Pyrrolidine Dithiocarbamate Prevents Neuroinflammation and Cognitive Dysfunction after Endotoxemia in Rats

Abstract

Systemic inflammation, for example as a result of infection, often contributes to long-term complications. Neuroinflammation and cognitive decline are key hallmarks of several neurological conditions, including advance age. The contribution of systemic inflammation to the central nervous system (CNS) remains not fully understood. Using a model of peripheral endotoxemia with lipopolysaccharide (LPS) we investigated the role of nuclear factor-κB (NF-κB) activity in mediating long-term neuroinflammation and cognitive dysfunction in aged rats. Herein we describe the anti-inflammatory effects of pyrrolidine dithiocarbamate (PDTC), a selective NF-κB inhibitor, in modulating systemic cytokines including tumor necrosis factor (TNF)-α and interleukin-1β (IL-1β) and CNS markers after LPS exposure in aged rats. In the hippocampus, PDTC not only reduced neuroinflammation by modulating canonical NF-κB activity but also affected IL-1β expression in astrocytes. Parallel effects were observed on behavior and postsynaptic density-95 (PSD95), a marker of synaptic function. Taken together these changes improved acute and long-term cognitive function in aged rats after LPS exposure.

Introduction

Inflammation is a critical risk factor in the development of neurological complications; neuroinflammation in particular has become a key hallmark of several conditions including neurodegenerative diseases and psychiatric illness (Lynch, 2010; Najjar et al., 2013; Heneka et al., 2015). Systemic perturbations, like infection, are known to affect the central nervous system (CNS) causing a constellation of symptoms referred to as “sickness behavior” (Dantzer, 2004). These events may predispose to significant complications, non-resolved inflammation, and persistent cognitive impairments especially to frail and elderly subjects (Perry et al., 2007; Cunningham et al., 2009). Microglia activation is a known hallmark of neuroinflammation (Lucin and Wyss-Coray, 2009) but other cell types in the CNS like astrocytes have been also implicated in inflammatory signaling and brain plasticity (Dong and Benveniste, 2001; Capani et al., 2016). During ageing, astrocytes demonstrate phenotypical changes that have been associated with cells that express a senescence-associated secretory phenotype (SASP; Campisi, 2005). These features include enhanced expression of glial fibrillary acidic protein (GFAP), increased expression of several pro-inflammatory cytokines, and a sustained low-level oxidative stress (Cotrina and Nedergaard, 2002; Salminen et al., 2011). Within the aged brain, astrocyte activation has been implicated with higher cytokines levels including tumor necrosis factor (TNF)-α, interleukin (IL)-1β, and IL-6 (Campuzano et al., 2009). These cytokines are known to interfere with neuronal function, synaptic plasticity, and memory processes (Henry et al., 2009; Cunningham, 2013).

In our previous work we reported a specific role for IL-1β and nuclear factor-κB (NF-κB) signaling in astrocytes causing long-term neuroinflammation up to day 30 after lipopolysaccharide (LPS) exposure (Fu et al., 2014). NF-κB is a crucial regulator of immunity (Karin and Lin, 2002) and an important nuclear transcription factor involved in SASP-associated inflammation and inflammatory signaling (Salminen et al., 2012). Phosphorylation of the IKKβ pathway is central to the canonical activation of NF-κB, thus allowing nuclear translocation and transcription of several inflammatory genes. Many of these genes, including TNF-α, IL-1β, IL-6, and cyclooxygenase-2 (COX-2) mediate neuroinflammation in a number of conditions (Shih et al., 2015). The aim of the current study was to evaluate the protective effects of pyrrolidine dithiocarbamate (PDTC), a well-described inhibitor of the canonical NF-κB signaling pathway with low-molecular weight and blood-brain barrier (BBB) permeability (Schreck et al., 1992; Ziegler-Heitbrock et al., 1993; Chabicovsky et al., 2010) on neuroinflammation and memory function after LPS exposure in aged rats. Several studies have described protective effects of PDTC through suppression of NF-κB translocation into the nucleus (Ohta et al., 2002; Hirata et al., 2007), yet the full therapeutic potential of PDTC in the context of neuroinflammation and immune-to-brain signaling pathway is poorly known. Based on the above, we hypothesized that PDTC, would improve memory outcome in aged rats. Overall, we demonstrate a key role for NF-κB inhibition in preventing systemic inflammation, prolonged neuroinflammation, and behavioral changes in the hippocampus of aged rats. PDTC pretreatment aside from reducing IL-1β up regulation in astrocytes also prevented changes in postsynaptic density-95 (PSD-95), a major scaffolding protein in the excitatory PSD, thus improving neurological function.

Materials and Methods

Animal

Male Wistar rats (20 months old) weighing 550–850 g were used in all the experiments. Rats were bred and maintained under standardized housing conditions with controlled temperature, humidity, and 12-h light/dark cycle. Standard food chow and water were provided ad libitum. The experimental protocol was approved by the Capital Medical University Biomedical Ethics Committee Experimental Animal Ethics Branch (Approval No. LA2012-38) and all efforts were made to minimize pain and suffering of the animals.

Rats were randomly separated into four groups:

• Vehicle control (0.9% NaCl i.p.),

• LPS (2 mg/kg i.p., 055:B5, Sigma, St Louis, MO, USA),

• LPS + PDTC (LPS + PDTC) (LPS and PDTC 30 mg/kg i.p., P8765, Sigma, St. Louis, MO, USA), and

• PDTC alone (30 mg/kg i.p.).

