Super-resolution microscopy of genome organization
- Authors
- Shim, Sang-Hee
- Issue Date
- 3월-2021
- Publisher
- SPRINGER
- Keywords
- Chromatin structure; Fluorescence microscopy; Genome architecture; Super& #8208; resolution microscopy
- Citation
- GENES & GENOMICS, v.43, no.3, pp.281 - 287
- Indexed
- SCIE
SCOPUS
KCI
- Journal Title
- GENES & GENOMICS
- Volume
- 43
- Number
- 3
- Start Page
- 281
- End Page
- 287
- URI
- https://scholar.korea.ac.kr/handle/2021.sw.korea/137748
- DOI
- 10.1007/s13258-021-01044-9
- ISSN
- 1976-9571
- Abstract
- Recent advancements in sequencing and imaging technologies are providing new perspectives in solving the mystery of three-dimensional folding of genome in a nucleus. Chromosome conformation capture sequencing has discovered new chromatin structures such as topologically associated domains and loops in hundreds of kilobases. Super-resolution fluorescence microscopy with nanometer resolutions, in particular multiplexed approaches with sequence-specificity, has visualized chromatin structures from the rough folds of whole chromosomes to the fine loops of cis-regulatory elements in intact individual nuclei. Here, recent advancements in genome visualization tools with highly multiplexed labeling and reading are introduced. These imaging technologies have found ensemble behavior consistent to sequencing results, while unveiling single-cell variations. But, they also generated contradictory results on the roles of architectural proteins (like cohesion and CTCF) and enhancer-promoter interactions. Live-cell labeling methods for imaging specific genomic loci, especially the CRISPR/dCas9 system, are reviewed in order to give perspectives in the emergence of tools for visualizing genome structural dynamics.
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Collections - College of Science > Department of Chemistry > 1. Journal Articles
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