Abstract
Background
50% to 60% of the people who have recovered from the first episode of depression experience a relapse. The immune system of the people suffering from depression is in a permanent state of pathological pro-inflammatory readiness. There are some reports that depressive episodes cause sensitization of immune-inflammatory pathways and that staing of depression (e.g. number of depressive episodes) is correlated with immune-inflammatory markers.
The main objective of the study was to delineate whether recurrent major depression (rDD) is characterized by alterations in selected immune-inflammatory biomarkers as compared with first episode of depression (ED-I), i.e. expression of mRNA and enzymatic activity of manganese superoxide dismutase (MnSOD, SOD-2), myeloperoxidase (MPO), inducible nitric oxide synthase (iNOS, NOS-2), and cyclooxygenase-2 (COX-2).
Methods
The study was carried out in a group of 131 patients: ED-I group – 42 patients, rDD group – 89 patients. Depression severity was assessed with the 17-item Hamilton Depression Rating Scale (HDRS). The number of depression episodes and the disease duration periods were recorded in each patient. For the patients, HDRS was administered at admission during the symptomatic phase, which would generally be either before or shortly after modification of the previous antidepressant drug regimen. Reassessment of the mental condition was conducted after 8 weeks of the pharmacological treatment also with the use of the HDRS scale.
Results
No significant statistical differences were found between the analysed groups as regards the intensity of depressive disorders. No differences in the expression of MnSOD, MPO, COX-2 and i-NOS genes on the level of both mRNA and protein were observed between both groups. No significant interrelation was noticed between the number of depression episodes experienced and the expression of selected genes on the mRNA level and protein level.
Conclusions
There is no significant difference in MnSOD, MPO, COX-2 and i-NOS between patients with recurrent depressive disorders and those in a first episode of depression. These findings suggest that these enzymes are trait markers of depression and are not related to staging of depression.
Similar content being viewed by others
Background
Annual prevalence of depression in the adult population oscillates between 6% and 12%, and – according to different sources – varies from 5% to even 30% among people over the age of 65 [1]. Depression often accompanies other diseases, which means its symptoms are observed in approximately 10% of all adults within one year (this corresponds to 100 million cases).
Episodes of lower mood last relatively long – from 6 to 9 months. The disease may also take a chronic form, resistant to treatment. Age, at which the first episode takes place, as well as duration, frequency and intensity of episodes are characterised by individual variability [2].
50% to 60% of the people who have recovered from the first episode of depression experience a relapse. In the majority of hospitalised patients another depressive episode appears within the next two years of discharging from the hospital. It is estimated that some 20% of the affected with diagnosed recurrent depressive disorders experience two depressive stages during their life, and 60% – three or more such stages (3–4 on average) [3]. Every successive episode is associated with a less positive prognosis and poorer response to pharmacological treatment [4].
The first hypothesis that macrophages may play a role in depression was published in 1991 by Ronald Smith [5], whereas the first original reports on activation of immune-inflammatory pathways in depression were reported as of 1990 by Maes et al. Today, it is agreed that the immune system of the people suffering from depression is in a permanent state of pathological pro-inflammatory readiness [6]. The symptoms of an ongoing inflammatory process, like fatigue, sleep disorders, anxiety, low mood, loss of appetite or anhedonia, correspond to the symptoms of depressive disorders [7,8]. On the other hand, not only proinflammatory cytokines, e.g. tumor necrosis factor-alpha – (TNF-α), the interleukins (IL) and interferon-gamma (IFN-gamma), but also anti-inflammatory cytokines are released by CNS and peripheral-derived immune cells and play a powerful role in depression [9]. There are data that depressive episodes are accompanied by an increased sensitization of immune-inflammatory pathways and that the number of depressive episodes is correlated with immune-inflammatory markers such as TNF-α and neopterin [10].
