Thiol/Disulfide Homeostasis in Bipolar and Unipolar Depression.

OBJECTIVE: Bipolar disorder and unipolar depressive disorder are complex phenotypes. There appear to be phenotypical, mechanistic, and therapeutic differences between bipolar depression (BD) and unipolar depression (UD). There is a need for understanding the underlying biological variation between these clinical entities. The role of oxidative processes underlying bipolar disorder and depression has been demonstrated. Thiol-disulfide homeostasis (TDH) is a recent oxidative stress marker. In this study, we aimed to inspect patients with bipolar depression and unipolar depression in terms of thiol-disulfide balance and to compare them with healthy controls.
METHODS: Patients admitted to the outpatient clinic of Ankara Numune Training and Research Hospital and diagnosed either as a depressive episode with bipolar disorder (n = 37) or unipolar depression (n = 24) according to DSM-5 criteria, along with healthy controls (HC) (n = 50), were included in the study. Native thiol, total thiol, and disulfide levels were compared across the groups.
RESULTS: In comparison to HC, both BD and UD groups had higher disulfide levels, disulfide/native thiol ratio, and disulfide/total thiol ratio. No significant differences between BD and UD were detected in terms of disulfide level, disulfide/ native thiol ratio, and disulfide/total thiol ratio.
CONCLUSION: Increased levels of disulfide, native thiol, and disulfide/total thiol ratios compared to healthy controls in both UD and BD groups may be indicative of the presence of oxidative damage in these two clinical conditions. To clarify the role of oxidative stress in the pathophysiology of depressive disorders and investigate TDH, longitudinal studies in patients with medication-free UD and BD are required.

INTRODUCTION

Bipolar disorder and unipolar depression (UD) cause impairments in functioning and health-related quality of life [1,2]. Mood disorders have an array of active constituents such as neurotransmission and immune dysfunction, chronobiology and mitochondrial dysfunction [3]. Recent studies on the inflammatory and oxidative processes have accelerated the understanding of the pathophysiology of mental disorders [4,5]. There is a fast-growing set of evidence suggesting that oxidative stress is involved in the pathophysiology of UD and bipolar disorder [6,7].

Excessive production of free radicals (reactive oxygen species) play an important role in the promotion of permanent degradation of equilibrium among antioxidants in cell and prooxidant processes, in oxidative stress. Free radicals cause damage to proteins, lipids and deoxyribonucleic acid (DNA) in the cell, triggering apoptosis and cell death [8]. Mental disorders, including UD, bipolar disorder, and schizophrenia are affected by oxidative stress through this mechanism [9-11].

There are different methods for evaluating oxidative processes. One of them is thiol/disulfide homeostasis (TDH) [12]. Thiols contain a sulfhydryl group (-SH) that is composed of hydrogen and sulfur atoms attached to a carbon atom. Thiols can respond to free radicals for protecting tissues and cells from the damage caused by organic compounds containing reactive oxygen products [13]. A problem in this homeostasis results in a variety of disorders, as the ratio of thiol disulfide plays a critical role in antioxidant protection, detoxification, and signal transduction, regulation of enzymatic activity, apoptosis and cellular signaling mechanisms [14,15].

As a result, thiol/disulfide balance may provide information about the oxidative processes in the human body. The direction of the distortion in this balance may be a sign of oxidative status [16]. Examining dynamic TDH can provide significant insight into diverse biochemical processes, either normal or abnormal [17]. In this regard, the abnormal state of TDH may affect the pathogenesis of several clinical conditions, such as schizophrenia, neurodegenerative disorders, and bipolar disorder [18-22].

In the light of the findings from previous studies investigating TDH in mental disorders, we investigated whether TDH might be helpful in explaining underlying biological differences such as oxidative processes in UD and bipolar depression (BD).

METHODS

In this study, the participants were 61 patients diagnosed with BD (n = 37) and UD (n = 24) according to Diagnostic and Statistical Manual of Mental Disorders, fifth edition, and 50 healthy controls (HC) with no psychiatric and neurologic disorder. Patients with bipolar disorder depressive episode (BD) and unipolar depressive disorder (UD) were diagnosed by two experienced psychiatrists. The participants were evaluated using the Turkish versions of the Hamilton Depression Rating Scale [23-25] and the Young Mania Rating Scale [26,27]. The age range for the inclusion of the participants was 18−65 years old.

