PARP1 Activation Controls Stress Granule Assembly after Oxidative Stress and DNA Damage

DNA damage causes PARP1 activation in the nucleus to set up the machinery responsible for the DNA damage response. Here, we report that, in contrast to cytoplasmic PARPs, the synthesis of poly(ADP-ribose) by PARP1 opposes the formation of cytoplasmic mRNA-rich granules after arsenite exposure by reducing polysome dissociation. However, when mRNA-rich granules are pre-formed, whether in the cytoplasm or nucleus, PARP1 activation positively regulates their assembly, though without additional recruitment of poly(ADP-ribose) in stress granules. In addition, PARP1 promotes the formation of TDP-43- and FUS-rich granules in the cytoplasm, two RNA-binding proteins which form neuronal cytoplasmic inclusions observed in certain neurodegenerative diseases such as amyotrophic lateral sclerosis and frontotemporal lobar degeneration. Together, the results therefore reveal a dual role of PARP1 activation which, on the one hand, prevents the early stage of stress granule assembly and, on the other hand, enables the persistence of cytoplasmic mRNA-rich granules in cells which may be detrimental in aging neurons.


Introduction
Stress granules (SGs) are dynamic compartments found in the cytoplasm of eukaryotic cells in response to a wide variety of stress, including oxidative stress, hypoxia and viral infections [1]. SGs are considered dynamic and reversible compartments containing non-polysomal mRNAs, 40S ribosomal subunits, translation initiation factors and mRNAbinding proteins (RBPs) [1]. The mRNA and protein composition of SGs varies according to the type of stress at the origin of their formation, probably to coordinate a stress-specific translational response in cells [2,3]. SGs are formed following the dissociation of polysomes, which is generally orchestrated by dedicated kinases after cellular stress that blocks the initiation of translation [3,4]. The assembly of non-polysomal mRNAs in SGs is subsequently regulated by base pairings between mRNA molecules [5] and interactions between self-associated RBPs such as G3BP-1 [6][7][8], which form a bridge between molecules of mRNA. Recently, several reports have indicated that ADP-ribosyl transferases (for example, tankyrase (PARP5a), PARP12, isoforms PARP13 (1 and 2), PARP14 and PARP15) could localize to SGs and play a critical role in the regulation of cytoplasmic SG formation [9][10][11][12]. ADP-ribosyl transferases of the diphtheria toxin-like family (ARTD), also called PARPs, catalyze the transfer of ADP-ribose units from NAD + onto amino acid residues of target proteins, resulting in their (ADP-ribosyl)ation [13]. Some PARPs have the ability to covalently attach a single ADP-ribose to an amino acid residue (protein mono(ADP-ribosyl)ation, MARylation), while others attach a poly(ADP-ribose) (PAR) chain, linear or branched (protein poly(ADP-ribosyl)ation, PARylation). Since SGs are formed in the cytoplasm, most research was focused on cytoplasmic PARPs such has as PARP5a and PARP5b [12]. The action of cytoplasmic PARPs generally positively regulates SG formation and alters their ation by preventing the dissociation of pre-formed mRNA-rich granules. In the latter case, nuclear PARPs may indirectly promote the persistence of mRNA-rich protein condensates in the cytoplasm, for instance, via the PARylation of SG-related proteins, phosphorylation events or by buffering mRNA-stabilizing factors such as YB-1 or HuR.

Plasmid and siRNA Transfection
Fresh culture medium with 5% serum was added to the cells before the transient transfections. HeLa cells were transfected with 1.5 µg/mL of FUS-GFP or TDP-43-GFP encoding plasmids for each well by using the ratio of 1/1000 Lipofectamine 2000 (Thermo Fisher Scientific, Waltham, MA, USA, #11668019) and medium, respectively. The cells were analyzed at 24 h after plasmid DNA transfection. The efficiency of transfection was controlled by immunofluorescence.
For silencing, HeLa cells were then transfected with 20 nM of small interfering RNA duplex FlexiTube GeneSolution for PARP1 (QIAGEN, Hilden, Germany, #GS14) or for PARG (QIAGEN, #GS8505) by using the ratio of 1/1000 Lipofectamine 2000 and medium, respectively. A non-targeting sequence siRNA (AllStars Negative Control siRNA, QIAGEN, #1027281) was used as a negative control. Cells transfected with the siRNA were placed in an incubator for 6 h, then the medium was replaced with fresh medium with 10% FBS, and cells were incubated for 48 h.

Oxidative Stress Conditions and Drug Treatments
For oxidative stress induction, HeLa cells were treated with 300 µM or 1 mM hydrogen peroxide (H 2 O 2 ) or 300 µM sodium arsenite for the indicated period of time.
For induction of SGs in nucleus, cells were treated with 4 µM actinomycin D (ActD) (Thermo Fisher Scientific, #11805017) for 1 h before treatment with 300 µM H 2 O 2 .
For induction of SGs in cytoplasm, cells were treated for 60 min with 300 µM sodium arsenite or 200 µM puromycin (Sigma, St. Louis, MO, USA, #P9620) for 1 h before treatment with 300 µM H 2 O 2 .
To study the disassembly of SGs formed by treatment with sodium arsenite, cells were treated with 300 µM sodium arsenite for 60 min, then the culture medium was replaced with fresh medium containing DMSO (control), 300 µM H 2 O 2 or 3 µM olaparib or 300 µM H 2 O 2 , as indicated, and then the cells were left alone for one hour for further fixation and analysis.
After incubation with the drugs at indicated time points, the cells were washed with PBS and fixed with 4% paraformaldehyde (PFA) in PBS for 45 min at 37 • C, if another cell fixation method is not indicated.

