Activation of GPR39 with TC-G 1008 attenuates neuroinflammation via SIRT1/PGC-1α/Nrf2 pathway post-neonatal hypoxic–ischemic injury in rats

Hypoxic–ischemic encephalopathy (HIE) is a severe anoxic brain injury that leads to premature mortality or long-term disabilities in newborns, such as cerebral palsy, cognitive deficits, and mental retardation [1–3]. HIE contributed to 23% of neonatal deaths globally and has an incidence of 26 per 1000 live births in developing countries [4, 5]. The established standard of treatment for HIE is therapeutic hypothermia, but it can only provide limited neuroprotection [6]. In recent years, researchers have focused on finding new therapies to improve efficiency, enhance neuroprotection, and reduce side effects. For example, some peptides, activated by severe anoxic injury, might be involved in perinatal HIE’s pathophysiology and could be the potential therapeutic target for HIE.

As one of HIE pathophysiology’s main events, inflammatory responses take place within minutes post-HIE injury and mediate secondary neuronal death [7, 8]. The activation of neuroglial cells promotes the release of a large number of pro-inflammatory cytokines and reactive oxygen species (ROS), thereby leading to neuronal apoptosis. On the other hand, emerging evidence has demonstrated that inflammatory responses also play a beneficial role, and anti-inflammation is also one of the present neuroprotective agents’ main mechanisms. Activated microglia/macrophages can induce phagocytosis and the production of anti-inflammatory cytokines, which inhibits neuroinflammation and protects remaining viable neurons from death [9–12].

G-protein-coupled receptor 39 (GPR39), a plasma membrane G-protein-coupled receptor, was first cloned and identified in 1997 [13]. GPR39 is expressed in the gastrointestinal tract, amygdala, hippocampus, and auditory cortex, and zinc was thought to be a natural ligand of GPR39 [14, 15]. Activation of GPR39 and related subsequent signaling cascade has been identified in several cells and shown to regulate a vast array of physiological functions, such as proliferation, differentiation, ion transport and tight junction formation [16]. Moreover, activation of GPR39 has been demonstrated to promote wound healing, ameliorate symptoms of inflammatory bowel diseases, dampen epileptic seizure activity, reduce anxiety-like behaviors and regulate insulin secretion and malignant progression of several cancers [17–24]. Recently, accumulating in vitro evidence demonstrated that GPR39 exhibits anti-inflammatory activity by reducing the expression of pro-inflammatory cytokines (IL-1β, IL-6), enhancing anti-inflammatory cytokines production (IL-10), ameliorating oxidative stress and mitochondrial dysfunction [25–27].

A small amount of literature confirms that GPR39 might play a neuroprotective role in neuronal injury by inhibiting apoptosis and ameliorating endoplasmic reticulum stress [28–30]. However, whether GPR39 activation has protective and anti-inflammatory effects post-HIE remains unexplained. In the present study, we hypothesized that GPR39 agonist, TC-G 1008, attenuates inflammation via sirtuin 1(SIRT1)/PPARG coactivator 1 alpha (PGC-1α)/nuclear factor, erythroid 2 like 2(Nrf2), leading to improvement of neurological function in a rat model of neonatal HIE.

In order to further explore the role of signaling pathway proteins in the anti-neuroinflammatory effect of TC-G 1008, SIRT1 inhibitor EX527 and PGC-1α CRISPR were used.

The results showed that EX527 abolished the effects of TC-G 1008, resulting in a decrease in PGC-1α and Nrf2 expression, and an increase in IL-6, IL-1β and TNF-α expression. Similarly, PGC-1α CRISPR significantly decreased PGC-1α expression, thereby abolishing the effects of TC-G 1008, resulting in a decrease in Nrf2 expression, and an increase in IL-6, IL-1β and TNF-α expression.

The trend of the western blot results of inflammatory factors was consistent with the findings of our immunofluorescence staining of IL-1β and MPO.

In this study, we aimed at evaluating the anti-inflammatory effects and the potential underlying mechanisms of GPR39 in a rat model of neonatal HIE. Our findings demonstrated that (1) the expression of GPR39 and pathway-related proteins, SIRT1, PGC-1α and Nrf2 were increased in a time-dependent manner, peaking at 24 h or 48-h post-HIE. (2) GPR39 was expressed in microglia at 48-h post-HIE. (3) Intranasal administration of TC-G 1008 (15 mg/kg) reduced the percent infarcted area and improved short-term and long-term neurological deficits. (4) TC-G 1008 attenuated neuroinflammation in part via the SIRT1/PGC-1α/Nrf2 pathway in a rat model of neonatal HIE.

