Hostname: page-component-586b7cd67f-t8hqh Total loading time: 0 Render date: 2024-11-24T12:45:39.626Z Has data issue: false hasContentIssue false
  • English
  • Français

Nutritional rehabilitation of mitochondrial aberrations in aplastic anaemia

Published online by Cambridge University Press:  14 December 2010

Ling He ,
Xiaoyan Miao ,
Guangyan Lv ,
Peiman Yang ,
Wenguo Wu  and
Li Jia
Ling He
Affiliation:
College of Laboratory Medicine, Dalian Medical University, 9 Lushunnan Road Xiduan, Dalian 116044, Liaoning Province, China
Xiaoyan Miao
Affiliation:
College of Laboratory Medicine, Dalian Medical University, 9 Lushunnan Road Xiduan, Dalian 116044, Liaoning Province, China
Guangyan Lv
Affiliation:
Central Laboratory, Dalian Medical University, Dalian 116044, Liaoning Province, China
Peiman Yang
Affiliation:
Department of Histology and Embryology, Dalian Medical University, Dalian 116044, Liaoning Province, China
Wenguo Wu
Affiliation:
ZHEN-AO Group Company, Dalian, Liaoning Province, China
Li Jia*
Affiliation:
College of Laboratory Medicine, Dalian Medical University, 9 Lushunnan Road Xiduan, Dalian 116044, Liaoning Province, China
*
*Corresponding author: Dr Li Jia, email [email protected]
Rights & Permissions [Opens in a new window]

Abstract

Aplastic anaemia (AA) is a disease characterised by bone marrow hypocellularity and peripheral blood pancytopenia. AA is also associated with mitochondrial aberrations. The present study was undertaken primarily to test the hypothesis that a nutrient mixture could affect the nutritional rehabilitation of mitochondrial aberrations in AA mice. BALB/c AA mice were induced by a combination of hypodermic injections of acetylphenylhydrazine (100 mg/kg), X-rays (2·0 Gy) and intraperitoneal injections of cyclophosphamide (80 mg/kg). We treated these mice with nutrient mixture-supplemented diets in a dose-dependent manner (1445·55, 963·7, 674·59 mg/kg per d), and the effects of the nutrient mixture for mitochondrial rehabilitation were analysed in AA mice. Transmission electron microscopy showed that mitochondrial ultrastructural abnormalities in bone marrow cells, splenocytes and hepatocytes of the nutrient mixture groups were restored markedly, compared with the AA group. Mitochondrial membrane potentials of the nutrient mixture groups were increased remarkably. Western blot analysis also revealed that the nutrient mixture significantly inhibited cytochrome c release of mitochondria in the AA group. Furthermore, the mitochondrial DNA content of the nutrient mixture groups was also increased. Our data suggest that the nutrient mixture may promote the rehabilitation of mitochondrial aberrations, and consequently protects against mitochondrial dysfunction in AA mice.

Keywords

Nutrient mixtureAplastic anaemiaMitochondria
Type
Full Papers
Information
British Journal of Nutrition , Volume 105 , Issue 8 , 28 April 2011 , pp. 1180 - 1187
Copyright
Copyright © The Authors 2010

Aplastic anaemia (AA) is a serious medical disorder that is characterised by bone marrow hypocellularity and peripheral blood pancytopenia. The major signs and symptoms are exhaustion, infections and bleedings(Reference Young1). AA is a heterogeneous disease, which involves destruction of haematopoietic stem cells, disturbance of haematopoietic microenvironment, immune-mediated reaction against haematopoietic tissue or a combination of factors(Reference Laveder and Marcolongo2). Clinical and experimental evidence suggests that AA has been strongly associated with exposure to environmental factors including radiation, drugs and chemicals and viruses(Reference Young1). In our experiments, the AA mouse model was induced by a combination of acetylphenylhydrazine, X-rays and cyclophosphamide, and this model shared many similarities with the human condition of AA(Reference Benzi, Corona and Frico3Reference Stojanović, Milenković and Jovcić5).

Mitochondria are double-membrane organelles that are present in the cytoplasm of most eukaryotic cells. Mitochondria generate most of the cellular ATP via oxidative phosphorylation in an oxygen-dependent process. In addition to supplying cellular energy, mitochondria are involved in cell signalling, cellular differentiation and apoptosis, as well as in the control of the cell cycle and cell growth. The number of mitochondria in a cell varies widely by organism and tissue type(Reference Naviaux6). Mitochondrial dysfunction is a hallmark of almost all diseases, including cancer and multiple neurodegenerative diseases(Reference Seppet, Gruno and Peetsalu7). Mitochondria are under the dual genetic control of both mitochondrial genome (mtDNA) and nuclear DNA(Reference He, Luo and Proctor8). Mutations in mtDNA may be associated with some haematological diseases, including acquired sideroblastic anaemia, myelodysplastic syndromes and acquired AA(Reference Gattermann9Reference Kim, Shin and Kim11).