LPS dosing was based on previous work (Fu et al., 2014). PDTC was administered 1 h before LPS injection at a dose (30 mg/kg) shown to inhibit NF-κB activation (Cvek and Dvorak, 2007). Vehicle group received an identical volume of saline.

Sample Preparation

A cohort of rats was sacrificed at 0.5 h, 2 h, 6 h, 1 day, 3 days, 7 days, 15 days, and 30 days (n = 8 per time point per group) after LPS or saline injection. Under deep isoflurane anesthesia (Forene, Abbott Laboratories, Queensborough, UK) blood was taken from the inferior vena cava. Samples were allowed to clot for 2 h before centrifugation at 4°C for 20 min at 1000× g. Serum was collected and stored at −80°C.

Brains were rapidly dissected following decapitation. All dissections were performed on an ice-cold frosted glass plate. The entire brains (n = 4 per time point) were mounted in OCT compound (Sakura Finetek USA, Inc., Torrance, CA, USA), frozen in liquid nitrogen, and stored at −80°C for later immunofluorescence. The hippocampal tissues were isolated from the entire brains from the remaining batch (n = 4 per time point), frozen in liquid nitrogen, and stored at −80°C used for RT-PCR and ELISA analyses. The investigator was blinded to the tested groups for biochemical and behavioral analyses.

Immunofluorescence

Brains were processed on a freezing microtome (CM1850, Leica Microsciences, Mannheim, Germany) and consecutive 20-μm thick hippocampal coronal sections were selected from Bregma −2.30 and Bregma −3.60 according to the atlas by Paxinos and Watson. Briefly, sections were post-fixed in ice-cold 4% paraformaldehyde for 15 min and rinsed in PBS four times for 10 min each time. The sections were permeabilized using 0.3% Triton X-100 (Sigma-Aldrich, St Louis, MO, USA) for 1 h, blocked with 5% horse serum (8178102, Gibco) for 1 h at room temperature and then incubated with primary antibodies: goat anti-IL-1β IgG (1:100; catalog number AF-501-NA, R&D, Systems Inc., Minneapolis, MN, USA), rabbit anti-PSD-95 (1:100; catalog number 04-1066, Millipore, Billerica, MA, USA), rabbit anti-GFAP IgG (1:1000; catalog number Z0334; Dako), rabbit anti-IBA-1 IgG (1:500, catalog number 019-19741 Wako) and mouse anti-NeuN IgG (1:100; catalog number MAB360, Millipore) for 2 h at room temperature, and then overnight at 4°C. The sections were washed three times with PBS and incubated for 2 h with secondary antibodies: Alexa-594-coupled donkey anti-goat IgG (1:500; catalog number: A11058, Invitrogen), Alexa-594-coupled donkey anti-rabbit IgG (1:500; catalog number: A21207, Invitrogen), Alexa 488-coupled donkey anti-rabbit IgG (1:500; catalog number: A21206, Invitrogen), Alexa-488-coupled donkey anti-mouse IgG (1:500; catalog number: A21202, Invitrogen, Paisley, UK). Negative control sections in which primary antibodies or secondary antibodies were replaced by PBS showed no labeled cells. The nuclei of tissues were counterstained with Hoechst 33342 (1:1000; Roche, Mannheim, Germany). Sections from all time points were stained simultaneously to provide uniform conditions for subsequent quantitative analysis by fluorescence staining. Samples were analyzed with a confocal microscope (Leica TCS SP5, Leica, Benshein, Germany) and the rate of IL-1β positive expression in the GFAP-positive astrocytes of the hippocampal DG region were analyzed using Adobe Photoshop CS3V10.0.1.0. Mean gray values of PSD-95 were measured using an image analyzing software (Optimas 6.5, CyberMetrics, Scottsdale, AZ, USA). Ten visual fields were counted for each section, and 10 values of positive expression were counted and the mean value calculated by averaging the counts from the results of the three experiments at different time points (Fu et al., 2014).

mRNA and RT-PCR

Total RNA was extracted from the hippocampus using Trigol (NEP019-2, Dingguo Changsheng) and DNA contaminants removed by RQ1 RNase-free DNase (M610A, Promega). The integrity of total RNA was measured by agarose gel electrophoresis and cDNA was synthesized with Toyobo Reverse transcription Kit (including M-MLV and 5× RT Buffer) according to the manufacturer’s protocol (TRT-101, Toyobo). DNA amplification was carried out using Sybr Green I (10×) (GG1301-500UL, Genviw) for 35 cycles (each cycle consisting of denaturation for 30 s at 94°C, annealing for 30 s at 56°C or 47°C, extension for 30 s at 72°C). Primers used are described in Table 1. The fold expression in gene was determined by double-standard curves method of relative quantification PCR. Data are expressed as the relative level of the target gene in the hippocampus normalized to the endogenous control (GAPDH) and relative to the control group.

