Abstract
YAP and its neuronal isoform YAPdeltaC are implicated in various cellular functions. We found that expression of YAPdeltaC during development, but not adulthood, rescued neurodegeneration phenotypes of mutant ataxin-1 knock-in (Atxn1-KI) mice. YAP/YAPdeltaC interacted with RORα via the second WW domain and served as co-activators of its transcriptional activity. YAP/YAPdeltaC formed a transcriptional complex with RORα on cis-elements of target genes and regulated their expression. Both normal and mutant Atxn1 interacted with YAP/YAPdeltaC, but only mutant Atxn1 depleted YAP/YAPdeltaC from the RORα complex to suppress transcription on short timescales. Over longer periods, mutant Atxn1 also decreased RORα in vivo. Genetic supplementation of YAPdeltaC restored the RORα and YAP/YAPdeltaC levels, recovered YAP/YAPdeltaC in the RORα complex and normalized target gene transcription in Atxn1-KI mice in vivo. Collectively, our data suggest that functional impairment of YAP/YAPdeltaC by mutant Atxn1 during development determines the adult pathology of SCA1 by suppressing RORα-mediated transcription.
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Introduction
Spinocerebellar ataxia type 1 (SCA1) is a neurological disease that mainly affects Purkinje cells in the cerebellum and motoneurons in the spinal cord1,2,3. It has been more than 20 years since the discovery of the causative gene, Ataxin-1 (ATXN1)4. Since then, a great deal of knowledge has accumulated regarding the mechanisms of SCA1, including the identities of the Atxn1-interacting factors involved in transcription and splicing5,6,7,8,9. However, SCA1 remains intractable, and no disease-modifying therapy has reached the clinical bedside.
Meanwhile, as with other neurodegenerative diseases, our conception of spinocerebellar ataxias (including SCA1) has changed substantially. First, it has become clear that the types of affected neurons are not as specific as originally believed. For example, we now know that SCAs affect not only cerebellar neurons but also cerebral neurons, sometimes leading to cognitive impairment in patients with SCA110. Second, the effects of these disorders are not limited to single organs: polyQ diseases like Huntington’s disease affect not only the brain but also muscle, adipose, pancreas, and heart tissues11, and this may also be the case in SCAs. Third, SCA might be a developmental disorder that affects cerebellar neurons during embryogenesis or in early childhood12.
In regard to the third point, a study by the Orr group revealed the developmental molecular pathology of SCA1 by showing that Atxn1 indirectly interacts with RORα, an orphan nuclear receptor with similarities to retinoic acid receptors12. Expression of mutant Atxn1 protein, encoded by a gene containing a CAG expansion, decreases RORα levels and thus broadly affects expression of target genes necessary for cerebellar development12.
We previously showed that the transcriptional co-factor YAP is involved in an atypical form of necrosis induced by alpha-amanitin, transcriptional repression-induced atypical cell death (TRIAD) in which C-terminal truncated isoforms of YAP (ins13, ins25, and ins61 possessing additional mini-exon sequences between exon 5 and exon 6) play critical roles13. In subsequent experiments, we expressed these isoforms in developing Drosophila under the control of the tubulin Gal4 driver, fed the larvae alpha-amanitin, and monitored the survival ratio from larva to pupa. The results revealed that YAPdeltaC-ins61 had the strongest anti-TRIAD activity (our unpublished data). Therefore, we took YAPdeltaC-ins61 (hereafter, “YAPdeltaC”) as the representative of three isoforms. Biochemical and morphological data support the idea that TRIAD actually occurs in human Huntington’s disease brains14, and overexpression of YAPdeltaC prevents TRIAD in Huntington’s disease in vitro models15.
In this study, we tested the therapeutic effect of YAPdeltaC on SCA1 pathology using a newly developed Tet-ON YAPdeltaC system in Atxn1-KI (Sca1154Q/2Q) mice. Unexpectedly, adulthood expression of YAPdeltaC did not ameliorate the pathology and symptoms of Atxn1-KI mice. By contrast, YAPdeltaC expression during development markedly rescued the pathology and symptoms in adulthood. We found that YAP/YAPdeltaC functioned as a transcriptional co-activator of RORα. Normal Atxn1 collaborated with YAP/YAPdeltaC to activate RORα, whereas mutant Atxn1 inhibited incorporation of YAP/YAPdeltaC into the RORα transcription complex. Supplementation of YAP/YAPdeltaC overcame the toxic effect of mutant Atxn1 and restored the transcriptional activity of RORα. These results elucidate the molecular function of YAPdeltaC in the developmentally determined pathology of SCA1.
Results
Developmental YAPdeltaC rescues adult phenotype of KI mice
We generated transgenic mice expressing YAPdeltaC using the advanced Tet-ON system (see Methods). When fed doxycycline (Dox), these transgenic mice express YAPdeltaC under the control of the neuron-specific enolase (NSE) promoter. To investigate the temporal specificity of the potential therapeutic effect of YAPdeltaC, the Tet-ON mice were crossed with mutant heterozygous Atxn1-KI (Sca1154Q/2Q) mice16. The double-transgenic mice (Tet-ON YAPdeltaC; Atxn1-KI) expressed mutant Atxn1 (Atxn1-154Q) from E0 to death, but expressed YAPdeltaC specifically in neurons only when fed Dox. All mice were of the C57BL/6 genetic background.
In Group I, mother mice were fed Dox during pregnancy and breast-feeding (from E0 to 3 weeks of age); after 3 weeks, the double-transgenic progeny received Dox in drinking water (Fig. 1a). In Group II, the double-transgenic mice received Dox in drinking water from 8 weeks of age until death (Fig. 1a). No Dox group of the double-transgenic mice received no Dox during embryogenesis and after birth (Fig. 1a). The induction of YAPdeltaC by Dox in Group I mice was confirmed by analysis of cerebellar tissues from Group I, Group II, No-Dox, and C57BL/6 mice (without Dox feeding) at P21 (3 weeks of age) (Fig. 1b).
The lifespans of the four groups were investigated, and their motor functions were evaluated using the Rotarod test. In Atxn1-KI mice, the onset of motor dysfunction was quite early, and Rotarod test scores declined at 7 weeks. In Group II and No Dox, the decline of motor function was similar to that in Atxn1-KI mice (Fig. 1). By contrast, the scores remained high in Group I, and the improvement was statistically significant from 11 to 21 weeks of age (Fig. 1c).
Developmental expression, but not adulthood expression, of YAPdeltaC was also effective in lengthening lifespan (Fig. 1d). In the background control group (C57BL/6), mean lifespan was longer than 400 days. By contrast, in Atxn1-KI mice, mean and maximum lifespans were 224.1 and 274 days, respectively; in Group I (Tet-ON-YAPdeltaC;Atxn1-KI, Dox+ from E0 to death), 318.3 and 400 day; and in Group II (Tet-ON-YAPdeltaC;Atxn1-KI, Dox+ from 8 weeks to death), 238.4 and 297 days; in No Dox (Tet-ON-YAPdeltaC;Atxn1-KI, Dox−), 238.3 and 290 days. These differences in lifespan confirmed that the critical period for YAPdeltaC expression is the developmental stage (E0–8 weeks). We confirmed that YAPdeltaC protein was rapidly induced within 1 week after initiation of Dox-feeding at 8 weeks of age (Fig. 1e).
