RIG-I contributes to the innate immune response after cerebral ischemia

Background Focal cerebral ischemia induces an inflammatory response that when exacerbated contributes to deleterious outcomes. The molecular basis regarding the regulation of the innate immune response after focal cerebral ischemia remains poorly understood. Methods In this study we examined the expression of retinoic acid-inducible gene (RIG)-like receptor-I (RIG-I) and its involvement in regulating inflammation after ischemia in the brain of rats subjected to middle cerebral artery occlusion (MCAO). In addition, we studied the regulation of RIG-I after oxygen glucose deprivation (OGD) in astrocytes in culture. Results In this study we show that in the hippocampus of rats, RIG-I and IFN-α are elevated after MCAO. Consistent with these results was an increased in RIG-I and IFN-α after OGD in astrocytes in culture. These data are consistent with immunohistochemical analysis of hippocampal sections, indicating that in GFAP-positive cells there was an increase in RIG-I after MCAO. In addition, in this study we have identified n-propyl gallate as an inhibitor of IFN-α signaling in astrocytes. Conclusion Our findings suggest a role for RIG-I in contributing to the innate immune response after focal cerebral ischemia.


Background
Stroke is a major problem affecting populations worldwide. It is the second most common cause of death in the world after heart disease. In the United States stroke is the fourth leading cause of death, and the societal costs are approximately 80 billion dollars, which are expected to double by the year 2030 [1]. As a result, it is important to identify new and better therapies aimed at successfully treating this patient population.
Inflammation is a major contributor to the deleterious effects that present after an ischemic event such as stroke [2]. A component of inflammation is the innate immune response, which is characterized by the activation of pattern recognition receptors (PRR) such as Tolllike receptors (TLRs), NOD-like receptors (NLRs) or RIG-like receptors (RLRs). TLRs have been previously studied in regards to their deleterious and beneficial effects following stroke [3][4][5][6][7][8]. Similarly NOD-like receptors (NLRs), such as NLRP1 or NLRP3, have been shown to contribute to the inflammatory response after stroke through the formation of inflammasomes [9][10][11][12][13]. However, not much is known about the contribution of RLR signaling to the pathology after focal cerebral ischemia.
RLR signaling is typically involved in the production of type I IFNs such as IFN-α following RNA viral infections. We have previously shown that in the central nervous system (CNS), RLR signaling contributes to the process of reactive astrogliosis following spinal cord injury [14], and that retinoic acid-inducible gene-I (RIG-I), an RLR PRR, is elevated in the cortex of patients with early signs of Alzheimer's disease (mild cognitive impairment), contributing to the production of amyloid precursor protein and amyloid-β [15]. However, the role of RIG-I to the regulation of inflammation after cerebral ischemia remains unexplored.
In the present project, we have studied the involvement of RIG-I after focal cerebral ischemia in rats. Here we also show the effects of oxygen glucose deprivation (OGD) on RIG-I signaling activation in astrocytes and identify n-propyl gallate (nPG) as an inhibitor of IFN-α in astrocytes.

Animals and focal cerebral ischemia
All animal procedures were approved by the Institutional Animal Care and Use Committee of the University of Miami (protocol number . To induce transient middle cerebral artery occlusion (MCAO), male Sprague-Dawley rats were anesthetized with 3 % isoflurane in a mixture of 70 % N 2 O/30 % O 2 for 5 min. Rats were intubated and immobilized with pancuronium bromide (0.35 mg/kg, IV) and mechanically ventilated. Brain and body temperature were monitored and the animals were maintained at a normothermic (37°C) temperature. A catheter was implanted into the tail artery for blood-gas monitoring during surgery. The right common carotid artery was exposed with a midline neck incision and dissected from the surrounding nerves. The external carotid artery and superior thyroid artery were then ligated. A 4-cm length of 3-0 suture that was heatblunted with a 20 mm section coated with poly-l-lysine solution (0.1 % wt/vol) was used for the occlusion. This suture was inserted at the proximal external carotid artery into the internal carotid artery to the MCA. The MCA was occluded for 90 min, then released for reperfusion. The neck incision was closed with staples and the animals were allowed to wake-up from the anesthesia. The animal was then taken to a cage supplied with food and water until termination of the study. Animals that presented with difficulty eating, presented blood pressure abnormalities, respiratory difficulties or brains that were not well perfused were euthanized and excluded from the study.

