Tyrosine phosphorylation regulates hnRNPA2 granule protein partitioning &amp; reduces neurodegeneration

Ryan, Veronica H.; Perdikari, Theodora Myrto; Naik, Mandar T.; Saueressig, Camillo; Lins, Jeremy; Dignon, Gregory L.; Mittal, Jeetain; Hart, Anne C.; Fawzi, Nicolas L.

doi:10.1101/2020.03.15.992768

Cited by 9 publications

(19 citation statements)

References 74 publications

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“…Indeed, while both D290V and P298L formed aggregates over time, the addition of RNA prevented formation of both liquid droplets and solid aggregates at these conditions (Figure 4B , C). This prevention of aggregation was even greater than that exerted by partial tyrosine phosphorylation ( 33 ), as here neither D290V nor P298L showed any droplets in the presence of RNA.…”

Section: Resultsmentioning

confidence: 56%

“…the LLPS assay is performed at concentrations below the dissociation constant), a majority of the RNA is not predicted to bind two copies of the protein simultaneously, perhaps contributing to the lack of stimulation of LLPS by addition of rA2RE21. Here, we performed all LLPS assays at 15 μM hnRNPA2 FL as hnRNPA2 FL undergoes robust LLPS at that concentration ( 10 , 33 ). Despite the fact that at these concentrations (given the binding affinities we found for rA2RE11 and rA2RE21) only a fraction of hnRNPA2 RRMs would be expected to bind RNA, we do see a profound disruption of LLPS by addition of RNA on LLPS.…”

Section: Resultsmentioning

confidence: 99%

“…In contrast to previous reports ( 5 ), we find that both the 11mer and 21mer RNA oligomers bind to hnRNPA2 1–189 weakly (Figure 5 ), with a binding affinity on the order of tens of micromolar. Given that we have recently shown hnRNPA2 is highly prone to phase separate and aggregate and requires careful use of solubility tags and RNA removal to prevent pre-aggregation ( 10 , 22 , 30 , 33 ), it is possible that self-interactions between full-length hnRNPA2 molecules (e.g. pre-formed aggregates) and protein-surface interactions complicated previous bio-sensor measurements performed with full-length recombinant protein.…”

Section: Discussionmentioning

confidence: 99%

“…The impact of physiological arginine methylation, which alters hnRNPA2 LC self-interaction and LLPS ( 10 ), on hnRNPA2 LC interactions with RNA will be important to study in the future. Though our focus here is on the RNA-binding properties of the hnRNPA2 RRMs to the A2RE, it is possible that the in vitro LLPS experiments may not represent the effect of RNA on hnRNPA2 phase separation in cells where other protein and RNA interactions may cooperate with the A2RE interaction with hnRNPA2 RRMs to stabilize a granule ( 33 ).…”

Section: Discussionmentioning

confidence: 99%

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Weak binding to the A2RE RNA rigidifies hnRNPA2 RRMs and reduces liquid–liquid phase separation and aggregation

Ryan

Watters

Amaya

et al. 2020

Nucleic Acids Research

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hnRNPA2 is a major component of mRNA transport granules in oligodendrocytes and neurons. However, the structural details of how hnRNPA2 binds the A2 recognition element (A2RE) and if this sequence stimulates granule formation by enhancing phase separation of hnRNPA2 has not yet been studied. Using solution NMR and biophysical studies, we find that each of the two individual RRMs retain the domain structure observed in complex with RNA but are not rigidly confined (i.e. they move independently) in solution in the absence of RNA. hnRNPA2 RRMs bind the minimal rA2RE11 weakly but at least, and most likely, two hnRNPA2 molecules are able to simultaneously bind the longer 21mer myelin basic protein A2RE. Upon binding of the RNA, NMR chemical shift deviations are observed in both RRMs, suggesting both play a role in binding the A2RE11. Interestingly, addition of short A2RE RNAs or longer RNAs containing this sequence completely prevents in vitro phase separation of full-length hnRNPA2 and aggregation of the disease-associated mutants. These findings suggest that RRM interactions with specific recognition sequences alone do not account for nucleating granule formation, consistent with models where multivalent protein:RNA and protein:protein contacts form across many sites in granule proteins and long RNA transcripts.