The main objective of the study was to examine whether recurrent major depression (rDD) is accompanied by more profound inflammatory disturbances than the first episode of depression (ED-I), i.e. expression of mRNA and protein levels of four inflammatory enzymes, i.e. manganese superoxide dismutase (MnSOD, SOD-2), myeloperoxidase (MPO), inducible nitric oxide synthase (iNOS, NOS-2), and cyclooxygenase-2 (COX-2). Not only do the aforementioned compounds take part in an inflammatory reaction, but they are also active in the production of free radicals, and damage proteins, fatty acids and cellular DNA [11,12]. In our previous studies, we demonstrated that the selected variables (COX-2, iNOS, MnSOD, MPO) can have a significant impact on cognitive functioning in patients with rDD. Therefore, we have made an attempt to assess the level of selected indicators at different stages of the disease (rDD).
Subjects
The study was carried out in a group of 131 patients: ED-I group – 42 patients, rDD group – 89 patients. All patients were hospitalised at Department of Adult Psychiatry Medical University of Lodz (Poland). The selection of individuals for the study group was performed randomly without replacement sampling.
The patients were selected for the study based on the inclusion criteria for ED and rDD outlined in ICD-10 (F32.0-7.32.2, F33.0-F33.8) [13]. The presence of axis I and II disorders, other than depressive episode, and the diagnosis of somatic diseases and injuries of the central nervous system (CNS), were regarded as exclusion criteria. Other exclusion criteria were: inflammatory or autoimmune disorders and unwilling to give informed consent. For all the subjects, a case history was obtained prior to participation using the standardised Composite International Diagnostic Interview (CIDI) [14].
All the subjects were free from medical illnesses, including infections and inflammatory or allergic reactions. None of the control subjects or depressed patients was treated with drugs known to influence lipid metabolism, immune response or endocrine function. None of the participants were drinkers or heavy smokers, and none had ever taken psychotropic drugs.
Methods
Severity of depression
Depression severity was assessed with the 17-item Hamilton Depression Rating Scale (HDRS). A description of HDRS has been presented elsewhere [15,16].
All the subjects were examined during the course of their hospitalisation. The study group included subjects, hospitalised for the first time for depressive episode and depression treatment-naïve, as well as those, treated for many years before and with multiple hospitalisation episodes in history, the latter admitted for various degrees of health deterioration. The number of depression episodes and the disease duration periods were recorded in each patient.
For the patients, HDRS was administered at admission during the symptomatic phase, which would generally be either before or shortly after modification of the previous antidepressant drug regimen. Reassessment of the mental condition was conducted after 8 weeks of the pharmacological treatment also with the use of the HDRS scale. Examination of patients was conducted by the same person in each case.
Whole blood samples from the patients were collected in 5 ml EDTA-containing tubes than centrifuge at 1000xg for 10 min at 4 degrees C and used for isolation peripherial blood lymphocytes. Lymphocytes and serum stored at – 70°C until analysed
mRNA and serum protein expression
COX-2 mRNA and serum protein expression
Analyses were performed according to methods previously described: mRNA expression in the peripheral blood lymphocytes was quantified by real-time PCR using ABI Prism 7000 Sequence Detection System (Applied Biosystems, Foster City, Calif., USA) according to the manufacturer’s protocol [17], serum protein level by ELISA method (COX-2 ELISA Kit, Calbiochem, Merck KGaA, Darmstadt, Germany).
iNOS mRNA and serum protein expression [18]
Nitric oxide was estimated in plasma with the use of Nitric Oxide Non-Enzymatic Assay (cat. No. 12111) Oxis International, Inc. Bioxytech.
Concentration of NO was measured in terms of its products nitrite (NO2-) and nitrate (NO3-). The test is based on the reduction of nitrate to nitrite using the granulated cadmium and conversion, using Greiss reagent, of nitrite into a purple compound – chromophore, which is measured colometrically at 540 nm. NO products are expressed as μM/L of plasma. The human iNOS and GADPH expression the peripheral blood lymphocytes was quantified by real-time PCR using ABI Prism 7000 Sequence Detection System (Applied Biosystems, Foster City, Calif., USA) according to the manufacturer’s protocol [18].