Immunofluorescence Staining and Image Analysis
For PAR (PAR Affinity Rabbit Polyclonal Antibody, Trevigen, Gaithersburg, MD, USA, #4336-BPC-100) or MAR/PAR (Poly/Mono-ADP Ribose (E6F6A) Rabbit mAb, Cell Signaling, Danvers, MA, USA, #83732) immunofluorescence staining, cells were fixed with 100% ice-cold methanol for 15 min at −20 • C and then washed with PBS and additionally fixed with 4% paraformaldehyde (PFA) in PBS for 20 min at 37 • C. After washing with PBS, coverslips were kept with blocking buffer (50 mM Tris pH 7.5, 100 mM NaCl, BSA 2%, 0.15% Triton X-100) for 40 min at 37 • C in order to permeabilize the cells and reduce nonspecific recognition by antibodies. Blocking buffer was removed and cells were washed and then incubated for 1 h at room temperature with primary antibodies diluted in blocking buffer. The cells were washed 5 times with PBS and incubated for 1 h with secondary antibodies (Goat anti-Rabbit IgG (H + L), Alexa Fluor 594, #11012 or Goat anti-Mouse IgG1, Alexa Fluor 488, #21121, both from Thermo Fisher Scientific) in 50 mM Tris  After final washes with PBS, the cells were stained with 300 nM DAPI to visualize  the nuclei and mounted for fluorescence microscopy analysis. For anti-HA-tag (HA-Tag Antibody, Santa Cruz, CA, USA, #sc-7392) or anti-PARP1 (rabbit polyclonal, Santa Cruz, CA, USA, #sc-7150) immunofluorescence staining, cells were washed with PBS and fixed with 4% paraformaldehyde (PFA) in PBS for 45 min at 37 • C.
The measurements of PAR, MAR/PAR, FUS, TDP-43 and mRNA inside SGs and nuclear granules were defined as the immunofluorescence signal of anti-PAR, anti-PAR/MAR, anti-HA-tag or mRNA (oligo d(T)40 Cy3-conjugated oligonucleotides, Sigma) minus the integrated intensity in the surrounding cytoplasmic (or nuclear) background and were performed using the "CellProfiler" software (version 4.0.7), Broad Institute, Cambridge, MA, USA, https://cellprofiler.org/, 2020 year). SGs, nuclear granules and protein-rich condensates were identified using the "CellProfiler" software as areas close in shape to a sphere or oval and in which the intensity of the detected mRNA exceeded the intensity of the background by 1.2-2 times or more.

RNA Hybridization In Situ
In situ hybridization was performed to image poly(A) mRNA in HeLa cells as follows. Cells were fixed with 4% PFA as explained above. Cells were then incubated with 100% ice-cold methanol for 10 minutes at −20 • C, in ice-cold 70% ethanol for 10 min at −20 • C, and then 1 M Tris-HCl pH 8.0 for 5 min. Poly(T) conjugated to Cy3 (cy3-labelled poly(dT), 40 nucleotides) at 1 µg/µL in the hybridization buffer (0.005% BSA, 1 mg/mL yeast RNA, 10% dextran sulfate, 25% formamide in 2XSSC) was then used to reveal mRNAs. Slides were then placed in a humidity chamber for 1 h at 37 • C with gentle shaking. Following hybridization, cells were washed twice with 4X SSC buffer and once with 2X SSC buffer. After cells were stained with 300 nM DAPI to visualize the nuclei, they were directly mounted for fluorescence microscopy analysis or were proceeded to incubation with primary antibodies (as described above) to obtain immunofluorescence staining of PAR and proteins.

Preparation of Extracts and Polysome Fractionation Analysis
Polysome fractionation analysis was performed as previously described [33]. Briefly, to prepare the cytoplasmic extract, HeLa cells were grown on 15 cm Petri dishes with 70% coverage (approximately 13 million cells per dish) and treated with reagents as indicated and described in the cell culture section. Next, the cells were treated with cycloheximide (Apexbio Technology, #A4154) [33] before cell dissociation from the dish surface according to the standard protocol of trypsin cell culture, after which the cells were centrifuged, lysed and fractionated to obtain cytoplasmic extract by using specific buffer conditions and the procedure fully described in the protocol [33]. After that, the cytoplasmic cell extracts were applied to the sucrose gradient (10-50%) in the buffer conditions according to the protocol [33] and centrifuged at 18,000× g rpm in a Beckman SW40Ti swinging-bucket rotor for 11 h at 4 • C.
Next, the sucrose gradient was fractionated using a "Milichrom" microcolumn liquid chromatograph equipped with a UV detector to monitor the UV adsorption profile at 260 nm in order to obtain a sedimentation curve of the mRNA in the sucrose gradient. Sedimentation curves were drawn (polysome profile) representing the amount (adsorption intensity on 260 nm) of mRNA distributed according to the sedimentation coefficient, which depends on the mass and size of the mRNA and mRNA-polysome complexes.
The polysome profile for each sample includes fractions without ribosomal material, and fractions with 40S, 60S complexes or 80S (monosome), and low-and high-molecularweight polysomes. The distribution of mRNA fractions and mRNA-polysome complexes in whole extracts from cells treated with various reagents (300 µM arsenite, 300 µM H 2 O 2 , 200 µM puromycin, 10 µM olaparib.) can be compared between themselves and relative to the control profile obtained in this experiment [33]. For analysis and comparison of the relative amount of polysomes in cell extract samples, the area under the sedimentation curve occupied by the polysome and the 80S monosome fractions in OD 260 absorbance profile was measured and then normalized to the area under the total absorbance of the sample at 260 nm. The polysomal fraction corresponds to the translated mRNA, and 80S corresponds to the untranslated mRNA fractions and allows us to make a relative assessment of the level of association of polysomes in the cell.

