Age-related obesity and type 2 diabetes dysregulate neuronal associated genes and proteins in humans

INTRODUCTION

The homeostasis of blood glucose levels is maintained by both insulin and glucagon synthesis, which is functionally tightly regulated by the pancreatic β-cells and α-cells respectively. When blood glucose levels rise (hyperglycemia), pancreatic β-cells synthesize and secrete insulin to the bloodstream to regulate glucose levels. On the contrary, when circulating glucose levels fall below normal values (hypoglycemia), pancreatic α-cells produce and release glucagon to the bloodstream to tune up glucose concentrations via conversion of stored glycogen into glucose and its release into the circulation [1, 2]. Thus, a disruption in blood glucose regulation leads to the hyperglycemia state so-called diabetes. There are two types of aged-related [3, 4] diabetes; type 1 diabetes (T1D) and type 2 diabetes (T2D). Diminished or dysregulation of insulin by β-cells in T1D and T2D respectively are caused by cell aging process. T1D is an autoimmune disease that pancreatic β-cells are targeted to be broken down by antibodies produced by immune B cells. In this regard, the main production site of insulin is diminished by β-cells [5–9]. In contrast, in age-related-T2D the pancreatic β-cells are still active and do synthesize insulin but at dysregulated levels and not sensitive enough [10–13]. In a normal state, there is a homeostatic balance and cross talk between skeletal muscle, liver and adipose tissue (AT) organs with respect to glucose levels, which is strictly under control of insulin [14]. In this regard, insulin 1- promotes glucose uptake and inhibits lipolysis by the skeletal muscle, 2- stimulates glycogenesis and suppress glucose formation and release from the liver, and 3- stimulates adipogenesis and prevent lipolysis in AT-associated adipocytes [14]. In an obese state, insulin shows a function completely opposite to the normal state in these three organs. Moreover, it has been recently shown that other cells such as adipocytes, macrophages also synthesize insulin [15]. Patients with either T1D or T2D diabetes are at high risk for serious complications such as cardiovascular diseases (CVDs) [16] and diabetic neuropathy (DN) [17–23]. Obesity plays an important role in the development of T2D and its complications via the promotion of an inflammatory state [16]. In this regard, Systems biology could be a solution to find etiology of aged-related diseases such as T1D, T2D, neurodegenerative and cardiovascular diseases [24].

DNs are the most common micro-vascular complications that occur in both T1 and T2 diabetes (40–60%) [18–20, 25, 26]. DNs-associated syndromes are classified into two groups; diffuse and focal. The former neuropathies are usually chronic and more common among diabetic patients, while focal neuropathies are acute [25]. In general, DNs occur in progressive damages of neuronal cells that commonly appear with symptoms such as severe pain, loss of sensation and disability [19, 22, 25].

Despite the general agreement that hyperglycemia plays a key role in initiation and development of DNs, the underlying mechanisms for the development of DNs is unknown and remains to be investigated [19, 22, 27]. Numerous studies have shown that hyperglycemia leads to the overload of electron transport chain in mitochondria and subsequent oxidative stress. The imbalance in the mitochondrial redox state, in favor of oxidation conditions, leads to the accumulation of reactive oxygen species (ROS). Subsequently, oxidative stress affects several metabolic pathways [such as insulin signaling pathway and protein kinase C (PKC) pathway; advanced glycation end products (AGEs) and mitogen activated protein kinase (MAPKs)] associated with glucose metabolism with enhanced oxidative stress and, in turn, inflammatory reactions [20, 21, 25, 28–32].

Although numerous drugs and therapies have been proposed to treat the DNs, the majority of these drugs and treatments were restricted to target the redox and glucose metabolic pathways [20, 32]. None of the drugs that targeted glucose metabolic pathways showed any efficient effect in the treatment of DNs [19, 22]. Also, despite identification of the genes [19] and metabolic pathways associated with DNs, the molecular causes of DNs events still occur in a large scale. These studies suggest that beside hyperglycemia other genetic components and factors may contribute to the development of DNs. For instance, tight links between oxidative stress and obesity were recently reported, which may provide new insight for investigation of the genes associated with DNs [21]. Meijer et al. have recently shown that metabolic dysfunction leads to the adipocytes hypertrophy (the main cause of obesity), which primes inflammation in AT [15, 16] and, in turn, is implicated in pathophysiological states such as energy storage disruption within adipocytes (e.g. triglycerides breakdown, FFAs, glycerol et cetera), insulin resistance (IR), and hyperglycemia as hallmark of T2D.

