After correcting for confounders, significant positive associations between BDNF and most symptom clusters; depression, somatization, interpersonal sensitivity, anxiety, phobic anxiety, and psychoticism, as well as a Global severity Index were found in the subgroup of patient not using psychotropic medication. For the patient group taking psychotropic medication a positive association between BDNF and symptom clusters was seen only for the paranoid ideation cluster. Regarding hs-CRP we did not find any association with symptom clusters in any of the groups.
BDNF is suggested as a biomarker in mental disorders [13]. For the unmedicated patient group we found a positive association between level of BDNF and intensity of symptoms in several SCL-90 clusters. In line with our findings a recent study reported higher levels of BDNF in bipolar disorder, where higher levels of BDNF were associated with longer illness duration [14]. Some studies found significant relation of BDNF with negative symptoms in schizophrenia and it has been suggested that the increased level of BDNF represents a compensatory response to the underlying neuropathology in the brain regions implicated [15]. Our findings also are in keeping with the findings of Kheirouri et al [16] in patients with major depressive disorder (MDD).
However, most previous studies report a negative association between mental suffering and level of BDNF. This negative association is reported to reverse with successful treatment [2]. Our findings of significant positive associations between BDNF and most symptom clusters in non-medicated patients including depression, somatization, anxiety and psychoticism may be explained through the involvement of BDNF in the hypothalamic-pituitary-adrenal (HPA) axis in depression: The psychological stress of depression, causes an upregulated level of BDNF that in turn causes an increase in corticotrophin-releasing hormone leading to glucocorticoid release [16]. The findings need to be repeated.
Reasons why we did not see the pattern with inverse association between psychiatric symptoms and BDNF that has been reported in many other studies, may be related to our patient population and the assessment and sampling one week after admittance. At the time of assessment patients are expected to be improving from their mental suffering. One explanation may be that the body and brain conduct self-repair and compensates by upregulating BDNF. The group of patients using psychotropic medication did not show this upregulation despite the same symptom burden as reported by SCL-90-R.
We did not find any significant association between symptom clusters and hs-CRP when adjusted for confounding factors. Other studies have found that hs-CRP is related to severity of depressive symptoms [17]. Increased hs-CRP has been reported in patients with fibromyalgia and chronic fatigue syndrome [10] as well as in depression and anxiety [18]. We do not have a group of healthy controls and thus cannot claim that our patients actually have increased hs-CRP, but a mean level 2.7 still represent moderately increased risk of cardiovascular disease (low risk cut off < 1 mg/L).
Overall, we could not reproduce the findings from other studies in hs-CRP, and the findings on BDNF may seem in conflict with previous reports. Factors contributing to inconsistency in this field may be variations in methodology, symptom severity, medication, measure used to diagnose and size and ethnicity of the sample [19]. Previous studies have demonstrated associations between serum BDNF and lifestyle factors as smoking, BMI and physical activity [20], as well use of psychotropic medication [2]. It is also known that age and gender can affect the BDNF level. A higher BDNF serum level is associated with increasing age, residence in high degree of urbancy and smoking [19].
There are several limitations to the study. Information on symptoms, smoking, weight and height in our study were obtained from the self-report questionnaire with a risk of biased reporting. The sample size is small, especially regarding the subgroup with no use of psychotropic medication. However, other similar studies published in this field report smaller numbers (n < 100) [13], [16], [19]. Our aim was to search for association between BDNF and mental suffering in the two groups; with or without psychotropic medication. We did not study BDNF in relation to diagnoses or symptoms compared to a healthy control group, and this is a main limitation. However, we are still able to compare general mental suffering with BDNF and hsCRP adjusting for the known confounding factors. We do not use psychiatric diagnostic groups in this study, thus we cannot relate the findings directly to other studies based on diagnostic groups. Also, this is a cross sectional natural study. Patients were not randomised to either medication or non-medication. Furthermore, as mentioned they were not acutely ill. One main originality of our study is the focus on symptoms and symptom clusters rather than diagnostic groups. Another original factor in our study is that the data were sampled roughly 7 days after admittance to reduce potential stress achieved by the admittance itself for the patients and thereby to reduce any possible stress-induced alterations in the biological markers. During these 7 days patients will also have been exposed to care, safety, professional milieu therapy, psychotherapy, often improved sleep and nutrition. All of which could contribute to reduce the possible stress of admittance to the inpatient setting. Also, the focus on a general open ward inpatient group may add information to the field regarding effect of different degrees of illness compared to patient groups in other studies.
There also are several general strengths. We adjusted for smoking, weight and height as well as use of psychotropic medication. Regarding biological measures, serum was sampled after rest and fasting in the morning to avoid effects of diurnal variation. As serum BDNF levels have been shown to be significantly lower if blood is drawn in the afternoon and diurnal variations of BDNF plasma levels are known [20] we sampled sera fasting in the morning, and without previous exercise. Furthermore, the laboratory used a standardized protocol for analysis and with an experienced technician performing the analysis.