Hostname: page-component-cd9895bd7-gxg78 Total loading time: 0 Render date: 2024-12-22T21:01:46.710Z Has data issue: false hasContentIssue false

Association of CACNA1C polymorphisms with serum BDNF levels in bipolar disorder

Published online by Cambridge University Press:  18 July 2019

Erik Smedler*
Affiliation:
Postdoctoral Fellow, Section of Psychiatry and Neurochemistry, Sahlgrenska Academy at Gothenburg University, Sweden
Erik Pålsson
Affiliation:
Associate Professor, Section of Psychiatry and Neurochemistry, Sahlgrenska Academy at Gothenburg University, Sweden
Kenji Hashimoto
Affiliation:
Professor, Division of Clinical Neuroscience, Chiba University Center for Forensic Mental Health, Japan
Mikael Landén
Affiliation:
Professor, Section of Psychiatry and Neurochemistry, Sahlgrenska Academy at Gothenburg University; and Department of Medical Epidemiology and Biostatistics, Karolinska Institutet, Sweden.
*
Correspondence: Erik Smedler, Blå Stråket 15, Sahlgrenska Universitetssjukhuset, 41345Göteborg, Sweden. Email erik.smedler@gu.se
Rights & Permissions [Opens in a new window]

Abstract

Variation in the CACNA1C gene has been associated with bipolar disorder in several genome-wide association studies. This gene encodes the alpha 1C subunit of L-type voltage-gated calcium channels, which play an essential role in neurons. We analysed 39 biomarkers in either cerebrospinal fluid or serum in relation to six different CACNA1C variants in 282 patients with bipolar disorder and 90 controls. We report associations of CACNA1C risk alleles with serum levels of BDNF as well as tissue plasminogen activator, which converts pro-BDNF to mature BDNF. This sheds light on links between CACNA1C genetic variants and pathophysiological mechanisms in bipolar disorder.

Type
Short report
Copyright
Copyright © The Royal College of Psychiatrists 2019

Bipolar disorder is a serious mental disorder, characterised by recurrent episodes of depression and mania, with a lifetime risk around 1%. The pathoaetiology has not been clarified but heritability estimates of up to 90% signify the importance of genetic factors. Commonly occurring single-nucleotide polymorphisms (SNPs) in the CACNA1C gene have been associated with bipolar disorder in several genome-wide association studies.1 CACNA1C encodes the alpha 1C subunit of Lc-type voltage-gated calcium (Ca2+) channels, which lead to an influx of extracellular Ca2+ into a cell upon depolarisation. There are several common variants in the CACNA1C gene, but the strongest association with bipolar disorder has been seen for the SNP rs1006737 in the third intron.Reference Ferreira, O'Donovan, Meng, Jones, Ruderfer and Jones2 Genetic association results need to be explored by studying allelic variation in relation to biomarkers and clinical phenotypes. Risk-associated CACNA1C SNPs predicted higher scores on depression and anxiety questionnaires in healthy individuals,Reference Erk, Meyer-Lindenberg, Schnell, von Boberfeld C, Esslinger and Kirsch3,Reference Roussos, Giakoumaki, Georgakopoulos, Robakis and Bitsios4 and decreased the hyperphosphorylated tau/total tau ratio in cerebral spinal fluid (CSF) from patients with bipolar disorder.Reference Jakobsson, Palsson, Sellgren, Rydberg, Ekman and Zetterberg5

Here, we investigate associations between CACNA1C polymorphisms and CSF or serum biomarkers in patients with bipolar disorder and controls. We report that CACNA1C polymorphisms are associated with serum levels of brain-derived neurotrophic factor (BDNF) and the enzyme converting pro-BDNF to mature BDNF, tissue plasminogen activator (tPA).

Method

The sample includes 282 patients with bipolar disorder and 90 healthy controls (see Supplementary Table 1 available at https://doi.org/10.1192/bjp.2017.173 for details). Patients and controls were recruited from the St. Göran Bipolar Project, enrolling patients from the bipolar unit at the Northern Stockholm Psychiatric Clinic, Stockholm, Sweden.Reference Rolstad, Jakobsson, Sellgren, Ekman, Blennow and Zetterberg6 The study was approved by the Regional Ethics Committee in Stockholm (approval number Dnr 2005/554-31/3) and conducted in accordance with the Helsinki Protocol. After a complete description of the study, all enrolled patients and controls consented orally and in writing to participate in the study. In brief, the Swedish version of the Affective Disorder EvaluationReference Sachs, Thase, Otto, Bauer, Miklowitz and Wisniewski7 was the key clinical assessment method. Bipolar diagnoses were made according to DSM-IV criteria as per the Structured Clinical Interview for DSM-IV.Reference Kübler, Gellman and Turner8

