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Dynamic Changes to the Skeletal Muscle Proteome and Ubiquitinome Induced by the E3 Ligase, ASB2β

https://doi.org/10.1016/j.mcpro.2021.100050Get rights and content
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Highlights

Proteomic and ubiquitinomic analysis of increased ASB2β in skeletal muscle

ASB2β increased the abundance of proteome and cytoskeletal proteins

ASB2β reduced the abundance of mitochondrial and contractile proteins

No simple relationship between changes in protein abundance and ubiquitination

Abstract

Ubiquitination is a posttranslational protein modification that has been shown to have a range of effects, including regulation of protein function, interaction, localization, and degradation. We have previously shown that the muscle-specific ubiquitin E3 ligase, ASB2β, is downregulated in models of muscle growth and that overexpression ASB2β is sufficient to induce muscle atrophy. To gain insight into the effects of increased ASB2β expression on skeletal muscle mass and function, we used liquid chromatography coupled to tandem mass spectrometry to investigate ASB2β-mediated changes to the skeletal muscle proteome and ubiquitinome, via a parallel analysis of remnant diGly-modified peptides. The results show that viral vector-mediated ASB2β overexpression in murine muscles causes progressive muscle atrophy and impairment of force-producing capacity, while ASB2β knockdown induces mild muscle hypertrophy. ASB2β-induced muscle atrophy and dysfunction were associated with the early downregulation of mitochondrial and contractile protein abundance and the upregulation of proteins involved in proteasome-mediated protein degradation (including other E3 ligases), protein synthesis, and the cytoskeleton/sarcomere. The overexpression ASB2β also resulted in marked changes in protein ubiquitination; however, there was no simple relationship between changes in ubiquitination status and protein abundance. To investigate proteins that interact with ASB2β and, therefore, potential ASB2β targets, Flag-tagged wild-type ASB2β, and a mutant ASB2β lacking the C-terminal SOCS box domain (dSOCS) were immunoprecipitated from C2C12 myotubes and subjected to label-free proteomic analysis to determine the ASB2β interactome. ASB2β was found to interact with a range of cytoskeletal and nuclear proteins. When combined with the in vivo ubiquitinomic data, our studies have identified novel putative ASB2β target substrates that warrant further investigation. These findings provide novel insight into the complexity of proteome and ubiquitinome changes that occur during E3 ligase-mediated skeletal muscle atrophy and dysfunction.

Keywords

skeletal muscle atrophy
protein degradation
muscle contraction
ubiquitination
proteasome
adeno-associated viral vectors
autophagy
mitochondria
filamin
titin

Abbreviations

2D nano-UHPL-MS/MS
two-dimensional nano-ultrahigh-performance mass spectrometry
CMV
cytomegalovirus
CSA
cross-sectional area
diGly
di-glycine
dSOCS
deleted C-terminal SOCS box domain
DUB
deubiquitinase
E-C
excitation-contraction
EDL
extensor digitorum longus
ETC
electron transport chain
GFP
green fluorescent protein
GO
gene ontology
HBSS
Hank’s buffered saline solution
MCS
multiple cloning site
mTORC1
mechanistic target of rapamycin complex 1
OMM
outer mitochondrial membrane
PVDF
polyvinylidene difluoride
rAAV
recombinant adeno-associated virus
ROS
reactive oxygen species
SOCS
suppressor of cytokine signaling
TA
tibialis anterior
TCA
tricarboxylic acid
TEAB
tetraethylammonium tetrahydroborate
TFA
trifluoroacetic acid
TMT
tandem mass tag
UIM
ubiquitin-interacting motif
UPS
ubiquitin proteasome system
WT
wild type

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Joint Primary Authors. These authors contributed equally to this work.