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김채운

Kim, Chae Un
High Pressure X-ray Science Lab.
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Cryogenic single-molecule fluorescence imaging

Author(s)
Yu, Phil SangKim, Chae UnLee, Jong-Bong
Issued Date
2025-01
DOI
10.5483/BMBRep.2024-0180
URI
https://scholarworks.unist.ac.kr/handle/201301/86280
Citation
BMB REPORTS, v.58, no.1, pp.2 - 7
Abstract
Cryo-fixation techniques, including cryo-electron and cryo- fluorescence microscopy, enable the preservation of bio-logical samples in a near-native state by rapidly freezing them into an amorphous ice phase. These methods prevent the structural distortions often caused by chemical fixation, allowing for high-resolution imaging. At low temperatures, fluorophores exhibit improved properties, such as extended fluorescence lifetimes, reduced photobleaching, and enhanced signal-to- noise ratios, making single-molecule imaging more accurate and insightful. Despite these advantages, challenges remain, including limitations in numerical aperture of objectives and cryo-stage for single-molecule imaging, which can affect pho-ton detection and spatial resolution. Recent advancements at low temperatures have mitigated these issues, achieving resolutions at the nanometer scale. Looking forward, innovations in super-resolution techniques, optimized fluorophores, and Artificial Intelligence (AI)-based data analysis promise to further advance the field, providing deeper insights into biomolecular dynamics and interactions. In this mini-review, we will introduce low-temperature single-molecule fluorescence imaging techniques and discuss future perspectives in this field.
Publisher
KOREAN SOCIETY BIOCHEMISTRY & MOLECULAR BIOLOGY
ISSN
1976-6696
Keyword (Author)
Cryogenicsingle-molecule imagingPhotoblinkingSolid-immersion lens (SIL)Cryogenic fluorescence microscopy (Cryo-FM)
Keyword
CORRELATIVE SUPERRESOLUTION FLUORESCENCEELECTRON-MICROSCOPYCOLOCALIZATION MICROSCOPYLOCALIZATIONBLINKINGCELLS

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