Enzyme-Linked Immunosorbent Assay

Isolated hippocampal tissues were homogenized in 100 mg tissue/ml RIPA Lysis Buffer (20-188, Millipore, MA, USA). Immediately prior to use, protease inhibitor (Roche Diagnostics, Indianapolis, IN, USA) and phosphatase inhibitor (pepstatin, Roche Diagnostics, Indianapolis, IN, USA) were added into the RIPA Lysis Buffer. The resulting suspension was sonicated with an ultrasonic cell disrupter (Bandelin, OSTC) and centrifuged at 14,000× g at 4°C for 15 min. Supernatant was collected and stored at −80°C. Nuclear protein extraction was performed with NE-PER^TM Nuclear and Cytoplasmic Extraction Reagents (78833, Thermo) according to the manufacturer’s instructions, samples were stored at −80°C. Protein quantification was performed using BCA Protein Assay Kit (23227, Thermo, USA). ELISAs were performed according to the manufacturer’s instructions (IL-1β RLB00; TNF-α RTA00, R&D Systems; NF-κB ab133128; p-IκBα ab176643, Abcam; PSD-95, LS-F6865, LifeSpan BioSciences, Inc.) and optical density determined at 450 with a microplate reader (BioRad, Richmond, CA, USA).

Morris Water Maze Test

One day after treatment, learning ability and memory for spatial orientation of the rats were assessed by Morris water maze (MWM) test in a separate cohort of animals (n = 8–10/group) as previously described with some modification (Yang et al., 2012). The MWM consisted of a circular black painted pool and was placed in a dimly lit room with several visual clues around. The pool was filled to a depth of 20 cm water (25 ± 2°C) and with a hidden submerged platform located 1.5 cm below the water surface in one fixed quadrant. Rats were gently placed in one quadrant facing the wall of MWM pool. The rats were allowed to swim for 60 s to locate the hidden platform during each trial. When successful, the rat was allowed to stay for 5 s on the platform. If unsuccessful within 60 s, the rat was then physically placed on the platform for 20 s. A 3–5 min interval was allowed between each trial. The time spent to locate the platform, swimming speed and distance were recorded by a video camera and analyzed by Videomot software (version 2.4.50923; TSE Systems, Bad Homburg, Germany). Four spatial acquisition trials were performed on each rat per day with the starting location in each quadrant and five consecutive days of training were conducted (day 1–5). On day 7, a probe trial was conducted with the platform removed. Rats were placed in the quadrant opposite to the original location of the platform, and allowed to swim in the pool for 30 s. The times crossover the platform location and the percentage of time spent in the previous platform quadrant were recorded. From day 31 to 35, spatial acquisition trials were repeated followed with a probe trial on day 37. The time line of MWM protocol is shown in Figure 5A.

Statistical Analyses

For statistical analyses Prism v5 software (GraphPad Software Inc., La Jolla, CA, USA) was used. All values in the figures are presented as mean ± SEM. MWM test was analyzed by repeated-measures two-way ANOVA followed by Bonferroni post hoc analysis. All other data were analyzed by two-way ANOVA followed by Bonferroni post hoc analysis. P values < 0.05 were considered statistically significant.

Results

PDTC Reduces Pro-Inflammatory Systemic Cytokines After LPS Administration

The circulating TNF-α and IL-1β levels were significantly affected by LPS and PDTC (F_(2,34) = 152.8 and 40.92, p < 0.0001 respectively). Post hoc comparisons of two-way ANOVA showed serum TNF-α significantly increased at 0.5 h, 2 h and 6 h after LPS injection compared to the vehicle group (333.10 ± 102.90, 1033.00 ± 68.55 and 614.20 ± 75.89 vs. 6.28 ± 1.50 pg/ml, p < 0.01 and p < 0.001 respectively, Figure 1A); while serum IL-1β was significantly increased at 2 h, 6 h and 24 h after LPS injection compared to the vehicle group (835.40 ± 203.00, 1203.00 ± 74.31 and 136.80 ± 44.46 vs. 3.59 ± 1.53 pg/ml, p < 0.01, 0.001 and 0.05 respectively, Figure 1B). PDTC pretreatment significantly decreased serum TNF-α from 0.5 h to 6 h compared to LPS group (p < 0.01 and p < 0.001 respectively, Figure 1A). In addition, the LPS induced increase of circulating IL-1β was significantly reduced by PDTC pretreatment at 2 h and 6 h (p < 0.05, p < 0.001 respectively, Figure 1B).

Figure 1

Effects of PDTC on Astrocytes and IL-1β Expression in the Hippocampus

Previous studies have shown that acute systemic inflammation triggered by a single administration of LPS resulted in chronic neuroinflammation (Qin et al., 2007; Gao et al., 2011). Here we focused on the effects of PDTC on GFAP-positive astrocytes in hippocampus DG region as minimal immunoreactivity was observed in microglia by Iba-1 immunofluorescence (Supplementary Figure S3). The immunofluorescence staining showed IL-1β in astrocytes was significantly affected by LPS and PDTC (F_(2,45) = 747.60, p < 0.0001 respectively). The IL-1β positive astrocytes in hippocampus were significantly increased from day 1 to 15 in both LPS and LPS + PDTC groups compared to the vehicle (Figures 2A,B). However, PDTC pretreatment significantly reduced LPS induced IL-1β expression in astrocytes (p < 0.01, p < 0.001, p < 0.001 and p < 0.05 vs. LPS group respectively). In addition, we measured IL-1β protein level in hippocampus using ELISA. LPS and PDTC showed significant effects on hippocampal IL-1β protein level (F_(1,30) = 34.16; p < 0.0001). LPS significantly increased IL-1β level in hippocampus at day 7 compared to vehicle (10.50 ± 1.12 vs. 4.02 ± 0.51 pg/mg, p < 0.001), which was significantly attenuated by PDTC pretreatment (7.02 ± 0.70, p < 0.05 vs. LPS group, Figure 2C). In addition, LPS and PDTC significantly affected the hippocampal IL-1β mRNA expression (F_(2,45) = 13.44; p < 0.0001). LPS i.p. caused significant increase of IL-1β mRNA expression in hippocampus at day 3 and 7 compared to vehicle (p < 0.01 respectively), which were significantly attenuated by PDTC pretreatment (p < 0.01 and p < 0.05 vs. LPS group respectively, Figure 2D).