MnSOD mRNA and serum protein expression
The test protein levels were measured in blood serum levels for each patient. These tests were preceded by a determination of serum total protein. Two measurement techniques were employed [19]. For the quantitative detection of serum SOD2 protein levels, a commercial kit, NWLSSTM MnSOD ELISA, was used (Northwest Life Science Specialties LLC, Vancouver, Wash., USA). The human MnSOD and GADPH expression the peripheral blood lymphocytes was quantified by real-time PCR using ABI Prism 7000 Sequence Detection System (Applied Biosystems, Foster City, Calif., USA) according to the manufacturer’s protocol [19].
MPO mRNA and serum protein expression
For the quantitative detection of circulating serum MPO protein level, the commercial Human MPO Immunoassay from R&D Systems, Inc. (Minneapolis, MN, USA), was used. Total RNA (1 μg) was extracted from the the peripheral blood lymphocytes using Trizol reagent (Life Technologies Inc.), and was processed directly to cDNA synthesis using the TaqMan Reverse Transcription Reagents kit (Applied Biosystem) according to the manufacturer’s protocol [20].
Statistical analysis
A statistical analysis of the collected material included calculation of both descriptive and inferential statistics. A two-tailed critical region was employed in the statistical hypothesis testing.
Qualitative characteristics of the experimental and control groups were expressed as frequencies shown as percentages. To characterise the average values for quantitative features, the arithmetical mean (M) and median (Me) were calculated. The measures of statistical dispersion included the range of values between the minimum and the maximum, and the standard deviation (SD).
Distributions were analysed using the Shapiro-Wilk test. To compare nonparametric variables in the test groups, the following tests were used: the Pearson χ2 for qualitative variables, the Wilcoxon signed-rank test for two related groups for quantitative variables, and the Mann–Whitney U test for two independent groups to determine the coincidence of distributions. To evaluate the relations between the analysed variables, Spearman's R rank order correlation coefficients were estimated. For all analyses, statistical significance was defined as p <0.05 [21]. All data analyses were performed using STATISTICA PL, version 10.
Ethics
Before deciding to participate in the study, the subjects were informed of the purpose of the study, assured for voluntary participation, and guaranteed with personal data confidentiality. Written informed consent was obtained according to the study protocol that was approved by the Bioethical Committee of the Medical University of Lodz (No. RNN/728/12/KB).
Results
Average age of all the examined patients (N = 131) was: M = 48.53 years, SD = 11.05; minimum age – 20 years, maximum – 67 years. In the ED-I group, average age was: M = 44.72, SD = 13.03, and in the rDD group: M = 49.89, SD = 9.68. The characteristics of the examined group in Table 1.
No significant statistical differences were found between the examined groups in terms of sex (χ2 = 4.14, p = 0.41) and education (χ2 = 3.27, p = 0.35), only in terms of age (Z = 2.21, p = 0.03).
Significant statistical differences were observed between severity of depression as measured with the HDRS scale in the ED-I and rDD groups on the day of admission to the experiment and after obtaining a response to the applied pharmacological treatment (respectively Z = 5.64, p < 0.001 and Z = 8.18, p < 0.001). This result indicates an improvement in the effect of the incorporated treatment in both the examined groups.
No significant statistical differences were found between the analysed groups as regards the severity of depressive disorders (Table 2). Neither were such differences observed on the day of admission of the patients to the experiment as well as after receiving a response to the implemented pharmacological treatment. In both groups, average level of the symptoms of depressive disorders on the first day of the experiment corresponded to severe level of depressive disorders acc. to the HDRS scale and remission of depressive disorders according the HDRS scale after 8 weeks of the pharmacological therapy.
