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用于自发荧光无干扰的活体斑马鱼发育过程长期体内成像的时门控 FRET 纳米探针。

Time-Gated FRET Nanoprobes for Autofluorescence-Free Long-Term In Vivo Imaging of Developing Zebrafish.

机构信息

Institute for Integrative Biology of the Cell (I2BC), Université Paris-Saclay, CNRS, CEA, Orsay Cedex, 91405, France.

Institut des Neurosciences Paris-Saclay, Université Paris-Saclay, CNRS, Gif-sur-Yvette, 91190, France.

出版信息

Adv Mater. 2020 Oct;32(39):e2003912. doi: 10.1002/adma.202003912. Epub 2020 Aug 16.

DOI:10.1002/adma.202003912
PMID:33252168
Abstract

The zebrafish is an important vertebrate model for disease, drug discovery, toxicity, embryogenesis, and neuroscience. In vivo fluorescence microscopy can reveal cellular and subcellular details down to the molecular level with fluorescent proteins (FPs) currently the main tool for zebrafish imaging. However, long maturation times, low brightness, photobleaching, broad emission spectra, and sample autofluorescence are disadvantages that cannot be easily overcome by FPs. Here, a bright and photostable terbium-to-quantum dot (QD) Förster resonance energy transfer (FRET) nanoprobe with narrow and tunable emission bands for intracellular in vivo imaging is presented. The long photoluminescence (PL) lifetime enables time-gated (TG) detection without autofluorescence background. Intracellular four-color multiplexing with a single excitation wavelength and in situ assembly and FRET to mCherry demonstrate the versatility of the TG-FRET nanoprobes and the possibility of in vivo bioconjugation to FPs and combined nanoprobe-FP FRET sensing. Upon injection at the one-cell stage, FRET nanoprobes can be imaged in developing zebrafish embryos over seven days with toxicity similar to injected RNA and strongly improved signal-to-background ratios compared to non-TG imaging. This work provides a strategy for advancing in vivo fluorescence imaging applications beyond the capabilities of FPs.

摘要

斑马鱼是疾病、药物发现、毒性、胚胎发生和神经科学的重要脊椎动物模型。活体荧光显微镜可以通过荧光蛋白 (FP) 揭示细胞和亚细胞细节,达到分子水平,目前 FP 是斑马鱼成像的主要工具。然而,成熟时间长、亮度低、光漂白、宽发射光谱和样品自发荧光等缺点是 FP 难以克服的。这里,我们提出了一种明亮且稳定的铽-量子点(QD)荧光共振能量转移(FRET)纳米探针,它具有窄且可调发射带,可用于细胞内活体成像。长的光致发光(PL)寿命使时间门控(TG)检测成为可能,而无需自发荧光背景。使用单个激发波长的细胞内四色复用以及原位组装和与 mCherry 的 FRET 证明了 TG-FRET 纳米探针的多功能性以及与 FP 进行体内生物偶联和组合纳米探针-FP FRET 传感的可能性。在单细胞阶段注射后,FRET 纳米探针可以在发育中的斑马鱼胚胎中成像七天,其毒性与注射的 RNA 相似,与非 TG 成像相比,信号与背景的比值大大提高。这项工作为推进 FP 能力之外的活体荧光成像应用提供了一种策略。

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