Activation of PARP1 following Oxidative DNA Damage Prevents Arsenite-Induced SG Formation and Influences Polysome Dissociation
Arsenite is a potent inducer of SGs that triggers the rapid phosphorylation of the eukaryotic translation initiation factor 2A (eIF2A), which inhibits translation initiation. The ensuing polysome dissociation resulting from arsenite treatment then leads to the formation of cytoplasmic SGs, in which non-polysomal mRNA is recruited [4,34]. The involvement of cytoplasmic PARPs and PAR in the regulation of SG assembly has been shown for arsenite-treated cells [11]. For this reason, we also considered to investigate the features of SG formation under H 2 O 2 -induced stress conditions, which induce DNA damage and would significantly activate PAR synthesis compared to arsenite [35]. Of note, the assembly of SGs in H 2 O 2 -treated cells has been the focus of many studies [36][37][38][39][40][41]. It turned out that H 2 O 2 is not a reliable agent to induce SG assembly with either no SG assembly [36,40,42,43] or SG assembly [37,38] being reported. In an extensive study, the appearance of SGs in cells was detected only at a high concentration of H 2 O 2 (≥1 mM) [36,40]. Therefore, we explored the role of nuclear PAR synthesis in SG assembly in HeLa cells exposed to arsenite, H 2 O 2 , H 2 O 2 then arsenite or arsenite then H 2 O 2 . A low concentration of H 2 O 2 (300 µM), which induces PAR synthesis without triggering SG formation, was used for these experiments ( Figure 1A,B and Figure S1A,B). Strikingly, when cells were treated with H 2 O 2 prior to arsenite treatment, the formation of SGs was significantly impaired ( Figure 1A,B). In addition, cell treatment with H 2 O 2 after arsenite exposure led to a strong increase in the number of SGs per cell ( Figure 1A,B).
Since H 2 O 2 not only causes the activation of nuclear PARPs but also an additional stress when combined with arsenite, we wondered whether the inhibition/stimulation of SG assembly in H 2 O 2 /arsenite and arsenite/H 2 O 2 -treated cells was dependent on PARP1 activation. To test this hypothesis, we used olaparib or talazoparib, two PARP inhibitors [44], before inducing cellular stress ( Figure 1A,B and Figure S1C). As a control, PARP inhibition moderately reduced SG assembly triggered by arsenite only, which is consistent with the possible participation of cytoplasmic PARPs in SG assembly, whose activities can also be affected by the same inhibitors [11,44]. However, in cells pretreated with PARP inhibitors, H 2 O 2 and then exposed to arsenite or vice versa, PARP inhibition led to the suppression/stimulation of SG assembly ( Figure 1A,B). To further investigate whether nuclear PARP activity inhibits arsenite-mediated SG formation, we decreased PARP1 expression by using siRNA and then analyzed the level of SG formation in cells treated with arsenite or H 2 O 2 /arsenite ( Figure 1C,D). PARP1 silencing with siRNA allows the recovery of SG formation in cells treated with H 2 O 2 prior to arsenite ( Figure 1C,D), as observed with PARP inhibitors. Altogether, our findings suggest a negative regulation of SG assembly when H 2 O 2 treatment causes the activation of PARP1 prior to cell exposure to arsenite. ylation. For this purpose, we directly compared the polysome profiles of HeLa cells treated with arsenite, H2O2 and H2O2/arsenite in the presence or absence of the PARP1 inhibitor olaparib ( Figure 1E,F). As expected, arsenite induced a nearly complete dissociation of polysomes in cells under our experimental condition ( Figure 1E). In contrast to arsenite, H2O2 alone did not significantly affect the overall polysome profile. Interestingly, when cells were pretreated with H2O2 prior to arsenite, the dissociation of polysomes was noticeably reduced ( Figure 1E,F). Figure 1. PARP1 activation upon cell exposure to H2O2 prevents polysome dissociation and thus arsenite-mediated SG assembly. (A) HeLa cells were exposed to indicated treatments (300 µ M H2O2 for 30 min; 300 µ M arsenite for 60 min). DMSO (control), to inhibit PARP1 10 µ M olaparib or 1 µ M talazoparib were added 1 h prior to indicated treatment. mRNA was then detected to reveal the presence of SGs in the cytoplasm. Blue: DAPI (nuclei). Grey: mRNA (in situ hybridization with cy3- Figure 1. PARP1 activation upon cell exposure to H 2 O 2 prevents polysome dissociation and thus arsenite-mediated SG assembly. (A) HeLa cells were exposed to indicated treatments (300 µM H 2 O 2 for 30 min; 300 µM arsenite for 60 min). DMSO (control), to inhibit PARP1 10 µM olaparib or 1 µM talazoparib were added 1 h prior to indicated treatment. mRNA was then detected to reveal the presence of SGs in the cytoplasm. Blue: DAPI (nuclei). Grey: mRNA (in situ hybridization with cy3-labelled poly(dT) probe). Scale bar: 10 µm. (B) The number of SGs for 50 cells and their fluorescent intensity (in situ hybridization of mRNA) were measured for the indicated conditions. SGs were detected automatically from cell images by using the Cell Profiler software. **, p < 0.001; t-test. (C) HeLa cells were treated with siRNA directed against mRNA encoding PARP1 and then exposed to the same treatments as those indicated in (A). Scale bar: 10 µm. As H 2 O 2 treatment does not cause the phosphorylation of eIF2A, in contrast to arsenite [36], we tested the hypothesis that massive eIF2A phosphorylation can be affected by cell pretreatment with puromycin and puromycin/H 2 O 2 and also in combination with olaparib. We compared the phosphorylation of eIF2A in cells after treatment with arsenite or H 2 O 2 in the presence or absence of puromycin/olaparib (Supplementary Figure S1D). We noticed a marked increase in eIF2A phosphorylation in cells exposed to arsenite compared to other conditions, but H 2 O 2 , olaparib/arsenite or puromycin/olaparib/H 2 O 2 has no noticeable influence on the level of eIF2A phosphorylation (Supplementary Figure S1D), which is somewhat in accordance with a previous report [36]. To further decipher the mechanism by which PARP1 activation prevents SG assembly, we explored whether PARP1 could influence the dissociation of polysomes independently of eIF2A phosphorylation. For this purpose, we directly compared the polysome profiles of HeLa cells treated with arsenite, H 2 O 2 and H 2 O 2 /arsenite in the presence or absence of the PARP1 inhibitor olaparib ( Figure 1E,F). As expected, arsenite induced a nearly complete dissociation of polysomes in cells under our experimental condition ( Figure 1E). In contrast to arsenite, H 2 O 2 alone did not significantly affect the overall polysome profile. Interestingly, when cells were pretreated with H 2 O 2 prior to arsenite, the dissociation of polysomes was noticeably reduced ( Figure 1E,F).
This result is consistent with previous studies indicating that H 2 O 2 treatment may slow down or stall translation elongation, which freezes ribosomes on mRNA [10,45]. Preventing the dissociation of ribosomes from mRNA should suppress SG assembly, as observed after cycloheximide treatment, an inhibitor of translation elongation [4,34]. Importantly, PARP1 inhibition with olaparib neutralized the effect of cell treatment with H 2 O 2 prior to arsenite, which therefore induces the dissociation of polysomes. Thus, H 2 O 2 -induced PARP1 activation appears to prevent the dissociation of polysomes in arsenite-treated cells independently of changes in the eIF2A phosphorylation status and thereby might prevent the assembly of SGs in the cytoplasm.

