ALS-linked cytoplasmic FUS assemblies are compositionally different from physiological stress granules and sequester hnRNPA3, a novel modifier of FUS toxicity

Haiyan An; Gioana Litscher; Naruaki Watanabe; Wenbin Wei; Tadafumi Hashimoto; Takeshi Iwatsubo; Vladimir L Buchman; Tatyana A Shelkovnikova

doi:10.1016/j.nbd.2021.105585

ALS-linked cytoplasmic FUS assemblies are compositionally different from physiological stress granules and sequester hnRNPA3, a novel modifier of FUS toxicity

Neurobiol Dis. 2022 Jan:162:105585. doi: 10.1016/j.nbd.2021.105585. Epub 2021 Dec 14.

Authors

Haiyan An¹, Gioana Litscher¹, Naruaki Watanabe², Wenbin Wei³, Tadafumi Hashimoto², Takeshi Iwatsubo², Vladimir L Buchman⁴, Tatyana A Shelkovnikova⁵

Affiliations

¹ Medicines Discovery Institute, Cardiff University, Cardiff CF10 3AT, United Kingdom.
² Department of Neuropathology, University of Tokyo, Tokyo, Japan.
³ Department of Biosciences, Durham University, Durham DH1 3LE, United Kingdom.
⁴ School of Biosciences, Cardiff University, Cardiff CF10 3AX, United Kingdom; Belgorod State National Research University, Belgorod 308015, Russian Federation.
⁵ Medicines Discovery Institute, Cardiff University, Cardiff CF10 3AT, United Kingdom. Electronic address: t.shelkovnikova@sheffield.ac.uk.

Abstract

Formation of cytoplasmic RNA-protein structures called stress granules (SGs) is a highly conserved cellular response to stress. Abnormal metabolism of SGs may contribute to the pathogenesis of (neuro)degenerative diseases such as amyotrophic lateral sclerosis (ALS). Many SG proteins are affected by mutations causative of these conditions, including fused in sarcoma (FUS). Mutant FUS variants have high affinity to SGs and also spontaneously form de novo cytoplasmic RNA granules. Mutant FUS-containing assemblies (mFAs), often called "pathological SGs", are proposed to play a role in ALS-FUS pathogenesis. However, structural differences between mFAs and physiological SGs remain largely unknown therefore it is unclear whether mFAs can functionally substitute for SGs and how they affect cellular stress responses. Here we used affinity purification to isolate mFAs and physiological SGs and compare their protein composition. We found that proteins within mFAs form significantly more physical interactions than those in SGs however mFAs fail to recruit many factors involved in signal transduction. Furthermore, we found that proteasome subunits and certain nucleocytoplasmic transport factors are depleted from mFAs, whereas translation elongation, mRNA surveillance and splicing factors as well as mitochondrial proteins are enriched in mFAs, as compared to SGs. Validation experiments for a mFA-specific protein, hnRNPA3, confirmed its RNA-dependent interaction with FUS and its sequestration into FUS inclusions in cultured cells and in a FUS transgenic mouse model. Silencing of the Drosophila hnRNPA3 ortholog was deleterious and potentiated human FUS toxicity in the retina of transgenic flies. In conclusion, we show that SG-like structures formed by mutant FUS are structurally distinct from SGs, prone to persistence, likely cannot functionally replace SGs, and affect a spectrum of cellular pathways in stressed cells. Results of our study support a pathogenic role for cytoplasmic FUS assemblies in ALS-FUS.

Keywords: ALS; FUS; FUS aggregate; Proteomics; RNP granule; SG core; Stress granule; hnRNPA3.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Amyotrophic Lateral Sclerosis* / metabolism
Animals
Cytoplasm / metabolism
Inclusion Bodies / metabolism
Mice
Mutation
RNA-Binding Protein FUS / genetics
RNA-Binding Protein FUS / metabolism
Stress Granules
Stress, Physiological

Substances

RNA-Binding Protein FUS