Cerebellar ataxias are severe neurodegenerative disorders with an early onset and progressive and inexorable course of the disease. Here, we report a single point mutation in the gene encoding Elongator complex subunit 6 causing Purkinje neuron degeneration and an ataxia-like phenotype in the mutant wobbly mouse. This mutation destabilizes the complex and compromises its function in translation regulation, leading to protein misfolding, proteotoxic stress, and eventual neuronal death. In addition, we show that substantial microgliosis is triggered by the NLRP3 inflammasome pathway in the cerebellum and that blocking NLRP3 function in vivo significantly delays neuronal degeneration and the onset of ataxia in mutant animals. Our data provide a mechanistic insight into the pathophysiology of a cerebellar ataxia caused by an Elongator mutation, substantiating the increasing body of evidence that alterations of this complex are broadly implicated in the onset of a number of diverse neurological disorders.
Ataxias are the most common neurological deficit resulting from cerebellar dysfunction1,2. These are progressive and currently incurable disorders with gradual deterioration in signs and symptoms, most commonly due to neurodegeneration of an unknown etiology. Affected neurons are Purkinje neurons (PNs) and, rarely, granule neurons. Previous mouse models of cerebellar ataxia have provided insight into the neuropathology of the disease3, however, the precise molecular mechanisms of neuronal loss remain largely unknown.
Using an ab initio N-ethyl-N-nitrosourea (ENU) mutagenesis screen, here we identify a yet uncharacterized Elp6 mutation, which perturbs the stability and function of the murine Elongator complex, and results in a severe ataxic phenotype, the wobbly mouse, with associated microgliosis and degeneration of cerebellar PNs. Elp6 is one of the six subunits (Elp1–6) of the highly conserved eukaryotic Elongator complex, which is organized in two subcomplexes, namely Elp123 and Elp456. It has been shown that all Elongator subunits equally contribute to the stability, integrity, and functionality of the complex in yeast4. Involvement of the complex in various cellular processes, including transcription, cell motility, cytoskeleton organization, exocytosis and intracellular trafficking, has been highlighted by a number of reports5. However, recent studies provide evidence that the above mentioned functions assigned to the complex are downstream effects of its master activity as a global translational regulator6,7. In detail, Elongator-dependent modifications of uridines in the wobble position of tRNA anticodons seem to be of key importance for the fidelity and kinetics of translational elongation, which also guides and directs cotranslational folding dynamics8,9. Over the past decade, a number of studies have showed that the Elongator complex is involved in various cellular activities that govern the development and maintenance of the nervous system10,11,12,13,14. Moreover, several studies have linked the occurrence of specific mutations in Elongator subunits with the onset of various neurological disorders15,16,17,18,19,20. Our results define a mechanism in the pathology of cerebellar ataxias whereby subtle deregulation of tRNA function caused by the Elp6 mutation, leads to protein misfolding, proteome aggregation, and consecutive neuronal death resulting in a severe manifestation of the disease.
Microgliosis following neuronal loss is a normal physiological response to injury, but when this usually transient event becomes chronic and self-propagating, it can lead to sustained neurodegeneration21,22. Hence, microglia do not just provide neuroprotection, but can also promote neurotoxicity. Inflammasomes play a central role in microglia activation, being multiprotein complexes that sense various cellular and environmental stress signals23. The NLRP3 inflammasome is expressed and functional in brain microglia24, and associated with neurodegenerative disorders such as Alzheimer’s disease25, Parkinson’s disease26, multiple sclerosis27, and prion-like diseases28, and is the only inflammasome known to be activated by misfolded proteins and their aggregates via a yet not fully defined mechanism29. It has been suggested that the activation of the NLRP3 inflammasome occurs in response to infection or injury, and involves consequential NLRP3 oligomerization, which serves as a scaffold to nucleate an apoptosis-associated speck-like protein containing a caspase recruitment domain (ASC) that further acts as a docking platform for pro-caspase-1. Ultimately, NLRP3 activation leads to activation of caspase-1, which itself promotes pro-interleukin-1β (IL-1β) processing and release of the mature cytokine IL-1β30. Subsequently, cytokine release promotes inflammation and leads to further damage to neurons already primed for degeneration. Here, we demonstrate that blocking microglial priming by inhibiting the NLRP3 pathway can attenuate PN degeneration and the ataxic phenotype in wobbly mice.
Cerebellar ataxia and PN degeneration in wobbly mice
The wobbly mouse was identified in a recessive ENU-mutagenesis screen on the basis of its wobbly gait. Ataxic symptoms commence at postnatal day (P) 60 in the form of loss of gait coordination and balance, reduced locomotor activity, and abnormal hindlimb clasping, which is commonly observed in mice with a neurodegenerative defect31 (Fig. 1a and Supplementary Fig. 1). The phenotype gradually becomes more pronounced and is most severely manifested by P100. The mutant mice also showed an impaired performance on the rotarod, balance beam and tests in the Catwalk system (Supplementary Fig. 2). The defect was found to occur in a recessive manner, as the phenotype of heterozygous mice was indistinguishable from that of the wild-type animals (Fig. 1a and Supplementary Figs. 1 and 2). Notably, no differences were observed in the performance of male versus female wobbly animals in any of the performed tests (Supplementary Figs. 1 and 2). The mice show no alternations in overall life span, weight, and fertility.
