Abstract
The purpose of these studies is to investigate how Sphingosine-1-phosphate (S1P) signaling regulates glial phenotype, dedifferentiation of Müller glia (MG), reprogramming into proliferating MG-derived progenitor cells (MGPCs), and neuronal differentiation of the progeny of MGPCs. We found that S1P-related genes are highly expressed by retinal neurons and glia, and levels of expression were dynamically regulated following retinal damage. S1PR1 is highly expressed by resting MG and is rapidly downregulated following acute retinal damage. Drug treatments that activate S1PR1 or increase levels of S1P suppressed the formation of MGPCs, whereas treatments that inhibit S1PR1 or decreased levels of S1P stimulated the formation of MGPCs. Inhibition of S1PR1 or SPHK1 significantly enhanced the neuronal differentiation of the progeny of MGPCs. Further, ablation of microglia from the retina, wherein the formation of MGPCs in damaged retinas is impaired, has a significant impact upon expression patterns of S1P-related genes in MG. Inhibition of S1PR1 and SPHK1 partially rescued the formation of MGPCs in damaged retinas missing microglia. Finally, we show that TGFβ/Smad3 signaling in the resting retina maintains S1PR1 expression in MG. We conclude that the S1P signaling is dynamically regulated in MG and MGPCs and activation of S1P signaling depends, in part, on signals produced by reactive microglia.
Introduction
Different cell signaling pathways are known to regulate the reprogramming of Müller glia (MG) into MG-derived progenitor cells (MGPCs) in damaged retinas. For example, Jak/Stat-, MAPK-, mTOR-, and Wnt-signaling, as well as pro-inflammatory factors from reactive microglia, have been shown to play crucial roles in regulating MG reprogramming in the retinas of different vertebrate species (Fischer et al., 2009; Fischer et al., 2014; Nelson et al., 2012; Ramachandran et al., 2011; Todd et al., 2016; Todd et al., 2020; Wan et al., 2014; White et al., 2017). Nuclear Factor Kappa B (NFkB) is one the key cell signaling “hubs” that regulates the reactivity of MG, acts restore glial quiescence and suppress the neurogenic of MG-derived progenitors in the mouse retina (Hoang et al., 2020; Palazzo et al., 2022). We found that NFkB-signaling in damaged retinas is manifested in MG by pro-inflammatory signals produced by activated microglia (Palazzo et al., 2022; Palazzo et al., 2023). Further, we show that inhibition of NFkB-signaling results in diminished recruitment of immune cells in damaged retinas, increased neuronal survival, and increased formation of neuron-like cells from Ascl1-overexpressing MG (Palazzo et al., 2022). In the chick retina, by comparison, rapid activation of NFkB via signals produced by reactive microglia starts the process of MG activation and reprogramming, but sustained NFkB signaling suppresses the proliferating of MGPCs and neuronal differentiation of progeny (Palazzo et al., 2020). NFkB signaling is known to be coordinated with Sphingosine-1-phosphate (S1P) - signaling to regulate different cellular processes, including inflammation (Blom et al., 2010; Pérez-Jeldres et al., 2021; Zheng et al., 2019).
S1P signaling is a promising candidate to regulate the ability of MG to reprogram into proliferating, neurogenic progenitor cells. S1P is produced by sphingosine kinases (SPHK1 and SPHK2) and is degraded by a lyase (SGPL1). S1P can be exported from cells by a transporter (MFSD2A and SPNS2) or converted to sphingosine by a phosphatase (SGPP1) (Fig. 2a). Levels of sphingosine are increased by ASAH1 by conversion of ceramide or decreased by CERS2/5/6 by conversion to ceramide (Fig. 2a). S1P is known to activate G-protein coupled receptors, S1PR1 through S1PR5 (Fig. 2a). S1PRs are known to activate different cell signaling pathways including MAPK and PI3K/mTor, and crosstalk with pro-inflammatory pathways such as NFκB (Fig. 2a) (Hu et al., 2020). Alternatively, activation of S1PRs can activate Jak/Stat-signaling, which upregulates Egr1 to upregulate pro-inflammatory cytokines that secondarily activate NFkB (Gurgui et al., 2010). S1P signaling is an important pathway that has been widely implicated as mediating inflammatory responses, cellular proliferation, promote survival and regulate angiogenesis (Obinata and Hla, 2019). S1P signaling is required for vascular maturation, progenitor cell cycle exit, and axon guidance in the developing retina (Simón et al., 2019). However, S1P can have detrimental effects including migration of MG, angiogenesis, and inflammation associated with proliferative retinopathies and aging. Most of these studies in retinal cells were conducted in vitro, and these studies need to be followed-up by in vivo analyses to assess the coordinated impact of S1P signaling on the many different cell types in the retina. The functions of S1P signaling in normal and damaged retinas are poorly understood, and nothing is known about how S1P signaling impacts MG-mediated retinal regeneration.
Pro-inflammatory signaling represses reprogramming of mouse MG by promoting reactivity networks and anti-neurogenic factors, while increasing cell death in damage retinas (Palazzo et al., 2022). Therefore, it is important to understand how different cell signaling pathways impact inflammation to develop techniques to enhance neuronal survival and retinal regeneration. In this study we target S1P synthesis, S1P degradation and S1P receptors to investigate the roles of S1P-signaling during damage-dependent MG reprogramming and neurogenesis in the chick model system.
Methods
Animals
The animal use approved in these experiments was in accordance with the guidelines established by the National Institutes of Health and IACUC at The Ohio State University. Newly hatched P0 wildtype leghorn chicks (Gallus gallus domesticus) were obtained from Meyer Hatchery (Polk, Ohio). Post-hatch chicks were maintained in a regular diurnal cycle of 12 hours light, 12 hours dark (8:00 AM-8:00 PM). Chicks were housed in stainless-steel brooders at 25°C and received water and Purinatm chick starter ad libitum.
Intraocular Injections
Chicks were anesthetized with 2.5% isoflurane mixed with oxygen from a non-rebreathing vaporizer. The technical procedures for intraocular injections were performed as previously described (Fischer et al., 1998). With all injection paradigms, both pharmacological and vehicle treatments were administered to the right and left eye respectively. Compounds were injected in 20 μl sterile saline. Sphingosine and sphingosine-1 phosphate were injected with 0.05 mg/ml bovine serum albumin added as a carrier. 5-Ethynyl-2’-deoxyuridine (EdU) was injected into the vitreous chamber to label proliferating cells. Compounds included in this study are described in Table 1. Injection paradigms are included in each figure.