Table 3 presents average values, standard deviation, minimum and maximum values of expression on the mRNA level and the protein level for the analysed inflammation enzymes: MnSOD, MPO, COX-2 and iNOS in the examined group (N = 131).
Table 4 presents a comparison of expression of the analysed genes on the mRNA level and protein level in the affected from the ED-I and rDD group.
In case of all the variables included in the analysis, no significant statistical differences were found between the ED-I and rDD group. No differences in the expression of MnSOD, MPO, COX-2 and i-NOS genes on the level of both mRNA and protein were observed between the patients with the first episode of depression and diagnosed with rDD.
An average number of depression episodes totalled 6.48 among the patients suffering from rDD (Table 2). No significant interrelation was noticed between the number of depression episodes experienced and the expression of selected genes on the mRNA level and protein level.
In the examined group, there was no significant relationship between the severity of depressive disorders measured before and after pharmacotherapy and the expression on the mRNA level and protein level for the analysed genes.
Discussion
The working hypothesis presented in the introduction was not confirmed. The obtained results indicate no differences in the expression of inflammation enzymes (MnSOD, MPO, COX-2 and iNOS) between patients with the first episode of depression and rDD. However, in our previous experiments we showed that the expression of mRNA and enzyme activity of MnSOD was significantly lower in rDD patients than in controls [19], a phenomenon which could point toward an adaptive MnSOD response to inflammation and increased oxidative stress. Previously, we have shown that myeloperoxidase [20], cyclooxygenase-2 [17] and inducible nitric oxide synthase [18] mRNA expression and protein levels were significantly higher in patients with recurrent depressive disorders than in healthy controls. Therefore, the results may indicate actively progressing immune-inflammatory and oxidative stress processes in patients with depression, although the magnitude of biomarkers measured here does not depend of the phase of the disease Table 5.
There are no studies which have compared the biomarkers we have used between both depression groups and therefore we cannot compare our results with the reports of other researchers. However, referring to the work by Sarapas et al. [22] we shall use two expressions in this place – the so-called state effects and trait-like relationship. According to the first hypothesis, an increase of inflammation factors observed during an episode of depression is only a transient condition, which disappears in the period of disease remission. Based on the second hypothesis, increased pro-inflammatory and anti-inflammatory activation is a permanent feature accompanying patients who suffer from depression. The present results show that alterations in the enzymes measured here are trait markers, whereas previous research showed that increases in TNF-α and neopterin should be regarded as staging markers [10]. In any case, it seems justified to conclude that some activated immune-inflammatory and oxidative stress pathways may be considered as endophenotypic trait biomarkers of depression, whereas other assays are biomarkers of staging of depression.
In the examined group, there were no significant relationships between the severity of depressive disorders measured before and after pharmacological treatment and the expression of mRNA and protein levels of the enzymes. Moreover, the relationship between rDD level and MPO concentration in blood serum was not confirmed by Vaccarino et al. [23]. Meanwhile, in the experiments conducted by Sarandol et al. [24], a raised level of SOD-2 in the group of patients with the so-called major depressive disorder positively correlated with the intensity of symptoms of depressive disorders. Similar conclusions were drawn from the work by Su et al. [25], who evaluated the concentration of inflammatory markers such as IL-6 and C-reactive protein. Additionally, it was demonstrated that increased concentration of IL-2 correlated with the risk of an attempted suicide [26].
Antidepressant treatments may reduce oxidative stress [27-29]. However, Gałecki et al. [30] did not find a change in the concentration of antioxidative enzymes (catalase and zinc superoxide dismutase) after 3 months fluoxetine pharmacotherapy in patients with rDD (n = 50). The concentration of the said compounds – both before onset of the treatment and after observing a symptomatic improvement in the examined group of patients with rDD – was higher than in healthy individuals. In another paper [31], a desired outcome (concentration reduction of catalase and zinc superoxide dismutase in serum) was possible after combining fluoxetine-based pharmacotherapy with acetylsalicylic acid (non-steroid anti-inflammatory drug). Similar results were recorded by Whittle et al. [32] in an experiment based on an animal model.