Developmental YAPdeltaC rescues adult pathology of KI mice
In Atxn1-KI mice at P21, the number of Purkinje cells was not affected (Fig. 2a), but the thickness of the molecular layer was reduced (Fig. 2a). In addition, the diameters of Purkinje cell bodies were significantly reduced in these animals (Fig. 2a). These data obtained from the primary fissure side area of lobule IV–V, which corresponds to the upper vermis severely affected in human SCA1 patients, suggested that differentiation and maturation of Purkinje cells were impaired12, but cell death did not occur by P21. By 32 weeks, cell number was also decreased (Fig. 2b), indicating that cell death occurred between P21 and 32 weeks.
In Group I mice at P21, YAPdeltaC restored Purkinje cell body diameter and molecular layer thickness (Fig. 2a) and also prevented the decrease in Purkinje cell number at 32 weeks (Fig. 2b), in consistence with the late-onset effect of RORα-mediated transcription reported previously12, and suggested functional interaction between YAPdeltaC and RORα.
YAP/YAPdeltaC interact with RORα
Hence, we tested physical interaction between YAP/YAPdeltaC and RORα. We scanned the amino-acid sequence of RORα and found a PPLY sequence that matches the PPxY consensus for interaction with YAP WW domain (Fig. 3a)17,18,19. This PPLY motif also overlapped with a consensus sequence (PLYKELFT) for interaction with Tip60 NR box (Fig. 3a). To determine which YAP WW domain is essential for interaction with RORα, we generated YAP expression vectors mutated at the first and/or second WW domain (Fig. 3b). To investigate YAP binding to the PPLY consensus, we also constructed a RORα mutant in which PPLY was replaced to PPLA (Fig. 3b).
FLAG-tagged full-length YAP or YAPdeltaC was transiently expressed along with wild-type RORα in primary cerebellar neurons and immunoprecipitated by anti-FLAG and anti-RORα antibodies at 2 days after transfection. RORα reciprocally co-precipitated with both full-length YAP and YAPdeltaC (Fig. 3c, d left panels), and deletion of the C-terminal domain of YAP in YAPdeltaC did not markedly affect the interaction (Fig. 3c, d, left panels). FLAG-empty, used as a negative control, did not co-precipitate RORα (Fig. 3c, d, left panels). The interaction was retained when the first WW domain was mutated, but was completely lost in a YAP mutant lacking the second WW domain, as well as in the double mutant lacking both WW domains (Fig. 3c, d, middle panels). RORα harboring a mutation in the binding motif (Y507A) was not co-precipitated with full-length YAP or YAPdeltaC (Fig. 3c, d, right panels). These results indicated that the second WW domain of YAP/YAPdeltaC and the PPLY motif of RORα are essential for the interaction.
The similar experiments were further performed with COS-7 cells transiently overexpressing RORα at 2 days after transfection, in which endogenous expression of RORα is very low (Supplementary Fig. 1A, B). The results were exactly similar with those from primary cerebellar neurons and supported that the second WW domain of YAP/YAPdeltaC and the PPLY motif of RORα are essential for the interaction.
Atxn1 forms a complex with YAP/YAPdeltaC and RORα
Next, we tested the difference between normal and mutant Atxn1 (Fig. 4a, b). From primary cerebellar neurons expressing Myc-Atxn1 and FLAG-YAP/YAPdeltaC at 2 days after transfection, both normal and mutant Atxn1 proteins were co-precipitated with YAP/YAPdeltaC (Fig. 4a, b). Reciprocal co-precipitation of YAP/YAPdeltaC and Atxn1 did not significantly differ as a function of polyQ length (Fig. 4a, b, lower graphs).
In pull-down assays using His-tagged YAP and GST-tagged normal or mutant Atxn1 (Fig. 4c), His-YAP but not His-tagged tau as a negative control was pulled down by glutathione–Sepharose with both GST-Atxn1-33Q and GST-Atxn1-86Q (Fig. 4c, upper panel). In the reciprocal experiment, GST-Atxn1-33Q and GST-Atxn1-86Q, but not GST, were pulled down with His-YAP (Fig. 4c, lower panels). On the other hand, similar pull-down experiments did not reveal a direct interaction between GST-Atxn1 and RORα, as reported previously12.
Because RORα co-precipitated with normal but not mutant Atxn1 (Fig. 4a, b), and a direct interaction between Atxn1 and RORα was not confirmed in a previous report12, we hypothesized that the RORα–YAP–Atxn1 ternary complex forms via RORα–YAP and YAP–Atxn1 direct interactions. The ternary complex formed efficiently with normal Atxn1, but to a lesser extent with mutant Atxn1, suggesting that mutant Atxn1 might perturb integration of YAP into the ternary complex.
The similar experiments with 293T cells, which express RORα endogenously, at 2 days after transfection supported that normal and mutant Atxn1 equally interact with YAP/YAPdeltaC (Supplementary Fig. 1C, D). Again, RORα co-precipitated with normal but not mutant Atxn1, suggesting perturbation of YAP integration into the RORα–YAP–Atxn1 ternary complex by mutant Atxn1.
RORα–YAP/YAPdeltaC–Atxn1 complex is functional
Next, we investigated whether YAP/YAPdeltaC function as a transcription co-activator for RORα (Fig. 5a, b). As mentioned above, COS-7 cells express a very low level of RORα but a high level of full-length YAP (Fig. 5b). Co-transfection of an effector plasmid expressing RORα (RORα-pCI neo), but not RORα-Y507A mutant lacking affinity for YAP/YAPdeltaC, increased luciferase activity from a RORα-responsive element on a reporter plasmid (RORE-pGreenFire) (Fig. 5a). In the absence of RORα, overexpression of YAP/YAPdeltaC did not affect luciferase activity (Fig. 5a). YAP/YAPdeltaC increased transcriptional activity in the presence of wild-type RORα but not of RORα-Y507A (Fig. 5a). Collectively, these results supported that YAP/YAPdeltaC function as transcriptional co-activators for RORα.
We knocked down YAP and/or Tip60 using siRNA in 293T cells which express RORα and YAP endogenously (Fig. 5c). YAP-siRNA dramatically decreased the level of YAP protein, and suppressed transcriptional activity proportional to the degree of knockdown (Fig. 5c). Tip60-siRNA decreased Tip60 protein level, albeit less efficiently, and also proportionally suppressed transcription (Fig. 5c), suggesting that YAP and Tip60 are co-factors with equivalent activity. Double knockdown of YAP and Tip60 additively suppressed transcription from the RORα-responsive element (Fig. 5c), indicating that YAP and Tip60 have complementary functions.
In vitro pull-down assays revealed that YAP and Tip60 compete for binding to RORα. In these experiments, His-Tip60, His-YAP (full-length YAP2), and GST-RORα (a.a. 424–523, including the overlapping binding motifs) (Fig. 3a) were mixed in vitro, and GST-RORα was pulled down with glutathione–Sepharose. Increasing the amount of His-Tip60 decreased the amount of His-YAP pulled down with RORα, and vice versa (Fig. 5d).