Activation of PARP1 Upregulates the Assembly of H 2 O 2 -Induced SGs
Since H 2 O 2 -induced PARP1 activation prevents the dissociation of polysomes and SG assembly in arsenite-treated cells (Figure 1), we tested whether PARP1 may also affect the formation of SGs in cells exposed to H 2 O 2 alone at elevated concentrations. In agreement with another study made using the U2OS cell line [36], we also observed SG formation in HeLa cells only exposed to a high H 2 O 2 concentration (1 mM) ( Figure 2A).
Remarkably, SGs were not observed in cells treated with 1 mM of H 2 O 2 in the case of pretreatment with olaparib ( Figure 2A). Thus, PARP1 activation promotes SG formation during the stress response to a high concentration of H 2 O 2 raised to 1 mM. On the one hand, pretreatment with H 2 O 2 before arsenite impeded SG assembly ( Figure 1B). On the other hand, treatment with H 2 O 2 after arsenite or alone at a high concentration (1 mM) did not prevent SG formation and the dissociation of polysomes ( Figure 1A,B and Figure 2A). In order to understand these contrasting effects, further experiments were carried out by stimulating polysome dissociation with puromycin prior to H 2 O 2 treatment and PARP activation ( Figure 2B and Figure S2A). Puromycin induces premature chain termination during translation and promotes ribosome dissociation from mRNA but does not trigger SG assembly by itself [46]. Consistently, puromycin pretreatment before the addition of 300 µM H 2 O 2 contributes to the formation of SGs ( Figure 2B and Figure S2B). The results of the polysome profiling also show a decrease in polysomal mRNA when cells were treated with puromycin before H 2 O 2 (Supplementary Figure S3). Thus, the pretreatment of HeLa cells with puromycin may counteract the effect of the H 2 O 2 -induced block of polysome dissociation (Supplementary Figure S3B).  Figure 2C,D). Thus, all results are consistent with an involvement of PARP1 activation in SG assembly caused by both high and low concentrations of H2O2.
According to our data, PARP activity can both prevent the formation of SGs by blocking the dissociation of polysomes ( Figure 1E,F) and stimulate the formation of SGs if the polysomes are dissociated prior to PARP1 activation ( Figure 2 and Figure S2B).

Figure 2.
After polysome destabilization by puromycin, PARP1 activation triggers SG assembly. (A) HeLa cells were exposed to a high H2O2 concentration (1 mM for 1 h) to trigger SG assembly. Blue: DAPI (nuclei). Grey: mRNA (in situ hybridization with cy3-labelled poly(dT) probe). Lower panel: the number of SGs detected after cells were exposed to 1 mM H2O2 decreased sharply when cells were pretreated with olaparib (10 μM). Scale bar: 10 μm. Red dots represent the mean value of the data. (B) HeLa cells were exposed to indicated treatments (300 µ M H2O2 for 30 min; 200 µ M puromycin 60 min). DMSO (control), 10 µ M olaparib and 1 µ M talazoparib were added 1 h prior to indicated treatments to inhibit PARP1. mRNA was then detected to reveal the presence of SG sin the cytoplasm. Blue: DAPI (nuclei). Grey: mRNA (in situ hybridization with cy3-labelled poly(dT) probe). Scale bar: 10 μm. Lower panel: mRNA enrichment in detected SGs. **, p < 0.001; t test. (C) HeLa cells were treated with siRNA-directed mRNA encoding PARP1 and then exposed to indicated treatments. Green: anti-PARP1 antibody. Red: mRNA (in situ hybridization with cy3-labelled poly(dT) probe). Scale bar: 10 μm. (D) Percent of cells displaying SGs after pretreatments indicated in (B).

Figure 2.
After polysome destabilization by puromycin, PARP1 activation triggers SG assembly. (A) HeLa cells were exposed to a high H 2 O 2 concentration (1 mM for 1 h) to trigger SG assembly. Blue: DAPI (nuclei). Grey: mRNA (in situ hybridization with cy3-labelled poly(dT) probe). Lower panel: the number of SGs detected after cells were exposed to 1 mM H 2 O 2 decreased sharply when cells were pretreated with olaparib (10 µM). Scale bar: 10 µm. Red dots represent the mean value of the data. (B) HeLa cells were exposed to indicated treatments (300 µM H 2 O 2 for 30 min; 200 µM puromycin 60 min). DMSO (control), 10 µM olaparib and 1 µM talazoparib were added 1 h prior to indicated treatments to inhibit PARP1. mRNA was then detected to reveal the presence of SG sin the cytoplasm. Blue: DAPI (nuclei). Grey: mRNA (in situ hybridization with cy3-labelled poly(dT) probe). Scale bar: 10 µm. Lower panel: mRNA enrichment in detected SGs. **, p < 0.001; t test. (C) HeLa cells were treated with siRNA-directed mRNA encoding PARP1 and then exposed to indicated treatments. Green: anti-PARP1 antibody. Red: mRNA (in situ hybridization with cy3-labelled poly(dT) probe). Scale bar: 10 µm. (D) Percent of cells displaying SGs after pretreatments indicated in (B).
Next, we tested whether PARP1 activation contributes to SG assembly in HeLa cells pretreated with puromycin and then exposed to 300 µM H 2 O 2 . As in the case of cells treated with 1 mM H 2 O 2 , PARP inhibitors prevented SG assembly in puromycin/H 2 O 2 (300 µM)treated cells ( Figure 2B and Figure S2A). The polysomal profile also showed a slight increase in polysomal fraction and decrease in monosomal fraction (80S) in puromycin/H 2 O 2treated cells when PARP activation was inhibited with olaparib, which is consistent with the inhibition of SG assembly (Supplementary Figure S3B). This result indicates that PARP1 activation positively regulates SG assembly after H 2 O 2 treatment when polysomes are destabilized in the presence of puromycin ( Figure 2B, Figures S2 and S3B). To further strengthen this conclusion, we also found that puromycin followed by H 2 O 2 treatment failed to induce the formation of SGs in HeLa cells treated with PARP1 siRNA (Figure 2C,D). Thus, all results are consistent with an involvement of PARP1 activation in SG assembly caused by both high and low concentrations of H 2 O 2 .
According to our data, PARP activity can both prevent the formation of SGs by blocking the dissociation of polysomes ( Figure 1E,F) and stimulate the formation of SGs if the polysomes are dissociated prior to PARP1 activation (Figure 2 and S2B).