In summary, it is possible to confirm the necessity for further research studies as regards the presented issues and mutual interrelations between inflammatory processes and emotional and cognitive signs of depression.
Conclusions
There is no significant difference in MnSOD, MPO, COX-2 and i-NOS between patients with recurrent depressive disorders and those in a first episode of depression. These findings suggest that these enzymes are trait markers of depression and are not related to staging of depression.
Abbreviations
- CIDI:
-
Composite international diagnostic interview
- COX-2:
-
Cyclooxygenase-2
- ED-I:
-
First episode of depression
- HDRS:
-
Hamilton depression rating scale
- IFN-gamma:
-
Interferon-gamma
- IL:
-
Interleukins
- iNOS, NOS-2:
-
Inducible nitric oxide synthase
- MNSOD, SOD2:
-
Manganese superoxide dismutase
- MPO:
-
Myeloperoxidase
- rDD:
-
Recurrent depressive disorder
- TNF-α:
-
Tumor necrosis factor-alpha
References
Reynolds 3rd CF, Cuijpers P, Patel V, Cohen A, Dias A, Chowdhary N, et al. Early intervention to reduce the global health and economic burden of major depression in older adults. Annu Rev Public Health. 2012;33:123–35.
Rodgers M, Asaria M, Walker S, McMillan D, Lucock M, Harden M, et al. The clinical effectiveness and cost-effectiveness of low-intensity psychological interventions for the secondary prevention of relapse after depression: a systematic review. Health Technol Assess. 2012;16(28):1–130.
Mead GE, Morley W, Campbell P, Greig CA, McMurdo M, Lawlor DA. Exercise for depression. Cochrane Database Syst Rev. 2008;4, CD004366.
Richardson R, Richards DA, Barkham M. Self-help books for people with depression: a scoping review. J Ment Health. 2008;17:543–52.
Smith RS. The macrophage theory of depression. Med Hypotheses. 1991;35:298–306.
Schiepers OJ, Wichers MC, Maes M. Cytokines and major depression. Prog Neuropsychopharmacol Biol Psychiatry. 2005;29(2):201–17.
Maes M, Berk M, Goehler L, Song C, Anderson G, Gałecki P, et al. Depression and sickness behavior are Janus-faced responses to shared inflammatory pathways. BMC Med. 2012;10:66.
Maes M. The cytokine hypothesis of depression: inflammation, oxidative & nitrosative stress (IO&NS) and leaky gut as new targets for adjunctive treatments in depression. Neuro Endocrinol Lett. 2008;29(3):287–91.
Schmidt FM, Lichtblau N, Minkwitz J, Chittka T, Thormann J, Kirkby KC, et al. Cytokine levels in depressed and non-depressed subjects, and masking effects of obesity. J Psychiatr Res. 2014;55:29–34.
Maes M, Mihaylova I, Kubera M, Ringel K. Activation of cell-mediated immunity in depression: association with inflammation, melancholia, clinical staging and the fatigue and somatic symptom cluster of depression. Prog Neuropsychopharmacol Biol Psychiatry. 2012;36(1):169–75.
Aktan F. iNOS-mediated nitric oxide production and its regulation. Life Sci. 2004;75:639–53.
Valko M, Leibfritz D, Moncol J, Cronin MT, Mazur M, Telser J. Free radicals and antioxidants in normal physiological functions and human disease. Int J Biochem Cell Biol. 2007;39(1):44–84.
The ICD-10 Classification of Mental and Behavioural Disorders. Diagnostic criteria for research. Geneva: World Health Organization; 1992.
Patten S. Performance of the composite international diagnostic interview short form for major depression in community and clinical samples. Chronic Dis Canada. 1997;18(3):18–24.
Hamilton M. A rating scale for depression. J Neurol Neurosurg Psychiatry. 1960;23:56–62.
