Abstract

Muscle mass, function, and tissue repair after injury decrease with aging in skeletal muscle. Autophagy appears to play a critical role, but what the effects might be are still controversial. Confounding factors are the multiple types of cells present in the muscle (e.g. muscle fibers, satellite cells, macrophages), which may have different autophagy requirements, and how the autophagy machinery targets specific organelle types (e.g. mitochondria or lipid droplets). It is not known how autophagy changes in coexisting cell types in the aging skeletal muscle, how prevalent are organelle-specific autophagy, and whether there is coordination between organelle-specific autophagy types. Techniques to pinpoint to the molecular and cellular pathways behind the changes observed in complex tissues and co-existing forms of autophagy are not readily available. In order to address some of the current technological limitations, this application proposes the development and use of mass cytometry to carry out single cell proteomics and individual organelle capillary electrophoresis to investigate organelle populations of autophagy in aging skeletal muscle.
The aims of this proposal are: (1) Establish mass cytometry strategies to monitor at the single cell level autophagy-related molecular changes in muscle fibers, macrophages, and satellite cells. (2) Establish individual-organelle capillary electrophoretic strategies that selectively describe lipophagy and mitophagy in muscle fibers, macrophages, and satellite cells. (3) Define changes in lipophagy, mitophagy and global autophagy in a murine model of aging under basal and tissue injury/repair conditions using the methodologies developed under Aims 1 and 3. Completion of the proposed work will provide new technological advances to fine tune the characterization of autophagy and will provide more concrete answers to the controversial role of autophagy in the aging of the skeletal muscle system.

Public Health Relevance

Loss of muscle mass and function that occurs in aging compromises physical performance, lifestyle, and recovery after injury for half of those in their late seventies or older. Autophagy (degradation of cellular components) appears to play a role in the changes observed in the muscle system. This application proposes the development of new methodologies to understand the cell types involved in those changes and define in those cells how the degradation of their cellular components is affected by aging.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute on Aging (NIA)
Type
Research Project (R01)
Project #
5R01AG020866-15
Application #
9262110
Study Section
Enabling Bioanalytical and Imaging Technologies Study Section (EBIT)
Program Officer
Williams, John
Project Start
2002-04-15
Project End
2021-03-31
Budget Start
2017-04-01
Budget End
2018-03-31
Support Year
15
Fiscal Year
2017
Total Cost
$270,390
Indirect Cost
$85,890

  Institution

Name
University of Minnesota Twin Cities
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
555917996
City
Minneapolis
State
MN
Country
United States
Zip Code
55455

  Publications

Muratore, Katherine A; Najt, Charles P; Livezey, Nicholas M et al. (2018) Sizing lipid droplets from adult and geriatric mouse liver tissue via nanoparticle tracking analysis. Anal Bioanal Chem 410:3629-3638
Satori, Chad P; Ramezani, Marzieh; Koopmeiners, Joseph S et al. (2017) Checkpoints for Preliminary Identification of Small Molecules found Enriched in Autophagosomes and Activated Mast Cell Secretions Analyzed by Comparative UPLC/MSe. Anal Methods 9:46-54
Daniele, Joseph R; Esping, Daniel J; Garcia, Gilbert et al. (2017) ""High-Throughput Characterization of Region-Specific Mitochondrial Function and Morphology"". Sci Rep 7:6749
Muratore, Katherine A; Grundhofer, Heather M; Arriaga, Edgar A (2016) Capillary Electrophoresis with Laser-Induced Fluorescent Detection of Immunolabeled Individual Autophagy Organelles Isolated from Liver Tissue. Anal Chem 88:11691-11698
Luo, Jinghui; Muratore, Katherine A; Arriaga, Edgar A et al. (2016) Deterministic Absolute Negative Mobility for Micro- and Submicrometer Particles Induced in a Microfluidic Device. Anal Chem 88:5920-7
Palsuledesai, Charuta C; Ochocki, Joshua D; Kuhns, Michelle M et al. (2016) Metabolic Labeling with an Alkyne-modified Isoprenoid Analog Facilitates Imaging and Quantification of the Prenylome in Cells. ACS Chem Biol 11:2820-2828
Daniele, Joseph R; Heydari, Kartoosh; Arriaga, Edgar A et al. (2016) Identification and Characterization of Mitochondrial Subtypes in Caenorhabditis elegans via Analysis of Individual Mitochondria by Flow Cytometry. Anal Chem 88:6309-16
Kumar, Shailabh; Wolken, Gregory G; Wittenberg, Nathan J et al. (2015) Nanohole Array-Directed Trapping of Mammalian Mitochondria Enabling Single Organelle Analysis. Anal Chem 87:11973-7
Luo, Jinghui; Abdallah, Bahige G; Wolken, Gregory G et al. (2014) Insulator-based dielectrophoresis of mitochondria. Biomicrofluidics 8:021801
Hahn, Wendy S; Kuzmicic, Jovan; Burrill, Joel S et al. (2014) Proinflammatory cytokines differentially regulate adipocyte mitochondrial metabolism, oxidative stress, and dynamics. Am J Physiol Endocrinol Metab 306:E1033-45

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