Figure 2

PDTC Diminished LPS Induced NF-κB p65 Activity in the Hippocampus

To better understand the mechanisms underlying this neuroinflammatory response we measured NF-κB p65 and the phosphorylation of IκB-α in the hippocampus. NF-κB p65 protein and mRNA expression in hippocampus were significantly affected by LPS and PDTC treatment (F_(2,45) = 21.23 and 19.47, p < 0.0001 respectively). On day 3 and 7 after LPS administration NF-κB p65 protein levels and mRNA expression were significantly increased compared to vehicle (Protein level: p < 0.01 and p < 0.05 respectively; mRNA: p < 0.01 respectively). These changes were significantly attenuated in the LPS + PDTC group compared to LPS group (Protein level: p < 0.01 and p < 0.05 respectively, mRNA: p < 0.05 respectively Figures 3A,B). Further, the hippocampal IκB-α protein and mRNA expression were also affected by different treatments (F_(2,45) = 25 and 27.40, p < 0.0001 respectively). From day 1 to 7 after LPS administration, phosphorylated IκB-α was markedly increased in hippocampus compared to vehicle (p < 0.05, p < 0.01 and p < 0.001 respectively), these increase were significantly attenuated by PDTC pre-treatment (p < 0.05 respectively, Figure 3C). Accordingly, the mRNA expression of total IκB-α in hippocampus were significantly reduced from day 1 to 15 after LPS injection compared to vehicle group (p < 0.05 and p < 0.01 respectively). However, compared to LPS injection alone, rats with PDTC pretreatment showed reserved total IκB-α mRNA expression in the hippocampus, especially on day 3 and 7 (p < 0.05 respectively compared to LPS group, Figure 3D). No effects of PDTC alone were observed (Supplementary Figure S4).

Figure 3

PSD-95 Expression in the Hippocampus After PDTC Treatment

Next we measured the effects of LPS administration on scaffolding proteins focusing on the major molecule, PSD-95. The immunofluorescence staining showed LPS and PDTC significantly affected the PSD-95 level in hippocampus (F_(2,44) = 9.07; p = 0.0005, Figures 4A,B). On both day 3 and day 7 PSD-95 was significantly decreased compared to controls (gray value as 52.86 ± 6.27 and 42.38 ± 1.59 vs. 67.42 ± 6.64, p < 0.05 respectively, Figure 4B). This effect was abolished by PDTC pretreatment. The protein and mRNA level of PSD-95 in hippocampus was then measured. Hippocampal PSD-95 protein level was significantly affected by different treatment (F_(2,45) = 10.99, p = 0.0001, Figure 4C), that LPS significantly reduced hippocampal PSD-95 on day 3 and 7 (p < 0.01 and p < 0.05 respectively), and PDTC pretreatment restored the PSD-95 level at these time points (p < 0.05 vs. LPS respectively). Similar changes were observed in PSD-95 mRNA expression at day 7 (Figure 4D).

Figure 4

PDTC Improves LPS-Induced Cognitive Dysfunction

We used MWM to test learning and memory function in this model of endotoxemia. The escape latency was significantly affected by the testing days and treatment. All groups showed marked improvements in escape latencies over the 5 days of training (F_{(3, 144)} = 2.87, p < 0.0001, repeated measures ANOVA), indicating a memory in locating the escape platform. Repeated measures ANOVA revealed no interaction between training days and groups (F_{(12, 144)} = 1.21, p > 0.05). This suggests that all the rats effectively learned the task. Post hoc comparisons indicated that LPS significantly increased the escape latency at day 2–5 in the spatial acquisition trials compared to vehicle (p < 0.001 and 0.01 respectively), PDTC significantly improved the LPS-induced prolonged escape latency in the rats at day 3–5 (p < 0.01 respectively, Figure 5B). Furthermore, repeated-measures two-way ANOVA in the probe trial on day 7 revealed the effects of drug (F_(2,62) = 4.76, p < 0.05) and time (F_(1,62) = 6.56, p < 0.05) on the platform crossovers. Post hoc analysis indicated that rats with LPS challenge had significant less platform crossovers compared to vehicle or LPS + PDTC treated rats (p < 0.001 and p < 0.05 respectively). Similarly ANOVA revealed the effects of drug (F_(2,31) = 4.63, P < 0.05) and time (F_(1,31) = 4.98, p < 0.05) on the time in the target quadrant. Post hoc analysis indicated that rats with LPS challenge had significant less time spent in the target quadrant compared to vehicle or LPS + PDTC treated rats (p < 0.01 and p < 0.05 respectively, Figures 5C,D). However, in the second round of spatial acquisition test from day 31 to 35, rats accepted LPS alone only showed significant longer escape latency on day 31 compared to rats accepted vehicle or LPS + PDTC (39.40 ± 5.96 vs. 19.64 ± 2.65 and 21.53 ± 5.33 s, p < 0.05 respectively, Figure 5E). No significant differences were observed between groups regarding the platform crossover and time spent in the quadrant in the probe trial on day 37 (Figures 5F,G). The swimming speeds were similar between all groups throughout the MWM test (not shown).