Histological analyses at P60 revealed a specific and substantial loss of PNs in wobbly mice, as we were not able to detect any other changes in overall cerebellar morphology (Fig. 1b). Neuropathology was restricted to PNs in the cerebellum with other central nervous system structures and nonneuronal tissue being unaffected (Supplementary Fig. 3). The first histological signs of PN degeneration were already detectable at P40 and the cerebellum of mutant mice was completely depleted of PNs by P120 (Fig. 1c). Consistent with previous findings that Zebrin II can act as a neuroprotector32,33, we found that PNs of wobbly mice that did not express this molecular marker were more susceptible to cell death than Zebrin II-immuno-positive cells (Supplementary Fig. 4a). Individual variations in the severity of the wobbly phenotype manifestation appeared due to different magnitudes rather than localization of PN loss, which was shown to be consistent across all cerebellar functional subdivisions, from anterior to posterior lobe, across vermis and hemispheres (Supplementary Fig. 4b–j).
To test the functional impact of an underlying mutation, electrophysiological recordings were obtained from PNs in wobbly mice at P21–P24, before motor symptoms were apparent. Already at this stage, PNs exhibited altered passive and active membrane properties (Fig. 1d–f and Supplementary Table 1), and an altered synaptic excitation/inhibition balance (Supplementary Fig. 5 and Supplementary Table 1). In summary, mutant PNs were less excitable showing increased resting membrane potential and action potential threshold and being able to generate significantly fewer action potentials. Parallel fiber stimulation failed to evoke excitatory synaptic currents (EPSCs) in more than 50% of PNs, while evoked synaptic inhibition was shown to be stronger.
Elp6L126Q underlies wobbly mouse phenotype
Whole-exome sequencing of wobbly mice identified a T/A substitution in the Elp6 gene (Fig. 2a), leading to a single amino acid L/Q substitution at position 126 in the protein (Elp6L126Q). To further define Elp6 function in vivo, we generated Elp6 knockout (KO) mice (Supplementary Fig. 6a). Consistent with previous studies that have identified developmental defects following Elp1 and Elp3 ablation20,34, we found that a loss of Elp6 (Elp6−/−) also results in early embryonic lethality (Supplementary Fig. 6b, c). To confirm that the Elp6L126Q allele drives the pathology observed in the wobbly mutant, we crossed Elp6+/− to wobbly mice and screened their progeny for main features of the phenotype. The compound heterozygous (Elp6L126Q/−) animals expressed a more rapidly progressive phenotype than wobbly mice, demonstrating that Elp6L126Q likely functions as a hypomorph. Furthermore, Elp6L126Q/− displayed a decreased survival rate, with 80% of animals not surviving beyond P40 (Fig. 2b). Histological and behavioral analyses of these mice demonstrated a full recapitulation of the wobbly phenotype (Fig. 2c, d). No phenotypic abnormalities were found in Elp6+/− animals, indicating that one copy of wild-type Elp6 is sufficient for proper functioning of the Elongator complex.
In agreement with its here described role, in situ hybridization confirmed wide expression of the Elp456 subcomplex throughout the cerebellum (Supplementary Fig. 7). To establish whether Elp6L126Q-mediated degeneration was an intrinsic defect of PN neurons, a transgenic rescue of the wobbly phenotype was initiated by crossing wobbly mice to transgenic animals expressing the HA-tagged wild-type Elp6 driven by the PN-specific Pcp2 promoter (Pcp2-Elp6-HA; Fig. 3a). Ataxic phenotype and neurodegeneration in Pcp2-Elp6-HA; wobbly mice were fully rescued by the transgene (Fig. 3b–d), demonstrating that despite the widespread expression of the Elongator complex in the cerebellum, PN degeneration is mainly initiated cell-autonomously.
Elp6L126Q negatively affects stability and function of the Elongator complex
Taking advantage of the high sequence conservation of the Elongator subunits among eukaryotes35, the recently determined crystal structure of the yeast Elp456 (yElp456) subcomplex36, and the electron microscopy reconstruction of the fully assembled Elongator complex37, we were able to assess the precise location of the mutated residue within the Elongator complex (Fig. 4a). Despite its detrimental effects, Elp6L126Q resides on the periphery of the complex, distant from known tRNA-, ATP-, SAM-, or acetyl-CoA binding sites and on the side of the Elp456 ring, which is located opposite from the enzymatically active Elp3 subunit and proposed tRNA binding and modification pocket. To understand the consequences of the Elp6L126Q mutation on the molecular level, we produced recombinant mElp456 in bacteria and purified it to homogeneity. The three murine subunits, like yElp456, are able to form a dimeric Elp56 intermediate and a hexameric Elp456 assembly (Fig. 4b and Supplementary Fig. 8a). The introduced Elp6L126Q mutation leads to the destabilization of mElp6 itself (Supplementary Fig. 8b) and the disappearance of the Elp56 intermediate, but still permits hexamer formation (Fig. 4b and Supplementary Fig. 8c). Notably, we observed decreased thermal stability of Elp6L126Q-containing mElp456 hexamers in comparison to wild-type mElp456 (Fig. 4c and Supplementary Fig. 8d). We detected the same effect for full length and truncated versions of Elp456 (lacking predicted disordered regions in the N- and C-termini of Elp4 and Elp5), indicating that the mutation indeed affects the integrity of the core of the complex. The decrease in protein stability appeared to be coupled to reduced tRNA binding capacity in vitro (Supplementary Fig. 8e) and reduced levels of wobble base modification (ncm5U and mcm5U) in brains of wobbly mice in vivo (Fig. 4d). As the decreased in vitro tRNA binding capacity of mutated mElp456 is not restricted to Elongator-modifiable tRNAs, it most likely results from the decreased stability of the hexameric assembly and does not affect the tRNA selection mechanisms. The induced appearance of aggregates in the Elp6L126Q sample at elevated temperatures and nanoDSF analyses independently confirm our thermofluor data and support the notion of a complex stability related reduction in tRNA affinity (Supplementary Fig. 8f). Other tRNA modifications, which are not conducted by Elongator, did not show decreased levels in the analyzed samples. This data demonstrate that Elp6L126Q destabilizes the complex and perturbs its function in the regulation of translation.