Feldman et al. reported several pathways involved in lipid, carbohydrate and energy metabolism modulating gene expression patterns in peripheral nerves on BKS db/db mouse sciatic nerve. Although this study support the hypothesis that hyperglycemia play an important role in nerve damage, lipid metabolism may involve neuronal damage and development of DNs as well [19]. Since both pancreas and AT are key tissues involved in age-induced T2D and its complications, this study was designed to investigate whether T2D alters the expression of genes with a function in neuronal processes in human pancreas and AT and that might be implicated in the insurgence of DNs.

RESULTS

The effect of type 2 diabetes on genes with a neuronal function

Pancreas

To investigate whether there are genes with a neuronal function that could show highly and clear changes in expression and that caused by age-induced T2D, we measured mRNA expression in human pancreas and adipose tissue (AT) with T2D. As depicted in Table 1 and Figure 1, two genes OLIG1 and BAG3 were highly up-regulated and eight genes PRDM16, GLDNA, APOA1, CCKBR, EDN3, VAV3, CXCR4, and GHRL were down regulated in pancreas with T2D as compared to pancreas control. Based on Gene Ontology database search, OLIG1 gene shows functions in neuron fate commitment, neurogenesis, generation of neurons, and neuron differentiation as shown in Figure 2. Based on database search, BAG3 gene showed only a neural function (i.e. neuron part). There were 24 neuron functions found for these 10 genes in pancreas of which chemokine C-X-C receptor (CXCR4) gene was shown to have a role in 17 neural functions based on Gene Ontology database (Figure 2). Among eight down-regulated genes in pancreas with T2D, VAV3 gene was highest down-regulated gene with approximately 246-fold (Table 1 and Figure 1).

Adipose tissue (AT)

The expression of 15 genes were found to be highly altered in AT caused by age-induced T2D (Table 2 and Figure 3). From these 15 genes, 8 gens were highly up-regulated and 7 genes highly down-regulated (Table 2, and Figure 3). The expression of synaptotagmin-4 (SYT4) gene were tremendously high up-regulated (approximately 392-fold) in AT-T2D as compared to AT-control, while VGF (neurosecretory protein) is highly down-regulated (approximately 119-fold) Table 2 and Figure 3). Another gene, which is very highly up-regulated in AT-T2D as compared to AT-control was MYRF (Myelin regulatory factor) as displayed in Table 2 and Figure 3. The fold changes of all 15 genes were reported in Table 2. Based on Gene Ontology database search, 52 neural functions were found for these 15 genes (Figure 4). Although VGF gene was highly down-regulated, only one neural function (i.e. neuropeptide hormone activity) was shown to be linked with this gene (Figure 4). SYT4 gene showed a link with 5 neural functions; 1- neurological system process, 2- neurotransmitter secretion, 3- neurotransmitter transport 4- neuron part and 5- neuron projection. Based on Gene Ontology search, PTN and LRNN4 genes showed only link with one neural function (Figure 4) and both genes were up-regulated, while the other genes showed multiple neural functions.

Pathway analysis

The in-silico functional analysis conducted on the list of 25 genes, led to the identification of several molecule-function/disease connections, as shown in Figure 5. Focusing on SYT4, VGF, BAG3, APOA1, and VAV3 and on their tightly related interactors, which in turn participated to lipid metabolism, insulin, protein kinase C (PKC), advanced glycation end (AGE) products and MAPK signaling pathways, as well as to the electron transport chain, oxidative stress and glucose metabolism biological processes, we have drawn a global interaction network (Figure 6). It contained 198 (13.8%) multi-process genes, with 31 (AKT2, CALM1, CALM2, CALM3, FOXA2, G6PC, HRAS, IKBKB, INSR, IRS1, MAPK1, MAPK3, MAPK8, MLYCD, PDK4, PRKAA1, PRKACA, PRKACB, PRKACG, PRKCG, PRKCZ, RAF1, SHC1, G6PD, PLA2G4A, SIRT1, SOD1, TNF, CASP3, EGFR and MAPK14) genes participating to 3 processes, 7 (FOXO1, INS, MAP2K1, MAPK9, PRKCA, PRKCB and NFKB1) genes participating to 4 processes and 2 (AKT1 and PPARGC1A) genes taking EGFR, SHC1 and INSR part in 5 processes. Due to its high node degree [33], BAG3 resulted highly central in the whole graph. Among the others, it was connected to 8 multi-process genes, including G6PD. APOA1 was mostly connected to lipid metabolism-related genes, with 3 multi-process genes, including AKT2. SYT4 was connected to 5 genes of which only 3 were bi-process. Half of the VAV3 interactors were multi-process, while VGF interacted with 7 genes, including 2 bi-process and MAPK3.