Effect size from our previous study [18] between patient and control was 0.56 for disulfide/native thiol ratio. A power analysis revealed that in order for d = 0.56 effect size of disulfide/native thio to be detected (80% power) as significant at the 5% level, a sample of 50 participants would be required for patient and control group comparison. The exclusion criteria were: having an anti-inflammatory treatment, pregnancy, mental retardation, alcohol or drug dependence, neurological illness, any systematic or metabolic disease that may influence oxidative marker concentrations.

The Ethics Committee of Ankara Numune Training and Research Hospital approved the study (Date: 2018, Number: E-18-2244). A written consent from all participants was obtained before the study.

Biochemical Tests

Blood samples were collected in plain tubes after an overnight fasting. Venous blood (5 ml) was collected from each participant. Serum samples were separated after centrifugation at 1,300 g for 10 minutes and stored at −80°C until TDH tests were performed. The automatic and spectrophotometric method developed by Erel and Neselioglu [12] were used to measure thiol/disulfide homeostasis. The mechanism of the method works as such; dynamic and reducible disulfide bonds in the samples were reduced to free functional thiol groups by using sodium borohydride (NaHB4). NaBH4 was removed with formaldehyde to prevent the reduction of unused reduced sodium borohydride to dithionite-2 nitrobenzoic (DTNB). Levels of Native thiol (SH), total thiol (ToSH), disulfide (SS) were measured. Native thiol and total thiol levels were determined after reaction with DTNB and their levels were measured ultimately. Disulfide bonds in the sample were calculated using the following equation: (total thiol−native thiol)/2. %CV values are 4%, 5%, and 13% for concentrations of 29.1, 16.0, and 7.15 mmol/L, respectively. Detection limit of measurement was 2.8−4,000 mmol/L.

Statistical Analysis

In this study, we tested the normal distribution condition using the Shapiro−Wilk test. Normally distributed data were reported as means with standard deviation, and compared with the two-sample ttest and one-way analysis of variance. Non-normally distributed data were reported as medians with minimum and maximum values, and compared using the Mann−Whitney Uand Kruskal−Wallis tests. In the case of pairwise comparison, the significance levels were adjusted using the Bonferroni method. Pearson’s chi-squared test and Fisher-Freeman- Halton tests were used to compare categorical variables. Correlations between variables were tested using the Pearson and Spearman correlation tests. The significance level was set at p < 0.05. Statistical analyses were performed with IBM SPSS ver. 23.0 (IBM Corp. Released 2015. IBM SPSS Statistics for Windows, Version 23.0; IBM Corp., Armonk, NY, USA).

RESULTS

In this study, there were no significant differences in terms of age and sex between all three groups. The socio-demographic characteristics of the sample are reported in Table 1. Of the BD group, 70% were on valproic acid/sodium valproate, 14% were on lithium, 5% were on carbamazepine, and 11% were not on any mood stabilizer treatment. While 78% of the BD group were on second generation and 3% were on first generation antipsychotic treatment, 19% of them were not prescribed with any antipsychotic treatment. Of the BD group, 19% were using antidepressant treatment. Of the UD group, 29% were on sertraline, 12.5% were on escitalopram, 33.3% were on fluoxetine, 17% were on venlafaxine, and 8.2% were on duloxetine.

Table 1

Evaluation of socio-demographic characteristics

Variable	Bipolar depression (n = 37)	Unipolar depression (n = 24)	Control (n = 50)	pvalue
Sex, female/male	23 (62.2)/14 (37.8)	15 (62.5)/9 (37.5)	30 (60)/20 (40)	0.970a
Age (yr)	38.4 ± 10.7	40.6 ± 14.1	37.2 ± 9.8	0.485b
Marital status				0.703c
Single	16 (43.2)	10 (41.7)	0 (0)
Married	21 (56.8)	13 (54.2)	50 (100)
Divorced	0 (0)	1 (4.2)	0 (0)
Age at disease onset (yr)	27.5 ± 10.2	36.1 ± 12.8	-	0.005e
Smoking (packet-yr)	0 (0−30)	0 (0−25)	-	0.315d
Duration of disease (yr)	8 (3−25)	2 (1−15)	-	< 0.001d
Number of hospitalizations	2 (0−8)	0 (0−2)	-	< 0.001d
Number of previous manic episodes	2 (0−6)	-	-	-
Number of depressive episodes	1 (0−4)	2 (1−4)	-	0.094d
Young mania rating scale score	3.2 ± 1.2	-	-	-
Hamilton depression scale score	28.8 ± 7.3	28.7 ± 4.9	-	0.722c