We next investigated the role of Atxn1 in RORα-mediated transcription using 293T cells, in which Atxn1 is expressed endogenously (Fig. 5e). Atxn1-siRNA but not a scrambled siRNA markedly suppressed transcriptional activity (Fig. 5e). Collectively, these results indicated that the RORα–YAP/YAPdeltaC–Atxn1 complex is functional in the normal state, and that all components in the complex are essential for transcriptional activity.
Mutant Atxn1 depletes YAP/YAPdeltaC from the RORα complex
We next asked how mutant Atxn1 affects interaction between YAP/YAPdeltaC and RORα in vivo. Using the cerebellar tissues prepared from mice at P7 and P21, we confirmed co-precipitation of full-length YAP (YAP2) and RORα (Fig. 6a, left panels). RORα co-precipitated with YAP was decreased in Atxn1-KI mice (No Dox) than C57BL/6 mice, but recovered in Group I mice (Fig. 6a, left upper panels). In the reciprocal precipitation of RORα, co-precipitated YAP was reduced in Atxn1-KI mice but recovered in Group I mice (Fig. 6a, left lower panels). Similarly, the in vivo interaction between YAPdeltaC and RORα was attenuated in Atxn1-KI mice (No Dox), but recovered in Group I mice (Fig. 6a, right middle left panel). Normal and mutant Atxn1 similarly interacted with YAP/YAPdeltaC (Fig. 6a right and middle right panels).
To investigate the in vivo protein–protein interaction between YAP/YAPdeltaC and RORα on cis-elements in the RORα target genes20 (Pcp2, Pcp4, or Slc1a6) in three groups of mice (C57BL/6, No-Dox, and Group 1) at P7 and P21 (Fig. 6b), we performed ChIP assays with anti-YAP2 or anti-YAPdeltaC-specific antibody (the latter targets the unique sequence of YAPdeltaC) and PCR-amplified the RORα-responsive elements in the upstream regions of the target genes (Fig. 6b, left panels). In all three genes, the amount of amplified RORα-responsive element was lower in Atxn1-KI mice (No Dox) than in background C57BL/6 mice, but recovered in Group I mice (Fig. 6b, left panels and right graphs). The RORα-responsive element was not amplified from a sample precipitated with anti-c-Jun antibody (negative control) (Fig. 6b). Collectively, the results of the immunoprecipitation assays (Fig. 6a) and ChIP assays (Fig. 6b) suggested that mutant Atxn1 deprived YAP/YAPdeltaC from the RORα transcription complex in vivo.
Next, we investigated in chronological order when mutant Atxn1 deprived YAP/YAPdeltaC from the RORα transcription complex on target genes (Fig. 6c). We transiently expressed Myc-tagged normal/mutant Atxn1 in primary cerebellar neurons, which endogenously express RORα, YAP/YAPdeltaC, and normal Atxn1, and subjected these cells to ChIP assays. Already at 2 days after transfection, YAP/YAPdeltaC were not present in the RORα transcription complex on RORα-responsive element (Fig. 6c), and the deprivation of YAP/YAPdeltaC continued to day 7 (Fig. 6c). Although RORα was invariably bound to the response element in its target genes, only Myc-Atxn1-33Q, but not Myc-Atxn1-86Q, was present in the RORα transcription complex on the cis-element (Fig. 6c). Since Myc-Atxn1-33Q and Myc-Atxn1-86Q were equivalently expressed in primary neurons (Fig. 6d), the results indicated that Myc-Atxn1-86Q could not efficiently approach to the RORα-responsive element.
We also performed ChIP assays in 293T cells. The results confirmed that Myc-Atxn1-33Q, but not Myc-Atxn1-86Q as well as bound YAP/YAPdeltaC, was present in the RORα transcription complex located on the cis-element of the three target genes (Supplementary Fig. 2A, B). Again, expression levels of Myc-Atxn1-33Q and Myc-Atxn1-86Q were equivalent in these samples (Supplementary Fig. 2B).
YAPdeltaC recovers RORα-transcription
To test the effects of mutant Atxn1 on RORα-dependent transcription, we performed luciferase assays in primary cerebellar neurons at 2 days after transfection. As expected, mutant Atxn1 suppressed transcription from RORα-responsive promoter, and YAP/YAPdeltaC rescued the suppression (Fig. 7a). The suppression by mutant Atxn1 and the rescue by YAP/YAPdeltaC were dose-dependent (Fig. 7b). In addition, we found that YAP/YAPdeltaC levels decreased from 4 days after transfection of mutant Atxn1 and RORα level followed from day 7 (Fig. 7c). Proteasome inhibitor MG-132 blocked the reduction of RORα and YAP/YAPdeltaC levels (Fig. 7c, right panels), suggesting that non-functional RORα and YAP/YAPdeltaC were degraded by the ubiquitin–proteasome system. Morphological analysis (Fig. 7d) and cell death assay with trypan blue staining (Fig. 7e) excluded the concern that these changes were due to the unhealthy state and/or cell death of primary cerebellar neurons by expression of mutant Atxn1.
Luciferase assays with 293T cells confirmed that YAP/YAPdeltaC rescued mutant Atxn1-induced suppression of RORα-dependent transcription (Supplementary Fig. 3A), that suppression and recovery were dose-dependent (Supplementary Fig. 3B), that mutant Atxn1 could suppress RORα-mediated transcription even without reduction of RORα (Supplementary Fig. 3A, B), and that mutant Atxn1 decreased YAP/YAPdeltaC and RORα sequentially (Supplementary Fig. 3C). The proteasome inhibitor MG-132 blocked the reduction in RORα and YAP/YAPdeltaC levels also in 293T cells (Supplementary Fig. 3C). Based on a phase-contrast image of the transfected cells, we can exclude that Atxn1-induced cell death affected transcriptional activity in the assay (Supplementary Fig. 3D).
Based on these results, we hypothesize that in vivo, mutant Atxn1 disturbs RORα-mediated transcription over short timescales by directly interacting with YAP/YAPdeltaC and depleting these co-activators from the transcriptional complex. Meanwhile, over longer periods, mutant Atxn1 accelerates degradation of YAP/YAPdeltaC and RORα, resulting in a reduction in their protein levels (Supplementary Fig. 4).
YAP/YAPdeltaC, RORα, and Atxn1 in Purkinje cells in vivo
To test the hypothesis that mutant Atxn1 in Atxn1-KI mice depletes YAP/YAPdeltaC from the transcription complex, thereby RORα-mediated transcription during development, we next sought to verify that all of the relevant factors are actually co-expressed in Purkinje cells, and examined how expression of mutant Atxn1 affects RORα and YAP/YAPdeltaC in Purkinje cells in vivo. For this purpose, we performed western blot of C57BL/6, No Dox, and Group I mice at P7, P21, and 32 weeks (Fig. 8).
