Engineering enhanced protein disaggregases for neurodegenerative disease

Jackrel, Meredith E.; Shorter, James

doi:10.1080/19336896.2015.1020277

Cited by 72 publications

(107 citation statements)

References 183 publications

(315 reference statements)

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“…6, A, C, and E). Previously, we had established that an important property of potentiated Hsp104 variants bearing mutations in the MD was increased disaggregase activity against disordered aggregates in the absence of Hsp70 and Hsp40 (62,63,(65)(66)(67). However, our findings with Hsp104 N728A (Figs.…”

Section: A503vcontrasting

confidence: 56%

“…By contrast, Hsp104 A503V strongly suppressed ␣-syn toxicity (Fig. 3A) (35,62,63,66). This rescue was severely impaired by the Y257A mutation and ablated by the Y662A or Y257A/Y662A mutations (Fig.…”

Section: A503vmentioning

confidence: 99%

“…Hsp104 has limited disaggregase activity against TDP-43 and FUS fibrils (62,63). Recently, we have engineered potentiated Hsp104 variants that mitigate TDP-43, FUS, and ␣-syn misfolding (62)(63)(64)(65)(66)(67). Missense mutations at disparate but specific positions in the MD or the small domain of NBD1 (immediately C-terminal to the MD) resulted in potentiated Hsp104 variants (62,67).…”

mentioning

confidence: 99%

“…Interestingly, two potentiated Hsp104 variants, Hsp104 A503S and Hsp104 Y257F/A503V/Y662F , rescue neurodegeneration in the metazoan nervous system and hold promise as possible treatments for neurodegenerative disease (62,66).…”

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confidence: 99%

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Mechanistic Insights into Hsp104 Potentiation

Torrente¹,

Chuang

Noll³

et al. 2016

Journal of Biological Chemistry

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Potentiated variants of Hsp104, a protein disaggregase from yeast, can dissolve protein aggregates connected to neurodegenerative diseases such as Parkinson disease and amyotrophic lateral sclerosis. However, the mechanisms underlying Hsp104 potentiation remain incompletely defined. Here, we establish that 2-3 subunits of the Hsp104 hexamer must bear an A503V potentiating mutation to elicit enhanced disaggregase activity in the absence of Hsp70. We also define the ATPase and substratebinding modalities needed for potentiated Hsp104 A503V activity in vitro and in vivo. Hsp104 A503V disaggregase activity is strongly inhibited by the Y257A mutation that disrupts substrate binding to the nucleotide-binding domain 1 (NBD1) pore loop and is abolished by the Y662A mutation that disrupts substrate binding to the NBD2 pore loop. A503V displays a more robust activity that is unperturbed by sensor-1 mutations that greatly reduce Hsp104 activity in vivo. Indeed, ATPase activity at NBD1 or NBD2 is sufficient for Hsp104 potentiation. Our findings will empower design of ameliorated therapeutic disaggregases for various neurodegenerative diseases.Protein misfolding and aggregation are associated with a wide variety of diseases, ranging from type II diabetes (1, 2) to neurodegenerative diseases, such as fatal familial insomnia (3, 4), Parkinson disease, and amyotrophic lateral sclerosis (ALS) (5-7). In Parkinson disease patients, ␣-synuclein (␣-syn) 6 forms toxic soluble oligomers as well as amyloid structures that accumulate in Lewy bodies and contribute to the death of dopaminergic neurons (8 -12). Similarly, toxic soluble oligomers and cytoplasmic inclusions of TDP-43 or FUS are associated with ALS and frontotemporal dementia (13-20). These misfolded protein conformers are recalcitrant and represent a colossal roadblock in the treatment of these diseases.Hsp104 is a 102-kDa AAAϩ ATPase (21) from Saccharomyces cerevisiae capable of dissolving disordered protein aggregates as well as dismantling amyloid fibrils and toxic soluble oligomers (22-33). It assembles into a homohexameric barrel structure with a central channel (34 -39). Hsp104 processes protein aggregates by directly translocating substrates either partially or completely through this channel (35, 36, 40 -46). Hsp104 encompasses an N-terminal domain, two nucleotidebinding domains (NBD1 and NBD2), a coiled-coil middle domain (MD), and a C-terminal domain important for oligomerization (Fig. 1A) (47). Both NBDs contain Walker A and Walker B motifs that are critical for nucleotide binding and hydrolysis, respectively (48). ATP hydrolysis takes place primarily at NBD1, whereas NBD2 has a nucleotide-dependent oligomerization function (29, 34, 49 -52).Remarkably, Hsp104 can remodel amyloid substrates alone, without the aid of any other chaperones (22,24,26,31,33,45,(53)(54)(55)(56). However, to disaggregate amorphous protein aggregates, Hsp104 usually needs to collaborate with the Hsp110, Hsp70, and Hsp40 chaperone system (23,26,30,32,57). Moreover, small heat shock proteins...

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Section: A503vcontrasting

confidence: 56%

Section: A503vmentioning

confidence: 99%

mentioning

confidence: 99%

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confidence: 99%

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Mechanistic Insights into Hsp104 Potentiation

Torrente¹,

Chuang

Noll³

et al. 2016

Journal of Biological Chemistry

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“…However, it is unclear how the cell limits the aggregation propensity of these domains and if therapies targeting these domains could be developed. Efforts to enhance the ability of cells to disassemble inclusions using disaggregase chaperones show promise (Jackrel & Shorter, 2015; March et al , 2016). We thought post‐translational modifications would be an alternative and potentially more pharmacologically tractable strategy to disrupt assembly directly at its source.…”

Section: Discussionmentioning

confidence: 99%

Phosphorylation of the FUS low‐complexity domain disrupts phase separation, aggregation, and toxicity

et al. 2017

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Neuronal inclusions of aggregated RNA‐binding protein fused in sarcoma (FUS) are hallmarks of ALS and frontotemporal dementia subtypes. Intriguingly, FUS's nearly uncharged, aggregation‐prone, yeast prion‐like, low sequence‐complexity domain (LC) is known to be targeted for phosphorylation. Here we map in vitro and in‐cell phosphorylation sites across FUS LC. We show that both phosphorylation and phosphomimetic variants reduce its aggregation‐prone/prion‐like character, disrupting FUS phase separation in the presence of RNA or salt and reducing FUS propensity to aggregate. Nuclear magnetic resonance spectroscopy demonstrates the intrinsically disordered structure of FUS LC is preserved after phosphorylation; however, transient domain collapse and self‐interaction are reduced by phosphomimetics. Moreover, we show that phosphomimetic FUS reduces aggregation in human and yeast cell models, and can ameliorate FUS‐associated cytotoxicity. Hence, post‐translational modification may be a mechanism by which cells control physiological assembly and prevent pathological protein aggregation, suggesting a potential treatment pathway amenable to pharmacologic modulation.

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