4.4 Article

Extracellular Vesicle Uptake Assay via Confocal Microscope Imaging Analysis

Journal

JOVE-JOURNAL OF VISUALIZED EXPERIMENTS
Volume -, Issue 180, Pages -

Publisher

JOURNAL OF VISUALIZED EXPERIMENTS
DOI: 10.3791/62836

Keywords

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Funding

  1. NCI [U54CA143803, CA163124, CA093900, CA143055]
  2. Ministry of Health & Welfare, Republic of Korea [HI19C1122]
  3. Institute for Basic Science [IBS-R020-D1]
  4. Korean Government
  5. Korea Health Technology R&D Project through the Korea Health Industry Development Institute (KHIDI)

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This study proposes an efficient method for quantifying cellular uptake of extracellular vesicles (EVs) through three-dimensional fluorescence confocal microscopy. The method involves fluorescently labeling EVs, preparing them using a microfluidic device, visualizing their location within cells, and analyzing the images using advanced image-processing software.
There is a need for practical assays to visualize and quantify the cells' extracellular vesicle (EV) uptake. EV uptake plays a role in intercellular communication in various research fields; cancer biology, neuroscience, and drug delivery. Many EV uptake assays have been reported in the literature; however, there is a lack of practical, detailed experimental methodology. EV uptake can be assessed by fluorescently labeling EVs to detect their location within cells. Distinguishing between internalized EVs in cells and the superficial EVs on cells is difficult, yet critical, to accurately determine the EV uptake. Therefore, an assay that efficiently quantifies EV uptake through three-dimensional (3D) fluorescence confocal microscopy is proposed in this work. Fluorescently labeled EVs were prepared using a nano-filtration-based microfluidic device, visualized by 3D confocal microscopy, and then analyzed through advanced image-processing software. The protocol provides a robust methodology for analyzing EVs on a cellular level and a practical approach for efficient analysis.

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