RORα signal intensity was not changed at P7 but decreased in Atxn1-KI mice at P21 and 32 weeks (Fig. 8). In this regard, our results in mutant Atxn1-KI mice (Sca1154Q/2Q) were consistent with those of a previous study reporting reduced expression of RORα at P35 (5 weeks)12 in Pcp2/L7 promoter-driven Tet-Off Atxn1-82Q transgenic mice21 and of a ROR-target gene EAAT4 at P21 (3 weeks) in B05 Pcp2/L7 promoter-driven Atxn1-82Q simple transgenic mice22, 23. Meanwhile, the decreases in YAP and YAPdeltaC levels in Atxn1-KI mice started at P7 and preceded the change in RORα at P21 (Fig. 8). All changes in RORα YAP, and YAPdeltaC levels were rescued by overexpression of YAPdeltaC in Group I mice from P7 to 32 weeks (Fig. 8). By contrast, the Tip60 level was not reduced in Atxn1-KI mice at any time point (Fig. 8).
Next, we performed immunohistochemistry analyses of YAP/YAPdeltaC, RORα, or Tip60 with Calbindin in C57BL/6, No Dox, and Group I mice at P7, P21, and 32 weeks (Fig. 9). In Purkinje cells of background mice, all four proteins were expressed at all time points (Fig. 9). Signal intensities of YAP and YAPdeltaC were reduced in Purkinje cells of Atxn1-KI from P7 to 32 weeks. Meanwhile RORα was decreased from P21. The discrepancy between YAP/YAPdeltaC and RORα at P7 was consistent with the result in western blot. All changes in RORα YAP and YAPdeltaC levels were rescued again by YAPdeltaC in Group I mice from P7 to 32 weeks (Fig. 9).
We checked the amount and intracellular distribution of Atxn1 using anti-Atxn1 antibody 11NQ, along with YAP, YAPdeltaC, RORα, or Tip60, at P21 (Supplementary Fig. 5) and 32 weeks (Supplementary Fig. 6). Expression levels of Atxn1 in the nucleus were not different significantly among three groups. Although the symptoms have already appeared by this age, nuclear inclusion bodies are not detected before 40 weeks16.
Collectively, immunohistochemistry revealed that all relevant factors are expressed in the most vulnerable Purkinje cells, and that not only RORα but also YAP/YAPdeltaC levels were reduced by mutant Atxn1 in vivo. Thus, the results supported our hypothesis based on the chronological relationship of these four molecules.
YAPdeltaC rescues RORα target genes in KI mice
Next, we investigated how RORα-dependent transcription was altered in the three groups of mice. To this end, we performed RT-qPCR analysis to evaluate expression levels of two RORα target genes24, A2BP1 and CYP19A1, using Purkinje cells punched out from frozen sections of mouse cerebellum, as described previously25 (Fig. 10). We selected these two target genes for qPCR (Fig. 10a), in addition to the target genes20 used for the ChIP assays (Pcp2, Pcp4, and Slc1a6) (Fig. 6b, c) in order to generalize the effect of YAPdeltaC on RORα target genes. As expected, expression levels of the additional genes were reduced in Purkinje cells of Atxn1-KI mice, but recovered in Group I mice (Fig. 10a). The decrease and recovery in expression levels of RORα target genes at P7 (Fig. 10a), when levels of the co-activators YAP/YAPdeltaC but not the transcription factor RORα itself were reduced (Figs. 8 and 9), were consistent with the reduced transcriptional activity in the luciferase assay with primary cerebellar neurons at day 2 after transfection, when YAP/YAPdeltaC but not RORα levels were reduced (Fig. 7). RT-qPCR analysis also revealed that expression of multiple YAP target genes26, 27 was similarly reduced and recovered in Purkinje cells of three types of mice (Fig. 10b).
YAP overexpression might make neurons more resistant to mutant Atxn1-induced cell death, dependently on the upregulation of anti-apoptotic genes in developing cerebellar neurons. However, expression levels of representative anti-apoptotic genes such as Bcl-2, c-Flip, and XIAP were not altered (Fig. 10c). Regarding Naip1, which was detected in our previous study as an increased gene during TRIAD13, was not changed at P7 and P21 (Fig. 10c). At 32 weeks, Naip1 was already increased in Atxn1-KI mice similarly to the condition of TRIAD13 (Fig. 10c). These results did not support that apoptosis is responsible for the decrease of Purkinje cell death in Atxn1-KI mice, while it remained possible that other types of cell death contribute to the pathological process from P21 to 8 weeks of age. These results supported our hypothesis that supplementation with YAPdeltaC ameliorates Atxn1-induced pathology in vivo via recovery of RORα-dependent transcription.
Furthermore, we tested whether YAP or YAPdeltaC induced de-differentiation of primary cerebellar neurons prepared at P7 (Supplementary Fig. 7). The concern was basically excluded, since YAP or YAPdeltaC even at high expression levels (Supplementary Fig. 7A) did not induce tumor-like foci (Supplementary Fig. 7B) or did not increase the number of cells positive for Ki67 (a tumor marker) and Sox2 (a de-differentiation marker), as revealed by immunohistochemistry (Supplementary Fig. 7C) or western blot analysis (Supplementary Fig. 7D).
YAPdeltaC rescues DNA damage in KI mice
YAP is an essential component of the Hippo signaling pathway, which influences DNA repair and apoptosis in cancer cells28, 29, YAP/YAPdeltaC protects against TRIAD13. Accordingly, we investigated whether supplementation with YAPdeltaC would rescue DNA damage in Purkinje cells of Atxn1-KI mice.
Consequently, we performed immunohistochemistry and western blot analyses to monitor the increase of DNA damage markers, such as γH2AX and 53BP1, in cerebellar tissues of Atxn1-KI mice at P21 (Supplementary Fig. 8A, B). Immunohistochemistry revealed that DNA damage was elevated, especially in Purkinje cells, and this increase in DNA damage was rescued by in vivo co-expression of YAPdeltaC in Group I mice (Supplementary Fig. 8A, B, upper panels). Western blot analyses of cerebellar tissues supported this conclusion (Supplementary Fig. 8A, B, lower panels). We also confirmed by western blot that the level of RpA1, a critical molecule for multiple forms of DNA repair involved in SCA1 pathology25, 30, was elevated in Purkinje cells, probably in response to the elevated DNA damage in Atxn1-KI mice, but was restored to normal by co-expression of YAPdeltaC in vivo (Supplementary Fig. 8C).
Discussion
The mouse genetic analyses performed in this study revealed that expression of YAPdeltaC during development, but not in adulthood, markedly ameliorated the behavioral and pathological phenotypes of Atxn1-KI mice in adulthood (Figs. 1 and 2). Our results suggest that certain molecular signatures generated during development significantly influence late-onset phenotypes, and that these signatures act by restoring gene expression to optimal levels. YAP/YAPdeltaC and RORα are candidate components of such a molecular signature. At short timescales, mutant Atxn1 binds to YAP/YAPdeltaC and disrupts RORα-mediated transcription by depleting YAP/YAPdeltaC from the RORα complex. Shuttling of nuclear proteins between nuclear bodies, where transcription-related factors are stored, and the nucleoplasm, where the factors assemble to on histone-free and relaxed regulatory elements of target genes, is impaired by mutant Atxn1 and other polyQ proteins31,32,33. Thus, mutant Atxn1 could slow down the dynamic interactions of direct binding partners such as YAP/YAPdeltaC, and thereby impair transcription.
