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Super-resolution Fluorescence Microscopy

JoVE Core
Cell Biology
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JoVE Core Cell Biology
Super-resolution Fluorescence Microscopy

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01:37 min

April 30, 2023

Super-resolution fluorescence microscopy (SRFM) provides a better resolution than conventional fluorescence microscopy by reducing the point spread function (PSF). PSF is the light intensity distribution from a point that causes it to appear blurred. Due to PSF, each fluorescing point appears bigger than its actual size, and it is the PSF interference of nearby fluorophores that causes the blurred image. Various approaches to achieving higher resolution through SRFM have recently been developed.

Photoactivated Localization Microscopy

Photoactivated localization microscopy (PALM) is a type of fluorescence microscopy that captures high-resolution images using a single-molecule detection and localization approach. For example, two fluorescent spots 75 nm apart may appear to be a single spot during imaging due to interference of their PSFs. In such cases, especially for live-cell imaging, PALM is a suitable technique to resolve the interference and provide a better resolution.

In PALM, a variant of green fluorescent protein (GFP) with a different excitation wavelength and high fluorescence is employed. In the first step, a few GFPs are activated and imaged with very high precision. In the next step, another set of GFPs is activated and imaged. Step by step, all the GFPs across the specimen are thus recorded. Finally, the data is processed to generate a high-resolution image.

Stochastic Optical Reconstruction Microscopy

In stochastic optical reconstruction microscopy (STORM), unique photo-switchable probes are used for specimen imaging. The emission from these probes can be switched on and off using lights of different wavelengths. Thus, only a few fluorophores can be activated at a point in time such that the number of activated fluorophores is significantly lesser than the number of deactivated fluorophores. This selective activation of probes helps determine their precise position in the specimen. Following this, the center of each fluorescent probe is identified and marked. The process is then repeated to record all the fluorescent probes in the specimen. Finally, a high-resolution composite image is constructed by superimposing these multiple images.