Protein misfolding and aggregation in wobbly PNs
Given that perturbation of wobble uridine modifications was shown to lead to ribosome pausing and protein misfolding and aggregation8, we next performed ultrastructural analyses of degenerating neurons to screen for signs of proteotoxic stress. The analyses using transmission electron microscopy revealed extensive autophagy, apoptotic cell features, and an accumulation of electron-dense globular structures that likely represent protein inclusions (Fig. 5a). No signs of necrosis and excitotoxicity were found in wobbly mouse PNs. Increased ubiquitination and upregulation of the molecular chaperone Hsp70 observed in wobbly PNs confirmed the presence of protein aggregates and induced proteotoxic stress response (Fig. 5b). Detection of activated caspase-3 supported apoptosis-mediated cell death. In addition, we show that these cells express the endoplasmic reticulum (ER) stress-induced transcription factor CHOP. This further suggests that apoptosis in wobbly mouse PNs is likely induced by the ER stress elicited by unfolded protein response, as previously described in various other neurodegenerative diseases38.
NLRP3-mediated inflammation contributes to the wobbly pathology
Next, we found prominent histopathological signs for substantial microgliosis (Iba1-marked glial population) (Fig. 6a–c) coupled to reactive astrogliosis (GFAP-marked glial population; Supplementary Fig. 9) in the cerebellum of wobbly mice. The appearance of these inflammatory markers is confined to the cerebellum and strictly associated with PN degeneration. Given that several studies in the past decade have demonstrated that neuroinflammation can be initiated by the inflammasome complexes in microglia activated by protein aggregates23, we further checked for inflammasome activation in our mutant mice cerebella. Notably, the cerebella of the ataxic wobbly mice showed a strong upregulation of key inflammasome effectors, including cleaved caspase-139 and ASC40 (Fig. 6b-d). ASC was shown to be overexpressed and formed so-called specks, previously demonstrated to activate cytokine cascade.
Given the accumulation of protein aggregates in wobbly PNs and recent findings that the NLRP3 inflammasome can specifically act as a sensor for intracellular misfolded proteins29, we used a potent and selective NLRP3-inhibitor MCC95041 to test whether activation of the NLRP3 inflammasome contributes to the progression of neurodegeneration in wobbly mice. Treatment of wobbly mice with MCC950 significantly delayed the onset of ataxia (Fig. 7a) and decreased the rate of neurodegeneration (Fig. 7b), as a consequence of reduced inflammation and inflammasome activity (Fig. 7c–e). To verify these findings, we took a parallel genetic approach by crossing wobbly mice to NLRP3 null animals. Analysis of the ataxic and neurodegenerative features of the double mutant progeny and controls showed that NLRP3 deficiency in vivo mirrored the phenotype of MCC950-treated mutant mice (Fig. 8a, b), further confirming that the NLRP3-driven inflammatory response contributes to the progressive neuropathology in wobbly animals. Reduction of the neuroinflammation in NLRP3 KO; wobbly mice was shown to be even stronger than in MCC950-treated mice (Supplementary Fig. 10a), likely due to a relatively short half-life time of the administrated drug41. Genetic ablation of caspase-1 function in wobbly mice not only reinforced the role of NLRP3 in the progression of neurodegeneration, but also identified caspase-1 as a potential therapeutic target in gliosis-associated ataxias in addition to NLRP3 itself (Fig. 8c, d). Microgliosis and ASC nucleation were found to be reduced to a lesser extent in caspase-1 KO; wobbly animals in comparison to NLRP3 KO; wobbly and MCC950-tretaed wobbly mutants, which is expected given that the inflammatory cascade in these mutants is inhibited downstream of ASC nucleation30.
Our data indicate a mechanistic route underlying neurodegeneration in cerebellar ataxias based on the perturbed function of the Elongator complex in the regulation of translation as a consequence of the destabilizing Elp6L126Q mutation. The mutation was identified in a mouse model for cerebellar ataxia, the wobbly mouse, which develops severe ataxic symptoms as a consequence of extensive Purkinje neurodegeneration. We characterized the ataxic wobbly phenotype in mice and found the induced neurodegeneration on the one hand to follow the pattern of neuroprotective Zebrin II expression and on the other hand to affect all cerebellar functional regions equally. We also showed that intrinsic cellular and synaptic changes of mutant PNs occur prior to clear pathologically recognizable degeneration, which is consistent with observations in other progressive neurodegenerative diseases, such as Alzheimer’s disease42.
