Project description:Lysosomal storage diseases (LSDs) comprised ~50 gene loci causing the accumulation of cellular material in the lysosome and associated defects in lysosomal function, but systematic molecular phenotyping is lacking. Here, we apply a nanoflow-based multi-omic single-shot technology (nMOST) workflow to simultaneously quantify HeLa cell proteomes and lipidomes from dozens of LSD mutants, revealing diverse molecular phenotypes. Defects in delivery of ferritin and its autophagic regulator NCOA4 to lysosomes (ferritinophagy) were pronounced in NPC2-/- cells, which correlated with increased lyso-phosphatidyl-choline species and dramatic multi-lamellar membrane structures visualized by cryo-electron tomography. Ferritinophagy defects correlated with loss of mitochondrial cristae, MICOS complex components, and electron transport chain complexes rich in iron-sulfur cluster proteins. Strikingly, these defects were rescued when iron was provided through the transferrin system. This resource reveals how loss of lysosomal function impacts organelle homeostasis in trans and highlights nMOST profiling as a discovery tool for illuminating distinct molecular phenotypes across LSDs.

Project description:This experiment describes the quantitative proteomic profiling of whole-cell, soma, and neuronal projection fractions from day 35 induced neurons (iN) derived from control and ASAH1 knockout human embryonic stem cells. Soma and projection compartments were physically separated using Transwell culture inserts, and triplicate biological replicates were processed using TMTpro 18-plex labeling and high-resolution Orbitrap mass spectrometry with FAIMS. Data were searched against the human proteome with stringent FDR control and reporter ion quantification, enabling compartment-resolved analysis of proteome alterations associated with ASAH1 deficiency.

Project description:Mitochondria are platforms for important processes including mitochondrial fusion and fission, protein and lipid transport, cytoskeletal trafficking, and the activation of mitophagy, apoptosis, and innate immune responses. How cells regulate the assembly of protein complexes at the mitochondrial surface to control these dynamic functions is incompletely understood. Here, we show that ARMC1 shuttles between the cytosol and distinct mitochondrial complexes. The assembly of ARMC1 with Miro, MTFR, and TMEM11 links together mitochondrial trafficking and shaping activities and is essential for MTFR stability. In another complex, ARMC1 engages, via MTCH2, DNAJC11, which facilitates ARMC1 recycling back into the cytosol. Disrupting the balance of ARMC1 between these complexes leads to aberrant cellular mitochondrial distributions. Thus, the stability and function of the Miro-MTFR complex is regulated by ARMC1, whose mito-cytoplasmic shuttling via DNAJC11 tunes mitochondrial dynamics. Our findings provide a paradigm for protein complex regulation through the spatial control of a linchpin subunit.

Project description:Mitochondria are platforms for important processes including mitochondrial fusion and fission, protein and lipid transport, cytoskeletal trafficking, and the activation of mitophagy, apoptosis, and innate immune responses. How cells regulate the assembly of protein complexes at the mitochondrial surface to control these dynamic functions is incompletely understood. Here, we show that ARMC1 shuttles between the cytosol and distinct mitochondrial complexes. The assembly of ARMC1 with Miro, MTFR, and TMEM11 links together mitochondrial trafficking and shaping activities and is essential for MTFR stability. In another complex, ARMC1 engages, via MTCH2, DNAJC11, which facilitates ARMC1 recycling back into the cytosol. Disrupting the balance of ARMC1 between these complexes leads to aberrant cellular mitochondrial distributions. Thus, the stability and function of the Miro-MTFR complex is regulated by ARMC1, whose mito-cytoplasmic shuttling via DNAJC11 tunes mitochondrial dynamics. Our findings provide a paradigm for protein complex regulation through the spatial control of a linchpin subunit.

Project description:This quantitative proteomic analysis of lysosome-enriched fractions isolated by immunoprecipitation (LysoIP) from HeLa cells expressing TMEM192-3xHA, untagged controls, and ASAH1 knockout lines. Triplicate biological replicates were processed using TMTpro 18-plex labeling and high-resolution Orbitrap mass spectrometry with FAIMS. Data were searched against the human proteome with stringent FDR filtering and reporter ion quantification, enabling comparative profiling of lysosomal protein composition and changes associated with ASAH1 deficiency.

Project description:Here, we mapped subcellular proteome changes to lysosomes, mitochondrion, EEA1-positive endosomes, and Golgi caused by the NLRP3 inflammasome agonists nigericin and CL097. We identified a number of common disruptions to retrograde trafficking pathways, including COPI and Shiga toxin-related transport, in line with recent studies. We further characterized mouse NLRP3 trafficking throughout its activation using temporal proximity proteomics, which supports a recent model of NLRP3 recruitment to endosomes during inflammasome activation. Collectively, these findings provide additional granularity to our understanding of the molecular events driving NLRP3 activation and serve as a valuable resource for cell biological research.

