Anatomy and Neuroscience - Research Publications

Permanent URI for this collection

http://hdl.handle.net/11343/181

Filters

2018 - 2019 4 2020 - 2024 26
30
Reset filters

Settings
Statistics
Citations
Start date: 2018 × Author: Parker, Benjamin ×

Search Results

Now showing 1 - 10 of 30
  • Item
    Thumbnail Image
    Liver-derived extracellular vesicles improve whole-body glycaemic control via inter-organ communication
    Miotto, PM ; Yang, C-H ; Keenan, SN ; De Nardo, W ; Beddows, CA ; Fidelito, G ; Dodd, GT ; Parker, BL ; Hill, AF ; Burton, PR ; Loh, K ; Watt, MJ (NATURE PORTFOLIO, 2024-02)
    Small extracellular vesicles (EVs) are signalling messengers that regulate inter-tissue communication through delivery of their molecular cargo. Here, we show that liver-derived EVs are acute regulators of whole-body glycaemic control in mice. Liver EV secretion into the circulation is increased in response to hyperglycaemia, resulting in increased glucose effectiveness and insulin secretion through direct inter-organ EV signalling to skeletal muscle and the pancreas, respectively. This acute blood glucose lowering effect occurs in healthy and obese mice with non-alcoholic fatty liver disease, despite marked remodelling of the liver-derived EV proteome in obese mice. The EV-mediated blood glucose lowering effects were recapitulated by administration of liver EVs derived from humans with or without progressive non-alcoholic fatty liver disease, suggesting broad functional conservation of liver EV signalling and potential therapeutic utility. Taken together, this work reveals a mechanism whereby liver EVs act on peripheral tissues via endocrine signalling to restore euglycaemia in the postprandial state.
  • Item
    No Preview Available
    Alpha kinase 3 signaling at the M-band maintains sarcomere integrity and proteostasis in striated muscle
    McNamara, JW ; Parker, BL ; Voges, HK ; Mehdiabadi, NR ; Bolk, F ; Ahmad, F ; Chung, JD ; Charitakis, N ; Molendijk, J ; Zech, ATL ; Lal, S ; Ramialison, M ; Karavendzas, K ; Pointer, HL ; Syrris, P ; Lopes, LR ; Elliott, PM ; Lynch, GS ; Mills, RJ ; Hudson, JE ; Watt, KI ; Porrello, ER ; Elliott, DA (SPRINGERNATURE, 2023-02)
    Abstract Muscle contraction is driven by the molecular machinery of the sarcomere. As phosphorylation is a critical regulator of muscle function, the identification of regulatory kinases is important for understanding sarcomere biology. Pathogenic variants in alpha kinase 3 (ALPK3) cause cardiomyopathy and musculoskeletal disease, but little is known about this atypical kinase. Here we show that ALPK3 is an essential component of the M-band of the sarcomere and define the ALPK3-dependent phosphoproteome. ALPK3 deficiency impaired contractility both in human cardiac organoids and in the hearts of mice harboring a pathogenic truncating Alpk3 variant. ALPK3-dependent phosphopeptides were enriched for sarcomeric components of the M-band and the ubiquitin-binding protein sequestosome-1 (SQSTM1) (also known as p62). Analysis of the ALPK3 interactome confirmed binding to M-band proteins including SQSTM1. In human pluripotent stem cell-derived cardiomyocytes modeling cardiomyopathic ALPK3 mutations, sarcomeric organization and M-band localization of SQSTM1 were abnormal suggesting that this mechanism may underly disease pathogenesis.
  • Item
    No Preview Available
    Impact of Bmal1 Rescue and Time-Restricted Feeding on Liver and Muscle Proteomes During the Active Phase in Mice
    Smith, JG ; Molendijk, J ; Blazev, R ; Chen, WH ; Zhang, Q ; Litwin, C ; Zinna, VM ; Welz, P-S ; Benitah, SA ; Greco, CM ; Sassone-Corsi, P ; Munoz-Canoves, P ; Parker, BL ; Koronowski, KB (ELSEVIER, 2023-11)