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Section: Resultsmentioning

confidence: 56%

Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

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Weak binding to the A2RE RNA rigidifies hnRNPA2 RRMs and reduces liquid–liquid phase separation and aggregation

Ryan

Watters

Amaya

et al. 2020

Nucleic Acids Research

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“…Therefore, computational studies can be an effective approach to screen a large number of PTM patterns and predict their role on regulating the molecular properties and phase separation of proteins (30,31). All-atom explicit solvent simulations readily incorporate posttranslationally modified amino acids (32)(33)(34)(35)(36) and have been used to probe the contacts leading to phase separation (37,38). However, the ability of atomistic force-fields to accurately capture the properties of IDRs depends strongly on parameterization (39,40).…”

Section: Introductionmentioning

confidence: 99%

A predictive coarse-grained model for position-specific effects of post-translational modifications on disordered protein phase separation

Perdikari

Jovic

Dignon

et al. 2020

Preprint

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Biomolecules undergo liquid-liquid phase separation (LLPS) resulting in the formation of multicomponent protein-RNA membraneless organelles in cells. However, the physiological and pathological role of post translational modifications (PTMs) on the biophysics of phase behavior is only beginning to be probed. To study the effect of PTMs on LLPS in silico, we extend our transferable coarse-grained model of intrinsically disordered proteins to include phosphorylated and acetylated amino acids. Using the parameters for modified amino acids available for fixed charge atomistic forcefields, we parameterize the size and atomistic hydropathy of the coarse-grained modified amino acid beads, and hence the interactions between the modified and natural amino acids. We then elucidate how the number and position of phosphorylated and acetylated residues alter the protein's single chain compactness and its propensity to phase separate. We show that both the number and the position of phosphorylated threonines/serines or acetylated lysines can serve as a molecular on/off switch for phase separation in the well-studied disordered regions of FUS and DDX3X, respectively. We also compare modified residues to their commonly used PTM mimics for their impact on chain properties. Importantly, we show that the model can predict and capture experimentally measured differences in the phase behavior for positionspecific modifications, showing that the position of modifications can dictate phase separation. In sum, this model will be useful for studying LLPS of post-translationally modified intrinsically disordered proteins and predicting how modifications control phase behavior with position-specific resolution. Statement of SignificancePost-translational modifications are important regulators of liquid-liquid phase separation (LLPS) which drives the formation of biomolecular condensates. Theoretical methods can be used to characterize the biophysical properties of intrinsically disordered proteins (IDPs). Our recent framework for molecular simulations using a Cαcentered coarse-grained model can predict the effect of various perturbations such as mutations (Dignon et al. PloS Comput. Biol, 2018) and temperature (Dignon et al, ACS Cent. Sci., 2019) on LLPS. Here, we expand this framework to incorporate modified residues like phosphothreonine, phosphoserine and acetylysine. This model will prove useful for simulating the phase separation of post-translationally modified IDPs and predicting how position-specific modifications can control phase behavior across the large family of proteins known to be phosphorylated and acetylated.

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Ubiquitin‐Modulated Phase Separation of Shuttle Proteins: Does Condensate Formation Promote Protein Degradation?

Dao

Castañeda

2020

BioEssays

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Liquid-liquid phase separation (LLPS) has recently emerged as a possible mechanism that enables ubiquitin-binding shuttle proteins to facilitate the degradation of ubiquitinated substrates via distinct protein quality control (PQC) pathways. Shuttle protein LLPS is modulated by multivalent interactions among their various domains as well as heterotypic interactions with polyubiquitin chains. Here, the properties of three different shuttle proteins (hHR23B, p62, and UBQLN2) are closely examined, unifying principles for the molecular determinants of their LLPS are identified, and how LLPS is connected to their functions is discussed. Evidence supporting LLPS of other shuttle proteins is also found. In this review, it is proposed that shuttle protein LLPS leads to spatiotemporal regulation of PQC activities by mediating the recruitment of PQC machinery (including proteasomes or autophagic components) to biomolecular condensates, assembly/disassembly of condensates, selective enrichment of client proteins, and extraction of ubiquitinated proteins from condensates in cells.

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Tyrosine phosphorylation regulates hnRNPA2 granule protein partitioning & reduces neurodegeneration

Cited by 9 publications

References 74 publications

Weak binding to the A2RE RNA rigidifies hnRNPA2 RRMs and reduces liquid–liquid phase separation and aggregation

Weak binding to the A2RE RNA rigidifies hnRNPA2 RRMs and reduces liquid–liquid phase separation and aggregation

A predictive coarse-grained model for position-specific effects of post-translational modifications on disordered protein phase separation

Ubiquitin‐Modulated Phase Separation of Shuttle Proteins: Does Condensate Formation Promote Protein Degradation?

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