In the central nervous system (CNS), it has been previously demonstrated that high GPR39 mRNA levels are present in the amygdala, hippocampus, and auditory cortex [15], with Zn²⁺ identified as the “physiological agonist” of GPR39 [39]. Extracellular Zn²⁺ activates ZnR/GPR39 receptor, thereby triggering multiple signaling pathways including, Gαs and Gαq/PLC/IP3 [40]. Previous studies indicated that a zinc-deficient diet led to the decreased expression of GPR39, and zinc supplementation for 4 weeks, significantly abolished the abnormal expression of GPR39 in the hippocampus [41]. Previous studies have reported that post-ischemia, neurons massively release extracellular Zn²⁺ to promote the production of pro-inflammatory cytokines [42]. In this study, we demonstrated that the expression of GPR39 was increased in a time-dependent manner post-HIE. Thus, the release of Zn²⁺ from neurons post-HIE may have led to the up-regulation of GPR39 expression that we observed.

As a specific agonist of GPR39, TC-G 1008 is widely used to explore the effect of GPR39 activation [25, 43, 44]. Previous studies have shown that treatment with TC-G 1008 (100 nM and 1 μM) enhanced keratinocyte proliferation through an ERK-dependent pathway [45]. Furthermore, TC-G 1008-mediated GPR39 activation promoted osteoblast differentiation and mineralization [43]. In a study where they investigated the effect of GPR39 on the intestinal barrier function, treatment with TC-G 1008 (1–10 μM) enhanced tight junction assembly in intestinal epithelial cells by PLC-CaMKKβ-AMPK pathways [46]. The expression of GPR39 in the hippocampus and hippocampal cells (HT-22) was upregulated following administration of TC-G 1008 [21, 28]. Advanced glycation end-products reduced GPR39 expression in a dose-dependent manner and TC-G 1008 reversed the effects of AGEs [47]. In this study, GPR39 was upregulated post-TC-G 1008 administration as seen from our immunofluorescence staining and mechanism studies, which is consistent with previous studies.

GPR39 plays an important role in wound healing, depression, inflammatory bowel diseases, alcohol use disorder, insulin secretion and several cancers [23, 46, 48–52]. However, the neuroprotective function of GPR39 has been partially confirmed. Studies have shown that GPR39 overexpression protected cells from undergoing cell death in a hippocampal cell line, and revealed its underlying mechanisms involving apoptosis and endoplasmic reticulum stress [29]. In another study, GPR39 exhibited its neuroprotective role by inhibiting apoptosis and thus protecting hippocampal neurons (HT-22) from corticosterone-induced injury [28]. Furthermore, it was observed that the zinc diet-treated group increased the expression of GPR39 and BMP protein, and improved cognitive impairment, while it showed to decrease hippocampal mossy fiber regenerative sprouting [41]. Therefore, GPR39 has been proposed as a potential therapeutic target for ischemia/reperfusion injury and neurodegenerative diseases [29]. In the present study, low and medium dose of TC-G 1008 showed to significantly reduce the percent infarcted area compared to vehicle group (Fig. 2A, B). In addition, medium dose of TC-G 1008 significantly reduced HIE-induced body weight loss of rat pups (Fig. 2E). As shown in rats’ performance in behavioral tests, TC-G 1008 improved long-term neurological function (Fig. 4). The behavioral tests were selected based on the neurological function that was being assessed. Negative geotaxis was used to evaluate reflex development, motor skills and vestibular labyrinth, and cerebellar integration, while righting reflex was used to reflect the muscle strength and subcortical maturation [53]. The rotarod test was used to assess the motor coordination of rodents and is especially sensitive in detecting cerebellar dysfunction [54]. The number of foot-faults indicates impaired movement correction and increased reaction time [55]. Morris water maze test was used to assess learning, memory, and visual ability. In general, activation of GPR39 with TC-G 1008 reduced the percent infarcted area and improved short-term and long-term neurological deficits.

Although the underlying mechanism is not completely understood, inflammation is one of the main contributors to the pathogenic cascade post-HIE. Hypoxia–ischemia initiates the inflammatory reaction in the brain parenchyma and the peripheral immune system, which mediates secondary brain injury and can last for a few days [7, 8]. Therefore, new agents that target inflammation will open new avenues for therapy of neonatal hypoxic–ischemic brain injury. GPR39, a recently discovered zinc-sensing receptor, has been proven to have anti-inflammatory effects in several studies [25–27, 56, 57].