On the molecular level, Elp6L126Q destabilizes the assembly and integrity of the heterohexameric Elp456 subcomplex, which is ultimately necessary for tRNA binding and tRNA modification activity of the Elongator complex. Furthermore, we demonstrated that this mutation negatively affects the Elongator activity by detecting lower levels of tRNA modifications in cerebella of mutant mice. Although reduction of tRNA modification levels is relatively modest, our data is in line with another report on the Elongator mutation that causes familial dysautonomia43. In this rare disease, similar levels of reduction in tRNA modifications were observed (29–36% of reduction) in patient-derived samples. Together these observations indicate a scenario, where a certain level of reduction in modification levels causes severe cellular malfunctions, but still permits survival of the patients.
The Elongator-dependent mcm5U and ncm5U modifications have been shown to be of crucial importance for the fidelity and kinetics of protein synthesis and cotranslational folding dynamics8,9. In concordance, we found defects in translational fidelity and protein folding in wobbly PNs. Hence, we show that the Elp6L126Q-mediated impaired function of the complex likely results in protein misfolding and aggregation that further induces ER-stress and subsequent apoptosis.
Protein aggregation is a common cause of neuronal death shared by various neurological disorders44,45, as aggregated proteins commonly lose their physiological function and gain undesired toxic properties. As in vast majority of neurodegenerative diseases, cellular pathology is only observed in a specific neuronal subtype in wobbly mice, namely PNs. Our transgenic complementation study demonstrates that Elongator is a key regulator of PN integrity and although the observed pathological findings were found to be cell-intrinsic in ataxic mice, the cause of this selectivity remains elusive. In general, neurons are known to be highly sensitive to the presence of misfolded proteins given that they are postmitotic and cannot dilute toxic aggregates by cell division. PNs may be particularly sensitive to deleterious effects of these toxic species as they have an extraordinary high metabolic demand11,46. Although codon-dependent regulation of translation by the Elongator complex has been previously reported6, protein aggregates induced in yeast and worms by Elongator depletion show no specific accumulation of these Elongator-codon enriched proteins. Therefore, the slightly decreased tRNA modification levels primarily might have a large impact on the proper translation of individual trigger proteins, which nucleate and propagate the appearance of large aggregates and induce proteotoxic stress in the context of whole proteome, as suggested by previous studies8. The study presented here adds to an emerging consensus that perturbations of the Elongator complex contribute to a range of neurological and neurodevelopmental disorders, including familial dysautonomia15, amyotrophic lateral sclerosis17,20, rolandic epilepsy18, and intellectual disability16,19. The mechanism by which specific mutations in different Elongator subunits cause different neuropathologies, remains intriguing and needs to be further clarified.
A number of studies in the past decade have demonstrated that neuroinflammation initiated by the activation of inflammasome complexes in microglia underlies a variety of neuronal phenotypes23. Here, we have demonstrated that despite the fundamental mechanism of neuronal death being cell autonomous, activation of the NLRP3 inflammasome contributes significantly to the rate of neuronal loss in wobbly mice. Thus, PNs are both dying due to an intrinsic defect and being killed by an extrinsic inflammatory response. Gliosis is a common observation in a number of neurodegenerative conditions and our findings in ataxic mice experimentally confirm an increasing body of evidence proposing a common mechanism of NLRP3-mediated neuroinflammation to underlie and contribute to the pathogenesis of various neurodegenerative diseases25,26,27,28. Whether NLRP3 activation is a direct consequence of the Elongator complex malfunction in wobbly mice or it is triggered by a release of danger-associated molecular patterns (DAMPs) from dying neurons, has to be investigated in the future. It has been previously established that NLRP3 activation is initiated by aggregated proteins, such as Lewy bodies in Parkinson’s disease26, amyloid-β peptides in Alzheimer’s disease25 and prions in prion-related disorders28. Thus, the NLRP3-mediated inflammatory cascade is likely to be triggered by the presence of protein aggregates in wobbly PNs. Previous studies demonstrated that the NLRP3 activation not only results in cytokine-induced neuronal damage, but also in poor microglial aggregate clearance resulting in accumulation of toxic aggregates that leads to further neuronal demise47,48. In order to assess whether aggregates are responsible for the NLRP3-mediated neuroinflammation in cerebellar ataxia or the inflammatory response is induced by neuron-derived DAMPs, different ataxia mouse models with and without the involvement of preoteinopathy need to be compared.
For cerebellar ataxia patients, prognosis is currently bleak and therapies in use are limited to symptomatic treatment with no pharmaceutical intervention available to ameliorate the disease pathology. Data presented here not only define a fundamental understanding of cerebellar neurodegeneration caused by the Elongator mutation, but also identify a potential therapeutic strategy to substantially delay the course of the disease. Hereditary ataxias display a variety of inheritance modes and the plethora of genetic pathways known to cause these conditions makes it difficult to conceive of a single pan-ataxia therapeutic approach. Though, several studies suggest that the majority of ataxias have some broad commonalities, such as protein aggregation, metabolic deficits, and perturbation in ion channel function49. Despite the potentially different biochemical bases that trigger neurodegeneration, a common feature of ataxias is the accompanying induction of neuroinflammation, and in particular microglial activation50,51,52,53. It is clear that the role of sterile inflammation in neurological diseases is a field that is generating great interest and our study provides the first instance that blocking inflammasome activation can significantly ameliorate neurodegeneration in ataxia by targeting the associated activated gliosis.
