF and Aβ+FS groups had liver weights similar to the vehicle control group.
a,b,c Mean values within a row with unlike superscript letters were significantly different (P < 0·05).
* Data were analysed by one-way ANOVA and Duncan's multiple range test.
† FD, MF and FS indicate no folate (dietary folate deprivation; 0 mg folic acid/kg diet), moderate folate (+8 mg folic acid/kg diet) and folic acid-supplemented (+8 mg folic acid/kg diet and 0·003 % folic acid in drinking-water: 68 μm) diets, respectively. The MF group receiving the vehicle microinjection was designated the control.
‡ Aβ(25–35) administration included an intracerebroventricular microinjection of 8 μl of Aβ(25–35) peptide (1 mg/ml). Vehicle administration included an intracerebroventricular microinjection of 8 μl of the vehicle solution (sterile distilled water).
Dietary FD for 4 weeks did not affect the crude brain weight in the cortical, hippocampal or medullary regions (Table 1) in either the vehicle- or Aβ-treated groups. Supplementation of folic acid in Aβ-treated rats significantly increased the crude weight of the hippocampus compared with the Aβ+FD, Aβ+MF and vehicle control groups (P < 0·05).
Dietary folate intake modulated folate levels of brain tissues and the liver in the presence/absence of an intracerebroventricular β-amyloid peptide injection
After consuming the FD diet for 4 weeks, folate levels in the hippocampal and medullary tissues of FD rats had significantly dropped by more than 50 % compared with vehicle control rats (P < 0·05; Table 2). The cortical folate levels of rats decreased to a lesser extent after 4 weeks of consuming the FD diet. After the 4-week FD diet, 80 % of hepatic folate was depleted, but without reaching statistical significance due to high measurement variations within the groups. An icv administration of Aβ(25–35) peptide did not further deplete folate levels of the liver or various brain tissues of FD rats. Feeding Aβ(25–35)-injected FD rats the FS diet caused a significant supplementation of hepatic and brain folate levels (hippocampal and medullary tissues) back to the levels of the counterpart tissues of vehicle control rats. The MF diet supplemented folate levels of Aβ(25–35)+FD rats only in the liver and medullary tissues (P < 0·05).
a,b,c Mean values within a row with unlike superscript letters were significantly different (P < 0·05).
* Data were analysed by one-way ANOVA and Duncan's multiple range test.
† Control, FD, MF and FS indicate no folate (dietary folate deprivation), moderate folate (+8 mg folic acid/kg diet; same folate levels as in the control diet) and folic acid-supplemented (+8 mg folic acid/kg diet and 0·003 % folic acid in drinking-water: 68 μm) diets, respectively. The MF group receiving the vehicle microinjection was designated the control.
‡ Aβ administration included an intracerebroventricular microinjection of 8 μl of Aβ(25–35) peptide (1 mg/ml). Vehicle administration included an intracerebroventricular microinjection of 8 μl of the vehicle solution (sterile distilled water).
Dietary folate intake modulated lipid peroxidation in the brains of rats in the presence/absence of β-amyloid peptide challenge
In the absence of an Aβ challenge, FD rats had significantly elevated TBARS levels in the hepatic and hippocampal tissues compared with vehicle control rats (Table 3). An icv Aβ injection did not further aggravate lipid peroxidation of FD rats in either tissue. In the presence of Aβ challenge, feeding the MS or FS diets did not significantly affect hepatic or hippocampal TBARS levels of FD rats. The medullary TBARS levels of rats increased after 4 weeks of consuming the FD diet, but without reaching statistical significance. An icv Aβ injection significantly elevated lipid peroxidation in the medullary tissue of FD rats (P < 0·05). Both the MF and FS diets significantly diminished the medullary TBARS levels of Aβ+FD rats to vehicle control values (P < 0·05). Neither changes in dietary folate levels nor Aβ challenge affected lipid peroxidation in the cerebral cortex.
a,b Mean values within a row with unlike superscript letters were significantly different (P < 0·05).
* Data were analysed by one-way ANOVA and Duncan's multiple range test.
† FD, MF and FS indicate no folate (dietary folate deprivation), moderate folate (+8 mg folic acid/kg diet) and folic acid-supplemented (+8 mg folic acid/kg diet) and 0·003 % folic acid in drinking-water: 68 μm) diets, respectively. The MF group receiving the vehicle microinjection was designated the control.
‡ Aβ administration included an intracerebroventricular microinjection of 8 μl of Aβ(25–35) peptide (1 mg/ml). Vehicle administration included an intracerebroventricular microinjection of 8 μl of the vehicle solution (sterile distilled water).
