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A noninvasive fluorescence imaging-based platform measures 3D anisotropic extracellular diffusion. | LitMetric

AI Article Synopsis

  • Diffusion is essential for understanding how tissue structures affect biochemical environments and functions.
  • A new noninvasive imaging technique called LiFT-FRAP measures 3D diffusion of biomolecules, achieving relevant physiological diffusion rates.
  • This method reveals limitations of traditional 2D diffusion measurements and highlights how disease and tissue composition changes impact diffusion, making it a key technology for research and clinical applications.

Article Abstract

Diffusion is a major molecular transport mechanism in biological systems. Quantifying direction-dependent (i.e., anisotropic) diffusion is vitally important to depicting how the three-dimensional (3D) tissue structure and composition affect the biochemical environment, and thus define tissue functions. However, a tool for noninvasively measuring the 3D anisotropic extracellular diffusion of biorelevant molecules is not yet available. Here, we present light-sheet imaging-based Fourier transform fluorescence recovery after photobleaching (LiFT-FRAP), which noninvasively determines 3D diffusion tensors of various biomolecules with diffusivities up to 51 µm s, reaching the physiological diffusivity range in most biological systems. Using cornea as an example, LiFT-FRAP reveals fundamental limitations of current invasive two-dimensional diffusion measurements, which have drawn controversial conclusions on extracellular diffusion in healthy and clinically treated tissues. Moreover, LiFT-FRAP demonstrates that tissue structural or compositional changes caused by diseases or scaffold fabrication yield direction-dependent diffusion changes. These results demonstrate LiFT-FRAP as a powerful platform technology for studying disease mechanisms, advancing clinical outcomes, and improving tissue engineering.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7997923PMC
http://dx.doi.org/10.1038/s41467-021-22221-0DOI Listing

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