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Nanoscale Resolution Imaging of Whole Mouse Embryos Using Expansion Microscopy

Authors
Sim, JueunPark, Chan E.Cho, InMin, KyeongbaeEom, MinhoHan, SeungjaeJeon, HyungjuCho, Eun-SeoLee, YunjeongYun, Young HyunLee, SunghoCheon, Deok-HyeonKim, JihyunKim, MuseongCho, Hyun-JuPark, Ji-WonKumar, AjeetChong, YosepKang, Jeong SeukPiatkevich, Kiryl D.Jung, Erica E.Kang, Du-SeockKwon, Seok-KyuKim, JinhyunYoon, Ki-JunLee, Jeong-SooKim, Cheol-HeeChoi, MyunghwanKim, Jin WooSong, Mi-RyoungChoi, Hyung JinBoyden, Edward S.Yoon, Young-GyuChang, Jae-Byum
Issue Date
18-Feb-2025
Publisher
American Chemical Society
Keywords
embryo imaging; expansion microscopy; peripheral nerve system; super-resolution imaging; whole-body imaging
Citation
ACS Nano, v.19, no.8, pp 7910 - 7927
Pages
18
Indexed
SCIE
SCOPUS
Journal Title
ACS Nano
Volume
19
Number
8
Start Page
7910
End Page
7927
URI
https://scholarx.skku.edu/handle/2021.sw.skku/120698
DOI
10.1021/acsnano.4c14791
ISSN
1936-0851
1936-086X
Abstract
Nanoscale imaging of whole vertebrates is essential for the systematic understanding of human diseases, yet this goal has not yet been achieved. Expansion microscopy (ExM) is an attractive option for accomplishing this aim; however, the expansion of even mouse embryos at mid- and late-developmental stages, which have fewer calcified body parts than adult mice, is yet to be demonstrated due to the challenges of expanding calcified tissues. Here, we introduce a state-of-the-art ExM technique, termed whole-body ExM, that utilizes cyclic digestion. This technique allows for the super-resolution, volumetric imaging of anatomical structures, proteins, and endogenous fluorescent proteins (FPs) within embryonic and neonatal mice by expanding them 4-fold. The key feature of whole-body ExM is the alternating application of two enzyme compositions repeated multiple times. Through the simple repetition of this digestion process with an increasing number of cycles, mouse embryos of various stages up to E18.5, and even neonatal mice, which display a dramatic difference in the content of calcified tissues compared to embryos, are expanded without further laborious optimization. Furthermore, the whole-body ExM’s ability to retain FP signals allows the visualization of various neuronal structures in transgenic mice. Whole-body ExM could facilitate studies of molecular changes in various vertebrates. © 2025 American Chemical Society.
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