Participants were subjected to serum and CSF sampling. Lumbar puncture and serum sampling was performed on the same occasion when patients were in a stable mood phase, as described previously.Reference Jakobsson, Palsson, Sellgren, Rydberg, Ekman and Zetterberg5 Assessment of depressive and manic symptoms are presented in Supplementary Table 7. Participants were genotyped for selected SNPs with KASP technology for Mac OS X (KBioscience, Hoddesdon, UK; see https://www.biosearchtech.com/products/pcr-kits-and-reagents/genotyping-assays/kasp-genotyping-chemistry). MATLAB (Mathworks version R2017b) and SPSS (IBM version 24), both for Mac OS X, were used for statistical calculations. The false discovery rate with threshold 0.1 was used to correct for multiple comparisons.

In total, 39 molecular species (including ratios) were measured from either CSF or serum, using a variety of analytic methods. Analytes included mature BDNF, pro-BDNF and the ratio. See Supplementary Materials and Methods for more details.

Results

Six SNPs for CACNA1C were studied, but only risk alleles for SNP rs1006737 were significantly more common in patients (64 v. 46%, P < 0.01, see Supplementary Tables 2 and 3). In total, 39 molecules were measured in either CSF or serum. Here, we analyse these biomarkers in relation to CACNA1C SNPs in patients with bipolar disorder and controls (see Supplementary Table 4 and Supplementary File 1 for complete results). The only significant difference that withstood correction for multiple comparisons was serum levels of BDNF variants. For patients with the rs2370411 risk allele, the mature BDNF/pro-BDNF ratio was 46% higher than in patients without the risk allele (mean: 1.74 (95% CI 1.46–2.02) v. 1.20 (95% CI 1.00–1.39)). Although there was no significant difference in either mature BDNF or pro-BDNF itself, the former was numerically higher and the latter lower, which is consistent with the ratio being higher. For controls with risk allele rs1006737, the serum level of mature BDNF was 18% lower than in those without the risk allele (27.15 ng/mL (95% CI 25.6–28.7) v. 33.15 ng/mL (95% CI 30.0–36.3)). There were no significant differences in mature BDNF/pro-BDNF ratio or in pro-BDNF in controls, although the first was higher and the second lower in those with the risk allele. As the serine protease tPA is known to convert pro-BDNF to mature BDNF,Reference Pang, Teng, Zaitsev, Woo, Sakata and Zhen9 serum concentrations of tPA were analysed post hoc in relation to CACNA1C genotype. For controls with the rs2370411 risk allele (dominant model), the mature BDNF/pro-BDNF ratio was significantly correlated with tPA (r = 0.56, P < 0.001, see Supplementary Table 5 for complete information). There were no differences between risk allele carriers and those with wild type concerning age, gender, smoking status, body mass index or medication (Supplementary Tables 6 and 7).

Discussion

Here, we screened for differences in biomarkers in both serum and CSF dependent on CACNA1C polymorphisms in patients with bipolar disorder and healthy controls. The main finding was that patients with the CACNA1C risk allele rs2370411 showed a 46% higher mature BDNF/pro-BDNF ratio in serum than patients without the risk allele. Further, in controls, the CACNA1C risk allele rs1006737 was associated with 18% lower mature BDNF serum levels.

The neurotrophic growth factor BDNF promotes the survival of existing neurons and induces differentiation and proliferation of developing neural precursors. By activating the extracellular protease plasmin, tPA regulates the cleavage of the immature form pro-BDNF to mature BDNF.Reference Pang, Teng, Zaitsev, Woo, Sakata and Zhen9 Importantly, pro-BDNF and mature BDNF impose opposite effects on several biological processes via different receptors.Reference Chao and Bothwell10 Multiple studies support the role of BDNF in bipolar disorder.Reference Sodersten, Palsson, Ishima, Funa, Landen and Hashimoto11 In one study, the authors analysed protein levels of different forms of BDNF in post mortem material of a group of patients with major depression, schizophrenia and bipolar disorder.Reference Yang, Ren, Zhang, Chen and Hashimoto12 In the parietal cortex, the concentration of the mature form was significantly lower in patients compared with healthy controls, whereas the concentration of the precursor form was higher. Also, all of tPA, mature BDNF and mature BDNF/pro-BDNF were found to be lower in patients with depression compared with controls.Reference Jiang, Chen, Li, Lu, Yue and Yin13 Our results suggest that BDNF levels in serum are associated with CACNA1C polymorphisms, possibly via tPA. Interestingly, tPA levels were positively correlated with mature BDNF/pro-BDNF in controls, but not in patients, for those with the risk allele rs2370411. The reasons for this discrepancy is unknown. A potential confounder is that lithium has a neuroprotective function by activating BDNF signaling.Reference Hashimoto, Takei, Shimazu, Christ, Lu and Chuang14 However, there was no difference in the proportion of patients treated with lithium in the two groups.