Nutritional rehabilitation has emerged as a promising component of comprehensive treatment and rehabilitation. It plays a significant role in improving metabolism, enhancing immunity of patients and maintaining normal physiology. Our previous data showed that a nutrient mixture played a key role in the nutritional rehabilitation of AA mice. Here, we first employed the AA mouse model to investigate the role by which a nutrient mixture mediates the rehabilitation of mitochondrial aberrations. A nutrient mixture (containing nucleotides, arginine, phosphatidylcholine, phosphatidylethanolamine, Mn, Zn, vitamin, folate, grape seed extract (GSE) powder, etc.) was administered to AA mice in a dose-dependent manner by intragastric administration over a 45 d dosing period. This experiment was devised to use the nutrient-mixture-treated AA mouse model to examine the changes in mitochondrial aberrations. The present results show that the nutrient mixture can promote the rehabilitation of mitochondrial aberrations in AA mice.

Materials and methods

Animals and treatments

Male BALB/c mice (8 weeks old) were obtained from Animal Facility of Dalian Medical University. Animals were individually housed in plastic cages and placed in an air-conditioned room with a 12 h light–12 h dark cycle, at a temperature of 20 ± 2°C and a relative humidity of 55 ± 10 %. They were maintained under specific pathogen-free conditions in the Animal Facility of Dalian Medical University and were fed ad libitum with the standard diet and water throughout the experimental period.

After a 1-week adaptation period, 100 mice were randomly divided into five groups with twenty in each group: the control group; the AA group; the three different doses of the nutrient-mixture-supplemented diet groups. The mice of the AA model group and of the three different doses of the nutrient mixture groups were treated with a combination of hypodermic injections of acetylphenylhydrazine (100 mg/kg; Sigma, St Louis, MO, USA), X-rays (2·0 Gy) and intraperitoneal injections of cyclophosphamide (80 mg/kg; Sigma). The control group was treated with lead shielding irradiation alone and injections of physiological saline. After the 7th day, the mice of the nutrient mixture groups were given a nutrient-mixture-supplemented diet in a dose-dependent manner (1445·55, 963·7, 674·59 mg/kg per d, according to a Chinese Medical Dictionary) by intragastric administration. The control and AA model groups were given a physiological saline (10 ml/kg per d)-supplemented diet by intragastric administration. During the supplemented dosing period, body weights of animals were determined daily throughout the course of the experiment.

After 7 weeks, mice were killed by cervical dislocation, and then the following physiological conditions were determined: blood, mitochondria of bone marrow, spleen and liver cells, mitochondrial membrane potential (MMP), mtDNA content and release of cytochrome c. All animal experiments were performed according to the guidelines for the care and use of animals approved by the Dalian Medical University.

The nutrient mixture was supplied by Zhen-Ao Group Co., Ltd (Dalian, China) and composed of nucleotides (22·8 %), arginine (5·7 %), lysine (5·7 %), cysteine (3·4 %), glycine (6·8 %), histidine (5·7 %), lecithin (27·4 %), cephalin (13·6 %), vitamin mix (containing vitamin E, vitamin C, vitamin B6, vitamin B12 and folate) (1·58 %), Zn (0·13 %), Mn (0·11 %), Fe (0·28 %), medlar polysaccharides (3·4 %) and GSE (3·4 %). According to the proto-prescription, oral application was prepared by decocting, ultrasound and concentrating.

Analysis of peripheral blood

Blood was obtained from mice and mixed immediately with dipotassium EDTA (Sigma). Blood samples were analysed using the Sysmex KX-21N Blood Cell analyser (Kobe, Japan).

Transmission electron microscopy studies

Fresh tissues (bone marrow, spleen and liver) were processed for transmission electron microscopy. These samples were first washed with phosphate-buffered saline for 5 min, fixed with 2·0 % glutaraldehyde in 0·1 m phosphate buffer (pH 7·4), washed in 0·1 m phosphate buffer and post-fixed in 1·0 % osmium tetroxide in 0·1 m phosphate buffer (pH 7·4). The samples were then dehydrated and were finally embedded in Epon 812 solution for ultrathin sectioning. The ultrathin sections were stained with uranyl acetate and lead citrate and were viewed with a JEM-2000EX transmission electron microscope at a voltage of 120 kV. Transmission electron microscopic examinations of ultrathin sections were under 100 fields of vision.

Cell isolation and culture

Under aseptic conditions, femora were removed, with the surrounding muscle, and placed in 5 ml of sterile 90 % Roswell Park Memorial Institute 1640 (RPMI-1640) medium (Gibco, Grand Island, NY, USA), supplemented with 10 % fetal bovine serum (Gibco). Then, the muscle and epiphyses were removed from femora and marrow and flushed into 5 ml of sterile 90 % RPMI-1640 medium supplemented with 10 % fetal bovine serum.