The Presence of PAR in SGs Is not Significantly Affected by PARP1 Activation Whether SGs Were Formed after Arsenite or H 2 O 2 Treatment
In cells treated with a high concentration of H 2 O 2 or puromycin/H 2 O 2 , SG assembly relies on PARP1 activation ( Figure 2). Therefore, we wondered whether PAR could be involved in the formation of SGs in this specific condition. As for arsenite [11,22], PAR may play a more prominent role as a scaffold-like molecule in the formation of SGs under H 2 O 2 treatment. So far, this hypothesis is partially supported by the positive regulation of SG assembly by cytoplasmic PARPs and their downregulation by PARG in the cells treated with arsenite [11]. Although some cytoplasmic PARPs can indeed synthesize long PAR chains [11], to what extent the synthesis of a long polymer would be sufficient to serve as a scaffold for SGs is unknown [10]. PAR has already been detected in arseniteinduced SGs with anti-PAR antibodies, but only when cell fixation was performed after its permeabilization [11]. During the extraction of small soluble molecules, PAR may appear brighter in SGs due to either an enrichment of PAR in SGs or trapping it in SG compartments. To explore whether PARP1 activation after treatment with H 2 O 2 could contribute to the formation of SG-enriched PAR, we performed a similar experiment but used a methanol fixation rather than PFA, because PFA fixation seems not to be optimal for PAR detection. Indeed, according to previous studies and our experience, PARylation might occur during the cell fixation process with PFA [47]. To perform this experiment, we used five different anti-PAR antibodies, but a transient increase in anti-PAR fluorescence in the nucleus was detected with only two of them within 30 min after exposure to 300 µm H 2 O 2 ( Figure 3A).
The two validated antibodies were raised against either poly(ADP-ribose) chains (anti-PAR) or against mono-and poly(ADP-ribose) (anti-MAR/PAR), the latter displaying a cytoplasmic localization under the control conditions without H 2 O 2 treatment ( Figure 3A). We failed to detect a significant PAR enrichment in SGs formed in response to either arsenite or puromycin/H 2 O 2 treatments (Supplementary Figure S4A). Although we did not detect PAR enriched in the SGs of H 2 O 2 -treated cells, both PARP1 and poly(ADP-ribose) glycohydrolase (PARG) activities impact the SG assembly under these stress conditions ( Figure 2D and Figure S5). As PARG represents a family of enzymes which is particularly active in digesting PAR chains in both the nucleus and cytoplasm in eukaryotic cells [48], we hypothesize that a rapid degradation of PAR in the nucleus occurs before its putative nucleocytoplasmic shuttling. Thus, PAR may already be hydrolyzed by PARG in the nucleus/cytoplasm for the time required for SG formation (60-90 min upon stress) or short PAR molecules present in the cytoplasm are not recognized by anti-PAR antibodies ( Figure 3A).

No PAR Enrichment in TDP-43 and FUS-Rich Condensates in the Cytoplasm
Nuclear PAR produced by PARP1 and protein PARylation could drive the translocation of RBPs from the nucleus to the cytoplasm to promote the formation of SGs. Previously, we demonstrated that H 2 O 2 treatment affects the nucleocytoplasmic shuttling of SG-associated proteins such as FUS, HuR or TDP-43 [30]. Each of these proteins could contribute to the assembly of SGs, interact with PAR or be PARylated [11,49]. To further probe how PARP1-dependent PAR synthesis may modulate stress granule assembly under H 2 O 2induced stress, we generated SGs in HeLa cells by overexpressing HA-tagged TDP-43 or FUS. The presence of these self-adhesive proteins harboring prion-like domains in the cytoplasm is sufficient to trigger the assembly of cytoplasmic granules without oxidative stress [50][51][52][53][54]. Like SGs, the formed granules were shown to be reversible upon cycloheximide treatment and contained mRNAs [4,54]. First, we observed that the level of HA-tagged protein enrichment in the granules remains similar in cells exposed to H 2 O 2 to activate PARP1 or not, although the number of SGs significantly increased, and its formation was sensitive to PARP1 inhibitors (Supplementary Figure S4B). Next, in the case of the anti-PAR antibody, no correlation in the fluorescence signal was detected between PAR and HA-tagged protein intensity in the SGs of cells overexpressing both FUS and TDP-43 by confocal microscopy ( Figure 3B,C). However, a correlation in the fluorescence between MAR/PAR and HA signals in granules was detected with anti-MAR/PAR antibody at least for FUS-rich granules ( Figure 3D,E). It is possible that the correlation of PAR intensity with the intensity of HA-labeled FUS in granules, in contrast to TDP-43, may be due to the ability of FUS to be PARylated and(or) to bind PAR with a high affinity and, by this way, attract MAR/PAR to SGs [30]. Compared with arsenite, MAR/PAR enrichment in these granules did not change after the H 2 O 2 -induced activation of PARP1 ( Figure 3D,E). Thus, MAR/PAR could be indeed a component of FUS-or TDP-43-rich cytoplasmic granules, although we have no clear evidence that an extensive synthesis of PAR in the nucleus upon PARP1 activation leads to the increased accumulation of PAR in SGs formed with the participation of FUS and TDP-43, which can potentially interact with PAR or be PARylated under oxidative stress.