It remains a question for further research to unravel the mechanism by which CACNA1C genetic variants lead to changes in BDNF expression. It is known that BDNF expression is regulated by Ca2+ signalling via activation of cAMP response element by CaM kinase IV.Reference Shieh, Hu, Bobb, Timmusk and Ghosh15 The Ca2+ channels that are encoded by CACNA1C are furthermore known to efficiently regulate transcription via cAMP response element.Reference Zhang, Fu, Altier, Platzer, Surmeier and Bezprozvanny16 One may therefore hypothesise that risk variants of CACNA1C lead to changes in Ca2+ signalling, and thus altered BDNF-dependent transcription. Although the CACNA1C risk allele rs1006737 has gained widest interest in relation to bipolar disorder,Reference Ferreira, O'Donovan, Meng, Jones, Ruderfer and Jones2 rs2370411 has also been reported to be involved in mood-related behaviour in humans and to interact with gender.Reference Dao, Mahon, Cai, Kovacsics, Blackwell and Arad17

To conclude, we report that different risk alleles of CACNA1C are associated with serum levels of BDNF in patients with bipolar disorder and controls. This sheds light on possible links between genetic variants and pathophysiological mechanisms in bipolar disorder, and opens up new lines of research.

Supplementary material

Supplementary material is available online at https://doi.org/10.1192/bjp.2019.173.

Acknowledgements

We thank all of the participants who have kindly given their time to participate in our research. We also thank the staff at the St. Göran bipolar affective disorder unit, including study nurses Martina Wennberg, Lena Lundberg, and data manager Mathias Kardell. Yngve Hallström and Auris Pelanis are acknowledged for performing lumbar punctures. We finally thank the BBMRI.se and KI Biobank at Karolinska Institutet for professional biobank service.

Funding

This research was supported by grants from the Swedish Research Council (2018-02653), the Swedish foundation for Strategic Research (KF10-0039), the Swedish Brain foundation, and the Swedish Federal Government under the LUA/ALF agreement (ALF 20170019, ALFGBG-716801), all to M.L.. E.S. was funded by ALF Grants Västra Götalandsregionen. The funding source was not involved in analysis, interpretation of data or in writing the manuscript.

Footnotes

Declaration of interest None.