    Molecular clocks and daily feeding cycles support metabolism in peripheral tissues. Although the roles of local clocks and feeding are well defined at the transcriptional level, their impact on governing protein abundance in peripheral tissues is unclear. Here, we determine the relative contributions of local molecular clocks and daily feeding cycles on liver and muscle proteomes during the active phase in mice. LC-MS/MS was performed on liver and gastrocnemius muscle harvested 4 h into the dark phase from WT, Bmal1 KO, and dual liver- and muscle-Bmal1-rescued mice under either ad libitum feeding or time-restricted feeding during the dark phase. Feeding-fasting cycles had only minimal effects on levels of liver proteins and few, if any, on the muscle proteome. In contrast, Bmal1 KO altered the abundance of 674 proteins in liver and 80 proteins in muscle. Local rescue of liver and muscle Bmal1 restored ∼50% of proteins in liver and ∼25% in muscle. These included proteins involved in fatty acid oxidation in liver and carbohydrate metabolism in muscle. For liver, proteins involved in de novo lipogenesis were largely dependent on Bmal1 function in other tissues (i.e., the wider clock system). Proteins regulated by BMAL1 in liver and muscle were enriched for secreted proteins. We found that the abundance of fibroblast growth factor 1, a liver secreted protein, requires BMAL1 and that autocrine fibroblast growth factor 1 signaling modulates mitochondrial respiration in hepatocytes. In liver and muscle, BMAL1 is a more potent regulator of dark phase proteomes than daily feeding cycles, highlighting the need to assess protein levels in addition to mRNA when investigating clock mechanisms. The proteome is more extensively regulated by BMAL1 in liver than in muscle, and many metabolic pathways in peripheral tissues are reliant on the function of the clock system as a whole.
  • Item
    No Preview Available
    Glycoproteomics
    Bagdonaite, I ; Malaker, SA ; Polasky, DA ; Riley, NM ; Schjoldager, K ; Vakhrushev, SY ; Halim, A ; Aoki-Kinoshita, KF ; Nesvizhskii, AI ; Bertozzi, CR ; Wandall, HH ; Parker, BL ; Thaysen-Andersen, M ; Scott, NE (SPRINGERNATURE, 2022-06-23)
  • Item
    No Preview Available
    urPTMdb/TeaProt: Upstream and Downstream Proteomics Analysis
    Molendijk, J ; Yip, R ; Parker, BL (AMER CHEMICAL SOC, 2023-02-03)
    We have developed the underrepresented post-translational modification (PTM) database (urPTMdb), a PTM gene set database to accelerate the discovery of enriched protein modifications in experimental data. urPTMdb provides curated lists of proteins reported to be substrates of underrepresented modifications. Their enrichment in proteomics datasets can reveal unexpected PTM regulations. urPTMdb can be implemented in existing workflows, or used in TeaProt, an online Shiny tool that integrates upstream transcription factor enrichment analysis with downstream pathway analysis through an easy-to-use interactive interface. TeaProt annotates user-uploaded data with drug-gene interactions, subcellular localizations, phenotypic functions, gene-disease associations, and enzyme-gene interactions. TeaProt enables gene set enrichment analysis (GSEA) to discover enrichments in gene sets from various resources, including MSigDB, CHEA, and urPTMdb. We demonstrate the utility of urPTMdb and TeaProt through the analysis of a previously published Western diet-induced remodeling of the tongue proteome, which revealed altered cellular processes associated with energy metabolism, interferon alpha/gamma response, adipogenesis, HMGylation substrate enrichment, and transcription regulation through PPARG and CEBPA. Additionally, we analyzed the interactome of ADP-ribose glycohydrolase TARG1, a key enzyme that removes mono-ADP-ribosylation. This analysis identified an enrichment of ADP-ribosylation, ribosomal proteins, and proteins localized in the nucleoli and endoplasmic reticulum. TeaProt and urPTMdb are accessible at https://tea.coffeeprot.com/.
  • Item
    No Preview Available