Figure 5

Discussion

In this study we focused on the effects of a single systemic dose of LPS in aged rats and assessed long-term changes in systemic cytokines, neuroinflammation, and behavior. Using a selective NF-κB inhibitor, PDTC, we report neuroprotective effects through inhibition of the canonical NF-κB signaling pathway, reduction of IL-1β expression in astrocytes, and stabilization of PSD-95. Taken together, PDTC offered sufficient protection to improve memory dysfunction after endotoxemia in aged rats.

Inflammation is a critical component of almost every clinical condition ranging from cancer to neurodegenerative disorders; yet non-resolving inflammation remains one of the major challenges in biomedical research (Nathan and Ding, 2010). Systemic infections can lead to significant consequences in elderly subjects and may contribute to the acceleration of pathologies like Alzheimer’s disease (Cunningham et al., 2009). LPS, a key component of Gram-negative bacteria outer membrane, has been used as a robust activator of innate immunity. Its effects on behavior have been well documented (Dantzer et al., 1998), but the mechanisms underlying cognitive impairments after endotoxemia are not fully understood. Inflammatory molecules can access the CNS through different immune-to-brain mechanisms, both blood-borne and neuronal (Capuron and Miller, 2011; Xu et al., 2014). After LPS exposure, we found a significant increase in systemic pro-inflammatory cytokines, including TNF-α and IL-1β, which initiate a pro-inflammatory response that affects long-term CNS function. LPS acts mainly peripherally, with minimal penetration of the intact BBB (Banks and Robinson, 2010). However, evidence from high-resolution magnetic resonance imaging analysis of the BBB in the living human brains found selective BBB breakdown during ageing, which may contribute to cognitive impairment (Montagne et al., 2015). Thus, it is possible that age-induced BBB opening as well as direct transport of blood-borne factors and cytokines contribute to subsequent neuroinflammation and memory dysfunction in our model (Banks et al., 1995; He et al., 2012).

To support a role for systemic inflammation in mediating secondary CNS effects, in this study treatment with PDTC was able to significantly reduce pro-inflammatory cytokines with levels returning to baseline within 24 h. TNF-α and IL-1β are two prototypical cytokines hardwired to NF-κB signaling (Lawrence, 2009) and are implicated in the development of age-related postoperative complications including delirium and postoperative cognitive dysfunction (Androsova et al., 2015). In mice, modulation of IL-1β signaling after endotoxemia using IL-1 receptor antagonist or genetic intervention (IL-1R^−/−) prevents cognitive dysfunction by attenuating microglia activation (Terrando et al., 2010). Microglia and astrocytes play pivotal roles in surveilling the CNS microenvironment, supporting neuronal homeostasis and protecting the brain from danger signals (Streit et al., 2004). Modulation of microglia activation was also reported after PDTC treatment in LPS-induced sepsis, improving long-term behavioral outcomes (Anderson et al., 2015). Previously we described an important role for astrocytes activation and cytokine expression in this model of LPS-induced neuroinflammation (Fu et al., 2014). Here we found PDTC was able to attenuate IL-1β expression in GFAP-positive cells in the hippocampus, confirming an important role for IL-1β and NF-κB signaling in ensuing CNS complications. In addition, pretreatment with PDTC regulated NF-κB activity by inhibiting IκB-α phosphorylation and p65 translocation into the nucleus. IκB phosphorylation is critical for activating the canonical and alternative NF-κB pathways and allowing nuclear translocation and downstream gene activation (Karin and Lin, 2002). Given PDTC is well tolerated in models of acute and chronic inflammation (Cuzzocrea et al., 2002), this could represent a suitable target for novel therapeutic discoveries.

Aside the effects of PDTC on NF-κB signaling we also describe a novel interaction with the excitatory postsynaptic marker, PSD-95. Synaptic proteins, especially PSD-95, play a critical role in regulating dendritic spine morphogenesis and plasticity, which are closely implicated in memory function and cognition (El-Husseini et al., 2000). Loss of PSD-95 coincided with NF-κB activation in the hippocampus on day 3 and 7 after LPS exposure, suggesting neuroinflammation impairs synaptic plasticity by modulating scaffolding protein at glutamatergic excitatory synapses. PSDs are essential structures for N-methyl-D-aspartate receptor signaling, thus exerting critical functions in synaptic processes, glutamate excitatory neurotransmission and calcium influx (Kennedy, 2000). Inflammation can impair synaptic plasticity especially during the ageing process or as a result of injury (Barrientos et al., 2006; Terrando et al., 2013). Changes in long-term potentiation, the molecular surrogate for memory dysfunction, have been implicated in LPS-induced changes in memory and behavior (Vereker et al., 2000). In our study PDTC rescued LPS-induced memory impairment as a result of its anti-inflammatory effects on NF-κB/cytokines signaling and stabilization of PSD-95 in the hippocampus. Improved memory function after PDTC treatment has been reported in other models of neuroinflammation and cognitive disorders (Li et al., 2012; Zhang et al., 2014). Since PDTC compounds have been used already in the clinic (Reisinger et al., 1990), inhibition of NF-κB pathway may offer therapeutic benefit for neuroinflammation and cognitive dysfunction.