The Translocation of Nuclear RBPs upon PARP1 Activation May Promote Stress Granule Assembly but FUS Translocation Is Not Enough
To further understand how PARP1 activation and RBPs could promote SG formation, we decided to explore the involvement of endogenous FUS, HuR and TDP-43 in SG formation under H 2 O 2 /puromycin or arsenite stress conditions. It is important to note that the translocation of FUS to the cytoplasm and the retention of HuR in the nucleus was found to depend directly on PARP1 inhibition (Supplementary Figure S6), as previously reported [30]. To test the involvement of endogenous FUS, HuR and TDP-43 in SG formation under H 2 O 2 treatment, we analyzed the enrichment of these proteins in SGs formed under arsenite or puromycin/H 2 O 2 treatment (Supplementary Figure S7A). In contrast to HuR, we found that SGs in H 2 O 2 /puromycin-treated cells were enriched in endogenous FUS and TDP-43 compared to arsenite-treated cells (Supplementary Figure S7A). Although TDP-43-rich granules were more abundant in the case of H 2 O 2 -treated cells, the translocation of TDP-43 from the nucleus to the cytoplasm upon treatment with H 2 O 2 was shown not to be PARP1-dependent [30]; thus, the protein cannot strongly influence the level of H 2 O 2 -induced SG assembly after PARP1 inhibition.
We then considered the possibility that PARP1 could promote SG assembly indirectly through the translocation of FUS, as its translocation has been shown to be dependent on PARP1 [30]. Nevertheless, we found that silencing the expression of FUS by using the CRISPR/Cas9 technology did not prevent the formation of SGs in cells treated with puromycin/H 2 O 2 (Supplementary Figure S7B). This result is consistent with several genome-wide analyses showing only a few RBPs are critical for SG assembly, FUS not being one of them [55,56]. Alternatively, under H 2 O 2 -induced stress conditions, HuR, a mRNA-stabilizing factor, may act as a negative factor for SG assembly [57], and PAR synthesis in the nucleus may thus favor SG assembly by preventing the translocation of HuR in the cytoplasm (Supplementary Figure S6).
In summary, SGs formed in the cytoplasm after H 2 O 2 treatment are enriched in FUS and TDP-43 compared to those formed in the presence of arsenite (Supplementary Figure S7A). Therefore, H 2 O 2 -induced stress influences the composition of SGs. The detection of granules enriched with FUS suggests that this protein could act downstream of PARP1 activation in the process of SG formation, because FUS translocation is strongly dependent on PARP1 activation [30].
3.6. PARP1 Activation Promotes mRNA-rich Granule Assembly in the Nucleus without any Mixing with PAR As we did not evidence any enrichment of PAR in cytoplasmic SGs after PARP-1 activation, we then devised to explore whether PAR can be recruited in nuclear SGs, where anti-PAR and anti-PAR/MAR antibodies clearly reveal an increase in PAR levels 30 min after H 2 O 2 treatment ( Figure 3A). In the nucleus, mRNAs are synthetized in the nucleus by RNA polymerase II and then processed by splicing factors [58]. We therefore perturbed these tightly regulated machineries by using actinomycin D (ActD), a general inhibitor of transcription and potent inhibitor of SG formation in the cytoplasm [4,59]. In cells pretreated with ActD, we evidenced the presence of small granule-like structures containing mRNA in the nucleus ( Figure 4A).
We then analyzed the putative recruitment of PAR inside the nuclear mRNA-rich granules observed after ActD or ActD/H 2 O 2 treatment, when mRNA synthesis was stopped and PARP1 was activated ( Figure 4B,C). As observed in the cytoplasm (Figure 3), we found no evidence for an enrichment of PAR in mRNA-rich nuclear granules. We thus did not gather any data to support the presence of abundant long PAR chains in mRNArich granules. However, importantly, the nuclear mRNA-rich granules were significantly more numerous and gathered more mRNA inside ActD/H 2 O 2 -treated cells than in ActDtreated cells ( Figure 4B,C). Under the same conditions, PARP inhibition by olaparib led to a significant downregulation of mRNA-rich nuclear granules in HeLa cells treated with ActD/H 2 O 2 ( Figure 4A,B), suggesting a common mechanism by which PARP1 activation could positively regulate SG assembly in H 2 O 2 -treated cells, whether in the cytoplasm or the nucleus (Figures 2 and 4).
Therefore, the activation of PARP1 by DNA damage-induced oxidative stress positively regulates the formation of mRNA-rich granules in the nucleus and cytoplasm of HeLa cells, but without any additional enrichment of PAR in these granules.