Dietary folate intake modulated mitochondrial DNA4834 deletions in the brains of rats in the presence/absence of β-amyloid peptide challenge
In the absence of an Aβ challenge, FD rats had increased frequencies of mtDNA4834 deletions in the hippocampal region compared with the counterpart tissue of control rats (Table 4). A similar elevation with a less extent of accumulated mtDNA deletions was observed in the medulla of FD rats (P < 0·05). An icv administration of Aβ(25–35) did not augment accumulated mtDNA4834 deletions in various brain regions of FD rats. Compared with Aβ+FD rats, rats fed the FS diet had reduced levels of mtDNA4834 deletions in hippocampal, medullary and hepatic tissues (P < 0·05), alleviating the brain mtDNA damage of Aβ+FD rats to background levels of the vehicle control group. Similar changes in mtDNA deletions in response to dietary folate intake were observed in the cortical tissue of Aβ+FD rats, but without statistical significance.
a,b,c Mean values within a row with unlike superscript letters were significantly different (P < 0·05).
* Data were analysed by one-way ANOVA and Duncan's multiple range test.
† FD, MF and FS indicate no folate (folate deprivation), moderate folate (+8 mg folic acid/kg diet) and folic acid-supplemented (+8 mg folic acid/kg diet and 0·003 % folic acid in drinking-water: 68 μm) diets, respectively. The MF group receiving the vehicle microinjection was designated the control. Aβ administration included an intracerebroventricular microinjection of 8 μl of Aβ(25–35) peptide (1 mg/ml). Vehicle administration included an intracerebroventricular microinjection of 8 μl of the vehicle solution (sterile distilled water).
‡ The quantity of mtDNA4834 deletions was determined by co-amplifying the mtDNA D-loop and mtDNA4834 deletion in a real-time PCR assay. The relative frequencies of mtDNA4834 deletions to mtDNA were calculated using ΔC t = mt C t del − mt C t D-loop; a smaller ΔC t value indicates more deletions.
Relationships between folate levels and mitochondrial DNA4834 deletions in various brain regions and liver of rats
We pooled the data of the vehicle- and Aβ-injected groups to study the relationships between tissue folate levels and mtDNA deletions in brain regions and the liver. Fig. 1 shows that increased frequencies of mtDNA4834 deletions were significantly associated with reduced folate levels in hippocampal (r − 0·593, P = 0·001), medullary (r − 0·345, P = 0·042) and hepatic tissues (r − 0·547, P = 0·002). Such a folate level–mt genotoxicity relationship was not observed in the cortex tissue (r − 0·242, P = 0·133).
Dietary folate modulated neuronal death of rats in the presence/absence of an β-amyloid peptide challenge
To investigate whether dietary folate intake and/or Aβ challenge may involve in alternative mechanisms to affect the cortex region, the neuronal death of the frontal cortical brain tissues of rats fed various folate diets was assayed. Fig. 2 shows that neuronal cell death was only occasionally observed in the cortex brain of control rats (Fig. 2(A)). Neuronal death in brain tissues of FD rats significantly increased by 2·5-fold compared with the counterpart tissue of the control group (Fig. 2(B) and (E)). Administration of Aβ(25–35) did not aggravate the neuronal death rate of FD rats (Fig. 2(C) and (E)). Aβ-treated rats fed the FS diet had significantly reduced neuronal death compared with Aβ+FD rats (Fig. 2(D) and (E)). When compared with the control group, feeding rats the FS diet completely prevented Aβ+FD-promoted neuron death (Fig. 2(E)).
Discussion
Our data demonstrated that hippocampal, as opposed to cortical and medullary, tissue was the most vulnerable brain region for oxidative lipid damage in response to dietary FD. Feeding rats an FD diet for 4 weeks significantly elevated TBARS levels in the hippocampus tissue compared with the counterpart tissue of control rats. The hippocampal oxidative injuries of FD rats might have been partially, if not totally, due to rapid folate depletion, as 4 weeks of the FD diet significantly decreased hippocampal folate levels by 50 % without affecting cortical folate levels (Table 2). Folate was proposed to possess in vitro and in vivo antioxidant capabilities to scavenge free radicals(Reference Joshi, Adhikari and Patro39, Reference Doshi, McDowell and Moat40). Numerous investigations have shown that folate deficiency promotes H2O2 generation and lipid peroxidation in human cells and rodent tissues(Reference Chen, Huang and Wei41–Reference Huang, Hsu and Lin43). Alternatively, a folate deficiency induced elevated homocysteine levels in neuronal cells, a well-known pro-oxidant to elicit lipid peroxidation and elevated oxidative stress(Reference Chern, Huang and Chen42–Reference Kruman, Kumaravel and Lohani45). Consistently, we have previously shown that feeding rats an FD diet for 4 weeks elevated serum homocysteine levels, which were associated with brain oxidative DNA damage as well as increased hepatic lipid peroxidation(Reference Chou, Yu and Huang25, Reference Huang, Hsu and Lin43). Although elevated brain homocysteine levels were not measured in the present study, our data showed that 4 weeks of the FD diet significantly promoted higher levels of TBARS in the liver of rats, in parallel with FD-induced hippocampal folate depletion and oxidative lipid damage (Tables 2 and 3). Collectively, the findings suggest that rats fed an FD diet attained various degrees of brain folate depletion, which may be partially ascribed to the different magnitude of lipid peroxidation in brain regions.
