AI Article Synopsis

  • A new super-resolution optical imaging method enhances spatial positioning of fluorescent reporters using temporal information, allowing high precision even with scattered light.
  • This technique employs a cost function based on a diffusion equation forward model, aiming for micron-scale resolution over several centimeters of tissue.
  • It offers promising applications for in vivo imaging, potentially enabling the localization of individual neuron activity in a rodent brain.

Article Abstract

A super-resolution optical imaging method is presented that relies on the distinct temporal information associated with each fluorescent optical reporter to determine its spatial position to high precision with measurements of heavily scattered light. This multiple-emitter localization approach uses a diffusion equation forward model in a cost function, and has the potential to achieve micron-scale spatial resolution through centimeters of tissue. Utilizing some degree of temporal separation for the reporter emissions, position and emission strength are determined using a computationally efficient time stripping multiresolution algorithm. The approach circumvents the spatial resolution challenges faced by earlier optical imaging approaches using a diffusion equation forward model, and is promising for in vivo applications. For example, in principle, the method could be used to localize individual neurons firing throughout a rodent brain, enabling direct imaging of neural network activity.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7012689PMC
http://dx.doi.org/10.1109/TIP.2019.2931080DOI Listing

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