The ELISA of SYT4, VGF, BAG3, ApoA1, and VAV3 proteins in plasma of 41 human subjects

To confirm the mRNA expression data derived from AT and pancreas with and without T2D, we measured five proteins SYT4, VGF, BAG3, ApoA1, and VAV3 in four different groups of 41 human subjects; 1- Lean (control), 2- Obese, 3- Obese with T2D without receiving insulin (obese+T2D-INS), and 4- Obese with T2D receiving insulin (obese+T2D+INS).

SYT4 and VGF proteins

Although the protein concentration of SYT4 was not significantly changed in obese, obese-T2D with and without receiving insulin human subjects as compared to lean group, there was a clear up-regulation trend (Figure 7A), which is in agreement with SYT4 gene up-regulation. As depicted in Figure 7B, VGF protein concentration was significantly increased in both obese-T2D with and without receiving insulin subjects as compared to lean group. Although there was no significant difference between obese and lean group, the average of VGF protein concentration was clearly higher in obese subjects than lean group (Figure 7B).

BAG3, APOA1, and VAV3 proteins

The plasma protein concentration of BAG3 was found to be similar in obese, obese-T2D without receiving insulin and lean subjects. However, there was a trend towards reduction in obese-T2D subjects receiving insulin as compared to the other three groups (Figure 8A). The protein levels of ApoA1 were not significantly reduced in all three experimental groups of patients as compared to the control lean group (Figure 8B). However, when obese-T2D subjects were injected with insulin, the plasma concentration of ApoA1 goes up comparing with obese and obese-T2D without injection of insulin as displayed in Figure 8B. Plasma VAV3 protein levels (Figure 8C) show a similar pattern as ApoA1, which is mirrored by down-regulation of ApoA1 and VAV3 genes. All statistical analysis obtained by ANOVA and ANCOVA was summarized in Table 3.

DISCUSSION

Aging can be expressed simply as “functionality reduction of biological process” or as “loss or reduction of the regulated cell function”. Of note, the aging process can be distinguished between early or premature aging and regulated (normal) or healthy aging. Thus, all diseases such as obesity, IR, diabetes, degenerative disease, and cancer could be just referred to aging or aging-related diseases. The discovery of the factors responsible for premature aging or healthy aging will provide us information to correct premature aging or extend healthy aging [23].

Although the underlying mechanisms for the development of human T1D (autoimmune disease) are completely different from T2D, insulin signaling pathway, glucose levels, and energy storage components are involved in both types of diabetes. Both age-induced T1D and T2D are associated with many complications such as DNs. We hypothesized that AT and pancreas could be involved in the development of DNs in age-related T2D. AT is important during the insurgence of insulin resistance in the frame of obesity and produce factors involved in energy metabolism, such as chemokines/cytokines, and the pancreas is implicated in insulin production. There is little known about the genes involved in DNs in these two organs (with or without T2D). This study was designed to select only genes with very highly up-regulated or down-regulated in AT and pancreas with age-related T2D (the cut off was adjusted to ≥ 32 (=2⁵) times). This selection criterion was chosen to prevent false positive gene differences between control and T2D in these two organs of human.

Overall, 10 genes with a neural function were found in pancreas-T2D of which 8 genes were highly down-regulated and 2 genes highly up-regulated. Although it is difficult from our studies to infer about the mechanism behind each gene in the development of DNs, we assume that these 10 genes could be potentially major players in DNs.

One of the functions of CXCR4 is known to regulate neuronal signaling and promotes hippocampal-neuron survival [34–38], while the mutation affected the gene and, in turn, suppression of CXCR4 function. Thus, down-regulation of CXCR4 function may lead to the promotion of neuronal apoptosis. Of note, the CXCR4 was down-regulated in pancreas-T2D. Neuronal survival and regulation of neuronal signaling by CXCR4 might be reduced in T2D patients, and this may play a critical role in the development of DNs. Moreover, Based on Gene Ontology database search, 17 hits with neuronal function were found for CXCR4.