Animals and genotyping strategies
All animal experiments were approved by the University of Queensland Molecular Biosciences Ethics Committee (project license numbers IMB/098/14 and IMB/097/14). Mice were housed under a 12 h light cycle in a specific-pathogen-free climate-controlled facility with food and water provided ad libitum. Genomic DNA for genotyping purposes was obtained from tail tips using QuickExtract DNAextraction solution (Epicenter) as per the manufacturer’s instructions. The genetic background of all animals, including wobbly, Elp6 KO, transgenic (Pcp2-Elp6-HA), NLRP3 KO and Casp-1 KO mice, was C57BL/6. No gender-related phenotypic differences were observed in all mice strains. Both sexes were found to be fertile with normal life span and body weight. The wobbly mutation arose from an ENU-mutagenesis phenotype-driven screen at the Australian Phenomic Facility, the Australian National University. This strain has been archived with the Australian Phenome Bank, ID 4118. Whole-exome sequencing revealed the homozygous Elp6L126Q mutation. A custom TaqMan SNP genotyping assay was used to genotype the animals through qPCR reaction based on allelic discrimination. Primers used were: forward 5′-AAACCTGCAGTCACTGTATACGTT-3′ and reverse 5′-CAACAGACTGGGTACTTCCAT-3′, with the cycling conditions: 95 °C for 10 min, followed by 40 cycles of denaturation step at 92 °C for 15 s, and annealing and extension at 60 °C for 90 s. The amplified product of 88 bp was further annealed with either VIC-labeled wild-type Elp6 sequence 5′-AGGACACCCTGAAGCC-3′ or fluorescein-labeled wobbly (Elp6L126Q) sequence 5′-AGGACACCCAGAAGCC-3′. For MCC950 treatment studies, wobbly mice were dosed orally via drinking water (0.3 mg/ml), from P21 until sacrifice. Elp6 functional KO mice were generated using CRISPR-Cas9 technology with the gRNA sequence: 5′-CCCCAGACAAGACCGAGCAG-3′ (Supplementary Fig. 3a). Primers used for genotyping were: forward 5′-CCCTGAGCCATCTCTTTGGC-3′ and reverse 5′-AGTGTTCCGTGCAACCTGTAA-3′, with an amplified product of 920 bp, further analyzed by Sanger sequencing. Transgenic animals were generated by pro-nuclear injection of the Pcp2-Elp6-HA construct into fertilized egg. Pcp2 minigene was previously reported and was a generous gift from Professor Jaroslaw Barski54. Elp6 cDNA was HA-tagged at the C-terminus and inserted into exon 4 of the Pcp2 minigene, followed by linearization of the construct by Hind III and EcoRI digestion, purification and pro-nuclear injection. Transgenic mice were genotyped by PCR reaction using forward 5′-GCCTTGGTATCCTCCTG-3′ and reverse 5′-CCAGGAACACAAGCTGCCCTCTGTCCCG-3′ primers, which generated a 671 bp product in Pcp2-Elp6-HA animals. PCR products were amplified using the following conditions: initial denaturation for 4 min at 94 °C followed by 35 cycles of 94 °C for 30 s, 58 °C for 30 s and 72 °C for 60 s, and a final single extension step of 72 °C for 10 min.
The simple composite phenotype scoring system used was a modified version of the scoring system for evaluating mouse models for spinocerebellar ataxias55. The system was based on the hindlimb clasping, open field and ledge tests. All tests were scored on a scale of 0–2, with a combined total of 0–6 for all three tests. Each test was repeated three times and the mean value of the scores was recorded. Time points chosen for testing mice were P21, P40, P60, P80, P100, and P120.
The ledge test: a mouse was lifted from the cage and placed on the cage’s ledge. A score of 0: a mouse walked along the ledge without losing its balance, and lowered itself back into the cage using its paws. A score of 1: a mouse showed signs of tremor and lost its footing while walking along the ledge. A score of 2: severe tremor was observed and the mouse fell off the ledge, or shaked and refused to move despite encouragement.
Hindlimb clasping: a mouse was grasped by the tail near its base and lifted to observe the hindlimb position for 10 s. A score of 0: the hindlimbs were consistently splayed outward, away from the abdomen. A score of 1: both hindlimbs were partially retracted toward the abdomen for more than 50% of the observation time. A score of 2: hindlimbs were entirely retracted and touching the abdomen for more than 50% of the observation time.
Locomotor activity: the test was performed in an arena with walls to prevent escape. A mouse was placed in the center of the open field, and its movement around the arena (horizontal activity) together with the rearing (vertical activity) was recorded for 5 min. A score of 0: a mouse moved normally, with its body weight supported on all limbs, and actively explored its surrounding, showing normal horizontal and vertical activity. A score of 1: tremor was present in both, horizontal and vertical activity of the mouse, and both activities were decreased. A score of 2: a mouse had difficulty to move forward and/or fell down on a side while walking, therefore showing a significant decrease in horizontal activity, while no vertical activity was observed.
P100 animals were additionally tested using rotarod, balance beam and Catwalk system. Mice were trained for three days (three trials a day) prior to recording the final score.
Rotarod: maximum time allowed for the rotarod test was 120 s. The acceleration was from 4 to 40 rpm within 60 s. The latency to fall (time spent on the rotating road) and the speed at the time of drop (rmp) were recorded.
Balance beam: mice were trained to walk from a start platform along a wooden beam elevated 30 cm above the ground, 80 cm long and 3 cm wide gradually narrowing to 1 cm, ending at the goal box. The mouse was placed on the wide end of the beam and allowed to walk the beam distance and enter the goal box. The distance crossed (cm) and the number of missteps was recorded.