    Phosphoproteomics of three exercise modalities identifies canonical signaling and C18ORF25 as anAMPK substrate regulating skeletal muscle function
    Blazev, R ; Carl, CS ; Ng, Y-K ; Molendijk, J ; Voldstedlund, CT ; Zhao, Y ; Xiao, D ; Kueh, AJ ; Miotto, PM ; Haynes, VR ; Hardee, JP ; Chung, JD ; McNamara, JW ; Qian, H ; Gregorevic, P ; Oakhill, JS ; Herold, MJ ; Jensen, TE ; Lisowski, L ; Lynch, GS ; Dodd, GT ; Watt, MJ ; Yang, P ; Kiens, B ; Richter, EA ; Parker, BL (CELL PRESS, 2022-10-04)
    Exercise induces signaling networks to improve muscle function and confer health benefits. To identify divergent and common signaling networks during and after different exercise modalities, we performed a phosphoproteomic analysis of human skeletal muscle from a cross-over intervention of endurance, sprint, and resistance exercise. This identified 5,486 phosphosites regulated during or after at least one type of exercise modality and only 420 core phosphosites common to all exercise. One of these core phosphosites was S67 on the uncharacterized protein C18ORF25, which we validated as an AMPK substrate. Mice lacking C18ORF25 have reduced skeletal muscle fiber size, exercise capacity, and muscle contractile function, and this was associated with reduced phosphorylation of contractile and Ca2+ handling proteins. Expression of C18ORF25 S66/67D phospho-mimetic reversed the decreased muscle force production. This work defines the divergent and canonical exercise phosphoproteome across different modalities and identifies C18ORF25 as a regulator of exercise signaling and muscle function.
  • Item
    Thumbnail Image
    Proteome-wide systems genetics identifies UFMylation as a regulator of skeletal muscle function
    Molendijk, J ; Blazev, R ; Mills, RJ ; Ng, Y-K ; Watt, K ; Chau, D ; Gregorevic, P ; Crouch, PJ ; Hilton, JBW ; Lisowski, L ; Zhang, P ; Reue, K ; Lusis, AJ ; Hudson, JE ; James, DE ; Seldin, MM ; Parker, BL (eLIFE SCIENCES PUBL LTD, 2022-12-06)
    Improving muscle function has great potential to improve the quality of life. To identify novel regulators of skeletal muscle metabolism and function, we performed a proteomic analysis of gastrocnemius muscle from 73 genetically distinct inbred mouse strains, and integrated the data with previously acquired genomics and >300 molecular/phenotypic traits via quantitative trait loci mapping and correlation network analysis. These data identified thousands of associations between protein abundance and phenotypes and can be accessed online (https://muscle.coffeeprot.com/) to identify regulators of muscle function. We used this resource to prioritize targets for a functional genomic screen in human bioengineered skeletal muscle. This identified several negative regulators of muscle function including UFC1, an E2 ligase for protein UFMylation. We show UFMylation is up-regulated in a mouse model of amyotrophic lateral sclerosis, a disease that involves muscle atrophy. Furthermore, in vivo knockdown of UFMylation increased contraction force, implicating its role as a negative regulator of skeletal muscle function.
  • Item
    Thumbnail Image
    Temporal profiling of the breast tumour microenvironment reveals collagen XII as a driver of metastasis
    Papanicolaou, M ; Parker, AL ; Yam, M ; Filipe, EC ; Wu, SZ ; Chitty, JL ; Wyllie, K ; Tran, E ; Mok, E ; Nadalini, A ; Skhinas, JN ; Lucas, MC ; Herrmann, D ; Nobis, M ; Pereira, BA ; Law, AMK ; Castillo, L ; Murphy, KJ ; Zaratzian, A ; Hastings, JF ; Croucher, DR ; Lim, E ; Oliver, BG ; Mora, FV ; Parker, BL ; Gallego-Ortega, D ; Swarbrick, A ; O'Toole, S ; Timpson, P ; Cox, TR (NATURE PORTFOLIO, 2022-08-06)