Descriptive statistics were presented as number (%), mean ± standard deviation or median (minimum−maximum) for continuous variables.

Pearson chi-square test. bOne-way ANOVA (analysis of variance). cFisher-Freeman-Halton test. dMann−Whitney Utest. eIndependent samples ttest. The significance level was set at p < 0.05.

There were differences in SS, SS/SH, SS/ToSH between the BD and the control group, and between the UD and the control group. SS, SS/SH, SS/ToSH were higher in patients with BD and in patients with UD than in the control group (Table 2).

Table 2

Levels of native thiol, total thiol, disulfide, disulfide/native thiol, disulfide/total thiol, and native/total thiol according to groups

Variable	Bipolar depression	Unipolar depression	Control	pvalue	Pairwise comparison
Native thiol (SH)	310.6 ± 51.6	327.3 ± 53.3	344.4 ± 49.5	0.011a	BD vs. UD, p = 0.518
					BD vs. C, p = 0.009
					UD vs. C, p = 0.447
Total thiol (ToSH)	358.0 ± 53.5	377.9 ± 54.7	383.8 ± 52.1	0.081a	-
Disulfide (SS)	22.15 (12.35−49.3)	25.95 (17.65−33)	19.23 (12.55−31.35)	< 0.001b	BD vs. UD, p = 0.132
					BD vs. C, p = 0.015
					UD vs. C, p < 0.001
Disulfide/native thiol (SS/SH)	6.64 (4.38−28.97)	7.91 (5.3−12.32)	5.72 (3.71−8.26)	< 0.001b	BD vs. UD, p = 0.494
					BD vs. C, p = 0.001
					UD vs. C, p < 0.001
Disulfide/total thiol (SS/ToSH)	5.86 (4.03−18.34)	6.83 (4.8−9.89)	5.13 (3.46−7.09)	< 0.001b	BD vs. UD, p = 0.491
					BD vs. C, p = 0.001
					UD vs. C, p < 0.001
Native thiol/total thiol (SH/ToSH)	88.28 (63.32−91.94)	86.35 (80.23−90.41)	89.74 (85.83−93.09)	< 0.001b	BD vs. UD, p = 0.489
					BD vs. C, p < 0.001
					UD vs. C, p = 0.001

Descriptive statistics were presented as mean ± standard deviation or median (minimum−maximum) for continuous variables.

BD, bipolar depression; UD, unipolar depression; C, control.

ANOVA (analysis of variance). bKruskal−Wallis test. Bonferroni correction was used for pairwise comparisons. The significance level was set at p < 0.05.

The HAM-D scores were positively correlated with SS concentrations (r = 0.341, p = 0.007), SS/SH ratio (r = 0.505, p < 0.001), and SS/ToSH ratio (r = 0.513, p < 0.001) in BD group. There was no statistically significant correlation between TDH parameters and the HAM-D scores in UD group (data not shown). In both groups, there was no statistically significant correlation of TDH parameters with duration of illness or number of past episodes (data not shown).

DISCUSSION

TDH as an antioxidant parameter has been previously investigated in a variety of clinical conditions, such as schizophrenia, bipolar disorder in manic episode and remission, major depressive disorder, general anxiety disorder [18,21,22,28,29]. To the best of our knowledge, this is the first study investigating dynamic TDH in bipolar disorder patients with depressive episodes.

Our findings showing higher SS, SS/SH, SS/ToSH in both BD and UD than in controls are in line with the previous meta-analysis that has reported decreased antioxidants and antioxidant enzymes in unipolar depression, and increased oxidative stress in both UD and BD [6,30,31]. However, we found no evidence for TDH differences between BD and UD.