Other mechanisms are likely to be involved in PDTC-mediated neuroprotection. The effects on oxidative stress are well known (Tsai et al., 1996) and these processes are tightly related with the ageing process. Increased reactive oxygen species and lipid peroxidation is found during brain ageing, contributing to microglia priming, SASP and cognitive decline (Norden and Godbout, 2013). This inherited vulnerability contributes to the prolonged and amplified immune response as noted in this study after a single LPS challenge. This “immune-priming” is likely to contribute to non-resolving inflammation and long-lasting modifications in behavior and CNS molecular markers (Bossù et al., 2012). Mechanistically, since PDTC crosses the BBB (Schreck et al., 1992; Ziegler-Heitbrock et al., 1993; Chabicovsky et al., 2010) and aged rats may have deficits in endothelial function, the drug could exert direct CNS effects both as anti-inflammatory on glia cells but also neurons. Some limitations of our study must be pointed out. We focused our study in aged rats as a clinically relevant model for a more vulnerable system to general perturbations like infection. We did not include or compare the effects of LPS and PDTC in a younger cohort, however previous studies demonstrated similar protective effects on neuroinflammation and cognitive outcomes in younger rodent models (Anderson et al., 2015). Also, the role of NF-κB modulation on different CNS cell types awaits future investigations with the use of more selective strategies to target exaggerated neuroinflammation, astrocyte activation, and brain dysfunction.

In conclusion, LPS-induced acute systemic cytokines can induce prolonged neuroinflammation in the ageing brain. Inhibition of NF-κB signaling regulates key processes in the CNS, including IL-1β up regulation in astrocytes and PSD-95 expression in the hippocampus. The anti-inflammatory and neuroprotective effects provide an important target for dampening neuroinflammation and improving cognitive decline.

Funding

This work was supported by grants from Beijing 215 High Level Healthcare Talent Plan-Academic Leader (008-0027) and Beijing Municipal Administration of Hospitals’ ascent Plan (DFL20150802).

References

• 1

  AndersonS. T.ComminsS.MoynaghP. N.CooganA. N. (2015). Lipopolysaccharide-induced sepsis induces long-lasting affective changes in the mouse. Brain Behav. Immun.43, 98–109. 10.1016/j.bbi.2014.07.007

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 2

  AndrosovaG.KrauseR.WintererG.SchneiderR. (2015). Biomarkers of postoperative delirium and cognitive dysfunction. Front. Aging Neurosci.7:112. 10.3389/fnagi.2015.00112

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 3

  BanksW. A.KastinA. J.BroadwellR. D. (1995). Passage of cytokines across the blood-brain barrier. Neuroimmunomodulation2, 241–248. 10.1159/000097202

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 4

  BanksW. A.RobinsonS. M. (2010). Minimal penetration of lipopolysaccharide across the murine blood-brain barrier. Brain Behav. Immun.24, 102–109. 10.1016/j.bbi.2009.09.001

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 5

  BarrientosR. M.HigginsE. A.BiedenkappJ. C.SprungerD. B.Wright-HardestyK. J.WatkinsL. R.et al. (2006). Peripheral infection and aging interact to impair hippocampal memory consolidation. Neurobiol. Aging27, 723–732. 10.1016/j.neurobiolaging.2005.03.010

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 6

  BossùP.CutuliD.PalladinoI.CaporaliP.AngelucciF.LaricchiutaD.et al. (2012). A single intraperitoneal injection of endotoxin in rats induces long-lasting modifications in behavior and brain protein levels of TNF-alpha and IL-18. J. Neuroinflammation9:101. 10.1186/1742-2094-9-101

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 7

  CampisiJ. (2005). Senescent cells, tumor suppression and organismal aging: good citizens, bad neighbors. Cell120, 513–522. 10.1016/j.cell.2005.02.003

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 8

  CampuzanoO.Castillo-RuizM. M.AcarinL.CastellanoB.GonzalezB. (2009). Increased levels of proinflammatory cytokines in the aged rat brain attenuate injury-induced cytokine response after excitotoxic damage. J. Neurosci. Res.87, 2484–2497. 10.1002/jnr.22074

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 9

  CapaniF.QuarracinoC.CaccuriR.SicaR.E.P. (2016). Astrocytes as the main players in primary degenerative disorders of the human central nervous system. Front. Aging Neurosci.8:45. 10.3389/fnagi.2016.00045

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 10

  CapuronL.MillerA. H. (2011). Immune system to brain signaling: neuropsychopharmacological implications. Pharmacol. Ther.130, 226–238. 10.1016/j.pharmthera.2011.01.014

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 11

  ChabicovskyM.Prieschl-GrassauerE.SeipeltJ.MusterT.SzolarO. H.HebarA.et al. (2010). Pre-clinical safety evaluation of pyrrolidine dithiocarbamate. Basic Clin. Pharmacol. Toxicol.107, 758–767. 10.1111/j.1742-7843.2010.00573.x

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 12

  CotrinaM. L.NedergaardM. (2002). Astrocytes in the aging brain. J. Neurosci. Res.67, 1–10. 10.1002/jnr.10121

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 13

  CunninghamC. (2013). Microglia and neurodegeneration: the role of systemic inflammation. Glia61, 71–90. 10.1002/glia.22350

