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A fluorogenic complementation tool kit for interrogating lipid droplet-organelle interaction.

Xiao LiRico GamuyaoMing-Lun WuWoo Jung ChoSharon V KingR A PetersenDaniel R StableyCaleb LindowLeslie K ClimerAbbas ShirinifardFrancesca FerraraRobert E ThromCamenzind G RobinsonYiwang ZhouAlexandre F CariseyAlison G TeboChi-Lun Chang
Published in: The Journal of cell biology (2024)
Contact sites between lipid droplets and other organelles are essential for cellular lipid and energy homeostasis upon metabolic demands. Detection of these contact sites at the nanometer scale over time in living cells is challenging. We developed a tool kit for detecting contact sites based on fluorogen-activated bimolecular complementation at CONtact sites, FABCON, using a reversible, low-affinity split fluorescent protein, splitFAST. FABCON labels contact sites with minimal perturbation to organelle interaction. Via FABCON, we quantitatively demonstrated that endoplasmic reticulum (ER)- and mitochondria (mito)-lipid droplet contact sites are dynamic foci in distinct metabolic conditions, such as during lipid droplet biogenesis and consumption. An automated analysis pipeline further classified individual contact sites into distinct subgroups based on size, likely reflecting differential regulation and function. Moreover, FABCON is generalizable to visualize a repertoire of organelle contact sites including ER-mito. Altogether, FABCON reveals insights into the dynamic regulation of lipid droplet-organelle contact sites and generates new hypotheses for further mechanistical interrogation during metabolic regulation.
Keyphrases
  • endoplasmic reticulum
  • living cells
  • fatty acid
  • high throughput
  • single cell
  • mass spectrometry
  • single molecule
  • binding protein
  • quantum dots
  • label free
  • capillary electrophoresis