PARP1 Activation upon H 2 O 2 Exposure Negatively Regulates SG Disassembly and Positively Regulates Preexisting TDP-43 and FUS-Rich Granules
As PARP1 positively regulates SG assembly in arsenite/H 2 O 2 -or H 2 O 2 -treated cells when puromycin prematurely disengages ribosomes from polysomes ( Figures 1B and 2B), we then considered whether H 2 O 2 may regulate the dissociation of pre-formed SGs. To this end, we pre-formed SGs in cells treated with arsenite. After that, arsenite was washed out and cells were left to recover with fresh culture medium. SG disassembly was easily captured as the number of cells harboring SGs decreases after 90 min, in agreement with the reversible nature of SGs [60]. However, when cells were treated with 300 µM H 2 O 2 during the recovery period, the disassembly of SGs was impaired ( Figure 5A,B). Cells 2022, 11, x FOR PEER REVIEW 13 of 21  when puromycin prematurely disengages ribosomes from polysomes ( Figures 1B and 2B), we then considered whether H2O2 may regulate the dissociation of pre-formed SGs. To this end, we pre-formed SGs in cells treated with arsenite. After that, arsenite was washed out and cells were left to recover with fresh culture medium. SG disassembly was easily captured as the number of cells harboring SGs decreases after 90 min, in agreement with the reversible nature of SGs [60]. However, when cells were treated with 300 µ M H2O2 during the recovery period, the disassembly of SGs was impaired ( Figure 5A,B).  In addition, we also noticed that the number of SGs and the mean fluorescence intensity of mRNA is significantly higher in control cells than in cells pretreated with olaparib to prevent PARP1 activation, which may indicate a change in their structure and composition during cell recovery with the H 2 O 2 treatment ( Figure 5B).
The inhibition of PARP1 activation by olaparib reversed this pattern as fewer SGs and less mRNA were detected inside them ( Figure 5A,B). Thus, PARP1 activity prevents the disassembly of pre-existing SGs formed under arsenite treatment, influencing the enrichment of mRNA in SGs.
We then further explored the hypothesis of the persistence of SGs after PARP1 activation but, this time, in the absence of arsenite pretreatment, which may be the source of biases. Therefore, we again used HeLa cells overexpressing HA-target TDP-43 or FUS, which induces the formation of cytoplasmic granules without stress conditions (Figures 3 and 5C). Although the level of HA-tagged proteins in the condensates remained similar in all conditions (Supplementary Figure S4B), we observed an enrichment of mR-NAs in TDP-43 or FUS-rich granules and also an increase in the number of granules after H 2 O 2 treatment ( Figure 5D). Importantly, the increase in mRNA-rich granule assembly in TDP-43 and FUS-overexpressing cells was PARP1-dependent, since these cells pretreated with olaparib displayed a reduced number of SGs even after H 2 O 2 treatment ( Figure 5C,D).
Therefore, in pre-formed SGs, PARP1 activation delayed SG disassembly upon recovery from arsenite stress ( Figure 5A) and upregulated the assembly of cytoplasmic TDP-43 and FUS-positive granules and their enrichment of RNA ( Figure 5C).

Discussion
At present, both PARylated proteins and protein-free PAR (or mono(ADP-ribose)) formed during the action of PARG appears to be involved in the mRNA metabolism-related processes during stress, one of which is SG formation [58]. The involvement of PAR in the regulation of SG assembly in the cytoplasm is a subject of intensive research, which is focused mainly on the PARP, PARG99 and PARG102 isoforms present in the cytoplasm [9][10][11][12]. Nonetheless, the direct role of PARP1 in SG formation has not been fully elucidated. Genotoxic stress causes a strong increase in the cellular PAR level, and this is mainly due to the activation of nuclear PARP1, which is responsible for the synthesis of most PAR in the cell (up to 80-90%) upon DNA damage [21]. At the same time, PARGs, the major enzymes that hydrolyze PAR, are highly active in cells [61]. The half-life of the major population of PAR may be close to one minute, but we cannot exclude that a small fraction of the polymer may have a cell half-life of several hours and be implicated in the cellular adaptation to stress conditions [21,62].
In this context, we investigated the relationship between PARP1 and the formation of mRNA-rich granules in the nucleus and cytoplasm of HeLa cells under different stress conditions induced by H 2 O 2 treatment alone or in combination with arsenite, transcription inhibitor ActD or translation inhibitor puromycin. Our results indicate a previously unsuspected link between the activation of PARP1 and the efficiency of cytoplasmic mRNA-rich granule assembly under H 2 O 2 -induced stress and suggest a direct relationship between PARP1 activation and translation regulation in mammalian cells ( Figure 6). Moreover, we found an association of PARP1 activity with the formation and genesis/maturation of FUS-rich cytoplasmic inclusions, which are found in neurons of patients affected by certain major neurodegenerative diseases, including ALS [32,[63][64][65][66].

PARP1 Activation Prevents the Assembly of Arsenite-Induced SGs by Preventing Polysome Dissociation
When cells have no pre-formed SGs in the cytoplasm, surprisingly, oxidative stress generated by H 2 O 2 very efficiently prevents SG assembly, even if arsenite is added afterward, and this effect depends on PARP1 activity ( Figure 6A). We found that H 2 O 2 treatment prevents polysome dissociation, and PARP1 inhibitors in turn restore polysome dissociation in H 2 O 2 /arsenite-treated cells ( Figure 1A,B). Thus, this effect of H 2 O 2 on the stability of polysomes is PARP1 activity-dependent but eIF2A phosphorylation-independent (Supplementary Figure S1D). Therefore, PARP1 activation appears to induce an elongation block, preventing polysome dissociation. A translation elongation block has already been reported after H 2 O 2 treatment in different organisms, notably via the phosphorylation of elongation factors [45], but not associated directly to nuclear PARP1 activity. Future works may highlight whether PARP1 activation controls the phosphorylation or PARylation status of elongation factors in cells or whether other cellular mechanisms come into play.

PARP1 Activation Prevents the Assembly of Arsenite-Induced SGs by Preventing Polysome Dissociation
When cells have no pre-formed SGs in the cytoplasm, surprisingly, oxidative stress generated by H2O2 very efficiently prevents SG assembly, even if arsenite is added afterward, and this effect depends on PARP1 activity ( Figure 6A). We found that H2O2 treatment prevents polysome dissociation, and PARP1 inhibitors in turn restore polysome dissociation in H2O2/arsenite-treated cells ( Figure 1A,B). Thus, this effect of H2O2 on the stability of polysomes is PARP1 activity-dependent but eIF2A phosphorylation-independent (Supplementary Figure S1D). Therefore, PARP1 activation appears to induce an elongation block, preventing polysome dissociation. A translation elongation block has already been reported after H2O2 treatment in different organisms, notably via the phosphorylation of elongation factors [45], but not associated directly to nuclear PARP1 activity. Future works may highlight whether PARP1 activation controls the phosphorylation or PARylation status of elongation factors in cells or whether other cellular mechanisms come into play.

