Abstract
Schizophrenia is a neuropsychiatric illness with no single definitive aetiology, making its treatment difficult. Antipsychotics are not fully effective because they treat psychosis rather than the cognitive or negative symptoms. Antipsychotics fail to alleviate symptoms when patients enter the chronic stage of illness. Topical application of niacin showed diminished skin flush in the majority of patients with schizophrenia compared to the general population who showed flushing. The niacin skin flush test is useful for identifying patients with schizophrenia at their ultra-high-risk stage, and understanding this pathology may introduce an effective treatment. This review aims to understand the pathology behind the diminished skin flush response, while linking it back to neurons and microglia. First, it suggests that there are altered proteins in the GPR109A-COX-prostaglandin pathway, inflammatory imbalance, and kinase signalling pathway, c-Jun N-terminal kinase (JNK), which are associated with diminished flush. Second, genes from the GPR109A-COX-prostaglandin pathway were matched against the 128-loci genome wide association study (GWAS) for schizophrenia using GeneCards, suggesting that G-coupled receptor-109A (GPR109A) may have a genetic mutation, resulting in diminished flush. This review also suggests that there may be increased pro-inflammatory mediators in the GPR109A-COX-prostaglandin pathway, which contributes to the diminished flush pathology. Increased levels of pro-inflammatory markers may induce microglial-activated neuronal death. Lastly, this review explores the role of JNK on pro-inflammatory mediators, proteins in the GPR109A-COX-prostaglandin pathway, microglial activation, and neuronal death. Inhibiting JNK may reverse the changes observed in the diminished flush response, which might make it a good therapeutic target.
Keywords: diminished GPR109A-flushed effect, niacin, microglia, JNK treatment, schizophrenia, c-Jun N-terminal kinase (JNK) pathway, neuron
Introduction
Our society has neglected satisfactory categorisation of mental illness for over 2,000 years (1). In the past, schizophrenia had failed to be defined and understood as its own entity (2). The term schizophrenia was coined by Blueler (3, 4). Blueler and Kraepelin described the symptoms and aetiology of the illness (5). Schizophrenia is diagnosed by its symptoms, where positive symptoms include hallucinations, delusions, disorganised thoughts, and speech; negative symptoms include anhedonia, apathy, and social withdrawal; and cognitive symptoms include inattention, impaired working memory, and dysfunctional executive functions, which affect thoughts, intelligence, and ability to plan. Most individuals diagnosed with schizophrenia undergo a prodromal stage before full-blown psychotic symptoms appear, where individuals experience changes in both cognition and behavioural function (6, 7). The early onset of symptoms usually occurs between the ages of 14 to 29 (4); therefore, identifying the ultra-high-risk population is crucial for initiating early intervention.
Schizophrenia represents one percent of the global population and remains one of the top 25 leading disability worldwide (8). The World Health Organisation estimated that the direct cost for schizophrenia ranges from US$94 million to $102 billion (9). However, the substantial burden of the illness has been linked to its early onset and incurable nature with persistent symptoms (10). Heterogeneous illnesses have other problems, where a majority of research focuses on the altered neurotransmitter function of schizophrenia, typically dopamine or glutamate, in which treatments associated with this paradigm (currently dopamine antagonists) fail to alleviate negative and cognitive symptoms in 30–60% of the patients (11–14). Current antipsychotics increase the risk of other comorbidities associated with the heart (15) or diabetes (16).
Alternative approaches should be considered when treating this complex disorder. Both Kraepelin and Bluer identified that the aetiology of schizophrenia is a consequence of gene-environment interactions (5). Dr. Hoffer proposed megavitamin B3 therapy, in which niacin (vitamin B3) intake over time reduces symptoms of schizophrenia (17). The general population exposed to niacin showed skin flush as a side effect (18), whereas, niacin exposure in the majority of schizophrenia patients showed diminished skin flush (19–22). The diminished flush response serves as an endophenotype and separates patients with schizophrenia from other mood disorders such as depression (23), bipolar disorder (24, 25), and social phobia (26).
Prostaglandins in the cyclooxygenase (COX) pathway have been connected to flushing (Figure 1). However, it is unclear how these prostaglandins are deactivated or reduced in patients with schizophrenia. Other factors that have been thought to influence diminished flush include smoking (32, 33), alcohol consumption, caffeine intake, use of medicine (34), and altered chemical mediators such as nitric oxide (NO) (35, 36), histamine, and adrenaline (37). The aberrant immune response observed in these patients may be related to a diminished flush response (38–44). While current studies link the diminished flush in peripheral immune cells, this review aims to investigate possible links between diminished niacin-GPR109A flush responses mediated via the GPR109A-COX-prostaglandin pathway in microglia and neuronal cells. This study aimed to investigate the link between altered protein expression or activity in the GPR109A-COX-prostaglandin pathway with associated inflammatory mediators and the c-Jun N-terminal kinase (JNK) signalling pathway in patients with schizophrenia. Furthermore, GeneCards were used to manually identify chromosome numbers of genes from the GPR109A-COX-prostaglandin pathway with a 128-loci GWAS for schizophrenia (45).