Preparation of clodronate liposomes
Clodronate liposomes were prepared as described previously (Fischer et al., 2014; Van Rooijen, 1989). In short, 50 ng cholesterol (Sigma C3045) and 8 mg L-α-phosphatidyl-DL-glycerol sodium salt (Sigma P8318) were dissolved in chloroform and evaporated into a thin film in a round-bottom flask. Then, the liposome film was dissolved in sterile PBS containing 158 mg dichloro-methylene diphosphonate (Sigma D4434). The clodronate was encapsulated by the liposomes via sonication at 42,000 Hz. The clodronate liposomes in PBS were centrifuged at 10,000 RCF, gently resuspended in 150 ml sterile PBS, and injected 20 ul/eye immediately. Our previous studies have shown that this method ablates >99% of microglia/macrophages 2 days after intraocular injection (El-Hodiri et al., 2023).
Fixation, sectioning, and immunocytochemistry
Retinas were fixed, sectioned, and immunolabeled as described previously (Fischer et al., 1998). To identify MG, we labeled sections for Sox2 or Sox9. Antibodies to Sox2 and Sox9 are known to label the nuclei or MG in the INL and the nuclei of astrocytes at the vitread surface of the retina (Fischer et al., 2010). None of the observed labeling was due to non-specific labeling of secondary antibodies or auto-fluorescence because sections labeled with secondary antibodies alone were devoid of fluorescence. Primary antibodies used in this study are described in Table 2. Secondary antibodies included donkey-anti-goat-Alexa488/594/647 (Life Technologies A11055; A11058; A21447), donkey-anti-rabbit-Alexa488/594 (Life Technologies A21206; A21207); and goat-anti-mouse-Alexa488/568 (Life Technologies A11001; A-11004) diluted to 1:1000 in PBS plus 0.2% Triton X-100. Nuclear staining was accomplished using DRAQ5 (Thermo 62251).
Labeling for EdU
For the detection of nuclei that incorporated EdU, immunolabeled sections were fixed in 4% formaldehyde in 0.1M PBS pH 7.4 for 5 minutes at room temperature. Samples were washed for 5 minutes with PBS, permeabilized with 0.5% Triton X-100 in PBS for 1 minute at room temperature and washed twice for 5 minutes in PBS. Sections were incubated for 30 minutes at room temperature in a buffer consisting of 100 mM Tris, 8 mM CuSO4, and 100 mM ascorbic acid in dH2O. The Alexa Fluor 647 Azide (Thermo Fisher Scientific A10277) was added to the buffer at a 1:500 dilution.
Terminal deoxynucleotidyl transferase dUTP nick end labeling (TUNEL)
The TUNEL method was used to identify dying cells with fragmented DNA. We used an in-situ Cell Death Detection kit from Roche (Fluorescein, 11684795910) according to manufacturer instructions.
Fluorescent in situ hybridization
Standard procedures were used for fluorescent in-situ hybridization (FISH), as described previously (Campbell et al., 2021a). In short, retinas from P9 eyes were fixed for 4 hours RT in 4% paraformaldehyde buffered in 0.1M dibasic sodium phosphate, washed in PTW (PBS + 0.2% Tween), and incubated in 30% sucrose at 4°C overnight. The retinas were embedded in OCT-compound and cryosectioned at 12 microns.
Tissue sections were processed for in situ hybridization with a split-initiator probe pair (Molecular Instruments) according to the manufacturer protocol for fresh/fixed frozen tissues. For slides in which immunocytochemistry was conducted with FISH, primary antibodies incubated overnight with the hairpin amplification buffer solution, and secondary antibodies incubated for one hour the next day. Slides were mounted with glycerol and glass coverslips.
Measurement of S1P with LC-MS/MS
Sample preparation
After intraocular injections of saline, NMDA, saline + PF-543, NMDA + PF543, or NMDA + SGPL-in-31, whole retinal tissue samples were collected into a 10-fold volume of methanol acidified with 0.1% formic acid.
Sphingosine-1-shosphate(d18:1) (S1P) and Sphingosine(d17:1) (Avanti Polar Lipids) were used as internal standards. Retinal samples were extracted with 80% methanol at a ratio of 1:20 (w/v) in a 2 mL Eppendorf tube. The samples were vortexed for 30 seconds, sonicated in water bath for 10 minutes, and followed by centrifugation at 10,000 rcf for 5 minutes at room temperature. One hundred microliter of supernatant was transferred out to a 2 mL HPLC vial and spiked with Sphingosine to a final concentration of 100 ppb. All the samples were analyzed in triplicates.
The matrix blank sample was prepared exactly as samples. Standard addition calibration levels were subsequently prepared by spiking 10, 25, 50, 100, 250, and 500 ppb of S1P into the matrix blank supernatant with final volume of 100 µL. The internal standard of Sphingosine was spiked in each calibration levels at 100 ppb. Finally, five microliters of the standard addition levels were injected and analyzed by LC-MS/MS.
Quantification
Quantification was carried out on a Vanquish UHPLC coupled to an Orbitrap Exploris 480 mass spectrometer (Thermo Fisher, MA, USA). The analytes were separated on a Accucore C18 2.6 μm 2.1 × 100 mm column using the binary solvents of 0.1% formic acid in water (v/v) (solvent A), and 0.1% formic acid in acetonitrile (v/v) (solvent B). The gradient was as follow: 0–0.5 min, holding at 10% B; 0.5–6 min, 10% to 95% B; 6-8 min, holding at 95% B; 8-8.01 min, 95% to 10% B; 8.01-10 min, holding at 10% B. The flow rate was 0.4 mL/min.
The following mass spectrometer instrument settings were used: ion source = H-ESI; positive ion = 3500 V; sheath gas = 35; aux gas = 7; ion transfer tube temperature = 320°C; vaporizer temperature = 275°C; HCD collision energy = 50%; RF lens = 40%.
The S1P and Sphingosine were quantified using the transition from 380.2560 m/z to 264.27 m/z, and transition from 286.2741 m/z to 268.26 m/z, respectively.
Results
The standard addition curves demonstrated great linearity with R2 above 0.99. Significance of difference was determined using a one-way ANOVA with Šidák correction for multiple comparisons.
Photography, immunofluorescence measurements, and statistics
Wide-field photomicroscopy was performed using a Leica DM5000B microscope equipped with epifluorescence and Leica DC500 digital camera. Confocal images were obtained using a Leica SP8 imaging system at the Department of Neuroscience Imaging Facility at the Ohio State University. Images were optimized for color, brightness and contrast, multiple channels over laid and figures constructed using Adobe Photoshop. Cell counts were performed on representative images. To avoid the possibility of region-specific differences within the retina, cell counts were consistently made from the same region of retina for each data set.