Immunoblotting
For detection of RLR proteins after MCAO, protein lysates ipsilateral to the ischemic side, of hippocampal brain areas were obtained and resolved by immunoblotting. We did not detect any effects of MCAO on RIG-I signaling on the contralateral side (data not shown). Sham animals were used as controls. Animals were sacrificed at different time points after ischemia (1 h, 4 h, 1d and 3d after MCAO) and then lysates were prepared and resolved by immunoblotting as described in de Rivero Vaccari et al. [16] using antibodies against RIG-I (1:1000, Anaspec), IFN-α (1:1000, Abcam) and β-actin (1:5000, Sigma). Data was normalized to β-actin.

Perfusion fixation
For immunohistochemical analysis rats were anesthetized and perfusion-fixed with 4 % paraformaldehyde (PFA) as described in de Rivero Vaccari et al. [16].

Immunohistochemistry and confocal microscopy
Immunostained brain sections of sham and 4 h MCAO animals were examined with an Olympus FV-1000 Laser Scanning Confocal Microscope (Olympus). Rats were perfused with 4 % paraformaldehyde as described [16] and processed for cryostat sectioning (Leica SM 2000R Sliding Microtome). Sections (50 μm) were prepared for immunohistochemical analysis as described in de Rivero Vaccari et al. [16] with a primary antibody to RIG-I (1:500, Abcam) and with the astrocytic marker anti-glial fibrillary acidid protein (GFAP) (Millipore Bioscience Research Reagents). Alexa-Fluor secondary antibody conjugates (1:500, Invitrogen) were used. Secondary antibodies alone were used as control for antibody specificity.

Astrocyte culture preparation
Primary rat astrocyte cells (Lonza) were plated and grown in culture for 7 days prior to experimentation at a density of 4×10 4 cells/9.5 cm 2 as described in de Rivero Vaccari et al. [14]. Cells were grown in Astrocyte Basic Medium (Lonza).

Oxygen Glucose Deprivation (OGD)
Astrocyte cultures were grown as described above. For OGD, cultures were exposed to 95 % nitrogen and 5 % CO 2 atmosphere maintained by constant gas flow at 37°C in all experiments. Oxygen tension was kept at 5 % during the duration of the experiment. The Nitrogen/CO2 content was controlled with the ProOx P110 Oxygen Controller with an E702 Oxygen Sensor (model #P-110-E70) with single set point controller (#P110) (Biospherix). The media used in these OGD experiments consisted of hypoglycemic medium containing normal salts, 1 mg/mL bovine serum albumin (BSA) and 55 μM glucose (1 % of the normal glucose concentration). Control groups were grown under normal culture conditions (5 % CO 2 and 95 % Oxygen).

NF-κB activation assay
To test for NF-κB activation, protein lysates (Control, 2, 3 and 4 h after OGD) were obtained from rat astrocytes and assayed with the PathScan Phospho-NF-κB p65 (Ser536) Sandwich Elisa kit (Cell Signaling) according to manufacturer's instructions. Briefly, 100 μl of cell lysate were added and sealed to the appropriate wells for a 2 h incubation period at 37°C. Each well was washed 4 times with 1X Wash Buffer. A detection antibody was added to each well and incubated at 37°C for 1 h. Then 100 μl of reconstituted HRP-Linked secondary antibody were added to each well and incubated for 30 min followed by adding 100 μl of TMB Substrate to each well for 10 min and a STOP solution. The plate was read using a spectrophotometer (Victor 3 1420 multilabel counter, Perkin Elmer) at 450 nm.