Dietary FD significantly increased the accumulation of large mtDNA deletions in the hippocampal and medullary regions of rats, but not in the cortex tissue. The frequencies of mtDNA deletions in the hippocampal and medullary regions were significantly and inversely correlated with their respective brain folate levels (Fig. 1). This finding is in accordance with our previous observation that an FD diet depleted brain folate levels and promoted the accumulation of large mtDNA deletions in whole-brain homogenates of rats(Reference Chou, Yu and Huang25). A study has revealed that FD impaired mt antioxidant status, promoted superoxide overproduction and elevated mt protein oxidative damage(Reference Chang, Yu and Lu46). As reactive oxygen species production can lead to the loss of mtDNA molecules(Reference Suematsu, Tsutsui and Wen47), the FD-elicited oxidative stress inside FD neurons may be attributable to increased mtDNA deletions of the hippocampal and medullary regions. Such oxidative injuries in mtDNA, however, were not found in the cortex tissue of rats fed with the 4-week FD diet. As the 4-week FD did not significantly affect cortex folate levels (Table 2), the lack of oxidative mtDNA damage in the FD cortex region further supports the antioxidant role of folate. It has been reported that feeding rats a folate/methyl-deficient diet for 16–18 weeks induced oxidative stress and DNA damage in the cortex of the brain(Reference Bagnyukovaa, Powell and Oleksandra Pavliv48), suggesting a long-term effect of FD on cortical oxidative injuries.
Dietary FD was shown to sensitise neurons to amyloid toxicity(Reference Kruman, Kumaravel and Lohani45), a hallmark of AD. Our data extend this previous finding to demonstrate that a single icv injection of the aggregated Aβ peptide augmented lipid peroxidation in the medullary tissue of folate-deprived rats, which could be ameliorated by feeding FD rats with the MF and FS diets. This observation supports the antioxidant role of folate against Aβ-promoted oxidative injuries. Furthermore, we found that the FS diet, but not the MF diet, significantly diminished mtDNA deletions in the hippocampus and medulla of FD rats upon Aβ challenge. It suggests a threshold effect of dietary folate levels, which protect against FD-associated mtDNA degeneration. Consistently, results of several studies have shown that high levels of folic acid supplementation may counteract mtDNA oxidative injuries and mt dysfunction in macrophage cells and hepatocytes(Reference Chang, Yu and Lu46, Reference Huang, Yaong and Chen49). By folic acid supplementation, the mt respiratory function and mt-associated death signalling were modulated to reduce apoptotic death(Reference Huang, Yaong and Chen49, Reference Ye, Chan and Liu50). Given the fact that feeding the FS diet significantly reduced cortical neuronal death of Aβ-treated and folate-deprived rats (Fig. 2), the finding implied a folate-associated death signalling involved in the neuronal death of FD rats. Whether or not this is the alternative mechanism behind the reported association between folate and cortical neuronal death remains to be definitively established.
The present study had a number of limitations. The relatively small sample size due to the premature death of animals receiving injection surgery may reduce the statistical power for subgroup analysis. Several groups(Reference Sun and Alkon30, Reference Stepanichev, Moiseeva and Lazareva33) used Aβ(35–25), an 11-amino acid with a sequence that was the reversal of ordering of Aβ(25–35), as a control to test the specificity of the toxic amino acid sequence of Aβ(25–35). Whether the oxidative stress of brain regions induced by Aβ(25–35) injection was specific to the toxic effect of Aβ(25–35) remains to be clarified. As haematoxylin–eosin staining used in the present study is not a good assay to evaluate apoptotic death, alternative measurements for chromatin condensation and caspase activation will be used for further studies.
Given the assumptions and limitations of the in vivo study, the results in the present study suggest that dietary FD differentially depleted brain folate, and increased lipid peroxidation and mtDNA4834 deletions in various brain regions. The hippocampal tissue was the most vulnerable brain region for oxidised lipid and mtDNA damage in response to dietary FD. The FS diet was biologically effective at enriching brain folate, and protecting AD-susceptible brains against FD-induced mt genotoxicity and neurotoxicity upon Aβ challenge. Whether the effects of folic acid supplementation found in the present in vivo study have physiological relevance in humans remains to be clarified.
Acknowledgements
The present study was funded by a grant from the National Science Council, Taiwan, ROC (NSC97-2815-C-030-009-B) and by grants-in-aid from Fu-Jen University (9991A15/109631060995-6; 109731060995-6; and 109831060995-6). None of the authors has any conflict of interest to declare. T.-F. C., M.-J. C. and C.-T. H. contributed equally to technical support and data analysis. M.-C. T., S.-J. W. and C.-C. W. contributed to animal care and surgery. R.-F. S. H. contributed to the study design, supervision of experimental execution and manuscript preparation.