Over longer periods of more than 7 days, the interaction with mutant Atxn1 decreased YAP/YAPdeltaC and RORα levels in a cell culture model via accelerated proteasome-mediated degradation (Fig. 7c). A similar decrease in YAP/YAPdeltaC and RORα levels was confirmed in vivo in mutant Atxn1-KI mice at 21 days and 32 weeks of age (Fig. 8, Supplementary Fig. 5 and 6). Therefore, both acute and chronic mechanisms are likely to contribute to the suppression of RORα-mediated transcription of critical target genes that eventually causes the late-onset pathology of SCA1.
We employed the NSE promoter for our Tet-ON system. If this promoter drove YAPdeltaC in cells other than Purkinje cells, this expression might have affected RORα-mediated transcription or TRIAD and contributed to the lifespan elongation observed in Group I mice. To explore this possibility, it will be necessary to characterize the gene expression patterns of NSE in other cell types, other regions of the brain, and other organs. Based on publicly available information in databases such as GeneCards (http://www.genecards.org/cgi-bin/carddisp.pl?gene=ENO2) and MGI (http://www.informatics.jax.org/gxd#gxd=nomenclature%3DNSE%26vocabTerm%3D%26annotationId%3D%26locations%3D%26locationUnit%3Dbp%26structure%3D%26structureID%3D%26theilerStage%3D0%26results%3D100%26startIndex%3D0%26sort%3D%26dir%3Dasc%26tab%3Dresultstab), expression levels of NSE are very low in organs other than the brain, and within the brain expression is restricted to neurons. Based on our previous results, obtained using transgenic mice in which the same NSE promoter drove HMGB125, we can speculate about the gene’s expression pattern. Although expression was detected in neurons of various brain regions, the levels in Purkinje cells were substantially higher than in other neurons in different regions25. We also measured NSE expression in other organs, and confirmed that the levels were very low (data not shown).
Therefore, although the effects of YAPdeltaC on RORα-mediated transcription or TRIAD (discussed later) in other brain regions or organs might have additively contributed to the phenotypic recovery of Group I mice, we consider it likely that a large proportion of the rescue effect of YAPdeltaC is derived from its activity in Purkinje cells. This hypothesis effectively explains why our results in Atxn1-KI mice (Sca1154Q/2Q) were consistent, but slightly improved with respect to lifespan with previous results obtained in transgenic mice harboring Pcp2/L7-promoter-driven Atxn1-82Q21, in which mutant Atxn1 expression could be switched on or off specifically in Purkinje cells12. This speculation is also consistent with recent observations of polyQ/CAG repeat disease pathology in non-neuronal cells11.
Moreover, in human patients, most cases progress motor ataxia due to the loss of Purkinje cells, become bed-ridden, suffer insufficient food intake and aspiration pneumonia due to ataxia of pharyngeal muscles, and die. SCA1 patients with severer loss of Purkinje cells die at younger ages than SCA6 patients in which loss of Pukinje cells are not prominent. Therefore, the lifespan shortening/recovery in our mouse models based on Purkinje cell pathology may mimic the human natural history better than previous experimental reports.
Our findings revealed that YAP/YAPdeltaC interacts with RORα via the second WW domain (Fig. 3). Interestingly, YAP/YAPdeltaC also use the second WW domain to interact with mutant Htt15. In both cases, YAP/YAPdeltaC are deprived of their partner transcription factors. In HD pathology, transcription mediated by TEAD, a partner transcription factor of YAP/YAPdeltaC, is impaired15. This study provides the first evidence that RORα is a partner transcription factor of YAP/YAPdeltaC, and that RORα-mediated transcription is impaired in SCA1 pathology. Together, these two studies imply that YAP/YAPdeltaC-related gene expression represents a common pathological mechanism shared by multiple polyQ diseases.
It is possible that YAP/YAPdeltaC influence apoptosis and increase resistance against SCA1-associated cerebellar degeneration, including the reduction in Purkinje cell numbers, independently of the hypothesized effect of YAP/YAPdeltaC on RORα-mediated transcription. However, YAP/YAPdeltaC did not affect expression levels of anti-apoptotic genes in Purkinje cells from P7 to 32 weeks (Fig. 10). Since previous data suggested that cell death of Purkinje cells occur from 16 to 32 weeks in Atxn1-KI mice16, 25, 34,35,36, these data do not support the idea that the late-onset effects of YAPdeltaC in Group I mice are due to suppression of apoptosis.
Another important observation was the delay in cell death downstream of YAP/YAPdeltaC dysfunction. Recently, we reported that a new form of necrosis, dependent on Hippo pathway signaling, contributes to the pathology of Huntington’s disease15. The impairment of TEAD–YAP-mediated transcription leads to a lengthy process of necrotic cell death. The morphological and molecular features of TEAD–YAP-dependent cell death were very similar to those of TRIAD15, a Type 3 necrotic cell death induced by repression of transcription with the RNA polymerase II inhibitor α-amanitin13. Accordingly, these two forms of cell death are considered identical. Ultra-structural and biochemical analyses of human postmortem tissue revealed that TRIAD actually occurs in human HD brains14. Given that target genes of TEAD-YAP transcription were suppressed in Atxn1-KI mice and recovered in Group I mice (Fig. 10), TEAD-YAP-mediated TRIAD might be a possible explanation for the late-onset effect of YAPdeltaC in Group I mice.
From the perspective of neuronal dysfunction, dendrite abnormalities were observed in Atxn1-KI mice at 13 weeks, an age when the cell death of Purkinje cells was not obvious34. Interestingly, the Hippo pathway has recently been implicated in synapse formation in Drosophila 37. These observations suggest that functional impairment of YAP/YAPdeltaC during development until 8 weeks of age induces sequential processes, ranging from neuronal dysfunction to cell death in adulthood. Given that RORα plays a critical role in SCA1-associated neurodegeneration12, and considering that the results our study reveal the close relationship between YAP/YAPdeltaC and RORα, it is very plausible that YAP/YAPdeltaC contribute to the adult-onset functional pathology of SCA1 by impairing RORα-mediated transcription during development. However, the effect exerted by YAP/YAPdeltaC on SCA1 pathology via TEAD-mediated transcription should be investigated in future studies.
During the process of our paper evaluation, another group reported that TAZ, the mammalian homolog of YAP, functioned as a co-activator of ROR to promote Th17 cell differentiation through similar biochemical mechanism38. These two independent but consistent results might open a new pathway from Hippo pathway to ROR family receptors that could be applied to multiple organs.
Our results revealed that mutant, but not wild-type, Atxn1 depletes YAP/YAPdeltaC from the RORα complex. The first mechanism underlying the depletion would be proteasome-dependent degradation of YAP/YAPdeltaC after the YAP/YAPdeltaC–mutant Atxn1 complex formation (Fig. 7c, Supplementary Fig. 3C). Second, presumably the nuclear dynamics of YAP/YAPdeltaC would be impaired by interaction with mutant Atxn1, as with RpA1 and VCP, whose nuclear dynamics are slowed and diminished by interaction with the mutant protein30, 39. In addition, the nuclear sites of interaction between YAP/YAPdeltaC and Atxn1 and between RORα and YAP/YAPdeltaC are likely to differ, as demonstrated previously for different combinations of transcription factors that ultimately execute integrated functions40. Therefore, interaction of mutant Atxn1 with YAP/YAPdeltaC in one subdomain would prevent interaction of YAP/YAPdeltaC with RORα in another. However, the second explanation remains a hypothesis that should be critically tested in future analyses.