Demyttenaere K, De Fruyt J. Getting what you ask for: on the selectivity of depression rating scales. Psychother Psychosom. 2003;72:61–70.
Gałecki P, Talarowska M, Bobińska K, Szemraj J. COX-2 gene expression is correlated with cognitive function in recurrent depressive disorder. Psychiatry Res. 2014;215(2):488–90.
Kowalczyk M, Talarowska M, Zajączkowska M, Szemraj J, Gałecki P. iNOS gene expression correlates with cognitive impairment. Med Sci Tech. 2013;54:16–21.
Talarowska M, Orzechowska A, Szemraj J, Kuan-Pin S, Maes M, Gałecki P. Manganese superoxide dismutase gene expression and cognitive functions in recurrent depressive disorder. Neuropsychobiology. 2014;70(1):23–8.
Talarowska M, Szemraj J, Gałecki P. Myeloperoxidase gene expression and cognitive functions in depression. Adv Med Sci. 2014;60(1):1–5.
Kirkwood BR, Sterne JAC. Essential Medical Statistics. 2nd ed. New Jersey: Blackwell Publishing; 2003.
Sarapas C, Shankman SA, Harrow M, Goldberg JF. Parsing trait and state effects of depression severity on neurocognition: evidence from a 26-year longitudinal study. J Abnorm Psychol. 2012;121(4):830–7.
Vaccarino V, Brennan ML, Miller AH, Bremner JD, Ritchie JC, Lindau F, et al. Association of major depressive disorder with serum myeloperoxidase and other markers of inflammation: a twin study. Biol Psychiatry. 2008;64:476–83.
Sarandol A, Sarandol E, Eker SS, Erdinc S, Vatansever E, Kirli S. Major depressive disorder is accompanied with oxidative stress: short-term antidepressant treatment does not alter oxidative-antioxidative systems. Hum Psychopharmacol. 2007;22:67–73.
Su S, Miller AH, Snieder H, Bremner JD, Ritchie J, Maisano C, et al. Common genetic contributions to depressive symptoms and inflammatory markers in middle-aged men: the Twins Heart Study. Psychosom Med. 2009;71(2):152–8.
Penttinen J. Hypothesis: low serum cholesterol, suicide, and interleukin-2. Am J Epidemiol. 1995;141:716–8.
Behr GA, Moreira JC, Frey BN. Preclinical and clinical evidence of antioxidant effects of antidepressant agents: implications for the pathophysiology of major depressive disorder. Oxid Med Cell Longev. 2012;2012:609421.
Bilici M, Efe H, Koroglu A, Uydu HA, Bekaroglu M, Deger O. Antioxidative enzyme activities and lipid peroxidation in major depression: alterations by antidepressant treatments. Affect Disord. 2001;64:43–51.
Khanzode SD, Dakhale GN, Khanzode SS, Saoji A, Palasodkar R. Oxidative damage and major depression: the potential antioxidant action of selective serotonin-re-uptake inhibitors. Redox Rep. 2003;8(6):365–70.
Gałecki P, Szemraj J, Bieńkiewicz M, Florkowski A, Gałecka E. Lipid peroxidation and antioxidant protection in patients during acute depressive episodes and in remission after fluoxetine treatment. Pharmacol Rep. 2009;61(3):436–47.
Gałecki P, Szemraj J, Bieńkiewicz M, Zboralski K, Gałecka E. Oxidative stress parameters after combined fluoxetine and acetylsalicylic acid therapy in depressive patients. Hum Psychopharmacol. 2009;24(4):277–86.
Whittle N, Li L, Chen WQ, Yang JW, Sartori SB, Lubec G, et al. Changes in brain protein expression are linked to magnesium restriction-induced depression-like behavior. Amino Acids. 2011;40(4):1231–48.
Müller GJ, Lassmann H, Johansen F. Anti-apoptotic signaling and failure of apoptosis in the ischemic rat hippocampus. Neurobiol Dis. 2007;25:582–93.
