TDP-43 and RNA form amyloid-like myo-granules in regenerating muscle

Vogler, Thomas O.; Wheeler, Joshua; Nguyen, Éric; Hughes, Michael P.; Britson, Kyla A.; Lester, Evan; Rao, Bhalchandra S.; Betta, Nicole Dalla; Whitney, Oscar N.; Ewachiw, Theodore; Gomes, Edward; Shorter, James; Lloyd, Thomas E.; Eisenberg, David; Taylor, J. Paul; Johnson, Aaron; Olwin, Bradley B.; Parker, Roy

doi:10.1038/s41586-018-0665-2

Cited by 181 publications

(198 citation statements)

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“…Identifying human genes affected by cryptic exon insertion arising from TDP-43 dysfunction and understanding the consequences of their disruption is thus important for understanding both the normal mechanisms whereby TDP-43 ensures splicing fidelity as well as the contributions of aberrant mRNA splicing to disease pathology. In addition to regulating mRNA splicing, TDP-43 has also been implicated in the regulation of other aspects of RNA biology including: transcription, microRNA processing, RNA stability and regulation of cytoplasmic ribonucleoprotein complexes such as stress granules, myo-granules involved in muscle regeneration and granules involved in axonal RNA transport in neurons (Gopal et al, 2017;Ratti and Buratti, 2016;Vogler et al, 2018).…”

Section: Introductionmentioning

confidence: 99%

Pleiotropic requirements for human TDP-43 in the regulation of cell and organelle homeostasis

Roczniak-Ferguson

Ferguson

2019

Preprint

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TDP-43 is an RNA-binding protein that forms cytoplasmic aggregates in multiple neurodegenerative diseases. Although the loss of normal TDP-43 functions likely contributes to disease pathogenesis, the cell biological consequences of human TDP-43 depletion are not well understood. We therefore generated human TDP-43 knockout cells and subjected them to parallel cell biological and transcriptomic analyses. These efforts yielded three important discoveries. First, complete loss of TDP-43 resulted in widespread morphological defects related to multiple organelles including: Golgi, endosomes, lysosomes, mitochondria and the nuclear envelope. Second, we identified a new role for TDP-43 in controlling mRNA splicing of Nup188 (nuclear pore protein). Third, analysis of multiple amyotrophic lateral sclerosis (ALS) causing TDP-43 mutations revealed a broad ability to support splicing of TDP-43 target genes. However, as some TDP-43 disease causing mutants failed to support the regulation of specific target transcripts, our results raise the possibility of mutation-specific loss-of-function contributions to disease pathology.

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Section: Introductionmentioning

confidence: 99%

Pleiotropic requirements for human TDP-43 in the regulation of cell and organelle homeostasis

Roczniak-Ferguson

Ferguson

2019

Preprint

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“…In ALS, skeletal muscle harbours the characteristic protein aggregates (composed principally of TDP-43) [15] whose burden in the CNS predicts neurodegeneration [16,17]. In muscle, these TDP-43 protein aggregates may disrupt the transport of mRNAs essential for muscle fibre regeneration [18,19]. Together these findings support a direct contribution of skeletal muscle to the ALS phenotype.…”

Section: Introductionmentioning

confidence: 88%

“…Overall, 179, 18, 286 and 135 SNPs were associated with GS, MG, MS and, ALS, respectively, at a suggestive level of significance (p ≤ 5x10 -6 ). Using the CoDeS3D algorithm [40], we mapped spatial regulatory connections between each phenotype-associated SNP and one or more gene coding regions (GENCODE release 19). For each SNP-gene pair, spatial contacts were identified from existing Hi-C [38] chromatin contact data derived from eight immortalized cell lines representing human germ layer lineages (GM12878, IMR90, HMEC, NHEK, K562, HUVEC, HeLa and KBM7) [41] and one tissue (Psoas muscle) [42] (Table S1).…”

Section: Identification Of Functionally Significant Spatial Regulatormentioning

confidence: 99%

Shared regulatory pathways reveal novel genetic correlations between grip strength and neuromuscular disorders

Gokuladhas

Schierding

Cameron‐Smith

et al. 2019

Preprint

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AbstractBackgroundMuscle weakness and muscle wasting can be a consequence of aging (sarcopenia) and neuromuscular disorders (NMD). Genome-wide association (GWA) studies have identified genetic variants associated with grip strength (GS, an inverse measure of muscle weakness) and NMD (multiple sclerosis (MS), myasthenia gravis (MG) and amyotrophic lateral sclerosis (ALS)). However, how these variants contribute to the muscle weakness caused by aging or NMD remains obscure.MethodsWe have integrated GS and NMD associated SNPs in a multimorbid analysis that leverages high-throughput chromatin interaction (Hi-C) data and expression quantitative trait loci (eQTL) data to identify allele-specific gene regulation (i.e. eGenes). Pathways and shared drug targets that are enriched by colocalised eGenes were then identified using pathway and drug enrichment analysis.ResultsWe identified gene regulatory mechanisms (eQTL-eGene effects) associated with GS, MG, MS and ALS. The eQTLs associated with GS regulate a subset of eGenes that are also regulated by the eQTLs of MS, MG and ALS. Yet, we did not find any eGenes commonly regulated by all four phenotypes associated eQTLs. By contrast, we identified three pathways (mTOR signaling, axon guidance, and alcoholism) that are commonly affected by the gene regulatory mechanisms associated with all four phenotypes. 13% of the eGenes we identified were known drug targets, and GS shares at least one druggable eGene and pathway with each of the NMD phenotypes.ConclusionsCollectively, these findings identify significant biological overlaps between GS and NMD, demonstrating the potential for spatial genetic analysis to identify mechanisms underlying muscle weakness due to aging and NMD.