Spleens and livers were dissected from mice, followed by the preparation of single cell suspensions under aseptic conditions. They were dissected and cut into small pieces, rinsed twice with phosphate-buffered saline and minced with forceps and scalpel. The suspension was passed through a 100 μm stainless-steel mesh, treated with a hypotonic buffer (0·15 m-NH4Cl, 0·01 m-KHCO3, 0·1 mm-Na2EDTA, pH 7·4) for 5 min at room temperature to lyse erythrocytes, centrifuged (1200 rpm, 10 min) and washed twice with cell medium (90 % RPMI-1640 supplemented with 10 % fetal bovine serum and 1 % antibiotic). Splenocytes were incubated in dishes for 2 h to remove adherent cells, and the cells obtained were cultured in cell medium. Hepatocytes were incubated in cell medium (90 % RPMI-1640 containing 0·05 % collagenase, supplemented with 10 % fetal bovine serum and 1 % antibiotic).

The viability of the cells was determined by trypan blue (Sigma) exclusion, and cell density was adjusted to 5 × 105 cells/ml for the MMP assay.

Mitochondrial membrane potential assay

Rhodamine 123 (Rh123) is a voltage-sensitive mitochondrial dye that is able to enter the mitochondrial matrix and accumulate in the mitochondria according to the MMP. The mitochondrial uptake of Rh123 has been measured to determine the MMP(Reference Johnson, Walsh and Chen12). Bone marrow cells from the mice were harvested and washed thrice with phosphate-buffered saline. The cells were resuspended to 5 × 105 cells/ml in fresh incubation medium containing 1·0 μm-Rh123 and incubated at 37°C in a thermostatic bath for 10 min with gentle shaking. They were then separated by centrifugation, and the amount of Rh123 remaining in the incubation medium was measured using a fluorescence spectrophotometer set (Hitachi 650-60; Tokyo, Japan) at 490 nm excitation and 520 nm emission wavelengths. Results are shown as the fluorescence retained within the cells.

Changes in the MMP of splenocytes and hepatocytes were examined according to the methods described earlier.

Isolation of mitochondria and cytosol

Mitochondria were extracted from bone marrow-nucleated cells, splenocytes and hepatocytes according to the manufacturer's protocol of the KeyGen mitochondria isolation kit. The cells were harvested and washed twice with phosphate-buffered saline for 5 min at 800 g at 4°C to the amount of 5 × 107, and were mixed with ice-cold lysis buffer (1·5 ml) and triturated fifty times at 0°C. The suspension was then centrifuged for 5 min at 800 g at 4°C, and then its supernatant was added to ice-cold medium buffer and centrifuged for 10 min at 15 000 g at 4°C. The supernatant thus obtained was used to detect cytochrome c in cytosolic fractions, while the pellet was resuspended in wash buffer and centrifuged for 10 min at 15 000 g at 4°C to remove its supernatant for extracting mtDNA.

Western blot analysis

Western blot analysis was performed to evaluate cytochrome c protein levels. The cytosolic proteins were subjected to 10 % SDS-PAGE, blotted onto polyvinylidene fluoride membranes (Pall Corporation, Pensacola, FL, USA) and detected by using an enhanced chemiluminescence Western blot kit (Amersham Biosciences, Little Chalfont, Buckinghamshire, UK). Rabbit anti-mouse cytochrome c (sc-7159; Santa Cruz Biotechnology, Santa Cruz, CA, USA) and glyceraldehyde-3-phosphate dehydrogenase (sc-20 741; Santa Cruz Biotechnology) polyclonal antibody were purchased from Santa Cruz Biotechnology. The bands were analysed with LabWorks (TM version 4.6; UVP, BioImaging Systems, Upland, CA, USA).

Mitochondrial DNA content assay

mtDNA was extracted from mitochondria according to the manufacturer's protocol of the General AllGen Kit (Beijing CoWin Biotech Co., Ltd, Beijing, China). Mitochondria were suspended in ice-cold buffer CL (300 μl) and agitated for 10 s. RNase A (1·5 μl) was added to the suspension and mixed adequately for 45 min at 37°C. After standing on ice for 1 min, buffer PP was added to the suspension and agitated for 20 s, and then centrifuged for 3 min at 12 000 g. Its supernatant was suspended to isopropanol and centrifuged for 1 min at 12 000 g. Its pellet was suspended in 70 % alcohol (300 μl) and centrifuged for 1 min at 12 000 g. Its supernatant was removed, and mtDNA was dried at room temperature for 15 min. Buffer CL was added to the mtDNA to detect its level with an ultraviolet spectrophotometer.