To date, apolipoprotein A-1 (APOA1) was shown to be synthesized in the liver and in the small intestine and it is a major constituent protein of plasma high-density lipoprotein (HDL). APOA1 plays a major role in reverse cholesterol transport, as it has a high capacity to drive cholesterol efflux [39–41]. Intriguingly, APOA1 was highly expressed in control pancreas but highly down-regulated in pancreas-T2D. Several studies have shown that the mutation in APOA1 is involved in the pathogenesis of polyneuropathy [42–46]. Also, APOA1 convincingly plays a role not only in the early stage but also in late neuropathy [42–46]. These studies support our finding that APOA1 is highly down-regulated in pancreas-T2D, and it is involved in 6 neural processes.

GHRL is also known as appetite-regulating hormone; it is highly down-regulated in pancreas-T2D and shows 2 neural functions. GHRL has been reported to protect neurons from damage and to improve neurons survival [47]. This may suggest that a down-regulation of GHRL could result in a decreased neural protection and neural survival [47].

OLIG1, also known as oligodendrocyte transcription factor 1, is very highly up-regulated in pancreas-T2D with four neural function hits and is involved in the formation of oligodendrocytes and together with OLIG2 establish precursor motorneuron (pMN) of embryonic neural tube [48]. Based on literature search, we could only find one study related to up-regulation of OLIG1 and disease [49]. In this study, OLIG1 was highly expressed in oligodendrogliomas and considered as biomarker for glial brain tumors. Thus, the up-regulation of OLIG1 in pancreas-T2D suggests that new studies are crucial to better elucidate OLIG1 function (s).

The major action of VAV3 (also guanine nucleotide exchange factor (GEF)) is in angiogenesis and it has been recently shown that loss of VAV3 in mice on chow diet resulted in liver steatosis and age-induced T2D [50]. Surprisingly, when the same mice were fed a high fat diet, they showed resistance against diet-induced obesity and metabolic syndrome [51]. However, our findings in humans do not support the data collected from mice deficient in VAV3. VAV3 showed a down-regulated of approximately 246-fold in human pancreas with T2D as compared to control pancreas. This finding indeed suggests that the action of VAV3 in human is completely different from that in mice with manipulated VAV3 gene: the restoration of VAV3 in pancreas-T2D could contribute to less severe DNs.

In AT-T2D, 8 genes were highly up-regulated and 7 genes down-regulated with neuronal hits. It is beyond the scope of this study to unravel and discuss the individual mechanism of each gene in the development of DNs. We assume that these 15 genes could be potentially major players in DNs. This study provides preliminary evidence for further investigations.

SYT4 (Synaptotagmin-4) and VGF (neurosecretory protein) genes are dramatically up-regulated and down-regulated in AT-T2D, respectively. SYT4 is mainly detectable in brain and neuroendocrine system and it has been suggested to have a neuroendocrine role [52, 53]. These authors showed that up-regulation of SYT4 blocked the release of oxytocin, which in turn resulted in an obese phenotype [52, 53]. On the contrary, down-regulation of SYT4 normalized oxytocin release, indicating that obesity and its afflictions are under regulation of hypothalamic neuropeptides [52, 53]. Based on our novel finding (overexpression of SYT4 in AT-T2D) and intriguing finding by Zhang et al. [52], we hypothesize that SYT4 can be used as a new biomarker for obesity and T2D and may be considered as prognostic marker for age-induced T2D, and negative regulation of SYT4 could potentially repair or reduce the degree of DNs.

The main function of VGF (also called neuroendocrine regulatory peptide (NERP)) is synaptogenesis and they are mainly present in neuron and neuroendocrine cells [53–55]. Body fluid homeostasis was also maintained by VGF through regulation of vasopressin release [54, 55]. Moreover, VGF or VGF-derived peptides increase lipolysis in AT and in turn energy consumption in VGF deficient mice (knock-out), which are lean [56]. However, VGF was highly down-regulated in AT-T2D, which does not support the results obtained from VGF knock-out mice [56]. These contradictory results could be due to specific differences between mice and humans. Based on this evidence, we speculate that the VGF up-regulation (e.g. by an agonist) together with down-regulation of SYT4 could restore the homeostatic balance between energy consumption and energy storage regulation, which could repair or reduce DNs.

