4.7 Article

Bioenergetics underlying single-cell migration on aligned nanofiber scaffolds

Journal

AMERICAN JOURNAL OF PHYSIOLOGY-CELL PHYSIOLOGY
Volume 318, Issue 3, Pages C476-C485

Publisher

AMER PHYSIOLOGICAL SOC
DOI: 10.1152/ajpcell.00221.2019

Keywords

bioenergetics; glycolysis; migration; mitochondria; single cell

Funding

  1. NIH National Heart, Lung, and Blood Institute [HL-123647]
  2. U.S. Department of Agriculture National Institute of Food and Agriculture Hatch Project [1017927]
  3. National Science Foundation [1437101, 1762634]
  4. Directorate For Engineering
  5. Div Of Civil, Mechanical, & Manufact Inn [1762634] Funding Source: National Science Foundation
  6. Directorate For Engineering
  7. Div Of Civil, Mechanical, & Manufact Inn [1437101] Funding Source: National Science Foundation

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Cell migration is centrally involved in a myriad of physiological processes, including morphogenesis, wound healing, tissue repair, and metastatic growth. The bioenergetics that underlie migratory behavior are not fully understood, in part because of variations in cell culture media and utilization of experimental cell culture systems that do not model physiological connective extracellular fibrous networks. In this study, we evaluated the bioenergetics of C2C12 myoblast migration and force production on fibronectin-coated nanofiber scaffolds of controlled diameter and alignment, fabricated using a nonelectrospinning spinneret-based tunable engineered parameters (STEP) platform. The contribution of various metabolic pathways to cellular migration was determined using inhibitors of cellular respiration, ATP synthesis, glycolysis, or glucose uptake. Despite immediate effects on oxygen consumption, mitochondrial inhibition only modestly reduced cell migration velocity, whereas inhibitors of glycolysis and cellular glucose uptake led to striking decreases in migration. The migratory metabolic sensitivity was modifiable based on the substrates present in cell culture media. Cells cultured in galactose (instead of glucose) showed substantial migratory sensitivity to mitochondrial inhibition. We used nanonet force microscopy to determine the bioenergetic factors responsible for single-cell force production and observed that neither mitochondrial nor glycolytic inhibition altered single-cell force production. These data suggest that myoblast migration is heavily reliant on glycolysis in cells grown in conventional media. These studies have wide-ranging implications for the causes, consequences, and putative therapeutic treatments aimed at cellular migration.

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