    The tumour stroma, and in particular the extracellular matrix (ECM), is a salient feature of solid tumours that plays a crucial role in shaping their progression. Many desmoplastic tumours including breast cancer involve the significant accumulation of type I collagen. However, recently it has become clear that the precise distribution and organisation of matrix molecules such as collagen I is equally as important in the tumour as their abundance. Cancer-associated fibroblasts (CAFs) coexist within breast cancer tissues and play both pro- and anti-tumourigenic roles through remodelling the ECM. Here, using temporal proteomic profiling of decellularized tumours, we interrogate the evolving matrisome during breast cancer progression. We identify 4 key matrisomal clusters, and pinpoint collagen type XII as a critical component that regulates collagen type I organisation. Through combining our proteomics with single-cell transcriptomics, and genetic manipulation models, we show how CAF-secreted collagen XII alters collagen I organisation to create a pro-invasive microenvironment supporting metastatic dissemination. Finally, we show in patient cohorts that collagen XII may represent an indicator of breast cancer patients at high risk of metastatic relapse.
  • Item
    Thumbnail Image
    SILAC kinase screen identifies potential MASTL substrates
    Marzec, KA ; Rogers, S ; McCloy, R ; Parker, BL ; James, DE ; Watkins, DN ; Burgess, A (NATURE PORTFOLIO, 2022-06-22)
    Microtubule-associated serine/threonine kinase-like (MASTL) has emerged as a critical regulator of mitosis and as a potential oncogene in a variety of cancer types. To date, Arpp-19/ENSA are the only known substrates of MASTL. However, with the roles of MASTL expanding and increased interest in development of MASTL inhibitors, it has become critical to determine if there are additional substrates and what the optimal consensus motif for MASTL is. Here we utilized a whole cell lysate in vitro kinase screen combined with stable isotope labelling of amino acids in cell culture (SILAC) to identify potential substrates and the residue preference of MASTL. Using the related AGC kinase family members AKT1/2, the kinase screen identified several known and new substrates highly enriched for the validated consensus motif of AKT. Applying this method to MASTL identified 59 phospho-sites on 67 proteins that increased in the presence of active MASTL. Subsequent in vitro kinase assays suggested that MASTL may phosphorylate hnRNPM, YB1 and TUBA1C under certain in vitro conditions. Taken together, these data suggest that MASTL may phosphorylate several additional substrates, providing insight into the ever-increasing biological functions and roles MASTL plays in driving cancer progression and therapy resistance.
  • Item
    Thumbnail Image
    Trafficking regulator of GLUT4-1 (TRARG1) is a GSK3 substrate
    Duan, X ; Norris, DM ; Humphrey, SJ ; Yang, P ; Cooke, KC ; Bultitude, WP ; Parker, BL ; Conway, OJ ; Burchfield, JG ; Krycer, JR ; Brodsky, FM ; James, DE ; Fazakerley, DJ (PORTLAND PRESS LTD, 2022-06)
    Trafficking regulator of GLUT4-1, TRARG1, positively regulates insulin-stimulated GLUT4 trafficking and insulin sensitivity. However, the mechanism(s) by which this occurs remain(s) unclear. Using biochemical and mass spectrometry analyses we found that TRARG1 is dephosphorylated in response to insulin in a PI3K/Akt-dependent manner and is a novel substrate for GSK3. Priming phosphorylation of murine TRARG1 at serine 84 allows for GSK3-directed phosphorylation at serines 72, 76 and 80. A similar pattern of phosphorylation was observed in human TRARG1, suggesting that our findings are translatable to human TRARG1. Pharmacological inhibition of GSK3 increased cell surface GLUT4 in cells stimulated with a submaximal insulin dose, and this was impaired following Trarg1 knockdown, suggesting that TRARG1 acts as a GSK3-mediated regulator in GLUT4 trafficking. These data place TRARG1 within the insulin signaling network and provide insights into how GSK3 regulates GLUT4 trafficking in adipocytes.