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电阻脉冲传感与荧光寿命成像显微镜联用用于区分单个脂质体

Resistive-Pulse Sensing Coupled with Fluorescence Lifetime Imaging Microscopy for Differentiation of Individual Liposomes.

作者信息

Young Tanner W, Cox-Vázquez Sarah J, Call Ethan D, Shah Dhari C, Jacobson Stephen C, Vázquez Ricardo J

机构信息

Department of Chemistry, Indiana University, Bloomington, Indiana 47405-7102, United States.

出版信息

ACS Nano. 2025 Jan 21;19(2):2162-2170. doi: 10.1021/acsnano.4c10813. Epub 2025 Jan 1.

DOI:10.1021/acsnano.4c10813
PMID:39741459
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC11811929/
Abstract

Characterization of individual biological nanoparticles can be significantly improved by coupling complementary analytical methods. Here, we combine resistive-pulse sensing (RPS) with fluorescence lifetime imaging microscopy (FLIM) to differentiate liposomes at the single-particle level. RPS measures the particle volume, shape, and surface-charge density, and FLIM determines the fluorescence lifetime of the fluorophore associated with the lipid membrane. The RPS devices are fabricated in-plane on a glass substrate to facilitate coupling of RPS with FLIM measurements. For proof-of-concept, we studied liposomes containing various cholesterol concentrations with membrane-intercalated Di-8-ANEPPS, whose fluorescence lifetime is known to be sensitive to cholesterol concentrations in the membrane. RPS-FLIM revealed that increasing cholesterol concentrations in the liposome from 0% to 50% increased the fluorescence lifetimes from 2.1 ± 0.2 to 3.4 ± 0.5 ns, respectively. Moreover, RPS-FLIM discerned liposome populations with the same cholesterol concentration but labeled with dyes that have different fluorescence lifetimes (Di-8-ANEPPS and COE-S6), parsing two particle populations with statistically identical volumes, cholesterol concentration, and lipid composition. Interrogation with RPS-FLIM occurred with individual particles making a single pass through the detection region and overcomes issues with fluorescence spectral overlap that limits traditional methods. We envision RPS-FLIM as a versatile and scalable technique with the potential to differentiate biological particles at the single-particle level to simultaneously inform on particle size, surface-charge density, membrane composition, and identity.

摘要

通过结合互补的分析方法,可以显著改善对单个生物纳米颗粒的表征。在这里,我们将电阻脉冲传感(RPS)与荧光寿命成像显微镜(FLIM)相结合,以在单颗粒水平上区分脂质体。RPS测量颗粒的体积、形状和表面电荷密度,而FLIM则确定与脂质膜相关的荧光团的荧光寿命。RPS装置在玻璃基板上平面制造,以促进RPS与FLIM测量的耦合。为了验证概念,我们研究了含有不同胆固醇浓度且膜插入Di-8-ANEPPS的脂质体,已知其荧光寿命对膜中的胆固醇浓度敏感。RPS-FLIM显示,脂质体中胆固醇浓度从0%增加到50%时,荧光寿命分别从2.1±0.2 ns增加到3.4±0.5 ns。此外,RPS-FLIM能够区分胆固醇浓度相同但用具有不同荧光寿命的染料(Di-8-ANEPPS和COE-S6)标记的脂质体群体,解析出两个在体积、胆固醇浓度和脂质组成上统计上相同的颗粒群体。RPS-FLIM对单个颗粒进行单次通过检测区域的询问,并克服了限制传统方法的荧光光谱重叠问题。我们设想RPS-FLIM是一种通用且可扩展的技术,有潜力在单颗粒水平上区分生物颗粒,同时提供颗粒大小、表面电荷密度、膜组成和身份等信息。

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本文引用的文献

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Fluorescence Lifetime Multiplex Imaging in Expansion Microscopy with Tunable Donor-Acceptor Polymer Dots.基于可调供体-受体聚合物点的扩展显微镜中的荧光寿命多重成像。
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用于电阻脉冲传感的集成平面纳米流体装置
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Simultaneous Multipass Resistive-Pulse Sensing and Fluorescence Imaging of Liposomes.脂质体的多次电阻脉冲传感和荧光成像的同时检测。
ACS Nano. 2024 Mar 5;18(9):7241-7252. doi: 10.1021/acsnano.3c12627. Epub 2024 Feb 20.
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Characterization of Extracellular Vesicles by Resistive-Pulse Sensing on In-Plane Multipore Nanofluidic Devices.平面多微孔纳米流控器件上电阻脉冲传感法对细胞外囊泡的表征。
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