Statistics

Statistical analysis was performed using SPSS 12.0 software. Each assay was performed at least three times. Data are expressed as means and standard deviations, and Student's t test was used to determine the significance of differences in multiple comparisons. P < 0·05 was considered to be statistically significant.

Results

Nutrient mixture effects on the peripheral blood of aplastic anaemia mice

We used the Sysmex KX-21N Blood Cell analyser to test the effects of nutrient mixture on the peripheral blood of AA mice. After 7 weeks, a significant peripheral blood pancytopenia was evident in AA mice (Table 1). Erythrocytes, leucocytes, Hb and the platelet mean count were conspicuously reduced to 64·5, 75·3, 53·4 and 60·2 % of the control mean values, respectively (P < 0·05 for all parameters).

Table 1 The effect of nutrient mixture on the peripheral blood of mice (Mean values and standard deviations)

Plt, platelets; AA, aplastic anaemia.* Mean value was significantly different from that of the control group (P < 0·05).† Mean value was significantly different from that of the AA group (P < 0·05).

The profound effects of the nutrient mixture on AA mice were also observed in the peripheral blood parameters. Erythrocytes, leucocytes, Hb and platelet counts in the three different doses of the nutrient mixture groups were higher than in the AA group in a dose-dependent manner (P < 0·05; Table 1). This result showed that the nutrient mixture indeed had an effect on peripheral blood cell levels in AA mice.

Nutrient mixture restores mitochondrial ultrastructure in aplastic anaemia mice

We performed transmission electron microscopic studies on the bone marrow, spleen and liver of AA mice and found that mitochondrial ultrastructure was clearly affected by the nutrient mixture diet (Fig. 1). The size and shape of mitochondria of the control group were normal. In contrast, in the AA group, mitochondria had enlarged globular structures, accompanied by the disruption or disappearance of the cristae (Fig. 1(a–c)).

Fig. 1 Effects of nutrient mixture on the mitochondrial morphology of aplastic anaemia (AA) mice. (a) Representative transmission electron micrographs (20 000 × ) of mitochondrial structures from haematopoietic cells in the control mice, AA mice and nutrient-mixture-treated AA mice are shown. (b) Representative transmission electron micrographs (20 000 × ) of mitochondrial structures from spleens of the control mice, AA mice and nutrient-mixture-treated AA mice are shown. (c) Representative transmission electron micrographs (20 000 × ) of mitochondrial structures from livers of the control mice, AA mice and nutrient-mixture-treated AA mice are shown.

Remarkably, mitochondrial ultrastructure was restored in the nutrient mixture groups, compared with the AA group. These results showed that nutrient mixture might promote mitochondrial rehabilitation in AA mice.

Nutrient mixture effects on the mitochondrial membrane potential in aplastic anaemia mice

As transmission electron microscopy findings revealed mitochondrial damage, we assayed through a fluorescence spectrophotometer set to determine the nutrient mixture effect on the MMP in AA mice. We examined the MMP by measuring the relative differences in the fluorescence of Rh123 among three kinds of cells in the five groups. The results showed that the Rh123 fluorescence of bone marrow cells in the AA group (19·7 (sd 2·26)) was lower than that in the control group (31·9 (sd 3·62); P < 0·05), and the Rh123 fluorescence of splenocytes in the AA group (17·2 (sd 1·21)) was lower than in the control group (19·6 (sd 1·23); P < 0·05). In addition, the Rh123 fluorescence of hepatocytes in the AA group (25·6 (sd 2·13) was lower than that in the control group (13·2 (sd 1·02); P < 0·05) (Fig. 2). However, the Rh123 fluorescence of the three kinds of cells in the three different doses of the nutrient mixture groups was higher than that in the AA group in a dose-dependent manner (P < 0·05) (Fig. 2). This result showed that nutrient mixture affected remarkably the recovery of the MMP of AA mice in a dose-dependent manner.

Fig. 2 Effects of nutrient mixture on the mitochondrial membrane potential in cells of aplastic anaemia (AA) mice. ■: Bone marrow cells from the control mice, AA mice and nutrient-mixture-treated AA mice were stained with rhodamine 123; □: splenocytes from the control mice, AA mice and nutrient-mixture-treated AA mice were stained with rhodamine 123; : hepatocytes from the control mice, AA mice and nutrient-mixture-treated AA mice were stained with rhodamine 123 (* P < 0·05 v. control; † P < 0·05 v. AA).

Nutrient mixture effects on the release of cytochrome c of aplastic anaemia mice

To examine the effect of nutrient mixture on the release of cytochrome c of AA mice, Western blot analysis was employed to analyse the release of cytochrome c, which is from the mitochondria to the cytosol. Cytochrome c expression was variable among the mouse models, with a higher cytochrome c level detected in the cells of the AA group and no detectable level in the cells of the control group. However, the cytochrome c levels of the three kinds of cells in the nutrient mixture groups were markedly lower than that in the AA group (Fig. 3), indicating that nutrient mixture mediated the decrease in cytochrome c levels of AA mice in a dose-dependent manner.