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 14

  CunninghamC.CampionS.LunnonK.MurrayC. L.WoodsJ. F.DeaconR. M.et al. (2009). Systemic inflammation induces acute behavioral and cognitive changes and accelerates neurodegenerative disease. Biol. Psychiatry65, 304–312. 10.1016/j.biopsych.2008.07.024

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 15

  CuzzocreaS.ChatterjeeP. K.MazzonE.DugoL.SerrainoI.BrittiD.et al. (2002). Pyrrolidine dithiocarbamate attenuates the development of acute and chronic inflammation. Br. J. Pharmacol.135, 496–510. 10.1038/sj.bjp.0704463

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 16

  CvekB.DvorakZ. (2007). Targeting of nuclear factor-kappaB and proteasome by dithiocarbamate complexes with metals. Curr. Pharm. Des.13, 3155–3167. 10.2174/138161207782110390

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 17

  DantzerR. (2004). Cytokine-induced sickness behaviour: a neuroimmune response to activation of innate immunity. Eur. J. Pharmacol.500, 399–411. 10.1016/j.ejphar.2004.07.040

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 18

  DantzerR.BluthéR. M.GheusiG.CremonaS.LayeS.ParnetP.et al. (1998). Molecular basis of sickness behavior. Ann. N Y Acad. Sci.856, 132–138.

  • Pubmed Abstract
  • Google Scholar

• 19

  DongY.BenvenisteE. N. (2001). Immune function of astrocytes. Glia36, 180–190. 10.1002/glia.1107

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 20

  El-HusseiniA. E.SchnellE.ChetkovichD. M.NicollR. A.BredtD. S. (2000). PSD-95 involvement in maturation of excitatory synapses. Science290, 1364–1368. 10.1126/science.290.5495.1364

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 21

  FuH. Q.YangT.XiaoW.FanL.WuY.TerrandoN.et al. (2014). Prolonged neuroinflammation after lipopolysaccharide exposure in aged rats. PLoS One9:e106331. 10.1371/journal.pone.0106331

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 22

  GaoH. M.ZhangF.ZhouH.KamW.WilsonB.HongJ. S. (2011). Neuroinflammation and alpha-synuclein dysfunction potentiate each other, driving chronic progression of neurodegeneration in a mouse model of Parkinson’s disease. Environ. Health Perspect.119, 807–814. 10.1289/ehp.1003013

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 23

  HeH. J.WangY.LeY.DuanK. M.YanX. B.LiaoQ.et al. (2012). Surgery upregulates high mobility group box-1 and disrupts the blood-brain barrier causing cognitive dysfunction in aged rats. CNS Neurosci. Ther.18, 994–1002. 10.1111/cns.12018

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 24

  HenekaM. T.CarsonM. J.El KhouryJ.LandrethG. E.BrosseronF.FeinsteinD. L.et al. (2015). Neuroinflammation in Alzheimer’s disease. Lancet Neurol.14, 388–405. 10.1016/S1474-4422(15)70016-5

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 25

  HenryC. J.HuangY.WynneA. M.GodboutJ. P. (2009). Peripheral lipopolysaccharide (LPS) challenge promotes microglial hyperactivity in aged mice that is associated with exaggerated induction of both pro-inflammatory IL-1beta and anti-inflammatory IL-10 cytokines. Brain Behav. Immun.23, 309–317. 10.1016/j.bbi.2008.09.002

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 26

  HirataI.YasumotoS.ToshinaK.InoueT.NishikawaT.MuranoN.et al. (2007). Evaluation of the effect of pyrrolidine dithiocarbamate in suppressing inflammation in mice with dextran sodium sulfate-induced colitis. World J. Gastroenterol.13, 1666–1671. 10.3748/wjg.v13.i11.1666

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 27

  KarinM.LinA. (2002). NF-kappaB at the crossroads of life and death. Nat. Immunol.3, 221–227. 10.1038/ni0302-221

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 28

  KennedyM. B. (2000). Signal-processing machines at the postsynaptic density. Science290, 750–754. 10.1126/science.290.5492.750

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 29

  LawrenceT. (2009). The nuclear factor NF-kappaB pathway in inflammation. Cold Spring Harb. Perspect. Biol.1:a001651. 10.1101/cshperspect.a001651

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 30

  LiJ.ShengW.FengC.ZuoZ. (2012). Pyrrolidine dithiocarbamate attenuates brain Abeta increase and improves long-term neurological outcome in rats after transient focal brain ischemia. Neurobiol. Dis.45, 564–572. 10.1016/j.nbd.2011.09.013

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 31

  LucinK. M.Wyss-CorayT. (2009). Immune activation in brain aging and neurodegeneration: too much or too little?. Neuron64, 110–122. 10.1016/j.neuron.2009.08.039

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 32

  LynchM. A. (2010). Age-related neuroinflammatory changes negatively impact on neuronal function. Front. Aging Neurosci.1:6. 10.3389/neuro.24.006.2009

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 33

  MontagneA.BarnesS. R.SweeneyM. D.HallidayM. R.SagareA. P.ZhaoZ.et al. (2015). Blood-brain barrier breakdown in the aging human hippocampus. Neuron85, 296–302. 10.1016/j.neuron.2014.12.032