Of note, the gene-expression data do not have enough power without the confirmation of gene product (i.e. protein). For this reason, five from 25 genes was selected to measure their protein levels. SYT4 and VGF proteins were chosen from AT-associated 15 genes, because SYT4 gene was highest and VGF lowest expressed in AT-T2D respectively. Although plasma VGF protein concentration in three groups of patients did not correspond with VGF gene expression, both plasma SYT4 and VGF protein concentrations were increased and decreased in obese-T2D with insulin injection as compared to without insulin injection in human subjects respectively. The effect of insulin was also observed for BAG3, APOA1 and VAV3 in obese-T2D with and without insulin injection in human subjects. Based on these data, it is then logic to assume that insulin has an effect on the concentrations of these five proteins and this role of insulin could be considered as so-called “corrector”. Importantly, VGF gene expression did not correspond to VGF protein levels and one reason could be that post translational modifications (PTMs) determine VGF protein levels and not transcriptional phase. Although we did not observe any significant differences between three patient groups and lean subjects with respect to SYT4, BAG3, APOA1, and VAV3, except for VGF protein, there was a trend between the expression of these four genes and their protein levels.

The majority of investigations and drug developments for DNs conducted so far focused on glucose metabolic pathways. Neuropathies still remains a great problem in patients with diabetes. The expression of APOA1 in control pancreas and severe down-regulation in pancreas with T2D is very novel and important finding, which open new avenues on lipid metabolism, HDL, cardiovascular events, diabetes and its complications such as neuropathies, and will help to design new future studies. GHRL and VAV3 are also expressed in pancreas and subjected to extreme level changes in pancreas-T2D. SYT4 and VGF were synthesized in AT and the levels alter in AT-T2D dramatically. Based on this study, we conclude that not only diabetes but also its complications such as DNs are multifactorial diseases. Also, this study provides us a list of most important genes affected by diabetes involved in neuronal processes, which opens new avenues for new investigations for drug development (using agonists or antagonists) and new pathway(s) for the treatment of DNs.

MATERIALS AND METHODS

Human biopsies and gene expression procedures

Total RNA was isolated from human adult normal visceral AT and AT-T2D. Total RNA was collected from 5 pooled human normal pancreases and one pancreas with T2D provided by AMS Biotechnology (Amsbio, England). The quality and concentrations of RNAs were assessed in a Bioanalyzer (Experion), (Bio-Rad, USA/The Netherlands) using the Agilent RNA 6000 Nano kit (Agilent, The Netherlands). Amplification Kit was applied to amplify and label the RNA (Applied Biosystems, The Netherlands). Total RNA was reverse-transcribed into cDNA, and the concentrations were determined in NanoDrop. RNA Amplification Kit (Ambion, USA) was used to biotinylate cRNA according to the manufacturer’s instructions. Samples were purified using the RNeasy kit (Qiagen, The Netherlands). Hybridization to the Sentrix Human Expression BeadChip, washing, and scanning were performed according to the BeadStation 500 manual (revision C). One BeadChip with 12 samples was used. Each slide was scanned immediately. After the scanning, the following steps were performed: 1: quality check; 2: background correction; 3: normalization to housekeeping genes; and 4: utile normalization of the data using Beadstudio Expression module v 3.2.7. After these 4 steps, a relative mRNA intensity of ²log was considered cut-off. Each pancreas sample was three times and AT samples two times measured. The methods were carried out in “accordance” with the approved guidelines.

Human subjects and plasma collection

41 human subjects divided into four groups of 10 (except lean group 11 subjects), independent of age and gender, as follows: Group 1-Lean subjects with a body mass index (BMI) between 20.1 and 25.6 kg/m2, Group 2- Obese subjects with a BMI greater than or equal to 30 kg/m2, Group 3- Obese subjects with T2D without receiving insulin (obese+T2D-INS) and a BMI greater than or equal to 30 kg/m2 30 and Group 4- Obese subjects with T2D, receiving insulin (obese+T2D+INS) and BMI greater than or equal to 30 kg/m2. All patients were well-selected based on their BMI. Blood was drawn from each subject after informed consent by venipuncture into tubes containing Ethylene Diamine Tetra Acetic Acid (EDTA) as anticoagulant. Subsequently, plasma was isolated by centrifugation at 1500× g for 15 min at 4°C and stored at –80°C for further analysis.