Fig. 3 Effects of nutrient mixture on the cytochrome c (cyt c) release of mitochondria in aplastic anaemia (AA) mice. The cyt c release assay was performed by Western blot analysis, which was performed on the cytosolic protein fractions of cells (bone marrow cells (a), splenocytes (b) and hepatocytes (c)). After the cells (bone marrow cells, splenocytes and hepatocytes) were lysed, the cytosolic fraction was isolated and SDS-PAGE was carried out. Monoclonal antibody detected an 11 kDa band containing cyt c. Glyceraldehyde-3-phosphate dehydrogenase (GAPDH) blotting was used as the control. The relative expression of cytosolic cyt c was expressed as a percentage of GAPDH (* P < 0·05 v. control; † P < 0·05 v. AA).

Nutrient mixture effects on the mitochondrial DNA content of aplastic anaemia mice

In order to determine whether the nutrient mixture had effects on the mtDNA content of AA mice, an ultraviolet spectrophotometer assay was used to measure mtDNA content in the three kinds of cells in the five groups. The results showed that the mtDNA content of bone marrow cells in the AA group (0·24 (sd 0·01) μg/ml) was lower than that in the control group (0·53 (sd 0·02) μg/ml; P < 0·05). The mtDNA content of splenocytes in the AA group (0·85 (sd 0·12) μg/ml) was lower than that in the control group (0·98 (sd0·13) μg/ml; P < 0·05), and the mtDNA content of hepatocytes in the AA group (1·03 (sd 0·06 μg/ml) was lower than that in the control group (1·86 (sd 0·24) μg/ml, P < 0·05) (Fig. 4). However, the mtDNA content of the three kinds of cells in the three different doses of the nutrient mixture groups was higher than that in the AA group in a dose-dependent manner (P < 0·05) (Fig. 4). These results suggested that the nutrient mixture could promote the recovery of mtDNA content of the AA mice in a dose-dependent manner.

Fig. 4 Effects of nutrient mixture on the mitochondrial DNA content of aplastic anaemia (AA) mice. ■: Mitochondrial DNA (mtDNA) content of bone marrow cells from the control mice, aplastic anaemia (AA) mice and nutrient-mixture-treated AA mice; □: mtDNA content of splenocytes from the control mice, AA mice and nutrient-mixture-treated AA mice; : mtDNA content of hepatocytes from the control mice, AA mice and nutrient-mixture-treated AA mice. (* P < 0·05 v. control; † P < 0·05 v. AA).

Discussion

AA is characterised by hypocellular bone marrow resulting from damage to haemopoietic stem cells. This produces pancytopenia with the risk of severe anaemia, major haemorrhage and life-threatening infections. However, the fundamental pathophysiology of AA is not well understood. In the present study, this new animal model of AA is convenient to use and has the potential for further investigation of roles of the nutrient mixture to mediate the mitochondrial rehabilitation of AA mice.

In our experiments, the AA mouse model was induced by the combination of acetylphenylhydrazine, X-rays and cyclophosphamide. Animals show statistically significant reductions in peripheral blood leucocytes, erythrocytes, Hb and platelets (Table 1), and even more severe reductions in humeral marrow cells and marrow-committed progenitor cells. These are clinical characteristics of AA. Although many factors are involved in assessing overall health status in patients with AA, nutrition plays a significant role in influencing AA biology, co-morbid conditions and responses to treatment. In the present study, we found that the nutrient mixture could mediate the mitochondrial rehabilitation of AA mice. This stress response, mediated by the complex interaction of nucleotides, arginine, phosphatidylcholine, phosphatidylethanolamine, Mn, Zn, vitamin, folate, GSE powder, etc., can ultimately lead to a nutritional rehabilitation of mitochondrial aberrations in AA mice.

