4.6 Article

Cell Tracking by Magnetic Particle Imaging: Methodology for Labeling THP-1 Monocytes with Magnetic Nanoparticles for Cellular Imaging

Journal

CELLS
Volume 11, Issue 18, Pages -

Publisher

MDPI
DOI: 10.3390/cells11182892

Keywords

magnetic nanoparticles; magnetic particle spectroscopy; magnetic particle imaging; cell tracking; THP-1 monocytes; microscopy

Categories

Funding

  1. German Research Foundation (DFG) [455706279]
  2. German Research Foundation (DFG) within collaborative research center Matrix in Vision (SFB 1340/2 2022) [322486779]

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Magnetic particle imaging (MPI) is a noninvasive imaging technique that allows for the visualization of magnetic nanoparticles (MNPs) with high accuracy. In this study, a method for preparing magnetically labeled THP-1 monocytes for MPI cell tracking was developed. The factors influencing the loading of MNPs onto cells were systematically investigated, providing a foundation for the development of a reliable MPI monocyte tracking method in the future.
Magnetic particle imaging (MPI) is a noninvasive tomographic imaging modality for the quantitative visualization of magnetic nanoparticles (MNPs) with high temporal and spatial resolution. The general capability of MPI for cell tracking (e.g., monitoring living cells labeled with MNPs) has successfully been shown. MNPs in cell culture media are often subjected to structural and magnetic changes. In addition to the deteriorating reproducibility, this also complicates the systematic study of the relationship between the MNP properties and their cellular uptake for MPI. Here, we present a method for the preparation of magnetically labeled THP-1 (Tamm-Horsfall Protein-1) monocytes that are used in MPI cell tracking. The method development was performed using two different MPI tracers, which exhibited electrostatic and steric stabilizations, respectively. In the first step, the interaction between the MNPs and cell culture media was investigated and adjusted to ensure high structural and magnetic stability. Furthermore, the influences of the incubation time, MNP concentration used for cellular uptake, and individual preparation steps (e.g., the washing of cells) were systematically investigated. Finally, the success of the developed loading method was demonstrated by the MPI measurements. The presented systematic investigation of the factors that influence the MNP loading of cells will help to develop a reliable and reproducible method for MPI monocyte tracking for the early detection of inflammation in the future.

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