Cell reporter assay for RLR signaling activation in astrocytes
Astrocytes were grown in culture as described above in a 96-well plate. RLR signaling was stimulated in cells with poly(I:C)LMW (low molecular weight) at 3 different concentrations (1, 3 and 6 μg/ml, dissolved in sterile water) for 24 h. On day 2, 150 μl per well of B16-BLUE IFN-α/β cells (Invivogen) in suspension (50,000 cells) were added and incubated overnight at 37°C in 5 % CO 2 . On day 3, 50 μl per well of the supernatant were added to 150 μl of QUANTI-Blue (Invivogen). The plate was incubated for 2 h at 37°C and read at 600 nm in a spectrophotometer (Victor 3 1420 multilabel counter, Perkin Elmer). A similar procedure was carried to test n-propyl-gallate (n-PG, dissolved in dimethyl sulfoxide (DMSO), MP Biomedicals) as a blocker of type I IFN signaling at different concentrations (5, 10 and 50 μM).

Statistical analysis
Statistical comparisons between the different groups were done using a two-tailed Student's t-test or a oneway ANOVA followed by Dunnett's multiple comparison tests. P-values of significance used were P < 0.05.

RLR signaling protein expression is altered in the hippocampus of rats after MCAO
To determine if RLR protein expression is altered after MCAO, we analyzed protein lysates obtained from the hippocampus (ipsilateral side to MCAO) of rats at different time points after ischemia (1 h, 4 h, 1d and 3d) and in sham-operated animals for the expression of RIG-I and IFN-α (Fig. 1). MCAO resulted in increased protein expression of RIG-I at 4 h, 1d and 3d (Fig. 1b) as well as of IFN-α at 3d (Fig. 1c) in the hippocampus of rats. These data indicate an involvement of RIG-I after focal cerebral ischemia.

MCAO induces alterations in RIG-I protein expression in astrocytes
Confocal images of frozen sections were double stained with RIG-I (A, red) and the astrocyte marker GFAP (green). Four hours after MCAO, there was an increased in the immunoreactivity of RIG-I in astrocytes (arrows) when compared to sham-operated animals (Fig. 2). These findings indicate that RIG-I expression increased after MCAO in astrocytes after ischemia.

OGD induces RLR signaling components in astrocytes
Since RIG-I protein expression is increased by ischemia in astrocytes (Fig. 2), we wanted to establish whether OGD induces RLR signaling in astrocytes in culture. Primary astrocytes were grown in culture and subjected to OGD for 2, 3 and 4 h. Cells grown under standard culture conditions (no OGD) were used as a control (C). As shown in Fig. 3, there is a statistically significant increase in RIG-I and IFN-α at 3 and 4 h after OGD in astrocytes in culture. Consistent with these results is the activation of NF-κB at 3 and 4 h as determined by an NF-κB activation assay. NF-κB is involved in the production of type I IFNs such as IFNα. This is consistent with well-established evidence indicating that NF-κB is activated after cerebral ischemia [17,18]. The levels of phosphorylated IRF3/7 did not differ among the different

Propyl Gallate (n-PG) inhibits RLR signaling in primary astrocytes
To identify a potential inhibitor of RLR signaling, we used a cell reporter assay that produces IFN-α/β after stimulation. We stimulated astrocytes in culture with the RLR ligand poly(I:C)LMW for 18 h at concentrations of 1, 3 and 6 μg/ml. Our findings indicate that at concentrations of 3 and 6 μg/ml of poly(I:C)LMW, RLR signaling increased (Fig. 4a). Then we stimulated cells in a similar manner with 6 μg/ml of poly(I:C)LMW combined with n-PG treatment at concentrations of 5, 10 and 50 μM. At all of these concentrations n-PG was able  to lower RLR signaling activation when compared to the poly(I:C)LMW-treated/n-PG-untreated group, as determined by the cell reporter assay (Fig. 4b). In addition, astrocytes were pretreated with 50 μM n-PG for 2 h prior to 4 h of OGD. The 50 μM, 2 h n-PG-treatment resulted in decreased IFN-α production (Fig. 4c); thus suggesting that n-PG can be used to inhibit RLR signaling in astrocytes after ischemia.