Where significance of difference was determined between two treatment groups accounting for inter-individual variability (means of treated-control values) we performed a two-tailed, paired t-test. Where significance of difference was determined between two treatment groups, we performed a two-tailed, unpaired t-test. Significance of difference between multiple groups was determined using ANOVA followed by Tukey’s test. GraphPad Prism 6 was used for statistical analyses and generation of histograms and bar graphs.
scRNA-seq
We analyzed scRNA-seq libraries that were generated and characterized previously (Campbell et al., 2021b; Campbell et al., 2022; El-Hodiri et al., 2022; El-Hodiri et al., 2023, 2021; Hoang et al., 2020; Li et al., 2023; Lyu et al., 2023).
Dissociated cells were loaded onto the 10X Chromium Cell Controller with Chromium 3’ V2, V3 or Next GEM reagents. Using Seurat toolkits (Powers and Satija, 2015; Satija et al., 2015), Uniform Manifold Approximation and Projection (UMAP) for dimensional reduction plots were generated from 9 separate cDNA libraries, including 2 replicates of control undamaged retinas, and retinas at different times after NMDA-treatment. Seurat was used to construct gene lists for differentially expressed genes (DEGs), violin/scatter plots, and dot plots. Significance of difference in violin/scatter plots was determined using a Wilcoxon Rank Sum test with Bonferroni correction. Genes that were used to identify different types of retinal cells included the following: (1) Müller glia: GLUL, VIM, SCL1A3, RLBP1, (2) MGPCs: PCNA, CDK1, TOP2A, ASCL1, (3) microglia: C1QA, C1QB, CCL4, CSF1R, TMEM22, (4) ganglion cells: THY1, POU4F2, RBPMS2, NEFL, NEFM, (5) amacrine cells: GAD67, CALB2, TFAP2A, (6) horizontal cells: PROX1, CALB2, NTRK1, (7) bipolar cells: VSX1, OTX2, GRIK1, GABRA1, and (7) cone photoreceptors: CALB1, GNAT2, GNB3, OPN1LW, and (8) rod photoreceptors: RHO, NR2E3, ARR3. The MG have an over-abundant representation in the scRNA-seq databases. This likely resulted from fortuitous capture-bias and/or tolerance of the MG to the dissociation process.
Results
S1P-signaling regulates the formation of MGPCs in damaged retinas
We first probed for patterns of expression of S1P-related genes in a large aggregate scRNA-seq library of >180,000 cells isolated from retinas treated with saline, NMDA, or 2 or 3 doses insulin+FGF2 and the combination of NMDA and insulin+FGF2 (Fig. 1a), as described previously (Campbell et al., 2021b; Campbell et al., 2022; El-Hodiri et al., 2022). Retinal cell types ordered into different UMAP clusters were identified based on well-established markers (Fig. 1b,c), as described in the methods. S1PR1 was most prominently expressed by resting MG and MG returning to a resting state, whereas S1PR3 was detected in relatively few scattered cells in clusters of MG, ganglion cells, horizontal cells, bipolar cells, amacrine cells, photoreceptors, oligodendrocytes, microglia and NIRG cells (Fid. 1d). NIRG cells, or Non-astrocytic Inner Retinal Glial cells, are a distinct type of glial cell that arise from optic nerve progenitors (Rompani and Cepko, 2008) and have described in retinas of chicks (Zelinka et al., 2012) and some species of reptiles (Todd et al., 2015). S1PR2 was not widely expressed in retinal cells (Fig. 1d). SPHK1 was detected in scattered cells in all cell types (Fig. 2e). SGPL1 was detected in scattered cells in all cell types with prominent expression in rod photoreceptors (Fig. 2e). ASAH1 (encoding acid ceramidase enzyme) was prominently expressed in microglia and cone photoreceptors, with expression in cells scattered in all other types of retinal cells (Fig. 2f). Genes encoding ceramide synthase enzymes showed variable patterns of expression. CERS6 was prominently detected in all types of inner retinal neurons (Fig. 2f), whereas CERS5 was detected in relatively few cells scattered across clusters of different types of cells (Fig. 2f).
We bioinformatically isolated the MG (>70,000 cells) and re-embedded these cells into a UMAP plot (Fig. 1g). The UMAP ordering of MG revealed clusters that were comprised of cells from distinct treatments and different times after treatment (Fig. 1h,i). We find that S1P-related genes are dramatically up- or downregulated in MG in damaged retinas and during the formation of MGPCs. Dynamic changes of mRNA levels are strongly correlated with changes in protein levels and function (Liu et al., 2016). We found that levels of S1PR1 and CERS6 were very high in resting MG and significantly downregulated in MG and MGPCs from treated retinas (Fig. 1j; supplemental table 1). S1PR3 was significantly higher in MGPCs, namely the MGPC2 cluster, compared to MG in all other UMAP clusters (Fig. 1j; supplemental table 1).
Levels of SPHK1 were relatively high in resting MG and significantly downregulated in MG and MGPCs from retinas treated with NMDA and/or insulin+FGF2 (Fig. 1j; supplemental table 1). CERS5 was significantly upregulated in MG at 24hrs after NMDA and MGPCs compared to resting MG and MG treated with insulin and FGF2 (Fig. 1j; supplemental table 1).
We next analyzed the expression of S1P-related genes in a scRNA-seq database that we generated for early time-points, 3 and 12 hours, after NMDA-treatment (Campbell et al., 2021b; Campbell et al., 2022; El-Hodiri et al., 2023). These scRNA-seq libraries did not integrate well with older libraries likely because these libraries were generated with different reagents with different sensitivities. UMAP ordering of cells revealed distinct clusters of neurons and glia, with MG forming distinct clusters based on time after NMDA-treatment (Fig. 1k,l). Resting MG were identified based on high levels of expression of genes such as GLUL and RLBP1, activated MG were identified based of high levels of expression of genes such as TGFB2 and PMP2, and proliferating MGPCs were identified based on high levels of expression of CDK1 and TOP2A (supplemental Fig. 1). Consistent with previous observations, S1PR1 was highly and exclusively expressed by resting MG and is rapidly (<3hrs) downregulated following NMDA-induced damage (Fig. 1m; supplemental Fig. 1). Levels of SPHK1 were very low in this aggregate scRNA-seq library possibly because the transcripts are very low-copy or the mRNA is labile (not shown). SGPL1 and ASAH1 are rapidly downregulated, and CERS6 is upregulated at different times after NMDA-treatment (Fig. 1e,f,m,n), suggesting a downregulation of S1P levels following damage in the chick retina.