The roles of YAP in DNA repair remain controversial. Two previous studies reported that YAP induces apoptosis in DNA-damaged cancer cells28, 29. This function is mediated by the YAP–p73 complex, which promotes expression of pro-apoptotic genes41. Meanwhile, in non-dividing neurons, YAP/YAPdeltaC functions as a protective factor against transcriptional repression-induced necrosis dependent on the YAP–TEAD complex13, 15. In that context, DNA damage is promoted by transcriptional inhibition42, whereas YAP/YAPdeltaC decreases the level of DNA damage (Supplementary Fig. 8). Conversely, the discrepant functions of YAP/YAPdeltaC in DNA repair suggest that the proteins’ primary roles are related to transcriptional regulation, and that any effects on DNA damage are secondary.
Regardless of the causative pathway, elevated DNA damage in stem cells decreases production of neurons. However, we did not observe a reduction in the abundance Purkinje cells at P21 (Fig. 2a). Instead, our analysis revealed that developmental expression of YAP/YAPdeltaC before 8 weeks (Fig. 1a) is protective against late-onset death of Purkinje cells after 16 weeks16, 25, 34,35,36 (Fig. 2b). Atxn1 expression begins at E13.5–15 (http://www.informatics.jax.org/marker/MGI:104783), and markedly increases at P1443. In addition, protein aggregation and RNA foci of Atxn1 was not detected in Atxn1-KI mice until 40 weeks16 far later than the onset age of motor symptom. Collectively, these findings suggest that the key mechanism by which YAPdeltaC ameliorates delayed cell death would be normalization of RORα-dependent and/or TEAD-dependent genes between E13.5 and 8 weeks (Fig. 1a). Therefore, identification of these downstream target genes would enable us to manipulate the late-onset cell death of SCA1 in the future.
Methods
Ethics
This study was performed in strict compliance with the recommendations in the Guide for the Care and Use of Laboratory Animals of the National Institutes of Health (USA). This study was also approved by the Committees on Gene Recombination Experiments, Human Ethics, and Animal Experiments of the Tokyo Medical and Dental University (2010-215C13, 2014-5-4, and 0160328A, respectively).
Animals
The mutant Atxn1-KI mouse (Sca1154Q/2Q mouse) was a generous gift from Professor Huda Y. Zoghbi (Baylor College of Medicine, TX, USA)16. The original background of the Sca1154Q/2Q mouse was B6.129S, but subsequently the Zoghbi group backcrossed the strain with C57BL/6. Atxn1-154Q male mice were further crossed with C57BL/6 female mice more than 10 times in our laboratory, and the phenotypes of the resultant Sca1154Q/2Q mice in the B6 background were described previously25. Next, conditional and inducible YAPdeltaC-ins61 transgenic mice were generated using the Tet-on system. Briefly, reverse tetracycline-controlled transactivator (rtTA) transgenic mice under the control of the rat NSE (neuron-specific enolase) promoter (NSE-rtTA) were crossed with TRE (tetracycline-responsive element) promoter-regulated YAPdeltaC-ins61 transgenic mice. Double-heterozygous transgenic mice were crossed to generate double-homozygous transgenic mice, and the resultant female double-homozygous transgenic mice (NSE-rtTA/YAPdeltaC) were crossed with male Sca1154Q/2Q mice in the B6 background to generate triple-transgenic mice (rtTA/YAPdeltaC/Atxn1-KI mice). Thus, the genetic backgrounds of YAPdeltaC-Tg, NSE-rtTA, NSE-rtTA/YAPdeltaC, and NSE-rtTA/YAPdeltaC/Atxn1-KI mice were all C57BL/6.
Rotarod test
Male 5–21-week-old control (C57BL/6J mice), Atxn1-KI, and Atxn1-KI/YAP∆C mice were tested. Mice were placed on a rotating rod (shaft diameter: 3.2 cm, lane width: 5.7 cm, fall height: 16.5 cm. Five Station Rota-Rod Standalone for Mouse, ENV-577M, MED Associates Inc®, USA) in accelerating speed mode 8 (i.e., rotation speed was linearly increased from 3.5 to 35 r.p.m. over 300 s and then maintained at 35 r.p.m. for additional 600 s). The amount of time spent on the drum until the mouse fell off was measured four times per day over 3 days, with 10-min rest intervals between the measurements.
Plasmid construction
Human and rat YAP2 (full-length YAP) and rat YAPdeltaC (YAPdeltaC-ins61) cDNAs were generated previously13. The cDNAs were subcloned into pCIneo (Promega, Madison, WI, USA) containing the FLAG tag (FLAG-YAP-pCIneo and FLAG-YAPdeltaC-pCIneo). Plasmids with mutations in the first and/or second WW domain mutations were purchased from Addgene (2xFlag CMV2-YAP2-1st and/or 2nd WW mutation, MA, USA). To construct human RORα-pCIneo, human RORα cDNA (1591 bp, nt 86-1657 of NM_136241) was amplified from total RNA of 293T cells using primers 5′-CCGGAATTCATGGAGTCAGCTCCGGCA-3′, and 5′-ACGCGTCGACTTACCCATCAATTTGCATTGCTGGC-3′. After digestion with EcoRI or SalI, the RORα cDNA was subcloned into pCI-neo (Promega). The Y507A mutation (RORα-Y507A-pCIneo) was generated using primers 5′-CATTTTCCTCCATTAGCCAAG-3′, and 5′-GTGAACAACTCCTTGGCTAAT-3′. To construct human RORE (RORα-responsive element)-pGreenfire, the upstream genomic fragment of human NR1D1 gene containing RORα response element (1844 bp, nuclear receptor subfamily 1 group D member 1, nt 632–2476 of NM_021724) was amplified from human genomic DNA (#6550-1, CLONTECH, CA, USA) using primers 5′-CCGGAATTCAAAGGGGGTCACATTTCCTTTCC-3′ and 5′-CTAGTCTAGATGCCCCAGTGACACACTTTT-3′, and subcloned into pGreenFire1 (#TR011PA-1, System Biosciences, CA, USA) after digestion with EcoRI or XbaI. Myc-Atxn1-0Q, Myc-Atxn1-33Q, and Myc-Atxn1-86Q were generated as described previously44.
Cerebellar neuron culture and plasmid transfection
Cerebellar neurons were prepared from C57BL/6J mice at postnatal day 7. Briefly, dissected cerebella were digested at 37 °C with 0.05% trypsin (GIBCO) for 15 min. Tissue was passed through a 70-μm cell strainer (BD). Cells were cultured in DMEM (Sigma) containing 25 mM d-glucose, 4 mM l-glutamine, 25 mM KCl, and 10% fetal bovine serum in the presence of 2 μM AraC. Plasmid transfections were performed using Viromer Red (OriGene).
