Lifetime imaging of the discrete nanophosphors in biological systems

A. O. Zvyagintcev, A. V. Yudintsev, A. Maleki, V. Vodeneev, A. Zvyagin
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引用次数: 0

Abstract

The aim. Demonstrate a novel modality of laser-scanning multiphoton microscopy suitable for rapid acquisition of images of samples labelled with phosphorescent materials characterised by long emission lifetime measured in microseconds. The reported microscopy represents an advancement over the existing laser-scanning modalities, where the acquisition of images of phosphorescent materials takes unpractically long time.Materials and methods. The reported method is based on rapid scanning of the focussed excitation beam across a sample while continuously recording the photoluminescent (PL) signal. The resultant images of discrete phosphorescent nanoparticles appeared blurred. The diffraction-limited image was reconstructed by using a deconvolution algorithm, where the PL lifetime was the key input parameter. To test the method, two types of upconversion nanoparticles (UCNP) were synthesised, NaYF4:Yb3+:Er3+/NaYF4 (E-UCNP), β-NaYF4:Yb3+, Tm3+/NaYF4 (T-UCNP) and used to test a possibility of demultiplexing the two types of UCNPs ex vivo taken up in the mouse liver.Results. The resultant images of E-UCNP, T-UCNP on the background of the liver were fully reconstructed and exhibited the enhanced signal-to-noise ratio. Besides, the method allowed rapid (at the scale of seconds) acquisition of the UCNP PL lifetime and clear discrimination of the two types of UCNPs.Conclusion. We demonstrated a new approach for rapid PL image acquisition of samples containing PL materials, such as biological specimens labelled with discrete UCNPs. Blurred images were shown to be reconstructed at the post-processing stage by applying a deconvolution procedure. This enabled demonstration of multiplexing/demultiplexing using lifetime imaging mode, where the lifetime was engineered by the UCNP synthesis and reconstructed during multiphoton image acquisition using the deconvolution algorithm. The power of this method was demonstrated by the identification of two types of UCNPs accumulated in the liver of a laboratory animal. We believe that the demonstrated method can be useful for rapid lifetime imaging where several molecular specific labelling agents are required.
生物系统中离散纳米荧光粉的寿命成像
的目标。演示一种新型的激光扫描多光子显微镜,适用于快速获取带有磷光材料的样品图像,其特征是在微秒内测量长发射寿命。报道的显微镜代表了现有的激光扫描模式的进步,其中获取磷光材料的图像需要不实际的长时间。材料和方法。所报道的方法是基于快速扫描聚焦激发光束穿过样品,同时连续记录光致发光(PL)信号。所得的离散磷光纳米颗粒图像显得模糊。使用反卷积算法重构衍射受限图像,其中PL寿命是关键输入参数。为了验证该方法,我们合成了两种类型的上转换纳米颗粒(UCNP),即NaYF4:Yb3+:Er3+/NaYF4 (E-UCNP), β-NaYF4:Yb3+, Tm3+/NaYF4 (T-UCNP),并用于测试小鼠肝脏中两种类型的UCNP在体外解复用的可能性。得到的E-UCNP、T-UCNP在肝脏背景下的图像被完全重建,并表现出增强的信噪比。此外,该方法可以快速(以秒为尺度)获取UCNP的PL寿命,并可以明确区分两种类型的UCNP。我们展示了一种快速获取含有PL材料样品的PL图像的新方法,例如用离散UCNPs标记的生物标本。通过应用反卷积程序,在后处理阶段显示了模糊图像的重建。这使得使用寿命成像模式的复用/解复用演示成为可能,其中寿命由UCNP合成设计,并在多光子图像采集期间使用反卷积算法进行重建。通过鉴定在实验动物肝脏中积累的两种类型的UCNPs,证明了该方法的有效性。我们相信所演示的方法可用于需要几种分子特异性标记剂的快速终身成像。
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