In microglia, levels of ASAH1 and SGPL1 were significantly increased at 48hrs after NMDA-treatment (Fig. 1n; supplemental table 1). In cone photoreceptors, only ASAH1 was significantly decreased following NMDA-treatment (Fig. 1n; supplemental table 1). In bipolar cells, there were significant decreases in levels of S1PR1 and CERS6 following NMDA-treatment (Fig. 1n; supplemental table 1). In amacrine cells, there were significant decreases in levels of S1PR1, ASAH1 and CERS6 following NMDA-treatment (Fig. 1n; supplemental table 1). In RGCs, there were significant decreases in expression levels of CERS6 and SGPL1 at different times after NMDA-treatment (Fig. 1n; supplemental table 1). There were no significant changes in S1P-related genes in rod photoreceptors or horizontal cells in damaged retinas (not shown). Collectively, these findings indicate that there is dynamic expression of genes related to S1P synthesis and degradation in retinal neurons, and this may impact signaling through S1PR1 in MG.
Validation of patterns of expression of S1PR1, S1PR3, and SPHK1:
To validate some of the findings from scRNA-seq libraries, we performed fluorescence in situ hybridization (FISH) on normal and NMDA-damaged retinas. We applied antibodies to S1pr1 and Sphk1(Santa Cruz, sc-48356; Novus, NB120-11424; Bioss, bs-2652R), but these antibodies did not reveal plausible patterns of labeling (not shown). By comparison, FISH for S1PR1 revealed distinct puncta that were concentrated around the Sox2-positive nuclei of resting MG in undamaged retinas, consistent with scRNA-seq data (Fig. 2a,b). 100% of the Sox2-positive MG nuclei in the INL were associated with S1PR1 FISH puncta (Fig. 2b). In damaged retinas at 3 HPI (hour post injury), S1PR1 was significantly reduced in the INL and very few puncta were observed in close proximity to MG nuclei (Fig. 2b). At 48 and 72 HPI, S1PR1 signal increased and was observed with Sox2+ nuclei of MG that were delaminated away from the middle of the INL (Fig. 2b). In undamaged retinas, we found very few S1PR3 FISH puncta associated with MG nuclei and across the retina (Fig. 2c,d). In contrast, we identified S1PR3 puncta associated with some MG nuclei at 48 HPI; these results are consistent with scRNA-data (Fig. 2d). In undamaged retinas, we found SPHK1 FISH puncta associated with MG nuclei, consistent with scRNA-seq data (Fig. 2e,f). At 48HPI, we observed an increase in SPHK1 FISH puncta associated with delaminating MG nuclei, which was similar to findings from scRNA-seq data (Fig. 2e,f).
Activation of cell signaling pathways by S1P
S1P signaling is known to activate different cell signaling pathways including MAPK and PI3K/mTor, and crosstalk with pro-inflammatory pathways such as NFκB (reviewed by Cui et al, 2021). Alternatively, activation of S1PRs can activate Jak/Stat-signaling, which upregulates the immediate early gene Egr1 (Gurgui et al., 2010; Liang et al., 2013; Sato et al., 2000). To probe for the activation of different cell signaling pathways in the retina, we delivered S1P to undamaged eyes and collected retinas 24hrs later. In retinas treated with exogenous S1P, levels of pS6 and pSTAT3 levels were significantly increased in MG (Fig. 3a,b). By comparison, levels of pERK1/2 and cFos were unaffected by S1P-treatment (Fig. 3a,b). We did not observe significant changes in the total number of microglia in the retina, indicating that S1P delivery did not initiate any recruitment of macrophages into the retina (Fig 3c,d). However, we found that S1P-treatment significantly increased the accumulation of microglia to the inner limiting membrane (Fig 3c,d). Collectively, these data indicate that the signaling pathways activated by S1P include Jak/Stat and mTOR, but not MAPK. These pathways are predominantly activated in MG, and high levels of S1P may elicit a migratory response in resident retinal microglia. S1P receptor transcripts are not highly expressed in microglia (see Figure 1); it is most probable that this response is elicited indirectly through S1PRs expressed by MG and secondary production of chemotactic signaling. There are no reliable cell-level readouts of NFkB-signaling in the chick retina (Palazzo, 2020). Thus, we did not probe for activation of NFkB in retinas treated with S1P.
S1P signaling and the formation of proliferating MGPCs
We next investigated how activation or inhibition of S1P-signaling influences the formation of proliferating MGPCs in damaged retinas. To test how S1P-signaling influences the formation of MGPCs, we applied different small molecule agonists and antagonists to different enzymes and receptors involved in S1P signaling before, with and after NMDA-treatment (Fig. 4a). We found that the S1PR1 agonist SEW2871 significantly reduced numbers of EdU+Sox2+ MGPCs in damaged retinas (Fig. 4a,c).
Consistent with these findings, S1PR1 antagonists, MT1303 and NIBR-0213, significantly increased numbers of proliferating MGPCs in damaged retinas (Fig. 4a,d,e). Similarly, S1PR1/3 antagonist, VPC23019, significantly increased numbers of proliferating MGPCs (Fig. 4a,f). S1P-receptor modulator, FTY720, significantly reduced numbers of proliferating MGPCs (Fig. 4a,h). FTY720 is known to act as an agonist at S1P receptors and then induce internalization and deactivation after continuous exposure, whereas other agonists are believed to induce persistent signaling (Jo et al, 2005; Sykes et al, 2014). Inhibition of SPHK1 with PF543 or SKI-1788, which are expected to decrease levels of S1P, significantly increased numbers of proliferating MGPCs (Fig. 4a,h,i) By comparison, inhibition of SGPL1 with S1PL-in-31, which is expected to increase levels of S1P, significantly decreased in numbers of proliferating MGPCs (Fig. 4a,b,j).
To corroborate findings from EdU incorporation studies, we probed for numbers of MGPCs that were labeled for neurofilament, Sox9 and phospho-histone H3 (pHisH3). MGPCs are known to upregulate neurofilament and pHisH3 during late G2 and M phase of the cell cycle at 3 days after NMDA-treatment (Fischer and Re, 2001; Zelinka et al., 2016; Palazzo et al., 2020). Consistent with findings from EdU-incorporation, we found significant increases in numbers of MGPCs labeled for Sox9, neurofilament and pHisH3 in damaged retinas treated with S1PR1 antagonist (MT1303) or SPHK1 antagonist (PF543) (Fig. 4k,m,o). Further, we found significant decreases in numbers of MGPCs labeled for Sox9, neurofilament and pHisH3 in damaged retinas treated with S1PR1 modulator (FTY720) or SGPL1 antagonist (S1PL-in-31; Fig. 4n,p).
None of the agonists or antagonists had a significant effect on the proliferation of microglia/macrophage in NMDA-damaged retinas (supplemental Fig. 2a-g). Similarly, except for the S1PR1 antagonist MT1301, none of the agonists or antagonists significantly affected numbers of dying cells (supplemental Fig. 3a-f). In damaged retinas treated with MT1303 we found a significant decrease in numbers of TUNEL-positive cells in the inner INL (supplemental Fig. 2a,c). In summary, treatments that increase levels of S1P or activate signaling through S1P-receptors result in decreased proliferation of MGPCs, whereas treatments that decrease levels of S1P or inhibit signaling through S1P-receptors result in increased proliferation of MGPCs, without significant effects upon cell death or the proliferation/accumulation of microglia.
