All-Optical Wide-Field Selective Imaging of Fluorescent Nanodiamonds in Cells, In Vivo and Ex Vivo

荧光 纳米金刚石 荧光寿命成像显微镜 自体荧光 分子成像 材料科学 纳米探针 临床前影像学 生物分子 体内 纳米技术 生物物理学 光学 物理 生物 钻石 生物技术 复合材料
作者
Tamami Yanagi,Kiichi Kaminaga,Michiyo Suzuki,Hiroshi Abe,Hiroki Yamamoto,Takeshi Ohshima,Akihiro Kuwahata,Masaki Sekino,Tatsuhiko Imaoka,Shizuko Kakinuma,Takuma Sugi,Wataru Kada,Osamu Hanaizumi,Ryuji Igarashi
出处
期刊:ACS Nano [American Chemical Society]
卷期号:15 (8): 12869-12879 被引量:22
标识
DOI:10.1021/acsnano.0c07740
摘要

Fluorescence imaging is a critical tool to understand the spatial distribution of biomacromolecules in cells and in vivo, providing information on molecular dynamics and interactions. Numerous valuable insights into biological systems have been provided by the specific detection of various molecular species. However, molecule-selective detection is often hampered by background fluorescence, such as cell autofluorescence and fluorescence leakage from molecules stained by other dyes. Here we describe a method for all-optical selective imaging of fluorescent nanodiamonds containing nitrogen-vacancy centers (NVCs) for wide-field fluorescence bioimaging. The method is based on the fact that the fluorescence intensity of NVCs strictly depends on the configuration of ground-state electron spins, which can be controlled by changing the pulse recurrence intervals of microsecond excitation laser pulses. Therefore, by using regulated laser pulses, we can oscillate the fluorescence from NVCs in a nanodiamond, while oscillating other optical signals in the opposite phase to NVCs. As a result, we can reconstruct a selective image of a nanodiamond by using a series of oscillated fluorescence images. We demonstrate application of the method to the selective imaging of nanodiamonds in live cells, in microanimals, and on a hippocampal slice culture obtained from a rat. Our approach potentially enables us to achieve high-contrast images of nanodiamond-labeled biomolecules with a signal-to-background ratio improved by up to 100-fold over the standard fluorescence image, thereby providing a more powerful tool for the investigation of molecular dynamics in cells and in vivo.
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