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Probing Methionine Uptake in Live Cells by Deuterium Labeling and Stimulated Raman Scattering.

Spencer J SprattKenichi OguchiKeisuke MiuraMasato AsanumaHina KosakamotoFumiaki ObataYasuyuki Ozeki
Published in: The journal of physical chemistry. B (2022)
The small biomolecule methionine (Met) is a fundamental amino acid required for a vast range of biological processes such as protein synthesis, cancer metabolism, and epigenetics. However, it is still difficult to visualize the subcellular distribution of small biomolecules including Met in a minimally invasive manner. Here, we demonstrate stimulated Raman scattering (SRS) imaging of cellular uptake of deuterated methionine (d 8 -Met) in live HeLa cells by way of comparison to the previously used alkyne-labeled Met analogue─homopropargylglycine (Hpg). We show that the solutions of d 8 -Met and Hpg have similar SRS signal intensities. Furthermore, by careful image analysis with background subtraction, we succeed in the SRS imaging of cellular uptake of d 8 -Met with a much greater signal intensity than Hpg, possibly reflecting the increased and minimally invasive uptake kinetics of d 8 -Met compared with Hpg. We anticipate that d 8 -Met and other deuterated biomolecules will be useful for investigating metabolic processes with subcellular resolution.
Keyphrases
  • tyrosine kinase
  • minimally invasive
  • amino acid
  • induced apoptosis
  • cell cycle arrest
  • high resolution
  • robot assisted
  • signaling pathway
  • mass spectrometry
  • endoplasmic reticulum stress