Short-wavelength excitation two-photon intravital microscopy of endogenous fluorophores

被引:4
|
作者
Wu, Ting [1 ,2 ,3 ]
Liao, Jiuling [1 ,3 ]
Xiang, Feng [1 ,3 ]
Yu, Jia [1 ,3 ]
Gao, Yufeng [1 ,3 ]
Liu, Lina [1 ,3 ]
Ye, Shiwei [1 ,3 ]
Li, Hui [1 ,3 ]
Shi, Kebin [4 ,5 ,6 ]
Zheng, Wei [1 ,3 ]
机构
[1] Chinese Acad Sci, Shenzhen Inst Adv Technol, Res Ctr Biomed Opt & Mol Imaging, Shenzhen 518055, Peoples R China
[2] Univ Chinese Acad Sci, 19 A Yuquan Rd, Beijing 100049, Peoples R China
[3] Shenzhen Inst Adv Technol, Shenzhen Key Lab Mol Imaging, Guangdong Prov Key Lab Biomed Opt Imaging Technol, Shenzhen 518055, Peoples R China
[4] Peking Univ, Frontiers Sci Ctr Nanooptoelectron, Sch Phys, Beijing 100871, Peoples R China
[5] Peking Univ, State Key Lab Mesoscop Phys, Beijing 100871, Peoples R China
[6] Peking Univ, Natl Biomed Imaging Ctr, Beijing 100871, Peoples R China
来源
BIOMEDICAL OPTICS EXPRESS | 2023年 / 14卷 / 07期
基金
中国国家自然科学基金;
关键词
MULTIPHOTON MICROSCOPY; IN-VIVO; FLUORESCENCE; LIFETIME; TRYPTOPHAN; SPECTROSCOPY; PROTEINS; ORIGIN;
D O I
10.1364/BOE.493015
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
The noninvasive two-photon excitation autofluorescence imaging of cellular and subcellular structure and dynamics in live tissue could provide critical in vivo information for biomedical studies. However, the two-photon microscopy of short-wavelength endogenous fluorophores, such as tryptophan and hemoglobin, is extremely limited due to the lack of suitable imaging techniques. In this study, we developed a short-wavelength excitation time -and spectrum-resolved two-photon microscopy system. A 520-nm femtosecond fiber laser was used as the excitation source, and a time-correlated single-photon counting module connected with a spectrograph was used to provide time-and spectrum-resolved detection capability. The system was specially designed for measuring ultraviolet and violet-blue fluorescence signals and thus was very suitable for imaging short-wavelength endogenous fluorophores. Using the system, we systematically compared the fluorescence spectra and fluorescence lifetimes of short-wavelength endogenous fluorophores, including the fluorescent molecules tyrosine, tryptophan, serotonin (5-HT), niacin (vitamin B3), pyridoxine (vitamin B6), and NADH and the protein group (keratin, elastin, and hemoglobin). Then, high-resolution three-dimensional (3D) label-free imaging of different biological tissues, including rat esophageal tissue, rat oral cheek tissue, and mouse ear skin, was performed in vivo or ex vivo. Finally, we conducted time-lapse imaging of leukocyte migration in the lipopolysaccharide injection immunization model and a mechanical trauma immunization model. The results indicate that the system can specifically characterize short-wavelength endogenous fluorophores and provide noninvasive label-free 3D visualization of fine structures and dynamics in biological systems. The microscopy system developed here can empower more flexible imaging of endogenous fluorophores and provide a novel method for the 3D monitoring of biological events in their native environment.& COPY; 2023 Optica Publishing Group under the terms of the Optica Open Access Publishing Agreement
引用
收藏
页码:3380 / 3396
页数:17
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