Ceramide synthesis and ceramidase genes have variable patterns of expression in the resting and damaged chick retina (Fig. 1). S1P and ceramides have been described as a rheostat that regulates cell survival; S1P is protective, and ceramides trigger apoptotic pathways (Simón et al., 2019). ASAH1 (acid ceramidase) acts to restrict ceramide accumulation and is dynamically regulated in the chick retina (Fig. 1). To investigate whether ceramide accumulation regulates cell survival and MGPC proliferation, we applied an acid ceramidase inhibitor (Ceranib-2) before and following NMDA treatment (supplemental Fig. 4). We observed no significant differences in cell death, microglia reactivity, MGPC proliferation between Ceranib-2 treated retinas and control damaged retinas (supplemental Fig. 4). Thus, ceramide accumulation may not impact cell survival or the responses of MG to retinal damage.
Cell signaling downstream of SPHK1 inhibition in damaged retinas
There are several known downstream targets of S1PR1 signaling which may be active in MG after retinal damage. To identify second messenger pathways that were affected by diminished levels of S1P in damaged retinas, we applied SPHK1 inhibitor before, with and after NMDA-treatment and collected retinas 24 HPI. We found a significant decrease in levels of ATF3, pS6, and pSmad1/5/9 in MG in damaged retinas treated with SPHK1 inhibitor (Fig. 5a-e). By comparison, phosphorylated ERK1/2 and cFos were not significantly different in MG in damaged retinas treated with SPHK1 inhibitor (supplemental Fig. 5a,b). These findings were relatively consistent with our previous findings, where mTOR activation was observed with exogenous S1P treatment, but there was no change to pERK1/2 or immediate early gene cFOS (Figure 3).
Next, we sought to validate S1P levels using liquid chromatography-mass spectrometry (LC/MS). We collected whole retinas 48 hours after saline treatment, Sphk1-inhibitor (PF543) treatment, NMDA treatment, NMA + PF543 treatment, or NMDA + S1P lyase inhibitor (S1PLin31) treatment. As predicted, Sphk1 inhibitor treatment decreased levels of S1P in undamaged retinas (Fig 5e). We found that S1P levels increased in NMDA-treated retinas, which correlated well with increased Sphk1 transcript levels after damage. Surprisingly, SPHK1 inhibitor treatment was not sufficient to ameliorate high levels of S1P induced by NMDA. It is possible that the effects of PF-543 (koff t1/2=8.5 min) subsided in the 24 hours prior to tissue collection. Alternatively, this observation may reflect the rapid and transient nature of SPHK1 activity after damage, which is consistent with prior experimental observations; we found that S1P/S1PR1-targeting drugs had to be applied prior to NMDA damage to produce robust effects on MGPC proliferation (data not shown). S1P lyase inhibitor treatment robustly boosted levels of S1P in damaged retinas (Fig 5f). In summary, differences in levels of S1P between undamaged retinas and NMDA treatment are consistent with observed Sphk1 RNA levels (Fig. 2e,f). Further, we validated the targeting activity of two drugs, PF543 and S1PLin31.
Inhibition of S1P signaling and neurogenesis
We next investigated whether S1P signaling affects the neural differentiation of MGCPs after NMDA-treatment. We find that levels of S1PR1 were rapidly downregulated in activated MG but later rose in MG returning to resting, and S1PR3 was highly expressed in a percent of MGPCs (see Fig.1). We hypothesized that S1P receptor activity during this period of cell-fate specification of MGPC progeny may restrict neural differentiation. We applied S1P pathway inhibitors starting 2 days after NMDA, after MG have committed to cell cycle re-entry (Fischer and Reh, 2003). We found that SPHK1, S1PR1, and S1PR1/3 inhibitors applied after NMDA had no significant effect on the proliferation of MGPCs (Fig. 6a,b). We found a significant increase in EdU+ amacrine-like cells that express HuC/D (Fig 6c,d). There was no significant difference in new Calretinin+ (Fig 6e,f) or Ap2a+ neurons (not shown) across treatment groups. Further, we found that while many EdU+ progeny migrated distally into the ONL, these cells did not co-label for the photoreceptor marker visinin (Fig 6g). These findings suggest that inhibiting S1P synthesis or receptor activity enhances the neural differentiation of MGPC progeny to differentiate into HuC/D+ amacrine-like neurons after retinal damage. However, the increase in differentiation of amacrine-like cells did not include differentiation of subsets of amacrine cells that express Ap2a or calretinin.
Inhibition of S1P signaling rescues MGPC proliferation in damaged retinas missing microglia
In chicks and zebrafish, depletion of microglia prior to damage stunts the formation of MGPCs and neural regeneration in the retina (Fischer et al., 2014; Huang et al., 2012). We have previously identified several factors that can “rescue” reprogramming in the absence of microglia, including NFkB activators, FGF2, and HBEGF (El-Hodiri et al., 2023; Palazzo et al., 2020). In addition, we have found increased numbers of dying cells in NMDA-damaged retinas missing microglia (Todd et al., 2019). Given that S1P signaling is known to be involved in regulating inflammatory responses involving immune cells (Obinata and Hla, 2019), we sought to determine whether the ablation of microglia/macrophages from the retina influenced the expression of S1P-related genes. Accordingly, we probed scRNA-seq libraries of normal and damaged retinas with and without microglia (saline and clodronate saline, respectively); the generation of these libraries has been described previously (El-Hodiri et al., 2023), In short, eyes were treated with saline or clodronate liposomes at P6, treated with saline or NMDA at P10, and retinas were harvested at P11. Consistent with previous reports (Fischer et al., 2014; Zelinka et al., 2012), a single intravitreal injection of clodronate-liposomes effectively eliminated >99% of microglia from the retina (not shown). Analyses of scRNA-seq libraries of MG from undamaged and NMDA-damaged retinas with and without microglia showed that many components of S1P signaling were upregulated in resting MG in undamaged retinas (Fig 7a-i). These genes included S1PR1, S1PR3, SPHK1, SGPL1 and ASAH1 (Fig. 7d-i). Notably, S1PR1 expression was significantly diminished in undamaged retinas treated with clodronate (microglia-ablated) (Fig. 7d,j). Interestingly, CERS6 was significantly upregulated in MG and other retinal cells in undamaged saline clodronate retinas (Fig. 7j-m). In MG other S1P-related factors that were up- or downregulated with NMDA-treatment were not significantly affected by the ablation of microglia. However, in neuronal cells many factors (including SPGL1) normally upregulated with NMDA showed diminished levels of expression when microglia were absent, indicating that microglial reactivity is a driver of S1P metabolism in retinal neurons (Fig 7k-m).