Project description:During nutrient stress, macroautophagy is employed to degrade cellular macromolecules, thereby providing biosynthetic building blocks while simultaneously remodeling the proteome. While the machinery responsible for initiation of macroautophagy is well characterized, our understanding of the extent to which individual proteins, protein complexes and organelles are selected for autophagic degradation, and the underlying targeting mechanisms is limited. Here, we use orthogonal proteomic strategies to provide a global molecular inventory of autophagic cargo during nutrient stress in mammalian cell lines. Through prioritization of autophagic cargo, we identify a heterodimeric pair of membrane-embedded proteins, YIPF3 and YIPF4, as receptors for Golgiphagy. During nutrient stress, YIPF4 is mobilized into ATG8-positive vesicles that traffic to lysosomes as measured via Golgiphagy flux reporters in a process that requires the VPS34 and ULK1-FIP200 arms of the autophagy system. Cells lacking YIPF3 or YIPF4 are selectively defective in elimination of Golgi membrane proteins during nutrient stress. By merging absolute protein abundance with autophagic turnover, we create a global protein census describing how autophagic degradation maps onto protein abundance and subcellular localization. Our results, available via an interactive web tool, reveal that autophagic turnover prioritizes membrane-bound organelles (principally Golgi and ER) for proteome remodeling during nutrient stress.

Project description:Localised translation broadly enables spatiotemporal control of gene expression yet currently there are limited tools for monitoring subcellular translation in mammalian cells. Here we present LOCL-TL (LOV-domain Controlled Ligase for Translation Localisation) an optogenetic approach for labelling ribosomes at any defined subcellular location and quantitatively determining their translation with codon precision through ribosome profiling. Application of LOCL-TL to mitochondrially localised translation revealed that ~20% of human nuclear-encoded mitochondrial genes are robustly translated on the outer mitochondrial membrane (OMM). Mitochondrially-translated messages form two classes distinguished by the length of proteins they encode, and the mechanism, and function of their recruitment. An evolutionarily ancient mechanism allows nascent chains to drive the cotranslational recruitment of long proteins via a bipartite targeting signal, which acts on mostly mitochondrial matrix proteins of bacterial origin. Conversely, mRNAs of short proteins, especially eukaryotic origin electron transport chain (ETC) components, are directly recruited to the OMM, in a manner that depends on the 3’UTR, mRNA splicing and the OMM protein A-Kinase Anchoring Protein 1 (AKAP1) and disruption of localised translation through the loss of AKAP1 lowers ETC production. Our studies thus reveal a hierarchical strategy used to enable preferential translation of a subset of proteins on the OMM.

Project description:Inguinal white adipose tissue (iWAT) is essential for the beneficial effects of exercise training on metabolic health. The underlying mechanisms for these effects are not fully understood and here, we test the hypothesis that exercise training results in a more favorable iWAT structural phenotype. Using biochemical, imaging, and multi-omics analyses we find that 11-days of wheel running in male mice causes profound iWAT remodeling including decreased extracellular matrix (ECM) deposition, increased vascularization and innervation. We identify adipose stem cells as one of the main contributors to training-induced ECM remodeling, show that the PRDM16 transcriptional complex is necessary for iWAT remodeling and beiging, and discover neuronal growth regulator 1 (NEGR1) as a link between PRDM16 and neuritogenesis. Moreover, we find that training causes a shift from hypertrophic to insulin-sensitive adipocyte subpopulations. Exercise training leads to remarkable adaptations to iWAT structure and cell-type composition that can confer beneficial changes in tissue metabolism.

Project description:During nutrient stress, macroautophagy is employed to degrade cellular macromolecules, thereby providing biosynthetic building blocks while simultaneously remodeling the proteome. While the machinery responsible for initiation of macroautophagy is well characterized, our understanding of the extent to which individual proteins, protein complexes and organelles are selected for autophagic degradation, and the underlying targeting mechanisms is limited. Here, we use orthogonal proteomic strategies to provide a global molecular inventory of autophagic cargo during nutrient stress in mammalian cell lines. Through prioritization of autophagic cargo, we identify a heterodimeric pair of membrane-embedded proteins, YIPF3 and YIPF4, as receptors for Golgiphagy. During nutrient stress, YIPF4 is mobilized into ATG8-positive vesicles that traffic to lysosomes as measured via Golgiphagy flux reporters in a process that requires the VPS34 and ULK1-FIP200 arms of the autophagy system. Cells lacking YIPF3 or YIPF4 are selectively defective in elimination of Golgi membrane proteins during nutrient stress. By merging absolute protein abundance with autophagic turnover, we create a global protein census describing how autophagic degradation maps onto protein abundance and subcellular localization. Our results, available via an interactive web tool, reveal that autophagic turnover prioritizes membrane-bound organelles (principally Golgi and ER) for proteome remodeling during nutrient stress.