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“…Under conditions of cellular stress, both TDP-43 and FUS re-localize into cytoplasmic stress granules (SGs) [6,7], which are dynamic mRNA-protein assemblies implicated in regulating mRNA function [8,9]. Given this, and in light of ALS-associated mutations that generally reduce SG dynamics, SGs have been theorized to promote formation of TDP-43 and FUS aggregates that are observed in ALS patients [10,11], though recent studies suggest SG-independent aggregation mechanism also likely exist [12][13] [14]. Regardless, various studies indicate that TDP-43 and FUS aggregates, or simply excessive cytoplasmic localization of TDP-43 or FUS, may result in a toxic gain of function that leads to motor-neuron degeneration [15][16][17][18][19] [20,21].…”

Section: Introductionmentioning

confidence: 99%

Cdc48/VCP and endocytosis regulate TDP-43 and FUS toxicity and turnover

Liu¹,

Byrd²,

Pei³

et al. 2019

Preprint

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Amyotrophic lateral sclerosis (ALS) is a fatal motor neuron degenerative disease. TDP-43 (TAR DNA-binding protein 43) and FUS (fused in sarcoma) are aggregation-prone RNA-binding proteins that in ALS can mis-localize to the cytoplasm of affected motor neuron cells, often forming cytoplasmic aggregates in the process. Such mis-localization and aggregation are implicated in ALS pathology, though the mechanisms of TDP-43 and FUS cytoplasmic toxicity remains unclear.Recently, we determined that the endocytic function aids turnover of TDP-43 and reduces TDP-43 toxicity. Here, we identified that Cdc48 and Ubx3, a Cdc48 co-factor implicated in endocytic function, regulates the turnover and toxicity of TDP-43 and FUS expressed in S. cerevisiae. Cdc48 physically interacts and co-localizes with TDP-43, as does VCP in ALS patient tissue. In yeast, FUS toxicity also depends strongly on endocytic function, but not autophagy under normal conditions. FUS expression also impairs endocytic function, as previously observed with TDP-43. Taken together, our data identifies a role for Cdc48/VCP and endocytosis function in regulating TDP-43 and FUS toxicity and turnover. Furthermore, endocytic dysfunction may be a common defect affecting cytoplasmic clearance of ALS aggregation-prone proteins and may represent a novel therapeutic target of promise. KeywordsCdc48, VCP, Endocytosis, TDP-43, FUS, ALS Abbreviations ALS -Amyotrophic Lateral Sclerosis CORVET -class C core vacuole/endosome tethering CHX -Cycloheximide EGFR -Epidermal growth factor receptor FTLD -Frontotemporal lobar dementia FUS -Fused in Sarcoma HOPS -homotypic fusion and vacuole protein sorting IBMPFD -Inclusion Body Myopathy with early onset Pagets disease and Frontotemporal Dementia RRM -RNA Recognition Motif SG -Stress granule TDP-43 -TAR DNA binding protein 43 VCP -Vasolin containing proteinUnder conditions of cellular stress, both TDP-43 and FUS re-localize into cytoplasmic stress granules (SGs) [6,7], which are dynamic mRNA-protein assemblies implicated in regulating mRNA function [8,9]. Given this, and in light of ALS-associated mutations that generally reduce SG dynamics, SGs have been theorized to promote formation of TDP-43 and FUS aggregates that are observed in ALS patients [10,11], though recent studies suggest SG-independent aggregation mechanism also likely exist [12][13] [14]. Regardless, various studies indicate that TDP-43 and FUS aggregates, or simply excessive cytoplasmic localization of TDP-43 or FUS, may result in a toxic gain of function that leads to motor-neuron degeneration [15][16][17][18][19] [20,21]. While the mechanism of such toxicity remains unclear, preventing aggregation and/or enhancing clearance of cytoplasmic TDP-43 and FUS is of considerable therapeutic interest. This approach has shown promise in various ALS models where preventing SG assembly or upregulating cytoplasmic protein turnover has been tested [22][23][24][25][26].Recently, we and others demonstrated that under normal growth conditions, TDP-43 toxicity, aggregation and prote...

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TDP-43 and RNA form amyloid-like myo-granules in regenerating muscle

Cited by 181 publications

References 46 publications

Pleiotropic requirements for human TDP-43 in the regulation of cell and organelle homeostasis

Pleiotropic requirements for human TDP-43 in the regulation of cell and organelle homeostasis

Shared regulatory pathways reveal novel genetic correlations between grip strength and neuromuscular disorders

Cdc48/VCP and endocytosis regulate TDP-43 and FUS toxicity and turnover

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