Western blot analysis
Mouse cerebellum tissues were dissolved in lysis buffer (10 mM Tris-HCl (pH 7.5), 150 mM NaCl, 1 mM EDTA, 1% NP-40) with protease inhibitor cocktail (#539134, 1:100 dilution, Calbiochem, CA, USA) for 1 h at 4 °C. After centrifugation (12,000×g × 10 min), supernatants were mixed with an equal volume of sample buffer (62.5 mM Tris-HCl (pH 6.8), 2% (w/v) SDS, 2.5% (v/v) 2-mercaptoethanol, 5% (v/v) glycerol, and 0.0025% (w/v) bromophenol blue). The BCA method (Pierce BCA Protein Assay Kit; Thermo Scientific, IL, USA) was used to determine protein concentrations, which were subsequently equalized across samples. Samples were separated by SDS-PAGE, transferred onto polyvinylidene difluoride membrane Immobilon-P (Millipore) by the semi-dry method, blocked with 5% milk in TBST (10 mM Tris/HCl (pH 8.0), 150 mM NaCl, 0.05% Tween-20), and reacted with the following primary and secondary antibodies diluted in TBST with 0.1% skim milk or Can Get Signal solution (Toyobo, Osaka, Japan): rabbit anti-YAPdeltaC13, 1:20,000 (raised against the common COOH-terminal peptide [SVFSRDDSGIEDNDNQ]); rabbit anti-FLAG, 1:2000 (F7425, SIGMA, IL, USA); mouse anti-c-Myc, 1:2000, (#sc-40 Santa Cruz Biotechnology, Dallas, TX, USA); rabbit anti-RORα, 1:1000 (#sc-28612, Santa Cruz Biotechnology); mouse anti-RGS-His, 1:5000 (#34650, Qiagen, Hilden, Germany); rabbit anti-GST, 1:3000 (sc-469, Santa Cruz Biotechnology); rabbit anti-YAP, 1:5000 (#14074S, Cell Signaling Technology, MA, USA); rabbit anti-Tip60, 1:5000 (#PA5-23290, Thermo Scientific); anti-Atxn1, 1:2000 (#MABN37, Millipore, MA, USA); mouse anti-RpA1, 1:1000 (H-7, Santa Cruz Biotechnology), anti-γH2AX, 1:1000 (Ser139, #05-636, Millipore); anti-53BP1, 1:10,000 (NB100-304, Novus Biologicals, CO, USA): anti-GAPDH, 1:5000 (MAB374, Millipore, MA, USA); anti-α-tubulin, 1:3000 (T6199, Millipore); anti-β-actin, 1:1000 (sc-47778, Santa Cruz Biotechnology); HRP-linked anti-rabbit IgG, 1:3000 (NA934, GE Healthcare, IL, USA); HRP-linked anti-mouse IgG, 1:3000 (NA931, GE Healthcare). Primary and secondary antibodies were incubated overnight at 4 °C and for 1 h at room temperature (RT), respectively. ECL Prime Western Blotting Detection Reagent (RPN2232, GE Healthcare) and a luminescent image analyzer (ImageQuant LAS 500, GE Healthcare) were used to detect proteins. Uncropped western blots are shown in Supplementary Fig. 9.
Immunoprecipitation
293T or COS-7 cells were transfected with the indicated plasmids and harvested 48 h after transfection. Cells were lysed with TNE buffer (10 mM Tris-HCl (pH 7.5), 150 mM NaCl, 1 mM EDTA, 1% Nonidet P-40). Lysates were collected by centrifugation (15,000×g × 10 min). Aliquots were incubated for 2 h with a 50% slurry of Protein G–Sepharose beads (GE Healthcare). After centrifugation (2000×g × 3 min), the supernatants were incubated with 1 μg of rabbit anti-FLAG antibody (#F7425, SIGMA, St. Louis, MO, USA), mouse anti-Myc antibody (#sc-40, Santa Cruz Biotechnology), or rabbit anti-RORα antibody (#sc-28612, Santa Cruz Biotechnology) overnight at 4 °C; incubated with Protein G–Sepharose beads for 2 h; washed with TNE buffer; and eluted with sample buffer.
Immunohistochemistry
Mouse brains were fixed in 4% paraformaldehyde for 12 h. Paraffin sections (thickness, 5 μm) were de-paraffinized in xylene, re-hydrated, dipped in 0.01 M citrate buffer (pH 6.0), and microwaved at 120 °C for 15 min. After blocking with 10% FBS containing PBS, sections were incubated with primary antibody for 12 h at 4 °C, washed with PBS three times at RT, and incubated with secondary antibodies at RT for 1 h. All procedures were performed in parallel for all mouse groups being compared.
The antibodies used for immunohistochemistry were diluted as follows: rabbit anti-calbindin D-28K antibody, 1:2000 (C2724, Sigma); mouse anti-calbindin D-28K antibody, 1:2000 (C9848, Sigma); rabbit anti-YAP antibody, 1:100 (#sc-15407, Santa Cruz Biotechnology); rabbit anti-YAPdeltaC antibody, 1:1000 (raised against the common COOH-terminal peptide [SVFSRDDSGIEDNDNQ]); rabbit anti-RORα, 1:100 (#sc-28612, Santa Cruz Biotechnology); rabbit anti-Tip60, 1:100 (#sc-25378, Santa Cruz Biotechnology); mouse anti-Atxn1, 1:100 (#MABN37, Millipore); anti-γH2AX, 1:100 (#05-636, Millipore); rabbit anti-53BP1, 1:5000 (NB100-304, Novus Biologicals); mouse anti-RpA1, 1:100 (H-7, Santa Cruz Biotechnology, CA, USA); Cy3-conjugated anti-rabbit IgG, 1:500 (711-165-152, Jackson Laboratory, Bar Harbor, ME, USA); Alexa Fluor 488–conjugated anti-mouse IgG, 1:1000 (A21202, Molecular Probes, Eugene, OR, USA); Cy3-conjugated anti-mouse IgG, 1:500 (715-165-150, Jackson Laboratory); Alexa Fluor 488-conjugated anti-rabbit IgG, 1:1000 (A21206, Molecular Probes).
Confocal microscopy analysis
Fluorescence confocal images were acquired on a laser scanning confocal microscope (LSM510META, Carl Zeiss, Germany; UPLANSAPO ×10, ×40, and ×60; multiline Argon and HeNe(G) lasers; three channels). Acquired images were analyzed using the ImageJ software (http://imagej.nih.gov/ij/) for measurements of signal intensity. The mean values of nuclear signals were compared among three groups (C57BL/6, Atxn1-KI, and Group I).
Luciferase assay
The following plasmids (0.5 μg) were transiently transfected into COS-7 cells (1 × 105 cells/well) using Lipofectamine 2000 (Invitrogen, MA, USA), and luciferase assays were performed using the Dual-Glo Luciferase assay system (Promega, WI, USA) 24 h after transfection. Effector plasmids were RORα-pCIneo, RORα-Y507A-pCIneo, full-length YAP2-pCIneo, and YAPdeltaC-pCIneo, and the reporter plasmid was NRD1-RORE-pGreenfire.