Nucleotides are essential nutrients that modulate cell proliferation and differentiation, lipid metabolism and immune function. Dietary nucleotide supplementation promotes the redox state, efficiency of protein synthesis and restoration of the function and number of mitochondria(Reference Pιrez, Sαnchez-Medina and Torres13). Amino acids play a significant role in nutrition and disease in humans. Arginine displays crucial metabolic and regulatory versatility in cells. As the physiological nitrogenous precursor for the synthesis of NO, arginine can increase NO synthesis, which mediates the stimulatory action of arginine on the mitochondrial oxidation of energy substrates(Reference Fu, Haynes and Kohli14). Glycine prevents hypoxia, free radical formation, cell swelling and the hypermetabolic state(Reference Zhong, Li and Yamashina15). Dietary supplementation of patients taking Cylosporin A with glycine should be useful to prevent some side effects of this immunosuppressive drug(Reference Zhong, Li and Yamashina15, Reference Zhong, Arteel and Connor16). Humans and other mammals cannot synthesise vitamins and folate, so they must be obtained from exogenous sources via absorption in the intestine. Vitamins are important micronutrients for humans. Vitamin E is the major lipid-soluble, chain-breaking antioxidant and plays an essential role in maintaining the integrity of biological membranes, reproduction, preventing lipid peroxidation and other radical-driven oxidative events(Reference Brigelius-Flohι and Traber17). As a factor, vitamin E participates in the mitochondrial electron transport system, and vitamin E deficiency may cause a respiratory decline in mitochondria(Reference Chen and Chang18). So dietary vitamin E can prevent mitochondrial damage and restore mitochondrial function. As an aqueous free radical trap, vitamin C can increase the antioxidant effectiveness of vitamin E; however, it is itself a kind of antioxidant(Reference Heaney, Gardner and Karasavvas19). The effect of vitamin C on viability, reactive oxygen species and MMP has been determined(Reference Heaney, Gardner and Karasavvas19). Vitamin B6 deficiency affects ultrastructural abnormalities in the central nervous system. On account of vitamin B12 containing the metal cobalt, it is also called cobalamin. An adequate supply of vitamin B12 and folic acid is essential for human health and well-being; thus there is a variety of clinical abnormalities that can occur as a result of vitamin B12 and folic acid deficiency(Reference Hanna, Lachover and Rajarethinam20, Reference Said, Chatterjee and Haq21). Zn is an essential cofactor that serves a variety of biochemical processes including cellular respiration, cellular utilisation of oxygen, DNA and RNA, reproduction, maintenance of cell membrane integrity and sequestration of free radicals(Reference Yousef, El-Hendy and El-Demerdash22). As an enzyme activator, Mn plays a significant role in enzymatic synthesis, and Mn deficiency can result in membrane damage, which is due to the accumulation of free inside the mitochondria(Reference de Rosa, Keen and Leach23). Fe, a kind of microelement, is related to biological function. Fe deficiency can result in mitochondrial dysfunction and mtDNA damage(Reference Walter, Knutson and Paler-Martinez24). GSE is a complex mixture of polyphenols including procyanidins and proanthocyanidins. As a free radical scavenger, GSE has a protective effect on oxidant-induced production and deposition of extracellular matrix components(Reference Dulundu, Ozel and Topaloglu25).

In the present study, AA mice were treated with the nutrient-mixture-supplemented diets in a dose-dependent manner including the above-mentioned nutritive substances, and changes were measured. The results presented in Table 1 demonstrated that AA mice treated with the nutrient-mixture-supplemented diets appear to be sensitive to the nutrient mixture, and the haematological parameters of these animals become more significantly affected than the changes observed in the AA group. There was a very significant increase in Hb, erythrocytes, leucocytes and platelet counts (P < 0·05 v. AA group). This result showed that the nutrient mixture had indeed an effect on peripheral blood cell levels in AA mice.

Mitochondria are double-membrane organelles that play a major role in providing energy and in regulating osmotic pressure, Ca homeostasis and cell signalling(Reference He, Luo and Proctor8). Mitochondrial aberration is often accompanied by changes in mitochondrial morphology. The results demonstrated that the mitochondria of bone marrow cells, splenocytes and hepatocytes were swollen, and the cristae were fragmented and solubilised in the AA group. However, the structure of mitochondria in different doses of the nutrient mixture groups was restored (Fig. 1). This is consistent with previously reported results that dietary nutrient mixtures can promote mitochondrial rehabilitation(Reference Brigelius-Flohι and Traber17Reference Heaney, Gardner and Karasavvas19).

MMP, a significant indicator of cellular viability, is important for an integrated appraisal of mitochondrial function(Reference Zhong, Li and Yamashina15). Cytochrome c is a critical factor in the apoptotic process, and rupture of the mitochondrial membrane can result in the release of cytochrome c from the mitochondria into the cytosol(Reference Kluck, Bossy-Wetzel and Green26). We first examined cytochrome c release using Western blot analysis. We found that the nutrient mixture inhibited cytochrome c release (Fig. 3), and that the nutrient mixture changed the MMP (Fig. 2). We also found that dietary supplementation of AA mice with the nutrient mixture mediated these changes in a dose-dependent manner. Similar results were demonstrated that vitamin B6 supplementation prevented the altered MMP in U937 monocytes(Reference Kannan and Jain27).

Mutations and the instability of mtDNA have recently been demonstrated in a wide variety of diseases. Mitochondrial dysfunction and the decrease in the amount of mitochondria may result in the reduction of mtDNA. The present results showed that the nutrient mixture could restore the mtDNA content in a dose-dependent manner, in accordance with the previously reported results that folic acid supplementation may be protective against mtDNA deletions(Reference Branda, Brooks and Chen28).