We next tested whether intravitreal injections of inhibitors to SPHK1 and S1PR1 rescued the deficit in MGPC proliferation and increased cell death in damaged retinas missing microglia. As described previously, delivery of clodronate liposomes prior to damage dramatically reduced numbers of EdU+ MGPCs (Fig. 8a-d). However, injections of S1PR1 or SPHK1 inhibitors with and following NMDA significantly increased numbers of proliferating MGPCs in retinas missing microglia (Fig. 8a,b,c,d). However, the number of proliferating MGPCs in S1P inhibitor-treated retinas was significantly lower than in NMDA-treated retinas with activated microglia (Fig. 8b,c,d), indicating a partial rescue of MGPC proliferation. Reactive microglia appear to support neuroprotection in the mouse retina (Todd et al., 2019), but exacerbate NMDA-dependent cell death in the chick retina (Fischer et al., 2015). Interestingly, we found that there were differences in cell death between different S1PR1 inhibitors. Similar to retinas where microglia were present (supplemental Fig. 3a,c), there were significantly fewer TUNEL+ nuclei in retinas treated with MT1303 compared to numbers seen in control clodronate/NMDA retinas (Fig 8e). However, NIBR0213-treated retinas without microglia contained higher numbers of TUNEL+ nuclei (Fig 8f), suggesting that the two S1PR1 inhibitors may have different specificities or toxicities. We found that SPHK1 inhibitor-treated retinas had less cell death compared to clodronate/NMDA retinas (Fig 8g). In summary, these findings indicate that S1P-signaling is regulated by signals produced by microglia in the retina, and inhibition of S1P-signaling is partially rescues the proliferation of MGPCs and reduces cell death in microglia-depleted retinas.
In retinas where microglia have been ablated, levels of S1PR1 may be transcriptionally maintained by microglia:MG communication in resting conditions. One of the top inferred ligand:receptor interactions identified between resting microglia and MG is TGFB1:CD109 (El-Hodiri et al., 2023). Additionally, we have previously shown that TGFβ2 suppresses MGPC proliferation via pSmad3; inhibition of Smad3 by the small molecule inhibitor SIS3 stimulates MGPC proliferation in damaged retinas (Todd et al., 2017). Thus, we tested whether TGFβ/Smad3-signaling regulates levels of S1PR1 in resting MG. We intravitreally delivered SIS3 to retinas at P7 and P8, then harvested retinas at P9. Consistent with earlier findings (Fig. 2), numerous S1PR1 FISH puncta were associated with Sox2+ MG nuclei in the middle of the INL in undamaged retinas (Fig. 9a). SIS3 treatment significantly reduced numbers of S1PR1 puncta in the INL of undamaged retinas (Fig. 9a,b). These findings suggest that TGFβ/Smad3-signaling between microglia and MG maintains high levels of S1PR1, and the proliferation-inducing effects of Smad3-inhibition may, in part, be mediated by downregulation of S1P-signaling in MG.
Patterns of expression for S1P-related genes in human and zebrafish retinas
Comparative analyses of expression have proven useful in implicating important genes with highly conserved patterns of expression. For example, we have reported that NFIA and NFIB show similar patterns of expression in MG of zebrafish, chicks, mice, and large mammals early after retinal damage (Clark et al., 2019; El-Hodiri et al., 2022; Hoang et al., 2020). However, Nfib is upregulated in non-neurogenic mouse MG returning to a resting state after NMDA, whereas NFIA/B/X expression is lowered in late neurogenic MGPCs of chicks and zebrafish (Hoang et al., 2020). These comparative studies led to the development of Nfia/b/x;Rbpj cKO mice in which ∼45% of targeted MG transdifferentiate into neurons without retinal damage (Le et al., 2023). Accordingly, we sought to compare patterns and levels of expression of S1P-related genes in human and zebrafish retinas.
We interrogated snRNA-seq libraries of human retinas generated by Dr. Rui Chen’s group (Li et al., 2023). UMAP ordering of cells revealed discrete clusters of all major retinal cell types (Fig. 10a). A large distinct cluster of MG was distinguished based on high levels of expression of GLUL and RLBP1 (Fig. 10b). Some of these MG expressed genes associated with an activated phenotype including TGFB2 and HBEGF, and these cells coincided with diminished expression of GLUL and RLBP1 (Fig. 10b,c). Similar to patterns of expression seen in the chick retina, S1PR1 and S1PR3 were detected in putative resting and activated MG, respectively, whereas S1PR2 was not widely expressed (Fig. 10d). Similar to patterns of expression seen in chick retinas, SGPL1 was detected in rod photoreceptors and a few cells scattered among the different clusters of inner retinal neurons and MG (Fig. 10e). Unlike patterns of expression seen in chick retinas, SPHK1 was detected in putative activated MG (Fig. 10e). In addition, S1PR3 and SPHK1 were detected in human retinal astrocytes (Fig. 10d,e).
We next interrogated snRNA-seq libraries of zebrafish retinas recently described and generated by the Lyu and colleagues (Lyu et al., 2023). UMAP ordering of this large aggregate library revealed distinct clusters of all major retinal cell types (Fig. 10f). MG, MGPCs and differentiating progeny formed distinct clusters and “branches” of UMAP-ordered cells (Fig. 10f-h), and these clusters contained cells from different times after light damage and NMDA-treatment (not shown). Resting MG formed a distinct cluster of cells that expressed high levels of glula and rlbp1a (Fig. 10g). The resting MG were contiguous with a “branch” of cells that extended in MGPCs that expressed top2a and ascl1a (Fig. 10h). The UMAP “branches” of cells represent a continuum of phenotypes shifting from resting MG to MGPCs to differentiation of progeny stretched across different times after light- and NMDA-damage. The MGPCs were contiguous and extended into branches that included differentiating amacrine cells, bipolar cells, rod photoreceptors, and cod photoreceptors that expressed neurod1 and neurod4 (Fig. 10h). Similar to patterns of expression seen in chick and human retinas, s1pr1 was observed at high levels in resting MG and was downregulated in MGPCs (Fig. 10i). In addition, s1pr1 was observed in a branch of cells projecting from the MGPCs into putative differentiating amacrine cells (Fig. 10i). By comparison, s1pr2 was detected in microglia and horizontal cells (Fig. 10i). s1pr3a and s1pr3b were not detected at significant levels (not shown). Similarly, sphk1 was detected in very few cells in the retina (Fig. 10j). By comparison, sphk2 was detected in a few bipolar cells and rod photoreceptors (Fig. 10j). Similar to patterns of expression seen in chick and human retinas, sgpl1 was detected in microglia and a few cells scattered among the different clusters of inner retinal neurons and rod photoreceptors (Fig. 10j). Collectively, these findings indicate that S1PR1 is expressed by resting MG in the retinas of different vertebrate classes, suggesting conservation of cells, and possibly functions, of S1P-signaling and degradation in the vertebrate retina.