Neuroinflammation
A meta-analysis observed a neuroinflammatory imbalance in patients in the early stage of schizophrenia (46, 47). There have been alterations in inflammatory markers such as cytokines, reactive oxygen species (ROS), reactive nitrogen species (RNS), and nitrogen oxygen species (NOS) (47). This section provides evidence for altered neuroinflammatory markers in schizophrenia and links it to neuronal and microglial cells. Inflammatory markers play an important role in regulating flush response and microglial activation. Furthermore, it has been observed that the cytokine subtype released (Figure 2) and oxidants levels (Figure 3) regulates the activation of microglia (80). This may raise questions as to how peripheral cytokines may enter the brain. It may be assumed that patients with schizophrenia have poor blood-brain barrier; however, cytokines can enter the brain in different ways (Figure 4). The brain is vulnerable to oxidative stress, such as ROS, NOS, and superoxide species (75). Oxidative stress is defined as the imbalance between pro-and anti-oxidative processes, and there is an imbalance of oxidative stress throughout the different stages of schizophrenia (74, 89–91). Likewise, there is evidence of abnormal antioxidants in the peripheral blood (92–94), CSF (65) and post-mortem brain tissue (74, 95) of patients with schizophrenia. In conclusion, this evidence suggests that the lack of balance between the pro-oxidant and anti-oxidant may contribute to the neuronal abnormalities observed in schizophrenia patients.
Microglia Activation
The microglia hypothesis (43, 44) suggests that activated microglia are present from prenatal infection to adolescence. When the immune system is challenged, microglial cells are exacerbated, and therefore, prolonged microglial hyperactivity causes cellular or neuronal apoptosis (96). The two-hit process supported by this hypothesis may explain why people who may have exposure to infection in childhood may not go to develop the illness.
Microglia have been shown to be more activated in schizophrenia than in control subjects (97). Studies using positron emission tomography (PET) and peripheral benzodiazepine receptor ligand, (11)C-(R)-PK11195, detected microglial activation in the hippocampus (38) and grey matter (97) of patients with schizophrenia. Bloomfield et al. (98) observed that ultra-high-risk individuals showed increased microglial activation.
Neurons
Patients with schizophrenia have a selective loss of grey matter volume, including the left superior temporal gyrus (STG), left Heschl gyrus (HG), left planum temporale (PT), and reduced spine density in the frontal cortex and hippocampus (99–103). The frontal cortex and hippocampus are associated with cognitive functions and reduction in neurons in brain regions, resulting in the cognitive deficits observed in schizophrenia (104). In the cellular pathology of diminished flush response, there are elevated levels of IL-1B and TNF-α, which might mean that microglia are activated. Active microglia and increased pro-inflammatory levels alter the functioning role of LTP, and AMPA and GABA receptors result in neuronal damage. Cognitive deficits may be due to impaired microglia-neuronal function, as microglia and neurons share bidirectional communication (Figure 5).
JNK
Schizophrenia is a complex disorder that involves disruption of metabolism, neurotransmission, and cell signalling, and requires the coordination of kinase-mediated signalling events. There has been a signalling imbalance, which may be associated with diminished flush in schizophrenia. MAPKs are a family of serine/threonine protein kinases that are directly modified by ROS/RNS. MAPK can be activated by its upstream MAPKK, MAPKKK, or ROS/RNS (115). The MAPK pathway links inflammation and microglial activation (116). The MAPK family consists of the ERK, JNK, and p38 pathways. JNK has been the most affected kinase in the anterior cingulate circuit (ACC) of patients with chronic schizophrenia (117). This review focuses on JNK, and (Figure 6) shows the characteristic profile of JNK. JNK interacts with both microglia and neurons (Figure 7) through inflammatory mediators.