On the basis of the above-mentioned analysis, the present study has demonstrated that the nutrient mixture promotes the rehabilitation of mitochondrial aberrations in AA mice. To the best of our knowledge, this is the first study to evaluate a nutrient mixture for its nutritional rehabilitation of mitochondrial aberrations, and consequently protects against mitochondrial dysfunction.

Acknowledgements

We thank W. W. for providing the nutrient mixture. Financial support was provided by the Dalian Municipal Science and Technology Plan Project (special item of innovative drugs). L. H. and L. J. had the idea for the study. L. H., P. Y. and L. J. conceived, conceptualised and supervised the study. L. H. performed the experiments. L. H., X. M. and G. L. performed the analysis and interpreted the data. X. M. and G. L. contributed reagents/materials/analysis tools. L. J. revised the manuscript critically. None of the authors had any conflicts of interest.

References

1Young, NS (2002) Acquired aplastic anemia. Ann Intern Med 136, 534546.Google Scholar
2Laveder, F & Marcolongo, R (1996) Uncontrolled triggering of programmed cell death (apoptosis) in haematopoietic stem cells: a new hypothesis for the pathogenesis of aplastic anaemia. Immunol Cell Biol 74, 159162.Google Scholar
3Benzi, G, Corona, GL & Frico, GM (1964) Effect of cobalt on anemia caused by acetylphenylhydrazine. I. Research in normal rats. Boll Soc Ital Biol Sper 40, 12891292.Google ScholarPubMed
4Knospe, WH, Blom, J & Crosby, WH (1968) Regeneration of locally irradiated bone marrow. II. Induction of regeneration in permanently aplastic medullary cavities. Blood 31, 400405.CrossRefGoogle ScholarPubMed
5Stojanović, N, Milenković, P, Jovcić, G, et al. (1989) Polycythemic mice – an appropriate model for investigation of granulopoiesis. Haematologica 74, 1924.Google Scholar
6Naviaux, RK (2000) Mitochondrial DNA disorders. Eur J Pediatr 159, S219S226.Google Scholar
7Seppet, E, Gruno, M, Peetsalu, A, et al. (2009) Mitochondria and energetic depression in cell pathophysiology. Int J Mol Sci 10, 22522303.CrossRefGoogle ScholarPubMed
8He, L, Luo, L, Proctor, SJ, et al. (2003) Somatic mitochondrial DNA mutations in adult-onset leukaemia. Leukemia 17, 24872491.Google Scholar
9Gattermann, N (2004) Mitochondrial DNA mutations in the hematopoietic system. Leukemia 18, 1822.Google Scholar
10Gattermann, N, Retzlaff, S, Wang, YL, et al. (1997) Heteroplasmic point mutations of mitochondrial DNA affecting subunit I of cytochrome c oxidase in two patients with acquired idiopathic sideroblastic anemia. Blood 90, 49614972.CrossRefGoogle ScholarPubMed
11Kim, HR, Shin, MG, Kim, MJ, et al. (2008) Mitochondrial DNA aberrations of bone marrow cells from patients with aplastic anemia. Korean Med Sci 23, 10621067.Google Scholar
12Johnson, LV, Walsh, ML & Chen, LB (1980) Localization of mitochondria in living cells with rhodamine 123. Proc Natl Acad Sci U S A 77, 990994.Google Scholar
13Pιrez, MJ, Sαnchez-Medina, F, Torres, M, et al. (2004) Dietary nucleotides enhance the liver redox state and protein synthesis in cirrhotic rats. J Nutr 134, 25042508.Google Scholar
14Fu, WJ, Haynes, TE, Kohli, R, et al. (2005) Dietary l-arginine supplementation reduces fat mass in Zucker diabetic fatty rats. J Nutr 135, 714721.Google Scholar
15Zhong, Z, Li, X, Yamashina, S, et al. (2001) Cyclosporin A causes a hypermetabolic state and hypoxia in the liver: prevention by dietary glycine. J Pharmacol Exp Ther 299, 858865.Google Scholar
16Zhong, Z, Arteel, GE, Connor, HD, et al. (1998) Cyclosporin A increases hypoxia and free radical production in rat kidneys: prevention by dietary glycine. Am J Physiol 275, F595F604.Google Scholar
17Brigelius-Flohι, R & Traber, MG (1999) Vitamin E: function and metabolism. FASEB J 13, 11451155.Google Scholar
18Chen, LH & Chang, ML (1978) Effect of dietary vitamin E and vitamin C on respiration and swelling of guinea pig liver mitochondria. J Nutr 108, 16161620.CrossRefGoogle ScholarPubMed
19Heaney, ML, Gardner, JR, Karasavvas, N, et al. (2008) Vitamin C antagonizes the cytotoxic effects of antineoplastic drugs. Cancer Res 68, 80318038.CrossRefGoogle ScholarPubMed
20Hanna, S, Lachover, L & Rajarethinam, RP (2009) Vitamin b(12) deficiency and depression in the elderly: review and case report. Prim Care Companion J Clin Psychiatry 11, 269270.Google Scholar
21Said, HM, Chatterjee, N, Haq, RU, et al. (2000) Adaptive regulation of intestinal folate uptake: effect of dietary folate deficiency. Am J Physiol Cell Physiol 279, C1889C1895.Google Scholar
22Yousef, MI, El-Hendy, HA, El-Demerdash, FM, et al. (2002) Dietary zinc deficiency induced-changes in the activity of enzymes and the levels of free radicals, lipids and protein electrophoretic behavior in growing rats. Toxicology 175, 223234.Google Scholar
23de Rosa, G, Keen, CL, Leach, RM, et al. (1980) Regulation of superoxide dismutase activity by dietary manganese. J Nutr 110, 795804.CrossRefGoogle ScholarPubMed
24Walter, PB, Knutson, MD, Paler-Martinez, A, et al. (2002) Iron deficiency and iron excess damage mitochondria and mitochondrial DNA in rats. Proc Natl Acad Sci U S A 99, 22642269.CrossRefGoogle ScholarPubMed
25Dulundu, E, Ozel, Y, Topaloglu, U, et al. (2007) Grape seed extract reduces oxidative stress and fibrosis in experimental biliary obstruction. J Gastroenterol Hepatol 22, 885892.Google Scholar
26Kluck, RM, Bossy-Wetzel, E, Green, DR, et al. (1997) The release of cytochrome c from mitochondria: a primary site for Bcl-2 regulation of apoptosis. Science 275, 11321136.CrossRefGoogle ScholarPubMed
27Kannan, K & Jain, SK (2004) Effect of vitamin B6 on oxygen radicals, mitochondrial membrane potential, and lipid peroxidation in H2O2-treated U937 monocytes. Free Radic Biol Med 36, 423428.Google Scholar
28Branda, RF, Brooks, EM, Chen, Z, et al. (2002) Dietary modulation of mitochondrial DNA deletions and copy number after chemotherapy in rats. Mutat Res 501, 2936.Google Scholar
Figure 0