Catwalk: mice were allowed to walk across the glass walkway in an unforced manner at least six times a day. Mouse tracks that were straight without any interruption or hesitation were treated as successful runs. Runs with any wall climbing, grooming, and staying on the walkway were not analyzed. Mice that failed the Catwalk training were excluded from the study. An average number of eight replicate crossings made by each mouse was recorded. The Catwalk software was used to analyze crossings that had at least five cycles of complete steps. Gait parameters, such as regularity index and base of support, were collected and compared between groups.
All behavioral analyses were performed by researchers blinded to the genotype of the animals.
MCC950 treatment studies
Mice were dosed orally via drinking water (0.3 mg/ml) ad libitum starting at P21 until sacrificed at P120. The MCC950 dose to be used was established in a pilot study where we assessed the penetrance of the drug into the brain tissue of mice at levels above the IC50 of the drug (n = 3 for MCC950-treated and control animals). The concentration of the drug was measured in blood plasma and brain tissue upon transcardial perfusion with PBS.
Tissue and embryo collection
Experimental animals were anaesthetized using Dormitor (1 mg/kg, i.p.) and Zoletil (50 mg/kg, i.p.) and transcardial perfusion was performed with PBS, followed by 4% PFA solution. The brains were dissected and drop-fixed in 4% PFA at 4 °C for 12 h under constant agitation. The following day, brains were washed twice with PBS and left overnight in PBS. Brains were processed in the Leica TP1020 tissue processor over 15 h as per the user’s guide and subsequently embedded in paraffin and sectioned at 7 μm either in the transverse or sagittal plain using Leica RM2235 microtome. Sections were transferred to glass slides and dried overnight at 45 °C. Embryos were explanted and placed into cold PBS, followed by 4% PFA fixation for 6 h at 4 °C and subsequent series of PBS washing.
Following deparaffinization, slides were stained in Hematoxylin (Sigma Aldrich) for 3 min. The excess of Hematoxylin stain was removed by short immersion of slides in 1% HCl acid solution followed by another short immersion in 0.1% LiCO3 solution. Samples were then stained with Eosin Y solution (Sigma Aldrich) for 30 s and dehydrated using 70, 90, and 100% ethanol for 30 s each, followed by xylene for 10 min. Slides were mounted with Entellan mounting medium (ProSciTech) and dried for 1 h. Images were obtained using Olympus BX-51 upright bright-field microscope.
Upon deparaffinization and hydration, the slides underwent heat-induced antigen retrieval using citrate buffer-based antigen unmasking solution (Abacus) at 100 °C for 10 min. Mouse on Mouse (M.O.M.) blocking reagent (Vector) was used to block endogenous mouse antibody in the tissue section (when a primary antibody was raised in mouse) or bovine serum albumin was used to block unspecific binding of antibodies (when an antibody was not in other specie than mouse). Slides were incubated with primary antibodies: Pcp2 (1:100; sc-49072), Zebrin II (1:50; ab115212), Iba1 (1:400; ab5076), ASC (1:400; Al177), Casp-3 (1:100; ab2302), Hsp70 (1:100; sc-66048), Ub (1:100; ab7780), and HA (1:100; ab9110), followed by incubation with an AF488, AF594, or AF647-labeled donkey anti-mouse, anti-rabbit or anti-goat IgG antibody (1:250; Invitrogen), and counterstained with DAPI (Sigma Aldrich). Images were captured using Zeiss LSM 710 upright confocal microscope as Z-stacks and presented as the sum of the Z-projection. The number of Pcp2-labeled or Iba1-labeled cells was determined separately in every visible lobule of the vermis and in the hemispheres. For each mouse, three nonadjacent sections (separated by 70 μm) from the region of vermis were analyzed and the mean value was recorded. Total of five mutant and five control animals was included in each of the studies.
Excised cerebella were quickly trimmed and immediately immersed in 2.5% glutaraldehyde in cacodylate buffer for 48 h and then postfixed in reduced osmium, en-bloc stained with 2% uranyl acetate and dehydrated through ethanol solutions, before final embedding in Epon812 resin (ProSciTech). Ultra-thin sections were cut on a Leica UC6 Ultra microtome and viewed on a JEOL 1011 electron microscope (JEOL Australasia Pty Ltd) at 80 kV. Images were captured using iTEM software (Soft Imaging System, Olympus).
In situ hybridization
Total RNA was extracted from granule neuron precursors isolated from P7 wild-type animals56 using RNeasy micro kit (QIAGEN) following the protocol supplied. Subsequently, cDNA was obtained using the protocol from SuperScript III first-strand synthesis kit (Thermo Fisher). The probes were amplified using above mentioned PCR conditions. Primers were designed in the 3′UTR region of the Elp4-6 cDNA: Elp4 forward 5′-CGACTGCATTTGCCTCCAGACTTGTCAGAC-3′ and reverse 5′-GTTCTACACTCTATGGGGTGTGCCATGCC-3′, Elp5 forward 5′-GCTTCATGGCCCAGGCTCCATGGG-3′ and reverse 5′-CACACTCATCCTAGCTTGATGCTGCTCCTTGGC-3′, Elp6 forward 5′-GCCTCACCTGCCTGTTTTTG-3′ and reverse 5′-GTCCCAGTGCCATGCTTTTG-3′. DIG RNA labeling kit (Roche) was used to synthesize the RNA probes and the probes were purified using the RNA cleanup protocol from the RNeasy mini kit (QIAGEN). In situ hybridization on P21 sagittal brain sections was carried out following the established protocol57.