Niacin-GPR109A Flush Response
PGD2 and PGE2 are potent vasodilators, and studies have linked them to diminished flush responses (27, 131). However, it is not fully understood how they are reduced in patients with schizophrenia. In addition, niacin is an antioxidant in many diseases and has a high affinity for its receptor, GPR109A (132–134). It is not well understood why niacin binding to GPR109A is ineffective in lowering the levels of pro-inflammatory mediators observed in schizophrenia. This indicates that there are other potential mediators associated with this aberrant response. This section will discuss (Figure 8) and explore inflammation involvement with the cellular mechanism behind the diminished flush response. It explores the link between the GPR109A-COX-prostaglandin pathway and inflammatory mediators, all of which are relevant to cellular biology behind diminished flush, signal transduction, and inflammation.
Lipid Peroxidation and Inflammation
Membrane phospholipids contain polysaturated fatty acids (PUFAs), which have a high content of n-6 arachidonic acid (AA) (135). PUFAs contain phosphatidylethanolamine (PE), phosphatidylserine (PS), phosphatidylcholine (PC), and phosphatidylinositol (PI) (136). An inflammatory phospholipid, lysophosphatidylcholine (LPC), is generated when cPLA2 cleaves the acyl ester bond of PC (137). LPC uses ATP-gated P2X7 receptor (P2X7R), which is abundant in microglia, to induce IL-1B, IL-18, ROS, and NOS and activate microglia (138). PUFA exposure to oxidative stress is called lipid peroxidation, which induces ROS (139). NOS, ROS, and RNS activate pro-inflammatory mediators, NF-kB, and AP-1 (180) and mediate GSH deficiency (72). The inflammatory imbalance activates NF-κB. Active NF-κB can activate AP-1, which regulates the transcription of Jun and Fos, which are responsible for cell growth and differentiation (140, 141). In contrast, transcription factors may be regulated by ROS-stimulated MAPK (142). This means that the transcription factor may be controlled by MAPK independent of the oxidative species. HNE, a biomarker of lipid peroxidation, has been observed to activate both NF-κB, AP-1, and c-Jun expression, and cell signalling pathways, JNK and p38, when exposed to ROS (143, 144, 180). Therefore, pro-oxidants activate HNE-induced activation of the cell signalling pathway.
(15d-PGJ2) and (PPARγ) in Anti-inflammation
15d-PGJ2 increased the transcriptional activity of PPARγ. This downregulates the pro-inflammatory markers, COX-2, iNOS, AP-1, Stat-1, NF-kB, TNF-α, IL-1β, and PGE2, and increases antioxidant enzymes, hemeoxygenase-1 (HO-1) and GSH by PPARγ and 15d-PGJ2, respectively. PPAR-y and 15d-PGJ2 negatively regulate microglial activation and prevent neuronal apoptosis (145–153). NF-κB may be activated by ROS, cytokines, JNK (154), AP-1, and COX-2 (155). 15d-PGJ2 participates in the feedback mechanism (156) by PPARy, which inhibits activated NF-κB by increasing IKB expression (157, 158). PPAR-y activates antioxidant enzymes such as SOD, HO-1, and GSH to reduce ROS.
Transduction Signal Role in GPR109A Components
Gi, GRK2, and B-arrestin 3 are important for receptor internalisation (159). Upon activation of the GPR109A receptor by niacin, the Gi subunit is released from the GBY subunit, followed by desensitisation, which catalyses and phosphorylates the activated receptor by G protein-coupled receptor kinase (GRK2). Activated GPR109A promotes translocation and binding of B-arrestin 3 to the plasma membrane, resulting in receptor internalisation (159). Gi is involved in GRK2 recruitment to phosphorylate the C-terminus of GPR109A and subsequent ERK1/2 activation (160, 161). Phosphorylated ERK1/2 has been observed to potentiate GRK2 activity, resulting in the inhibition of leukocyte migration. In comparison, p38 blocks GRK2 function and facilitates cell migration (162, 163). The ERK pathway uses GRK2 to activate GPR109A; conversely, the ERK pathway is GPR109A independent, when activating B-arrestin 1. B-arrestin 2 phosphorylates and activates JNK3 in endosomes (164). It has also been observed that disrupted, ubiquitinated B-arrestin 2 promotes NF-κB signalling (165). ERK has been associated with B-Arestin 1, whereas it may be inferred that B-arrestin 2 may be associated with the JNK pathway, as it is both a precursor for c-Jun and an activator of NF-kB.