GPR39 mediates synovial inflammation by ameliorating the expression of pro-inflammatory cytokines such as IL-βand IL-6 [25]. In the process of GPR39 regulating the activity of endothelial cells, Zn + is involved in the regulation of some inflammation-related key molecules including heme oxygenase-1, selectin L and IL-10 [56]. GPR39 was upregulated in thioglycollate-induced peritoneal macrophages and exerted its anti-inflammatory effects by increasing the production of IL-10 [27]. It has been shown that treatment with TC-G 1008 abolished the increased expression of pro-inflammatory cytokines induced by ox-LDL in the prevention of atherosclerosis [26]. However, in the process of promoting wound healing, the activation of GPR39 has the effect of promoting inflammation by increasing the production of pro-inflammatory cytokines IL-6 [57]. In the present study, we first discovered its anti-inflammatory effect in the brain by reducing the production of IL-6, IL-1β and TNF-α, as showed from the result of immunofluorescence staining of MPO and IL-1β and western blotting (Figs. 6, 7, 8, 9).

Numerous studies have shown that activation of SIRT1 is a neuroprotective agent for ischemic stroke through several mechanisms [58–61]. TC-G 1008 treatment mitigated IL-1b-induced inhibition of SIRT1, and the effect of TC-G 1008 on p53 acetylation and chondrocyte senescence were abrogated when SIRT1 was silenced [44]. Previous studies have indicated that PGC-1α was a major regulator of ROS metabolism and mitochondria biogenesis, which is closely related to the pathology of ischemic diseases and neurodegenerative diseases [62]. Several studies focusing on ischemic injury implied that the expression and activity of PGC1-α are at least partially dependent on SIRT1. Icariin has a neuroprotective effect in mice subjected to post-MCAO via increasing the SIRT1 and PGC-1a expression [63]. Ghrelin significantly attenuates brain damage post-HIE via the GHSR-1α/AMPK/Sirt1/PGC-1α/UCP2 signaling pathway [64]. Activation of the PGC-1α/Nrf-2/HO-1 signaling pathway plays a critical role in tannic acid (TA) administration against traumatic brain injury through reducing oxidative damage, mitochondrial impairment, and inflammation [65]. In addition, the expression levels of SIRT1 PGC1-a and Nrf2 were significantly up-regulated post-HIE [64, 66], which is consistent with the results observed in our study. The activation of GPR39 increased the expression of SIRT1, PGC-1α and Nrf2, and reduced the expression of pro-inflammatory cytokines (Fig. 7), but this effect was reversed by GPR39 CRISPR. EX527 and PGC-1α CRISPR abolished the effects of TC-G 1008, resulting in a decrease in PGC-1α and Nrf2 expression, and an increase in IL-6, IL-1β and TNF-α expression. Similar effects have also been observed in our immunofluorescence staining experiments of IL-1β and MPO. Therefore, the anti-inflammatory effect of GPR39 is partly dependent on the SIRT1/PGC-1α/Nrf2 signaling pathway post-HIE. The role of other neuroprotective functions and underlying mechanisms will need to be further investigated.

In conclusion, intranasal administration of TC-G 1008 reduced the percent infarcted area and improved short-term and long-term neurological deficits post-HIE. TC-G 1008 attenuated neuroinflammation in part via the SIRT1/PGC-1α/Nrf2 pathway in a rat model of neonatal HIE. TC-G 1008 may be a novel therapeutic target for treatment post-neonatal HIE injury. Activating GPR39 may be a promising therapeutic target to attenuate neuroinflammation post-neonatal HIE.

Not applicable.

This study was designed by SCX, DMD, JPT, and JHZ. The experiments were completed by SCX, HS, PJ, LG, RL, XH, and JX. SCX, XIJ, and LNZ performed the statistical analysis. SCX, XLJ, and LNZ finished writing the manuscript. LNZ, JPT and JHZ provided supervision and final check. All the authors read the final version of this paper and approved it. All authors read and approved the final manuscript.

This study was supported by grants from the National Institutes of Health (NS104083) to John H. Zhang, and a grant from Key Research and Development Project of Hainan Province (ZDYF2019147) to Shucai Xie.

The data supporting the findings of this study are available from the corresponding author upon reasonable request.

Lina Zhang, Email: zln7095@163.com.

John H. Zhang, Email: johnzhang3910@yahoo.com