The measurement of protein concentrations of SYT4, VGF, BAG3, APOA1, and VAV3 by ELISA

96-well microtitration plates (NuncSorb) were coated with primary antibodies (100 μl at 5 μg/ml in PBS, 4°C). After four washes with PBS, the wells are saturated with BSA (200 μl, 3% in PBS, at least 2 h at RT). After four washes with PBS, 25 μl of each human serum sample were deposited in the wells and protein were allowed to bind to their specific mAb during 3 h at RT. All proteins not specifically bound were eliminated by four washes with PBS. Then the HRP-conjugated secondary antibodies were added (100 μl at 1 μg/ml in PBS, 45 min at RT). After four washes with PBS, 100 μl of HRP substrate (TMB: 3,3′,5,5′-tetramethylbenzidine; Thermo Scientific Pierce) were deposited and reaction was allowed during 15 min in dark (upon oxidation, TMB forms a water-soluble blue reaction product that can be measured spectrophotometrically at 650 nm). Reaction was then stopped by addition of 100 μl H2SO4 2 M (upon acidification, the reaction product becomes yellow with an absorbance peak at 450 nm). Absorbance at 450 nm (yellow) was monitored on a plate-reader device. Primary antibodies were purchased from SIGMA (SYT4, APOA1, BAG3), from Santa Cruz Biotechnology (VAV3) and Abcam (VGF). HRP-coupled secondary antibodies (anti-mouse, anti-goat, anti-rabbit) were purchased from Abcam.

Interaction network-based pathway analysis

Genes belonging to lipid metabolism, insulin, protein kinase C, advanced glycation end (AGE) products and MAPK signaling pathways, together with those participating to the electron transport chain, oxidative stress and glucose metabolism biological processes were collected [57–58]. Considering that correlation of gene expression and protein to protein interactions have been shown to cluster genes of similar function [59], we queried UniProtKB, Mentha [60], STRING [61] and BioGRID [62] in search of any evidence of connection between these genes and BAG3, APOA1, VGF, VAV3 and SYT4. Interactions were represented as edges of graphs, while nodes denoted genes, as already explained in [63]. Genes were colored according to the biological processes/pathways they were participating in. Light blue nodes represented genes that took part to multiple processes and pathways. Differential expressions of BAG3, APOA1, VGF, VAV3 and SYT4 genes between normal and patient samples were evaluated by unpaired student t-test at significance level of α = 5%. A global view of the functional involvement of the 25 genes into the abovementioned critical processes and pathways has been further obtained by the Ingenuity Pathway Analysis workbench. A gene-function mixed network was generated, where edges corresponded to literature-confirmed scientific evidences of interaction between any two genes. Dashed edges represented indirect interactions. Green colored genes were down-regulated in our case-study, while red genes were up-regulated. Molecule shapes correspond to as many kinds of molecules, as for functions or diseases (octagons and crosses).

Statistics

ANOVA was performed as statistical analysis to identify the protein levels of SYT4, VGF, VAV3, APOA1 and BAG3 for each BMI group (1- lean, 2- obese, 3- obese+T2D-INS and 4- obese+T2D+INS).

Analysis of covariance (ANCOVA) was used to identify differentially proteins concentrations of SYT4, VGF, VAV3, apoA1, and BAG3 across the four groups as controlling for the effects of confounding variables including age and gender. ANCOVA analysis was done using change of proteins concentrations in groups as dependent variable; ordinal variable of four groups (lean, obese, obese- T2D-INS, obese-T2D+INS) as a fixed effect and the effects of confounders were controlled in analysis as covariates (Table 3). The choice for a post-hoc analysis was due to having five proteins profiles across four groups. All statistical tests were two-sided and performed at a significance level of α = 5%. Data analyses were performed using SPSS statistical software (version 22; SPSS Inc., Chicago, USA).

ACKNOWLEDGMENTS AND FUNDING

The authors would like to thank the Erasmus Medical Center Rotterdam for their financial support of this study.

Ethics statement

This study was approved by the Medical Ethical Committee of the Erasmus Medical Center, Medical University of Rotterdam, under MEC number: 2009–242. Written informed consent was obtained from all participants. The methods were carried out in “accordance” with the approved guidelines.

COMPETING FINANCIAL INTERESTS

The authors declare no competing financial interests.

Authors have nothing to disclose.

Author contributions

MR and FR wrote the paper. FR conceived, designed and coordinated the study. MV edited paper, MV and VP performed ELISA. BO, FWMDR and ES provided patients and edited paper. MP edited paper. MA and FR performed statistics. FS, MD, TM, and FR prepared the figures. FR analyzed ELISA. MMM, VK, MM, MMP, FR analyzed gene data and edited manuscript.

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