Function of Enzymes in Diminished Flush Response and Inflammation
Phosphorylated cPLA2a releases AA to induce pro-inflammatory markers, NADPH oxidase, superoxide, PGE2, INOS expression, and NO production, which activate microglia cells (166, 167). AA release produces ROS as a by-product, which activates JNK, NF-κB, TNF-α, and IL-1 to further activate COX-2 (168–171). Overactive COX-2 increases pro-inflammatory, iNOS, PGE2, nitric oxide, and peroxynitrite anions, which attack membrane phospholipids and lower their antioxidant defence (172). There was a synergistic effect between COX-2 and PGE2 expression; an increase in one would increase the expression of the other. PGE2 acts as a pro-inflammatory mediator and increases M1 microglial activation by increasing COX-2, IL-1B, and IL-6 levels (173–176). Active PGE2 activates the EP2 receptor, which increases cAMP production and activates cAMP response element-binding protein (CREB), which is responsible for increasing COX-2 expression (177–179). Different receptors induce different functions; for example, EP2 receptors regulate TNF-α, whereas EP4 receptors mediate IL-1B secretion (173). JNK inhibitor is known to reduce COX-2 expression, mediated by IL-1B, and it may be questioned whether this is also mediated through the EP4 receptor. H202 partially activates JNK (180) and AP-1 protein (181) to increase c-Jun and c-Fos (182) and resulting in cell apoptosis.
Phospholipid Abnormality
The membrane phospholipid hypothesis suggests that the abnormality observed in schizophrenia may be due to altered phospholipid metabolism (183, 184). LPC levels are disrupted in schizophrenia (185–187). LPC inflammatory activity is controlled by NLRP3 and NLRC4 genes (110).
Fatty Acid Abnormality
Fusar-Poli and Berger (188) showed reduced PUFA levels in patients with schizophrenia. PUFA is responsible for both membrane fluidity and its ligand-receptor interaction; it increases the concentration of receptors in the membrane and allows the ligand to interact with the receptor (189). Disrupted ligand-receptor interaction might be a reason for the reduced binding between GPR109A and its ligand, niacin, and therefore, its inability to release PGD2 and PGE2, resulting in a diminished flush response. Niacin has anti-inflammatory properties, and less exposure to niacin may contribute to the inflammatory imbalance observed in schizophrenia. Smesny et al. (190) suggested that structural changes observed in grey matter may be due to lipid membrane alterations, and that antipsychotics may influence lipid metabolism. A meta-analysis (191) showed that PUFA supplement intake and omega-3 or 6 reduced TNF-α levels and delayed onset of illness in ultra-high-risk patients with schizophrenia (192).
Biomarkers of Lipid Peroxidation
Lipid peroxidation is described as an oxidant that attacks PUFAs by inserting oxygen into the carbon-carbon double bond and altering the membrane structure (193). Lipid peroxidation can form secondary products such as malondialdehyde (MDA), propanal, and 4-hydroxynonenal (4-HNE) (91, 194). It has been observed that 4-HNE at low levels is metabolised, and therefore maintains a homeostatic environment, but at high levels, it can cause cell death and damage cell signalling proteins (195). HNE increases intracellular calcium levels in neurons (196), which may activate MAPK proteins, activate the COX pathway, or induce neuronal toxicity (197). Uchida et al. (180) confirmed that JNK is an important signalling mediator in cellular defence against toxic products generated from lipid peroxidation. MDA is a specific biomarker for lipid peroxidation in omega-6 fatty acids (198). MDA exposure alters membrane fluidity, resulting in the loss of membrane integrity (199). However, there is a heterogeneous distribution of MDA in schizophrenia, which may be due to confounders such as antipsychotics, which were not separated in the study (200). The sensitivity of biomarkers can also be an issue when measuring lipid peroxidation. There have been reports of increased F2-isoprostane (201) and microRNAs (miRNAs) in schizophrenia (202–205), which are more sensitive biomarkers of lipid peroxidation (201, 206–208).
Arachidonic Acid
Glen et al. (209), McNamara et al. (210), and Yao et al. (211) reported AA depletion in red blood cells (RBCs) in patients with schizophrenia. There is a controversy about the cause of the depleted AA; some researchers suggest that it may be due to niacin blunted response (212), whereas others would argue that niacin blunted response has been observed at normal AA levels, and instead may be due to disrupted AA metabolism (213). Skosnik and Yao (11), Horrobin (214), and du Bois et al. (215) suggested that oxidative stress reduces AA levels and modifies the signal transduction pathways to cause neuronal damage, as observed in schizophrenia. Cao et al. (216) and Covault et al. (217) reported that increased long-chain fatty acid-CoA ligase, type 4 (FACL4) activity as a result of genetic mutation leads to more rapid sequestration of free AA, resulting in reduced AA.