Mouse cerebellum whole-tissue lysate was prepared by homogenization in radioimmunoprecipitation assay (RIPA) buffer. Protein concentrations were determined using BCA protein assay (Pierce). The XCell SureLock mini-cell electrophoresis system (Thermo Fisher Scientific) was used for SDS-PAGE and wet protein transfer. Proteins were transferred onto nitrocellulose membranes at 25 V for 90 min and detected by immunoblotting using relevant primary and horseradish peroxidase-conjugated secondary antibodies. Peroxidase activity was further detected using SuperSignal West Pico chemiluminescent reagent (Thermo Fisher Scientific). The membrane was exposed to an X-ray film for 30 s–2 min prior to development using X-omat film developer. Densitometric analysis of western blot images was performed using ImageJ software.
Whole-cell recordings were obtained from PNs in 300 μm-thick sagittal brain slices from P21–26 wobbly and wild-type mice. Mice were anesthetized with isoflurane, decapitated, and 300 μm-thick sagittal brain slices prepared in an ice-cold sucrose solution using a vibratome (Leica). Brain slices were continuously perfused with oxygenated aCSF (32 °C) and whole-cell patch-clamp recordings were performed as previously described58. Spiking was evoked using current injections applied in increments of 20 pA from −60 to 340 pA. In the case of spontaneous excitatory postsynaptic current (sEPSC) recordings, Purkinje cells were clamped at −60 mV and recorded for 10 min. For electrical stimulation, a theta-glass stimulator (Harvard apparatus glass capillaries) was filled with aCSF and placed in the molecular layer of cerebellar sagittal slices to stimulate parallel fibers. Induced inhibitory postsynaptic current (IPSC) and EPSC were recorded, while holding PNs at −40 and −60 mV, respectively. Input resistance, action potential threshold, amplitude, delay, half width, rise time, sEPSCs, IPSCs, and EPSCs were analyzed offline. No corrections were made for liquid junction potentials.
tRNA modification analyses
Total RNA was isolated from ~100 mg cerebellar tissue using TRIzol reagent (Life Technologies). After TRIzol addition, the tissue was homogenized with ceramic beads (Sapphire Bioscience) in tissue homogenizer (Bertin Technologies). Total tRNA was isolated from low melting point agarose gel (Progen) following the protocol for β-agarase I provided by manufacturer (NEB). After completion of gel digestion reaction, tRNA was extracted with water-saturated phenol followed by repetitive chloroform extraction and precipitation by ethanol; 8–10 ng of tRNA was recovered for each sample. tRNA purity and quality was confirmed by 8% urea–PAGE electrophoresis in TBE–buffer. Hydrolysis of tRNA to nucleosides was performed as previously described59. A Prominence ultra high performance liquid chromatography (HPLC) system (Shimadzu, Australia) was used to perform reversed phase separation of the samples using a Luna Omega 1.6 µm, Polar-C18 100A column (150 mm × 2.1 mm, Phenomenex, Australia) at a temperature of 35 °C. A 10-µl aliquot of the samples in 0.1% formic acid (aq) was injected onto the HPLC column. The mobile phase consisted of solvent A (0.1% formic acid (aq)) and solvent B (acetonitrile/0.1% formic acid). Chromatographic separation was achieved using a gradient elution program of 0% buffer B for 4 min, 0–20% for 21 min, 20–40% for 2 min, 40–80% buffer B for 1 min, followed by washing with 80% buffer for 2 min and returning to 0% for equilibration of the column before the next sample injection. The flow rate was 200 µl/min. The RP-HPLC column was directly connected to the TurboIonSpray source of the mass spectrometer. Selected reaction ion monitoring (SRM) mass spectrometry experiments were performed on a hybrid quadrupole/linear ion trap 4000 QTRAP MS/MS system (SCIEX, California, USA). All analyses were performed using SRM positive ion acquisition mode. Mass spectrometer parameters were optimized for targeted ribonucleosides using multiple injections of 0.1–1 ng of uridine, cytidine, adenine, guanine, as well as commercially obtained 5-methylcytidine (Abcam), 7-methylguanosine, inosine, 5-methyluridine and 2′-O-methyladenosine (MetaGene). The obtained retention times were superimposed with the previously published results59. Mass Spectrometer Source conditions used were: Declustering Potential, DP: 60, Curtain Gas: 40, Collision Gas (CAD): Medium, Ion Spray Voltage: 5300, Temperature GS2: 500, Ion Source Gas 1: 70, Ion Source Gas 2: 80. SRM Transitions: Resolution set to Unit, Unit for both Q1 and Q3 respectively; Dwell Time 130 ms except for U, which was 5 ms, was used for data analysis and quantification. An analytical method was developed for the simultaneous analysis of 33 modified ribonucleosides of which 5 compounds of interest were targeted for quantification (Supplementary Table 2). 5-Methylcytidine served as an internal normalization standard. To confirm the correct retention time, the standard was added to control sample aliquots at 0.01 or 0.1 ng. Analyst 1.6.2 software was used for peak assignment, area calculation and normalization. Corresponding structures and molecular masses were obtained from Modomics database60
Localization of mElp456L126Q within the structure of the Elongator complex
Elp6 from S. cerevisiae (Q04868) was used as a template to identify and align Elp6 sequences from mouse (Q8BK75) and human (AAH00623). Structural comparisons and models were prepared using Phyre261 and Modeler62. Atomic models of Elp456 (PDB ID 4A8J) and holoElongator were used to identify L126Q and to prepare structural figures using Pymol63.