Discussion
Pro-inflammatory signaling acts differentially across species to influence the regenerative capacity of MG after damage. It is important to understand how pro-inflammatory signaling fits into the complex network of pathways that control MG reprogramming. We provide evidence that S1P signaling is among the network of pro-inflammatory pathways the regulate the responses of MG to retinal damage. Here, we report patterns of expression of S1P signaling components and the effects of activating or inhibiting S1P signaling on regeneration in the chick retina. This study highlights the significant role of S1PR1, which is highly expressed in resting MG and non-neurogenic MGPCs, in suppressing damage-dependent MGPC proliferation and neuronal differentiation. Inhibition of S1PR1 promoted MGPC cell cycle re-entry and enhanced the number of regenerated amacrine-like cells after retinal damage. Inhibition of S1P synthesis produced similar effects to inhibiting S1PR1 to promote MGPC formation, and inhibiting S1P degradation produced similar effects to activating S1PR1 to inhibit MGPC formation.
Regulation of S1PR1 Expression
The identity of factors that downregulate S1PR1 in MG in damaged retinas remains uncertain. Similarly, the identity of the factors that maintain S1PR1 expression in MG in undamaged resting retinas remains uncertain. Previous studies have found S1P production and S1P receptor activation are regulated by several growth factor receptors, including EGFR and VEGFR (Igarashi et al., 2003; Paugh et al., 2008; Sukocheva et al., 2006). In the current study, FGF and insulin treatment were sufficient to downregulate S1PR1 without retinal damage. Further, we found that TGFβ-dependent Smad3 activity stimulates S1PR1 expression in resting retinas. These findings support prior in vitro studies which report that TGFβ treatment robustly drives upregulation of S1PR1-3 mRNA and protein (Lin et al., 2022; Yang et al., 2018). We have previously reported that TGFβ1 is expressed by microglia and TGFβ3 is expressed by neurons in resting retinas, and TGFβ-treatment in damaged retinas suppresses MGPC formation (El-Hodiri et al., 2023; Todd et al., 2017). Thus, homeostatic TGFβ/Smad2/3 signaling between microglia and Muller glia may maintain S1PR1 expression to promote quiescence in MG.
Several TFs have been found to influence S1PR1 expression. KLF2, FOXF1, STAT1, and YAP have been found to directly bind to the S1PR1 promoter to positively regulate transcription (Cai et al., 2016; Carlson et al., 2006; Tao et al., 2023; Xin et al., 2020; Zheng et al., 2023). Notably, due to the sequestering of NFκB co-activators by KLF2, S1PR1 transcription is linked to the silencing of NFκB-related pro-inflammatory genes (Jha and Das, 2017). Conversely, S1PR1 activity has been shown to promote downstream NFκB-mediated gene transcription (Rostami et al., 2019). Thus, signaling through S1PR1 is part of an intricate bidirectional regulatory network that imparts influence through the NFκB pathway. Taken together with present findings, this is consistent with the reported roles of NFkB signaling in rapid microglia-mediated activation of MG and thereafter suppression of MGPC formation in damaged retinas (Palazzo et al., 2020).
S1PR1 activation and downstream inflammatory signaling
We and others have reported that inflammatory cytokine signaling is necessary for the initiation of Muller glia cell-cycle re-entry in chicks and zebrafish (Fischer et al., 2014; Silva et al., 2020), but persistent microglial reactivity and NFκB signaling suppress MG reprogramming (Palazzo et al., 2020; White et al., 2017). In the current study, we report that S1PR1 activity suppresses MGPC proliferation and neurogenesis without impacting microglia. We report differential activation of Jak/Stat, mTOR, and Smad pathways in MG treated with exogenous S1P or SPHK1 inhibitor. These pathways are activated following NMDA-treatment and are necessary for MGPC formation (Todd et al., 2016; Todd et al., 2017; Zelinka et al., 2016).
S1PR1 inhibitors and NFκB inhibitors produce similar effects on MGPC proliferation in damaged retinas (Palazzo et al., 2020). In the absence of microglia, S1PR1 inhibition promoted damage-dependent MGPC formation but application of an NFκB activator was found to increase MGPCs. A comparison of these findings may support the notion that NFκB signaling must be transiently activated to initiate dedifferentiation but must be later suppressed to release the glial phenotype and permit cell-cycle reentry. It is probable that S1PR1 activation potentiates downstream NFκB signaling to suppress regeneration, but we could not confirm this in the current study; we have not identified antibodies to NFκB pathway components that produce plausible patterns of expression in chick retinas.
S1P and neuronal differentiation
We found that inhibitors to SPHK1, S1PR1 or S1PR1/3 increased numbers of cells that differentiated as amacrine-like cells that expressed HuC/D. However, none the progeny of MGPCs differentiated into cells that expressed calretinin (a subset of amacrine cells) or visinin (photoreceptors). There is currently no evidence that MGPCs in the chick retina can produce progeny that differentiate into photoreceptors. By contrast, we recently reported that inhibition of ID factors enhances neuronal differentiation of calretinin-expressing MGPC-derived cells (Taylor et al., 2024).
Calretinin may be expressed by a subset of amacrine cells not specified by inhibition of S1P receptors. Alternatively, the progeny of MGPC do not fully differentiate to the point where calretinin is expressed when S1P signaling is diminished. Control over the differentiation of MGPC progeny is regulated by different cell signaling pathways. For example, activation of retinoic acid receptors stimulates neuronal differentiation (Todd et al., 2018), whereas signaling through Notch (Ghai et al., 2010; Hayes et al., 2007), glucocorticoid receptors (Gallina et al, 2014), and Jak/Stat3 pathway (Todd et al., 2016) suppress neuronal differentiation. It is possible that activation of S1P receptors acts through Jak/Stat3 or possibly NFκB to suppress the neuronal differentiation of MGPC progeny. Our data indicate that S1PR1 is downregulated by activated MG and proliferating MGPCs. However, S1PR3 is upregulated in MGPCs and, thus, it is likely that signaling through S1PR3 mediates the cell fate specification of MGPC progeny.