AA and JNK
In phagocytic cells, AA translocates activated rac from the cytosol to the membrane to activate NADPH oxidase and activate JNK, respectively (218–220). However, it has been observed that JNK activation is independent of AA metabolism. Minden et al. (221) showed that the antioxidant N-acetylcysteine blocked two-thirds of AA-induced JNK activation. It may be inferred that activated JNK is more dependent on oxidative species than AA.
Prostaglandin
A systemic imbalance of pro-inflammatory and anti-inflammatory prostaglandin levels has been reported in patients with schizophrenia (222). This imbalance may be associated with altered mediators involved in the niacin-GPR109A-COX pathway. The degradation of phospholipid membranes into eicosanoids results in the production of free radicals, which may contribute to the imbalance (223).
PGD2 and PGE2
Morrow et al. (224) used gas chromatography-mass spectrometry to detect large levels of PGD2 and its metabolite 9a,11 β-PGF2 following oral niacin. However, (225, 226) suggested that flushing is strictly related to PGE2. Furthermore, (227) suggested that increased cAMP production by their receptors, DP1, EP2, and EP4, contributes to flushing. However, Wise et al. (228) countered earlier studies by showing that DP1 and EP2 receptor knockout showed 40 and 20% reduced flushing, respectively. In addition, laropiprant, which is an antagonist with high selectivity for DP1, showed reduced flushing when compared to placebo, but 70% of the time, the participants still had flushes (229). This suggests that PGD2, PGE2, and their receptors are important in the flushing response, but partially contribute to its effect.
Moreover, PGE2 is synergistic with COX-2 to activate microglia (173–176), and active microglia can damage neurons. COX-2 inhibitors serve as neuroprotectants by reducing PGE2 levels (230). High concentrations of PGD2 have also been observed to be neurotoxic (231, 232). This is interesting because the diminished flush effect resulted in low PGD2 levels. PGD2 exerts anti-inflammatory properties through PPAR-Y; therefore, it may be suggested that high PGD2 would be beneficial for cells. Furthermore, Liang et al. (233) cleared our understanding by stating PGD2 concentration of 1 nM-1 μM, and PGE2 at concentrations of 0.01–1 μM are neuroprotective.
PGE2 Level Controversy
Cytosolic PGE2 levels were observed to be reduced in the temporal cortex of patients (234). Other studies have suggested that PGE2 levels (64, 235–238). Pierre et al. (239) and Quraishi et al. (240) showed that PDE2 can be modulated by peroxisome proliferator-activated receptor γ (PPARy), a nuclear receptor stimulated by prostaglandin J2 (PGJ2). As PGE2 is a pro-inflammatory mediator, this may suggest that PPARy may regulate both pro- and anti-inflammatory properties based on its interaction with the prostaglandin type. A recent study, which considered the acute phase of schizophrenia, eliminated potential confounders such as drug dependency, alcohol consumption, development delay, and dementia, and matched patients based on their age, sex, marital status, education, and onset of illness, confirmed that there are lower serum levels of PGE2, 15d-PGJ2, and PPARy levels in patients (241). In contrast, Martínez-Gras et al. (222) showed reduced levels of 15d-PGJ2, PPARy, and IkBa, but increased levels of PGE2. However, participants in the study had been using antipsychotic drugs and did not match the severity of the illness. The variation in PGE2 levels may depend on the severity of illness and the use of antipsychotic drugs.
PPARy and 15d-PGJ2 Role
PGD2 can be degraded non-enzymatically to form a J-series, 15-deoxy-Δ12, 14-PGJ2 (15d-PGJ2), which binds to PPAR-γ (242, 243). 15d-PGJ2 is a cyclopentenone prostaglandin, which reportedly exerts anti-inflammatory effects on microglia (150). 15d-PGJ2 is the first endogenous ligand of PPAR-γ. PPAR-γ plays an important role in lipid metabolism, inflammation, proliferation, and differentiation of cells. Furthermore, PPARy is considered a negative regulator of activated macrophages, and can stimulate or inhibit 15d-PGJ2 gene expression by altering transcription factors, AP-1, STAT, and NF-kB (148, 158). To reverse macrophage activation, transcription factors are downregulated by PPARγ. PPARy regulates the relationship between microglia and neurons by modulating cytokines IL-18 expression in microglia, which has an inhibitory effect on LTP. PPARy agonist reverses IL-18 mediated attenuation of LTP by enhancing synaptic plasticity (148, 244). JNK inhibitors are also known to act as PPARy agonists, supporting their anti-inflammatory role (245–248).