Protein expression and purification
Coexpression constructs encoding mouse Elongator subunits were designed as previously described for yElp4569. Constructs encoding truncations and mutations of mElp4, mElp5, and full-length mElp6 were created using standard quick-change protocol. mElp6 and mElp6L126Q were cloned into pETM11 using standard cloning procedures. All constructs were expressed in E. coli (BL21 pRARE) after transformation using electroporation. In detail, bacteria were grown in TB at 37 °C until an OD600 of ~1.2, followed by induction with 1 mM IPTG and subsequent incubation at 18 °C for 12–15 h. Bacteria were lysed in 50 mM HEPES (pH 7.5), 300 Mm NaCl, 10 mM imidazole, 1 mM β-mercaptoethanol, 5% (v/v) glycerol, DNAse and protease inhibitors using a homogenizer. The soluble fractions were cleared by centrifugation (70,000×g for 45 min at 4 °C), and proteins were further purified using NiNTA affinity chromatography, followed by size-exclusion chromatography on a 16/600 HiLoad Superdex 200 pg column (GE Healthcare) and/or Superdex 200 Increased (10/300) in 20 mM HEPES (pH 7.5), 150 mM NaCl and 5 mM DTT. Respective fractions were analyzed by SDS-PAGE, pooled and concentrated.
Thermal shift assay
Thermal shift assays were performed to monitor protein unfolding using thermofluor technology64. Thermofluor assays were conducted in the CFX96 Real-Time System C1000 Touch Thermal Cycler (Biorad). Varying concentrations of protein samples (1–0.25 mg/ml) were incubated with SYPRO Orange and 20 mM HEPES (pH 7.5), 150 mM NaCl, 5 mM DTT buffer. Samples were gradually heated from 4 to 98 °C at a heating rate of 0.2 °C/10 s. The fluorescence intensity was measured at probe specific excitation (470 nm) and emission (570 nm) wavelengths.
Microscale thermophoresis (MST) experiments were performed to determine binding affinities of Cy5-labeled tRNAAla and tRNACys from S. cerevisiae (at concentration 210 and 55 nM) and purified Elp456 complexes. Proteins were titrated in a 1:1 dilution series in 20 mM HEPES pH 7.5, 50 mM NaCl, 2 mM DTT, 0.05% Tween, whereas labeled tRNA concentrations stayed constant. Samples were loaded into Monolith™ NT.115 MST Premium Coated Capillaries (NanoTemper Technologies) and measured using a Monolith NT.115 at room temperature (light-emitting diode (LED)/excitation power setting 20%, MST power setting 20%). Data was analyzed using MO. Affinity analysis software at the standard MST on time of 5 s.
Nano differential scanning fluorimetry
NanoDSF experiments were performed to determine protein stability employing intrinsic tryptophan or tyrosine fluorescence of purified Elp456 complexes. Proteins were diluted to concentration 100 µg/ml in 20 mM HEPES pH 7.5, 50 mM NaCl, 2 mM DTT. Samples were loaded into Prometheus NT.48 Series nanoDSF Grade High Sensitivity Capillaries (NanoTemper Technologies) and measured using a Prometheus NT.48 at temperature range from 20 to 95 °C (LED/excitation power setting 10%, temperature slope 2 °C/min). Data was analyzed using NanoTemper software, n = 3.
Data analysis and statistics
Statistical analyses were performed using the GraphPad Prism software V6. To determine statistical significance, the unpaired two-tailed t test was performed. For the simple composite phenotype scoring system for cerebellar ataxia and the quantification of PNs, Iba1 and ASC specks at different ages, two-way-analysis of variance (ANOVA) was used. To test for difference of each dependent variable in different age groups, Sidak’s test was used.
Data generated in this publication are available from corresponding authors on reasonable request.
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The authors acknowledge the facilities, and the scientific and technical assistance of the Australian Phenomics Facility (APF), the Australian National University. The APF is supported by the Australian Phenomics Network (APN). The APN is supported by the Australian Government through the National Collaborative Research Infrastructure Strategy (NCRIS) program. We are very grateful to Jelena Bezbradica Mirkovic and Kate Schroder for providing NLRP3 KO and Caspase-1 KO animals and for their valuable discussion. We also thank Avril Robertson and Matthew Cooper for the gift of MCC950 and Trent Woodruff for advice regarding the administration of MCC950. We acknowledge Ting-Yu Lin and Andrzej Chramiec-Głąbik for providing labeled tRNAs. This work was supported by the POLONEZ1 Grant UMO-2015/19/P/NZ1/02514 from the National Science Centre, Poland and received funding from the European Union’s Horizon 2020 research and innovation program under the Marie Skłodowska-Curie grant agreement No. 665778 (M.G. and A.S.-K.) and the First Team grant First TEAM/2016-1/2 from the Foundation for Polish Science (S.G.).
The authors declare no competing interests.
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Kojic, M., Gaik, M., Kiska, B. et al. Elongator mutation in mice induces neurodegeneration and ataxia-like behavior. Nat Commun 9, 3195 (2018). https://doi.org/10.1038/s41467-018-05765-6
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