Table 1 The effect of nutrient mixture on the peripheral blood of mice (Mean values and standard deviations)

Figure 1

Fig. 1 Effects of nutrient mixture on the mitochondrial morphology of aplastic anaemia (AA) mice. (a) Representative transmission electron micrographs (20 000 × ) of mitochondrial structures from haematopoietic cells in the control mice, AA mice and nutrient-mixture-treated AA mice are shown. (b) Representative transmission electron micrographs (20 000 × ) of mitochondrial structures from spleens of the control mice, AA mice and nutrient-mixture-treated AA mice are shown. (c) Representative transmission electron micrographs (20 000 × ) of mitochondrial structures from livers of the control mice, AA mice and nutrient-mixture-treated AA mice are shown.

Figure 2

Fig. 2 Effects of nutrient mixture on the mitochondrial membrane potential in cells of aplastic anaemia (AA) mice. ■: Bone marrow cells from the control mice, AA mice and nutrient-mixture-treated AA mice were stained with rhodamine 123; □: splenocytes from the control mice, AA mice and nutrient-mixture-treated AA mice were stained with rhodamine 123; : hepatocytes from the control mice, AA mice and nutrient-mixture-treated AA mice were stained with rhodamine 123 (* P < 0·05 v. control; † P < 0·05 v. AA).

Figure 3

Fig. 3 Effects of nutrient mixture on the cytochrome c (cyt c) release of mitochondria in aplastic anaemia (AA) mice. The cyt c release assay was performed by Western blot analysis, which was performed on the cytosolic protein fractions of cells (bone marrow cells (a), splenocytes (b) and hepatocytes (c)). After the cells (bone marrow cells, splenocytes and hepatocytes) were lysed, the cytosolic fraction was isolated and SDS-PAGE was carried out. Monoclonal antibody detected an 11 kDa band containing cyt c. Glyceraldehyde-3-phosphate dehydrogenase (GAPDH) blotting was used as the control. The relative expression of cytosolic cyt c was expressed as a percentage of GAPDH (* P < 0·05 v. control; † P < 0·05 v. AA).

Figure 4

Fig. 4 Effects of nutrient mixture on the mitochondrial DNA content of aplastic anaemia (AA) mice. ■: Mitochondrial DNA (mtDNA) content of bone marrow cells from the control mice, aplastic anaemia (AA) mice and nutrient-mixture-treated AA mice; □: mtDNA content of splenocytes from the control mice, AA mice and nutrient-mixture-treated AA mice; : mtDNA content of hepatocytes from the control mice, AA mice and nutrient-mixture-treated AA mice. (* P < 0·05 v. control; † P < 0·05 v. AA).