G-Coupled Receptor
PUMA-G in mice is an orthologue of the human GPR109A receptor. Mice lacking PUMA-G did not release PGD2 or PGE2, and therefore, did not show flushing (35). The alteration of receptor components has been associated with diminished flush. B-arrestin is used for cell signalling, receptor desensitisation, and internalisation (249). Internalisation is involved in receptor desensitisation and signalling, and contributes to the diversity of GPCR-dependent signalling (250). B-arrestin1 is a biassed agonist because it may induce a flushing response independent of the GPR109A receptor by increasing cPLA2 phosphorylation, while depletion of B-arrestin1 reduces activated cPLA2 (249). B-arrestin2/3 was significantly reduced in the schizophrenia group compared to that in the control group. Furthermore, reduced GRK in the frontal cortex was observed in both younger and older patients with schizophrenia. However, Bychkov et al. (251) observed a difference in GRK levels in both young and older patients with schizophrenia compared to controls. In young patients with schizophrenia, GRK3 had been reduced, whereas in the older schizophrenia group, GRK6 showed the greatest reduction. It may be inferred that disrupted B-arrestin or GRKs may result in diminished flush response, and confirmed that age is an important factor in schizophrenia.
Enzymes
Enzymes are biological catalysts that convert essential fatty acids to prostaglandins in the GPR109A-COX-prostaglandin pathway. Horrobin (252) suggested that one of the factors behind diminished flush was dysfunctional enzyme activity, which contributes to reduced prostaglandin levels. Furthermore, the GPR109A flushing response can be ablated by inhibiting PLA2 and COX-1/COX-2 activity (253). Figures 9, 10 shows the profiles for the PLA2 and COX families, respectively.
PLA2
Controversy in Phospholipase Activity
There is increased PLA2 activity in the cortex and thalamus in patients with first-onset schizophrenia (190). This study provides an insight that PLA2 activity is dependent on the stage of illness, and its activity may vary based on the brain region and use of medication. However, the study has limitations, as it did not indicate which PLA2 activity is being measured, as different PLA2 have different functions and activities.
Dr. Horrobin's membrane hypothesis suggests that elevated levels of calcium-dependent cytosolic group IVA PLA2a (cPLA2a) observed in schizophrenia are responsible for the depletion of AA (183). Messamore et al. (288) and Kim et al. (289) reported an increase in intracellular calcium concentration, which may result in increased cPLA2 activity. Instead, (290–293) suggested that there is increased iPLA2 and decreased cPLA2 activity in patients with schizophrenia. The iPLA2 may be increased as negative feedback by producing an antioxidant that mediates increased oxidative stress, as observed in schizophrenia patients (294–296). The reduced cPLA2 has a higher preference for cleaving AA, which may explain the reduced AA levels in patients with schizophrenia. It may be concluded that the variation in cPLA2 activity may be due to confounders such as age, medication, disease stage, ethnicity, and other medical status which induce pro-inflammatory and anti-inflammatory imbalances.
cPLA2, JNK and Its Effect on Cells
Phosphorylation of Ser505, Ser515, and Ser727 activates cPLA2 (297, 298). Activated cPLA2 cleaves AA and induces the production of inflammatory mediators such as eicosanoids (299–301). There are insufficient studies regarding Ser515 and Ser727 and their effect on cPLA2. However, phosphorylation of ser505 on cPLA2a increases phospholipase binding to membrane phospholipids at low calcium concentrations, altering the PLA2 conformation to ensure a better fit to the catalytic domain of membrane phospholipids (298). Some studies have suggested a relationship between MAPK and cPLA2 activity. However, in macrophages, there have been inconsistent reports of ERK1/2 and p38 links in phosphorylating cPLA2 at ser505 (302–304). Casas et al. (305) used MAPK inhibitors for ERK, p38, and JNK and found that only the JNK inhibitor effectively blocked cPLA2a phosphorylation in macrophages. This advances our understanding of the prominent role of JNK in cPLA2a phosphorylation in macrophages. Microglia are resident macrophages of the brain, which share similar functional and morphological properties to macrophages (306), therefore it may be inferred that microglia would have similar effects. However, there is no study linking MAPK and cPLA2a to neurons, although from our understanding of how microglia and neurons influence each other, there is a possibility that alteration in cPLA2 activity in microglia might affect neuronal functions. Furthermore, it has been observed that cPLA2 and dopamine are inversely related (307), where increased dopamine levels reduced cPLA2. The mechanism is not understood properly, but studies have shown that dopamine and glutamate alternation have specifically affected cPLA2 mediated AA release, but not mediators downstream of AA (289, 308).
