Shou Jingwen, Oda Robert, Hu Fanghao, Karasawa Keiko, Nuriya Mutsuo, Yasui Masato, Shiramizu Bruce, Min Wei, Ozeki Yasuyuki
Department of Electrical Engineering and Information Systems, The University of Tokyo, Tokyo 113-8656, Japan.
Department of Molecular Biosciences and Bioengineering, The University of Hawaii, Manoa, 1955 East West Road, Honolulu, Hawaii 96822, USA.
iScience. 2021 Jul 9;24(8):102832. doi: 10.1016/j.isci.2021.102832. eCollection 2021 Aug 20.
Observing multiple molecular species simultaneously with high spatiotemporal resolution is crucial for comprehensive understanding of complex, dynamic, and heterogeneous biological systems. The recently reported super-multiplex optical imaging breaks the "color barrier" of fluorescence to achieve multiplexing number over six in living systems, while its temporal resolution is limited to several minutes mainly by slow color tuning. Herein, we report integrated stimulated Raman and fluorescence microscopy with simultaneous multimodal color tunability at high speed, enabling super-multiplex imaging covering diverse molecular contrasts with temporal resolution of seconds. We highlight this technique by demonstrating super-multiplex time-lapse imaging and image-based cytometry of live cells to investigate the dynamics and cellular heterogeneity of eight intracellular components simultaneously. Our technique provides a powerful tool to elucidate spatiotemporal organization and interactions in biological systems.
以高时空分辨率同时观察多个分子物种对于全面理解复杂、动态和异质的生物系统至关重要。最近报道的超多重光学成像打破了荧光的“颜色障碍”,在活体系统中实现了超过六种的复用数量,但其时间分辨率主要受缓慢的颜色调谐限制,仅为几分钟。在此,我们报告了集成受激拉曼和荧光显微镜,具有高速同步多模态颜色可调性,实现了涵盖多种分子对比度且时间分辨率为秒级的超多重成像。我们通过展示活细胞的超多重延时成像和基于图像的细胞计数来突出这项技术,以同时研究八种细胞内成分的动态和细胞异质性。我们的技术为阐明生物系统中的时空组织和相互作用提供了一个强大的工具。
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