In patients with UD and BD, depressive episodes often relapse. In a recent study, SH and ToSH levels were lower in first episode major depressive patients than in healthy controls [32]. There are also studies reporting that levels of lipid peroxidation products such as malondialdehyde (MDA), are higher in patients with recurrent depression compared to patients with single episode [33]. In the light of these findings, it can be speculated that oxidative damage may be observed even in the first episode and may indicate that the oxidative damage could increase in recurring episodes. In our study, however, we did not observe an association of TDH with the duration of illness or the number of past depressive episodes.

In a study conducted in untreated female patients with major depressive disorder; serum SS level was lower in patients compared with controls, while serum SH level was higher in the patient group than in the control group [29]. This was considered to be the result of an anti-oxidative compensation mechanism [29].

Our findings revealed positive correlations between oxidative stress markers (SS, SS/SH, SS/ToSH) and the HAM-D scores in BD. A recent study showed that SH and ToSH levels were negatively correlated with PANSS scores in untreated patients with schizophrenia [21]. In a previous study conducted in female patients with untreated major depressive disorder, a negative correlation was found between plasma SS/ToSH ratio and HAM-D score, which was explained with the anti-oxidative compensation mechanism [29]. Our study indicates that the increase in SS, SS/SH, SS/ToSH levels may be related to disease severity. Future studies are needed to understand whether these markers serve as determinants of disease severity over the course of illness progression.

Antipsychotics, mood stabilizers, and antidepressants can also affect the oxidation process. A recent study examining the level of thiol-disulfide in patients with schizophrenia patients shows that the oxidative processes are influenced by atypical antipsychotic treatment [34]. Mood stabilizer drugs may reduce the level of lipid peroxidation [35]. In the literature, it was also argued that atypical antipsychotic drugs might affect oxidative status by increasing the antioxidant levels and decreasing the oxidative stress [36-39]. A recent study showed that compared to controls, SH and ToSH levels were higher in patients with schizophrenia, who were on atypical antipsychotic drugs [34]. In our study, although the majority of the patients with BD were using antipsychotics, there was a shift toward the oxidative stress in the TDH in these patients.

The other studies showed that MDA levels returned to normal levels after antidepressant treatment in patients with depression [40,41]. Despite the use of antidepressants in patients with UD in our study, there was a shift toward the oxidative direction in TDH. The recent meta-analysis shows that following an antidepressant medication, the antioxidant levels increase, while the oxidative damage product levels decrease [42].

Previously, we showed that the native thiol and total thiol levels were lower in patients with mania compared to those in remission and controls; and speculated that this might be related to malnutrition during manic episodes [18]. There were not any significant differences between the bipolar mania, remission and control groups in terms of their disulfide level in our previous study. In this study, however, disulfide level is higher in UD and BD groups than the control group and disulfide level in BD group also correlated with HAM-D score. This might be an indicator of oxidative stress in depression.

Limitations

Although TDH has been previously investigated in depression, this is the first study to investigate TDH homeostasis in bipolar depression. Therefore, our findings from the current exploratory analysis require further confirmation in future studies. There are several limitations that should be considered when interpreting the results. The sample size was relatively small. In particular, the low number of UD and BD participants may be insufficient to detect small effect-size differences in TDH homeostasis between UD and BD.

We could not evaluate the effects of the drugs on the patients since all patients were on treatment in our study. Also, the patients did not have a homogeneous distribution in terms of the medication categories. Another limitation of our study was the failure to eliminate other potential factors that might influence oxidative stress, such as obesity, life-style, and smoking. However, the high prevalence rates of smoking in the general population in Turkey might have mitigated the confounding effects of this limitation. Further, there was no difference in smoking frequencies (packet per year) between UD and BD patients.

Conclusion

Our findings suggest that there might be an increase in oxidative stress in patients with bipolar and unipolar depression patients compared with that in healthy controls. We found no difference in thiol/disulfide balance between BD and UD, which may imply that there is a common oxidative damage in both disorders. In the future, longitudinal studies with larger sample sizes with medication-free patients are required to understand the role of TDH homeostasis in depressive disorders.