COX
Activators of COX
PGD2, PDE2 mediated by COX-1 and COX-2, play an important role in the flushing response (35, 228). COX-2 knockout reduces both pro-inflammatory, PGE2, and NF-kB (309–311). Deng et al. (312) suggests that overexpression of COX-2 activity has been associated with increased histone acetyl transferase (HAT) and p300 gene, which is located near the NF-kB promoter, deletion or suppression of these transcriptional activators, and reduced COX-2 expression. Future studies need to investigate the link between HAT, p300, and COX-2 overexpression in schizophrenia. Ultimately, IL-1B is a potent inducer of COX and induces the synthesis and activity of PLA2 in cells (313). Therefore, it may be used as a target to control both the activation levels of COX and PLA2 by JNK.
COX in Microglia
COX-2 is important for producing inflammatory responses, which can activate microglia (314). During prostaglandin production via the COX pathway, ROS are generated as a by-product, along with the production of inflammatory agents such as cytokines and oxidative stress (282), all of which contribute to microglial activation.
Inhibitors of COX-2 Expression
When there is a high inflammation level, antipsychotics are less effective in reducing psychosis (315, 316). COX-2 overexpression has been linked to cognitive deficits in schizophrenia; COX-2 inhibition has been shown to have therapeutic effects, particularly when administered in the early stage of the disease (317–324). Mattson et al. (325) Weggen et al. (326), and Morihara et al. (327) suggested that nonsteroidal anti-inflammatory drugs (NSAIDs) regulate NF-κB and can serve as a therapeutic target for several psychiatric disorders. Nitta et al. (319) observed that NSAID celecoxib and risperidone are more beneficial in patients than the administration of antipsychotic risperidone alone. Niederberger et al. (328) and Tegeder et al. (329) showed that patients who used both NSAIDs and antipsychotic drugs had a higher psychotic relapse rate. These reports suggest that NSAIDs may play a controversial role in upregulating COX-2 expression, instead of downregulating COX-2. Harris et al. (330) theory on COX-2 as a double agent may influence the role of NSAIDs or COX-2 inhibitors. COX-2 can also participate in both pro-inflammatory and anti-inflammatory effects. During the development of inflammation, pro-inflammatory (via PGE2), but anti-inflammatory (via PGD2 and 15d-PGJ2) during resolution. Therefore, there is a chance that COX-2 inhibitors may instead inhibit anti-inflammatory properties, therefore, exacerbating schizophrenic symptoms. Therefore, alternative methods should be explored to ensure the selective downregulation of overactive COX-2 expression.
Increased COX-2 expression is dependent on MAPK activation (331). Yang et al. (332) showed that IL-1B induction is responsible for elevated COX-2 expression in hippocampal neurons. Rösch et al. (331) showed fibroblasts released PGE2 when stimulated with IL-1B, were also found to have overexpressed COX-2 and defective JNK signalling. To confirm this finding, the JNK inhibitor, SP600125, along with IL-1B, lowered both PGE2 and COX-2 expression (333–336). It may be inferred that schizophrenia patients with overexpressed COX-2 may present with increased levels of pro-inflammatory mediators. Therefore, to maintain inflammatory balance, the JNK inhibitor SP600125 may be administered, which may downregulate pro-inflammatory mediators. Other inhibitors such as glucocorticoids and minocycline have been shown to downregulate AP-1 or NF-κB in microglial cells and protect against neurotoxicity, while improving cognitive and negative symptoms of schizophrenia (337, 338).
Hydroperoxide
Stimulated hydrogen peroxide produces NADPH oxidase, otherwise known as phagocytic oxidase (PHOX), which converts microglia to an activated or cytotoxic state (339).
Exosomes
Exosomes transmit genetic information between cells, and miRNAs are found inside exosomes. These exosomes can be secreted by neurons or astrocytes (340). These exosomes circulate around the body to nearby and distant cells (341). Exosomal miRNAs have also been shown to be involved in the inflammatory response (342). A recent study found an association between dysregulated exosomes and schizophrenia (343). Du et al. reported a pattern between dysregulated exosomes and glycerophospholipid metabolism. The relationship between exosomes and GPR109A receptor should be investigated in future studies.
Genes
Schizophrenia is caused by the cumulative effects of risk variants in over 100 genes (45, 344). Most these genes are associated with neurons, neurotransmitters or synaptic plasticity (345–347). Table 1 attempts to match the current GWAS for schizophrenia with genes which may be involved in the diminished flush response. A negative result may be a false negative, whereas a positive match may be false positive. As observed in the table, GPR109A has been a match, which may suggest that risk variants in GPR109A may contribute to the aetiology of schizophrenia, as well as to an abnormal flushing response. GPR109A showed a positive match, indicating genetic mutation. This matched with the review analysis which suggested that there is an alteration in the receptor protein conformation and components, B-Arestin and GRK. We would have expected alternation in cPLA2 and COX-2, as there had been strong evidence in this review suggesting alterations in its genetic, protein expression, and activity. The dual role of PPARG in inflammation and its reduced expression in patients with schizophrenia would make it a good target. We would not expect much alteration in prostaglandin enzymes and receptors, as strong evidence suggests that they do not significantly contribute to the flushing response.