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 34

  NajjarS.PearlmanD. M.AlperK.NajjarA.DevinskyO. (2013). Neuroinflammation and psychiatric illness. J. Neuroinflammation10:142. 10.1186/1742-2094-10-142

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 35

  NathanC.DingA. (2010). Nonresolving inflammation. Cell140, 871–882. 10.1016/j.cell.2010.02.029

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 36

  NordenD. M.GodboutJ. P. (2013). Review: microglia of the aged brain: primed to be activated and resistant to regulation. Neuropathol. Appl. Neurobiol.39, 19–34. 10.1111/j.1365-2990.2012.01306.x

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 37

  OhtaK.NakayamaK.KurokawaT.KikuchiT.YoshimuraN. (2002). Inhibitory effects of pyrrolidine dithiocarbamate on endotoxin-induced uveitis in Lewis rats. Invest. Ophthalmol. Vis. Sci.43, 744–750.

  • Pubmed Abstract
  • Google Scholar

• 38

  PerryV. H.CunninghamC.HolmesC. (2007). Systemic infections and inflammation affect chronic neurodegeneration. Nat. Rev. Immunol.7, 161–167. 10.1038/nri2015

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 39

  QinL.WuX.BlockM. L.LiuY.BreeseG. R.HongJ. S.et al. (2007). Systemic LPS causes chronic neuroinflammation and progressive neurodegeneration. Glia55, 453–462. 10.1002/glia.20467

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 40

  ReisingerE. C.KernP.ErnstM.BockP.FladH. D.DietrichM. (1990). Inhibition of HIV progression by dithiocarb. German DTC study group. Lancet335, 679–682. 10.1016/0140-6736(90)90802-c

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 41

  SalminenA.KauppinenA.KaarnirantaK. (2012). Emerging role of NF-kappaB signaling in the induction of senescence-associated secretory phenotype (SASP). Cell. Signal.24, 835–845. 10.1016/j.cellsig.2011.12.006

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 42

  SalminenA.OjalaJ.KaarnirantaK.HaapasaloA.HiltunenM.SoininenH. (2011). Astrocytes in the aging brain express characteristics of senescence-associated secretory phenotype. Eur. J. Neurosci.34, 3–11. 10.1111/j.1460-9568.2011.07738.x

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 43

  SchreckR.MeierB.MannelD. N.DrogeW.BaeuerleP. A. (1992). Dithiocarbamates as potent inhibitors of nuclear factor kappa-B activation in intact-cells. J. Exp. Med.175, 1181–1194. 10.1084/jem.175.5.1181

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 44

  ShihR. H.WangC. Y.YangC. M. (2015). NF-kappaB signaling pathways in neurological inflammation: a mini review. Front. Mol. Neurosci.8:77. 10.3389/fnmol.2015.00077

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 45

  StreitW. J.MrakR. E.GriffinW. S. (2004). Microglia and neuroinflammation: a pathological perspective. J. Neuroinflammation1:14. 10.1186/1742-2094-1-14

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 46

  TerrandoN.Gómez-GalánM.YangT.CarlströmM.GustavssonD.HardingR. E.et al. (2013). Aspirin-triggered resolvin D1 prevents surgery-induced cognitive decline. FASEB J.27, 3564–3571. 10.1096/fj.13-230276

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 47

  TerrandoN.Rei FidalgoA.VizcaychipiM.CibelliM.MaD.MonacoC.et al. (2010). The impact of IL-1 modulation on the development of lipopolysaccharide-induced cognitive dysfunction. Crit. Care14:R88. 10.1186/cc9019

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 48

  TsaiJ. C.JainM.HsiehC. M.LeeW. S.YoshizumiM.PattersonC.et al. (1996). Induction of apoptosis by pyrrolidinedithiocarbamate and N-acetylcysteine in vascular smooth muscle cells. J. Biol. Chem.271, 3667–3670. 10.1074/jbc.271.7.3667

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 49

  VerekerE.CampbellV.RocheE.McenteeE.LynchM. A. (2000). Lipopolysaccharide inhibits long term potentiation in the rat dentate gyrus by activating caspase-1. J. Biol. Chem.275, 26252–26258. 10.1074/jbc.m002226200

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 50

  XuG.YangT.TerrandoN. (2014). The role of inflammation in postoperative cognitive dysfunction. J. Anesth. Perioper. Med.1, 97–103.

  • Google Scholar

• 51

  YangT.ZhuangL.Rei FidalgoA. M.PetridesE.TerrandoN.WuX.et al. (2012). Xenon and sevoflurane provide analgesia during labor and fetal brain protection in a perinatal rat model of hypoxia-ischemia. PLoS One7:e37020. 10.3410/f.716598068.792003118

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 52

  ZhangJ.JiangW.ZuoZ. (2014). Pyrrolidine dithiocarbamate attenuates surgery-induced neuroinflammation and cognitive dysfunction possibly via inhibition of nuclear factor kappaB. Neuroscience261, 1–10. 10.1016/j.neuroscience.2013.12.034

  • Pubmed Abstract
  • CrossRef
  • Google Scholar

• 53

  Ziegler-HeitbrockH. W.SternsdorfT.LieseJ.BelohradskyB.WeberC.WedelA.et al. (1993). Pyrrolidine dithiocarbamate inhibits NF-kappa B mobilization and TNF production in human monocytes. J. Immunol.151, 6986–6993.

  • Pubmed Abstract
  • Google Scholar