PARP1 Activation Upregulates the Assembly of H 2 O 2 -Induced SGs
The mechanism of SG formation in response to H 2 O 2 treatment has been a source of debate [37,38]. It should be noted that, in most previously published reports, H 2 O 2 by itself triggers SG assembly only at concentrations above 1 mM, which may be due to the significant inhibition of translation initiation at such elevated concentrations of H 2 O 2 [36]. Remarkably, we observed that 1mM H 2 O 2 -induced SG assembly in the cytoplasm is controlled by PARP1 ( Figure 6B). Milder stress conditions, H 2 O 2 at 300 µM, are sufficient to trigger a very efficient PARP1 activation in HeLa cells, but not SG formation ( Figure 2B). Furthermore, when cells are pretreated by puromycin, which counteracts the elongation block and promotes polysome dissociation, H 2 O 2 at 300 µM strongly induces the assembly of SGs ( Figure 2B). In addition, SG assembly in puromycin/H 2 O 2 -treated cells is strictly dependent on PARP1 activity (Figure 2A,C,D). Thus, if translation initiation is inhibited by a high dose of H 2 O 2 or translation elongation is blocked by puromycin, causing the polysome dissociation, PARP1 activation promotes cytoplasmic SG assembly ( Figure 6B).

PARP1 Activation Positively Regulates Pre-Formed Nuclear and Cytoplasmic mRNA-Rich Granules but Does Not Induce PAR Accumulation in SGs
Although the putative role of cytoplasmic PARPs in the formation of SGs has been already shown [9][10][11][12], the direct involvement of PARP1 in the building of SGs is not fully understood [22]. Here, we found that the presence and accumulation of H 2 O 2induced cytoplasmic, but more importantly, nuclear, SG-like structures directly depend on PARP1 activity. We also detected a co-localization of MAR/PAR with FUS or TDP-43 in cytoplasmic granules that were formed under H 2 O 2 -induced stress conditions in HeLa cell-overexpressed FUS (or TDP-43) ( Figure 3C). This fact may be in agreement with the hypothesis that PAR is a scaffold for triggering the assembly of specific sets of proteins in condensates [14], as observed with purified FUS and PAR in vitro [15,30,67]. However, we failed to detect an increase in PAR enrichment in SGs, whether they were induced by arsenite or H 2 O 2 treatment. In spite of the fact that the H 2 O 2 -induced SG formation is upregulated by PARP1 activity, our data do not provide additional support for a role of PAR as a scaffold promoting the assembly of mRNA-rich granules under this stress condition. Nevertheless, PARP1 activation could drive the translocation of FUS to the cytoplasm, and H 2 O 2 -induced cytoplasmic SGs are much more abundant ( Figure 6C).
We also analyzed PAR enrichment in mRNA-rich granules in the nucleus, formed after H 2 O 2 treatment in combination with ActD, and found that H 2 O 2 enhances the nuclear granules' formation and their enrichment of mRNA, and their effect is weakened by the PARP1 inhibitor; nevertheless, we again failed to observe an enrichment of PAR in these nuclear granules (Figure 4). Thus, it is possible that condensates formed by mRNA or PAR do not mix or fuse with each other, which is important to investigate further.

PARP1 Activation Promotes Assembly of Pre-Formed SGs and Prevents Their Dissociation
Although the pretreatment of cells by H 2 O 2 strongly inhibits SG formation after arsenite stress ( Figure 1A), the dissociation of SGs pre-formed in the presence of arsenite is prevented in a PARP1-dependent manner ( Figure 5A,B and Figure 6D). In the case of cytoplasmic pre-formed TDP-43-and FUS-rich granules, H 2 O 2 exposure caused a significant increase in the number of FUS-rich granules in a PARP1-dependent manner ( Figure 5C,D and Figure 6C). Both TDP-43 and FUS translocate from the nucleus to the cytoplasm during aging in neurons of ALS and FTLD patients [49,68] and form cytoplasmic inclusions that can participate directly in the progression of these diseases. Finding a link between PARP1 activation and the maintenance of TDP-43 and FUS condensates could be of interest since recent reports propose a critical role for poly(ADP-ribosyl)ation in association with neurodegeneration [20,26,28,29].
However, we cannot conclude whether preventing SG assembly would be beneficial or detrimental for the progression of neurodegenerative diseases [69]. Since the presence of TDP-43 or FUS in SGs may either promote the formation of protein aggregates, for instance, a local increase in TDP-43 and FUS in SGs [65], or inhibit their formation, we may consider that mRNA present in SGs behaves as TDP-43 and FUS chaperones to prevent a transition from reversible liquid-like condensates to irreversible protein aggregates [12,52,54].

Conclusions
The formation of H 2 O 2 -induced cytoplasmic and nuclear mRNA-rich granules directly correlates with PARP1 activity. In sum, three hypotheses can be proposed: (i) SG protein components are PARylated, including FUS [70], which may in turn promote RNA granule assembly; (ii) PARP1 activation may also activate signals via phosphorylation events [71,72] to force the assembly of mRNA-rich granules; (iii) as PAR is not found inside nuclear mRNA-rich granules after PARP1 activation (Figure 3, Figure 4 and Figure S3A), PAR may compete with mRNA for binding to RBPs [30,67]. In this latter model, mRNA-stabilizing proteins would rather bind PAR than mRNA. PAR would then promote the formation of pre-formed mRNA granules without being part of these granules itself. However, this model is more likely to take place in the nucleus than in the cytoplasm, owing to the net increase in PAR in the nucleus after PARP1 activation, but we cannot exclude that nuclear PAR may prevent the shuttling of nuclear mRNA-stabilizing proteins to the cytoplasm, as observed with HuR (Supplementary Figure S5A,B).

Supplementary Materials:
The following supporting information can be downloaded at: https:// www.mdpi.com/article/10.3390/cells11233932/s1, Figure S1. Exposure of cells to H2O2, in contrast to arsenite, leads to a strong activation of PARP1, but does not cause significant phosphorylation of eIF2A; Figure S2. PARP1 activity contributes to stress assembly; Figure S3. PARP1 activity contributes to stress assembly if the polysomes were previously destabilized; Figure S4. PAR enrichment was not observed in SG formed in the H2O2-and arsenite-induced stress conditions; Figure S5. Western blot analysis of PARG expression; Figure S6. PARP1 activation may prevent the shuttling of HuR to the cytoplasm; Figure S7. Analysis of stress granule composition and assembly; Table S1 and S2.