Table 1.
Gene | Aliases for gene | (GRCh37/hg19) | 128 GWAS Chr. position |
---|---|---|---|
HCAR2 | Hydroxycarboxylic Acid Receptor 2 (GPR109A) | chr12:123,185,840–123,187,904 | Yes |
PLA2G4A | Phospholipase A2 Group IVA (cPLA2) | chr1:186,798,032–186,958,113 | No |
PLA2G6 | Phospholipase A2, Group VI (iPLA2) | chr22:38,507,502–38,601,697 | No |
PTGS1 | Prostaglandin-endoperoxide Synthase 1 (COX-1) | chr9:125,132,824–125,157,982 | No |
PTGS2 | Prostaglandin-endoperoxide synthase 2 (COX-2) | chr1:186,640,923–186,649,559 | No |
PTGDS | Prostaglandin D2 Synthase | chr9:139,871,956–139,879,887 | No |
PTGES2 | Prostaglandin E Synthase 2 | chr9:130,882,972–130,890,741 | No |
PEGER2 | Prostaglandin E Receptor 2 | chr14:52,781,016–52,795,324 | No |
PTGER4 | Prostaglandin E Receptor 4 | chr5:40,679,600–40,693,837 | No |
PPARG | Peroxisome Proliferator Activated Receptor Gamma (PPAR-y) | chr3:12,328,867–12,475,855 | No |
Conclusion
This review shows altered cellular pathology behind a diminished flush response. First, diminished flush is not only caused by vasodilators, but also by altered protein expression, protein activity, and inflammatory imbalance. Altered protein levels in the GPR109A-COX-prostaglandin pathways include membrane phospholipids, GPR109A, enzymes, cPLA2 and COX-2, and prostaglandins with their receptors and downstream products, such as PGD2, PGE2, DP1, EP2, EP4, 15d-PGJ2, and PPAR-y. Furthermore, we found that there was an inflammatory imbalance in the flush response. Although there is a possibility of genetic alteration in GPR109A, it is possible that environmental factors, such as oxidative stress, may alter receptor conformation, causing reduced receptor-ligand bonds, resulting in diminished flush. Second, as patient demographics interfere with the flush effect, future studies should consider the age, illness stage, ethnicity, use of antipsychotics, and presence of health comorbidities in their participants. The niacin skin flush test is essentially used to diagnose patients at their prodromal stage; however, this review contains limited research on the altered cell pathology at the prodromal stage. This review well supports the evidence for M1 microglia activation; however, evidence on neurons is weak, as there is no direct evidence linking diminished flush response to neurons. Given that microglia and neurons share a bidirectional relationship, it is likely that M1 activation may indirectly influence neuronal apoptosis. Lastly, JNK inhibition can inhibit M1 activation, neuronal apoptosis, and reduce inflammatory mediators, NF-κB, IL-1B, and TNF-α, and influence protein phosphorylation or expression, cPLA2, COX-2, and PPAR-y, respectively. Although further investigation is required to understand whether ROS-mediated JNK may influence GPR109A, we believe that the ability of JNK to control multiple targets in the diminished flush response would make it a good therapeutic target for schizophrenia. Future research should investigate whether stimulation of GPR109A results in PGD2 or PGE2 release from microglial cells and whether this is mediated by the JNK pathway. Future research should also bear in mind that Table 1 has established a match with 128 GWAS, which may be essential for the updated GWAS for schizophrenia in the future.
Author Contributions
The author confirms being the sole contributor of this work and has approved it for publication.
Acknowledgements
I would like to thank my Supervisor, Dr. Brian Morris for his support and guidance which has enabled me to complete this review.
Conflict of Interest
The author declares that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.
Publisher's Note
All claims expressed in this article are solely those of the authors and do not necessarily represent those of their affiliated organizations, or those of the publisher, the editors and the reviewers. Any product that may be evaluated in this article, or claim that may be made by its manufacturer, is not guaranteed or endorsed by the publisher.
Supplementary Material
The Supplementary Material for this article can be found online at: https://www.frontiersin.org/articles/10.3389/fpsyt.2021.771144/full#supplementary-material
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