Radenović L, Selaković V, Kartelija G. Mitochondrial superoxide production and MnSOD activity after exposure to agonist and antagonists of ionotropic glutamate receptors in hippocampus. Ann N Y Acad Sci. 2005;1048:363–5.
Gałecki P, Florkowski A, Bobińska K, Śmigielski J, Bieńkiewicz M, Szemraj J. Functional polymorphismof the myeloperoxidase gene (G-463A) in depressive patients. Acta Neuropsychiatr. 2010;5:218–22.
Hansson M, Olsson I, Nauseef WM. Biosynthesis, processing, and sorting of human myeloperoxidase. Arch Biochem Biophys. 2006;445:214–24.
Winterbourn CC. Biological reactivity and biomarkers of the neutrophil oxidant, hypochlorous acid. Toxicol. 2002;181–182:223–7.
Madrigal JL, Moro MA, Lizasoain I, Lorenzo P, Fernández AP, Rodrigo J, et al. Induction of cyclooxygenase-2 accounts for restraint stress-induced oxidative status in rat brain. Neuropsychopharmacology. 2003;28:1579–88.
Casolini P, Catalani A, Zuena AR, Angelucci L. Inhibition of COX-2 reduces the age-dependent increase of hippocampal inflammatory markers, corticosterone secretion, and behavioral impairments in the rat. J Neurosci Res. 2002;68:337–43.
Feil R, Kleppisch T. NO/cGMP-dependent modulation of synaptic transmission. Handb Exp Pharmacol. 2008;184:529–60.
Ankarali S, Ankarali HC, Marangoz C. Further evidence for the role of nitric oxide in maternal aggression: effects of L-NAME on maternal aggression towards female intruders in Wistar rats. Physiol Res. 2009;58(4):591–8.
Calabrese V, Mancuso C, Calvani M, Rizzarelli E, Butterfield DA, Stella AM. Nitric oxide in the central nervous system: neuroprotection versus neurotoxicity. Nat Rev Neurosci. 2007;8:766–75.
Acknowledgements
Monika Talarowska - this study was supported with scientific research grants from the National Science Centre, no. 2011/01/D/HS6/05484 (in the collection of data).
Piotr Gałecki - this study was supported with scientific research grants from the National Science Centre, no. 2012/05/B/NZ5/01452 (in the linguistic revision).
Author information
Authors and Affiliations
Corresponding author
Additional information
Competing interests
The authors declare that they have no competing interests.
Authors’ contributions
MT has made a substantial contribution to the conception design, analysis and interpretation of the data. She has made a substantial contribution to the drafting the manuscript and has given final approval of the version of the article to be published and can certify that no other individuals not listed as authors have made substantial contributions to the paper. She has written the first draft of the article. She has also made a statistical analysis and she has made a substantial contribution to the acquisition of data. PG has made a substantial contribution to the conception design interpretation of the data. MB has made a substantial contribution to drafting the article and reviewing it critically. MM has made a substantial contribution to drafting the article and reviewing it critically. JS has made a substantial contribution to the acquisition of data and has given final approval of the version of the article to be published and can certify that no other individuals not listed as authors have made substantial contributions to the paper. All authors read and approved the final manuscript.
Rights and permissions
This article is published under an open access license. Please check the 'Copyright Information' section either on this page or in the PDF for details of this license and what re-use is permitted. If your intended use exceeds what is permitted by the license or if you are unable to locate the licence and re-use information, please contact the Rights and Permissions team.
About this article
Cite this article
Talarowska, M., Szemraj, J., Berk, M. et al. Oxidant/antioxidant imbalance is an inherent feature of depression. BMC Psychiatry 15, 71 (2015). https://doi.org/10.1186/s12888-015-0454-5
Received:
Accepted:
Published:
DOI: https://doi.org/10.1186/s12888-015-0454-5