References

1Psychiatric GWAS Consortium Bipolar Disorder Working Group. Large-scale genome-wide association analysis of bipolar disorder identifies a new susceptibility locus near ODZ4. Nat Genet 2011; 43(10): 977–83.CrossRefGoogle Scholar
2Ferreira, MA, O'Donovan, MC, Meng, YA, Jones, IR, Ruderfer, DM, Jones, L, et al. Collaborative genome-wide association analysis supports a role for ANK3 and CACNA1C in bipolar disorder. Nat Genet 2008; 40(9): 1056–8.CrossRefGoogle ScholarPubMed
3Erk, S, Meyer-Lindenberg, A, Schnell, K, von Boberfeld C, Opitz, Esslinger, C, Kirsch, P, et al. Brain function in carriers of a genome-wide supported bipolar disorder variant. Arch Gen Psychiatry 2010; 67(8): 803–11.CrossRefGoogle ScholarPubMed
4Roussos, P, Giakoumaki, SG, Georgakopoulos, A, Robakis, NK, Bitsios, P. The CACNA1C and ANK3 risk alleles impact on affective personality traits and startle reactivity but not on cognition or gating in healthy males. Bipolar Disord 2011; 13(3): 250–9.CrossRefGoogle ScholarPubMed
5Jakobsson, J, Palsson, E, Sellgren, C, Rydberg, F, Ekman, A, Zetterberg, H, et al. CACNA1C polymorphism and altered phosphorylation of tau in bipolar disorder. Br J Psychiatry 2016; 208(2): 195–6.CrossRefGoogle ScholarPubMed
6Rolstad, S, Jakobsson, J, Sellgren, C, Ekman, CJ, Blennow, K, Zetterberg, H, et al. Cognitive performance and cerebrospinal fluid biomarkers of neurodegeneration: a study of patients with bipolar disorder and healthy controls. PLoS One 2015; 10(5): e0127100.CrossRefGoogle ScholarPubMed
7Sachs, GS, Thase, ME, Otto, MW, Bauer, M, Miklowitz, D, Wisniewski, SR, et al. Rationale, design, and methods of the systematic treatment enhancement program for bipolar disorder (STEP-BD). Biol Psychiatry 2003; 53: 1028–42.CrossRefGoogle Scholar
8Kübler, U. Structured Clinical Interview for DSM-IV (SCID). In Encyclopedia of Behavioral Medicine (eds Gellman, MD, Turner, JR): 19191920. Springer, 2013.CrossRefGoogle Scholar
9Pang, PT, Teng, HK, Zaitsev, E, Woo, NT, Sakata, K, Zhen, S, et al. Cleavage of proBDNF by tPA/plasmin is essential for long-term hippocampal plasticity. Science 2004; 306(5695): 487–91.CrossRefGoogle ScholarPubMed
10Chao, MV, Bothwell, M. Neurotrophins: to cleave or not to cleave. Neuron 2002; 33(1): 912.CrossRefGoogle ScholarPubMed
11Sodersten, K, Palsson, E, Ishima, T, Funa, K, Landen, M, Hashimoto, K, et al. Abnormality in serum levels of mature brain-derived neurotrophic factor (BDNF) and its precursor proBDNF in mood-stabilized patients with bipolar disorder: a study of two independent cohorts. J Affect Disord 2014; 160: 19.CrossRefGoogle ScholarPubMed
12Yang, B, Ren, Q, Zhang, JC, Chen, QX, Hashimoto, K. Altered expression of BDNF, BDNF pro-peptide and their precursor proBDNF in brain and liver tissues from psychiatric disorders: rethinking the brain-liver axis. Transl Psychiatry 2017; 7(5): e1128.CrossRefGoogle ScholarPubMed
13Jiang, H, Chen, S, Li, C, Lu, N, Yue, Y, Yin, Y, et al. The serum protein levels of the tPA-BDNF pathway are implicated in depression and antidepressant treatment. Transl Psychiatry 2017; 7(4): e1079.CrossRefGoogle ScholarPubMed
14Hashimoto, R, Takei, N, Shimazu, K, Christ, L, Lu, B, Chuang, DM. Lithium induces brain-derived neurotrophic factor and activates TrkB in rodent cortical neurons: an essential step for neuroprotection against glutamate excitotoxicity. Neuropharmacology 2002; 43(7): 1173–9.CrossRefGoogle ScholarPubMed
15Shieh, PB, Hu, SC, Bobb, K, Timmusk, T, Ghosh, A. Identification of a signaling pathway involved in calcium regulation of BDNF expression. Neuron 1998; 20(4): 727–40.CrossRefGoogle ScholarPubMed
16Zhang, H, Fu, Y, Altier, C, Platzer, J, Surmeier, DJ, Bezprozvanny, I. Ca1.2 and CaV1.3 neuronal L-type calcium channels: differential targeting and signaling to pCREB. Eur J Neurosci 2006; 23(9): 2297–310.CrossRefGoogle ScholarPubMed
17Dao, DT, Mahon, PB, Cai, X, Kovacsics, CE, Blackwell, RA, Arad, M, et al. Mood disorder susceptibility gene CACNA1C modifies mood-related behaviors in mice and interacts with sex to influence behavior in mice and diagnosis in humans. Biol Psychiatry 2010; 68(9): 801–10.CrossRefGoogle ScholarPubMed
Supplementary material: File

Smedler et al. supplementary material

Smedler et al. supplementary material 1

Download Smedler et al. supplementary material(File)
File 81.1 KB
Supplementary material: File

Smedler et al. supplementary material

Smedler et al. supplementary material 2

Download Smedler et al. supplementary material(File)
File 81.3 KB
Supplementary material: File

Smedler et al. supplementary material

Smedler et al. supplementary material 3

Download Smedler et al. supplementary material(File)
File 29.1 KB
Submit a response

eLetters

No eLetters have been published for this article.