Tianxiang Wu scite author profile

In vivo fluorescence imaging in the second near-infrared window (NIR-II) has been considered as a promising technique for visualizing mammals. However, the definition of the NIR-II region and the mechanism accounting for the excellent performance still need to be perfected. Herein, we simulate the photon propagation in the NIR region (to 2340 nm), confirm the positive contribution of moderate light absorption by water in intravital imaging and perfect the NIR-II window as 900–1880 nm, where 1400–1500 and 1700–1880 nm are defined as NIR-IIx and NIR-IIc regions, respectively. Moreover, 2080–2340 nm is newly proposed as the third near-infrared (NIR-III) window, which is believed to provide the best imaging quality. The wide-field fluorescence microscopy in the brain is performed around the NIR-IIx region, with excellent optical sectioning strength and the largest imaging depth of intravital NIR-II fluorescence microscopy to date. We also propose 1400 nm long-pass detection in off-peak NIR-II imaging whose performance exceeds that of NIR-IIb imaging, using bright fluorophores with short emission wavelength.

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Long-term monitoring of intravital biological processes using fluorescent protein-assisted NIR-II imaging

Chen

Feng

Fan

et al. 2022

Nat Commun

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High spatial resolution, low background, and deep tissue penetration have made near-infrared II (NIR-II) fluorescence imaging one of the most critical tools for in vivo observation and measurement. However, the relatively short retention time and potential toxicity of synthetic NIR-II fluorophores limit their long-term application. Here, we report the use of infrared fluorescent proteins (iRFPs) as in vitro and in vivo NIR-II probes permitting prolonged continuous imaging (up to 15 months). As a representative example, iRFP713 is knocked into the mouse genome to generate a transgenic model to allow temporal and/or spatial expression control of the probe. To demonstrate its feasibility in a genuine diagnostic context, we adopt two liver regeneration models and successfully track the process for a week. The performance and monitoring efficacy are comparable to those of μCT and superior to those of indocyanine green dye. We are also able to effectively observe the pancreas, despite its deep location, under both physiological and pathological conditions. These results indicate that the iRFP-assisted NIR-II fluorescence system is suitable for monitoring various tissues and in vivo biological processes, providing a powerful noninvasive long-term imaging platform.

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Aggregation-induced emission nanoprobe assisted ultra-deep through-skull three-photon mouse brain imaging

Zhang

et al. 2022

Nano Today

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Aggregation-induced emission fluorophores towards the second near-infrared optical windows with suppressed imaging background

Feng

et al. 2022

Coordination Chemistry Reviews

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Tianxiang Wu

Perfecting and extending the near-infrared imaging window

Long-term monitoring of intravital biological processes using fluorescent protein-assisted NIR-II imaging

Aggregation-induced emission nanoprobe assisted ultra-deep through-skull three-photon mouse brain imaging

Aggregation-induced emission fluorophores towards the second near-infrared optical windows with suppressed imaging background

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