Discussion
Worldwide, stroke is the second most common cause of death after heart disease. Despite its prevalence, the therapies available for stroke patients remain limited and in most instances do not offer significant improvements. As a result, it is important to identify new targets that can be used for the development of treatments for cerebral ischemia. A promising target for the treatment of stroke is the inflammatory innate immune response.
The involvement of PRR such as TLR and NLR in brain ischemia has been previously described [11,13,[19][20][21][22][23]. In the present study we extend the knowledge regarding the role of PRR in brain ischemia by studying the effects of focal cerebral ischemia on RIG-I expression after MCAO. RIG-I is a RLR involved in the process of reactive astrogliosis after spinal cord injury [14]. In this study we have identified RIG-I as a PRR altered by focal cerebral ischemia in the hippocampus of rats after MCAO. When looking at whole hippocampal proteins lysates, RIG-I protein expression increased after MCAO. The increase in RIG-I expression was consistent with the increase in IFN-α. When analyzing the hippocampus of rats in immunohistochemical sections after MCAO, we detected increased immunoreactivity of RIG-I in astrocytes, suggesting that indeed RIG-I is increased after MCAO in the hippocampus. Moreover, our data in culture indicate that in astrocytes, RIG-I expression increased after OGD, which is consistent with our immunohistochemistry findings in GFAP-positive cells in vivo. This increase in RIG-I by OGD in cultured astrocytes was consistent with an increase in IFN-α expression, which is produced in a NF-κB dependent manner. In addition, in vivo, RIG-I expression was more prevalent in astrocytes.
Propyl gallate has been previously shown to be beneficial in the treatment of dilated cardiomyopathy in mice [24], and it is usually found as a food additive to prevent oxidation due to its strong anti-oxidant effects [25]. At the same time, n-PG has anti-inflammatory effects by down-regulating NF-κB or by suppressing the phosphorylation of c-Jun NH(2)-terminal kinase 1/2 (JNK1/2) [26,27]. Consistent with these findings, in the present study, we have identified n-PG as an inhibitor of IFN-α signaling in astrocytes. Future studies should also look into more Fig. 4 n-PG inhibits RLR signaling in primary astrocytes. a Bar-graph showing the results of a cell reporter assay for the activation of RLR signaling activation/production of IFN-α/β following stimulation of primary rat astrocytes with the RLR ligand poly(I:C)LMW at a concentration of 1, 3 or 6 μg/ml for 18 h. C = control (untreated cells). b Bar-graph showing the results of a cell reporter assay for the activation of RLR signaling activation/production of IFN-α/β following stimulation of primary rat astrocytes with the RLR ligand poly(I:C)LMW at a concentration of 6 μg/ml and treated with n-PG at a concentration of 5, 10, 50 μM for 18 h. C = control (untreated cells). c Representative immunoblot analysis of astrocyte lysates of cells in culture subjected to OGD (4 h) and astrocytes pretreated with 50 μM n-PG for 2 h and then subjected to OGD. Cell lysates were immunoblotted with an antibody against IFN-α. β-Actin was used as a standard and control for protein loading. Data presented as mean+/−SEM. *p < 0.05. N = 6 OGD and 8 OGD + nPG specific blockers of RIG-I or should use RIG-I knockout animals to better elucidate the contribution of RIG-I to the pathology of brain ischemia.

Conclusion
To the best of our knowledge, this is the first report to indicate an involvement of RIG-I in the inflammatory response after stroke, and we have identified n-PG as a potential anti-inflammatory drug after cerebral ischemia. Whether RLR signaling is beneficial or detrimental after stroke is under investigation. However, it has been suggested that inhibition of type I IFN signaling is beneficial in reducing hypoxia-induced neuroinflammation [28]. In contrast, other reports indicate that delivery of IFN-β has anti-inflammatory properties after ischemic stroke in rats by decreasing infiltration of neutrophils and monocytes into the brain [29]. As a result, the role of RLRs and type I IFN signaling after cerebral ischemia needs further investigation in order to obtain a better idea regarding the potential therapeutic potential of targeting RIG-I signaling under these conditions.