Pull-down assay
GST-RORα (human partial RORα, a.a. 424–523; Abnova, Taipei, Taiwan), His-Tip60 (Cat#10783, Cayman Chemical, Ann Arbor, MI, USA) and His-YAP (MBS717875, MyBioSource, CA, USA) proteins were mixed in 400 μl of reaction solution (PBS with 0.1% Tween-20 and the protease inhibitor cocktail) and incubated for 12 h at 4 °C. After addition of 50 μl of 50% glutathione–Sepharose suspended in reaction solution (Cat#17513201, GE Healthcare), the mixture was incubated for another 3 h at 4 °C, centrifuged at 500×g for 1 min, washed with PBS three times, and solubilized in sample buffer. The samples were then subjected to western blotting. Primary and secondary antibodies were as follows: rabbit anti-YAP (#14074, Cell Signaling Technology, MA, USA); mouse anti-RGS-His (34650, Qiagen); rabbit anti-GST (sc-459, Santa Cruz Biotechnology); HRP-linked anti-mouse IgG, 1:3000 (NA931, GE Healthcare); and HRP-linked anti-rabbit IgG, 1:3000 (NA934, GE Healthcare). Primary and secondary antibodies were incubated overnight at 4 °C and for 1 h at room temperature, respectively. ECL Prime Western Blotting Detection Reagent and an ImageQuant LAS 500 luminescent image analyzer were used to detect proteins.
ChIP assay
ChIP assays were performed using the SimpleChIP plus Enzymatic Chromatin IP kit (Cell Signaling Technology, #9005) following the manufacturer’s protocol with some modifications. In brief, mouse cerebellar tissues (10 mg) were minced in 1 ml of ice-cold PBS; 42.5 μl of 37% formaldehyde was added, and the mixture was incubated for 20 min at room temperature to allow cross-linking. After addition of glycine to stop the cross-linking reaction, the suspended tissues were centrifuged, washed twice with ice-cold PBS, homogenized using a type B Dounce homogenizer, re-suspended in kit Buffer A to perforate the cell membrane, and incubated for 20 min at 37 °C with micrococcal nuclease. Nuclei were destroyed by sonication, and the debris was removed by centrifugation. The clarified nuclear extracts were incubated overnight at 4 °C with anti-YAP antibody or anti-YAPΔC antibody and immunoprecipitated with protein G magnetic beads; the resultant protein–DNA complex was subjected to PCR amplification of the RORE in promoters of target genes. PCR was performed using PrimeSTAR HS DNA polymerase (R010A, Takara Bio Inc., Shiga, Japan). Forward and reverse primers for amplification of RORE were used as follows: Pcp2, 5′-CAGTCCTTAACCTGCAAGGC-3′ and 5′-CCTGGAACTCCTGCTGTCAT-3′; Pcp4, 5′-AATCAACAACCCTCGCTGTC-3′ and 5′-GTTTGGGGTCACCATAGCTT-3′; Slc1A6 5′-GGGCATGTGATTCAGTTGGT-3′ and 5′-GCTTGTGAGCTCTTGTGCAG-3′. PCR conditions were as follows: 35 cycles of 98 °C for 10 s (denaturation), 65 °C for 15 s (annealing), and 72 °C for 60 s (extension).
Quantitative RT-PCR
Total RNA from mouse cerebellum was purified using the RNeasy mini kit (Qiagen, Limburg, Netherlands). Purified total RNA was reverse-transcribed using SuperScript VILO (Invitrogen). Quantitative PCR analyses were performed on a 7500 Real-Time PCR system (Applied Biosystems, Foster City, CA, USA) using the Thunderbird SYBR Green (Toyobo, Osaka, Japan). The primer sequences for RORα target genes, based on information in a previous report, were as follows24:
Mouse A2bp1: forward, 5′-AGACCACTGTCCCTGACCAC-3′; reverse, 5′-CATTTGTCGGAGGTCTGGAT-3′.
Mouse Cyp19a1: forward, 5′-CTTTCAGCCTTTTGGCTTTG-3′; reverse, 5′-ATTTCCACAAGGTGCCTGTC-3′.
Mouse Ctgf: forward, 5′-TGCGAAGCTGACCTGGAGGAAA-3′; reverse, 5′- CCGCAGAACTTAGCCCTGTATG-3′.
Mouse Cyr61: forward, 5′-GTGAAGTGCGTCCTTGTGGACA-3′; reverse, 5′- CTTGACACTGGAGCATCCTGCA-3′.
Mouse Ankrd1; forward, 5′-GCTTAGAAGGACACTTGGCGATC-3′; reverse, 5′-GACATCTGCGTTTCCTCCACGA-3′.
Mouse Bcl-2; forward, 5′-CCTGTGGATGACTGAGTACCTG-3′; reverse, 5′- AGCCAGGAGAAATCAAACAGAGG-3′.
Mouse c-Flip; forward, 5′-GCTCTACAGAGTGAGGCGGTTT-3′; reverse, 5′- CACCAATCTCCATCAGCAGGAC-3′.
Mouse XIAP; forward, 5′- GGCAGAATATGAAGCACGGATCG-3′; reverse, 5′- CACTTGGCTTCCAATCCGTGAG-3′.
Mouse Naip1: forward, 5′- CGAGGTCTCAGAGACAAACCAG-3′; reverse, 5′- GAACTCTCCAGGAAGGACTGAG-3′.
Statistics
One-way ANOVA followed by Tukey’s HSD test was used for comparisons among multiple groups. We performed power analysis to estimate the required sample size (n) for each experiments. All data are shown as mean ± SEM.
Data availability
The authors declare that the data supporting the findings of this study are available within the article and supplementary information or available from the corresponding author upon request.
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Acknowledgements
This work was supported by a Grant-in-Aid for Scientific Research on Innovative Areas (Foundation of Synapse and Neurocircuit Pathology, 22110001 and 22110002) from the Ministry of Education, Culture, Sports, Science and Technology of Japan, a Grant-in-Aid for Scientific Research (A) (16H02655) from Japan Society for Promotion of Science (JSPS), partly Brain Mapping by Integrated Neurotechnologies for Disease Studies (Brain/MINDS) and Strategic Research Program for Brain Sciences (SRPBS) from Japan Agency for Medical Research and Development (AMED), a CREST grant from Japan Science and Technology Agency (JST) and grants for research on intractable diseases from AMED (to H.O.) We thank Dr Huda Y. Zoghbi (Baylor College of Medicine) for Atxn1-KI mice. We also thank Ms. Ayako Seki (TMDU) for manuscript preparation and Dr Hikaru Ito, Mr. Keisuke Kurosu, and Ms. Tayoko Tajima (TMDU) for technical assistance.
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K.F., Y.M. and S.U. performed experiments and wrote the paper. X.C., H.S., T.T., H.I., K.W., H.H. and K.T. performed experiments. M.S. prepared materials and designed research. H.O. planned the project, designed research, and wrote the paper.
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Fujita, K., Mao, Y., Uchida, S. et al. Developmental YAPdeltaC determines adult pathology in a model of spinocerebellar ataxia type 1. Nat Commun 8, 1864 (2017). https://doi.org/10.1038/s41467-017-01790-z
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DOI: https://doi.org/10.1038/s41467-017-01790-z
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