S1P signaling & neuroprotection
The current study provides evidence that inhibition of the S1P pathway supports neuron survival in the damaged chick retinas. In retinas where microglia were absent, we found that SPHK1 inhibitor PF543 and S1PR1 inhibitor MT1303 alleviated retinal cell death. In retinas where microglia were present, only MT1303 significantly reduced numbers of dying cells. As mentioned previously, NFκB-related genes are regulated in a similar pattern to S1P-related genes; inhibiting NFκB signaling supports inner retinal cell and retinal ganglion cell survival (Palazzo et al., 2020). In contrast, we recently reported that Inhibitor of DNA-binding 4 (ID4) factor is transiently upregulated in MG after NMDA and may support the survival of inner retinal neurons (Taylor et al., 2024). Other factors such as fatty acid binding proteins (FABPs) and Midkine are also rapidly upregulated in activated MG and these factors are neuroprotective (Campbell et al., 2021a; Campbell et al., 2022).
Interestingly, one of the S1PR1 inhibitors, NIBR0213, increased cell death in damaged retinas where microglia were absent. This disparity might be explained by differences in inhibitor specificity. MT1303 is a potent functional antagonist which induces receptor internalization and degradation, whereas NIB0213 is slightly less potent and does not drive internalization (Quancard et al., 2012; Shimano et al., 2019). Further, MT1303 is a prodrug (requiring phosphorylation) and has an elimination half-life of several days, whereas direct-acting NIBR0213 has a half-life of a few hours (Quancard et al., 2012; Shimano et al., 2019). Studies in mice suggest that sphingosine kinase and receptor inhibition ameliorate the death of retinal ganglion cells following NMDA-treatment (Basavarajappa et al., 2023; Nakamura et al., 2021). Interestingly, studies have described the neuroprotective effects of fingolimod (S1PR1 modulator) in models of glaucoma in rodents (Shiwani et al., 2021). However, we did not find any effect of fingolimod on cell death.
S1P activity in retinal neurons and microglia
Although S1PR1 expression was predominantly observed in MG, S1P signaling components were not restricted to these glial cells. We found that SPHK1, which catalyzes the synthesis of S1P from sphingosine, was expressed by cells scattered across different types of retinal cells. Further, SGPL1, which catalyzes the degradation of S1P, had dynamic patterns of expression following NMDA-treatment in different types of retinal cells, including amacrine cells and microglia. These finding suggest that S1P is secreted by these cells to bind to S1P receptors on MG. S1P:S1PR paracrine signaling has been observed between neural cells and astrocytes and is hypothesized to be necessary for proper astrocyte morphogenesis during synapse formation (Alam et al., 2023; Singh et al., 2022). Another possibility is that S1P produced by SPHK2. However, SPHK2 is not annotated in the Gallus gallus genome, and we could not identify any genes that aligned significantly with SPHK2 from other bird species. Further, this gene was not expressed at significant levels in scRNA libraries created from mouse, zebrafish, or pig retinas. A final possibility is that changes in S1P metabolism in retinal neurons are a byproduct of the recycling of other sphingolipid molecules in response to NMDA damage.
The sphingolipid “rheostat” in the retina
S1P synthesis is dependent on the availability of ceramides and ceramide-related enzymes like acid ceramidase (ASAH1). Whereas S1P signaling triggers cell cycle re-entry, ceramide accumulation drives cellular senescence (Simón et al., 2019). Similarly, the protective effects of S1P are countered by ceramides, which activate intrinsic and extrinsic apoptotic pathways (Simón et al., 2019).. There is significant evidence that ceramide production must be tightly restricted by acid ceramidase, which converts ceramide into sphingosine, for retinal neurons to survive excitotoxic and hypoxic stress (Lewandowski et al., 2022; Nakamura et al., 2021; Sugano et al., 2019; Yu et al., 2019). Multiple groups have found that Cer 16:0 and CERS5 are markers for astrocytic inflammation and that astrocytic ceramide production is stimulated by TNF-α (de Wit et al., 2019; Fan et al., 2021; Kimura et al., 2000). In the current study, we observed dynamic regulation of ASAH1 expression after damage in the chick retina.
However, application of a small molecule inhibitor to acid ceramidase had no significant effect on numbers of MGPCs or dying cells (supplemental Fig. 4). Many studies have described the effects of ceramides on neuron survival, but additional research is needed to investigate the functional role of ceramides as part of the inflammatory and apoptotic signaling cascades in glial cells.
Conclusions
In summary, our findings indicate that S1P:S1PR1 signaling plays significant roles in the initiation of MG dedifferentiation, formation of proliferating of MGPCs and specification of progeny toward a neurogenic identity. Our findings suggest that S1PR1 activity maintains quiescence in MG and acts to drive activate toward a resting phenotype. The expression of S1PR1 is regulated by microglia, neuronal damage and TGFβ/Smad3 signaling. Inhibitors to S1P synthesis or S1PR1 signaling promoted MGPC cell cycle re-entry and enhanced neural differentiation. Interestingly, patterns of expression of S1P-related genes are highly conserved across vertebrates, namely high levels of expression of S1PR1 in the MG in chick, fish and human retinas. Activation of S1PR1 in MG is one of the key pro-inflammatory signaling pathways that control glial responses to neuronal damage, microglial activation, and the ability of MG to reprogram into neurogenic progenitor-like cells.
Acknowledgements
We thank Dr. Timothy Hla for advice regarding different agonists and antagonists to S1P-receptors. We also wish to thank the Mass Spectrometry and Proteomics Core at the Ohio State University Campus Chemical Instrument Center for their services.
Funding Sources
This work was supported by R01 EY032141-03 (AJF). Research reported in this publication was also supported by the Ohio State University Comprehensive Cancer Center under NIH Award Number Grant P30 CA016058.
Data availability
CellRanger output files for Gene-Cell matrices for scRNA-seq data for libraries from saline and NMDA-treated retinas are available through Sharepoint links for embryonic chick retina databases: https://osumc.sharepoint.com/:f:/s/Links/Eoto-Qg2uuxDn1bHWMM6gdkBTft4S_YSBjQJResxY-qehA?e=mdaPlg and post-hatch normal and treated chick retina databases: https://osumc.sharepoint.com/:f:/s/Links/Eoto-Qg2uuxDn1bHWMM6gdkBTft4S_YSBjQJResxY-qehA?e=mdaPlg. scRNA-seq datasets are deposited in GEO (GSE135406, GSE242796) and Gene-Cell matrices for scRNA-seq data for libraries chick retinas treated with saline or NMDA retinas are available through NCBI (GSM7770646, GSM7770647, GSM7770648, GSM7770649). Cell Ranger matrix, features and barcodes files for the snRNA-seq dataset of zebrafish retinas were downloaded through GEO (GSE239410). The Seurat object for the snRNA-seq dataset of human retinas was downloaded through the CELLxGENE collection (https://cellxgene.cziscience.com/collections/4c6eaf5c-6d57-4c76-b1e9-60df8c655f1e)
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